TY  - JOUR
A1  - Spikes, Montrai
A1  - Rodríguez-Silva, Rodet
A1  - Bennett, Kerri-Ann
A1  - Bräger, Stefan
A1  - Josaphat, James
A1  - Torres-Pineda, Patricia
A1  - Ernst, Anja
A1  - Havenstein, Katja
A1  - Schlupp, Ingo
A1  - Tiedemann, Ralph
T1  - A phylogeny of the genus Limia (Teleostei: Poeciliidae) suggests a single-lake radiation nested in a Caribbean-wide allopatric speciation scenario
JF  - BMC Research Notes
N2  - Objective
The Caribbean is an important global biodiversity hotspot. Adaptive radiations there lead to many speciation events within a limited period and hence are particularly prominent biodiversity generators. A prime example are freshwater fish of the genus Limia, endemic to the Greater Antilles. Within Hispaniola, nine species have been described from a single isolated site, Lake Miragoâne, pointing towards extraordinary sympatric speciation. This study examines the evolutionary history of the Limia species in Lake Miragoâne, relative to their congeners throughout the Caribbean.

Results
For 12 Limia species, we obtained almost complete sequences of the mitochondrial cytochrome b gene, a well-established marker for lower-level taxonomic relationships. We included sequences of six further Limia species from GenBank (total N  = 18 species). Our phylogenies are in concordance with other published phylogenies of Limia. There is strong support that the species found in Lake Miragoâne in Haiti are monophyletic, confirming a recent local radiation. Within Lake Miragoâne, speciation is likely extremely recent, leading to incomplete lineage sorting in the mtDNA. Future studies using multiple unlinked genetic markers are needed to disentangle the relationships within the Lake Miragoâne clade.
KW  - Cytochrome b
KW  - Island biogeography
KW  - Fresh water fish
KW  - Phylogeny
Y1  - 2021
U6  - https://doi.org/10.1186/s13104-021-05843-x
SN  - 1756-0500
VL  - 14
SP  - 1
EP  - 8
PB  - BMC Research Notes / Biomed Central
CY  - London
ER  - 
TY  - THES
A1  - Stanke, Sandra
T1  - AC electrokinetic immobilization of influenza viruses and antibodies on nanoelectrode arrays for on-chip immunoassays
T1  - AC elektrokinetische Immobilisierung von Influenzaviren und Antikörpern auf Nanoelektrodenarrays für on-Chip Immunoassays
N2  - In the present thesis, AC electrokinetic forces, like dielectrophoresis and AC electroosmosis, were demonstrated as a simple and fast method to functionalize the surface of nanoelectrodes with submicrometer sized biological objects. These nanoelectrodes have a cylindrical shape with a diameter of 500 nm arranged in an array of 6256 electrodes. Due to its medical relevance influenza virus as well as anti-influenza antibodies were chosen as a model organism. Common methods to bring antibodies or proteins to biosensor surfaces are complex and time-consuming. In the present work, it was demonstrated that by applying AC electric fields influenza viruses and antibodies can be immobilized onto the nanoelectrodes within seconds without any prior chemical modification of neither the surface nor the immobilized biological object. The distribution of these immobilized objects is not uniform over the entire array, it exhibits a decreasing gradient from the outer row to the inner ones. Different causes for this gradient have been discussed, such as the vortex-shaped fluid motion above the nanoelectrodes generated by, among others, electrothermal fluid flow. It was demonstrated that parts of the accumulated material are permanently immobilized to the electrodes. This is a unique characteristic of the presented system since in the literature the AC electrokinetic immobilization is almost entirely presented as a method just for temporary immobilization. The spatial distribution of the immobilized viral material or the anti-influenza antibodies at the electrodes was observed by either the combination of fluorescence microscopy and deconvolution or by super-resolution microscopy (STED). On-chip immunoassays were performed to examine the suitability of the functionalized electrodes as a potential affinity-based biosensor. Two approaches were pursued: A) the influenza virus as the bio-receptor or B) the influenza virus as the analyte. Different sources of error were eliminated by ELISA and passivation experiments. Hence, the activity of the immobilized object was inspected by incubation with the analyte. This resulted in the successful detection of anti-influenza antibodies by the immobilized viral material. On the other hand, a detection of influenza virus particles by the immobilized anti-influenza antibodies was not possible. The latter might be due to lost activity or wrong orientation of the antibodies. Thus, further examinations on the activity of by AC electric fields immobilized antibodies should follow. When combined with microfluidics and an electrical read-out system, the functionalized chips possess the potential to serve as a rapid, portable, and cost-effective point-of-care (POC) device. This device can be utilized as a basis for diverse applications in diagnosing and treating influenza, as well as various other pathogens.
N2  - In der vorliegenden Arbeit wurden AC elektrokinetische Kräfte, wie die Dielektrophorese und die AC Elektroosmose, als einfache und schnelle Methode zur Funktionalisierung der Oberfläche von Nanoelektroden mit biologischen Objekten in Submikrometergröße demonstriert. Diese Nanoelektroden haben eine zylindrische Form mit einem Durchmesser von 500 nm und sind in einem Array aus 6256 Elektroden angeordnet. Aufgrund ihrer medizinischen Relevanz wurden Influenzaviren sowie anti-Influenza Antikörper als Modellorganismus ausgewählt. Gängige Methoden, um Antikörper oder Proteine auf Biosensoroberflächen zu bringen, sind komplex und zeitaufwändig. In der vorliegenden Arbeit wurde gezeigt, dass durch die Anwendung elektrischer Wechselfelder Influenzaviren und Antikörper innerhalb von Sekunden auf den Nanoelektroden immobilisiert werden können, ohne dass zuvor eine chemische Modifikation der Oberfläche noch des immobilisierten biologischen Objekts erforderlich ist. Die Verteilung dieser immobilisierten Objekte ist über das gesamte Array ungleichmäßig. Es kommt zur Ausbildung eines Gradienten, welcher von der äußeren zur den inneren Reihen hin abnimmt. Verschiedene Ursachen für diesen Gradienten wurden diskutiert, beispielsweise der Vortex-förmige Flüssigkeitsstrom über den Nanoelektroden, der unter anderem durch elektrothermische Flüssigkeitsbewegung erzeugt wird. Es wurde gezeigt, dass Teile des akkumulierten Materials dauerhaft an den Elektroden immobilisiert sind. Dies ist ein Alleinstellungsmerkmal des vorgestellten Systems, da in der Literatur die AC elektrokinetische Immobilisierung fast ausschließlich als Methode nur zur temporären Immobilisierung dargestellt wird. Die räumliche Verteilung des immobilisierten Virusmaterials bzw. der anti-Influenza Antikörper an den Elektroden wurde entweder durch die Kombination aus Fluoreszenzmikroskopie und Dekonvolution oder durch super-resolution Mikroskopie (STED) betrachtet. Es wurden On-Chip-Immunoassays durchgeführt, um die Eignung der funktionalisierten Elektroden für einen potenziellen affinitätsbasierten Biosensor zu untersuchen. Dabei wurden zwei Ansätze verfolgt: A) Influenzaviren als Biorezeptor oder B) Influenzavirus als Analyt. Verschiedene Fehlerquellen wurden mittels ELISA und Passivierungsexperimente eliminiert. Infolgedessen wurde die Aktivität der immobilisierten Objekte durch Inkubation mit dem Analyten überprüft. Dies führte zum erfolgreichen Nachweis von anti-Influenza Antikörpern mittels immobilisiertem Virusmaterial. Andererseits war ein Nachweis von Influenzaviruspartikeln durch die immobilisierten anti-Influenza Antikörper nicht möglich. Letzteres könnte auf einen Aktivitätsverlust oder eine falsche Ausrichtung der Antikörper zurückzuführen sein. Daher sollten weitere Untersuchungen zur Aktivität von durch elektrische Wechselfelder immobilisierte Antikörper folgen. In Kombination mit Mikrofluidik und einem elektrischen Auslesesystem besitzen die funktionalisierten Chips das Potenzial, als schnelle, tragbare und kostengünstige Point-of-Care-Einheit (POC) zu dienen. Dieses Einheit kann als Grundlage für vielfältige Anwendungen bei der Diagnose und Behandlung von Influenza und verschiedenen anderen Krankheitserregern genutzt werden.
KW  - AC electrokinetics
KW  - AC Elektrokinetik
KW  - AC electroosmosis
KW  - AC Elektroosmosis
KW  - dielectrophoresis
KW  - Dielektrophorese
KW  - virus
KW  - Virus
KW  - influenza
KW  - Influenza
KW  - antibody
KW  - Antikörper
KW  - nanoelectrodes
KW  - Nanoelektroden
KW  - lab-on-chip
KW  - lab-on-chip
KW  - LOC
KW  - LOC
KW  - point-of-care
KW  - point-of-care
KW  - POC
KW  - POC
KW  - immunoassay
KW  - Immunoassay
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-617165
ER  - 
TY  - JOUR
A1  - Reeg, Jette
A1  - Strigl, Lea
A1  - Jeltsch, Florian
T1  - Agricultural buffer zone thresholds to safeguard functional bee diversity
BT  - Insights from a community modeling approach
JF  - Ecology and Evolution
N2  - Wild bee species are important pollinators in agricultural landscapes. However, population decline was reported over the last decades and is still ongoing. While agricultural intensification is a major driver of the rapid loss of pollinating species, transition zones between arable fields and forest or grassland patches, i.e., agricultural buffer zones, are frequently mentioned as suitable mitigation measures to support wild bee populations and other pollinator species. Despite the reported general positive effect, it remains unclear which amount of buffer zones is needed to ensure a sustainable and permanent impact for enhancing bee diversity and abundance. To address this question at a pollinator community level, we implemented a process-based, spatially explicit simulation model of functional bee diversity dynamics in an agricultural landscape. More specifically, we introduced a variable amount of agricultural buffer zones (ABZs) at the transition of arable to grassland, or arable to forest patches to analyze the impact on bee functional diversity and functional richness. We focused our study on solitary bees in a typical agricultural area in the Northeast of Germany. Our results showed positive effects with at least 25% of virtually implemented agricultural buffer zones. However, higher amounts of ABZs of at least 75% should be considered to ensure a sufficient increase in Shannon diversity and decrease in quasi-extinction risks. These high amounts of ABZs represent effective conservation measures to safeguard the stability of pollination services provided by solitary bee species. As the model structure can be easily adapted to other mobile species in agricultural landscapes, our community approach offers the chance to compare the effectiveness of conservation measures also for other pollinator communities in future.
KW  - agricultural landscape
KW  - buffer zones
KW  - community model
KW  - functional traits
KW  - solitary bees
KW  - spatially explicit
Y1  - 2022
U6  - https://doi.org/10.1002/ece3.8748
SN  - 2045-7758
VL  - 12
SP  - 1
EP  - 17
PB  - Wiley Online Library
CY  - Hoboken, New Jersey, USA
ET  - 3
ER  - 
TY  - JOUR
A1  - Warschburger, Petra
A1  - Wortmann, Hanna Rosalie
A1  - Gisch, Ulrike Alexandra
A1  - Baer, Nadja-Raphaela
A1  - Schenk, Liane
A1  - Anton, Verena
A1  - Bergmann, Manuela M.
T1  - An experimental approach to training interoceptive sensitivity
BT  - study protocol for a pilot randomized controlled trial
JF  - Nutrition Journal
N2  - Background
Eating in absence of hunger is quite common and often associated with an increased energy intake co-existent with a poorer food choice. Intuitive eating (IE), i.e., eating in accordance with internal hunger and satiety cues, may protect from overeating. IE, however, requires accurate perception and processing of one’s own bodily signals, also referred to as interoceptive sensitivity. Training interoceptive sensitivity might therefore be an effective method to promote IE and prevent overeating. As most studies on eating behavior are conducted in younger adults and close social relationships influence health-related behavior, this study focuses on middle-aged and older couples.

