TY  - JOUR
A1  - Nickerson, David
A1  - Atalag, Koray
A1  - de Bono, Bernard
A1  - Geiger, Joerg
A1  - Goble, Carole
A1  - Hollmann, Susanne
A1  - Lonien, Joachim
A1  - Mueller, Wolfgang
A1  - Regierer, Babette
A1  - Stanford, Natalie J.
A1  - Golebiewski, Martin
A1  - Hunter, Peter
T1  - The Human Physiome: how standards, software and innovative service infrastructures are providing the building blocks to make it achievable
JF  - Interface focus
N2  - Reconstructing and understanding the Human Physiome virtually is a complex mathematical problem, and a highly demanding computational challenge. Mathematical models spanning from the molecular level through to whole populations of individuals must be integrated, then personalized. This requires interoperability with multiple disparate and geographically separated data sources, and myriad computational software tools. Extracting and producing knowledge from such sources, even when the databases and software are readily available, is a challenging task. Despite the difficulties, researchers must frequently perform these tasks so that available knowledge can be continually integrated into the common framework required to realize the Human Physiome. Software and infrastructures that support the communities that generate these, together with their underlying standards to format, describe and interlink the corresponding data and computer models, are pivotal to the Human Physiome being realized. They provide the foundations for integrating, exchanging and re-using data and models efficiently, and correctly, while also supporting the dissemination of growing knowledge in these forms. In this paper, we explore the standards, software tooling, repositories and infrastructures that support this work, and detail what makes them vital to realizing the Human Physiome.
KW  - Human Physiome
KW  - standards
KW  - repositories
KW  - service infrastructure
KW  - reproducible science
KW  - managing big data
Y1  - 2016
U6  - https://doi.org/10.1098/rsfs.2015.0103
SN  - 2042-8898
SN  - 2042-8901
VL  - 6
SP  - 57
EP  - 61
PB  - Royal Society
CY  - London
ER  - 
TY  - JOUR
A1  - Metz, Johannes
A1  - Tielboerger, Katja
T1  - Spatial and temporal aridity gradients provide poor proxies for plant-plant interactions under climate change: a large-scale experiment
JF  - Functional ecology : an official journal of the British Ecological Society
N2  - 1. Plant-plant interactions may critically modify the impact of climate change on plant communities. However, the magnitude and even direction of potential future interactions remains highly debated, especially for water-limited ecosystems. Predictions range from increasing facilitation to increasing competition with future aridification. 2. The different methodologies used for assessing plant-plant interactions under changing environmental conditions may affect the outcome but they are not equally represented in the literature. Mechanistic experimental manipulations are rare compared with correlative approaches that infer future patterns from current observations along spatial climatic gradients. 3. Here, we utilize a unique climatic gradient in combination with a large-scale, long-term experiment to test whether predictions about plant-plant interactions yield similar results when using experimental manipulations, spatial gradients or temporal variation. We assessed shrub-annual interactions in three different sites along a natural rainfall gradient (spatial) during 9 years of varying rainfall (temporal) and 8 years of dry and wet manipulations of ambient rainfall (experimental) that closely mimicked regional climate scenarios. 4. The results were fundamentally different among all three approaches. Experimental water manipulations hardly altered shrub effects on annual plant communities for the assessed fitness parameters biomass and survival. Along the spatial gradient, shrub effects shifted from clearly negative to mildly facilitative towards drier sites, whereas temporal variation showed the opposite trend: more negative shrub effects in drier years. 5. Based on our experimental approach, we conclude that shrub-annual interaction will remain similar under climate change. In contrast, the commonly applied space-for-time approach based on spatial gradients would have suggested increasing facilitative effects with climate change. We discuss potential mechanisms governing the differences among the three approaches. 6. Our study highlights the critical importance of long-term experimental manipulations for evaluating climate change impacts. Correlative approaches, for example along spatial or temporal gradients, may be misleading and overestimate the response of plant-plant interactions to climate change.
KW  - annual plant communities
KW  - climate manipulation
KW  - competition
KW  - facilitation
KW  - Mediterranean shrubland
KW  - nurse plant
KW  - rainfall gradient
KW  - Sarcopoterium spinosum
KW  - semi-arid
KW  - stress-gradient hypothesis
Y1  - 2016
U6  - https://doi.org/10.1111/1365-2435.12599
SN  - 0269-8463
SN  - 1365-2435
VL  - 30
SP  - 20
EP  - 29
PB  - Wiley-Blackwell
CY  - Hoboken
ER  - 
TY  - JOUR
A1  - Bilton, Mark C.
A1  - Metz, Johannes
A1  - Tielboerger, Katja
T1  - Climatic niche groups: A novel application of a common assumption predicting plant community response to climate change
JF  - Perspectives in plant ecology, evolution and systematics
N2  - Defining species by their climatic niche is the simple and intuitive principle underlying Bioclimatic Envelope Model (BEM) predictions for climate change effects. However, these correlative models are often criticised for neglecting many ecological processes. Here, we apply the same niche principle to entire communities within a medium/long-term climate manipulation study, where ecological processes are inherently included. In a nine generation study in Israel, we manipulated rainfall (Drought -30%; Irrigation +30%; Control natural rainfall) at two sites which differ chiefly in rainfall quantity and variability. We analysed community responses to the manipulations by grouping species based on their climatic rainfall niche. These responses were compared to analyses based on single species, total densities, and commonly used taxonomic groupings. Climate Niche Groups yielded clear and consistent results: within communities, those species distributed in drier regions performed relatively better in the drought treatment, and those from wetter climates performed better when irrigated. In contrast, analyses based on other principles revealed little insight into community dynamics. Notably, most relationships were weaker at the drier, more variable site, suggesting that enhanced adaptation to variability may buffer climate change impacts. We provide robust experimental evidence that using climatic niches commonly applied in BEMs is a valid approach for eliciting community changes in response to climate change. However, we also argue that additional empirical information needs to be gathered using experiments in situ to correctly assess community vulnerability. Climatic Niche Groups used in this way, may therefore provide a powerful tool and directional testing framework to generalise and compare climate change impacts across habitats. (C) 2016 The Authors. Published by Elsevier GmbH.
KW  - Annual plant communities
KW  - Bioclimatic envelope modelling
KW  - Climate change manipulations
KW  - Experimental evidence
KW  - Plant functional groups
KW  - Rainfall niche
Y1  - 2016
U6  - https://doi.org/10.1016/j.ppees.2016.02.006
SN  - 1433-8319
VL  - 19
SP  - 61
EP  - 69
PB  - Elsevier
CY  - Jena
ER  - 
TY  - JOUR
A1  - Makowicz, Amber M.
A1  - Tiedemann, Ralph
A1  - Steele, Rachel N.
A1  - Schlupp, Ingo
T1  - Kin Recognition in a Clonal Fish, Poecilia formosa
JF  - PLoS one
N2  - Relatedness strongly influences social behaviors in a wide variety of species. For most species, the highest typical degree of relatedness is between full siblings with 50% shared genes. However, this is poorly understood in species with unusually high relatedness between individuals: clonal organisms. Although there has been some investigation into clonal invertebrates and yeast, nothing is known about kin selection in clonal vertebrates. We show that a clonal fish, the Amazon molly (Poecilia formosa), can distinguish between different clonal lineages, associating with genetically identical, sister clones, and use multiple sensory modalities. Also, they scale their aggressive behaviors according to the relatedness to other females: they are more aggressive to non-related clones. Our results demonstrate that even in species with very small genetic differences between individuals, kin recognition can be adaptive. Their discriminatory abilities and regulation of costly behaviors provides a powerful example of natural selection in species with limited genetic diversity.
Y1  - 2016
U6  - https://doi.org/10.1371/journal.pone.0158442
SN  - 1932-6203
VL  - 11
PB  - PLoS
CY  - San Fransisco
ER  - 
TY  - JOUR
A1  - Lah, Ljerka
A1  - Trense, Daronja
A1  - Benke, Harald
A1  - Berggren, Per
A1  - Gunnlaugsson, Porvaldur
A1  - Lockyer, Christina
A1  - Öztürk, Ayaka
A1  - Öztürk, Bayram
A1  - Pawliczka, Iwona
A1  - Roos, Anna
A1  - Siebert, Ursula
A1  - Skora, Krzysztof
A1  - Vikingsson, Gisli
A1  - Tiedemann, Ralph
T1  - Spatially Explicit Analysis of Genome-Wide SNPs Detects Subtle Population Structure in a Mobile Marine Mammal, the Harbor Porpoise
JF  - PLoS one
N2  - The population structure of the highly mobile marine mammal, the harbor porpoise (Phocoena phocoena), in the Atlantic shelf waters follows a pattern of significant isolation-by-distance. The population structure of harbor porpoises from the Baltic Sea, which is connected with the North Sea through a series of basins separated by shallow underwater ridges, however, is more complex. Here, we investigated the population differentiation of harbor porpoises in European Seas with a special focus on the Baltic Sea and adjacent waters, using a population genomics approach. We used 2872 single nucleotide polymor-phisms (SNPs), derived from double digest restriction-site associated DNA sequencing (ddRAD-seq), as well as 13 microsatellite loci and mitochondrial haplotypes for the same set of individuals. Spatial principal components analysis (sPCA), and Bayesian clustering on a subset of SNPs suggest three main groupings at the level of all studied regions: the Black Sea, the North Atlantic, and the Baltic Sea. Furthermore, we observed a distinct separation of the North Sea harbor porpoises from the Baltic Sea populations, and identified splits between porpoise populations within the Baltic Sea. We observed a notable distinction between the Belt Sea and the Inner Baltic Sea sub-regions. Improved delineation of harbor porpoise population assignments for the Baltic based on genomic evidence is important for conservation management of this endangered cetacean in threatened habitats, particularly in the Baltic Sea proper. In addition, we show that SNPs outperform microsatellite markers and demonstrate the utility of RAD-tags from a relatively small, opportunistically sampled cetacean sample set for population diversity and divergence analysis.
Y1  - 2016
U6  - https://doi.org/10.1371/journal.pone.0162792
SN  - 1932-6203
VL  - 11
PB  - PLoS
CY  - San Fransisco
ER  - 
TY  - JOUR
A1  - Zhu, Fangjun
A1  - Schlupp, Ingo
A1  - Tiedemann, Ralph
T1  - Sequence Evolution and Expression of the Androgen Receptor and Other Pathway-Related Genes in a Unisexual Fish, the Amazon Molly, Poecilia formosa, and Its Bisexual Ancestors
JF  - PLoS one
N2  - The all-female Amazon molly (Poecilia formosa) originated from a single hybridization of two bisexual ancestors, Atlantic molly (Poecilia mexicana) and sailfin molly (Poecilia latipinna). As a gynogenetic species, the Amazon molly needs to copulate with a heterospecific male, but the genetic information of the sperm-donor does not contribute to the next generation, as the sperm only acts as the trigger for the diploid eggs’ embryogenesis. Here, we study the sequence evolution and gene expression of the duplicated genes coding for androgen receptors (ars) and other pathway-related genes, i.e., the estrogen receptors (ers) and cytochrome P450, family19, subfamily A, aromatase genes (cyp19as), in the Amazon molly, in comparison to its bisexual ancestors. Mollies possess–as most other teleost fish—two copies of the ar, er, and cyp19a genes, i.e., arα/arβ, erα/erβ1, and cyp19a1 (also referred as cyp19a1a)/cyp19a2 (also referred to as cyp19a1b), respectively. Non-synonymous single nucleotide polymorphisms (SNPs) among the ancestral bisexual species were generally predicted not to alter protein function. Some derived substitutions in the P. mexicana and one in P. formosa are predicted to impact protein function. We also describe the gene expression pattern of the ars and pathway-related genes in various tissues (i.e., brain, gill, and ovary) and provide SNP markers for allele specific expression research. As a general tendency, the levels of gene expression were lowest in gill and highest in ovarian tissues, while expression levels in the brain were intermediate in most cases. Expression levels in P. formosa were conserved where expression did not differ between the two bisexual ancestors. In those cases where gene expression levels significantly differed between the bisexual species, P. formosa expression was always comparable to the higher expression level among the two ancestors. Interestingly, erβ1 was expressed neither in brain nor in gill in the analyzed three molly species, which implies a more important role of erα in the estradiol synthesis pathway in these tissues. Furthermore, our data suggest that interactions of steroid-signaling pathway genes differ across tissues, in particular the interactions of ars and cyp19as.
Y1  - 2016
U6  - https://doi.org/10.1371/journal.pone.0156209
SN  - 1932-6203
VL  - 11
PB  - PLoS
CY  - San Fransisco
ER  - 
TY  - JOUR
A1  - Marrone, F.
A1  - Havenstein, Katja
A1  - Tiedemann, Ralph
A1  - Ketmaier, V.
T1  - Identification and characterization of five polymorphic microsatellite loci in the freshwater copepod Hemidiaptomus gurneyi (Copepoda: Calanoida: Diaptomidae)
JF  - The Italian journal of zoology
N2  - Hemidiaptomus diaptomid copepods are known to be excellent biological indicators for the highly biodiverse crustacean communities inhabiting Mediterranean temporary ponds (MTPs), an endangered inland water habitat whose conservation is considered a priority according to the "Habitat Directive" of the European Union. This study reports on the characterization of five polymorphic microsatellite loci in Hemidiaptomus gurneyi, to be used as markers for fine-scale studies on the population genetic structure and metapopulation dynamics of a typical and obligate MTP dweller. The five selected loci proved to be polymorphic in the species, with three to five polymorphic loci per studied population. Overall, mean heterozygosity scored for all loci and populations was lower than that reported for the few other diaptomid species for which microsatellite loci have been to date described; this is possibly due to the intrinsically fragmented and isolated peculiar habitat inhabited by the species. Furthermore, the presence of indels within the flanking regions of selected loci was scored. This study, albeit confirming the technical difficulties in finding proper microsatellite markers in copepods, provides for the first time a set of useful polymorphic microsatellite loci for a Hemidiaptomus species, thus allowing the realization of fine-scale phylogeographic and population genetics studies of this flagship crustacean taxon for MTPs.
KW  - Mediterranean temporary ponds
KW  - diaptomid copepods
KW  - SSRs
Y1  - 2016
U6  - https://doi.org/10.1080/11250003.2015.1126363
SN  - 1125-0003
SN  - 1748-5851
VL  - 83
SP  - 146
EP  - 150
PB  - Springer
CY  - Abingdon
ER  - 
TY  - JOUR
A1  - Lah, Ljerka
A1  - Trense, Daronja
A1  - Benke, Harald
A1  - Berggren, Per
A1  - Gunnlaugsson, Þorvaldur
A1  - Lockyer, Christina
A1  - Öztürk, Ayaka
A1  - Öztürk, Bayram
A1  - Pawliczka, Iwona
A1  - Roos, Anna
A1  - Siebert, Ursula
A1  - Skóra, Krzysztof
A1  - Víkingsson, Gísli
A1  - Tiedemann, Ralph
T1  - Spatially Explicit Analysis of Genome-Wide SNPs Detects Subtle Population Structure in a Mobile Marine Mammal, the Harbor Porpoise
JF  - PLoS one
N2  - The population structure of the highly mobile marine mammal, the harbor porpoise (Phocoena phocoena), in the Atlantic shelf waters follows a pattern of significant isolation-by-distance. The population structure of harbor porpoises from the Baltic Sea, which is connected with the North Sea through a series of basins separated by shallow underwater ridges, however, is more complex. Here, we investigated the population differentiation of harbor porpoises in European Seas with a special focus on the Baltic Sea and adjacent waters, using a population genomics approach. We used 2872 single nucleotide polymorphisms (SNPs), derived from double digest restriction-site associated DNA sequencing (ddRAD-seq), as well as 13 microsatellite loci and mitochondrial haplotypes for the same set of individuals. Spatial principal components analysis (sPCA), and Bayesian clustering on a subset of SNPs suggest three main groupings at the level of all studied regions: the Black Sea, the North Atlantic, and the Baltic Sea. Furthermore, we observed a distinct separation of the North Sea harbor porpoises from the Baltic Sea populations, and identified splits between porpoise populations within the Baltic Sea. We observed a notable distinction between the Belt Sea and the Inner Baltic Sea sub-regions. Improved delineation of harbor porpoise population assignments for the Baltic based on genomic evidence is important for conservation management of this endangered cetacean in threatened habitats, particularly in the Baltic Sea proper. In addition, we show that SNPs outperform microsatellite markers and demonstrate the utility of RAD-tags from a relatively small, opportunistically sampled cetacean sample set for population diversity and divergence analysis.
Y1  - 2016
U6  - https://doi.org/10.1371/journal.pone.0162792
SN  - 1932-6203
VL  - 11
IS  - 10
PB  - PLoS
CY  - Lawrence, Kan.
ER  - 
TY  - JOUR
A1  - Zhu, Fangjun
A1  - Schlupp, Ingo
A1  - Tiedemann, Ralph
T1  - Sequence Evolution and Expression of the Androgen Receptor and Other Pathway-Related Genes in a Unisexual Fish, the Amazon Molly, Poecilia formosa, and Its Bisexual Ancestors
JF  - PLoS one
N2  - The all-female Amazon molly (Poecilia formosa) originated from a single hybridization of two bisexual ancestors, Atlantic molly (Poecilia mexicana) and sailfin molly (Poecilia latipinna). As a gynogenetic species, the Amazon molly needs to copulate with a heterospecific male, but the genetic information of the sperm-donor does not contribute to the next generation, as the sperm only acts as the trigger for the diploid eggs’ embryogenesis. Here, we study the sequence evolution and gene expression of the duplicated genes coding for androgen receptors (ars) and other pathway-related genes, i.e., the estrogen receptors (ers) and cytochrome P450, family19, subfamily A, aromatase genes (cyp19as), in the Amazon molly, in comparison to its bisexual ancestors. Mollies possess–as most other teleost fish—two copies of the ar, er, and cyp19a genes, i.e., arα/arβ, erα/erβ1, and cyp19a1 (also referred as cyp19a1a)/cyp19a2 (also referred to as cyp19a1b), respectively. Non-synonymous single nucleotide polymorphisms (SNPs) among the ancestral bisexual species were generally predicted not to alter protein function. Some derived substitutions in the P. mexicana and one in P. formosa are predicted to impact protein function. We also describe the gene expression pattern of the ars and pathway-related genes in various tissues (i.e., brain, gill, and ovary) and provide SNP markers for allele specific expression research. As a general tendency, the levels of gene expression were lowest in gill and highest in ovarian tissues, while expression levels in the brain were intermediate in most cases. Expression levels in P. formosa were conserved where expression did not differ between the two bisexual ancestors. In those cases where gene expression levels significantly differed between the bisexual species, P. formosa expression was always comparable to the higher expression level among the two ancestors. Interestingly, erβ1 was expressed neither in brain nor in gill in the analyzed three molly species, which implies a more important role of erα in the estradiol synthesis pathway in these tissues. Furthermore, our data suggest that interactions of steroid-signaling pathway genes differ across tissues, in particular the interactions of ars and cyp19as.
Y1  - 2016
U6  - https://doi.org/10.1371/JOURNAL.PONE.0156209
SN  - 1932-6203
VL  - 11
IS  - 6
PB  - PLoS
CY  - Lawrence, Kan.
ER  - 
TY  - THES
A1  - Breuer, David
T1  - The plant cytoskeleton as a transportation network
T1  - Modellierung des pflanzliche Zytoskeletts als Transportnetzwerk
N2  - The cytoskeleton is an essential component of living cells. It is composed of different types of protein filaments that form complex, dynamically rearranging, and interconnected networks. The cytoskeleton serves a multitude of cellular functions which further depend on the cell context. In animal cells, the cytoskeleton prominently shapes the cell's mechanical properties and movement. In plant cells, in contrast, the presence of a rigid cell wall as well as their larger sizes highlight the role of the cytoskeleton in long-distance intracellular transport. As it provides the basis for cell growth and biomass production, cytoskeletal transport in plant cells is of direct environmental and economical relevance. However, while knowledge about the molecular details of the cytoskeletal transport is growing rapidly, the organizational principles that shape these processes on a whole-cell level remain elusive.

This thesis is devoted to the following question: How does the complex architecture of the plant cytoskeleton relate to its transport functionality? The answer requires a systems level perspective of plant cytoskeletal structure and transport. To this end, I combined state-of-the-art confocal microscopy, quantitative digital image analysis, and mathematically powerful, intuitively accessible graph-theoretical approaches. 

This thesis summarizes five of my publications that shed light on the plant cytoskeleton as a transportation network: (1) I developed network-based frameworks for accurate, automated quantification of cytoskeletal structures, applicable in, e.g., genetic or chemical screens; (2) I showed that the actin cytoskeleton displays properties of efficient transport networks, hinting at its biological design principles; (3) Using multi-objective optimization, I demonstrated that different plant cell types sustain cytoskeletal networks with cell-type specific and near-optimal organization; (4) By investigating actual transport of organelles through the cell, I showed that properties of the actin cytoskeleton are predictive of organelle flow and provided quantitative evidence for a coordination of transport at a cellular level; (5) I devised a robust, optimization-based method to identify individual cytoskeletal filaments from a given network representation, allowing the investigation of single filament properties in the network context. The developed methods were made publicly available as open-source software tools.

Altogether, my findings and proposed frameworks provide quantitative, system-level insights into intracellular transport in living cells. Despite my focus on the plant cytoskeleton, the established combination of experimental and theoretical approaches is readily applicable to different organisms. Despite the necessity of detailed molecular studies, only a complementary, systemic perspective, as presented here, enables both understanding of cytoskeletal function in its evolutionary context as well as its future technological control and utilization.
N2  - Das Zytoskelett ist ein notwendiger Bestandteil lebender Zellen. Es besteht aus verschiedenen Arten von Proteinfilamenten, die ihrerseits komplexe, sich dynamisch reorganisierende und miteinander verknüpfte Netzwerke bilden. Das Zytoskelett erfüllt eine Vielzahl von Funktionen in der Zelle. In Tierzellen bestimmt das Aktin-Zytoskelett maßgeblich die mechanischen Zelleigenschaften und die Zellbewegung. In Pflanzenzellen hingegen kommt dem Aktin-Zytoskelett eine besondere Bedeutung in intrazellulären Transportprozessen zu, bedingt  insbesondere  durch die starre pflanzliche Zellwand sowie die Zellgröße. Als wesentlicher Faktor für Zellwachstum und somit auch die Produktion von Biomasse, ist Zytoskelett-basierter Transport daher von unmittelbarer ökologischer und ökonomischer Bedeutung. Während das Wissen über die molekularen Grundlagen Zytoskelett-basierter Transportprozesse beständig wächst, sind die zugrunde liegenden Prinzipien zellweiter Organisation bisher weitgehend unbekannt. 

Diese Dissertation widmet sich daher folgender Frage: Wie hängt die komplexe Architektur des pflanzlichen Zytoskeletts mit seiner intrazellulären Transportfunktion zusammen? Eine Antwort auf diese Frage erfordert eine systemische Perspektive auf Zytoskelettstruktur und -transport. Zu diesem Zweck habe ich Mikroskopiedaten mit hoher raumzeitlicher Auflösung sowie Computer-gestützte Bildanalysen und mathematische Ansätzen der Graphen- und Netzwerktheorie kombiniert.

