Role of Ccr4-Not complex in heterochromatin formation at meiotic genes and subtelomeres in fission yeast

Cotobal, Cristina; Rodríguez-López, Maria; Duncan, Caia D. S.; Hasan, Ayesha; Yamashita, Akira; Yamamoto, Masayuki; Bähler, Jürg; Mata, Juan

doi:10.1186/s13072-015-0018-4

Cited by 42 publications

(68 citation statements)

References 68 publications

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“…6A as DSRx3-2). Tandem DSRs promote the selective degradation of meiotic mRNAs expressed during vegetative growth of fission yeast, via their recognition by the YTHdomain protein Mmi1 (Harigaya et al 2006;Yamashita et al 2012), which interacts with the nuclear exosome and with the Ccr4-Not complex (Cotobal et al 2015;Ukleja et al 2016). During meiosis, Mmi1 is sequestered by a DSR-containing lncRNA transcribed at the sme2 locus (Harigaya et al 2006;Shichino et al 2014), allowing stabilization of DSR-containing meiotic mRNAs.…”

Section: Prt Lncrna Contains Multiple Potential Dsr Sequencesmentioning

confidence: 99%

Transcription of lncRNA prt, clustered prt RNA sites for Mmi1 binding, and RNA polymerase II CTD phospho-sites govern the repression of pho1 gene expression under phosphate-replete conditions in fission yeast

Chatterjee

Sánchez

Goldgur

et al. 2016

RNA

131

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Expression of fission yeast Pho1 acid phosphatase is repressed during growth in phosphate-rich medium. Repression is mediated by transcription of the prt locus upstream of pho1 to produce a long noncoding (lnc) prt RNA. Repression is also governed by RNA polymerase II CTD phosphorylation status, whereby inability to place a Ser7-PO 4 mark (as in S7A) derepresses Pho1 expression, and inability to place a Thr4-PO 4 mark (as in T4A) hyper-represses Pho1 in phosphate replete cells. Here we find that basal pho1 expression from the prt-pho1 locus is inversely correlated with the activity of the prt promoter, which resides in a 110-nucleotide DNA segment preceding the prt transcription start site. CTD mutations S7A and T4A had no effect on the activity of the prt promoter or the pho1 promoter, suggesting that S7A and T4A affect post-initiation events in prt lncRNA synthesis that make it less and more repressive of pho1, respectively. prt lncRNA contains clusters of DSR (determinant of selective removal) sequences recognized by the YTH-domain-containing protein Mmi1. Altering the nucleobase sequence of two DSR clusters in the prt lncRNA caused hyper-repression of pho1 in phosphate replete cells, concomitant with increased levels of the prt transcript. The isolated Mmi1 YTH domain binds to RNAs with single or tandem DSR elements, to the latter in a noncooperative fashion. We report the 1.75 Å crystal structure of the Mmi1 YTH domain and provide evidence that Mmi1 recognizes DSR RNA via a binding mode distinct from that of structurally homologous YTH proteins that recognize m 6 Amodified RNA.

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Section: Prt Lncrna Contains Multiple Potential Dsr Sequencesmentioning

confidence: 99%

Transcription of lncRNA prt, clustered prt RNA sites for Mmi1 binding, and RNA polymerase II CTD phospho-sites govern the repression of pho1 gene expression under phosphate-replete conditions in fission yeast

Chatterjee

Sánchez

Goldgur

et al. 2016

RNA

131

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“…At the same time, heterochromatic transcripts are degraded by RNAi. A link between various RNA degradation machineries and H3K9me at meiotic genes was also recently reported (Hiriart et al 2012;Zofall et al 2012;Egan et al 2014;Chalamcharla et al 2015;Cotobal et al 2015;Tucker et al 2016). Several of those studies suggested a direct recruitment of the H3K9 methyltransferase by different RNA degradation machineries to deposit H3K9me.…”

mentioning

confidence: 99%

Accumulation of RNA on chromatin disrupts heterochromatic silencing

Brönner¹,

Salvi²,

Zocco³

et al. 2017

Genome Res.