Methods
The present pilot randomized intervention study aims at investigating the feasibility and effectiveness of a 21-day mindfulness-based training program designed to increase interoceptive sensitivity. A total of N = 60 couples participating in the NutriAct Family Study, aged 50–80 years, will be recruited. This randomized-controlled intervention study comprises three measurement points (pre-intervention, post-intervention, 4-week follow-up) and a 21-day training that consists of daily mindfulness-based guided audio exercises (e.g., body scan). A three-arm intervention study design is applied to compare two intervention groups (training together as a couple vs. training alone) with a control group (no training). Each measurement point includes the assessment of self-reported and objective indicators of interoceptive sensitivity (primary outcome), self-reported indicators of intuitive and maladaptive eating (secondary outcomes), and additional variables. A training evaluation applying focus group discussions will be conducted to assess participants’ overall acceptance of the training and its feasibility.

Discussion
By investigating the feasibility and effectiveness of a mindfulness-based training program to increase interoceptive sensitivity, the present study will contribute to a deeper understanding of how to promote healthy eating in older age.
KW  - Digital intervention
KW  - Older adults
KW  - Interoception
KW  - Eating behavior
KW  - Intuitive eating
KW  - Partnership
KW  - Mindfulness
KW  - Randomized-controlled trial
KW  - NutriAct Family Study
KW  - Mixed methods
Y1  - 2022
U6  - https://doi.org/10.1186/s12937-022-00827-4
SN  - 1475-2891
VL  - 21
PB  - Springer Nature
CY  - London
ER  - 
TY  - THES
A1  - Rolo, David
T1  - Assembly of photosystem I in thylakoid membranes
T1  - Die Assemblierung des Photosystems I in der Thylakoidmembran
N2  - The light reactions of photosynthesis are carried out by a series of multiprotein complexes embedded in thylakoid membranes. Among them, photosystem I (PSI), acting as plastocyanin-ferderoxin oxidoreductase, catalyzes the final reaction. Together with light-harvesting antenna I, PSI forms a high-molecular-weight supercomplex of ~600 kDa, consisting of eighteen subunits and nearly two hundred co-factors. Assembly of the various components into a functional thylakoid membrane complex requires precise coordination, which is provided by the assembly machinery. Although this includes a small number of proteins (PSI assembly factors) that have been shown to play a role in the formation of PSI, the process as a whole, as well as the intricacy of its members, remains largely unexplored.
In the present work, two approaches were used to find candidate PSI assembly factors. First, EnsembleNet was used to select proteins thought to be functionally related to known PSI assembly factors in Arabidopsis thaliana (approach I), and second, co-immunoprecipitation (Co-IP) of tagged PSI assembly factors in Nicotiana tabacum was performed (approach II).
Here, the novel PSI assembly factors designated CO-EXPRESSED WITH PSI ASSEMBLY 1 (CEPA1) and Ycf4-INTERACTING PROTEIN 1 (Y4IP1) were identified. A. thaliana null mutants for CEPA1 and Y4IP1 showed a growth phenotype and pale leaves compared with the wild type. Biophysical experiments using pulse amplitude modulation (PAM) revealed insufficient electron transport on the PSII acceptor side. Biochemical analyses revealed that both CEPA1 and Y4IP1 are specifically involved in PSI accumulation in A. thaliana at the post-translational level but are not essential. Consistent with their roles as factors in the assembly of a thylakoid membrane protein complex, the two proteins localize to thylakoid membranes. Remarkably, cepa1 y4ip1 double mutants exhibited lethal phenotypes in early developmental stages under photoautotrophic growth. Finally, co-IP and native gel experiments supported a possible role for CEPA1 and Y4IP1 in mediating PSI assembly in conjunction with other PSI assembly factors (e.g., PPD1- and PSA3-CEPA1 and Ycf4-Y4IP1). The fact that CEPA1 and Y4IP1 are found exclusively in green algae and higher plants suggests eukaryote-specific functions. Although the specific mechanisms need further investigation, CEPA1 and Y4IP1 are two novel assembly factors that contribute to PSI formation.
N2  - Die Lichtreaktionen der Photosynthese werden von einer Reihe von Multiproteinkomplexen durchgeführt, die in Thylakoidmembranen eingebettet sind. Hier katalysiert das Photosystem I (PSI), das als Plastocyanin-Ferderoxin-Oxidoreduktase fungiert, die letzte Reaktion. Zusammen mit der lichtsammelnden Antenne I bildet PSI einen hochmolekularen Superkomplex von etwa 600 kDa, der aus achtzehn Untereinheiten und fast zweihundert Co-Faktoren besteht. Der Zusammenbau der verschiedenen Komponenten zu einem funktionsfähigen Thylakoidmembrankomplex erfordert eine präzise Koordination, die durch den Assemblierungsapparat gewährleistet wird. Obwohl dieser eine kleine Anzahl von Proteinen (PSI-Assemblierungsfaktoren) umfasst, die nachweislich eine Rolle bei der Bildung des PSI spielen, ist der Prozess als Ganzes sowie die Komplexität seiner Mitglieder noch weitgehend unerforscht.
In der vorliegenden Arbeit wurden zwei Ansätze verwendet, um Kandidaten für PSI-Assemblierungsfaktoren zu finden. Erstens wurde EnsembleNet verwendet, um Proteine auszuwählen, von denen angenommen wird, dass sie funktionell mit bekannten PSI-Assemblierungsfaktoren in Arabidopsis thaliana verwandt sind (Ansatz I), und zweitens wurde eine Co-Immunopräzipitation (Co-IP) von markierten PSI-Assemblierungsfaktoren in Nicotiana tabacum durchgeführt (Ansatz II).
Dabei wurden die neuartigen PSI-Assemblierungsfaktoren mit der Bezeichnung CO-EXPRESSED WITH PSI ASSEMBLY 1 (CEPA1) und Ycf4-INTERACTING PROTEIN 1 (Y4IP1) identifiziert. A. thaliana Nullmutanten für CEPA1 und Y4IP1 zeigten einen Wachstumsphänotyp und blasse Blätter im Vergleich zum Wildtyp. Biophysikalische Experimente unter Verwendung der Pulsamplitudenmodulation (PAM) zeigten einen unzureichenden Elektronentransport auf der PSII-Akzeptorseite. Biochemische Analysen ergaben, dass sowohl CEPA1 als auch Y4IP1 spezifisch an der PSI-Akkumulation in A. thaliana auf posttranslationaler Ebene beteiligt, jedoch nicht essentiell sind. Entsprechend ihrer Rolle als Faktoren für den Aufbau eines Thylakoidmembran-Proteinkomplexes sind die beiden Proteine an Thylakoidmembranen lokalisiert. Bemerkenswerterweise wiesen cepa1 y4ip1-Doppelmutanten in frühen Entwicklungsstadien unter photoautotrophem Wachstum tödliche Phänotypen auf. Schließlich untermauerten Co-IP- und native Gelexperimente eine mögliche Rolle von CEPA1 und Y4IP1 bei der Vermittlung des PSI-Aufbaus in Verbindung mit anderen PSI-Aufbaufaktoren (z. B. PPD1- und PSA3-CEPA1, und Ycf4-Y4IP1). Die Tatsache, dass CEPA1 und Y4IP1 ausschließlich in Grünalgen und höheren Pflanzen vorkommen, lässt auf eukaryontenspezifische Funktionen schließen. Obwohl die spezifischen Mechanismen noch weiter untersucht werden müssen, sind CEPA1 und Y4IP1 zwei neuartige Assemblierungsfaktoren, die zur PSI-Bildung beitragen.
KW  - photosynthesis
KW  - photosystem I
KW  - biogenesis
KW  - thylakoid membranes
KW  - assembly factor
KW  - Photosynthese
KW  - Photosystem I
KW  - Biogenese
KW  - Thylakoidmembran
KW  - Assemblierungsfaktor
Y1  - 2023
ER  - 
TY  - JOUR
A1  - Gasparatos, Nikolaos
A1  - Scheffler, Christiane
A1  - Hermanussen, Michael
T1  - Assessing the applicability of changepoint analysis to analyse short-term growth
JF  - Human biology and public health
N2  - Background: Assessing short-term growth in humans is still fraught with difficulties. Especially when looking for small variations and increments, such as mini growth spurts, high precision instruments or frequent measurements are necessary. Daily measurements however require a lot of effort, both for anthropologists and for the subjects. Therefore, new sophisticated approaches are needed that reduce fluctuations and reveal underlying patterns.