Die vorliegende Dissertation umfasst fünf meiner Publikationen, die sich einem systemischen Verständnis des pflanzlichen Zytoskeletts als Transportnetzwerk widmen: (1) Dafür habe ich Bilddaten-basierte Netzwerkmodelle entwickelt, die eine exakte und automatisierte Quantifizierung der Architektur des Zytoskeletts ermöglichen. Diese Quantifizierung kann beispielsweise in genetischen oder chemischen Versuchen genutzt werden und für eine weitere Erforschung der genetischen Grundlagen und möglicher molekularer Interaktionspartner des Zytoskeletts hilfreich sein; (2) Ich habe nachgewiesen, dass das pflanzliche Aktin-Zytoskelett Eigenschaften effizienter Transportnetzwerk aufweist und Hinweise auf seine evolutionären Organisationsprinzipien liefert; (3) Durch die mathematische Optimierung von Transportnetzwerken konnte ich zeigen, dass unterschiedliche Pflanzenzelltypen spezifische und optimierte Organisationsstrukturen des Aktin-Zytoskeletts aufweisen; (4) Durch quantitative Analyse des Transports von Organellen in Pflanzenzellen habe ich nachgewiesen, dass sich Transportmuster ausgehend von der Struktur des Aktin-Zytoskeletts vorhersagen lassen. Dabei spielen sowohl die Organisation des Zytoskeletts auf Zellebene als auch seine Geometrie eine zentrale Rolle. (5) Schließlich habe ich eine robuste, optimierungs-basierte Methode entwickelt, die es erlaubt, individuelle Filamente eines Aktin-Netzwerks zu identifizieren. Dadurch ist es möglich, die Eigenschaften einzelner Zytoskelettfilamente im zellulären Kontext zu untersuchen. Die im Zuge dieser Dissertation entwickelten Methoden wurden frei und quelloffen als Werkzeuge zur Beantwortung verwandter Fragestellung zugänglich gemacht.

Insgesamt liefern die hier präsentierten Ergebnisse und entwickelten Methoden quantitative, systemische Einsichten in die Transportfunktion des Zytoskeletts. Die hier etablierte Kombination von experimentellen und theoretischen Ansätzen kann, trotz des Fokusses auf das pflanzliche Zytoskelett, direkt auf andere Organismen angewendet werden. Als Ergänzung molekularer Studien bildet ein systemischer Blickwinkel, wie er hier entwickelt wurde, die Grundlage für ein Verständnis sowohl des evolutionären Kontextes als auch zukünftiger Kontroll- und Nutzungsmöglichkeiten des pflanzlichen Zytoskeletts.
KW  - systems biology
KW  - mathematical modeling
KW  - cytoskeleton
KW  - plant science
KW  - graph theory
KW  - image analysis
KW  - Systembiologie
KW  - mathematische Modellierung
KW  - Zytoskelett
KW  - Zellbiologie
KW  - Graphtheorie
KW  - Bildanalyse
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-93583
ER  - 
TY  - THES
A1  - Nietzsche, Madlen
T1  - Identifizierung und Charakterisierung neuer Komponenten der SnRK1-Signaltransduktion in Arabidopsis thaliana
T1  - Identification and characterization of novel components of SnRK1-Signalling in Arabidopsis thaliana
N2  - Für alle Organismen ist die Aufrechterhaltung ihres energetischen Gleichgewichts unter fluktuierenden Umweltbedingungen lebensnotwendig. In Eukaryoten steuern evolutionär konservierte Proteinkinasen, die in Pflanzen als SNF1-RELATED PROTEIN KINASE1 (SnRK1) bezeichnet werden, die Adaption an Stresssignale aus der Umwelt und an die Limitierung von Nährstoffen und zellulärer Energie. Die Aktivierung von SnRK1 bedingt eine umfangreiche transkriptionelle Umprogrammierung, die allgemein zu einer Repression energiekonsumierender Prozesse wie beispielsweise Zellteilung und Proteinbiosynthese und zu einer Induktion energieerzeugender, katabolischer Stoffwechselwege führt. Wie unterschiedliche Signale zu einer generellen sowie teilweise gewebe- und stressspezifischen SnRK1-vermittelten Antwort führen ist bisher noch nicht ausreichend geklärt, auch weil bislang nur wenige Komponenten der SnRK1-Signaltransduktion identifiziert wurden. In dieser Arbeit konnte ein Protein-Protein-Interaktionsnetzwerk um die SnRK1αUntereinheiten aus Arabidopsis AKIN10/AKIN11 etabliert werden. Dadurch wurden zunächst Mitglieder der pflanzenspezifischen DUF581-Proteinfamilie als Interaktionspartner der SnRK1α-Untereinheiten identifiziert. Diese Proteine sind über ihre konservierte DUF581Domäne, in der ein Zinkfinger-Motiv lokalisiert ist, fähig mit AKIN10/AKIN11 zu interagieren. In planta Ko-Expressionsanalysen zeigten, dass die DUF581-Proteine eine Verschiebung der nucleo-cytoplasmatischen Lokalisierung von AKIN10 hin zu einer nahezu ausschließlichen zellkernspezifischen Lokalisierung begünstigen sowie die Ko-Lokalisierung von AKIN10 und DUF581-Proteinen im Nucleus. In Bimolekularen Fluoreszenzkomplementations-Analysen konnte die zellkernspezifische Interaktion von DUF581-Proteinen mit SnRK1α-Untereinheiten in planta bestätigt werden. Außerhalb der DUF581-Domäne weisen die Proteine einander keine große Sequenzähnlichkeit auf. Aufgrund ihrer Fähigkeit mit SnRK1 zu interagieren, dem Fehlen von SnRK1Phosphorylierungsmotiven sowie ihrer untereinander sehr variabler gewebs-, entwicklungs- und stimulusspezifischer Expression wurde für DUF581-Proteine eine Funktion als Adaptoren postuliert, die unter bestimmten physiologischen Bedingungen spezifische Substratproteine in den SnRK1-Komplex rekrutieren. Auf diese Weise könnten DUF581Proteine die Interaktion von SnRK1 mit deren Zielproteinen modifizieren und eine Feinjustierung der SnRK1-Signalweiterleitung ermöglichen. Durch weiterführende Interaktionsstudien konnten DUF581-interagierende Proteine darunter Transkriptionsfaktoren, Proteinkinasen sowie regulatorische Proteine gefunden werden, die teilweise ebenfalls Wechselwirkungen mit SnRK1α-Untereinheiten aufzeigten. Im Rahmen dieser Arbeit wurde eines dieser Proteine für das eine Beteiligung an der SnRK1Signalweiterleitung als Transkriptionsregulator vermutet wurde näher charakterisiert. STKR1 (STOREKEEPER RELATED 1), ein spezifischer Interaktionspartner von DUF581-18, gehört zu einer pflanzenspezifischen Leucin-Zipper-Transkriptionsfaktorfamilie und interagiert in Hefe sowie in planta mit SnRK1. Die zellkernspezifische Interaktion von STKR1 und AKIN10 in Pflanzen unterstützt die Vermutung der kooperativen Regulation von Zielgenen. Weiterhin stabilisierte die Anwesenheit von AKIN10 die Proteingehalte von STKR1, das wahrscheinlich über das 26S Proteasom abgebaut wird. Da es sich bei STKR1 um ein Phosphoprotein mit SnRK1-Phosphorylierungsmotiv handelt, stellt es sehr wahrscheinlich ein SnRK1-Substrat dar. Allerdings konnte eine SnRK1-vermittelte Phosphorylierung von STKR1 in dieser Arbeit nicht gezeigt werden. Der Verlust von einer Phosphorylierungsstelle beeinflusste die Homo- und Heterodimerisierungsfähigkeit von STKR1 in Hefeinteraktionsstudien, wodurch eine erhöhte Spezifität der Zielgenregulation ermöglicht werden könnte. Außerdem wurden Arabidopsis-Pflanzen mit einer veränderten STKR1-Expression phänotypisch, physiologisch und molekularbiologisch charakterisiert. Während der Verlust der STKR1-Expression zu Pflanzen führte, die sich kaum von Wildtyp-Pflanzen unterschieden, bedingte die konstitutive Überexpression von STKR1 ein stark vermindertes Pflanzenwachstum sowie Entwicklungsverzögerungen hinsichtlich der Blühinduktion und Seneszenz ähnlich wie sie auch bei SnRK1α-Überexpression beschrieben wurden. Pflanzen dieser Linien waren nicht in der Lage Anthocyane zu akkumulieren und enthielten geringere Gehalte an Chlorophyll und Carotinoiden. Neben einem erhöhten nächtlichen Stärkeumsatz waren die Pflanzen durch geringere Saccharosegehalte im Vergleich zum Wildtyp gekennzeichnet. Eine Transkriptomanalyse ergab, dass in den STKR1-überexprimierenden Pflanzen unter Energiemangelbedingungen, hervorgerufen durch eine verlängerte Dunkelphase, eine größere Anzahl an Genen im Vergleich zum Wildtyp differentiell reguliert war als während der Lichtphase. Dies spricht für eine Beteiligung von STKR1 an Prozessen, die während der verlängerten Dunkelphase aktiv sind. Ein solcher ist beispielsweise die SnRK1-Signaltransduktion, die unter energetischem Stress aktiviert wird. Die STKR1Überexpression führte zudem zu einer verstärkten transkriptionellen Induktion von Abwehrassoziierten Genen sowie NAC- und WRKY-Transkriptionsfaktoren nach verlängerter Dunkelphase. Die Transkriptomdaten deuteten auf eine stimulusunabhängige Induktion von Abwehrprozessen hin und konnten eine Erklärung für die phänotypischen und physiologischen Auffälligkeiten der STKR1-Überexprimierer liefern.
N2  - For all living organism maintenance of energy homeostasis under changing environmental conditions is indispensable. In eukaryotes, evolutionary conserved protein kinases, such as the SNF1-RELATED PROTEIN KINASE1 (SnRK1) in plants, integrate environmental stress signals, nutrient availability and energy depletion during adaptational responses. Activation of SnRK1 triggers a broad transcriptional reprogramming, which in general represses energy consuming processes such as proliferation and protein biosynthesis and induces energy producing catabolic pathways. Although SnRK1 acts as a convergent point for many different environmental and metabolic signals to control growth and development, it is currently unknown how these many different signals could be translated into a cell-type or stimulusspecific response. This is also due to the fact that only a few proteins participating in SnRK1 signal transduction have yet been identified. In this work, a protein-protein interaction network of the Arabidopsis SnRK1α-subunits AKIN10/AKIN11 was established. Thereby, members of the plant specific DUF581 protein family were identified as SnRK1α interacting proteins. The highly conserved DUF581 domain possesses a zinc finger motif and mediates the interaction with AKIN10/AKIN11. In planta co-expression of AKIN10 with DUF581 proteins leads to a shift of subcellular localization from a nucleo-cytoplasmic distribution of both proteins to a nearly exclusive nuclear localization and show that AKIN10 and DUF581 proteins co-localize in nuclei of plant cells. Bimolecular fluorescence complementation analysis revealed that SnRK1α-subunits interact with DUF581 proteins in plants. Apart from their DUF581 domain there is no strong sequence similarity between DUF581 proteins. Because of their ability to interact with SnRK1, the absence of SnRK1-target motifs and their highly variable transcriptional regulation in a tissue-, development- or stimuli-specific manner, it is possible that DUF581 proteins act as adaptor proteins recruiting substrate proteins into the SnRK1 complex under defined physiological conditions. That said, DUF581 could modify the interaction of SnRK1 with its target proteins and facilitate fine-tuning of SnRK1 signal transduction. Additional interaction studies revealed further DUF581 interacting proteins such as transcription factors, protein kinases and regulatory proteins that in part were also able to interact with SnRK1α. One of these proteins which is supposed to be involved in SnRK1 signaling as a transcriptional regulator was characterized in more detail: Arabidopsis STKR1 (STOREKEPPER RELATED 1) a DUF581-18 interaction partner belongs to a plant specific leucine zipper transcription factor family and is able to interact with SnRK1 in yeast and in planta. Co-operative regulation of target genes by STKR1 and AKIN10 is supported by the specific interaction of these proteins inside the plant nucleus. Furthermore, AKIN10 seems to stabilize protein levels of STKR1 in that it attenuates its proteasomal turnover. Due to the fact that STKR1 is a phosphoprotein with putative SnRK1 target motives it is likely a SnRK1 substrate. However, SnRK1 mediated phosphorylation of STKR1 could not be shown in this work. Though, interaction studies in yeast revealed that a loss of putative phosphorylation sites influences the ability of homo- and hetero-dimerization of STKR1, possibly allowing a higher specificity during target gene regulation. Another part of this work was the phenotypic, physiological and molecular characterization of Arabidopsis plants with altered expression of STKR1. Whereas the absence of STKR1 expression results in plants without strong phenotypic abnormality compared to wildtype the overexpression leads to a strong decrease in plant growth as well as developmental retardations regarding to the induction of flowering and senescence reminiscent of SnRK1overexpressing plants. Plants of these lines were not able to accumulate anthocyanins and also contain reduced levels of chlorophyll and carotenoids. Besides a higher starch turnover in dark, these plants displayed lower sucrose contents. Microarray analysis revealed that under energy deficit stress, induced by extended darkness, a higher number of genes were differentially regulated in plants overexpressing STKR1 compared to wildtype than during the light period. This observation argues for a participation of STKR1 in processes, which are active under extended darkness, being the case for SnRK1 signaling which is strongly activated under energy deficient stress. Overexpression of STKR1 also leads to transcriptional induction of genes associated with defense like NAC and WRKY transcription factors after an extended dark. Results of transcriptome data analysis indicate a stimulus independent induction of defense associated processes and are suitable to explain phenotypical and physiological abnormality of the STKR1 overexpressing lines.
KW  - SnRK1
KW  - Proteinkinase
KW  - Phosphorylierung
KW  - Arabidopsis thaliana
KW  - Energiemangel
KW  - phosphorylation
KW  - energy starvation
KW  - protein kinase
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-98678
ER  - 
TY  - THES
A1  - Kloß, Lena
T1  - The link between genetic diversity and species diversity
BT  - patterns and processes in plants of agriculturally managed grassland
Y1  - 2016
ER  - 
TY  - THES
A1  - Bolger, Anthony
T1  - Sequencing the Genome of the stress-tolerant wild tomato Solanum pennellii and Novel Algorithms motivated thereby
Y1  - 2016
ER  - 
TY  - THES
A1  - Dotzek, Jana
T1  - Mitochondria in the genus Oenothera - Non-Mendelian inheritance patterns, in vitro structure and evolutionary dynamics
Y1  - 2016
ER  - 
TY  - JOUR
A1  - Klauschies, Toni
A1  - Vasseur, David A.
A1  - Gaedke, Ursula
T1  - Trait adaptation promotes species coexistence in diverse predator and prey communities
JF  - Ecology and evolution
N2  - Species can adjust their traits in response to selection which may strongly influence species coexistence. Nevertheless, current theory mainly assumes distinct and time-invariant trait values. We examined the combined effects of the range and the speed of trait adaptation on species coexistence using an innovative multispecies predator–prey model. It allows for temporal trait changes of all predator and prey species and thus simultaneous coadaptation within and among trophic levels. We show that very small or slow trait adaptation did not facilitate coexistence because the stabilizing niche differences were not sufficient to offset the fitness differences. In contrast, sufficiently large and fast trait adaptation jointly promoted stable or neutrally stable species coexistence. Continuous trait adjustments in response to selection enabled a temporally variable convergence and divergence of species traits; that is, species became temporally more similar (neutral theory) or dissimilar (niche theory) depending on the selection pressure, resulting over time in a balance between niche differences stabilizing coexistence and fitness differences promoting competitive exclusion. Furthermore, coadaptation allowed prey and predator species to cluster into different functional groups. This equalized the fitness of similar species while maintaining sufficient niche differences among functionally different species delaying or preventing competitive exclusion. In contrast to pre-
vious studies, the emergent feedback between biomass and trait dynamics enabled supersaturated coexistence for a broad range of potential trait adaptation and parameters. We conclude that accounting for trait adaptation may explain stable and supersaturated species coexistence for a broad range of environmental conditions in natural systems when the absence of such adaptive changes would preclude it. Small trait changes, coincident with those that may occur within many natural populations, greatly enlarged the number of coexisting species.
KW  - Coadaptation
KW  - equalizing and stabilizing mechanisms
KW  - maintenance of functional diversity
KW  - niche and fitness differences
KW  - supersaturated species coexistence
KW  - trait convergence and divergence
Y1  - 2016
U6  - https://doi.org/10.1002/ece3.2172
SN  - 2045-7758
PB  - John Wiley & Sons, Inc.
ER  - 
TY  - GEN
A1  - Klauschies, Toni
A1  - Vasseur, David A.
A1  - Gaedke, Ursula
T1  - Trait adaptation promotes species coexistence in diverse predator and prey communities
N2  - Species can adjust their traits in response to selection which may strongly influence species coexistence. Nevertheless, current theory mainly assumes distinct and time-invariant trait values. We examined the combined effects of the range and the speed of trait adaptation on species coexistence using an innovative multispecies predator–prey model. It allows for temporal trait changes of all predator and prey species and thus simultaneous coadaptation within and among trophic levels. We show that very small or slow trait adaptation did not facilitate coexistence because the stabilizing niche differences were not sufficient to offset the fitness differences. In contrast, sufficiently large and fast trait adaptation jointly promoted stable or neutrally stable species coexistence. Continuous trait adjustments in response to selection enabled a temporally variable convergence and divergence of species traits; that is, species became temporally more similar (neutral theory) or dissimilar (niche theory) depending on the selection pressure, resulting over time in a balance between niche differences stabilizing coexistence and fitness differences promoting competitive exclusion. Furthermore, coadaptation allowed prey and predator species to cluster into different functional groups. This equalized the fitness of similar species while maintaining sufficient niche differences among functionally different species delaying or preventing competitive exclusion. In contrast to previous studies, the emergent feedback between biomass and trait dynamics enabled supersaturated coexistence for a broad range of potential trait adaptation and parameters. We conclude that accounting for trait adaptation may explain stable and supersaturated species coexistence for a broad range of environmental conditions in natural systems when the absence of such adaptive changes would preclude it. Small trait changes, coincident with those that may occur within many natural populations, greatly enlarged the number of coexisting species.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 227 
KW  - Coadaptation
KW  - equalizing and stabilizing mechanisms
KW  - maintenance of functional diversity
KW  - niche and fitness differences
KW  - supersaturated species coexistence
KW  - trait convergence and divergence
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-91498
SN  - 1866-8372
ER  - 
TY  - THES
A1  - Beltran, Juan Camilo Moreno
T1  - Characterization of the Clp protease complex and identification of putative substrates in N. tabacum
Y1  - 2016
ER  - 
TY  - THES
A1  - Klauschies, Toni
T1  - Revealing causes and consequences of functional diversity using trait-based models
Y1  - 2016
ER  - 
TY  - THES
A1  - Reinecke, Antje Adriana
T1  - Impact of protein structure on the mechanics and assembly of mytilus byssal threads
Y1  - 2016
ER  - 
TY  - THES
A1  - Shahnejat-Bushehri, Sara
T1  - Unravelling the role of the Arabidopsis NAC transcription factor JUNGBRUNNEN1 (JUB1) for the regulation of growth and stress responses
Y1  - 2016
ER  - 
TY  - THES
A1  - Makower, Katharina
T1  - The roles of secondary metabolites in microcystis inter-strain interactions
T1  - Die Rolle von Sekundärmetaboliten in den Wechselbeziehungen zwischen Microcystis-Stämmen
N2  - Among the bloom-forming and potentially harmful cyanobacteria, the genus Microcystis represents a most diverse taxon, on the genomic as well as on morphological and secondary metabolite levels. Microcystis communities are composed of a variety of diversified strains. The focus of this study lies on potential interactions between Microcystis representatives and the roles of secondary metabolites in these interaction processes. 
The role of secondary metabolites functioning as signaling molecules in the investigated interactions is demonstrated exemplary for the prevalent hepatotoxin microcystin. The extracellular and intracellular roles of microcystin are tested in microarray-based transcriptomic approaches. While an extracellular effect of microcystin on Microcystis transcription is confirmed and connected to a specific gene cluster of another secondary metabolite in this study, the intracellularly occurring microcystin is related with several pathways of the primary metabolism. A clear correlation of a microcystin knockout and the SigE-mediated regulation of carbon metabolism is found. According to the acquired transcriptional data, a model is proposed that postulates the regulating effect of microcystin on transcriptional regulators such as the alternative sigma factor SigE, which in return captures an essential role in sugar catabolism and redox-state regulation. 
For the purpose of simulating community conditions as found in the field, Microcystis colonies are isolated from the eutrophic lakes near Potsdam, Germany and established as stably growing under laboratory conditions. In co-habitation simulations, the recently isolated field strain FS2 is shown to specifically induce nearly immediate aggregation reactions in the axenic lab strain Microcystis aeruginosa PCC 7806. In transcriptional studies via microarrays, the induced expression program in PCC 7806 after aggregation induction is shown to involve the reorganization of cell envelope structures, a highly altered nutrient uptake balance and the reorientation of the aggregating cells to a heterotrophic carbon utilization, e.g. via glycolysis. These transcriptional changes are discussed as mechanisms of niche adaptation and acclimation in order to prevent competition for resources.
N2  - Die Gattung Microcystis stellt unter den blüten-bildenden Cyanobakterien ein Taxon besonderer Diversität dar. Dies gilt sowohl für die Genomstruktur als auch für morphologische Charakteristika und Sekundärmetabolite. Microcystis-Communities weisen eine Zusammensetzung aus einer Vielzahl von diversifizierten Stämmen auf. Das Hauptaugenmerk dieser Arbeit lag darauf, potentielle Wechselwirkungen zwischen Microcystis-Vertretern zu charakterisieren und die Rolle von Sekundärmetaboliten in Interaktions-Prozessen zu untersuchen. 
Die Rolle von Sekundärmetaboliten als Signalstoffe in Microcystis-Interaktionen wurde exemplarisch für das Hepatotoxin Microcystin demonstriert. Sowohl die extrazelluläre als auch die intrazellulare Funktion von Microcystin wurde anhand von Microarray-basierten Transkriptomstudien getestet. Dabei konnte eine extrazelluläre Wirkung von Microcystin bestätigt werden und mit der Transkription eines spezifischen anderen Sekundärmetaboliten in Verbindung gebracht werden. Intrazellulär vorkommendes Microcystin wurde hingegen mit verschiedenen Stoffwechselwegen des Primärstoffwechsels verknüpft. Es konnte ein deutlicher Zusammenhang zwischen einem Microcystin-Knockout und der SigE-vermittelten Regulation des Kohlenstoffmetabolismus festgestellt werden. Anhand der erworbenen Transkriptionsdaten wurde ein Modell vorgeschlagen, das eine regulierende Wirkung von Microcystin auf Transkriptionsfaktoren wie den alternativen Sigmafaktor SigE postuliert, welcher seinerseits eine zentrale Rolle in Zuckerabbauprozessen und zellulärer Redoxregulation einnimmt. 
Mit dem Ziel, Community-ähnliche Bedingungen zu simulieren, wurden Microcystis-Freiland-Kolonien aus eutrophen Gewässern in der Umgebung von Potsdam isoliert und ein stabiles Wachstum unter Laborbedingungen etabliert. Es konnte gezeigt werden, dass der frisch isolierte Freilandstamm FS2 spezifisch eine starke Zellaggregation in Microcystis aeruginosa PCC 7806 (einem axenischen Labortstamm) auslösen konnte. In Transkriptionsstudien mit Hilfe von Microarrays wurden Expressionsprogramme gefunden, die sowohl einen Umbau von Zellhüllstrukturen, als auch einen stark veränderten transmembranen Nährstofftransport beinhalteten. Darüber hinaus konnte in den aggregierenden PCC 7806-Zellen eine Verlagerung zu heterotrophen Kohlenstoffabbauprozessen wie der Glykolyse gefunden werden. Die transkriptionellen Veränderungen wurden als Akklimationsmechanismen zur Positionierung in ökologische Nischen diskutiert, um Konkurrenzen um Ressourcen zu vermeiden.
KW  - microcystis
KW  - microcystin
KW  - secondary metabolites
KW  - transcriptomics
KW  - interactions
KW  - Sekundärmetabolite
KW  - Transkriptomik
KW  - Wechselwirkungen
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-93916
ER  - 
TY  - THES
A1  - Rolke, Daniel
T1  - Räumliche und zeitliche Expressionsmuster sowie Funktionen der Serotonin-Rezeptor-Subtypen der Honigbiene, Apis mellifera L., 1758
T1  - Spatial and temporal expression patterns as well as functions of the serotonin-receptor-subtypes in the honey bee, Apis mellifera L., 1758
N2  - Das biogene Amin Serotonin (5-Hydroxytryptamin, 5-HT) agiert als wichtiger chemischer Botenstoff bei einer Vielzahl von Organismen. Das durch 5 HT vermittelte Signal wird dabei durch spezifische Rezeptoren wahrgenommen und in eine zelluläre Reaktion umgesetzt. Diese 5 HT Rezeptoren gehören überwiegend zur Familie der G Protein gekoppelten Rezeptoren (GPCRs). Die Honigbiene Apis mellifera bietet unter anderem aufgrund ihrer eusozialen Lebensweise vielfältige Ansatzpunkte zur Erforschung der Funktionen des serotonergen Systems in Insekten. Bei A. mellifera wurden bereits vier 5-HT-Rezeptor-Subtypen beschrieben und molekular sowie pharmakologisch charakterisiert: Am5 HT1A, Am5 HT2α, Am5 HT2β und Am5 HT7. Ziel dieser Arbeit war es, gewebespezifische sowie alters- und tageszeitabhängige Expressionsmuster der 5 HT Rezeptor-Subtypen zu untersuchen, um zu einem umfassenden Verständnis des serotonergen Systems der Honigbiene beizutragen und eine Basis zur Hypothesenentwicklung für mögliche physiologische Funktionen zu schaffen. 
   Es wurde die Expression der 5 HT Rezeptorgene sowohl im zentralen Nervensystem, als auch in Teilen des Verdauungs-, Exkretions- und Speicheldrüsensystems gemessen. Dabei konnte gezeigt werden, dass die untersuchten 5-HT-Rezeptor-Subtypen generell weit im Organismus der Honigbiene verbreitet sind. Interessanterweise unterschieden sich die untersuchten Gewebe hinsichtlich der mRNA-Expressionsmuster der untersuchten Rezeptoren. Während beispielsweise im Gehirn Am5 ht1A und Am5 ht7 stärker als Am5 ht2α und Am5 ht2β exprimiert wurden, zeigte sich in Darmgewebe ein umgekehrtes Muster.
   Es war bereits bekannt, dass es bei der Expression der Am5-ht2-Gene zu alternativem Spleißen kommt. Dies führt zur Entstehung der verkürzten mRNA-Varianten Am5 ht2αΔIII und Am5 ht2βΔII. Die daraus resultierenden Proteine können nicht als funktionelle GPCRs agieren. Es konnte gezeigt werden, dass diese verkürzten Spleißvarianten dennoch ubiquitär in der Honigbiene exprimiert werden. Bemerkenswerterweise wurden gewebeübergreifende Ähnlichkeiten der Expressionsmuster der Spleißvarianten gegenüber deren zugehörigen Volllängenvarianten festgestellt, welche auf Funktionen der verkürzten Varianten in vivo hindeuten.
   Im Hinblick auf die bei A. mellifera hauptsächlich altersbedingte Arbeitsteilung wurde die Expression der 5 HT Rezeptor-Subtypen in Gehirnen von unterschiedlich alten Arbeiterinnen mit unterschiedlichen sozialen Rollen verglichen. Während auf mRNA-Ebene keines der vier 5 HT Rezeptor-Subtypen eine altersabhängig unterschiedliche Expression zeigte, konnte für das Am5-HT1A-Protein eine höhere Konzentration in den Gehirnen älterer Tiere gefunden werden. Dies deutet auf eine posttranskriptionale Regulation der 5 HT1A Rezeptorexpression hin, welche im Zusammenhang mit der Arbeitsteilung stehen könnte.
   Es erfolgte die Untersuchung tageszeitlicher Änderungen sowohl der Expression der 5 HT Rezeptor-Subtypen, als auch des biogenen Amins 5 HT selbst. Während es in den Gehirnen von Arbeiterinnen, welche unter natürlichen Bedingungen gehalten wurden, zu keiner tageszeitabhängigen Veränderung des 5 HT-Titers kam, zeigte die mRNA-Expression von Am5-ht2α und Am5-ht2β eine periodische Oszillation mit Zunahme während des Tages und Abnahme während der Nacht. Diese Regulation wird durch externe Faktoren hervorgerufen und ist nicht auf einen endogenen circadianen Rhythmus zurückzuführen. Dies ging aus der Wiederholung der Expressionsmessungen an Gehirnen von Bienen, welche unter konstanten Laborbedingungen gehalten wurden, hervor.
   Weiterhin wurde die Beteiligung des serotonergen Systems an der Steuerung von Aspekten des circadianen lokomotorischen Aktivitätsrhythmus anhand von Verhaltensexperimenten untersucht. Mit 5 HT gefütterte Arbeiterinnen zeigten dabei unter konstanten Bedingungen eine längere Periode des Aktivitätsrhythmus als Kontrolltiere. Dies deutet auf einen Einfluss von 5 HT auf die Modulation der Synchronisation der inneren Uhr hin.
   Die vorliegenden Ergebnisse tragen wesentlich zum tieferen Verständnis des serotonergen Systems der Honigbiene bei und bieten Ansatzpunkte für weitergehende Studien zur Funktion von 5 HT im Zusammenhang mit der Modulation von physiologischen Prozessen, Arbeitsteilung und circadianen Rhythmen.
N2  - The biogenic amine serotonin (5-hydroxytryptamine, 5-HT) acts as an important chemical messenger in a variety of organisms. The 5 HT-mediated signal is perceived by specific receptors and converted to a cellular response. This 5 HT receptors mainly belong to the family of G protein-coupled receptors (GPCRs). The honeybee offers various starting points to explore the functions of the serotonergic system in insects, among other things because of their eusocial lifestyle. In A. mellifera four 5-HT receptor subtypes have been described and molecularly and pharmacologically characterized: Am5 HT1A, Am5 HT2α, Am5 HT2β and Am5 HT7. The aim of this study was to investigate the tissue-specific and age- and daytime-dependent expression patterns of the 5 HT receptor subtypes in order to contribute to a comprehensive understanding of the serotonergic system in A. mellifera.
   The expression of the 5 HT receptor genes was measured in the central nervous system, as well as in parts of the digestive, excretory and salivary system. It was shown that the investigated 5-HT receptor subtypes are widely distributed in the honeybee. Interestingly, the tissues examined differed with regard to the mRNA expression pattern of the studied receptors. While in the brain the expression of Am5 ht1A and Am5 ht7 was higher than that of Am5 ht2α and Am5 ht2β, the opposite held true for intestinal tissue.
   It was already known that alternative splicing occurs in the expression of both Am5-ht2 genes. This leads to the formation of the truncated mRNA variants Am5 ht2αΔIII and Am5 ht2βΔII. The resulting proteins cannot act as functional GPCRs. However, it was demonstrated that these truncated splice variants are still ubiquitously expressed in the honeybee. Remarkably, similarities in the expression patterns of the shortened splice variants towards their corresponding full length variants were found throughout different tissues that indicate in vivo functions of the shortened variants.
   In view of the mainly age related division of labor in A. mellifera, the expression of the 5 HT receptor subtypes was compared in brains of different aged workers with different social roles. While none of the four 5 HT receptor subtypes showed an age-dependent differential expression at the mRNA level, a higher concentration in the brains of older animals could be found for the Am5-HT1A protein. This points to a post-transcriptional regulation of 5 HT1A receptor expression, which could be associated with the division of labor.
   It was carried out the investigation of diurnal changes in both the expression of the 5 HT receptor subtypes, and of the biogenic amine 5 HT itself. While in the brains of workers, which were kept under natural conditions, no daytime-dependent changes of the 5 HT titer could be found, the mRNA expression of Am5 ht2α and Am5-ht2β showed a periodic oscillation with an increase during the day and a decrease at night. This regulation is caused by external factors and not due to an endogenous circadian rhythm. That was shown by the repetition of the expression measurements on brains of bees, which were kept under constant laboratory conditions.
   Furthermore, the involvement of the serotonergic system in controlling aspects of circadian locomotor activity rhythm was investigated in behavioral experiments. Under constant conditions, worker bees which were fed with 5 HT showed a longer period of locomotor rhythm than control animals. This suggests an influence of 5 HT in the modulation of the synchronization of the internal clock.
   In conclusion, the present results contribute to a more detailed understanding of the serotonergic system of the honeybee and provide a basis for further studies on the function of 5 HT in connection with the modulation of physiological processes, division of labor and circadian rhythms.
KW  - Serotonin
KW  - Rezeptor
KW  - Honigbiene
KW  - serotonin
KW  - receptors
KW  - honey bee
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-96667
ER  - 
TY  - THES
A1  - Orf, Isabel
T1  - Photorespiratory metabolism in the cyanobacterial model Synechocystis sp. strain PCC 6803
BT  - a systems biology approach
Y1  - 2016
ER  - 
TY  - THES
A1  - Geyer, Juliane
T1  - Adapting biodiversity conservation management to climate change
Y1  - 2016
ER  - 
TY  - THES
A1  - Pellizzer, Tommaso
T1  - A novel approach to identify plastidic factors for plastome genome incompatibility and evidence for the central involvement of the chloroplast in leaf shaping
Y1  - 2016
ER  - 
TY  - THES
A1  - Korkuć, Paula
T1  - Spatial investigations of protein structures with regard to compound binding and post-translational modifications
Y1  - 2016
ER  - 
TY  - THES
A1  - Sokolowska, Ewelina Maria
T1  - Implementation of a plasmodesmata gatekeeper system, and its effect on intercellular transport
Y1  - 2016
ER  - 
TY  - THES
A1  - Sin, Celine
T1  - Post-transcriptional control of gene expression
T1  - Post-Transkription Steuerung der Genexpression
N2  - Gene expression describes the process of making functional gene products (e.g. proteins or special RNAs) from instructions encoded in the genetic information (e.g. DNA).  This process is heavily regulated, allowing cells to produce the appropriate gene products necessary for cell survival, adapting production as necessary for different cell environments.  Gene expression is subject to regulation at several levels, including transcription, mRNA degradation, translation and protein degradation.  When intact, this system maintains cell homeostasis, keeping the cell alive and adaptable to different environments.  Malfunction in the system can result in disease states and cell death.  In this dissertation, we explore several aspects of gene expression control by analyzing data from biological experiments.  Most of the work following uses a common mathematical model framework based on Markov chain models to test hypotheses, predict system dynamics or elucidate network topology.  Our work lies in the intersection between mathematics and biology and showcases the power of statistical data analysis and math modeling for validation and discovery of biological phenomena.
N2  - Das „zentrale Dogma der Molekularbiologie“ besagt, dass der Fluss genetischer Information mit der DNS startet, die dann auf die RNS kopiert und in Proteine übersetzt wird (Crick 1970). Dieses System der Informationsübertragung bietet zwei natürliche Eingriffspunkte, an denen Genausprägungen manipuliert werden können -- entweder auf dem Level der mRNS (z.B. durch Kontrolle der Transkriptions- oder mRNS- Degradationsprozesse) oder auf dem Level des Proteins (z.B. durch Kontrolle der Translations- oder Proteindegradationsprozesse). An jedem Eingriffspunkt sind eine Vielzahl unterschiedlicher Prozesse zeitgleich aktiv, um die Konzentrationen von mRNS und Proteinen präzise einzustellen. All diese Prozesse tragen dazu bei, die Zelle intern im stationäzen Zustand zu halten, denn eine Fehlfunktion im System kann zu Krankheitszuständen oder zum Zelltot führen. In dieser Arbeit untersuchen wir verschiedene Aspekte der Kontrolle der Genausprägungs, indem wir Daten biologischer Experimente analysieren. Unsere Arbeit liegt hierbei zwischen den Bereichen der mathematischer Modellierung und der Biologie und zeigt den immensen Nutzen von statistischen Analysemethoden und mathematischer Modellbildung zur Validierung und Neuentdeckung biologischer Phänomene auf.
KW  - mRNA degradation
KW  - protein degradation
KW  - gene expression control
KW  - mathematical modeling
KW  - stochastic modeling
KW  - data analysis and statistics
KW  - next generation sequencing (NGS)
KW  - ribosome
KW  - Datenanalyse und Statistik
KW  - Regulierung der Genexpression
KW  - mRNA Degradierung
KW  - mathematisches Modellierung
KW  - Proteindegradierung
KW  - Ribosom
KW  - stochastische Modellierung
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-102469
ER  - 
TY  - THES
A1  - Shikangalah, Rosemary Ndawapeka
T1  - An ecohydrological impact assessment in urban areas
BT  - urban water erosion in Windhoek, Namibia
N2  - Over the last decades, the world’s population has been growing at a faster rate, resulting in increased urbanisation, especially in developing countries. More than half of the global population currently lives in urbanised areas with an increasing tendency. The growth of cities results in a significant loss of vegetation cover, soil compaction and sealing of the soil surface which in turn results in high surface runoff during high-intensity storms and causes the problem of accelerated soil water erosion on streets and building grounds. Accelerated soil water erosion is a serious environmental problem in cities as it gives rise to the contamination of aquatic bodies, reduction of ground water recharge and increase in land degradation, and also results in damages to urban infrastructures, including drainage systems, houses and roads. Understanding the problem of water erosion in urban settings is essential for the sustainable planning and management of cities prone to water erosion. However, in spite of the vast existence of scientific literature on water erosion in rural regions, a concrete understanding of the underlying dynamics of urban erosion still remains inadequate for the urban dryland environments.

