@article{BalkenholKaltdorfMammadovaBachetal.2020,
  author    = {Balkenhol, Johannes and Kaltdorf, Kristin V. and Mammadova-Bach, Elmina and Braun, Attila and Nieswandt, Bernhard and Dittrich, Marcus and Dandekar, Thomas},
  title     = {Comparison of the central human and mouse platelet signaling cascade by systems biological analysis},
  series = {BMC Genomics},
  volume    = {21},
  journal   = {BMC Genomics},
  doi       = {10.1186/s12864-020-07215-4},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-230377},
  year      = {2020},
  abstract  = {Background Understanding the molecular mechanisms of platelet activation and aggregation is of high interest for basic and clinical hemostasis and thrombosis research. The central platelet protein interaction network is involved in major responses to exogenous factors. This is defined by systemsbiological pathway analysis as the central regulating signaling cascade of platelets (CC). Results The CC is systematically compared here between mouse and human and major differences were found. Genetic differences were analysed comparing orthologous human and mouse genes. We next analyzed different expression levels of mRNAs. Considering 4 mouse and 7 human high-quality proteome data sets, we identified then those major mRNA expression differences (81\%) which were supported by proteome data. CC is conserved regarding genetic completeness, but we observed major differences in mRNA and protein levels between both species. Looking at central interactors, human PLCB2, MMP9, BDNF, ITPR3 and SLC25A6 (always Entrez notation) show absence in all murine datasets. CC interactors GNG12, PRKCE and ADCY9 occur only in mice. Looking at the common proteins, TLN1, CALM3, PRKCB, APP, SOD2 and TIMP1 are higher abundant in human, whereas RASGRP2, ITGB2, MYL9, EIF4EBP1, ADAM17, ARRB2, CD9 and ZYX are higher abundant in mouse. Pivotal kinase SRC shows different regulation on mRNA and protein level as well as ADP receptor P2RY12. Conclusions Our results highlight species-specific differences in platelet signaling and points of specific fine-tuning in human platelets as well as murine-specific signaling differences.},
  language  = {en}
}
@article{LorenzinBenaryBaluapurietal.2016,
  author    = {Lorenzin, Francesca and Benary, Uwe and Baluapuri, Apoorva and Walz, Susanne and Jung, Lisa Anna and von Eyss, Bj{\"o}rn and Kisker, Caroline and Wolf, Jana and Eilers, Martin and Wolf, Elmar},
  title     = {Different promoter affinities account for specificity in MYC-dependent gene regulation},
  series = {eLife},
  volume    = {5},
  journal   = {eLife},
  doi       = {10.7554/eLife.15161},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-162913},
  pages     = {e15161},
  year      = {2016},
  abstract  = {Enhanced expression of the MYC transcription factor is observed in the majority of tumors. Two seemingly conflicting models have been proposed for its function: one proposes that MYC enhances expression of all genes, while the other model suggests gene-specific regulation. Here, we have explored the hypothesis that specific gene expression profiles arise since promoters differ in affinity for MYC and high-affinity promoters are fully occupied by physiological levels of MYC. We determined cellular MYC levels and used RNA- and ChIP-sequencing to correlate promoter occupancy with gene expression at different concentrations of MYC. Mathematical modeling showed that binding affinities for interactions of MYC with DNA and with core promoter-bound factors, such as WDR5, are sufficient to explain promoter occupancies observed in vivo. Importantly, promoter affinity stratifies different biological processes that are regulated by MYC, explaining why tumor-specific MYC levels induce specific gene expression programs and alter defined biological properties of cells.},
  language  = {en}
}
@article{BugaScholzKumaretal.2012,
  author    = {Buga, Ana-Maria and Scholz, Claus J{\"u}rgen and Kumar, Senthil and Herndon, James G. and Alexandru, Dragos and Cojocaru, Gabriel Radu and Dandekar, Thomas and Popa-Wagner, Aurel},
  title     = {Identification of New Therapeutic Targets by Genome-Wide Analysis of Gene Expression in the Ipsilateral Cortex of Aged Rats after Stroke},
  series = {PLoS One},
  volume    = {7},
  journal   = {PLoS One},
  number    = {12},
  doi       = {10.1371/journal.pone.0050985},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-130657},
  pages     = {e50985},
  year      = {2012},