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Long noncoding RNAs (lncRNAs) play a conserved role in regulating gene expression, chromatin dynamics, and cell differentiation. They serve as a platform for RNA interference (RNAi)-mediated heterochromatin formation or DNA methylation in many eukaryotic organisms. We found in Schizosaccharomyces pombe that heterochromatin is lost at transcribed regions in the absence of RNA degradation. We show that heterochromatic RNAs are retained on chromatin, form DNA: RNA hybrids, and need to be degraded by the Ccr4-Not complex or RNAi to maintain heterochromatic silencing. The Ccr4-Not complex is localized to chromatin independently of H3K9me and degrades chromatin-associated transcripts, which is required for transcriptional silencing. Overexpression of heterochromatic RNA, but not euchromatic RNA, leads to chromatin localization and loss of silencing of a distant ade6 reporter in wild-type cells. Our results demonstrate that chromatin-bound RNAs disrupt heterochromatin organization and need to be degraded in a process of heterochromatin formation.

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“…XND-1 protein sequence provides no hints as its function, although its localization to autosomes in the developing and adult germ cells hints at a role as a chromatin regulator. The association of Nanos proteins with the CCR4/ NOT complex that recently was shown to regulate heterochromatic loci in Saccromyces pombe 35 raises the tantalizing possibility that Nanos family members may accordingly facilitate heterochromatinization of the germ line.…”

Section: Functional Redundancy In Germ Line Differentiation Pathwaysmentioning

confidence: 99%

A twist of fate: How a meiotic protein is providing new perspectives on germ cell development

Rana

Yanowitz

2016

Worm

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The molecular pathways that govern how germ line fate is acquired is an area of intense investigation that has major implications for the development of assisted reproductive technologies, infertility interventions, and treatment of germ cell cancers. Transcriptional repression has emerged as a primary mechanism to ensure suppression of somatic growth programs in primordial germ cells. In this commentary, we address how xnd-1 illuminates our understanding of transcriptional repression and how it is coordinated with the germ cell differentiation program. We recently identified xnd-1 as a novel, early determinant of germ cell fates in Caenorhabditis elegans. Our study revealed that XND-1 is maternally deposited into early embryos where it is selectively enriched in the germ lineage and then exclusively found on chromatin in the germ lineage throughout development and into adulthood when it dissociates from chromosomes in late pachytene. This localization is consistent with a range of interesting germ cell defects that suggest xnd-1 is a pivotal determinant of germ cell characteristics. Loss of xnd-1 results in a unique "one PGC (primordial germ cell)" phenotype due to G2 cell cycle arrest of the germline precursor blastomere, P 4 , which predisposes the animal and its progeny for reduced fecundity. The sterility in xnd-1 mutants is correlated with an increase in the transcriptional activationassociated histone modification, dimethylation of histone H3 lysine 4 (H3K4me2), and aberrant expression of somatic transgenes but overlapping roles with nos-2 and nos-1 suggest that transcriptional repression is achieved by multiple redundant mechanisms.

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Role of Ccr4-Not complex in heterochromatin formation at meiotic genes and subtelomeres in fission yeast

Cited by 42 publications

References 68 publications

Transcription of lncRNA prt, clustered prt RNA sites for Mmi1 binding, and RNA polymerase II CTD phospho-sites govern the repression of pho1 gene expression under phosphate-replete conditions in fission yeast

Transcription of lncRNA prt, clustered prt RNA sites for Mmi1 binding, and RNA polymerase II CTD phospho-sites govern the repression of pho1 gene expression under phosphate-replete conditions in fission yeast

Accumulation of RNA on chromatin disrupts heterochromatic silencing

A twist of fate: How a meiotic protein is providing new perspectives on germ cell development

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