This study aimed at assessing water erosion and the associated socio-environmental determinants in a typical dryland urban area and used the city of Windhoek, Namibia, as a case study. The study used a multidisciplinary approach to assess the problem of water erosion. This included an in depth literature review on current research approaches and challenges of urban erosion, a field survey method for the quantification of the spatial extent of urban erosion in the dryland city of Windhoek, and face to face interviews by using semi-structured questionnaires to analyse the perceptions of stakeholders on urban erosion.

The review revealed that around 64% of the literatures reviewed were conducted in the developed world, and very few researches were carried out in regions with extreme climate, including dryland regions. Furthermore, the applied methods for erosion quantification and monitoring are not inclusive of urban typical features and they are not specific for urban areas. The reviewed literature also lacked aspects aimed at addressing the issues of climate change and policies regarding erosion in cities. In a field study, the spatial extent and severity of an urban dryland city, Windhoek, was quantified and the results show that nearly 56% of the city is affected by water erosion showing signs of accelerated erosion in the form of rills and gullies, which occurred mainly in the underdeveloped, informal and semi-formal areas of the city. Factors influencing the extent of erosion in Windhoek included vegetation cover and type, socio-urban factors and to a lesser extent slope estimates. A comparison of an interpolated field survey erosion map with a conventional erosion assessment tool (the Universal Soil Loss Equation) depicted a large deviation in spatial patterns, which underlines the inappropriateness of traditional non-urban erosion tools to urban settings and emphasises the need to develop new erosion assessment and management methods for urban environments. It was concluded that measures for controlling water erosion in the city need to be site-specific as the extent of erosion varied largely across the city.

The study also analysed the perceptions and understanding of stakeholders of urban water erosion in Windhoek, by interviewing 41 stakeholders using semi-structured questionnaires. The analysis addressed their understanding of water erosion dynamics, their perceptions with regards to the causes and the seriousness of erosion damages, and their attitudes towards the responsibilities for urban erosion. The results indicated that there is less awareness of the process as a phenomenon, instead there is more awareness of erosion damages and the factors contributing to the damages. About 69% of the stakeholders considered erosion damages to be ranging from moderate to very serious. However, there were notable disparities between the private householders and public authority groups. The study further found that the stakeholders have no clear understanding of their responsibilities towards the management of the control measures and payment for the damages. The private householders and local authority sectors pointed fingers at each other for the responsibilities for erosion damage payments and for putting up prevention measures. The reluctance to take responsibility could create a predicament for areas affected, specifically in the informal settlements where land management is not carried out by the local authority and land is not owned by the occupants.

The study concluded that in order to combat urban erosion, it is crucial to understand diverse dynamics aggravating the process of urbanisation from different scales. Accordingly, the study suggests that there is an urgent need for the development of urban-specific approaches that aim at: (a) incorporating the diverse socio-economic-environmental aspects influencing erosion, (b) scientifically improving natural cycles that influence water storages and nutrients for plants in urbanised dryland areas in order to increase the amount of vegetation cover, (c) making use of high resolution satellite images to improve the adopted methods for assessing urban erosion, (d) developing water erosion policies, and (e) continuously monitoring the impact of erosion and the influencing processes from local, national and international levels.
N2  - In den letzten Jahrzehnten ist die Erdbevölkerung mit großer Geschwindigkeit gewachsen. Das hatte eine verstärkte Urbanisierung zur Folge, insbesondere in den Entwicklungsländern. Zurzeit lebt über die Hälfte der globalen Bevölkerung in Stadtgebieten, mit steigender Tendenz. Städtewachstum geht mit einem signifikanten Verlust von Vegetationsbedeckung, sowie mit Bodenverdichtung und -versiegelung einher. Diese Faktoren führen bei  Starkregenereignissen zu einem hohen Oberflächenabfluss, und zu Problemen durch beschleunigte wasserbedingte Bodenerosion in Straßen und auf Baugelände. In Städten ist eine beschleunigte wasserbedingte Bodenerosion ist ein ernstzunehmendes Umweltproblem, denn sie verursacht eine Verschmutzung der Gewässer, eine verminderte Grundwasserneubildung und erhöhte Landdegradierung. Darüber hinaus kommt es zu erosionsbedingten Schäden in der städtischen Infrastruktur, inklusive der Entwässerungssysteme, sowie an Häusern und Straßen. Für ein nachhaltiges Planen und Management von erosionsanfälligen Städten ist es von essentieller Bedeutung, die Probleme der Wassererosion in städtischen Gebieten zu verstehen. Trotz der großen Anzahl wissenschaftlicher Studien über Wassererosion in ländlichen Gegenden bleibt unser Verständnis der zu Grunde liegenden Erosionsdynamiken in urbanen Trockengebieten unzureichend.

Diese Studie zielt darauf ab, Wassererosion, sowie die dazu beitragenden sozio-ökologischen Faktoren, in einem typischen urbanen Trockengebiet zu erfassen. Hierzu wurde ein fachübergreifender Ansatz am Fallbeispiel der Stadt Windhoek, Namibia, gewählt. Die Arbeit umfasst eine detaillierte Literaturanalyse der aktuellen Forschungsansätze zur urbanen Wassererosion und den damit verbundenen Herausforderungen. Außerdem wurde eine feldstudienbasierte Methode entwickelt, mit der das Ausmaß der Wassererosion in der Stadt Windhoek quantifiziert und räumlich erfasst wurde. Schließlich wurden persönliche Befragungen mit halbstrukturierten Fragebögen durchgeführt, um die Wahrnehmung der verschiedenen Interessenvertreter zum Thema Erosion in Stadtgebieten zu analysieren.

Die Literaturanalyse hat gezeigt, dass 64% der untersuchten Studien in der entwickelten Welt durchgeführt wurden und nur sehr wenige Regionen mit extremen Klimabedingungen, einschließlich Trockengebieten, untersucht wurden. Hinzu kommt, dass die verwendeten Methoden zur Erosionsquantifizierung und -beobachtung die für urbane Gebiete typischen Merkmale nicht beinhalten und dafür auch nicht ausgerichtet sind. Des Weiteren mangelt es der untersuchten Literatur an Ansätzen, die den Einfluss des Klimawandels und politische Aspekte in Bezug auf Erosion in Stadtgebieten thematisieren. In einer Feldstudie wurde das Ausmaß von Wassererosion in der trocken gelegenen Stadt Windhoek quantifiziert und räumlich erfasst. Beinahe 56% der Stadt waren von Wassererosion betroffen und wiesen Anzeichen beschleunigter Erosion in Form von Rinnen und Rillen auf. Letztere traten vor allem in den unterentwickelten, informellen und semi-formellen Stadtgebieten auf. Das Ausmaß der Erosion in Windhoek wurde unter anderem von der Vegetationsbedeckung und dem Vegetationstyp, von sozial-urbanen Faktoren, und zu einem geringeren Grad von dem geschätzten Gefälle bestimmt. Der Vergleich einer interpolierten feldstudienbasierten Erosionskarte mit Ergebnissen, die auf einer konventionellen Methode zur Erosionserfassung (der Allgemeinen Bodenabtragsgleichung (ABAG)) basieren, ergab eine starke Abweichung in den räumlichen Mustern. Das verdeutlicht die Unzulänglichkeit einer direkten Übertragung von traditionellen nicht-urbanen Methoden zur Erosionserfassung auf ein urbanes Umfeld und betont die Notwendigkeit, neue Methoden sowohl zur Erfassung als auch zum Management von Erosion für urbane Gebiete zu entwickeln. Aus der großen Variabilität des Erosionsausmaßes innerhalb der Stadt lässt sich folgern, dass Methoden zur Kontrolle von Wassererosion in Städten standortspezifisch sein sollten.

Anhand von halbstrukturierten Fragebögen wurde in einem weiteren Teil der Arbeit die Wahrnehmung und das Verständnis der unterschiedlichen Interessenvertreter zum Thema urbane Wassererosion in Windhoek untersucht. Insgesamt wurden 41 Interessenvertreter zu ihrem Verständnis der Wassererosionsdynamiken, zu ihrer Wahrnehmung in Bezug auf mögliche Ursachen und zum Ausmaß der Erosionsschäden, sowie zu ihrer Einstellung zur Verantwortlichkeit für die Erosion in der Stadt befragt. Die Ergebnisse deuten darauf hin, dass es eine geringe Wahrnehmung für das Phänomen der Erosion als Prozess gibt, dafür aber eine im Vergleich erhöhte Wahrnehmung der Erosionsschäden und der Faktoren, die zu den Schäden beitragen. Ungefähr 69% der Interessenvertreter stuften die Erosionsschäden als moderat bis sehr ernsthaft ein. Dabei gab es erkennbare Differenzen zwischen der Gruppe der privaten Haushalte und der der öffentlichen Behörden. Des Weiteren hat die Untersuchung ergeben, dass die Interessenvertreter kein klares Verständnis ihrer Verantwortung in Bezug auf das Management der Kontrollmaßnahmen, sowie ihrer finanziellen Verantwortung für die Schäden haben. Die privaten Haushalte und die örtlichen Behörden wiesen sich gegenseitig die Zahlungsverantwortung für die Erosionsschäden und für vorbeugende Maßnahmen zu. Der Unwille der einzelnen Akteure, Verantwortung zu übernehmen, könnte eine Zwickmühle für die betroffenen Gebiete werden. Dies gilt insbesondere für die informellen Siedlungen, in denen von den örtlichen Behörden kein Landmanagement durchgeführt wird, das Land aber auch nicht Eigentum der Bewohnern ist.

