Beißel, Christian

[["dc.bibliographiccitation.firstpage","499"],["dc.bibliographiccitation.issue","3"],["dc.bibliographiccitation.journal","Molecular Microbiology"],["dc.bibliographiccitation.lastpage","519"],["dc.bibliographiccitation.volume","104"],["dc.contributor.author","Ariyachet, Chaiyaboot"],["dc.contributor.author","Beissel, Christian"],["dc.contributor.author","Li, Xiang"],["dc.contributor.author","Lorrey, Selena"],["dc.contributor.author","Mackenzie, Olivia"],["dc.contributor.author","Martin, Patrick M."],["dc.contributor.author","O'Brien, Katharine"],["dc.contributor.author","Pholcharee, Tossapol"],["dc.contributor.author","Sim, Sue"],["dc.contributor.author","Krebber, Heike"],["dc.contributor.author","McBride, Anne E."],["dc.date.accessioned","2018-11-07T10:24:44Z"],["dc.date.available","2018-11-07T10:24:44Z"],["dc.date.issued","2017"],["dc.description.abstract","The morphological transition of the opportunistic fungal pathogen Candida albicans from budding to hyphal growth has been implicated in its ability to cause disease in animal models. Absence of styled-content NA-binding protein Slr1 slows hyphal formation and decreases virulence in a systemic candidiasis model, suggesting a role for post-transcriptional regulation in these processes. SR (serine-arginine)-rich proteins influence multiple steps in mRNA metabolism and their localization and function are frequently controlled by modification. We now demonstrate that Slr1 binds to polyadenylated RNA and that its intracellular localization is modulated by phosphorylation and methylation. Wildtype Slr1-GFP is predominantly nuclear, but also co-fractionates with translating ribosomes. The non-phosphorylatable slr1-6SA-GFP protein, in which six serines in SR/RS clusters are substituted with alanines, primarily localizes to the cytoplasm in budding cells. Intriguingly, hyphal cells display a slr1-6SA-GFP focus at the tip near the Spitzenkorper, a vesicular structure involved in molecular trafficking to the tip. The presence of slr1-6SA-GFP hyphal tip foci is reduced in the absence of the mRNA-transport protein She3, suggesting that unphosphorylated Slr1 associates with mRNA-protein complexes transported to the tip. The impact of SLR1 deletion on hyphal formation and function thus may be partially due to a role in hyphal mRNA transport."],["dc.identifier.doi","10.1111/mmi.13643"],["dc.identifier.isi","000399665400010"],["dc.identifier.pmid","28187496"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/42714"],["dc.notes.status","zu prüfen"],["dc.notes.submitter","PUB_WoS_Import"],["dc.publisher","Wiley"],["dc.relation.issn","1365-2958"],["dc.relation.issn","0950-382X"],["dc.title","Post-translational modification directs nuclear and hyphal tip localization of Candida albicans mRNA-binding protein Slr1"],["dc.type","journal_article"],["dc.type.internalPublication","yes"],["dc.type.peerReviewed","yes"],["dc.type.status","published"],["dspace.entity.type","Publication"]]

[["dc.bibliographiccitation.artnumber","4"],["dc.bibliographiccitation.issue","14"],["dc.bibliographiccitation.journal","Journal of Vision"],["dc.bibliographiccitation.volume","15"],["dc.contributor.author","Orlowski, Julius"],["dc.contributor.author","Beissel, Christian"],["dc.contributor.author","Rohn, Friederike"],["dc.contributor.author","Adato, Yair"],["dc.contributor.author","Wagner, Hermann"],["dc.contributor.author","Ben-Shahar, Ohad"],["dc.date.accessioned","2019-07-25T10:39:47Z"],["dc.date.available","2019-07-25T10:39:47Z"],["dc.date.issued","2015"],["dc.description.abstract","Visual pop-out is a phenomenon by which the latency to detect a target in a scene is independent of the number of other elements, the distractors. Pop-out is an effective visual-search guidance that occurs typically when the target is distinct in one feature from the distractors, thus facilitating fast detection of predators or prey. However, apart from studies on primates, pop-out has been examined in few species and demonstrated thus far in rats, archer fish, and pigeons only. To fill this gap, here we study pop-out in barn owls. These birds are a unique model system for such exploration because their lack of eye movements dictates visual behavior dominated by head movements. Head saccades and interspersed fixation periods can therefore be tracked and analyzed with a head-mounted wireless microcamera--the OwlCam. Using this methodology we confronted two owls with scenes containing search arrays of one target among varying numbers (15-63) of similar looking distractors. We tested targets distinct either by orientation (Experiment 1) or luminance contrast (Experiment 2). Search time and the number of saccades until the target was fixated remained largely independent of the number of distractors in both experiments. This suggests that barn owls can exhibit pop-out during visual search, thus expanding the group of species and brain structures that can cope with this fundamental visual behavior. The utility of our automatic analysis method is further discussed for other species and scientific questions."],["dc.identifier.doi","10.1167/15.14.4"],["dc.identifier.pmid","26448146"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/62051"],["dc.language.iso","en"],["dc.relation.eissn","1534-7362"],["dc.relation.issn","1534-7362"],["dc.title","Visual pop-out in barn owls: Human-like behavior in the avian brain"],["dc.type","journal_article"],["dc.type.internalPublication","no"],["dspace.entity.type","Publication"]]