  abstract  = {Background: Because most human stroke victims are elderly, studies of experimental stroke in the aged rather than the young rat model may be optimal for identifying clinically relevant cellular responses, as well for pinpointing beneficial interventions. Methodology/Principal Findings: We employed the Affymetrix platform to analyze the whole-gene transcriptome following temporary ligation of the middle cerebral artery in aged and young rats. The correspondence, heat map, and dendrogram analyses independently suggest a differential, age-group-specific behaviour of major gene clusters after stroke. Overall, the pattern of gene expression strongly suggests that the response of the aged rat brain is qualitatively rather than quantitatively different from the young, i.e. the total number of regulated genes is comparable in the two age groups, but the aged rats had great difficulty in mounting a timely response to stroke. Our study indicates that four genes related to neuropathic syndrome, stress, anxiety disorders and depression (Acvr1c, Cort, Htr2b and Pnoc) may have impaired response to stroke in aged rats. New therapeutic options in aged rats may also include Calcrl, Cyp11b1, Prcp, Cebpa, Cfd, Gpnmb, Fcgr2b, Fcgr3a, Tnfrsf26, Adam 17 and Mmp14. An unexpected target is the enzyme 3-hydroxy-3-methylglutaryl-Coenzyme A synthase 1 in aged rats, a key enzyme in the cholesterol synthesis pathway. Post-stroke axonal growth was compromised in both age groups. Conclusion/Significance: We suggest that a multi-stage, multimodal treatment in aged animals may be more likely to produce positive results. Such a therapeutic approach should be focused on tissue restoration but should also address other aspects of patient post-stroke therapy such as neuropathic syndrome, stress, anxiety disorders, depression, neurotransmission and blood pressure.},
  language  = {en}
}
@article{YanHongChenetal.2013,
  author    = {Yan, Yan and Hong, Ni and Chen, Tiansheng and Li, Mingyou and Wang, Tiansu and Guan, Guijun and Qiao, Yongkang and Chen, Songlin and Schartl, Manfred and Li, Chang-Ming and Hong, Yunhan},
  title     = {p53 Gene Targeting by Homologous Recombination in Fish ES Cells},
  series = {PLoS One},
  volume    = {8},
  journal   = {PLoS One},
  number    = {3},
  doi       = {10.1371/journal.pone.0059400},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-133416},
  pages     = {e59400},
  year      = {2013},
  abstract  = {Background: Gene targeting (GT) provides a powerful tool for the generation of precise genetic alterations in embryonic stem (ES) cells to elucidate gene function and create animal models for human diseases. This technology has, however, been limited to mouse and rat. We have previously established ES cell lines and procedures for gene transfer and selection for homologous recombination (HR) events in the fish medaka (Oryzias latipes). Methodology and Principal Findings: Here we report HR-mediated GT in this organism. We designed a GT vector to disrupt the tumor suppressor gene p53 (also known as tp53). We show that all the three medaka ES cell lines, MES1 similar to MES3, are highly proficient for HR, as they produced detectable HR without drug selection. Furthermore, the positive-negative selection (PNS) procedure enhanced HR by similar to 12 folds. Out of 39 PNS-resistant colonies analyzed, 19 (48.7\%) were positive for GT by PCR genotyping. When 11 of the PCR-positive colonies were further analyzed, 6 (54.5\%) were found to be bona fide homologous recombinants by Southern blot analysis, sequencing and fluorescent in situ hybridization. This produces a high efficiency of up to 26.6\% for p53 GT under PNS conditions. We show that p53 disruption and long-term propagation under drug selection conditions do not compromise the pluripotency, as p53-targeted ES cells retained stable growth, undifferentiated phenotype, pluripotency gene expression profile and differentiation potential in vitro and in vivo. Conclusions: Our results demonstrate that medaka ES cells are proficient for HR-mediated GT, offering a first model organism of lower vertebrates towards the development of full ES cell-based GT technology.},
  language  = {en}
}
@article{GoebMeyerNatusBenaventeetal.2011,
  author    = {G{\"o}b, Eva and Meyer-Natus, Elisabeth and Benavente, Ricardo and Alsheimer, Manfred},
  title     = {Expression of individual mammalian Sun1 isoforms depends on the cell type},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-68750},
  year      = {2011},