Abschließend hat die Studie ergeben, dass es für eine effektive Erosionsbekämpfung in der Stadt von ausschlaggebender Bedeutung ist, die verschiedenen, den Prozess der Urbanisierung auf negative Weise verstärkenden Dynamiken, auf ihren unterschiedlichen Skalen zu verstehen. Auf Grundlage der hier präsentierten Ergebnisse wird eine Entwicklung speziell auf Stadtgebiete ausgerichteter Ansätze mit folgenden Zielen dringend nahegelegt: (a) Einer Integration von diversen sozio-ökonomisch-ökologischen Aspekten, die sich auf Erosion auswirken; (b) Einer wissenschaftlich begründeten Verbesserung der natürlichen Kreisläufe, die sich positiv auf die Wasserspeicherung im Boden und die Nährstoffverfügbarkeit für Pflanzen auswirken, um dadurch einen höheren Vegetationsbedeckungsgrad zu erreichen; (c) Der Nutzung hoch aufgelöster Satellitendaten, um die Methoden zur Erosionserfassung für urbane Gebiete zu verbessern; (d) Der Entwicklung politischer Maßnahmen zur Bekämpfung von Wassererosion.
KW  - urban soil erosion
KW  - water erosion
KW  - risk mapping
KW  - urbane Bodenerosion
KW  - Wassererosion
KW  - Risikoabbildung
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-102356
ER  - 
TY  - THES
A1  - Kersten, Birgit
T1  - Proteom-weite Studien zur Phosphorylierung pflanzlicher Proteine mittels Proteinmikroarrays und Bioinformatik
Y1  - 2016
ER  - 
TY  - JOUR
A1  - Schmidt, Andreas
A1  - Rabsch, Wolfgang
A1  - Broeker, Nina K.
A1  - Barbirz, Stefanie
T1  - Bacteriophage tailspike protein based assay to monitor phase variable glucosylations in Salmonella O-antigens
JF  - BMC microbiology
N2  - Background

Non-typhoid Salmonella Typhimurium (S. Typhimurium) accounts for a high number of registered salmonellosis cases, and O-serotyping is one important tool for monitoring epidemiology and spread of the disease. Moreover, variations in glucosylated O-antigens are related to immunogenicity and spread in the host. However, classical autoagglutination tests combined with the analysis of specific genetic markers cannot always reliably register phase variable glucose modifications expressed on Salmonella O-antigens and additional tools to monitor O-antigen glucosylation phenotypes of S. Typhimurium would be desirable.

Results

We developed a test for the phase variable O-antigen glucosylation state of S. Typhimurium using the tailspike proteins (TSP) of Salmonella phages 9NA and P22. We used this ELISA like tailspike adsorption (ELITA) assay to analyze a library of 44 Salmonella strains. ELITA was successful in discriminating strains that carried glucose 1-6 linked to the galactose of O-polysaccharide backbone (serotype O1) from non-glucosylated strains. This was shown by O-antigen compositional analyses of the respective strains with mass spectrometry and capillary electrophoresis. The ELITA test worked rapidly in a microtiter plate format and was highly O-antigen specific. Moreover, TSP as probes could also detect glucosylated strains in flow cytometry and distinguish multiphasic cultures differing in their glucosylation state.