Objectives: Changepoints are abrupt variations in the properties of time series data. In the context of growth, such variations could be variation in mean height. By adjusting the variance and using different growth models, we assessed the ability of changepoint analysis to analyse short-term growth and detect mini growth spurts.

Sample and Methods: We performed Bayesian changepoint analysis on simulated growth data using the bcp package in R. Simulated growth patterns included stasis, linear growth, catch-up growth, and mini growth spurts. Specificity and a normalised variant of the Matthews correlation coefficient (MCC) were used to assess the algorithm’s performance. Welch’s t-test was used to compare differences of the mean.

Results: First results show that changepoint analysis can detect mini growth spurts. However, the ability to detect mini growth spurts is highly dependent on measurement error. Data preparation, such as ranking and rotating time series data, showed negligible improvements. Missing data was an issue and may affect the prediction quality of the classification metrics.

Conclusion: Changepoint analysis is a promising tool to analyse short-term growth. However, further optimisation and analysis of real growth data is needed to make broader generalisations.
KW  - changepoint analysis
KW  - changepoint detection
KW  - performance evaluation
KW  - mini growth spurt
KW  - short-term growth
Y1  - 2023
U6  - https://doi.org/10.52905/hbph2023.1.62
SN  - 2748-9957
VL  - 1
PB  - Universitätsverlag Potsdam
CY  - Potsdam
ER  - 
TY  - GEN
A1  - Kort, C. A. D. de
A1  - Peter, Martin G.
A1  - Koopmanschap, A. B.
T1  - Binding and degradation of juvenile hormone III by haemolymph proteins of the Colorado potato beetle: a re-examination
N2  - The haemolymph of the adult Colorado potato beetle, Lepinotarsa decemlineata Say, contains a high molecular weight (MW > 200,000) JH-III specific binding protein. The Kd value of the protein for racemic JH-III is 1.3 ± 0.2 × 10−7 M. It has a lower affinity for racemic JH-I and it does not bind JH-III-diol or JH-III-acid. The binding protein does discriminate between the enantiomers of synthetic, racemic JH-III as was determined by stereochemical anaysis of the bound and the free JH-III. Incubation of racemic JH-III with crude haemolymph results in preferential formation of (10S)-JH-III-acid, the unnatural configuration. The JH-esterase present in L. decemlineata haemolymph is not enantioselective. It is concluded that the most important function of the binding protein is that of a specific carrier, protecting the natural hormone against degradation by esterases. The carrier does not protect JH-I as efficiently as the lower homologue.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - paper 068 
KW  - Juvenile hormone
KW  - Leptinotarsa decemlineata
KW  - JH-III-specific carrier protein
KW  - enantioselectivity
Y1  - 1983
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus-16777
ER  - 
TY  - THES
A1  - Unterstab, Gunhild
T1  - Charakterisierung der viralen Genprodukte p10 und P des Borna Disease Virus
T1  - Characterization of the viral gene products p10 and P of the Borna disease virus
N2  - Das Borna Disease Virus (BDV, Bornavirus) besitzt ein einzelsträngiges RNA-Genom negativer Polarität und ist innerhalb der Ordnung Mononegavirales der Prototyp einer eigenen Virusfamilie, die der Bornaviridae. Eine außergewöhnliche Eigenschaft des Virus ist seine nukleäre Transkription und Replikation, eine weitere besteht in seiner Fähigkeit, als neurotropes Virus sowohl in vivo als auch in vitro persistente Infektionen zu etablieren. Die zugrunde liegenden Mechanismen sowohl der Replikation als auch der Persistenz sind derzeit noch unzureichend verstanden, auch deshalb, weil das Virus noch relativ „jung“ ist: Erste komplette Sequenzen des RNA-Genoms wurden 1994 publiziert und erst vor einigen Monaten gelang die Generierung rekombinanter Viren auf der Basis klonierter cDNA. Im Mittelpunkt dieser Arbeit standen das p10 Protein und das Phosphoprotein (P), die von der gemeinsamen Transkriptionseinheit II in überlappenden Leserahmen kodiert werden.  Als im Kern der Wirtszelle replizierendes Virus ist das Bornavirus auf zelluläre Importmechanismen angewiesen, um den Kernimport aller an der Replikation beteiligten viralen Proteine zu gewährleisten. Das p10 Protein ist ein negativer Regulator der viralen RNA-abhängigen RNA-Polymerase (L). In vitro Importexperimente zeigten, dass p10 über den klassischen Importin alpha/beta abhängigen Kernimportweg in den Nukleus transportiert wird. Dies war unerwartet, da p10 kein vorhersagbares klassisches Kernlokalisierungssignal (NLS) besitzt und weist darauf hin, dass der zelluläre Importapparat offensichtlich flexibler ist als allgemein angenommen. Die ersten 20 N-terminalen AS vermitteln sowohl Kernimport als auch die Bindung an den Importrezeptor Importin alpha. Durch Di-Alanin-Austauschmutagenese wurden die für diesen Transportprozess essentiellen AS identifiziert und die Bedeutung hydrophober und polarer AS-Reste demonstriert.  Die Fähigkeit des Bornavirus, persistente Infektionen zu etablieren, wirft die Frage auf, wie das Virus die zellulären antiviralen Abwehrmechanismen, insbesondere das Typ I Interferon (IFN)-System, unterwandert. Das virale P Protein wurde in dieser Arbeit als potenter Antagonist der IFN-Induktion charakterisiert. Es verhindert die Phosphorylierung des zentralen Transkriptionsfaktors IRF3 durch die zelluläre Kinase TBK1 und somit dessen Aktivierung. Der Befund, dass P mit TBK1 Komplexe bildet und zudem auch als Substrat für die zelluläre Kinase fungiert, erlaubt es, erstmalig einen Mechanismus zu postulieren, in dem ein virales Protein (BDV-P) als putatives TBK1-Pseudosubstrat die IRF3-Aktivierung kompetitiv hemmt.
N2  - The Borna Disease Virus (BDV) harbors a single stranded RNA genome of negative polarity. Within the order of Mononegavirales it is the prototype of a new virus family named Bornaviridae. Unique features of this neurotrope virus are its nuclear transcription and replication as well as its ability to establish persistent infections both in vivo and in vitro. The underlying mechanisms of BDV replication and persistence are currently not well understood amongst others due to the fact that BDV is quite a young virus: First complete sequences of the RNA genome have been published in 1994. Only a few months ago the generation of a recombinant Bornavirus from cloned cDNA has been accomplished.  The work presented here focused on the viral p10 protein and the phosphoprotein P that are both encoded by two overlapping reading frames of the transcription unit II.  Nuclear replication of the Bornavirus relies on cellular import mechanisms to allow for nuclear import of viral proteins involved in viral replication. The p10 protein has been described as a negative regulator of the viral RNA dependent RNA polymerase (L). In vitro import experiments revealed that p10 translocates into the nucleus via the classical importin alpha/beta; dependent pathway. This was unexpected since p10 does not contain a predictable classical nuclear localization signal (NLS) suggesting that the cellular import machinery is more flexible than generally believed. The first 20 amino acids mediate nuclear import and binding to the import receptor importin alpha. Analysis of di-alanine-exchange mutants identified essential amino acids and furthermore revealed the impact of hydrophobic and polar side chains in receptor binding and nuclear import.  The ability of the Bornavirus to establish persistent infections rises the question of how the virus circumvents cellular antiviral defense mechanisms, in particular the type I interferon system. This work characterizes the viral P protein as a potent antagonist of IFN beta induction. It prevents the activation of the central transcription factor IRF3 by interfering with the cellular kinase TBK1. The finding that P forms complexes with TBK1 and moreover serves as a kinase substrate allows to postulate a mechanism for the first time, in which a viral protein (BDV-P) acts as a putative TBK1 pseudo-substrate and thereby competitively inhibits IRF3 activation.
KW  - Interferon <beta->
KW  - Borna Disease Virus
KW  - Kernlokalisierungssignal
KW  - Importin
KW  - IRF3
KW  - TBK1
KW  - Borna disease virus
KW  - nuclear localization signal
KW  - importin
KW  - IRF3
KW  - TBK1
Y1  - 2005
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus-6905
ER  - 
TY  - THES
A1  - Oey, Melanie
T1  - Chloroplasts as bioreactors : high-yield production of active bacteriolytic protein antibiotics
T1  - Chloroplasten als Bioreaktoren : hocheffiziente Produktion von aktiven, bakteriolytischen Proteinantibiotika
N2  - Plants, more precisely their chloroplasts with their bacterial-like expression machinery inherited from their cyanobacterial ancestors, can potentially offer a cheap expression system for proteinaceous pharmaceuticals. This system would be easily scalable and provides appropriate safety due to chloroplasts maternal inheritance. In this work, it was shown that three phage lytic enzymes (Pal, Cpl-1 and PlyGBS) could be successfully expressed at very high levels and with high stability in tobacco chloroplasts. PlyGBS expression reached an amount of foreign protein accumulation (> 70% TSP) that has never been obtained before. Although the high expression levels of PlyGBS caused a pale green phenotype with retarded growth, presumably due to exhaustion of plastid protein synthesis capacity, development and seed production were not impaired under greenhouse conditions. Since Pal and Cpl-1 showed toxic effects when expressed in E. coli, a special plastid transformation vector (pTox) was constructed to allow DNA amplification in bacteria. The construction of the pTox transformation vector allowing a recombinase-mediated deletion of an E. coli transcription block in the chloroplast, leading to an increase of foreign protein accumulation to up to 40% of TSP for Pal and 20% of TSP for Cpl-1. High dose-dependent bactericidal efficiency was shown for all three plant-derived lytic enzymes using their pathogenic target bacteria S. pyogenes and S. pneumoniae. Confirmation of specificity was obtained for the endotoxic proteins Pal and Cpl-1 by application to E. coli cultures. These results establish tobacco chloroplasts as a new cost-efficient and convenient production platform for phage lytic enzymes and address the greatest obstacle for clinical application. The present study is the first report of lysin production in a non-bacterial system. The properties of chloroplast-produced lysins described in this work, their stability, high accumulation rate and biological activity make them highly attractive candidates for future antibiotics.
N2  - Lytische Enzyme aus Bakteriophagen bieten Eigenschaften, die sie zu vielversprechenden Medikamenten im Einsatz gegen bakterielle Krankheiten machen. Obwohl sie speziell beim Einsatz gegen bakterielle Infektionen, welche durch Antibiotika resistente Erreger hervorgerufen werden, eine maßgebende Rolle spielen könnten, waren bisher die hohen Produktionskosten ein Hindernis für die medizinische Anwendung. Ein kostengünstiges und einfach zu handhabendes System, wie beispielsweise Chloroplasten in Pflanzen, würde diese lytischen Enzyme zu einer effizienten Alternative zu herkömmlichen Antibiotika machen. In dieser Arbeit wird erstmals die erfolgreiche Produktion von lytischen Enzymen in Tabak-Chloroplasten vorgestellt, welche mit einem Fremdproteingehalt von mehr als 70% des gesamtlöslichen Proteins der Pflanze eine Menge beschreibt, die bisher mit diesem Verfahren noch nicht erreicht wurde. Alle in Chloroplasten hergestellten lytischen Enzyme zeigten hohe spezifische bakteriolytische Aktivität gegen die gewählten Humanpathogene und waren innerhalb von Minuten in der Lage diese Bakterien abzutöten. Zur Herstellung von zwei lytischen Enzymen wurde in dieser Arbeit ein spezieller Shuttle-Vektor entworfen, der die Expression von toxischen Genen innerhalb von E. coli Zellen im Zuge der DNA Replikation vermeidet, jedoch die Herstellung einer ungehinderten Expression der toxischen Gene in den Chloroplasten nach Beseitigung des Selektionsmarkers erlaubte. Ein Vergleich zwischen einem herkömmlich verwendeten Transformationsvektor und dem Shuttle-Vektor mittels eines Reportergens zeigte, dass das neu entwickelte System bis zu 4 mal mehr Protein produzierte. Diese Ergebnisse zeigen das Potential von Chloroplasten als kostengünstige und leicht zu handhabende Produktionsplattform für lytische Enzyme, welche als neue Generation von Antibiotika attraktive Alternativen zu herkömmlichen Therapien bieten.