  abstract  = {Mammalian Sun1 belongs to an evolutionarily conserved family of inner nuclear membrane proteins, which are known as SUN domain proteins. SUN domain proteins interact with KASH domain partners to form bridging complexes, so-called LINC complexes, that physically connect the nuclear interior to the cytoskeleton. LINC complexes are critical for nuclear integrity and play fundamental roles in nuclear positioning, shaping and movement. The mammalian genome codes for at least five different SUN domain proteins used for the formation of a number of different LINC complexes. Recently, we reported on the identification of everal Sun1 isoforms, which tremendously enlarges the alternatives to form functional LINC complexes. We now confirmed that Sun1 actually exists in at least seven distinct splice variants. Besides that, we observed that expression of individual Sun1 isoforms remarkably depends on the cell type, suggesting a cell type-specific adaption of Sun1 dependent LINC complexes to specific cellular and physiological requirements.},
  subject      = {Biologie},
  language  = {en}
}
@phdthesis{Leimeister1999,
  author    = {Leimeister, Cornelia},
  title     = {Identifizierung und Charakterisierung von Genen f{\"u}r die Entwicklung der Nieren und des Urogenitalsystems},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-1690},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {1999},
  abstract  = {Das Studium der Nierenentwicklung gibt Einblicke in generelle entwicklungsbiologische Prozesse wie induktive Wechselwirkungen, mesenchymale Kondensation, mesenchymale-epitheliale Umformung, Determinierung von Zellschicksal sowie Differenzierung und damit auch in die Entstehung congenitaler Fehlbildungen. Nach Induktion durch die Ureterknospe entstehen aus dem metanephrogenen Mesenchym die funktionellen Einheiten der Niere - die Nephrone - und das Nierenstroma. Diesen morphogenetischen Prozessen liegen komplexe regulatorische Ver{\"a}nderungen in der Genexpression zugrunde, die bislang nicht im Detail aufgekl{\"a}rt sind. Ziel dieser Arbeit war deshalb die Identifizierung bekannter und insbesondere neuer Gene, die durch Induktion im metanephrogenen Mesenchym reguliert werden. Mit Hilfe der ddPCR und Transfilter-Organkulturen wurde die Genexpression von induziertem versus nicht-induziertem Mesenchym aus M{\"a}use-Nierenanlagen untersucht. Einzelne Kandidaten wurden auf differenzielle Expression durch Northern Blot Analyse {\"u}berpr{\"u}ft und f{\"u}r die weitere Charakterisierung ausgew{\"a}hlt. Als eines der bekannten Gene wurde sFRP2 als im metanephrogenen Mesenchym induziert best{\"a}tigt und durch in situ Hybridisierung ganzer M{\"a}useembryonen und Paraffinschnitte n{\"a}her untersucht. Es zeigt eine spezifische und dynamische Expression w{\"a}hrend der Entwicklung der Niere und anderer Gewebe, die mit den Expressionsmustern von sFRP1 und sFRP4 verglichen wurde. Die detailierte Genexpressionsanalyse der sFRP-Familie in der murinen Embryonalentwicklung sollte als Grundlage f{\"u}r funktionelle Studien dieser erst k{\"u}rzlich entdeckten neuen Genfamilie dienen. Erste Untersuchungen der ddPCR-Produkte C0-5, J6-3 und M2-4 zeigten, daß es sich um neue Gene handelt, die unterschiedliche Expressionsmuster in der Niere zeigen. W{\"a}hrend C0-5 dynamisch in Epithelzellen von Ureter und Nephronvorl{\"a}ufern exprimiert ist, markiert J6-3 Stromazellen und M2-4 ist bereits im kondensierenden Mesenchym, sp{\"a}ter aber auch in den epithelialen Derivaten nachweisbar. Die Isolierung und Analyse der dem C0-5-ddPCR-Fragment entsprechenden cDNA zeigte, daß sie f{\"u}r ein kollagenartiges Protein codiert, welches beim Menschen in der N{\"a}he des EWS-Gens auf Chromosom 22q12 liegt. Dar{\"u}ber hinaus wurde eine neue zu hairy und dem E(spl)-Komplex verwandte Genfamile identifiziert. Aufgrund ihrer Verwandtschaft und einem charakteristischen YRPW-Tetrapeptid wurden sie als Hey-Gene bezeichnet f{\"u}r: "hairy- und E(spl)-verwandt mit YRPW-Motiv". Sie zeigen gegen{\"u}ber hairy/E(spl) oder den entsprechenden Vertebraten-Homologen der Hes-Genfamilie ver{\"a}nderte DNA- und Protein-Bindungseigenschaften. Dar{\"u}ber hinaus korrelieren ihre Expressionsmuster h{\"a}ufig mit Genen des Delta-Notch-Signaltransduktionsweg, was auf eine Beteiligung der Hey-Gene an Zelldeterminierung und Bildung von Zellgrenzen hinweist. Diese Vermutung konnte durch die Analyse von Dll1-Knockout-M{\"a}usen f{\"u}r die Somitogenese ansatzweise best{\"a}tigt werden. Die Kombination von Transfilter-Organkultur mit ddPCR erwies sich als geeignet, um transkriptionell regulierte Gene des metanephrogenen Mesenchyms zu identifizieren. Expressions- und Sequenzanalyse vor allem der neuen Gene deutet auf ihre Beteiligung an der Entwicklung der Niere und anderer Gewebe hin, die nun im Einzelnen untersucht werden muß. Mehr als 50 weitere Kandidaten f{\"u}r neue Gene bilden eine breite Basis zur weiteren Erforschung molekularer Grundlagen der Nierenentwicklung.},
  subject      = {Niere},
  language  = {de}
}