Conclusions

Tailspike proteins contain large binding sites with precisely defined specificities and are therefore promising tools to be included in serotyping procedures as rapid serotyping agents in addition to antibodies. In this study, 9NA and P22TSP as probes could specifically distinguish glucosylation phenotypes of Salmonella on microtiter plate assays and in flow cytometry. This opens the possibility for flow sorting of cell populations for subsequent genetic analyses or for monitoring phase variations during large scale O-antigen preparations necessary for vaccine production.
KW  - Salmonella Typhimurium
KW  - O-antigen
KW  - Tailspike protein
KW  - Bacteriophage
KW  - Phase variation
KW  - O-serotyping
KW  - Flow cytometry
Y1  - 2016
U6  - https://doi.org/10.1186/s12866-016-0826-0
SN  - 1471-2180
VL  - 16
PB  - BioMed Central
CY  - London
ER  - 
TY  - THES
A1  - Reichel, Victoria Eleonore
T1  - Biomedical applications and multifunctional nanostructures based on magnetite nanoparticles synthesized in presence of biological additives
Y1  - 2016
ER  - 
TY  - THES
A1  - Heinze, Johannes
T1  - The impact of soil microbiota on plant species performance and diversity in semi-natural grasslands
Y1  - 2016
ER  - 
TY  - THES
A1  - Wutke, Saskia
T1  - Tracing Changes in Space and Time
BT  - Paternal Diversity and Phenotypic Traits during Horse Domestication
N2  - The horse is a fascinating animal symbolizing power, beauty, strength and grace. Among all the animal species domesticated the horse had the largest impact on the course of human history due to its importance for warfare and transportation. Studying the process of horse domestication contributes to the knowledge about the history of horses and even of our own species.
Research based on molecular methods has increasingly focused on the genetic basis of horse domestication. Mitochondrial DNA (mtDNA) analyses of modern and ancient horses detected immense maternal diversity, probably due to many mares that contributed to the domestic population. However, mtDNA does not provide an informative phylogeographic structure. In contrast, Y chromosome analyses displayed almost complete uniformity in modern stallions but relatively high diversity in a few ancient horses. Further molecular markers that seem to be well suited to infer the domestication history of horses or genetic and phenotypic changes during this process are loci associated with phenotypic traits.
This doctoral thesis consists of three different parts for which I analyzed various single nucleotide polymorphisms (SNPs) associated with coat color, locomotion or Y chromosomal variation of horses. These SNPs were genotyped in 350 ancient horses from the Chalcolithic (5,000 BC) to the Middle Ages (11th century). The distribution of the samples ranges from China to the Iberian Peninsula and Iceland. By applying multiplexed next-generation sequencing (NGS) I sequenced short amplicons covering the relevant positions: i) eight coat-color-associated mutations in six genes to deduce the coat color phenotype; ii) the so-called ’Gait-keeper’ SNP in the DMRT3 gene to screen for the ability to amble; iii) 16 SNPs previously detected in ancient horses to infer the corresponding haplotype. Based on these data I investigated the occurrence and frequencies of alleles underlying the respective phenotypes as well as Y chromosome haplotypes at different times and regions. Also, selection coefficients for several Y chromosome lineages or phenotypes were estimated.
Concerning coat color differences in ancient horses my work constitutes the most comprehensive study to date. I detected an increase of chestnut horses in the Middle Ages as well as differential selection for spotted and solid phenotypes over time which reflects changing human preferences.
With regard to ambling horses, the corresponding allele was present in medieval English and Icelandic horses. Based on these results I argue that Norse settlers, who frequently invaded parts of Britain, brought ambling individuals to Iceland from the British Isles which can be regarded the origin of this trait. Moreover, these settlers appear to have selected for ambling in Icelandic horses.
Relating to the third trait, the paternal diversity, these findings represent the largest ancient dataset of Y chromosome variation in non-humans. I proved the existence of several Y chromosome haplotypes in early domestic horses. The decline of Y chromosome variation coincides with the movement of nomadic peoples from the Eurasian steppes and later with different breeding practices in the Roman period.
In conclusion, positive selection was estimated for several phenotypes/lineages
in different regions or times which indicates that these were preferred by humans. Furthermore, I could successfully infer the distribution and dispersal of horses in association with human movements and actions. Thereby, a better understanding of the influence of people on the changing appearance and genetic diversity of domestic horses could be gained. My results also emphasize the close relationship of ancient genetics and archeology or history and that only in combination well-founded conclusions can be reached.
KW  - ancient DNA
KW  - domestication
KW  - horse
KW  - equus caballus
KW  - locomotion
KW  - Y chromosome
KW  - coat colour
Y1  - 2016
ER  - 
TY  - THES
A1  - Avcilar-Kucukgoze, Irem
T1  - Effect of tRNA Aminoacylation and Cellular Resources Allocation on the Dynamics of Translation in Escherichia coli
Y1  - 2016
ER  - 
TY  - THES
A1  - Hofferek, Vinzenz
T1  - Starvation response of Drosophila melanogaster
BT  - a Lipidomic Approach
Y1  - 2016
ER  - 
TY  - GEN
A1  - Lah, Ljerka
A1  - Trense, Daronja
A1  - Benke, Harald
A1  - Berggren, Per
A1  - Gunnlaugsson, Þorvaldur
A1  - Lockyer, Christina
A1  - Öztürk, Ayaka
A1  - Öztürk, Bayram
A1  - Pawliczka, Iwona
A1  - Roos, Anna
A1  - Siebert, Ursula
A1  - Skóra, Krzysztof
A1  - Víkingsson, Gísli
A1  - Tiedemann, Ralph
T1  - Spatially Explicit Analysis of Genome-Wide SNPs Detects Subtle Population Structure in a Mobile Marine Mammal, the Harbor Porpoise
N2  - The population structure of the highly mobile marine mammal, the harbor porpoise (Phocoena phocoena), in the Atlantic shelf waters follows a pattern of significant isolation-by-distance. The population structure of harbor porpoises from the Baltic Sea, which is connected with the North Sea through a series of basins separated by shallow underwater ridges, however, is more complex. Here, we investigated the population differentiation of harbor porpoises in European Seas with a special focus on the Baltic Sea and adjacent waters, using a population genomics approach. We used 2872 single nucleotide polymorphisms (SNPs), derived from double digest restriction-site associated DNA sequencing (ddRAD-seq), as well as 13 microsatellite loci and mitochondrial haplotypes for the same set of individuals. Spatial principal components analysis (sPCA), and Bayesian clustering on a subset of SNPs suggest three main groupings at the level of all studied regions: the Black Sea, the North Atlantic, and the Baltic Sea. Furthermore, we observed a distinct separation of the North Sea harbor porpoises from the Baltic Sea populations, and identified splits between porpoise populations within the Baltic Sea. We observed a notable distinction between the Belt Sea and the Inner Baltic Sea sub-regions. Improved delineation of harbor porpoise population assignments for the Baltic based on genomic evidence is important for conservation management of this endangered cetacean in threatened habitats, particularly in the Baltic Sea proper. In addition, we show that SNPs outperform microsatellite markers and demonstrate the utility of RAD-tags from a relatively small, opportunistically sampled cetacean sample set for population diversity and divergence analysis.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 295 
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-100813
SN  - 1866-8372
ER  - 
TY  - GEN
A1  - Zhu, Fangjun
A1  - Schlupp, Ingo
A1  - Tiedemann, Ralph
T1  - Sequence Evolution and Expression of the Androgen Receptor and Other Pathway-Related Genes in a Unisexual Fish, the Amazon Molly, Poecilia formosa, and Its Bisexual Ancestors
N2  - The all-female Amazon molly (Poecilia formosa) originated from a single hybridization of two bisexual ancestors, Atlantic molly (Poecilia mexicana) and sailfin molly (Poecilia latipinna). As a gynogenetic species, the Amazon molly needs to copulate with a heterospecific male, but the genetic information of the sperm-donor does not contribute to the next generation, as the sperm only acts as the trigger for the diploid eggs’ embryogenesis. Here, we study the sequence evolution and gene expression of the duplicated genes coding for androgen receptors (ars) and other pathway-related genes, i.e., the estrogen receptors (ers) and cytochrome P450, family19, subfamily A, aromatase genes (cyp19as), in the Amazon molly, in comparison to its bisexual ancestors. Mollies possess–as most other teleost fish—two copies of the ar, er, and cyp19a genes, i.e., arα/arβ, erα/erβ1, and cyp19a1 (also referred as cyp19a1a)/cyp19a2 (also referred to as cyp19a1b), respectively. Non-synonymous single nucleotide polymorphisms (SNPs) among the ancestral bisexual species were generally predicted not to alter protein function. Some derived substitutions in the P. mexicana and one in P. formosa are predicted to impact protein function. We also describe the gene expression pattern of the ars and pathway-related genes in various tissues (i.e., brain, gill, and ovary) and provide SNP markers for allele specific expression research. As a general tendency, the levels of gene expression were lowest in gill and highest in ovarian tissues, while expression levels in the brain were intermediate in most cases. Expression levels in P. formosa were conserved where expression did not differ between the two bisexual ancestors. In those cases where gene expression levels significantly differed between the bisexual species, P. formosa expression was always comparable to the higher expression level among the two ancestors. Interestingly, erβ1 was expressed neither in brain nor in gill in the analyzed three molly species, which implies a more important role of erα in the estradiol synthesis pathway in these tissues. Furthermore, our data suggest that interactions of steroid-signaling pathway genes differ across tissues, in particular the interactions of ars and cyp19as.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 265 
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-97119
ER  - 
TY  - JOUR
A1  - Brzezinka, Krzysztof
A1  - Altmann, Simone
A1  - Czesnick, Hjördis
A1  - Nicolas, Philippe
A1  - Gorka, Michal
A1  - Benke, Eileen
A1  - Kabelitz, Tina
A1  - Jähne, Felix
A1  - Graf, Alexander
A1  - Kappel, Christian
A1  - Bäurle, Isabel
T1  - Arabidopsis FORGETTER1 mediates stress-induced chromatin memory through nucleosome remodeling
JF  - eLife
N2  - Plants as sessile organisms can adapt to environmental stress to mitigate its adverse effects. As part of such adaptation they maintain an active memory of heat stress for several days that promotes a more efficient response to recurring stress. We show that this heat stress memory requires the activity of the FORGETTER1 (FGT1) locus, with fgt1 mutants displaying reduced maintenance of heat-induced gene expression. FGT1 encodes the Arabidopsis thaliana orthologue of Strawberry notch (Sno), and the protein globally associates with the promoter regions of actively expressed genes in a heat-dependent fashion. FGT1 interacts with chromatin remodelers of the SWI/ SNF and ISWI families, which also display reduced heat stress memory. Genomic targets of the BRM remodeler overlap significantly with FGT1 targets. Accordingly, nucleosome dynamics at loci with altered maintenance of heat-induced expression are affected in fgt1. Together, our results suggest that by modulating nucleosome occupancy, FGT1 mediates stress-induced chromatin memory.
Y1  - 2016
U6  - https://doi.org/10.7554/eLife.17061
SN  - 2050-084X
VL  - 5
PB  - eLife Sciences Publications
CY  - Cambridge
ER  - 
TY  - THES
A1  - Stief, Anna
T1  - Genetics and ecology of plant heat stress memory
Y1  - 2016
ER  - 
TY  - THES
A1  - Brzezinka, Krzysztof
T1  - Chromatin dynamics during heat stress memory in plants
Y1  - 2016
ER  - 
TY  - JOUR
A1  - Schlägel, Ulrike E.
A1  - Lewis, Mark A.
T1  - A framework for analyzing the robustness of movement models to variable step discretization
JF  - Journal of mathematical biology
N2  - When sampling animal movement paths, the frequency at which location measurements are attempted is a critical feature for data analysis. Important quantities derived from raw data, e.g. travel distance or sinuosity, can differ largely based on the temporal resolution of the data. Likewise, when movement models are fitted to data, parameter estimates have been demonstrated to vary with sampling rate. Thus, biological statements derived from such analyses can only be made with respect to the resolution of the underlying data, limiting extrapolation of results and comparison between studies. To address this problem, we investigate whether there are models that are robust against changes in temporal resolution. First, we propose a mathematically rigorous framework, in which we formally define robustness as a model property. We then use the framework for a thorough assessment of a range of basic random walk models, in which we also show how robustness relates to other probabilistic concepts. While we found robustness to be a strong condition met by few models only, we suggest a new method to extend models so as to make them robust. Our framework provides a new systematic, mathematically founded approach to the question if, and how, sampling rate of movement paths affects statistical inference.
KW  - Animal movement
KW  - Random walk
KW  - Sampling rate
KW  - Discretization
KW  - GPS data
KW  - Parameter estimation
Y1  - 2016
U6  - https://doi.org/10.1007/s00285-016-0969-5
SN  - 0303-6812
SN  - 1432-1416
VL  - 73
SP  - 815
EP  - 845
PB  - Springer
CY  - Heidelberg
ER  - 
TY  - JOUR
A1  - Schlägel, Ulrike E.
A1  - Lewis, Mark A.
T1  - Robustness of movement models: can models bridge the gap between temporal scales of data sets and behavioural processes?
JF  - Journal of mathematical biology
KW  - Animal movement
KW  - Sampling rate
KW  - Resource selection
KW  - GPS data
KW  - Parameter estimation
KW  - Markov model
Y1  - 2016
U6  - https://doi.org/10.1007/s00285-016-1005-5
SN  - 0303-6812
SN  - 1432-1416
VL  - 73
SP  - 1691
EP  - 1726
PB  - Springer
CY  - Heidelberg
ER  - 
TY  - JOUR
A1  - Lamanna, Francesco
A1  - Kirschbaum, Frank
A1  - Ernst, Anja R. R.
A1  - Feulner, Philine G. D.
A1  - Mamonekene, Victor
A1  - Paul, Christiane
A1  - Tiedemann, Ralph
T1  - Species delimitation and phylogenetic relationships in a genus of African weakly-electric fishes (Osteoglossiformes, Mormyridae, Campylomormyrus)
JF  - Molecular phylogenetics and evolution
N2  - African weakly-electric fishes (Mormyridae) are able to communicate through species-specific electric signals; this feature might have favoured the evolutionary radiation observed in this family (over 200 species) by acting as an effective pre-zygotic isolation mechanism. In the present study we used mitochondria((cytb) and nuclear (rps7, scn4aa) markers in order to reconstruct a species-phylogeny and identify species boundaries for the genus Campylomormyrus, by applying inference methods based on the multispecies coalescent model. Additionally, we employed 16 microsatellite markers, landmark-based morphometric measurements, and electro-physiological analyses as independent lines of evidence to the results obtained from the sequence data. The results show that groups that are morphologically different are also significantly divergent at the genetic level, whereas morphologically similar groups, displaying dissimilar electric signals, do not show enough genetic diversity to be considered separate species. Furthermore, the data confirm the presence of a yet undescribed species within the genus Campylomormyrus. (C) 2016 Elsevier Inc. All rights reserved.
KW  - Mormyridae
KW  - Multispecies-coalescent
KW  - Campylomormyrus
KW  - Geometric morphometrics
KW  - Microsatellites
KW  - Species-delimitation
Y1  - 2016
U6  - https://doi.org/10.1016/j.ympev.2016.04.035
SN  - 1055-7903
SN  - 1095-9513
VL  - 101
SP  - 8
EP  - 18
PB  - Elsevier
CY  - San Diego
ER  - 
TY  - JOUR
A1  - Paul, Christiane
A1  - Kirschbaum, Frank
A1  - Mamonekene, Victor
A1  - Tiedemann, Ralph
T1  - Evidence for Non-neutral Evolution in a Sodium Channel Gene in African Weakly Electric Fish (Campylomormyrus, Mormyridae)
JF  - Journal of molecular evolution
N2  - Voltage-gated sodium channels, Nav1, play a crucial role in the generation and propagation of action potentials and substantially contribute to the shape of their rising phase. The electric organ discharge (EOD) of African weakly electric fish (Mormyroidea) is the sum of action potentials fired from all electrocytes of the electric organ at the same time and hence voltage-gated sodium channels are one factor—together with the electrocyte’s morphology and innervation pattern—that determines the properties of these EODs. Due to the fish-specific genome duplication, teleost fish possess eight copies of sodium channel genes (SCN), which encode for Nav1 channels. In mormyroids, SCN4aa is solely expressed in the electrocytes of the adult electric organ. In this study, we compared entire SCN4aa sequences of six species of the genus Campylomormyrus and identified nonsynonymous substitutions among them. SCN4aa in Campylomormyrus exhibits a much higher evolutionary rate compared to its paralog SCN4ab, whose expression is not restricted to the electric organ. We also found evidence for strong positive selection on the SCN4aa gene within Mormyridae and along the lineage ancestral to the Mormyridae. We have identified sites at which all nonelectric teleosts are monomorphic in their amino acid, but mormyrids have different amino acids. Our findings confirm the crucial role of SCN4aa in EOD evolution among mormyrid weakly electric fish. The inferred positive selection within Mormyridae makes this gene a prime candidate for further investigation of the divergent evolution of pulse-type EODs among closely related species.
KW  - Mormyridae
KW  - Mormyroidea
KW  - Campylomormyrus
KW  - SCN4aa
KW  - Voltage-gated sodium channel
KW  - Positive selection
Y1  - 2016
U6  - https://doi.org/10.1007/s00239-016-9754-8
SN  - 0022-2844
SN  - 1432-1432
VL  - 83
SP  - 61
EP  - 77
PB  - Springer
CY  - New York
ER  - 
TY  - JOUR
A1  - Hartmann, Bianca
A1  - Wai, Timothy
A1  - Hu, Hao
A1  - MacVicar, Thomas
A1  - Musante, Luciana
A1  - Fischer-Zirnsak, Björn
A1  - Stenzel, Werner
A1  - Gräf, Ralph
A1  - van den Heuvel, Lambert
A1  - Ropers, Hans-Hilger
A1  - Wienker, Thomas F.
A1  - Hübner, Christoph
A1  - Langer, Thomas
A1  - Kaindl, Angela M.
T1  - Homozygous YME1L1 Mutation Causes Mitochondriopathy with Optic Atrophy and Mitochondrial Network Fragmentation
JF  - eLife
N2  - Mitochondriopathies often present clinically as multisystemic disorders of primarily high-energy consuming organs. Assembly, turnover, and surveillance of mitochondrial proteins are essential for mitochondrial function and a key task of AAA family members of metalloproteases. We identified a homozygous mutation in the nuclear encoded mitochondrial escape 1-like 1 gene YME1L1, member of the AAA protease family, as a cause of a novel mitochondriopathy in a consanguineous pedigree of Saudi Arabian descent. The homozygous missense mutation, located in a highly conserved region in the mitochondrial pre-sequence, inhibits cleavage of YME1L1 by the mitochondrial processing peptidase, which culminates in the rapid degradation of YME1L1 precursor protein. Impaired YME1L1 function causes a proliferation defect and mitochondrial network fragmentation due to abnormal processing of OPA1. Our results identify mutations in YME1L1 as a cause of a mitochondriopathy with optic nerve atrophy highlighting the importance of YME1L1 for mitochondrial functionality in humans.
KW  - YME1L1
KW  - mitochondriopathy
KW  - intellectual disability
KW  - optic atrophy
KW  - OPA1
KW  - mitochondrial fragmentation
Y1  - 2016
U6  - https://doi.org/10.7554/eLife.16078
SN  - 2050-084X
VL  - 5
SP  - 1156
EP  - 1165
PB  - eLife Sciences Publications
CY  - Cambridge
ER  - 
TY  - JOUR
A1  - Putzler, Sascha
A1  - Meyer, Irene
A1  - Gräf, Ralph
T1  - CP91 is a component of the Dictyostelium centrosome involved in centrosome biogenesis
JF  - European journal of cell biology
N2  - The Dictyostelium centrosome is a model for acentriolar centrosomes and it consists of a three-layered core structure surrounded by a corona harboring microtubule nucleation complexes. Its core structure duplicates once per cell cycle at the G2/M transition. Through proteomic analysis of isolated centrosomes we have identified CP91, a 91-kDa coiled coil protein that was localized at the centrosomal core structure. While GFP-CP91 showed almost no mobility in FRAP experiments during interphase, both GFP-CP91 and endogenous CP91 dissociated during mitosis and were absent from spindle poles from late prophase to anaphase. Since this behavior correlates with the disappearance of the central layer upon centrosome duplication, CP91 is a putative component of this layer. When expressed as GFP-fusions, CP91 fragments corresponding to the central coiled coil domain and the preceding N-terminal part (GFP-CP91cc and GFP-CP91N, respectively) also localized to the centrosome but did not show the mitotic redistribution of the full length protein suggesting a regulatory role of the C-terminal domain. Expression of all GFP-fusion proteins suppressed expression of endogenous CP91 and elicited supernumerary centrosomes. This was also very prominent upon depletion of CP91 by RNAi. Additionally, CP91-RNAi cells exhibited heavily increased ploidy due to severe defects in chromosome segregation along with increased cell size and defects in the abscission process during cytokinesis. Our results indicate that CP91 is a central centrosomal core component required for centrosomal integrity, proper centrosome biogenesis and, independently, for abscission during cytokinesis. (c) 2016 Elsevier GmbH. All rights reserved.
KW  - Dictyostelium
KW  - Mitosis
KW  - Microtubules
KW  - Centrosome
KW  - Nucleus
Y1  - 2016
U6  - https://doi.org/10.1016/j.ejcb.2016.03.001
SN  - 0171-9335
SN  - 1618-1298
VL  - 95
SP  - 124
EP  - 135
PB  - Royal Society
CY  - Jena
ER  - 
TY  - GEN
A1  - Batsios, Petros
A1  - Ren, Xiang
A1  - Baumann, Otto
A1  - Larochelle, Denis A.
A1  - Gräf, Ralph
T1  - Src1 is a Protein of the Inner Nuclear Membrane Interacting with the Dictyostelium Lamin NE81
N2  - The nuclear envelope (NE) consists of the outer and inner nuclear membrane (INM), whereby the latter is bound to the nuclear lamina. Src1 is a Dictyostelium homologue of the helix-extension-helix family of proteins, which also includes the human lamin-binding protein MAN1. Both endogenous Src1 and GFP-Src1 are localized to the NE during the entire cell cycle. Immuno-electron microscopy and light microscopy after differential detergent treatment indicated that Src1 resides in the INM. FRAP experiments with GFP-Src1 cells suggested that at least a fraction of the protein could be stably engaged in forming the nuclear lamina together with the Dictyostelium lamin NE81. Both a BioID proximity assay and mis-localization of soluble, truncated mRFP-Src1 at cytosolic clusters consisting of an intentionally mis-localized mutant of GFP-NE81 confirmed an interaction of Src1 and NE81. Expression GFP-Src11–646, a fragment C-terminally truncated after the first transmembrane domain, disrupted interaction of nuclear membranes with the nuclear lamina, as cells formed protrusions of the NE that were dependent on cytoskeletal pulling forces. Protrusions were dependent on intact microtubules but not actin filaments. Our results indicate that Src1 is required for integrity of the NE and highlight Dictyostelium as a promising model for the evolution of nuclear architecture.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 263 
KW  - Dictyostelium
KW  - HeH-protein
KW  - LEM-domain protein
KW  - lamin
KW  - nuclear lamina
KW  - nucleolus
KW  - nucleus
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-97033
ER  - 
TY  - JOUR
A1  - Batsios, Petros
A1  - Ren, Xiang
A1  - Baumann, Otto
A1  - Larochelle, Denis A.
A1  - Gräf, Ralph
T1  - Src1 is a Protein of the Inner Nuclear Membrane Interacting with the Dictyostelium Lamin NE81
JF  - Cells
N2  - The nuclear envelope (NE) consists of the outer and inner nuclear membrane (INM), whereby the latter is bound to the nuclear lamina. Src1 is a Dictyostelium homologue of the helix-extension-helix family of proteins, which also includes the human lamin-binding protein MAN1. Both endogenous Src1 and GFP-Src1 are localized to the NE during the entire cell cycle. Immuno-electron microscopy and light microscopy after differential detergent treatment indicated that Src1 resides in the INM. FRAP experiments with GFP-Src1 cells suggested that at least a fraction of the protein could be stably engaged in forming the nuclear lamina together with the Dictyostelium lamin NE81. Both a BioID proximity assay and mis-localization of soluble, truncated mRFP-Src1 at cytosolic clusters consisting of an intentionally mis-localized mutant of GFP-NE81 confirmed an interaction of Src1 and NE81. Expression GFP-Src11–646, a fragment C-terminally truncated after the first transmembrane domain, disrupted interaction of nuclear membranes with the nuclear lamina, as cells formed protrusions of the NE that were dependent on cytoskeletal pulling forces. Protrusions were dependent on intact microtubules but not actin filaments. Our results indicate that Src1 is required for integrity of the NE and highlight Dictyostelium as a promising model for the evolution of nuclear architecture.
KW  - Dictyostelium
KW  - lamin
KW  - nuclear lamina
KW  - nucleus
KW  - nucleolus
KW  - HeH-protein
KW  - LEM-domain protein
Y1  - 2016
U6  - https://doi.org/10.3390/cells5010013
SN  - 2073-4409
VL  - 5
IS  - 1
PB  - MDPI
CY  - Basel
ER  - 
TY  - JOUR
A1  - Edlich, Alexander
A1  - Gerecke, Christian
A1  - Giulbudagian, Michael
A1  - Neumann, Falko
A1  - Hedtrich, Sarah
A1  - Schaefer-Korting, Monika
A1  - Ma, Nan
A1  - Calderon, Marcelo
A1  - Kleuser, Burkhard
T1  - Specific uptake mechanisms of well-tolerated thermoresponsive polyglycerol-based nanogels in antigen-presenting cells of the skin
JF  - European Journal of Pharmaceutics and Biopharmaceutics
N2  - Engineered nanogels are of high value for a targeted and controlled transport of compounds due to the ability to change their chemical properties by external stimuli. As it has been indicated that nanogels possess a high ability to penetrate the stratum corneum, it cannot be excluded that nanogels interact with dermal dendritic cells, especially in diseased skin. In this study the potential crosstalk of the thermore-sponsive nanogels (tNGs) with the dendritic cells of the skin was investigated with the aim to determine the immunotoxicological properties of the nanogels. The investigated tNGs were made of dendritic polyglycerol (dPG) and poly(glycidyl methyl ether-co-ethyl glycidyl ether) (p(GME-co-EGE)), as polymer conferring thermoresponsive properties. Although the tNGs were taken up, they displayed neither cytotoxic and genotoxic effects nor any induction of reactive oxygen species in the tested cells. Interestingly, specific uptake mechanisms of the tNGs by the dendritic cells were depending on the nanogels cloud point temperature (Tcp), which determines the phase transition of the nanoparticle. The study points to caveolae-mediated endocytosis as being the major tNGs uptake mechanism at 37 degrees C, which is above the Tcp of the tNGs. Remarkably, an additional uptake mechanism, beside caveolae-mediated endocytosis, was observed at 29 degrees C, which is the Tcp of the tNGs. At this temperature, which is characterized by two different states of the tNGs, macropinocytosis was involved as well. In summary, our study highlights the impact of thermoresponsivity on the cellular uptake mechanisms which has to be taken into account if the tNGs are used as a drug delivery system.
KW  - Dendritic cells
KW  - Drug delivery systems
KW  - Nanogel
KW  - Nanoparticle
KW  - Nanoparticle uptake
KW  - Nanotoxicology
Y1  - 2017
U6  - https://doi.org/10.1016/j.ejpb.2016.12.016
SN  - 0939-6411
SN  - 1873-3441
VL  - 116
SP  - 155
EP  - 163
PB  - Elsevier
CY  - Amsterdam
ER  - 
TY  - JOUR
A1  - Heinze, Johannes
A1  - Gensch, Sabine
A1  - Weber, Ewald
A1  - Joshi, Jasmin Radha
T1  - Soil temperature modifies effects of soil biota on plant growth
JF  - Journal of plant ecology
N2  - Aims Plants directly and indirectly interact with many abiotic and biotic soil components. Research so far mostly focused on direct, individual abiotic or biotic effects on plant growth, but only few studies tested the indirect effects of abiotic soil factors on plant growth. Therefore, we investigated how abiotic soil conditions affect plant performance, via changes induced by soil biota. Methods In a full-factorial experiment, we grew the widespread grass Dactylis glomerata either with or without soil biota and investigated the impact of soil temperature, fertility and moisture on the soil biota effects on plant growth. We measured biomass production, root traits and colonization by arbuscular mycorrhizal fungi as well as microbial respiration. Important Findings We found significant interaction effects between abiotic soil conditions and soil biota on plant growth for fertility, but especially for soil temperature, as an increase of 10 degrees C significantly changed the soil biota effects on plant growth from positive to neutral. However, if tested individually, an increase in soil temperature and fertility per se positively affected plant biomass production, whereas soil biota per se did not affect overall plant growth, but both influenced root architecture. By affecting soil microbial activity and root architecture, soil temperature might influence both mutualistic and pathogenic interactions between plants and soil biota. Such soil temperature effects should be considered in soil feedback studies to ensure greater transferability of results from artificial and experimental conditions to natural environmental conditions.
KW  - plant-soil interaction
KW  - soil biota
KW  - abiotic soil factors
KW  - root traits
KW  - plant growth
Y1  - 2016
U6  - https://doi.org/10.1093/jpe/rtw097
SN  - 1752-9921
SN  - 1752-993X
VL  - 10
SP  - 808
EP  - 821
PB  - Oxford Univ. Press
CY  - Oxford
ER  - 
TY  - JOUR
A1  - Dellinger, Agnes S.
A1  - Essl, Franz
A1  - Hojsgaard, Diego
A1  - Kirchheimer, Bernhard
A1  - Klatt, Simone
A1  - Dawson, Wayne
A1  - Pergl, Jan
A1  - Pysek, Petr
A1  - van Kleunen, Mark
A1  - Weber, Ewald
A1  - Winter, Marten
A1  - Hoerandl, Elvira
A1  - Dullinger, Stefan
T1  - Niche dynamics of alien species do not differ among sexual and apomictic flowering plants
JF  - New phytologist : international journal of plant science
N2  - We compiled global occurrence data sets of 13 congeneric sexual and apomictic species pairs, and used principal components analysis (PCA) and kernel smoothers to compare changes in climatic niche optima, breadths and unfilling/expansion between native and alien ranges. Niche change metrics were compared between sexual and apomictic species. All 26 species showed changes in niche optima and/or breadth and 14 species significantly expanded their climatic niches. However, we found no effect of the reproductive system on niche dynamics. Instead, species with narrower native niches showed higher rates of niche expansion in the alien ranges. Our results suggest that niche shifts are frequent in plant invasions but evolutionary potential may not be of major importance for such shifts. Niche dynamics rather appear to be driven by changes of the realized niche without adaptive change of the fundamental climatic niche.
KW  - adaptation
KW  - asexual reproduction
KW  - niche shifts
KW  - plant invasion
KW  - reproductive system
KW  - species distribution modelling
Y1  - 2016
U6  - https://doi.org/10.1111/nph.13694
SN  - 0028-646X
SN  - 1469-8137
VL  - 209
SP  - 1313
EP  - 1323
PB  - Wiley-Blackwell
CY  - Hoboken
ER  - 
TY  - JOUR
A1  - Westbury, Michael V.
A1  - Prost, Stefan
A1  - Seelenfreund, Andrea
A1  - Ramirez, Jose-Miguel
A1  - Matisoo-Smith, Elizabeth A.
A1  - Knapp, Michael
T1  - First complete mitochondrial genome data from ancient South American camelids - The mystery of the chilihueques from Isla Mocha (Chile)
JF  - Scientific reports
Y1  - 2016
U6  - https://doi.org/10.1038/srep38708
SN  - 2045-2322
VL  - 6
PB  - Nature Publ. Group
CY  - London
ER  - 
TY  - THES
A1  - Mengin, Virginie
T1  - Role of the clock in the regulation of growth and metabolism in stable and fluctuating environmental conditions
Y1  - 2016
ER  - 
TY  - JOUR
A1  - Lämke, Jörn
A1  - Brzezinka, Krzysztof
A1  - Altmann, Simone
A1  - Bäurle, Isabel
T1  - A hit-and-run heat shock factor governs sustained histone methylation and transcriptional stress memory
JF  - The EMBO journal
N2  - In nature, plants often encounter chronic or recurring stressful conditions. Recent results indicate that plants can remember a past exposure to stress to be better prepared for a future stress incident. However, the molecular basis of this is poorly understood. Here, we report the involvement of chromatin modifications in the maintenance of acquired thermotolerance (heat stress [HS] memory). HS memory is associated with the accumulation of histone H3 lysine 4 di- and trimethylation at memory-related loci. This accumulation outlasts their transcriptional activity and marks them as recently transcriptionally active. High accumulation of H3K4 methylation is associated with hyper-induction of gene expression upon a recurring HS. This transcriptional memory and the sustained accumulation of H3K4 methylation depend on HSFA2, a transcription factor that is required for HS memory, but not initial heat responses. Interestingly, HSFA2 associates with memory-related loci transiently during the early stages following HS. In summary, we show that transcriptional memory after HS is associated with sustained H3K4 hyper-methylation and depends on a hit-and-run transcription factor, thus providing a molecular framework for HS memory.
KW  - chromatin
KW  - H3K4 methylation
KW  - heat shock transcription factor
KW  - priming