KW  - Phagenlysine
KW  - Chloroplastentransformation
KW  - Antibiotikaersatz
KW  - Antibiotikaresistenz
KW  - Phage lysins
KW  - Chloroplast transformation
KW  - Antibiotic alternatives
KW  - Antibiotic resistance
Y1  - 2008
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus-28950
ER  - 
TY  - THES
A1  - Hoffmann, Toni
T1  - Cloning and characterisation of the HMA3 gene and its promoter from Arabidopsis halleri (L.) O'Kane and Al'Shehbaz and Arabidopsis thaliana (L.) Heynhold
T1  - Klonierung und Charakterisierung des HMA3 Genes und seines Promotors aus Arabidopsis halleri (L.) O'Kane und Al'Shehbaz und Arabidopsis thaliana (L.) Heynhold
N2  - Being living systems unable to adjust their location to changing environmental conditions, plants display homeostatic networks that have evolved to maintain transition metal levels in a very narrow concentration range in order to avoid either deficiency or toxicity. Hence, plants possess a broad repertoire of mechanisms for the cellular uptake, compartmentation and efflux, as well as for the chelation of transition metal ions. A small number of plants are hypertolerant to one or a few specific transition metals. Some metal tolerant plants are also able to hyperaccumulate metal ions. The Brassicaceae family member Arabidopis halleri ssp. halleri (L.) O´KANE and AL´SHEHBAZ is a hyperaccumulator of zinc (Zn), and it is closely related to the non-hypertolerant and non-hyperaccumulating model plant Arabidopsis thaliana (L.) HEYNHOLD. The close relationship renders A. halleri a promising emerging model plant for the comparative investigation of the molecular mechanisms behind hypertolerance and hyperaccumulation. Among several potential candidate genes that are probably involved in mediating the zinc-hypertolerant and zinc-hyperaccumulating trait is AhHMA3. The AhHMA3 gene is highly similar to AtHMA3 (AGI number: At4g30120) in A. thaliana, and its encoded protein belongs to the P-type IB ATPase family of integral membrane transporter proteins that transport transition metals. In contrast to the low AtHMA3 transcript levels in A. thaliana, the gene was found to be constitutively highly expressed across different Zn treatments in A. halleri, especially in shoots. In this study, the cloning and characterisation of the HMA3 gene and its promoter from Arabidopsis halleri (L.) O´KANE and AL´SHEHBAZ and Arabidopsis thaliana (L.) HEYNHOLD is described. Heterologously expressed AhHMA3 mediated enhanced tolerance to Zn and to a much lesser degree to cadmium (Cd) but not to cobalt (Co) in metal-sensitive mutant strains of budding yeast. It is demonstrated that the genome of A. halleri contains at least four copies of AhHMA3, AhHMA3-1 to AhHMA3-4. A copy-specific real-time RT-PCR indicated that an AhHMA3-1 related gene copy is the source of the constitutively high transcript level in A. halleri and not a gene copy similar to AhHMA3-2 or AhHMA3-4. In accordance with the enhanced AtHMA3mRNA transcript level in A. thaliana roots, an AtHMA3 promoter-GUS gene construct mediated GUS activity predominantly in the vascular tissues of roots and not in shoots. However, the observed AhHMA3-1 and AhHMA3-2 promoter-mediated GUS activity in A. thaliana or A. halleri plants did not reflect the constitutively high expression of AhHMA3 in shoots of A. halleri. It is suggested that other factors e. g. characteristic sequence inserts within the first intron of AhHMA3-1 might enable a constitutively high expression. Moreover, the unknown promoter of the AhHMA3-3 gene copy could be the source of the constitutively high AhHMA3 transcript levels in A. halleri. In that case, the AhHMA3-3 sequence is predicted to be highly homologous to AhHMA3-1. The lack of solid localisation data for the AhHMA3 protein prevents a clear functional assignment. The provided data suggest several possible functions of the AhHMA3 protein: Like AtHMA2 and AtHMA4 it might be localised to the plasma membrane and could contribute to the efficient translocation of Zn from root to shoot and/or to the cell-to-cell distribution of Zn in the shoot. If localised to the vacuolar membrane, then a role in maintaining a low cytoplasmic zinc concentration by vacuolar zinc sequestration is possible. In addition, AhHMA3 might be involved in the delivery of zinc ions to trichomes and mesophyll leaf cells that are major zinc storage sites in A. halleri.
N2  - Pflanzen sind lebende Systeme, die nicht in der Lage sind ihren Standort sich ändernden Umweltbedingungen anzupassen. Infolgedessen weisen Pflanzen homöostatischeNetzwerke auf, welche die Mengen an intrazellulären Übergangsmetallen in einem sehr engen Konzentrationsbereich kontrollieren um somit Vergiftungs- oder Mangelerscheinungen zu vermeiden. Eine kleine Anzahl von Pflanzen ist hypertolerant gegenüber einem oder mehreren Übergangsmetallen. Einige wenige dieser metalltoleranten Pflanzen sind fähig Übergangsmetalle in beträchtlichen Mengen zu speichern, sprich zu hyperakkumulieren, ohne Vergiftungserscheinungen zu zeigen. Die Haller’sche Schaumkresse (Arabidopis halleri ssp. halleri (L.) O´KANE und AL´SHEHBAZ) aus der Familie der Kreuzblütler (Brassicaceae) ist ein solcher Hyperakkumulator für Zink (Zn). Sie ist nah verwandt mit der Modellpflanze Ackerschmalwand (Arabidopsis thaliana (L.) HEYNHOLD), die jedoch nicht-hypertolerant und nicht-hyperakkumulierend für Übergangsmetalle ist. Diese nahe Verwandtschaft erlaubt vergleichende Studien der molekularen Mechanismen, die Hypertoleranz und Hyperakkumulation zu Grunde liegen. Zu der Gruppe von Kandidatengenen, die möglicherweise von Bedeutung für die Zink-hypertoleranten und -hyperakkumulierenden Eigenschaften von A. halleri sind, gehört AhHMA3, ein Gen mit großer Ähnlichkeit zu AtHMA3 (AGI Nummer: At4g30120) aus A. thaliana. Es kodiert ein Protein aus der Familie transmembraner Übergangsmetall-Transportproteine, den P-typ IB ATPasen. Im Gegensatz zu den niedrigen AtHMA3 Transkriptmengen in A. thaliana wird das AhHMA3 Gen in A. halleri in Gegenwart verschiedener Zn Konzentrationen konstitutiv hoch exprimiert, insbesondere im Spross der Pflanze. Diese Arbeit beschreibt die Klonierung und Charakterisierung des HMA3 Gens und seines Promoters aus A. halleri und A. thaliana. Es wurde gezeigt, dass heterolog exprimiertes AhHMA3 Protein in metallsensitiven Hefestämmen eine erhöhte Toleranz gegenüber Zink und zu einem geringen Grad gegenüber Kadmium (Cd) jedoch nicht gegenüber Kobalt (Co) vermittelt.Weiterhin wurden im Genom von A. halleri mindestens vier AhHMA3 Genkopien, AhHMA3-1 bis AhHMA3-4, nachgewiesen. Eine Genkopie-spezifische Echtzeit-RT-PCR (real-time RT-PCR) deutete darauf hin, dass eine zu AhHMA3-1 und nicht zu AhHMA3-2 oder AhHMA3-4 ähnliche Genkopie die Quelle der konstitutiv hohen Transkriptmengen in A. halleri ist. In Übereinstimmung mit erhöhten mRNS Transkriptmengen inWurzeln von A. thaliana, vermittelte ein AtHMA3 Promoter-GUS (ß-Glucuronidase) Genkonstrukt GUS-Aktivität hauptsächlich in den Leitgeweben der Wurzeln jedoch nicht des Sprosses. Die vermittelte GUS-Aktivität durch Promoterfragmente von AhHMA3-1 und AhHMA3-2 in A. thaliana oder A. halleri Pflanzen spiegelte jedoch nicht die konstitutiv hohe AhHMA3 Expression im Spross von A. halleri wieder. Es wird vermutet, dass andere Faktoren die konstitutiv hohe Expression ermöglichen wie zum Beispiel die gefundenen kopiespezifischen Sequenzinsertionen innerhalb des ersten AhHMA3-1 Introns. Weiterhin ist es denkbar, dass der unbekannte Promoter der AhHMA3-3 Genkopie die Quelle der konstitutiv hohen AhHMA3 Transkriptmengen ist. In diesem Fall wird eine sehr hohe Ähnlichkeit zwischen den Sequenzen von AhHMA3-3 und der AhHMA3-1 vorhergesagt. Es konnten keine deutlichen Ergebnisse zur intrazellulären Lokalisierung gemacht werden, die eine exakte Einordnung der Funktion des AhHMA3 Proteins erlauben würden. Die bisher ermittelten Ergebnisse schlagen jedoch mehrere mögliche Funktionen für AhHMA3 vor: Ähnlich den AhHMA3 homologen Proteinen, AtHMA2 und AtHMA4, könnte AhHMA3 in der Plasmamembran der Zelle sitzen und dort zur effizienten Translokation von Zink aus der Wurzel in den Spross und/oder zur Zell-zu-Zell Verteilung von Zn im Spross beitragen. Falls AhHMA3 in der Membran der Vakuole sitzt, könnte es eine Rolle bei der Aufrechterhaltung niedriger zytoplasmatischer Zinkkonzentrationen durch vakuoläre Zinksequestrierung spielen. Zusätzlich ist es denkbar, dass AhHMA3 an der Abgabe von Zinkionen an Trichome und Blattmesophyllzellen beteiligt ist, die die Haupteinlagerungsorte für Zink in A. halleri darstellen.
KW  - P-Typ ATPase
KW  - Übergangsmetalle
KW  - Hyperakkumulation
KW  - Zink
KW  - HMA
KW  - p-type ATPase
KW  - transition metals
KW  - hyperaccumulation
KW  - zinc
KW  - HMA
Y1  - 2007
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus-15259
ER  - 
TY  - JOUR
A1  - Weithoff, Guntram
A1  - Bell, Elanor Margaret
T1  - Complex Trophic Interactions in an Acidophilic Microbial Community
JF  - Microorganisms
N2  - Extreme habitats often harbor specific communities that differ substantially from non-extreme habitats. In many cases, these communities are characterized by archaea, bacteria and protists, whereas the number of species of metazoa and higher plants is relatively low. In extremely acidic habitats, mostly prokaryotes and protists thrive, and only very few metazoa thrive, for example, rotifers. Since many studies have investigated the physiology and ecology of individual species, there is still a gap in research on direct, trophic interactions among extremophiles. To fill this gap, we experimentally studied the trophic interactions between a predatory protist (Actinophrys sol, Heliozoa) and its prey, the rotifers Elosa woralli and Cephalodella sp., the ciliate Urosomoida sp. and the mixotrophic protist Chlamydomonas acidophila (a green phytoflagellate, Chlorophyta). We found substantial predation pressure on all animal prey. High densities of Chlamydomonas acidophila reduced the predation impact on the rotifers by interfering with the feeding behaviour of A. sol. These trophic relations represent a natural case of intraguild predation, with Chlamydomonas acidophila being the common prey and the rotifers/ciliate and A. sol being the intraguild prey and predator, respectively. We further studied this intraguild predation along a resource gradient using Cephalodella sp. as the intraguild prey. The interactions among the three species led to an increase in relative rotifer abundance with increasing resource (Chlamydomonas) densities. By applying a series of laboratory experiments, we revealed the complexity of trophic interactions within a natural extremophilic community.
KW  - acid mine drainage
KW  - extremophiles
KW  - food web
KW  - heliozoa
KW  - intraguild predation
KW  - mining lakes
KW  - Rotifera
Y1  - 2022
U6  - https://doi.org/10.3390/microorganisms10071340
SN  - 2076-2607
VL  - 10
SP  - 1
EP  - 10
PB  - MDPI
CY  - Basel, Schweiz
ET  - 7
ER  - 
TY  - JOUR
A1  - Perscheid, Cindy
T1  - Comprior
BT  - Facilitating the implementation and automated benchmarking of prior knowledge-based feature selection approaches on gene expression data sets
JF  - BMC Bioinformatics
N2  - Background
Reproducible benchmarking is important for assessing the effectiveness of novel feature selection approaches applied on gene expression data, especially for prior knowledge approaches that incorporate biological information from online knowledge bases. However, no full-fledged benchmarking system exists that is extensible, provides built-in feature selection approaches, and a comprehensive result assessment encompassing classification performance, robustness, and biological relevance. Moreover, the particular needs of prior knowledge feature selection approaches, i.e. uniform access to knowledge bases, are not addressed. As a consequence, prior knowledge approaches are not evaluated amongst each other, leaving open questions regarding their effectiveness.