[["dc.bibliographiccitation.firstpage","263"],["dc.bibliographiccitation.issue","2"],["dc.bibliographiccitation.journal","Glia"],["dc.bibliographiccitation.lastpage","276"],["dc.bibliographiccitation.volume","67"],["dc.contributor.author","Fischbach, Felix"],["dc.contributor.author","Nedelcu, Julia"],["dc.contributor.author","Leopold, Patrizia"],["dc.contributor.author","Zhan, Jiangshan"],["dc.contributor.author","Clarner, Tim"],["dc.contributor.author","Nellessen, Lara"],["dc.contributor.author","Beißel, Christian"],["dc.contributor.author","van Heuvel, Yasemin"],["dc.contributor.author","Goswami, Anand"],["dc.contributor.author","Weis, Joachim"],["dc.contributor.author","Denecke, Bernd"],["dc.contributor.author","Schmitz, Christopher"],["dc.contributor.author","Hochstrasser, Tanja"],["dc.contributor.author","Nyamoya, Stella"],["dc.contributor.author","Victor, Marion"],["dc.contributor.author","Beyer, Cordian"],["dc.contributor.author","Kipp, Markus"],["dc.date.accessioned","2019-07-25T10:37:37Z"],["dc.date.available","2019-07-25T10:37:37Z"],["dc.date.issued","2019"],["dc.description.abstract","Oligodendrocytes are integral to efficient neuronal signaling. Loss of myelinating oligodendrocytes is a central feature of many neurological diseases, including multiple sclerosis (MS). The results of neuropathological studies suggest that oligodendrocytes react with differing sensitivity to toxic insults, with some cells dying early during lesion development and some cells being resistant for weeks. This proposed graded vulnerability has never been demonstrated but provides an attractive window for therapeutic interventions. Furthermore, the biochemical pathways associated with graded oligodendrocyte vulnerability have not been well explored. We used immunohistochemistry and serial block-face scanning electron microscopy (3D-SEM) to show that cuprizone-induced metabolic stress results in an \"out of phase\" degeneration of oligodendrocytes. Although expression induction of stress response transcription factors in oligodendrocytes occurs within days, subsequent oligodendrocyte apoptosis continues for weeks. In line with the idea of an out of phase degeneration of oligodendrocytes, detailed ultrastructural reconstructions of the axon-myelin unit demonstrate demyelination of single internodes. In parallel, genome wide array analyses revealed an active unfolded protein response early after initiation of the cuprizone intoxication. In addition to the cytoprotective pathways, the pro-apoptotic transcription factor DNA damage-inducible transcript 3 (DDIT3) was induced early in oligodendrocytes. In advanced lesions, DDIT3 was as well expressed by activated astrocytes. Toxin-induced oligodendrocyte apoptosis, demyelination, microgliosis, astrocytosis, and acute axonal damage were less intense in the Ddit3-null mutants. This study identifies DDIT3 as an important regulator of graded oligodendrocyte vulnerability in a MS animal model. Interference with this stress cascade might offer a promising therapeutic approach for demyelinating disorders."],["dc.identifier.doi","10.1002/glia.23538"],["dc.identifier.pmid","30511355"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/62050"],["dc.language.iso","en"],["dc.relation.eissn","1098-1136"],["dc.relation.issn","0894-1491"],["dc.title","Cuprizone-induced graded oligodendrocyte vulnerability is regulated by the transcription factor DNA damage-inducible transcript 3"],["dc.type","journal_article"],["dc.type.internalPublication","no"],["dspace.entity.type","Publication"]]