KW  - transcriptional memory
Y1  - 2016
U6  - https://doi.org/10.15252/embj.201592593
SN  - 0261-4189
SN  - 1460-2075
VL  - 35
SP  - 162
EP  - 175
PB  - Wiley-Blackwell
CY  - Hoboken
ER  - 
TY  - JOUR
A1  - Nowak-Szczepanska, Natalia
A1  - Gomula, A.
A1  - Ipsen, Marie Josephin
A1  - Koziel, Slawomir
T1  - Different effects of living conditions on the variation in BMI and height in children before the onset of puberty
JF  - European journal of clinical nutrition
N2  - SUBJECTS/METHODS: The study included 5597 boys and 5479 girls aged 7-8 years of age. Socioeconomic status (SES) was defined in three categories: high, medium and low. RESULTS: Between 1966 and 2012, the mean values for height and BMI significantly increased in both sexes (P<0.001). The variation of these two parameters, however, showed a different pattern. Whereas the variation in Z-values for height remained unchanged in both sexes, the variation in BMI increased in boys (P<0.01) but not in girls. SES affected the variation in Z-BMI in 1978 in both sexes (P<0.001), whereas variation in Z-height between SES categories remained unchanged across all years of surveys in boys. Before the political transformation, significant regional differences were observed in the variances of Z-BMI (P<0.05) but not of Z-height. This pattern changed after the political transformation, when regional differences in variances of Z-BMI disappeared. CONCLUSIONS: It is concluded that the mean values and the variation of BMI are affected by a changing quality of life, whereas the variation in height is usually independent of living conditions.
Y1  - 2016
U6  - https://doi.org/10.1038/ejcn.2016.30
SN  - 0954-3007
SN  - 1476-5640
VL  - 70
SP  - 662
EP  - 666
PB  - Nature Publ. Group
CY  - London
ER  - 
TY  - THES
A1  - Xu, Ke
T1  - Functional characterization of two MYB transcription factors, MYB95 and MYB47, in Arabidopsis thaliana
Y1  - 2016
ER  - 
TY  - JOUR
A1  - Wacker, Alexander
A1  - Piepho, Maike
A1  - Harwood, John L.
A1  - Guschina, Irina A.
A1  - Arts, Michael T.
T1  - Light-Induced Changes in Fatty Acid Profiles of Specific Lipid Classes in Several Freshwater Phytoplankton Species
JF  - Frontiers in plant science : FPLS
N2  - We tested the influence of two light intensities [40 and 300 μmol PAR / (m2s)] on the fatty acid composition of three distinct lipid classes in four freshwater phytoplankton species. We chose species of different taxonomic classes in order to detect potentially similar reaction characteristics that might also be present in natural phytoplankton communities. From samples of the bacillariophyte Asterionella formosa, the chrysophyte Chromulina sp., the cryptophyte Cryptomonas ovata and the zygnematophyte Cosmarium botrytis we first separated glycolipids (monogalactosyldiacylglycerol, digalactosyldiacylglycerol, and sulfoquinovosyldiacylglycerol), phospholipids (phosphatidylcholine, phosphatidylethanolamine, phosphatidylglycerol, phosphatidylinositol, and phosphatidylserine) as well as non-polar lipids (triacylglycerols), before analyzing the fatty acid composition of each lipid class. High variation in the fatty acid composition existed among different species. Individual fatty acid compositions differed in their reaction to changing light intensities in the four species. Although no generalizations could be made for species across taxonomic classes, individual species showed clear but small responses in their ecologically-relevant omega-3 and omega-6 polyunsaturated fatty acids (PUFA) in terms of proportions and of per tissue carbon quotas. Knowledge on how lipids like fatty acids change with environmental or culture conditions is of great interest in ecological food web studies, aquaculture, and biotechnology, since algal lipids are the most important sources of omega-3 long-chain PUFA for aquatic and terrestrial consumers, including humans.
KW  - freshwater algae
KW  - light adaptation
KW  - lipid classes
KW  - fatty acid changes
Y1  - 2016
U6  - https://doi.org/10.3389/fpls.2016.00264
SN  - 1664-462X
VL  - 7
SP  - 1
EP  - 13
PB  - Frontiers Media
CY  - Lausanne
ER  - 
TY  - JOUR
A1  - Sperfeld, Erik
A1  - Raubenheimer, David
A1  - Wacker, Alexander
T1  - Bridging factorial and gradient concepts of resource co-limitation:
towards a general framework applied to consumers
JF  - Ecology letters
N2  - Organism growth can be limited either by a single resource or by multiple resources simultaneously (co-limitation). Efforts to characterise co-limitation have generated two influential approaches. One approach uses limitation scenarios of factorial growth assays to distinguish specific types of co-limitation; the other uses growth responses spanned over a continuous, multi-dimensional resource space to characterise different types of response surfaces. Both approaches have been useful in investigating particular aspects of co-limitation, but a synthesis is needed to stimulate development of this recent research area. We address this gap by integrating the two approaches, thereby presenting a more general framework of co-limitation. We found that various factorial (co-)limitation scenarios can emerge in different response surface types based on continuous availabilities of essential or substitutable resources. We tested our conceptual co-limitation framework on data sets of published and unpublished studies examining the limitation of two herbivorous consumers in a two-dimensional resource space. The experimental data corroborate the predictions, suggesting a general applicability of our co-limitation framework to generalist consumers and potentially also to other organisms. The presented framework might give insight into mechanisms that underlie co-limitation responses and thus can be a seminal starting point for evaluating co-limitation patterns in experiments and nature.
KW  - Consumer
KW  - essential nutrient
KW  - factorial design
KW  - food quality
KW  - growth rate
KW  - multi-nutrient limitation
KW  - nutritional ecology
KW  - performance landscape
KW  - substitutable resource
KW  - synergistic effect
Y1  - 2016
U6  - https://doi.org/10.1111/ele.12554
SN  - 1461-023X
SN  - 1461-0248
VL  - 19
SP  - 201
EP  - 215
PB  - Wiley-Blackwell
CY  - Hoboken
ER  - 
TY  - JOUR
A1  - Koussoroplis, Apostolos-Manuel
A1  - Wacker, Alexander
T1  - Covariance modulates the effect of joint temperature and food variance
on ectotherm life-history traits
JF  - Ecology letters
N2  - Understanding animal performance in heterogeneous or variable environments is a central question in ecology. We combine modelling and experiments to test how temperature and food availability variance jointly affect life-history traits of ectotherms. The model predicts that as mean temperatures move away from the ectotherm's thermal optimum, the effect size of joint thermal and food variance should become increasingly sensitive to their covariance. Below the thermal optimum, performance should be positively correlated with food–temperature covariance and the opposite is predicted above it. At lower temperatures, covariance should determine whether food and temperature variance increases or decreases performance compared to constant conditions. Somewhat stronger than predicted, the covariance effect below the thermal optimum was confirmed experimentally on an aquatic ectotherm (Daphnia magna) exposed to diurnal food and temperature variance with different amounts of covariance. Our findings have important implications for understanding ectotherm responses to climate-driven alterations of thermal mean and variance.
KW  - Biotic interactions
KW  - co-limitation
KW  - Daphnia
KW  - environmental fluctuations
KW  - heterogeneity
KW  - variability
KW  - vertical migration
KW  - zooplankton
Y1  - 2016
U6  - https://doi.org/10.1111/ele.12546
SN  - 1461-023X
SN  - 1461-0248
VL  - 19
SP  - 143
EP  - 152
PB  - Wiley-Blackwell
CY  - Hoboken
ER  - 
TY  - GEN
A1  - Wacker, Alexander
A1  - Piepho, Maike
A1  - Harwood, John L.
A1  - Guschina, Irina A.
A1  - Arts, Michael T.
T1  - Light-Induced Changes in Fatty Acid Profiles of Specific Lipid Classes in Several Freshwater Phytoplankton Species
N2  - We tested the influence of two light intensities [40 and 300 μmol PAR / (m2s)] on the fatty acid composition of three distinct lipid classes in four freshwater phytoplankton species. We chose species of different taxonomic classes in order to detect potentially similar reaction characteristics that might also be present in natural phytoplankton communities. From samples of the bacillariophyte Asterionella formosa, the chrysophyte Chromulina sp., the cryptophyte Cryptomonas ovata and the zygnematophyte Cosmarium botrytis we first separated glycolipids (monogalactosyldiacylglycerol, digalactosyldiacylglycerol, and sulfoquinovosyldiacylglycerol), phospholipids (phosphatidylcholine, phosphatidylethanolamine, phosphatidylglycerol, phosphatidylinositol, and phosphatidylserine) as well as non-polar lipids (triacylglycerols), before analyzing the fatty acid composition of each lipid class. High variation in the fatty acid composition existed among different species. Individual fatty acid compositions differed in their reaction to changing light intensities in the four species. Although no generalizations could be made for species across taxonomic classes, individual species showed clear but small responses in their ecologically-relevant omega-3 and omega-6 polyunsaturated fatty acids (PUFA) in terms of proportions and of per tissue carbon quotas. Knowledge on how lipids like fatty acids change with environmental or culture conditions is of great interest in ecological food web studies, aquaculture, and biotechnology, since algal lipids are the most important sources of omega-3 long-chain PUFA for aquatic and terrestrial consumers, including humans.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 223 
KW  - fatty acid changes
KW  - freshwater algae
KW  - light adaptation
KW  - lipid classes
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-90682
SP  - 1
EP  - 13
ER  - 
TY  - JOUR
A1  - Kabelitz, Tina
A1  - Brzezinka, Krzysztof
A1  - Friedrich, Thomas
A1  - Gorka, Michal
A1  - Graf, Alexander
A1  - Kappel, Christian
A1  - Bäurle, Isabel
T1  - A JUMONJI Protein with E3 Ligase and Histone H3 Binding Activities Affects Transposon Silencing in Arabidopsis
JF  - Plant physiology : an international journal devoted to physiology, biochemistry, cellular and molecular biology, biophysics and environmental biology of plants
N2  - Transposable elements (TEs) make up a large proportion of eukaryotic genomes. As their mobilization creates genetic variation that threatens genome integrity, TEs are epigenetically silenced through several pathways, and this may spread to neighboring sequences. JUMONJI (JMJ) proteins can function as antisilencing factors and prevent silencing of genes next to TEs. Whether TE silencing is counterbalanced by the activity of antisilencing factors is still unclear. Here, we characterize JMJ24 as a regulator of TE silencing. We show that loss of JMJ24 results in increased silencing of the DNA transposon AtMu1c, while overexpression of JMJ24 reduces silencing. JMJ24 has a JumonjiC (JmjC) domain and two RING domains. JMJ24 autoubiquitinates in vitro, demonstrating E3 ligase activity of the RING domain(s). JMJ24-JmjC binds the N-terminal tail of histone H3, and full-length JMJ24 binds histone H3 in vivo. JMJ24 activity is anticorrelated with histone H3 Lys 9 dimethylation (H3K9me2) levels at AtMu1c. Double mutant analyses with epigenetic silencing mutants suggest that JMJ24 antagonizes histone H3K9me2 and requires H3K9 methyltransferases for its activity on AtMu1c. Genome-wide transcriptome analysis indicates that JMJ24 affects silencing at additional TEs. Our results suggest that the JmjC domain of JMJ24 has lost demethylase activity but has been retained as a binding domain for histone H3. This is in line with phylogenetic analyses indicating that JMJ24 (with the mutated JmjC domain) is widely conserved in angiosperms. Taken together, this study assigns a role in TE silencing to a conserved JmjC-domain protein with E3 ligase activity, but no demethylase activity.
Y1  - 2016
U6  - https://doi.org/10.1104/pp.15.01688
SN  - 0032-0889
SN  - 1532-2548
VL  - 171
SP  - 344
EP  - 358
PB  - American Society of Plant Physiologists
CY  - Rockville
ER  - 
TY  - JOUR
A1  - Grzesiuk, Malgorzata
A1  - Wacker, Alexander
A1  - Spijkerman, Elly
T1  - Photosynthetic sensitivity of phytoplankton to commonly used pharmaceuticals and its dependence on cellular phosphorus status
JF  - Ecotoxicology
N2  - Recently pharmaceuticals have become significant environmental pollutants in aquatic ecosystems, that could affect primary producers such as microalgae. Here we analyzed the effect of pharmaceuticals on the photosynthesis of microalgae commonly found in freshwater-two species of Chlorophyceae and a member of the Eustigmatophyceae, via PAM fluorometry. As pharmaceuticals, three medicines often consumed in households were chosen: (i) fluoxetine, an antidepressant, (ii) propranolol, a beta-blocker and (iii) ibuprofen, an anti-inflammatory and analgesic medicine. The EC50 for the quantum yield of photosystem II in phytoplankton acclimated to inorganic phosphorus (P-i)-replete and P-i-limited conditions was estimated. Acute toxicity experiments over a 5 h exposure revealed that Nannochloropsis limnetica was the least sensitive to pharmaceuticals in its photosynthetic yield out of all species tested. Although the estimation of sub-lethal effects can be vital in contrast to that of LC(50)s, the EC50 values in all species and for all medicines were orders of magnitude higher than concentrations found in polluted surface water. Chlamydomonas reinhardtii was the most sensitive to fluoxetine (EC50 of 1.6 mg L-1), and propranolol (EC50 of 3 mg L-1). Acutodesmus obliquus was most sensitive to ibuprofen (EC50 of 288 mg L-1). Additionally, the sensitivity to the pharmaceuticals changed under a P-i-limitation; the green algae became less sensitive to fluoxetine and propranolol. In contrast, P-i-limited algal species were more sensitive to ibuprofen. Our results suggest that the sensitivity of algae to pharmaceuticals is (i) highly compound- and species-specific and (ii) dependent on the cellular P status.
KW  - Freshwater algae
KW  - Medicine
KW  - EC50
KW  - PAM fluorometry
KW  - Tolerance
Y1  - 2016
U6  - https://doi.org/10.1007/s10646-016-1628-8
SN  - 0963-9292
SN  - 1573-3017
VL  - 25
SP  - 697
EP  - 707
PB  - Springer
CY  - Dordrecht
ER  - 
TY  - JOUR
A1  - Lachmann, Sabrina C.
A1  - Maberly, Stephen C.
A1  - Spijkerman, Elly
T1  - ECOPHYSIOLOGY MATTERS: LINKING INORGANIC CARBON ACQUISITION TO ECOLOGICAL PREFERENCE IN FOUR SPECIES OF MICROALGAE (CHLOROPHYCEAE)
JF  - Journal of phycology
N2  - The effect of CO2 supply is likely to play an important role in algal ecology. Since inorganic carbon (C-i) acquisition strategies are very diverse among microalgae and C-i availability varies greatly within and among habitats, we hypothesized that C-i acquisition depends on the pH of their preferred natural environment (adaptation) and that the efficiency of C-i uptake is affected by CO2 availability (acclimation). To test this, four species of green algae originating from different habitats were studied. The pH-drift and C-i uptake kinetic experiments were used to characterize C-i acquisition strategies and their ability to acclimate to high and low CO2 conditions and high and low pH was evaluated. Results from pH drift experiments revealed that the acidophile and acidotolerant Chlamydomonas species were mainly restricted to CO2, whereas the two neutrophiles were efficient bicarbonate users. CO2 compensation points in low CO2-acclimated cultures ranged between 0.6 and 1.4 mu M CO2 and acclimation to different culture pH and CO2 conditions suggested that CO2 concentrating mechanisms were present in most species. High CO2 acclimated cultures adapted rapidly to low CO2 condition during pH-drifts. C-i uptake kinetics at different pH values showed that the affinity for C-i was largely influenced by external pH, being highest under conditions where CO2 dominated the C-i pool. In conclusion, C-i acquisition was highly variable among four species of green algae and linked to growth pH preference, suggesting that there is a connection between C-i acquisition and ecological distribution.
KW  - acidophile
KW  - carbon acquisition
KW  - CCM
KW  - Chlamydomonas
KW  - Chlorella
KW  - CO2 supply
KW  - extremophile
KW  - inorganic carbon uptake kinetics
KW  - pH-drift
KW  - Scenedesmus
Y1  - 2016
U6  - https://doi.org/10.1111/jpy.12462
SN  - 0022-3646
SN  - 1529-8817
VL  - 52
SP  - 1051
EP  - 1063
PB  - Wiley-Blackwell
CY  - Hoboken
ER  - 
TY  - JOUR
A1  - Spijkerman, Elly
A1  - Stojkovic, Slobodanka
A1  - Holland, Daryl
A1  - Lachmann, Sabrina C.
A1  - Beardall, John
T1  - Nutrient induced fluorescence transients (NIFTs) provide a rapid measure of P and C (co-)limitation in a green alga
JF  - European journal of phycology
N2  - Nutrient Induced Fluorescence Transients (NIFTs) have been shown to be a possible way of testing for the limiting nutrient in algal populations. In this study we tested the hypothesis that NIFTs can be used to detect a (co-)limitation for inorganic phosphorus (Pi) and CO2 in the green alga Chlamydomonas acidophila and that the magnitude of the NIFTs can be related to cellular P:C ratios. We show a co-limitation response for Pi and CO2 via traditional nutrient enrichment experiments in natural phytoplankton populations dominated by C. acidophila. We measured NIFT responses after a Pi- or a CO2-spike in C. acidophila batch cultures at various stages of Pi and inorganic C limitation. Significant NIFTs were observed in response to spikes in both nutrients. The NIFT response to a Pi-spike showed a strong negative correlation with cellular P:C ratio that was pronounced below 3 mmol P: mol C (equivalent to 0.2 pg P cell(-1)). Both cellular P and C content influenced the extent of the Pi-NIFT response. The NIFT response to a CO2-spike correlated to low CO2 culturing conditions and also had a negative correlation with cellular P content. A secondary response within the Pi-NIFT response was related to the CO2 concentration and potentially reflected co-limitation. In conclusion, NIFTs provided a quick and reliable method to detect the growth-limiting nutrient in an extremophile green alga, under Pi-, CO2- and Pi/CO2 (co-)limited growth conditions.
KW  - acidophile
KW  - Chlamydomonas
KW  - CO2 concentrating mechanism
KW  - CO2 limitation
KW  - extremophile
KW  - nutrient limitation
KW  - photosynthesis response
KW  - phytoplankton
KW  - stoichiometry
Y1  - 2016
U6  - https://doi.org/10.1080/09670262.2015.1095355
SN  - 0967-0262
SN  - 1469-4433
VL  - 51
SP  - 47
EP  - 58
PB  - Hindawi
CY  - Abingdon
ER  - 
TY  - THES
A1  - Brzezinka, Magdalena
T1  - Investigation of novel proteins and polysaccharides associated with coccoliths of Emiliania huxleyi
Y1  - 2016
ER  - 
TY  - THES
A1  - Rottstock, Tanja
T1  - Effects of plant community diversity and composition on fungal pathogens in experimental grasslands
Y1  - 2016
ER  - 
TY  - THES
A1  - Barahimipour, Rouhollah
T1  - Optimization of transgene expression in the nuclear genome of Chlamydomonas reinhardtii and characterization of Chlamydomonas expression strains
Y1  - 2016
ER  - 
TY  - THES
A1  - Sviben, Sanja
T1  - Calcite biomineralization in coccolithophores
BT  - new insights from ultrastructural and proteomic studies of Emiliania huxleyi
Y1  - 2016
ER  - 
TY  - THES
A1  - Armarego-Marriott, Tegan
T1  - From dark to light
BT  - an overexpression and systems biology approach to investigate the development of functional thylakoid membranes
Y1  - 2016
ER  - 
TY  - THES
A1  - Prokopović, Vladimir Z.
T1  - Light-triggered release of bioactive compounds from  HA/PLL multilayer films for stimulation of cells
T1  - Licht-induzierte Freisetzung von Biomolekülen aus Hyaluronsäure-Poly-L-Lysin-Schichten zur Stimulierung von Zellen
N2  - The concept of targeting cells and tissues by controlled delivery of molecules is essential in the field of biomedicine. The layer-by-layer (LbL) technology for the fabrication of polymer multilayer films is widely implemented as a powerful tool to assemble tailor-made materials for controlled drug delivery. The LbL films can as well be engineered to act as mimics of the natural cellular microenvironment. Thus, due to the myriad possibilities such as controlled cellular adhesion and drug delivery offered by LbL films, it becomes easily achievable to direct the fate of cells by growing them on the films.
The aim of this work was to develop an approach for non-invasive and precise control of the presentation of bioactive molecules to cells. The strategy is based on employment of the LbL films, which function as support for cells and at the same time as reservoirs for bioactive molecules to be released in a controlled manner. UV light is used to trigger the release of the stored ATP with high spatio-temporal resolution. Both physico-chemical (competitive intermolecular interactions in the film) and biological aspects (cellular response and viability) are addressed in this study. 
Biopolymers hyaluronic acid (HA) and poly-L-lysine (PLL) were chosen as the building blocks for the LbL film assembly. Poor cellular adhesion to native HA/PLL films as well as significant degradation by cells within a few days were shown. However, coating the films with gold nanoparticles not only improved cellular adhesion and protected the films from degradation, but also formed a size-exclusion barrier with adjustable cut-off in the size range of a few tens of kDa.
The films were shown to have high reservoir capacity for small charged molecules (reaching mM levels in the film). Furthermore, they were able to release the stored molecules in a sustained manner. The loading and release are explained by a mechanism based on interactions between charges of the stored molecules and uncompensated charges of the biopolymers in the film. Charge balance and polymer dynamics in the film play the pivotal role. 
Finally, the concept of light-triggered release from the films has been proven using caged ATP loaded into the films from which ATP was released on demand. ATP induces a fast cellular response, i.e. increase in intracellular [Ca2+], which was monitored in real-time. Limitations of the cellular stimulation by the proposed approach are highlighted by studying the stimulation as a function of irradiation parameters (time, distance, light power). Moreover, caging molecules bind to the film stronger than ATP does, which opens new perspectives for the use of the most diverse chemical compounds as caging molecules.
Employment of HA/PLL films as a nouvelle support for cellular growth and hosting of bioactive molecules, along with the possibility to stimulate individual cells using focused light renders this approach highly efficient and unique in terms of precision and spatio-temporal resolution among those previously described. With its high potential, the concept presented herein provides the foundation for the design of new intelligent materials for single cell studies, with the focus on tissue engineering, diagnostics, and other cell-based applications.
N2  - Das Konzept des Targetings von Zellen und Geweben mittels kontrollierter Wirkstoffverabreichung ist im Bereich der Biomedizin unerlässlich. Die layer-by-layer (LbL) Technologie ist eine etablierte Methode für die Herstellung von Polyelektrolyt-Multischichten, um intelligente, maßgeschneiderte Materialien für eine kontrollierte Wirkstoffabgabe aufzubauen. Die LbL Filme können das Verhalten einer natürlichen zellulären Mikroumgebung nachahmen. Wegen der unzähligen Möglichkeiten dieser Filme sind nicht nur das Wachstum und die Beeinflussung der Zellen, sondern auch die kontrollierte Wirkstoffabgabe leicht umzusetzen.
Das Ziel der vorliegenden Arbeit war die Entwicklung eines nicht-invasiven Systems für die präzise Verabreichung von Biomolekülen an einzelne Zellen. Die Strategie beruht auf LbL Filmen, die einerseits als geeignete Oberfläche für das Zellwachstum dienen, andererseits aber auch die kontrollierte Abgabe von Biomolekülen ermöglichen. Die zeitlich und räumlich präzise Freisetzung von ATP wurde durch UV Bestrahlung eingeleitet/ausgelöst. Sowohl die physiko-chemischen als auch die biologischen Eigenschaften des Verfahrens wurden analysiert.
Die LbL Filme wurden auf Basis der biokompatiblen Polymere Hyaluronsäure (HA) und Poly-L-Lysin (PLL) assembliert. Nach der Assemblierung waren die Filme zunächst zellabweisend und wurden von den Zellen innerhalb von ein paar Tagen abgebaut. Die Beschichtigung der Filme mit Gold-Nanopartikeln verbesserte nicht nur die Adhäsion der Zellen, sondern auch den Schutz gegen Abbau. Zudem wurde gezeigt, dass die Beschichtigung eine Molekulargewichtsausschlussgrenze mit verstellbarem cut-off in einem Bereich von nur einigen 10 kDa darstellt. 
Weiterhin wurde gezeigt, dass die Filme eine enorme Beladungskapazität aufweisen (bis hin zu einer Beladung im mM Bereich). Darüber hinaus konnten die Biomoleküle, die in diese Filme eingebettet wurden, langfristig und nachhaltig freigesetzt werden. Die Beladung und Freisetzung der Moleküle erfolgt durch die Interaktion zwischen eingebetteten Molekülen und freien Ladungen innerhalb des Polymerfilms. Das Ladungsverhältnis und die Polymerdynamik spielen dabei eine zentrale Rolle.
Schließlich wurde gezeigt, dass die in Filmen eingebetteten caged-ATP Moleküle gezielt durch einen Laser freigesetzt werden können. ATP verursacht die schnelle zelluläre Antwort durch den Anstieg von intrazellulären Ca2+-Ionen, der in Echtzeit beobachtet werden kann. Um die Limitierungen dieses Ansatzes bei der zellulären Stimulation hervorzuheben, wurden verschiedene Bestrahlungsparameter (Zeit, Abstand, Laserleistung) analysiert. Außerdem binden viele caging-Moleküle stärker an die Polymerfilme als ATP, wodurch eine Vielzahl von chemischen Verbindungen als geeignete Moleküle für die Caging zur Verfügung stehen. 
Der Einsatz von HA/PLL Filmen als neue Oberfläche für Zellwachstum und als Reservoire für die Einbettung bioaktiver Moleküle samt der Möglichkeit einzelne Zellen mittels fokussierter Laserbestrahlung anzuregen, machen die Methode hoch effizient und einzigartig. Die Vorteile dieser Methode kommen durch die zeitliche und räumliche Präzision zustande. In Zukunft kann das in dieser Arbeit beschriebene Konzept für den Entwurf neuer Materialien für Untersuchungen mit einzelnen Zellen eingesetzt werden; mit dem Fokus auf Tissue Engineering, Diagnostik und anderen Zell- und biomedizinisch-basierten Applikationen.
KW  - multilayer films
KW  - light-triggered
KW  - stimulation of cells
KW  - drug release
KW  - Polyelektrolyt-Multischichten
KW  - Licht-induzierte
KW  - kontrollierte Freisetzung von Biomolekülen
KW  - Stimulierung von Zellen
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-97927
ER  - 
TY  - JOUR
A1  - Cui, Huanhuan
A1  - Schlesinger, Jenny
A1  - Schoenhals, Sophia
A1  - Toenjes, Martje
A1  - Dunkel, Ilona
A1  - Meierhofer, David
A1  - Cano, Elena
A1  - Schulz, Kerstin
A1  - Berger, Michael F.
A1  - Haack, Timm
A1  - Abdelilah-Seyfried, Salim
A1  - Bulyk, Martha L.
A1  - Sauer, Sascha
A1  - Sperling, Silke R.
T1  - Phosphorylation of the chromatin remodeling factor DPF3a induces cardiac hypertrophy through releasing HEY repressors from DNA
JF  - Nucleic acids research
N2  - DPF3 (BAF45c) is a member of the BAF chromatin remodeling complex. Two isoforms have been described, namely DPF3a and DPF3b. The latter binds to acetylated and methylated lysine residues of histones. Here, we elaborate on the role of DPF3a and describe a novel pathway of cardiac gene transcription leading to pathological cardiac hypertrophy. Upon hypertrophic stimuli, casein kinase 2 phosphorylates DPF3a at serine 348. This initiates the interaction of DPF3a with the transcriptional repressors HEY, followed by the release of HEY from the DNA. Moreover, BRG1 is bound by DPF3a, and is thus recruited to HEY genomic targets upon interaction of the two components. Consequently, the transcription of downstream targets such as NPPA and GATA4 is initiated and pathological cardiac hypertrophy is established. In human, DPF3a is significantly up-regulated in hypertrophic hearts of patients with hypertrophic cardiomyopathy or aortic stenosis. Taken together, we show that activation of DPF3a upon hypertrophic stimuli switches cardiac fetal gene expression from being silenced by HEY to being activated by BRG1. Thus, we present a novel pathway for pathological cardiac hypertrophy, whose inhibition is a long-term therapeutic goal for the treatment of the course of heart failure.
Y1  - 2016
U6  - https://doi.org/10.1093/nar/gkv1244
SN  - 0305-1048
SN  - 1362-4962
VL  - 44
SP  - 2538
EP  - 2553
PB  - Oxford Univ. Press
CY  - Oxford
ER  - 
TY  - JOUR
A1  - de Vinuesa, Amaya Garcia
A1  - Abdelilah-Seyfried, Salim
A1  - Knaus, Petra
A1  - Zwijsen, An
A1  - Bailly, Sabine
T1  - BMP signaling in vascular biology and dysfunction
JF  - New journal of physics : the open-access journal for physics
N2  - The vascular system is critical for developmental growth, tissue homeostasis and repair but also for tumor development. Bone morphogenetic protein (BMP) signaling has recently emerged as a fundamental pathway of the endothelium by regulating cardiovascular and lymphatic development and by being causative for several vascular dysfunctions. Two vascular disorders have been directly linked to impaired BMP signaling: pulmonary arterial hypertension and hereditary hemorrhagic telangiectasia. Endothelial BMP signaling critically depends on the cellular context, which includes among others vascular heterogeneity, exposure to flow, and the intertwining with other signaling cascades (Notch, WNT, Hippo and hypoxia). The purpose of this review is to highlight the most recent findings illustrating the clear need for reconsidering the role of BMPs in vascular biology. (C) 2015 Elsevier Ltd. All rights reserved.
KW  - Bone morphogenetic proteins (BMP)
KW  - Signaling
KW  - Vasculature
KW  - Development
KW  - Disease
Y1  - 2016
U6  - https://doi.org/10.1016/j.cytogfr.2015.12.005
SN  - 1359-6101
SN  - 1879-0305
VL  - 27
SP  - 65
EP  - 79
PB  - Elsevier
CY  - Oxford
ER  - 
TY  - JOUR
A1  - Haack, Timm
A1  - Abdelilah-Seyfried, Salim
T1  - The force within: endocardial development, mechanotransduction and signalling during cardiac morphogenesis
JF  - Development : Company of Biologists
N2  - Endocardial cells are cardiac endothelial cells that line the interior of the heart tube. Historically, their contribution to cardiac development has mainly been considered from a morphological perspective. However, recent studies have begun to define novel instructive roles of the endocardium, as a sensor and signal transducer of biophysical forces induced by blood flow, and as an angiocrine signalling centre that is involved in myocardial cellular morphogenesis, regeneration and reprogramming. In this Review, we discuss how the endocardium develops, how endocardial-myocardial interactions influence the developing embryonic heart, and how the dysregulation of blood flowresponsive endocardial signalling can result in pathophysiological changes.
KW  - Endocardium
KW  - Cardiac development
KW  - Hemodynamics
KW  - Bmp
KW  - Kruppel-like factor 2
KW  - Vegf
KW  - Mechanotransduction
KW  - Zebrafish
KW  - Mouse
Y1  - 2016
U6  - https://doi.org/10.1242/dev.131425
SN  - 0950-1991
SN  - 1477-9129
VL  - 143
SP  - 373
EP  - 386
PB  - Company of Biologists Limited
CY  - Cambridge
ER  - 
TY  - JOUR
A1  - ´Cwiek-Kupczynska, Hanna
A1  - Altmann, Thomas
A1  - Arend, Daniel
A1  - Arnaud, Elizabeth
A1  - Chen, Dijun
A1  - Cornut, Guillaume
A1  - Fiorani, Fabio
A1  - Frohmberg, Wojciech
A1  - Junker, Astrid
A1  - Klukas, Christian
A1  - Lange, Matthias
A1  - Mazurek, Cezary
A1  - Nafissi, Anahita
A1  - Neveu, Pascal
A1  - van Oeveren, Jan
A1  - Pommier, Cyril
A1  - Poorter, Hendrik
A1  - Rocca-Serra, Philippe
A1  - Sansone, Susanna-Assunta
A1  - Scholz, Uwe
A1  - van Schriek, Marco
A1  - Seren, Ümit
A1  - Usadel, Bjorn
A1  - Weise, Stephan
A1  - Kersey, Paul
A1  - Krajewski, Pawel
T1  - Measures for interoperability of phenotypic data: minimum information requirements and formatting
JF  - Plant Methods
N2  - Background: Plant phenotypic data shrouds a wealth of information which, when accurately analysed and linked to other data types, brings to light the knowledge about the mechanisms of life. As phenotyping is a field of research comprising manifold, diverse and time-consuming experiments, the findings can be fostered by reusing and combining existing datasets. Their correct interpretation, and thus replicability, comparability and interoperability, is possible provided that the collected observations are equipped with an adequate set of metadata. So far there have been no common standards governing phenotypic data description, which hampered data exchange and reuse. Results: In this paper we propose the guidelines for proper handling of the information about plant phenotyping experiments, in terms of both the recommended content of the description and its formatting. We provide a document called "Minimum Information About a Plant Phenotyping Experiment", which specifies what information about each experiment should be given, and a Phenotyping Configuration for the ISA-Tab format, which allows to practically organise this information within a dataset. We provide examples of ISA-Tab-formatted phenotypic data, and a general description of a few systems where the recommendations have been implemented. Conclusions: Acceptance of the rules described in this paper by the plant phenotyping community will help to achieve findable, accessible, interoperable and reusable data.
KW  - Data standardisation and formatting
KW  - Experimental metadata
KW  - Minimum information recommendations
KW  - Plant phenotyping
KW  - Experiment description
Y1  - 2016
U6  - https://doi.org/10.1186/s13007-016-0144-4
SN  - 1746-4811
VL  - 12
PB  - BioMed Central
CY  - London
ER  - 
TY  - JOUR
A1  - Yan, Wenhao
A1  - Chen, Dijun
A1  - Kaufmann, Kerstin
T1  - Efficient multiplex mutagenesis by RNA-guided Cas9 and its use in the characterization of regulatory elements in the AGAMOUS gene
JF  - Plant methods
N2  - Background
The efficiency of multiplex editing in plants by the RNA-guided Cas9 system is limited by efficient introduction of its components into the genome and by their activity. The possibility of introducing large fragment deletions by RNA-guided Cas9 tool provides the potential to study the function of any DNA region of interest in its ‘endogenous’ environment.