Results
We present the Comprior benchmark tool, which facilitates the rapid development and effortless benchmarking of feature selection approaches, with a special focus on prior knowledge approaches. Comprior is extensible by custom approaches, offers built-in standard feature selection approaches, enables uniform access to multiple knowledge bases, and provides a customizable evaluation infrastructure to compare multiple feature selection approaches regarding their classification performance, robustness, runtime, and biological relevance.

Conclusion
Comprior allows reproducible benchmarking especially of prior knowledge approaches, which facilitates their applicability and for the first time enables a comprehensive assessment of their effectiveness
KW  - Feature selection
KW  - Prior knowledge
KW  - Gene expression
KW  - Reproducible benchmarking
Y1  - 2021
U6  - https://doi.org/10.1186/s12859-021-04308-z
SN  - 1471-2105
VL  - 22
SP  - 1
EP  - 15
PB  - Springer Nature
CY  - London
ER  - 
TY  - JOUR
A1  - Kindermann, Liana
A1  - Dobler, Magnus
A1  - Niedeggen, Daniela
A1  - Chimbioputo Fabiano, Ezequiel
A1  - Linstädter, Anja
T1  - Dataset on woody aboveground biomass, disturbance losses, and wood density from an African savanna ecosystem
JF  - Data in Brief
N2  - This dataset comprises tree inventories and damage assessments performed in Namibia's semi-arid Zambezi Region. Data were sampled in savannas and savanna woodlands along steep gradients of elephant population densities to capture the effects of those (and other) disturbances on individual-level and stand-level aboveground woody biomass (AGB). The dataset contains raw data on dendrometric measures and processed data on specific wood density (SWD), woody aboveground biomass, and biomass losses through disturbance impacts. Allometric proxies (height, canopy diameters, and in adult trees also stem circumferences) were recorded for n = 6,179 tree and shrub individuals. Wood samples were taken for each encountered species to measure specific wood density.

These measurements have been used to estimate woody aboveground biomass via established allometric models, advanced through our improved methodologies and workflows that accounted for tree and shrub architecture shaped by disturbance impacts. To this end, we performed a detailed damage assessment on each woody individual in the field. In addition to estimations of standing biomass, our new method also delivered data on biomass losses to different disturbance agents (elephants, fire, and others) on the level of plant individuals and stands.

The data presented here have been used within a study published with Ecological Indicators (Kindermann et al., 2022) to evaluate the benefits of our improved methodology in comparison to a standard reference method of aboveground biomass estimations. Additionally, it has been employed in a study on carbon storage and sequestration in vegetation and soils (Sandhage-Hofmann et al., 2021).

