TY  - JOUR
A1  - Moreno-Romero, Jordi
A1  - Probst, Aline V.
A1  - Trindade, Inês
A1  - Kalyanikrishna, 
A1  - Engelhorn, Julia
A1  - Farrona, Sara
T1  - Looking At the Past and Heading to the Future
BT  - Meeting Summary of the 6th European Workshop on Plant Chromatin 2019 in Cologne, Germany
JF  - Frontiers in Plant Science
N2  - In June 2019, more than a hundred plant researchers met in Cologne, Germany, for the 6th European Workshop on Plant Chromatin (EWPC). This conference brought together a highly dynamic community of researchers with the common aim to understand how chromatin organization controls gene expression, development, and plant responses to the environment. New evidence showing how epigenetic states are set, perpetuated, and inherited were presented, and novel data related to the three-dimensional organization of chromatin within the nucleus were discussed. At the level of the nucleosome, its composition by different histone variants and their specialized histone deposition complexes were addressed as well as the mechanisms involved in histone post-translational modifications and their role in gene expression. The keynote lecture on plant DNA methylation by Julie Law (SALK Institute) and the tribute session to Lars Hennig, honoring the memory of one of the founders of the EWPC who contributed to promote the plant chromatin and epigenetic field in Europe, added a very special note to this gathering. In this perspective article we summarize some of the most outstanding data and advances on plant chromatin research presented at this workshop.
KW  - EWPC2019
KW  - chromatin
KW  - epigenetics
KW  - transcription
KW  - nucleus
Y1  - 2020
U6  - https://doi.org/10.3389/fpls.2019.01795
SN  - 1664-462X
VL  - 10
IS  - 1795
SP  - 1
EP  - 12
PB  - Frontiers Media
CY  - Lausanne
ER  - 
TY  - GEN
A1  - Moreno-Romero, Jordi
A1  - Probst, Aline V.
A1  - Trindade, Inês
A1  - Kalyanikrishna, 
A1  - Engelhorn, Julia
A1  - Farrona, Sara
T1  - Looking At the Past and Heading to the Future
BT  - Meeting Summary of the 6th European Workshop on Plant Chromatin 2019 in Cologne, Germany
T2  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe
N2  - In June 2019, more than a hundred plant researchers met in Cologne, Germany, for the 6th European Workshop on Plant Chromatin (EWPC). This conference brought together a highly dynamic community of researchers with the common aim to understand how chromatin organization controls gene expression, development, and plant responses to the environment. New evidence showing how epigenetic states are set, perpetuated, and inherited were presented, and novel data related to the three-dimensional organization of chromatin within the nucleus were discussed. At the level of the nucleosome, its composition by different histone variants and their specialized histone deposition complexes were addressed as well as the mechanisms involved in histone post-translational modifications and their role in gene expression. The keynote lecture on plant DNA methylation by Julie Law (SALK Institute) and the tribute session to Lars Hennig, honoring the memory of one of the founders of the EWPC who contributed to promote the plant chromatin and epigenetic field in Europe, added a very special note to this gathering. In this perspective article we summarize some of the most outstanding data and advances on plant chromatin research presented at this workshop.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 1423 
KW  - EWPC2019
KW  - chromatin
KW  - epigenetics
KW  - transcription
KW  - nucleus
Y1  - 2020
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-511942
SN  - 1866-8372
ER  - 
TY  - THES
A1  - Putzler, Sascha
T1  - Molekulare Charakterisierung des Centrosom-assoziierten Proteins CP91 in Dictyostelium discoideum
T1  - Molecular characterization of the centrosome-associated protein CP91 in Dictyostelium discoideum
N2  - Das Dictyostelium-Centrosom ist ein Modell für acentrioläre Centrosomen. Es besteht aus einer dreischichtigen Kernstruktur und ist von einer Corona umgeben, welche Nukleationskomplexe für Mikrotubuli beinhaltet. Die Verdoppelung der Kernstruktur wird einmal pro Zellzyklus am Übergang der G2 zur M-Phase gestartet. Durch eine Proteomanalyse isolierter Centrosomen konnte CP91 identifiziert werden, ein 91 kDa großes Coiled-Coil Protein, das in der centrosomalen Kernstruktur lokalisiert. GFP-CP91 zeigte fast keine Mobilität in FRAP-Experimenten während der Interphase, was darauf hindeutet, dass es sich bei CP91 um eine Strukturkomponente des Centrosoms handelt. In der Mitose hingegen dissoziieren das GFP-CP91 als auch das endogene CP91 ab und fehlen an den Spindelpolen von der späten Prophase bis zur Anaphase. Dieses Verhalten korreliert mit dem Verschwinden der zentralen Schicht der Kernstruktur zu Beginn der Centrosomenverdopplung. Somit ist CP91 mit großer Wahrscheinlichkeit ein Bestandteil dieser Schicht. CP91-Fragmente der N-terminalen bzw. C-terminalen Domäne (GFP-CP91 N-Terminus, GFP-CP91 C-Terminus) lokalisieren als GFP-Fusionsproteine exprimiert auch am Centrosom, zeigen aber nicht die gleiche mitotische Verteilung des Volllängenproteins. Das CP91-Fragment der zentralen Coiled-Coil Domäne (GFP-CP91cc) lokalisiert als GFP-Fusionsprotein exprimiert, als ein diffuser cytosolische Cluster, in der Nähe des Centrosoms. Es zeigt eine partiell ähnliche mitotische Verteilung wie das Volllängenprotein. Dies lässt eine regulatorische Domäne innerhalb der Coiled-Coil Domäne vermuten. Die Expression der GFP-Fusionsproteine unterdrückt die Expression des endogenen CP91 und bringt überzählige Centrosomen hervor. Dies war auch eine markante Eigenschaft nach der Unterexpression von CP91 durch RNAi. Zusätzlich zeigte sich in CP91-RNAi Zellen eine stark erhöhte Ploidie verursacht durch schwere Defekte in der Chromosomensegregation verbunden mit einer erhöhten Zellgröße und Defekten im Abschnürungsprozess während der Cytokinese. Die Unterexpression von CP91 durch RNAi hatte auch einen direkten Einfluss auf die Menge an den centrosomalen Proteinen CP39, CP55 und CEP192 und dem Centromerprotein Cenp68 in der Interphase. Die Ergebnisse deuten darauf hin, dass CP91 eine zentrale centrosomale Kernkomponente ist und für den Zusammenhalt der beiden äußeren Schichten der Kernstruktur benötigt wird. Zudem spielt CP91 eine wichtige Rolle für eine ordnungsgemäße Centrosomenbiogenese und, unabhängig davon, bei dem Abschnürungsprozess der Tochterzellen während der Cytokinese.