Results
Here, an RNA-guided Cas9 system was optimized to enable efficient multiplex editing in Arabidopsis thaliana. We demonstrate the flexibility of our system for knockout of multiple genes, and to generate heritable large-fragment deletions in the genome. As a proof of concept, the function of part of the second intron of the flower development gene AGAMOUS in Arabidopsis was studied by generating a Cas9-free mutant plant line in which part of this intron was removed from the genome. Further analysis revealed that deletion of this intron fragment results 40 % decrease of AGAMOUS gene expression without changing the splicing of the gene which indicates that this regulatory region functions as an activator of AGAMOUS gene expression.

Conclusions
Our modified RNA-guided Cas9 system offers a versatile tool for the functional dissection of coding and non-coding DNA sequences in plants.
KW  - RNA-guided Cas9
KW  - Multiplex mutagenesis
KW  - Large fragment deletion
KW  - Germline transmission
Y1  - 2016
U6  - https://doi.org/10.1186/s13007-016-0125-7
SN  - 1746-4811
VL  - 12
SP  - 1
EP  - 9
PB  - BioMed Central
CY  - London
ER  - 
TY  - JOUR
A1  - Yan, Wenhao
A1  - Chen, Dijun
A1  - Kaufmann, Kerstin
T1  - Efficient multiplex mutagenesis by RNA-guided Cas9 and its use in the characterization of regulatory elements in the AGAMOUS gene
JF  - Plant Methods
N2  - Results: Here, an RNA-guided Cas9 system was optimized to enable efficient multiplex editing in Arabidopsis thaliana. We demonstrate the flexibility of our system for knockout of multiple genes, and to generate heritable large-fragment deletions in the genome. As a proof of concept, the function of part of the second intron of the flower development gene AGAMOUS in Arabidopsis was studied by generating a Cas9-free mutant plant line in which part of this intron was removed from the genome. Further analysis revealed that deletion of this intron fragment results 40 % decrease of AGAMOUS gene expression without changing the splicing of the gene which indicates that this regulatory region functions as an activator of AGAMOUS gene expression. Conclusions: Our modified RNA-guided Cas9 system offers a versatile tool for the functional dissection of coding and non-coding DNA sequences in plants.
KW  - RNA-guided Cas9
KW  - Multiplex mutagenesis
KW  - Large fragment deletion
KW  - Germline transmission
Y1  - 2016
U6  - https://doi.org/10.1186/s13007-016-0125-7
SN  - 1746-4811
VL  - 12
SP  - 2381
EP  - 2389
PB  - BioMed Central
CY  - London
ER  - 
TY  - JOUR
A1  - Yan, Wenhao
A1  - Chen, Dijun
A1  - Kaufmann, Kerstin
T1  - Molecular mechanisms of floral organ specification by MADS domain proteins
JF  - Current opinion in plant biology
N2  - Flower development is a model system to understand organ specification in plants. The identities of different types of floral organs are specified by homeotic MADS transcription factors that interact in a combinatorial fashion. Systematic identification of DNA-binding sites and target genes of these key regulators show that they have shared and unique sets of target genes. DNA binding by MADS proteins is not based on ‘simple’ recognition of a specific DNA sequence, but depends on DNA structure and combinatorial interactions. Homeotic MADS proteins regulate gene expression via alternative mechanisms, one of which may be to modulate chromatin structure and accessibility in their target gene promoters.
Y1  - 2016
U6  - https://doi.org/10.1016/j.pbi.2015.12.004
SN  - 1369-5266
SN  - 1879-0356
VL  - 29
SP  - 154
EP  - 162
PB  - Elsevier
CY  - London
ER  - 
TY  - JOUR
A1  - Memczak, Henry
A1  - Lauster, Daniel
A1  - Kar, Parimal
A1  - Di Lella, Santiago
A1  - Volkmer, Rudolf
A1  - Knecht, Volker
A1  - Herrmann, Andreas
A1  - Ehrentreich-Foerster, Eva
A1  - Bier, Frank Fabian
A1  - Stoecklein, Walter F. M.
T1  - Anti-Hemagglutinin Antibody Derived Lead Peptides for Inhibitors of Influenza Virus Binding
JF  - PLoS one
N2  - Antibodies against spike proteins of influenza are used as a tool for characterization of viruses and therapeutic approaches. However, development, production and quality control of antibodies is expensive and time consuming. To circumvent these difficulties, three peptides were derived from complementarity determining regions of an antibody heavy chain against influenza A spike glycoprotein. Their binding properties were studied experimentally, and by molecular dynamics simulations. Two peptide candidates showed binding to influenza A/Aichi/2/68 H3N2. One of them, termed PeB, with the highest affinity prevented binding to and infection of target cells in the micromolar region without any cytotoxic effect. PeB matches best the conserved receptor binding site of hemagglutinin. PeB bound also to other medical relevant influenza strains, such as human-pathogenic A/California/7/2009 H1N1, and avian-pathogenic A/MuteSwan/Rostock/R901/2006 H7N1. Strategies to improve the affinity and to adapt specificity are discussed and exemplified by a double amino acid substituted peptide, obtained by substitutional analysis. The peptides and their derivatives are of great potential for drug development as well as biosensing.
Y1  - 2016
U6  - https://doi.org/10.1371/journal.pone.0159074
SN  - 1932-6203
VL  - 11
SP  - 82
EP  - 90
PB  - PLoS
CY  - San Fransisco
ER  - 
TY  - JOUR
A1  - Connor, Daniel Oliver
A1  - Zantow, Jonas
A1  - Hust, Michael
A1  - Bier, Frank Fabian
A1  - von Nickisch-Rosenegk, Markus
T1  - Identification of Novel Immunogenic Proteins of Neisseria gonorrhoeae by Phage Display
JF  - PLoS one
N2  - Neisseria gonorrhoeae is one of the most prevalent sexually transmitted diseases worldwide with more than 100 million new infections per year. A lack of intense research over the last decades and increasing resistances to the recommended antibiotics call for a better understanding of gonococcal infection, fast diagnostics and therapeutic measures against N. gonorrhoeae. Therefore, the aim of this work was to identify novel immunogenic proteins as a first step to advance those unresolved problems. For the identification of immunogenic proteins, pHORF oligopeptide phage display libraries of the entire N. gonorrhoeae genome were constructed. Several immunogenic oligopeptides were identified using polyclonal rabbit antibodies against N. gonorrhoeae. Corresponding full-length proteins of the identified oligopeptides were expressed and their immunogenic character was verified by ELISA. The immunogenic character of six proteins was identified for the first time. Additional 13 proteins were verified as immunogenic proteins in N. gonorrhoeae.
Y1  - 2016
U6  - https://doi.org/10.1371/journal.pone.0148986
SN  - 1932-6203
VL  - 11
PB  - PLoS
CY  - San Fransisco
ER  - 
TY  - JOUR
A1  - Bader, Denise
A1  - Klier, Dennis Tobias
A1  - Hettrich, C.
A1  - Bier, Frank Fabian
A1  - Wessig, Pablo
T1  - Detecting carbohydrate-lectin interactions using a fluorescent probe based on DBD dyes
JF  - Analytical methods : advancing methods and applications
N2  - Herein we present an efficient synthesis of a biomimetic probe with modular construction that can be specifically bound by the mannose binding FimH protein - a surface adhesion protein of E. coli bacteria. The synthesis combines the new and interesting DBD dye with the carbohydrate ligand mannose via a Click reaction. We demonstrate the binding to E. coli bacteria over a large concentration range and also present some special characteristics of those molecules that are of particular interest for the application as a biosensor. In particular, the mix-and-measure ability and the very good photo-stability should be highlighted here.
Y1  - 2016
U6  - https://doi.org/10.1039/c5ay02991k
SN  - 1759-9660
SN  - 1759-9679
VL  - 8
SP  - 1235
EP  - 1238
PB  - Royal Society of Chemistry
CY  - Cambridge
ER  - 
TY  - GEN
A1  - Zancolli, Giulia
A1  - Baker, Timothy G.
A1  - Barlow, Axel
A1  - Bradley, Rebecca K.
A1  - Calvete, Juan J.
A1  - Carter, Kimberley C.
A1  - de Jager, Kaylah
A1  - Owens, John Benjamin
A1  - Price, Jenny Forrester
A1  - Sanz, Libia
A1  - Scholes-Higham, Amy
A1  - Shier, Liam
A1  - Wood, Liam
A1  - Wüster, Catharine E.
A1  - Wüster, Wolfgang
T1  - Is hybridization a source of adaptive venom variation in rattlesnakes?
BT  - a test, using a crotalus scutulatus × viridis hybrid zone in southwestern New Mexico
T2  - Toxins
N2  - Venomous snakes often display extensive variation in venom composition both between and within species. However, the mechanisms underlying the distribution of different toxins and venom types among populations and taxa remain insufficiently known. Rattlesnakes (Crotalus, Sistrurus) display extreme inter-and intraspecific variation in venom composition, centered particularly on the presence or absence of presynaptically neurotoxic phospholipases A2 such as Mojave toxin (MTX). Interspecific hybridization has been invoked as a mechanism to explain the distribution of these toxins across rattlesnakes, with the implicit assumption that they are adaptively advantageous. Here, we test the potential of adaptive hybridization as a mechanism for venom evolution by assessing the distribution of genes encoding the acidic and basic subunits of Mojave toxin across a hybrid zone between MTX-positive Crotalus scutulatus and MTX-negative C. viridis in southwestern New Mexico, USA. Analyses of morphology, mitochondrial and single copy-nuclear genes document extensive admixture within a narrow hybrid zone. The genes encoding the two MTX subunits are strictly linked, and found in most hybrids and backcrossed individuals, but not in C. viridis away from the hybrid zone. Presence of the genes is invariably associated with presence of the corresponding toxin in the venom. We conclude that introgression of highly lethal neurotoxins through hybridization is not necessarily favored by natural selection in rattlesnakes, and that even extensive hybridization may not lead to introgression of these genes into another species.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 443 
KW  - adaptation
KW  - Crotalus
KW  - evolution
KW  - hybridization
KW  - introgression
KW  - Mojave toxin
KW  - molecular evolution
KW  - venom
Y1  - 2018
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-407595
ER  - 
TY  - JOUR
A1  - Zancolli, Giulia
A1  - Baker, Timothy G.
A1  - Barlow, Axel
A1  - Bradley, Rebecca K.
A1  - Calvete, Juan J.
A1  - Carter, Kimberley C.
A1  - de Jager, Kaylah
A1  - Owens, John Benjamin
A1  - Price, Jenny Forrester
A1  - Sanz, Libia
A1  - Scholes-Higham, Amy
A1  - Shier, Liam
A1  - Wood, Liam
A1  - Wüster, Catharine E.
A1  - Wüster, Wolfgang
T1  - Is Hybridization a Source of Adaptive Venom Variation in Rattlesnakes? A Test, Using a Crotalus scutulatus x viridis Hybrid Zone in Southwestern New Mexico
JF  - Toxins
N2  - Venomous snakes often display extensive variation in venom composition both between and within species. However, the mechanisms underlying the distribution of different toxins and venom types among populations and taxa remain insufficiently known. Rattlesnakes (Crotalus, Sistrurus) display extreme inter-and intraspecific variation in venom composition, centered particularly on the presence or absence of presynaptically neurotoxic phospholipases A2 such as Mojave toxin (MTX). Interspecific hybridization has been invoked as a mechanism to explain the distribution of these toxins across rattlesnakes, with the implicit assumption that they are adaptively advantageous. Here, we test the potential of adaptive hybridization as a mechanism for venom evolution by assessing the distribution of genes encoding the acidic and basic subunits of Mojave toxin across a hybrid zone between MTX-positive Crotalus scutulatus and MTX-negative C. viridis in southwestern New Mexico, USA. Analyses of morphology, mitochondrial and single copy-nuclear genes document extensive admixture within a narrow hybrid zone. The genes encoding the two MTX subunits are strictly linked, and found in most hybrids and backcrossed individuals, but not in C. viridis away from the hybrid zone. Presence of the genes is invariably associated with presence of the corresponding toxin in the venom. We conclude that introgression of highly lethal neurotoxins through hybridization is not necessarily favored by natural selection in rattlesnakes, and that even extensive hybridization may not lead to introgression of these genes into another species.
KW  - adaptation
KW  - Crotalus
KW  - evolution
KW  - hybridization
KW  - introgression
KW  - Mojave toxin
KW  - molecular evolution
KW  - venom
Y1  - 2016
U6  - https://doi.org/10.3390/toxins8060188
SN  - 2072-6651
VL  - 8
PB  - MDPI
CY  - Basel
ER  - 
TY  - JOUR
A1  - González-Fortes, Gloria M.
A1  - Kolbe, Ben
A1  - Fernandes, Daniel
A1  - Meleg, Ioana N.
A1  - Garcia-Vazquez, Ana
A1  - Pinto-Llona, Ana C.
A1  - Constantin, Silviu
A1  - de Torres, Trino J.
A1  - Ortiz, Jose E.
A1  - Frischauf, Christine
A1  - Rabeder, Gernot
A1  - Hofreiter, Michael
A1  - Barlow, Axel
T1  - Ancient DNA reveals differences in behaviour and sociality between brown bears and extinct cave bears
JF  - Molecular ecology
N2  - Ancient DNA studies have revolutionized the study of extinct species and populations, providing insights on phylogeny, phylogeography, admixture and demographic history. However, inferences on behaviour and sociality have been far less frequent. Here, we investigate the complete mitochondrial genomes of extinct Late Pleistocene cave bears and middle Holocene brown bears that each inhabited multiple geographically proximate caves in northern Spain. In cave bears, we find that, although most caves were occupied simultaneously, each cave almost exclusively contains a unique lineage of closely related haplotypes. This remarkable pattern suggests extreme fidelity to their birth site in cave bears, best described as homing behaviour, and that cave bears formed stable maternal social groups at least for hibernation. In contrast, brown bears do not show any strong association of mitochondrial lineage and cave, suggesting that these two closely related species differed in aspects of their behaviour and sociality. This difference is likely to have contributed to cave bear extinction, which occurred at a time in which competition for caves between bears and humans was likely intense and the ability to rapidly colonize new hibernation sites would have been crucial for the survival of a species so dependent on caves for hibernation as cave bears. Our study demonstrates the potential of ancient DNA to uncover patterns of behaviour and sociality in ancient species and populations, even those that went extinct many tens of thousands of years ago.
KW  - ancient DNA
KW  - extinction
KW  - homing
KW  - sociality
KW  - Ursus arctos
KW  - Ursus spelaeus
Y1  - 2016
U6  - https://doi.org/10.1111/mec.13800
SN  - 0962-1083
SN  - 1365-294X
VL  - 25
SP  - 4907
EP  - 4918
PB  - Wiley-Blackwell
CY  - Hoboken
ER  - 
TY  - JOUR
A1  - Foti, Alessandro
A1  - Hartmann, Tobias
A1  - Coelho, Catarina
A1  - Santos-Silva, Teresa
A1  - Romao, Maria Joao
A1  - Leimkühler, Silke
T1  - Optimization of the Expression of Human Aldehyde Oxidase for Investigations of Single-Nucleotide Polymorphisms
JF  - Drug metabolism and disposition : the biological fate of chemicals
N2  - Aldehyde oxidase (AOX1) is an enzyme with broad substrate specificity, catalyzing the oxidation of a wide range of endogenous and exogenous aldehydes as well as N-heterocyclic aromatic compounds. In humans, the enzyme’s role in phase I drug metabolism has been established and its importance is now emerging. However, the true physiologic function of AOX1 in mammals is still unknown. Further, numerous single-nucleotide polymorphisms (SNPs) have been identified in human AOX1. SNPs are a major source of interindividual variability in the human population, and SNP-based amino acid exchanges in AOX1 reportedly modulate the catalytic function of the enzyme in either a positive or negative fashion. For the reliable analysis of the effect of amino acid exchanges in human proteins, the existence of reproducible expression systems for the production of active protein in ample amounts for kinetic, spectroscopic, and crystallographic studies is required. In our study we report an optimized expression system for hAOX1 in Escherichia coli using a codon-optimized construct. The codon-optimization resulted in an up to 15-fold increase of protein production and a simplified purification procedure. The optimized expression system was used to study three SNPs that result in amino acid changes C44W, G1269R, and S1271L. In addition, the crystal structure of the S1271L SNP was solved. We demonstrate that the recombinant enzyme can be used for future studies to exploit the role of AOX in drug metabolism, and for the identification and synthesis of new drugs targeting AOX when combined with crystallographic and modeling studies.
Y1  - 2016
U6  - https://doi.org/10.1124/dmd.115.068395
SN  - 0090-9556
SN  - 1521-009X
VL  - 44
SP  - 1277
EP  - 1285
PB  - American Society for Pharmacology and Experimental Therapeutics
CY  - Bethesda
ER  - 
TY  - THES
A1  - Connor, Daniel Oliver
T1  - Identifikation und Charakterisierung neuer immunogener Proteine und anschließende Generierung rekombinanter Antikörper mittels Phage Display
T1  - Identification and characterisation of novel immunogenic proteins and subsequent generation of recombinant antibodies by phage display
N2  - Seit der Einführung von Antibiotika in die medizinische Behandlung von bakteriellen Infektionskrankheiten existiert ein Wettlauf zwischen der Evolution von Bakterienresistenzen und der Entwicklung wirksamer Antibiotika. Während bis in die 80er Jahre verstärkt an neuen Antibiotika geforscht wurde, gewinnen multiresistente Keime heute zunehmend die Oberhand. Um einzelne Pathogene erfolgreich nachzuweisen und zu bekämpfen, ist ein grundlegendes Wissen über den Erreger unumgänglich. Bakterielle Proteine, die bei einer Infektion vorrangig vom Immunsystem prozessiert und präsentiert werden, könnten für die Entwicklung von Impfstoffen oder gezielten Therapeutika nützlich sein. Auch für die Diagnostik wären diese immundominanten Proteine interessant. Allerdings herrscht ein Mangel an Wissen über spezifische Antigene vieler pathogener Bakterien, die eine eindeutige Diagnostik eines einzelnen Erregers erlauben würden.
Daher wurden in dieser Arbeit vier verschiedene Humanpathogene mittels Phage Display untersucht: Neisseria gonorrhoeae, Neisseria meningitidis, Borrelia burgdorferi und Clostridium difficile. Hierfür wurden aus der genomischen DNA der vier Erreger Bibliotheken konstruiert und durch wiederholte Selektion und Amplifikation, dem sogenannten Panning, immunogene Proteine isoliert. Für alle Erreger bis auf C. difficile wurden immunogene Proteine aus den jeweiligen Bibliotheken isoliert. Die identifizierten Proteine von N. meningitidis und B. burgdorferi waren größtenteils bekannt, konnten aber in dieser Arbeit durch Phage Display verifiziert werden. Für N. gonorrhoeae wurden 21 potentiell immunogene Oligopeptide isoliert, von denen sechs Proteine als neue zuvor unbeschriebene Proteine mit immunogenem Charakter identifiziert wurden. Von den Phagen-präsentierten Oligopeptide der 21 immunogenen Proteine wurden Epitopmappings mit verschiedenen polyklonalen Antikörpern durchgeführt, um immunogene Bereiche näher zu identifizieren und zu charakterisieren. Bei zehn Proteinen wurden lineare Epitope eindeutig mit drei polyklonalen Antikörpern identifiziert, von fünf weiteren Proteinen waren Epitope mit mindestens einem Antikörper detektierbar. Für eine weitere Charakterisierung der ermittelten Epitope wurden Alaninscans durchgeführt, die eine detaillierte Auskunft über kritische Aminosäuren für die Bindung des Antikörpers an das Epitop geben.
Ausgehend von dem neu identifizierten Protein mit immunogenem Charakter NGO1634 wurden 26 weitere Proteine aufgrund ihrer funktionellen Ähnlichkeit ausgewählt und mithilfe bioinformatischer Analysen auf ihre Eignung zur Entwicklung einer diagnostischen Anwendung analysiert. Durch Ausschluss der meisten Proteine aufgrund ihrer Lokalisation, Membrantopologie oder unspezifischen Proteinsequenz wurden scFv-Antikörper gegen acht Proteine mittels Phage Display generiert und anschließend als scFv-Fc-Fusionsantikörper produziert und charakterisiert.
Die hier identifizierten Proteine und linearen Epitope könnten einen Ansatzpunkt für die Entwicklung einer diagnostischen oder therapeutischen Anwendung bieten. Lineare Epitopsequenzen werden häufig für die Impfstoffentwicklung eingesetzt, sodass vor allem die in dieser Arbeit bestimmten Epitope von Membranproteinen interessante Kandidaten für weitere Untersuchungen in diese Richtung sind. Durch weitere Untersuchungen könnten möglicherweise unbekannte Virulenzfaktoren entdeckt werden, deren Inhibierung einen entscheidenden Einfluss auf Infektionen haben könnten.
N2  - Since the advent of antibiotics into the field of medical therapy of bacterial infections, there has been a battle of effective antibiotics and the everlasting evolution of bacterial resistances. Until the 1980s many antibiotics were developed after invention of the first applied antibiotic penicillin in 1946. Since then, antibiotic research has been largely neglected resulting in the evolution of numerous strains from different bacteria with multiple resistances to available antibiotics. Therefore, extensive knowledge of a pathogen is crucial to detect and fight a particular disease. Hence, proteins that are processed and presented preferentially by the immune system during an infection could be beneficial for the development of vaccines and targeted therapeutic agents. Furthermore, immunodominant proteins could be interesting for the development of a diagnostic tool. However, many potential antigen targets of most pathogenic bacteria are still unknown.
On this account, four human pathogens were examined in this work utilising phage display: Neisseria gonorrhoeae, Neisseria meningitidis, Borrelia burgdorferi und Clostridium difficile. Phage libraries were constructed from genomic DNA of the four pathogens. These libraries were used to isolate immunogenic proteins by panning through repetitive rounds of selection and amplification. Immunogenic proteins were successfully isolated for all pathogens except C. difficile. The identified proteins from N. meningitidis and B. burgdorferi had mostly been described before. However, they were verified by phage display in this work. Twenty-one potentially immunogenic oligopeptides were isolated from the N. gonorrhoeae library. Six of those were identified as novel proteins with an immunogenic character and validated also as full length proteins. Epitope mappings were conducted for all of the 21 phage presented oligopeptides with different polyclonal antibodies to identify and characterise the immunogenic regions. Linear epitopes were found unambiguously for ten proteins with the three applied antibodies. In addition, epitopes for five proteins were identified with at least one antibody. The determined epitopes were then further characterized by alanine scans to investigate the impact of each individual amino acid on the binding of the antibody to the antigen’s epitope.
Based on the novel identified immunogenic protein NGO1634, 26 additional proteins were selected due to their functional resemblance. These proteins were analysed with bioinformatic tools and amongst others checked for their localisation, membrane topology and conservation of their protein sequence. Finally, scFv antibody fragments were isolated from a phage display library (HAL9/10) against eight proteins. The best antibodies were then produced as scFv-Fc fusion antibodies and their binding behaviour was further characterised.
The identified proteins and linear epitopes could serve as a starting point for the development of diagnostic or therapeutic tools. Further studies could unveil unknown virulence factors. Inhibition of those virulence factors could possibly have a vital impact on countering infections. Furthermore, linear epitopes are commonly used for vaccine development. Novel epitopes of membrane proteins could be interesting candidates for further immunization studies.
KW  - Immunogene Proteine
KW  - Phage Display
KW  - Rekombinante Antikörper
KW  - Neisseria gonorrhoeae
KW  - Neisseria meningitidis
KW  - Clostridium difficile
KW  - Borrelia burgdorferi
KW  - Epitopmapping
KW  - Immunogenic Proteins
KW  - Recombinant Antibodies
KW  - Epitope mapping
KW  - Phage Display
KW  - Neisseria gonorrhoeae
KW  - Neisseria meningitidis
KW  - Clostridium difficile
KW  - Borrelia burgdorferi
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-104120
ER  - 
TY  - JOUR
A1  - Correia, Marcia A. S.
A1  - Otrelo-Cardoso, Ana Rita
A1  - Schwuchow, Viola
A1  - Clauss, Kajsa G. V. Sigfridsson
A1  - Haumann, Michael
A1  - Romao, Maria Joao
A1  - Leimkühler, Silke
A1  - Santos-Silva, Teresa
T1  - The Escherichia coli Periplasmic Aldehyde Oxidoreductase Is an Exceptional Member of the Xanthine Oxidase Family of Molybdoenzymes
JF  - ACS chemical biology
N2  - The xanthine oxidase (XO) family comprises molybdenum-dependent enzymes that usually form homodimers (or dimers of heterodimers/trimers) organized in three domains that harbor two [2Fe-2S] clusters, one FAD, and a Mo cofactor. In this work, we crystallized an unusual member of the family, the periplasmic aldehyde oxidoreductase PaoABC from Escherichia coli. This is the first example of an E. coli protein containing a molybdopterin-cytosine-dinucleotide cofactor and is the only heterotrimer of the XO family so far structurally characterized. The crystal structure revealed the presence of an unexpected [4Fe-4S] cluster, anchored to an additional 40 residues subdomain. According to phylogenetic analysis, proteins containing this cluster are widely spread in many bacteria phyla, putatively through repeated gene transfer events. The active site of PaoABC is highly exposed to the surface with no aromatic residues and an arginine (PaoC-R440) making a direct interaction with PaoC-E692, which acts as a base catalyst. In order to understand the importance of R440, kinetic assays were carried out, and the crystal structure of the PaoC-R440H variant was also determined.
Y1  - 2016
U6  - https://doi.org/10.1021/acschembio.6b00572
SN  - 1554-8929
SN  - 1554-8937
VL  - 11
SP  - 2923
EP  - 2935
PB  - American Chemical Society
CY  - Washington
ER  - 
TY  - JOUR
A1  - Terao, Mineko
A1  - Romao, Maria Joao
A1  - Leimkühler, Silke
A1  - Bolis, Marco
A1  - Fratelli, Maddalena
A1  - Coelho, Catarina
A1  - Santos-Silva, Teresa
A1  - Garattini, Enrico
T1  - Structure and function of mammalian aldehyde oxidases
JF  - Archives of toxicology : official journal of EUROTOX
N2  - Mammalian aldehyde oxidases (AOXs; EC1.2.3.1) are a group of conserved proteins belonging to the family of molybdo-flavoenzymes along with the structurally related xanthine dehydrogenase enzyme. AOXs are characterized by broad substrate specificity, oxidizing not only aromatic and aliphatic aldehydes into the corresponding carboxylic acids, but also hydroxylating a series of heteroaromatic rings. The number of AOX isoenzymes expressed in different vertebrate species is variable. The two extremes are represented by humans, which express a single enzyme (AOX1) in many organs and mice or rats which are characterized by tissue-specific expression of four isoforms (AOX1, AOX2, AOX3, and AOX4). In vertebrates each AOX isoenzyme is the product of a distinct gene consisting of 35 highly conserved exons. The extant species-specific complement of AOX isoenzymes is the result of a complex evolutionary process consisting of a first phase characterized by a series of asynchronous gene duplications and a second phase where the pseudogenization and gene deletion events prevail. In the last few years remarkable advances in the elucidation of the structural characteristics and the catalytic mechanisms of mammalian AOXs have been made thanks to the successful crystallization of human AOX1 and mouse AOX3. Much less is known about the physiological function and physiological substrates of human AOX1 and other mammalian AOX isoenzymes, although the importance of these proteins in xenobiotic metabolism is fairly well established and their relevance in drug development is increasing. This review article provides an overview and a discussion of the current knowledge on mammalian AOX.
KW  - Aldehyde oxidase
KW  - Molybdo-flavoenzymes
KW  - Xanthine oxidoreductase
KW  - Drug metabolism
Y1  - 2016
U6  - https://doi.org/10.1007/s00204-016-1683-1
SN  - 0340-5761
SN  - 1432-0738
VL  - 90
SP  - 753
EP  - 780
PB  - Springer
CY  - Heidelberg
ER  - 
TY  - JOUR
A1  - Rotics, Shay
A1  - Kaatz, Michael
A1  - Resheff, Yehezkel S.
A1  - Turjeman, Sondra Feldman
A1  - Zurell, Damaris
A1  - Sapir, Nir
A1  - Eggers, Ute
A1  - Flack, Andrea
A1  - Fiedler, Wolfgang
A1  - Jeltsch, Florian
A1  - Wikelski, Martin
A1  - Nathan, Ran
T1  - The challenges of the first migration: movement and behaviour of juvenile vs. adult white storks with insights regarding juvenile mortality
JF  - Journal of animal ecology : a journal of the British Ecological Society
N2  - 1. Migration conveys an immense challenge, especially for juvenile birds coping with enduring and risky journeys shortly after fledging. Accordingly, juveniles exhibit considerably lower survival rates compared to adults, particularly during migration. Juvenile white storks (Ciconia ciconia), which are known to rely on adults during their first fall migration presumably for navigational purposes, also display much lower annual survival than adults.
2. Using detailed GPS and body acceleration data, we examined the patterns and potential causes of age-related differences in fall migration properties of white storks by comparing first-year juveniles and adults. We compared juvenile and adult parameters of movement, behaviour and energy expenditure (estimated from overall dynamic body acceleration) and placed this in the context of the juveniles’ lower survival rate.
3. Juveniles used flapping flight vs. soaring flight 23% more than adults and were estimated to expend 14% more energy during flight. Juveniles did not compensate for their higher flight costs by increased refuelling or resting during migration. When juveniles and adults migrated together in the same flock, the juvenile flew mostly behind the adult and was left behind when they separated. Juveniles showed greater improvement in flight efficiency throughout migration compared to adults which appears crucial because juveniles exhibiting higher flight costs suffered increased mortality.
4. Our findings demonstrate the conflict between the juveniles’ inferior flight skills and their urge to keep up with mixed adult–juvenile flocks. We suggest that increased flight costs are an important proximate cause of juvenile mortality in white storks and likely in other soaring migrants and that natural selection is operating on juvenile variation in flight efficiency.
KW  - flight
KW  - flight efficiency
KW  - juvenile mortality
KW  - migration
KW  - white stork
Y1  - 2016
U6  - https://doi.org/10.1111/1365-2656.12525
SN  - 0021-8790
SN  - 1365-2656
VL  - 85
SP  - 938
EP  - 947
PB  - Wiley-Blackwell
CY  - Hoboken
ER  - 
TY  - JOUR
A1  - Tanski, George
A1  - Couture, Nicole
A1  - Lantuit, Hugues
A1  - Eulenburg, Antje
A1  - Fritz, Michael
T1  - Eroding permafrost coasts release low amounts of dissolved organic carbon (DOC) from ground ice into the nearshore zone of the Arctic Ocean
JF  - Global biogeochemical cycles
N2  - Ice-rich permafrost coasts in the Arctic are highly sensitive to climate warming and erode at a pace that exceeds the global average. Permafrost coasts deliver vast amounts of organic carbon into the nearshore zone of the Arctic Ocean. Numbers on flux exist for particulate organic carbon (POC) and total or soil organic carbon (TOC, SOC). However, they do not exist for dissolved organic carbon (DOC), which is known to be highly bioavailable. This study aims to estimate DOC stocks in coastal permafrost as well as the annual flux into the ocean. DOC concentrations in ground ice were analyzed along the ice-rich Yukon coast (YC) in the western Canadian Arctic. The annual DOC flux was estimated using available numbers for coast length, cliff height, annual erosion rate, and volumetric ice content in different stratigraphic horizons. Our results showed that DOC concentrations in ground ice range between 0.3 and 347.0mgL(-1) with an estimated stock of 13.63.0gm(-3) along the YC. An annual DOC flux of 54.90.9Mgyr(-1) was computed. These DOC fluxes are low compared to POC and SOC fluxes from coastal erosion or POC and DOC fluxes from Arctic rivers. We conclude that DOC fluxes from permafrost coasts play a secondary role in the Arctic carbon budget. However, this DOC is assumed to be highly bioavailable. We hypothesize that DOC from coastal erosion is important for ecosystems in the Arctic nearshore zones, particularly in summer when river discharge is low, and in areas where rivers are absent.
KW  - Arctic
KW  - permafrost
KW  - coastal erosion
KW  - biogeochemistry
KW  - carbon cycle
Y1  - 2016
U6  - https://doi.org/10.1002/2015GB005337
SN  - 0886-6236
SN  - 1944-9224
VL  - 30
SP  - 1054
EP  - 1068
PB  - American Geophysical Union
CY  - Cambridge
ER  - 
TY  - GEN
A1  - Wessig, Pablo
A1  - Bader, Denise
A1  - Klier, Dennis Tobias
A1  - Hettrich, Cornelia
A1  - Bier, Frank Fabian
T1  - Detecting carbohydrate–lectin interactions using a fluorescent probe based on DBD dyes
N2  - Herein we present an efficient synthesis of a biomimetic probe with modular construction that can be specifically bound by the mannose binding FimH protein – a surface adhesion protein of E. coli bacteria. The synthesis combines the new and interesting DBD dye with the carbohydrate ligand mannose via a Click reaction. We demonstrate the binding to E. coli bacteria over a large concentration range and also present some special characteristics of those molecules that are of particular interest for the application as a biosensor. In particular, the mix-and-measure ability and the very good photo-stability should be highlighted here.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 314 
KW  - conformational-changes
KW  - green-i
KW  - protein
KW  - binding
KW  - assay
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-394382
SP  - 1235
EP  - 1238
ER  - 
TY  - JOUR
A1  - Cazelles, R.
A1  - Lalaoui, N.
A1  - Hartmann, Tobias
A1  - Leimkühler, Silke
A1  - Wollenberger, Ursula
A1  - Antonietti, Markus
A1  - Cosnier, S.
T1  - Ready to use bioinformatics analysis as a tool to predict immobilisation strategies for protein direct electron transfer (DET)
JF  - Polymer : the international journal for the science and technology of polymers
KW  - Bioinformatic
KW  - Bioelectrocatalysis
KW  - Electron transfer
KW  - Dehydrogenase
KW  - Nicotinamide
Y1  - 2016
U6  - https://doi.org/10.1016/j.bios.2016.04.078
SN  - 0956-5663
SN  - 1873-4235
VL  - 85
SP  - 90
EP  - 95
PB  - Elsevier
CY  - Oxford
ER  - 
TY  - JOUR
A1  - Roggenbuck, Dirk
A1  - Borghi, Maria Orietta
A1  - Somma, Valentina
A1  - Buettner, Thomas
A1  - Schierack, Peter
A1  - Hanack, Katja
A1  - Grossi, Claudia
A1  - Bodio, Caterina
A1  - Macor, Paolo
A1  - von Landenberg, Philipp
A1  - Boccellato, Francesco
A1  - Mahler, Michael
A1  - Meroni, Pier Luigi
T1  - Antiphospholipid antibodies detected by line immunoassay differentiate among patients with antiphospholipid syndrome, with infections and asymptomatic carriers
JF  - IEEE transactions on geoscience and remote sensing
N2  - Background: Antiphospholipid antibodies (aPL) can be detected in asymptomatic carriers and infectious patients. The aim was to investigate whether a novel line immunoassay (LIA) differentiates between antiphospholipid syndrome (APS) and asymptomatic aPL+ carriers or patients with infectious diseases (infectious diseases controls (IDC)). Methods: Sixty-one patients with APS (56 primary, 22/56 with obstetric events only, and 5 secondary), 146 controls including 24 aPL+ asymptomatic carriers and 73 IDC were tested on a novel hydrophobic solid phase coated with cardiolipin (CL), phosphatic acid, phosphatidylcholine, phosphatidylethanolamine, phosphatidylglycerol, phosphatidylinositol, phosphatidylserine, beta2-glycoprotein I (beta 2GPI), prothrombin, and annexin V. Samples were also tested by anti-CL and anti-beta 2GPI ELISAs and for lupus anticoagulant activity. Human monoclonal antibodies (humoAbs) against human beta 2GPI or PL alone were tested on the same LIA substrates in the absence or presence of human serum, purified human beta 2GPI or after CL-micelle absorption. Results: Comparison of LIA with the aPL-classification assays revealed good agreement for IgG/IgM a beta 2GPI and aCL. Anti-CL and anti-beta 2GPI IgG/IgM reactivity assessed by LIA was significantly higher in patients with APS versus healthy controls and IDCs, as detected by ELISA. IgG binding to CL and beta 2GPI in the LIA was significantly lower in aPL+ carriers and Venereal Disease Research Laboratory test (VDRL) + samples than in patients with APS. HumoAb against domain 1 recognized beta 2GPI bound to the LIA-matrix and in anionic phospholipid (PL) complexes. Absorption with CL micelles abolished the reactivity of a PL-specific humoAb but did not affect the binding of anti-beta 2GPI humoAbs. Conclusions: The LIA and ELISA have good agreement in detecting aPL in APS, but the LIA differentiates patients with APS from infectious patients and asymptomatic carriers, likely through the exposure of domain 1.
KW  - Antiphospholipid syndrome
KW  - Antiphospholipid antibody
KW  - Phospholipid binding proteins
KW  - Beta2-glycoprotein I
KW  - Line immunoassay
Y1  - 2016
U6  - https://doi.org/10.1186/s13075-016-1018-x
SN  - 1478-6354
SN  - 1478-6362
VL  - 18
PB  - BioMed Central
CY  - London
ER  - 
TY  - GEN
A1  - Hanack, Katja
A1  - Schloer, Anja
A1  - Holzloehner, Pamela
A1  - Listek, Martin
A1  - Bauer, Cindy
A1  - Butze, Monique
A1  - Micheel, Burkhard
A1  - Hentschel, Christian
A1  - Sowa, Mandy
A1  - Roggenbuck, Dirk
A1  - Schierack, Peter
A1  - Fuener, Jonas
A1  - Schliebs, Erik
A1  - Goihl, Alexander
A1  - Reinhold, Dirk
T1  - Camelid nanobodies specific to human pancreatic glycoprotein 2
T2  - The journal of immunology
N2  - Pancreatic secretory zymogen-granule membrane glycoprotein 2 (GP2) has been identified to be a major autoantigenic target in Crohn’s disease patients. It was discussed recently that a long and a short isoform of GP2 exists whereas the short isoform is often detected by GP2-specific autoantibodies. In the outcome of inflammatory bowel diseases, these GP2-specific autoantibodies are discussed as new serological markers for diagnosis and therapeutic monitoring. To investigate this further, camelid nanobodies were generated by phage display and selected against the short isoform of GP2 in order to isolate specific tools for the discrimination of both isoforms. Nanobodies are single domain antibodies derived from camelid heavy chain only antibodies and characterized by a high stability and solubility. The selected candidates were expressed, purified and validated regarding their binding properties in different enzyme-linked immunosorbent assays formats, immunofluorescence, immunohistochemistry and surface plasmon resonance spectroscopy. Four different nanobodies could be selected whereof three recognize the short isoform of GP2 very specifically and one nanobody showed a high binding capacity for both isoforms. The KD values measured for all nanobodies were between 1.3 nM and 2.3 pM indicating highly specific binders suitable for the application as diagnostic tool in inflammatory bowel disease.
Y1  - 2016
SN  - 0022-1767
SN  - 1550-6606
VL  - 196
SP  - 313
EP  - 328
PB  - American Assoc. of Immunologists
CY  - Bethesda
ER  - 
TY  - GEN
A1  - Maier, Natalia
A1  - Holzlöhner, Pamela
A1  - Hoenow, Anja
A1  - Scheunemann, Astrid
A1  - Weschke, Daniel
A1  - Hanack, Katja
T1  - Characterization of monoclonal antibodies generated by in vitro immunization
T2  - The journal of immunology
N2  - Monoclonal antibodies are highly valuable tools in biomedicine but the generation by hybridoma technology is very time-consuming and elaborate. In order to circumvent the consisting drawbacks an in vitro immunization approach was established by which murine as well as human monoclonal antibodies against a viral coat protein could be developed. The in vitro immunization process was performed by isolation of murine hematopoietic stem cells or human monocytes and an in vitro differentiation into immature dendritic cells. After antigen loading the cells were co-cultivated with naive T and B lymphocytes for three days in order to obtain antigen-specific B lymphocytes in culture, followed by fusion with murine myeloma cells or human/murine heteromyeloma cells. Antigen-specific hybridomas were selected and the generated antibodies were purified and characterized in this study by ELISA, western blot, gene sequencing, affinity measurements. Further the characteristics were compared to a monoclonal antibody against the same target generated by conventional hybridoma technology. Isotype detection revealed a murine IgM and a human IgG4 antibody in comparison to an IgG1 for the conventionally generated antibody. The antibodies derived from in vitro immunization showed indeed a lower affinity for the antigen as compared to the conventionally generated one, which is probably based on the significantly shorter B cell maturation (3 days) during the immunization process. Nevertheless, they were suitable for building up a sandwich based detection system. Therefore, the in vitro immunization approach seems to be a good and particularly fast alternative to conventional hybridoma technology.
Y1  - 2016
SN  - 0022-1767
SN  - 1550-6606
VL  - 196
PB  - American Assoc. of Immunologists
CY  - Bethesda
ER  - 
TY  - THES
A1  - Maier, Natalia
T1  - Aufbau eines Testsystems zum Nachweis von Ethylglucuronid (EtG) in Haaren
Y1  - 2016
ER  - 
TY  - GEN
A1  - Roggenbuck, Dirk
A1  - Borghi, Maria Orietta
A1  - Somma, Valentina
A1  - Büttner, Thomas
A1  - Schierack, Peter
A1  - Hanack, Katja
A1  - Grossi, Claudia
A1  - Bodio, Caterina
A1  - Macor, Paolo
A1  - von Landenberg, Philipp
A1  - Boccellato, Francesco
A1  - Mahler, Michael
A1  - Meroni, Pier Luigi
T1  - Antiphospholipid antibodies detected by line immunoassay differentiate among patients with antiphospholipid syndrome, with infections and asymptomatic carriers
T2  - Postprints der Universität Potsdam Mathematisch-Naturwissenschaftliche Reihe
N2  - Background