The raw data of dendrometric measurements can be subjected to other available allometric models for biomass estimation. The processed data can be used to analyze disturbance impacts on woody aboveground biomass, or for regional carbon storage estimates. The data on species-specific wood density can be used for application to other dendrometric datasets to (re-) estimate biomass through allometric models requiring wood density. It can further be used for plant functional trait analyses.
KW  - Damage assessment
KW  - Disturbance impacts
KW  - Disturbance indicator
KW  - Elephant disturbance
KW  - Tree allometry
KW  - Specific wood density
KW  - Woody aboveground biomass
KW  - Wood specific gravity
Y1  - 2022
U6  - https://doi.org/10.1016/j.dib.2022.108155
SN  - 2352-3409
VL  - 42
SP  - 1
EP  - 16
PB  - Elsevier
CY  - Amsterdam, Niederlande
ER  - 
TY  - JOUR
A1  - Boeker, Sonja
A1  - Hermanussen, Michael
A1  - Scheffler, Christiane
T1  - Dental age is an independent marker of biological age
JF  - Human biology and public health
N2  - Background: Biological age markers are a crucial indicator whether children are decelerated in growth tempo. Skeletal maturation is the standard measure. Yet, it relies on exposing children to x-radiation. Dental eruption is a potential, but highly debated, radiation free alternative. 

Objectives: We assess the interrelationship between dental eruption and other maturational markers. We hypothesize that dental age correlates with body height and skeletal age. We further evaluate how the three different variables behave in cohorts from differing social backgrounds.

Sample and Method: Dental, skeletal and height data from the 1970s to 1990s from Guatemalan boys were converted into standard deviation scores, using external references for each measurement. The boys, aged between 7 and 12, derived from different social backgrounds (middle SES (N = 6529), low-middle SES (N = 736), low SES Ladino (N = 3653) and low SES Maya (N = 4587).

Results: Dental age shows only a weak correlation with skeletal age (0.18) and height (0.2). The distinction between cohorts differs according to each of the three measurements. All cohorts differ significantly in height. In skeletal maturation, the middle SES cohort is significantly advanced compared to all other cohorts. The periodically malnourished cohorts of low SES Mayas and Ladinos are significantly delayed in dental maturation compared to the well-nourished low-middle and middle class Ladino children.