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 N-terminal and C-terminal domain (GFP-CP91N, and GFP-CP91C respectively) also localized to the centrosome but did not show the mitotic redistribution of the full length protein. The CP91 fragment corresponding to the central coiled coil domain (GFP-CP91cc) localized as a diffuse cluster close to the centrosome and did show a partially similar mitotic redistribution of the full length protein suggesting a regulatory role of the coiled coil 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. 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. Additionally, depletion of CP91 by RNAi had an immediate impact on the amount of the centrosomal core components CP39, CP55 and CEP192 and the centromere protein Cenp68 in interphase cells. Our results indicate that CP91 is a central centrosomal core component required for centrosomal integrity, proper centrosome biogenesis and, independently, for abscission during cytokinesis.
KW  - Centrosom
KW  - Dictyostelium
KW  - Mikrotubuli
KW  - Mitose
KW  - Zellkern
KW  - centrosome
KW  - dictyostelium
KW  - microtubules
KW  - mitosis
KW  - nucleus
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-394689
ER  - 
TY  - JOUR
A1  - Winck, Flavia Vischi
A1  - Kwasniewski, Miroslaw
A1  - Wienkoop, Stefanie
A1  - Müller-Röber, Bernd
T1  - An optimized method for the isolation of nuclei from chlamydomas Reinhardtii (Chlorophyceae)
JF  - Journal of phycology
N2  - The cell nucleus harbors a large number of proteins involved in transcription, RNA processing, chromatin remodeling, nuclear signaling, and ribosome assembly. The nuclear genome of the model alga Chlamydomonas reinhardtii P. A. Dang. was recently sequenced, and many genes encoding nuclear proteins, including transcription factors and transcription regulators, have been identified through computational discovery tools. However, elucidating the specific biological roles of nuclear proteins will require support from biochemical and proteomics data. Cellular preparations with enriched nuclei are important to assist in such analyses. Here, we describe a simple protocol for the isolation of nuclei from Chlamydomonas, based on a commercially available kit. The modifications done in the original protocol mainly include alterations of the differential centrifugation parameters and detergent-based cell lysis. The nuclei-enriched fractions obtained with the optimized protocol show low contamination with mitochondrial and plastid proteins. The protocol can be concluded within only 3 h, and the proteins extracted can be used for gel-based and non-gel-based proteomic approaches.
KW  - 2D gel electrophoresis
KW  - algae
KW  - Chlamydomonas
KW  - nuclear proteins
KW  - nucleus
KW  - proteomics
Y1  - 2011
U6  - https://doi.org/10.1111/j.1529-8817.2011.00967.x
SN  - 0022-3646
VL  - 47
IS  - 2
SP  - 333
EP  - 340
PB  - Wiley-Blackwell
CY  - Malden
ER  - 
TY  - JOUR
A1  - Batsios, Petros
A1  - Peter, Tatjana
A1  - Baumann, Otto
A1  - Stick, Reimer
A1  - Meyer, Irene
A1  - Gräf, Ralph
T1  - A lamin in lower eukaryotes?
JF  - Nucleus
N2  - Lamins are the major components of the nuclear lamina and serve not only as a mechanical support, but are also involved in chromatin organization, epigenetic regulation, transcription and mitotic events. Despite these universal tasks, lamins have so far been found only in metazoans. Yet, recently we have identified Dictyostelium NE81 as the first lamin-like protein in a lower eukaryote. Based on the current knowledge, we draw a model for nuclear envelope organization in Dictyostelium in this Extra View and we review the experimental data that justified this classification. Furthermore we provide unpublished data underscoring the requirement of posttranslational CaaX-box processing for proper protein localization at the nuclear envelope. Sequence comparison of NE81 sequences from four Dictyostelia with bona fide lamins illustrates the evolutional relationship between these proteins. Under certain conditions these usually unicellular social amoebae congregate to form a multicellular body. We propose that the evolution of the lamin-like NE81 went along with the invention of multicellularity.
KW  - dictyostelium
KW  - lamin
KW  - intermediate filament
KW  - centrosome
KW  - nucleus
Y1  - 2012
U6  - https://doi.org/10.4161/nucl.20149
SN  - 1949-1034
VL  - 3
IS  - 3
SP  - 237
EP  - 243
PB  - Landes Bioscience
CY  - Austin
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  -