Antiphospholipid antibodies (aPL) can be detected in asymptomatic carriers and infectious patients. The aim was to investigate whether a novel line immunoassay (LIA) differentiates between antiphospholipid syndrome (APS) and asymptomatic aPL+ carriers or patients with infectious diseases (infectious diseases controls (IDC)).
Methods

Sixty-one patients with APS (56 primary, 22/56 with obstetric events only, and 5 secondary), 146 controls including 24 aPL+ asymptomatic carriers and 73 IDC were tested on a novel hydrophobic solid phase coated with cardiolipin (CL), phosphatic acid, phosphatidylcholine, phosphatidylethanolamine, phosphatidylglycerol, phosphatidylinositol, phosphatidylserine, beta2-glycoprotein I (β2GPI), prothrombin, and annexin V. Samples were also tested by anti-CL and anti-β2GPI ELISAs and for lupus anticoagulant activity. Human monoclonal antibodies (humoAbs) against human β2GPI or PL alone were tested on the same LIA substrates in the absence or presence of human serum, purified human β2GPI or after CL-micelle absorption.
Results

Comparison of LIA with the aPL-classification assays revealed good agreement for IgG/IgM aß2GPI and aCL. Anti-CL and anti-ß2GPI IgG/IgM reactivity assessed by LIA was significantly higher in patients with APS versus healthy controls and IDCs, as detected by ELISA. IgG binding to CL and ß2GPI in the LIA was significantly lower in aPL+ carriers and Venereal Disease Research Laboratory test (VDRL) + samples than in patients with APS. HumoAb against domain 1 recognized β2GPI bound to the LIA-matrix and in anionic phospholipid (PL) complexes. Absorption with CL micelles abolished the reactivity of a PL-specific humoAb but did not affect the binding of anti-β2GPI humoAbs.
Conclusions

The LIA and ELISA have good agreement in detecting aPL in APS, but the LIA differentiates patients with APS from infectious patients and asymptomatic carriers, likely through the exposure of domain 1.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 436 
KW  - Antiphospholipid syndrome
KW  - Antiphospholipid antibody
KW  - Phospholipid binding proteins
KW  - Beta2 - glycoprotein I
KW  - Line immunoassay
Y1  - 2018
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-407211
SN  - 1866-8372
IS  - 436
ER  - 
TY  - GEN
A1  - Holzlöhner, Pamela
A1  - Butze, Monique
A1  - Hebel, Nicole
A1  - Weschke, Daniel
A1  - Schliebs, E.
A1  - Naumann, F.
A1  - Füner, J.
A1  - Micheel, Burkhard
A1  - Hanack, Katja
T1  - Monoclonal mouse antibodies against PBMC subpopulations of New World camelides
T2  - European journal of immunology
Y1  - 2016
SN  - 0014-2980
SN  - 1521-4141
VL  - 46
SP  - 1175
EP  - 1175
PB  - Wiley-Blackwell
CY  - Hoboken
ER  - 
TY  - JOUR
A1  - Schmidt, Carsten
A1  - Roediger, Stefan
A1  - Gruner, Melanie
A1  - Moncsek, Anja
A1  - Stohwasser, Ralf
A1  - Hanack, Katja
A1  - Schierack, Peter
A1  - Schroeder, Christian
T1  - Multiplex localization of sequential peptide epitopes by use of a planar microbead chip
JF  - Analytica chimica acta : an international journal devoted to all branches of analytical chemistry
N2  - Epitope mapping is crucial for the characterization of protein-specific antibodies. Commonly, small overlapping peptides are chemically synthesized and immobilized to determine the specific peptide sequence. In this study, we report the use of a fast and inexpensive planar microbead chip for epitope mapping. We developed a generic strategy for expressing recombinant peptide libraries instead of using expensive synthetic peptide libraries. A biotin moiety was introduced in vivo at a defined peptide position using biotin ligase. Peptides in crude Escherichia coli lysate were coupled onto streptavidin-coated microbeads by incubation, thereby avoiding tedious purification procedures. For read-out we used a multiplex planar microbead chip with size- and fluorescence-encoded microbead populations. For epitope mapping, up to 18 populations of peptide-loaded microbeads (at least 20 microbeads per peptide) displaying the primary sequence of a protein were analyzed simultaneously. If an epitope was recognized by an antibody, a secondary fluorescence-labeled antibody generated a signal that was quantified, and the mean value of all microbeads in the population was calculated. We mapped the epitopes for rabbit anti-PA28 gamma (proteasome activator 28 gamma) polyclonal serum, for a murine monoclonal antibody against PA28 gamma, and for a murine monoclonal antibody against the hamster polyoma virus major capsid protein VP1 as models. In each case, the identification of one distinct peptide sequence out of up to 18 sequences was possible. Using this approach, an epitope can be mapped multiparametrically within three weeks. (C) 2016 Elsevier B.V. All rights reserved.
KW  - Epitope mapping
KW  - In vivo biotinylation
KW  - Multiplexed assays
KW  - Microbeads
KW  - VideoScan technology
Y1  - 2016
U6  - https://doi.org/10.1016/j.aca.2015.12.030
SN  - 0003-2670
SN  - 1873-4324
VL  - 908
SP  - 150
EP  - 160
PB  - Elsevier
CY  - Amsterdam
ER  - 
TY  - GEN
A1  - Rainford, James L.
A1  - Hofreiter, Michael
A1  - Mayhew, Peter J.
T1  - Phylogenetic analyses suggest that diversification and body size evolution are independent in insects
T2  - BMC evolutionary biology
N2  - Background:
Skewed body size distributions and the high relative richness of small-bodied taxa are a fundamental
property of a wide range of animal clades. The evolutionary processes responsible for generating these distributions
are well described in vertebrate model systems but have yet to be explored in detail for other major terrestrial
clades. In this study, we explore the macro-evolutionary patterns of body size variation across families of Hexapoda
(insects and their close relatives), using recent advances in phylogenetic understanding, with an aim to investigate
the link between size and diversity within this ancient and highly diverse lineage.
Results:
The maximum, minimum and mean-log body lengths of hexapod families are all approximately log-normally
distributed, consistent with previous studies at lower taxonomic levels, and contrasting with skewed distributions
typical of vertebrate groups. After taking phylogeny and within-tip variation into account, we find no evidence for a
negative relationship between diversification rate and body size, suggesting decoupling of the forces controlling these
two traits. Likelihood-based modeling of the log-mean body size identifies distinct processes operating within
Holometabola and Diptera compared with other hexapod groups, consistent with accelerating rates of size evolution
within these clades, while as a whole, hexapod body size evolution is found to be dominated by neutral processes
including significant phylogenetic conservatism.
Conclusions:
Based on our findings we suggest that the use of models derived from well-studied but atypical clades,
such as vertebrates may lead to misleading conclusions when applied to other major terrestrial lineages. Our results
indicate that within hexapods, and within the limits of current systematic and phylogenetic knowledge, insect
diversification is generally unfettered by size-biased macro-evolutionary processes, and that these processes over large
timescales tend to converge on apparently neutral evolutionary processes. We also identify limitations on available
data within the clade and modeling approaches for the resolution of trees of higher taxa, the resolution of which may
collectively enhance our understanding of this key component of terrestrial ecosystems.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 441 
KW  - body size
KW  - diversification
KW  - hexapoda
KW  - insects
KW  - phylogeny
Y1  - 2018
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-407328
ER  -