Conclusion: Dental development is an independent system, that is regulated by different mechanisms than skeletal development and growth. Tooth eruption is sensitive to nutritional status, whereas skeletal age is more sensitive to socioeconomic background.
KW  - dental eruption
KW  - biological age
KW  - skeletal age
KW  - growth tempo
KW  - maturation
KW  - malnutrition
Y1  - 2022
U6  - https://doi.org/10.52905/hbph2021.3.24
SN  - 2748-9957
VL  - 2021
IS  - 3, Summer School Supplement
PB  - Universitätsverlag Potsdam
CY  - Potsdam
ER  - 
TY  - THES
A1  - Fritz, Christina
T1  - Der Einfluß des primären Stickstoffstoffwechsels auf den Aminosäure- und Sekundärstoffwechsel in Nicotiana tabacum L.
T1  - The impact of primary nitrogen metabolism on amino acid and secondary metabolism in Nicotiana tabacum L.
N2  - Es ist bekannt, dass Änderungen im Kohlenstoff- bzw. Stickstoffstaus der Pflanzen zu einer parallelen statt reziproken Änderung der kohlenstoff- und stickstoffhaltigen Primärmetabolite führen. Unter diesem Gesichtspunkt wurden in der vorliegenden Arbeit der Aminosäurestoffwechsel und der Sekundärstoffwechsel unter reduzierten Stickstoffbedingungen untersucht. Zur Beeinflussung des Stickstoffstoffwechsels wurden nitratmangelernährte Tabakwildtyppflanzen und Genotypen mit unterschiedlich stark reduzierter Nitratreduktase-Aktivität verwendet. Dieses experimentelle System erlaubt zusätzlich durch den Vergleich Nitrat defizienter Wildtyppflanzen mit Nitrat akkumulierenden NIA-Transformanten Prozesse zu identifizieren, die durch Nitrat gesteuert werden. Die Analysen der Primär- und Sekundärmetabolite wurde in allen Genotypen diurnal durchgeführt, um auch tageszeitlich abhängige Prozesse zu identifizieren. Die Analyse der absoluten Gehalte aller individuellen Aminosäuren enthüllte bei den meisten erstaunlich stabile diurnale Muster mit einem Anstieg während des Tages und einem Abfall in der Nacht in Wildtyppflanzen gewachsen mit ausreichend Nitrat. Dieses Ergebnis legt die Schlussfolgerung nahe, dass die Biosynthese der Aminosäuren koordiniert abläuft. In Pflanzen mit reduziertem Stickstoffstatus haben diese diurnalen Muster jedoch keinen Bestand. Die Kombination des erzeugten stickstoffbasierten Aminosäuredatensatz in Kombination mit einem bereits erzeugten Aminosäuredatensatz unter kohlenstofflimitierten Bedingungen von Matt et al. (2002) führte durch Hauptkomponentenanalyse (PCA) und Korrelationsanalyse zu dem Ergebnis, dass die Hypothese nach einer koordinierten Aminosäurebiosynthese nicht allgemeine Gültigkeit hat. Die PCA identifizierte Glutamin, Glutamat, Aspartat, Glycin, Pheny-lalanin und Threonin als Faktoren, die den Datensätzen ihre charakteristische Eigenschaft und deren Varianz verleihen. Die Korrelationsanalyse zeigte, dass die sehr guten Korrelationen der individuellen Aminosäuren untereinander in reduzierten Stickstoff- und Kohlenstoffbedingungen sich verschlechtern. Das Verhältnis einer einzelnen Aminosäure relativ zu den anderen führte zur Identifizierung einiger Aminosäuren, die individuelle Antworten auf Stickstoff- und/oder Kohlenstoffstatus zeigen, und/oder speziell auf Nitrat, Licht und/oder den E-nergiestatus der Thylakoidmembran. Glutamat beispielsweise verhält sich in den meisten Situationen stabil, Phenylalanin dagegen zeigt in jeder physiologischen Situation eine individuelle Antwort. Die Ergebnisse dieser Arbeit führen zu einer Erweiterung der Hypothese einer koordinierten Synthese der Aminosäuren dahingehend, dass diese nicht generell für alle Aminosäuren angenommen werden kann. Es gibt einige Aminosäuren deren, Anteile sich situationsbedingt anpassen. Die Reduktion des Stickstoffstatus in nitratmangelernährten Tabakwildtyppflanzen führte zu der, nach der „Carbon-Nutrient-Balance“ Hypothese erwarteten Verlagerung der kohlenstoffreichen Phenylpropanoide und des stickstoffreichen Nikotins. Die Erhöhung der Phenylpropanoidgehalte war nicht in der Nitrat akkumulierenden NIA-Transformante zu beobachten und somit konnte Nitrat als regulatorisches Element identifiziert werden. Ein Einfluss der Vorläufermetabolite konnte ausgeschlossen werden, da sowohl nitratmangelernährter Wildtyp als auch die Nitrat akkumulierende NIA-Transformante ähnliche Gehalte dieser aufwiesen. Genexpressionsanalysen über Mikroarray-Hybridisierung und quantitative RT-PCR zeigten, dass Nitrat durch noch nicht geklärte Mechanismen Einfluss auf die Expression einiger Gene nimmt, die dem Phenylpropanoidstoffwechsels zugeordnet sind. Aus der Arbeit hervorgegangene Veröffentlichungen: Christina Fritz, Natalia Palacios-Rojas, Regina Feil und Mark Stitt (2006) Regulation of Secondary Metabolism by the Carbon-Nitrogen Status in Tobacco: Nitrate Inhibits Large Sectors of Phenylpropanoid Metabolism. Plant Journal 46, 533 - 548 Christina Fritz, Petra Matt, Cathrin Müller, Regina Feil und Mark Stitt (2006) Impact of the Carbon-Nitrogen Status on the Amino Acid Profile in Tobacco Source Leaves. Plant, Cell and Environment 29 (11), 2009 - 2111
N2  - It is known that changes in carbon and nitrogen status of a plant lead to parallel rather than reciprocal changes of carbon and nitrogen containing primary metabolites. Based on this finding the influence of carbon and nitrogen status on the amino acid profile as well as on secondary metabolism was investigated in tobacco. Manipulations of the nitrogen status were carried out in two ways: Tobacco wild type plants were cultivated in nitrogen-replete and nitrogen starved conditions; in addition nitrate accumulating transformants with reduced nitrate reductase (NIA) activity were used. The comparison of the nitrate starved wild type and the nitrate accumulating NIA-transformant allows to distinguish processes which were driven by the nitrogen status of a plant or by nitrate itself. Due to the fact that most primary metabolites have diurnal changes the analysis of primary and secondary metabolites were done at six different time points per day in order to identify diurnal processes. Analysis of the absolute levels of individual amino acids under normal nitrogen supply conditions reveals characteristic diurnal patterns for the majority of amino acids with an increase during the day and a decrease during the night. This result indicates that amino acid biosynthesis might be coordinated. However these diurnal patterns are no longer stable in plants with reduced nitrogen status; furthermore absolute levels of individual amino acids differed over a wide range of concentrations. The hypothesis of a coordinated regulation of amino acid metabolism was further tested by combining this dataset with an amino acid dataset produced under carbon limited conditions (Matt et al., 2002) and applying Principal Component Analysis (PCA) and correlation analysis. Glutamine, glutamate, aspartate, glycine, phenylalanine and threonine were responsible for the clear separation of the different genotypes and experimental conditions in the PCA plot. The data from the correlation analysis show that most of the minor amino acids have very good correlations under carbon and nitrogen sufficient conditions. These correlations became weaker with decreasing carbon and nitrogen status of the plants. These results clearly indicate that a coordinated biosynthesis of amino acids is not a general phenomenon. Comparing the levels of each individual amino acid to the total amino acid pool revealed specific answers of a particular amino acid to carbon and/or nitrogen status, to nitrate and/or light and to energy status of the thylakoid membrane. Glutamate for instance is remarkably stable in most of the conditions and phenylalanine shows an individual response in every situation. From these results it was concluded that the hypothesis of a coordinated biosynthesis of amino acids might be true for some amino acids, but clearly needs to be extended because some amino acids adjust their levels in an individual fashion depending on the external conditions. The reduction of nitrogen status of nitrate starved wild type plants leads to a shift from carbon-rich phenylpropanoids to nitrogen-rich nicotine as predicted by the “carbon-nutrient-balance hypothesis”. Increased phenylpropanoids were not observed in nitrate accumulating NIA-transformants. Therefore nitrate could be identified as a regulatory element in phenyl-propanoid metabolism. A regulatory influence of precursors could be excluded since nitrate starved wild type and NIA-transformant had similar levels. Genexpression analysis via microarry hybridisation and quantitative RT-PCR shows that nitrate acts a transcriptional regulator of genes involved in phenylpropanoid metabolism. The elucidation of this regulatory role of nitrate requires further investigation.
KW  - Nitrat
KW  - Aminosäuren
KW  - sekundäre Pflanzenstoffe
KW  - Stickstoff
KW  - Tabak
KW  - nitrate
KW  - amino acids
KW  - plant secondary metabolites
KW  - nitrogen
KW  - tobacco
Y1  - 2006
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus-13322
ER  - 
TY  - GEN
A1  - Rancan, Fiorenza
A1  - Volkmann, Hildburg
A1  - Giulbudagian, Michael
A1  - Schumacher, Fabian
A1  - Stanko, Jessica Isolde
A1  - Kleuser, Burkhard
A1  - Blume-Peytavi, Ulrike
A1  - Calderón, Marcelo
A1  - Vogt, Annika
T1  - Dermal Delivery of the High-Molecular-Weight Drug Tacrolimus by Means of Polyglycerol-Based Nanogels
T2  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe
N2  - Polyglycerol-based thermoresponsive nanogels (tNGs) have been shown to have excellent skin hydration properties and to be valuable delivery systems for sustained release of drugs into skin. In this study, we compared the skin penetration of tacrolimus formulated in tNGs with a commercial 0.1% tacrolimus ointment. The penetration of the drug was investigated in ex vivo abdominal and breast skin, while different methods for skin barrier disruption were investigated to improve skin permeability or simulate inflammatory conditions with compromised skin barrier. The amount of penetrated tacrolimus was measured in skin extracts by liquid chromatography tandem-mass spectrometry (LC-MS/MS), whereas the inflammatory markers IL-6 and IL-8 were detected by enzyme-linked immunosorbent assay (ELISA). Higher amounts of tacrolimus penetrated in breast as compared to abdominal skin or in barrier-disrupted as compared to intact skin, confirming that the stratum corneum is the main barrier for tacrolimus skin penetration. The anti-proliferative effect of the penetrated drug was measured in skin tissue/Jurkat cells co-cultures. Interestingly, tNGs exhibited similar anti-proliferative effects as the 0.1% tacrolimus ointment. We conclude that polyglycerol-based nanogels represent an interesting alternative to paraffin-based formulations for the treatment of inflammatory skin conditions.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 1339 
KW  - tacrolimus formulation
KW  - nanogels
KW  - skin penetration
KW  - drug delivery
KW  - human excised skin
KW  - Jurkat cells
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-473270
SN  - 1866-8372
IS  - 1339
ER  - 
TY  - JOUR
A1  - Rancan, Fiorenza
A1  - Volkmann, Hildburg
A1  - Giulbudagian, Michael
A1  - Schumacher, Fabian
A1  - Stanko, Jessica Isolde
A1  - Kleuser, Burkhard
A1  - Blume-Peytavi, Ulrike
A1  - Calderon, Marcelo
A1  - Vogt, Annika
T1  - Dermal Delivery of the High-Molecular-Weight Drug Tacrolimus by Means of Polyglycerol-Based Nanogels
JF  - Pharmaceutics : Molecular Diversity Preservation International
N2  - Polyglycerol-based thermoresponsive nanogels (tNGs) have been shown to have excellent skin hydration properties and to be valuable delivery systems for sustained release of drugs into skin. In this study, we compared the skin penetration of tacrolimus formulated in tNGs with a commercial 0.1% tacrolimus ointment. The penetration of the drug was investigated in ex vivo abdominal and breast skin, while different methods for skin barrier disruption were investigated to improve skin permeability or simulate inflammatory conditions with compromised skin barrier. The amount of penetrated tacrolimus was measured in skin extracts by liquid chromatography tandem-mass spectrometry (LC-MS/MS), whereas the inflammatory markers IL-6 and IL-8 were detected by enzyme-linked immunosorbent assay (ELISA). Higher amounts of tacrolimus penetrated in breast as compared to abdominal skin or in barrier-disrupted as compared to intact skin, confirming that the stratum corneum is the main barrier for tacrolimus skin penetration. The anti-proliferative effect of the penetrated drug was measured in skin tissue/Jurkat cells co-cultures. Interestingly, tNGs exhibited similar anti-proliferative effects as the 0.1% tacrolimus ointment. We conclude that polyglycerol-based nanogels represent an interesting alternative to paraffin-based formulations for the treatment of inflammatory skin conditions.
KW  - tacrolimus formulation
KW  - nanogels
KW  - skin penetration
KW  - drug delivery
KW  - human excised skin
KW  - Jurkat cells
Y1  - 2019
U6  - https://doi.org/10.3390/pharmaceutics11080394
SN  - 1999-4923
VL  - 11
IS  - 8
PB  - MDPI
CY  - Basel
ER  - 
TY  - JOUR
A1  - Sagu Tchewonpi, Sorel
A1  - Huschek, Gerd
A1  - Waldbach Braga, Tess
A1  - Rackiewicz, Michal