[["dc.bibliographiccitation.firstpage","1085"],["dc.bibliographiccitation.issue","3"],["dc.bibliographiccitation.journal","International Journal of Molecular Sciences"],["dc.bibliographiccitation.volume","21"],["dc.contributor.author","Beißel, Christian"],["dc.contributor.author","Grosse, Sebastian"],["dc.contributor.author","Krebber, Heike"],["dc.date.accessioned","2020-12-10T18:47:10Z"],["dc.date.available","2020-12-10T18:47:10Z"],["dc.date.issued","2020"],["dc.identifier.doi","10.3390/ijms21031085"],["dc.identifier.eissn","1422-0067"],["dc.identifier.purl","https://resolver.sub.uni-goettingen.de/purl?gs-1/17332"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/78666"],["dc.language.iso","en"],["dc.notes.intern","DOI Import GROB-354"],["dc.notes.intern","Merged from goescholar"],["dc.rights","Goescholar"],["dc.rights.uri","https://goescholar.uni-goettingen.de/licenses"],["dc.title","Dbp5/DDX19 between Translational Readthrough and Nonsense Mediated Decay"],["dc.type","journal_article"],["dc.type.internalPublication","yes"],["dc.type.version","published_version"],["dspace.entity.type","Publication"]]

[["dc.bibliographiccitation.firstpage","4798"],["dc.bibliographiccitation.issue","9"],["dc.bibliographiccitation.journal","Nucleic Acids Research"],["dc.bibliographiccitation.lastpage","4813"],["dc.bibliographiccitation.volume","47"],["dc.contributor.author","Beissel, Christian"],["dc.contributor.author","Neumann, Bettina"],["dc.contributor.author","Uhse, Simon"],["dc.contributor.author","Hampe, Irene"],["dc.contributor.author","Karki, Prajwal"],["dc.contributor.author","Krebber, Heike"],["dc.date.accessioned","2019-07-25T10:31:21Z"],["dc.date.available","2019-07-25T10:31:21Z"],["dc.date.issued","2019"],["dc.description.abstract","Translation termination requires eRF1 and eRF3 for polypeptide- and tRNA-release on stop codons. Additionally, Dbp5/DDX19 and Rli1/ABCE1 are required; however, their function in this process is currently unknown. Using a combination of in vivo and in vitro experiments, we show that they regulate a stepwise assembly of the termination complex. Rli1 and eRF3-GDP associate with the ribosome first. Subsequently, Dbp5-ATP delivers eRF1 to the stop codon and in this way prevents a premature access of eRF3. Dbp5 dissociates upon placing eRF1 through ATP-hydrolysis. This in turn enables eRF1 to contact eRF3, as the binding of Dbp5 and eRF3 to eRF1 is mutually exclusive. Defects in the Dbp5-guided eRF1 delivery lead to premature contact and premature dissociation of eRF1 and eRF3 from the ribosome and to subsequent stop codon readthrough. Thus, the stepwise Dbp5-controlled termination complex assembly is essential for regular translation termination events. Our data furthermore suggest a possible role of Dbp5/DDX19 in alternative translation termination events, such as during stress response or in developmental processes, which classifies the helicase as a potential drug target for nonsense suppression therapy to treat cancer and neurodegenerative diseases."],["dc.identifier.doi","10.1093/nar/gkz177"],["dc.identifier.pmid","30873535"],["dc.identifier.purl","https://resolver.sub.uni-goettingen.de/purl?gs-1/16303"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/62049"],["dc.language.iso","en"],["dc.notes.intern","Merged from goescholar"],["dc.relation.eissn","1362-4962"],["dc.relation.issn","0305-1048"],["dc.relation.issn","1362-4962"],["dc.rights","CC BY 4.0"],["dc.rights.uri","https://creativecommons.org/licenses/by/4.0"],["dc.title","Translation termination depends on the sequential ribosomal entry of eRF1 and eRF3"],["dc.type","journal_article"],["dc.type.internalPublication","yes"],["dc.type.version","published_version"],["dspace.entity.type","Publication"]]