A1  - Homann, Thomas
A1  - Rawel, Harshadrai Manilal
T1  - Design of Experiment (DoE) for Optimization of HPLC Conditions for the Simultaneous Fractionation of Seven α-Amylase/Trypsin Inhibitors from Wheat (Triticum aestivum L.)
JF  - Processes : open access journal
N2  - Wheat alpha-amylase/trypsin inhibitors remain a subject of interest considering the latest findings showing their implication in wheat-related non-celiac sensitivity (NCWS). Understanding their functions in such a disorder is still unclear and for further study, the need for pure ATI molecules is one of the limiting problems. In this work, a simplified approach based on the successive fractionation of ATI extracts by reverse phase and ion exchange chromatography was developed. ATIs were first extracted from wheat flour using a combination of Tris buffer and chloroform/methanol methods. The separation of the extracts on a C18 column generated two main fractions of interest F1 and F2. The response surface methodology with the Doehlert design allowed optimizing the operating parameters of the strong anion exchange chromatography. Finally, the seven major wheat ATIs namely P01083, P17314, P16850, P01085, P16851, P16159, and P83207 were recovered with purity levels (according to the targeted LC-MS/MS analysis) of 98.2 ± 0.7; 98.1 ± 0.8; 97.9 ± 0.5; 95.1 ± 0.8; 98.3 ± 0.4; 96.9 ± 0.5, and 96.2 ± 0.4%, respectively. MALDI-TOF-MS analysis revealed single peaks in each of the pure fractions and the mass analysis yielded deviations of 0.4, 1.9, 0.1, 0.2, 0.2, 0.9, and 0.1% between the theoretical and the determined masses of P01083, P17314, P16850, P01085, P16851, P16159, and P83207, respectively. Overall, the study allowed establishing an efficient purification process of the most important wheat ATIs. This paves the way for further in-depth investigation of the ATIs to gain more knowledge related to their involvement in NCWS disease and to allow the absolute quantification in wheat samples.
KW  - wheat
KW  - α-amylase/trypsin inhibitors
KW  - fractionation
KW  - purification
KW  - reversed-phase chromatography
KW  - ion-exchange chromatography
KW  - design of experiment
KW  - LC–MS/MS
KW  - MALDI-TOF-MS
Y1  - 2022
U6  - https://doi.org/10.3390/pr10020259
SN  - 2227-9717
VL  - 10
SP  - 1
EP  - 18
PB  - MDPI
CY  - Basel, Schweiz
ET  - 2
ER  - 
TY  - THES
A1  - Köchert, Karl
T1  - Development of a method to assess EAAT1 transcription levels in Alzheimer's disease
N2  - Zur Zeit leiden ca. 24 Millionen Menschen auf der ganzen Welt unter Demenz, Alzheimer macht dabei 50-60% aller Demenzfälle aus. Da der Anteil der Bevölkerung, der an Demenz leidet, proportional zum Alter zunimmt und der Anteil älterer Menschen in der Gesellschaft von Jahr zu Jahr steigt, wird Alzheimer immer mehr zu einem ernstzunehmenden, gesellschaftlichen Problem. Zum Stand der heutigen Forschung ist es etabliert, dass die Aminosäure Glutamat - quantitativ einer der wichtigsten Neurotransmitter im Zentralen Nervensystem (ZNS) - toxische Konzentrationen erreichen kann wenn sie - im Zuge der Übertragung von Aktionspotentialen - nach ihrer Freisetzung nicht aus dem Synaptischen Spalt entfernt wird. Viele Studien haben gezeigt, dass in der Alzheimerschen Krankheit die Glutamataufnahme beeinträchtigt ist, was zu toxischen Konzentrationen von Glutamat und dem daraus folgenden Absterben von Neuronen führt. Der exitatorische Aminosäuretransporter 1 (EAAT1) gehört zu der Familie der Na+-abhängigen Glutamattransporter und stellt nach EAAT2 den quantitativ wichtigsten Glutamattransporter im ZNS dar. In diesem Projekt wurde eine bis dahin für den Menschen nicht bekannte EAAT1 Spleißvariante, in der Exon 3 ausgeschnitten wird, nachgewiesen. Diese Variante wurde EAAT1Δ3 genannt und stellt damit mit EAAT1Δ9 die zweite für EAAT1 nachgewiesene Spleißvariante dar. Eine auf real-time RT-PCR basierende Methode wurde entwickelt, um die Transkripte von EAAT1 wildtyp (EAAT1 wt), EAAT1Δ3 und EAAT1Δ9 zu quantifizieren. Proben aus verschiedenen Hirnarealen wurden aus einem Set von Kontrollen und Alzheimerfällen bei der Quantifizierung verwendet. Die gewählten Areale sind von der Alzheimerschen Krankheit unterschiedlich stark betroffen. Dies diente als interne Kontrolle für die durchgeführten Experimente und ermöglichte so die Differenzierung zwischen beobachteten Effekten: Nur Effekte die alleinig in von Alzheimer betroffenen Gehirnarealen auftreten, können als spezifisch für die Krankheit angesehen werden. Die Resultate diese Projektes zeigen, dass EAAT1Δ3 in sehr geringer Anzahl transkribiert wird, die nur 0.15% der EAAT1 wt Transkription entspricht. Dahingegen entspricht das EAAT1 Δ9 Transkript im Durchschnitt 26.6% des EAAT1 wt Transkripts. Es wurde nachgewiesen, dass die Transkriptionsrate aller EAAT1 Varianten in Alzheimerfällen signifikant reduziert ist (P<0.0001). Dies unterstützt die Theorie, dass bei Alzheimerfällen die EAAT1 Proteinexpression stark reduziert und der Glutamattransport, der normalerweise durch diesen Transporter gewährleistet wird, stark eingeschränkt ist. Dies wiederum resultiert in toxisch hohen Glutamatkonzentrationen und damit dem Absterben von Neuronen. Die gefundene Reduktion der EAAT1Transkription ist nicht spezifisch für Gehirnareale die von Alzheimer betroffen sind, sondern tritt in selbem Maße in nicht von Alzheimer betroffenen Gehirnarealen auf. Daraus lässt sich schließen, dass die Reduktion der EAAT1 Transkription eher ein Resultat eines in der Alzheimerschen Krankheit präsenten, grundlegenden Krankheitsmechanismus ist als deren Ursache.
N2  - Today about 24 Million people worldwide suffer from dementia, Alzheimer’s Disease accounts for approximately 50-60% of all dementia cases. As the prevalence of dementia grows with increasing age Alzheimer’s Disease becomes more and more of an issue for society as the proportion of elderly people increases from year to year. It is well established, that the amino acid glutamate - quantitatively being the most important neurotransmitter in the central nervous system (CNS) - may reach toxic concentrations if not cleared from the synaptic cleft into which it is released during transmittance of action potentials. In Alzheimer’s Disease there is strong evidence for a generally impaired glutamate uptake system which in turn is thought to result in toxic levels of the amino acid with the potential to kill off neurons. The excitatory amino acid transporter 1 (EAAT1) belongs to the family of Na+-dependent glutamate transporter and accounts together with EAAT2 for most of the glutamate uptake in the CNS. In this project a new splice variant of EAAT1, skipping exon 3 was detected in human brain samples and subsequently called EAAT1Δ3, this being the second splice variant found after the recent detection of EAAT1Δ9. A method was developed to quantify the transcript of EAAT1 wt, EAAT1Δ3 and EAAT1Δ9 by means of real-time PCR. Samples were taken from different brain areas of a set of control and AD cases. The areas chosen for examination are affected differently in Alzheimer’s Disease, this was used an internal control for the experiments done in this project as to determine whether any effect observed is specific for AD, i.e. AD affected areas or is generally seen in all areas examined. The results of this project show that EAAT1Δ3 is transcribed in very low copy numbers making up a proportion of 0.15% of EAAT1 wt whereas EAAT1Δ9 is transcribed in a considerably large proportion of EAAT1 wt of 26.6%. It was moreover found that all EAAT1 variants are transcribed at significantly lower rates (P<0.0001) in AD cases, supporting the theory that EAAT1 protein expression is reduced to a point where glutamate uptake normally mediated by this transporter is impaired. This in turn is thought to result in toxic levels glutamate accounting for neuronal loss in the disease. No area-dependent effects were found, suggesting that the reduction of EAAT1 transcription is rather a result of an underlying general mechanism present in AD. Further research will have to be done to assess the degree of EAAT1 expression in AD and whether those future findings match with the result of this project.
KW  - Morbus Alzheimer
KW  - Glutamat
KW  - EAAT1
KW  - Spleißvariante
KW  - Alzheimer's Disease
KW  - Glutamate
KW  - EAAT1
KW  - Splice Variant
Y1  - 2007
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus-15965
ER  - 
TY  - THES
A1  - Frenzel, Sabine
T1  - Die Rolle der Umamirezeptoruntereinheit Tas1r1 jenseits ihrer gustatorischen Bedeutung
T1  - The role of the umami receptor subunit Tas1r1 beyond its gustatory importance
BT  - Analyse ihrer Expression und Funktion in nichtgustatorischen Geweben gentechnisch modifizierter Mauslinien
N2  - Aminosäuren sind lebensnotwendige Moleküle für alle Organismen. Ihre Erkennung im Körper ermöglicht eine bedarfsgerechte Regulation ihrer Aufnahme und ihrer Verwertung. Welcher Chemosensor für diese Erkennung jedoch hauptverantwortlich ist, ist bisher unklar. In der vorliegenden Arbeit wurde die Rolle der Umamigeschmacksrezeptoruntereinheit Tas1r1 jenseits ihrer gustatorischen Bedeutung für die Aminosäuredetektion in der Mundhöhle untersucht.
In der histologischen Tas1r1-Expressionsanalyse nichtgustatorischer Gewebe der Mauslinie Tas1r1-Cre/ROSA26-tdRFP wurde über die Detektion des Reporterproteins tdRFP die Expression des Tas1r1 in allen untersuchten Geweben (Speiseröhre, Magen, Darm, Bauchspeicheldrüse, Leber, Niere, Muskel- und Fettgewebe, Milz, Thymus, Lymphknoten, Lunge sowie Hoden) nachgewiesen. Mit Ausnahme von Dünndarm und Hoden gelang hierbei der Nachweis erstmals spezifisch auf zellulärer Ebene. Caecum und Lymphknoten wurden zudem neu als Expressionsorte des Tas1r1 identifiziert.
Trotz der beobachteten weiten Verbreitung des Tas1r1 im Organismus – unter anderem auch in Geweben, die für den Proteinstoffwechsel besonders relevant sind – waren im Zuge der durchgeführten Untersuchung potentieller extraoraler Funktionen des Rezeptors durch phänotypische Charakterisierung der Mauslinie Tas1r1-BLiR nur schwache Auswirkungen auf Aminosäurestoffwechsel bzw. Stickstoffhaushalt im Falle eines Tas1r1-Knockouts detektierbar. Während sich Ernährungsverhalten, Gesamtphysiologie, Gewebemorphologie sowie Futterverdaulichkeit unverändert zeigten, war die renale Stickstoffausscheidung bei Tas1r1-Knockout-Mäusen auf eiweißarmer sowie auf eiweißreicher Diät signifikant verringert. Eine Überdeckung der Auswirkungen des Tas1r1-Knockouts aufgrund kompensatorischer Effekte durch den Aminosäuresensor CaSR oder den Peptidsensor Gpr93 war nicht nachweisbar. Es bleibt offen, ob andere Mechanismen oder andere Chemosensoren an einer Kompensation beteiligt sind oder aber Tas1r1 in extraoralem Gewebe andere Funktionen als die der Aminosäuredetektion übernimmt. Unterschiede im extraoralen Expressionsmuster der beiden Umamirezeptor-untereinheiten Tas1r1 und Tasr3 lassen Spekulationen über andere Partner, Liganden und Funktionen zu.
N2  - Amino acids are important nutrients for each organism. Recognition of amino acids in the body enables an adequate regulation of their absorption and use. Until now, it is ambiguous which chemosensor is mainly responsible for this recognition. In the present work, the role of the umami taste receptor subunit Tas1r1 was examined beyond its gustatory importance for the amino acid detection in the oral cavity.
By a histological expression analysis of non-gustatory tissues of the mouse strain Tas1r1-Cre/ROSA26-tdRFP, Tas1r1 expression has been proven in all of the analysed tissues (oesophagus, stomach, intestine, pancreas, liver, kidney, muscle and fat tissues, spleen, thymus, lymph nodes, lung and testes) via the detection of the reporter protein tdRFP. With the exception of small intestine and testes, the proof succeeded for the first time specifically at the cellular level. Moreover, caecum and lymph nodes were newly identified as expression sites of Tas1r1.
Despite the observed widespread distribution of Tas1r1 in the organism – including tissues which are particularly relevant in protein metabolism – only slight effects on amino acid metabolism and nitrogen balance respectively were detectable in the course of examinations of potentially extraoral functions of the receptor by a phenotypical characterization of the mouse strain Tas1r1-BLiR. The renal nitrogen excretion of Tas1r1 knockout mice on low protein and also high protein diet was significantly reduced, whereas dietary habit, overall physiology, tissue morphology and food digestibility remained unchanged. A superposition of the Tas1r1 knockout impact due to compensatory effects by the amino acid sensor CaSR or the peptide sensor Gpr93 was unverifiable. It remains open whether other mechanisms or chemosensors are involved in compensation or whether Tas1r1 takes over other functions in extraoral tissues than the amino acid detection. Differences in the extraoral expression pattern of the two umami receptor subunits Tas1r1 and Tas1r3 leave room for speculations about other partners, ligands and functions.
KW  - Tas1r1
KW  - Geschmacksrezeptor
KW  - taste receptor
KW  - umami
KW  - umami
KW  - Tas1r1
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-79502
ER  -