4.8 Article

Nuclear fate of yeast snoRNA is determined by co-transcriptional Rnt1 cleavage

Journal

NATURE COMMUNICATIONS
Volume 9, Issue -, Pages -

Publisher

NATURE PUBLISHING GROUP
DOI: 10.1038/s41467-018-04094-y

Keywords

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Funding

  1. Polish Ministry of Science and Higher Education [N N301 065740]
  2. Polish-Swiss Research Programme [PSPB-183/2010]
  3. National Science Centre [UMO-2011/01/N/NZ1/04344]
  4. EU Social Fund [UDAPOKL.04.01.01-00-072/09-00]
  5. EU Regional Development Fund [POIG.02.02.00-14-024/08-00]
  6. Sir Henry Dale Fellowship - Wellcome Trust [200473/Z/16/Z]
  7. Sir Henry Dale Fellowship - Royal Society [200473/Z/16/Z]
  8. Wellcome Trust Programme Grant [091805/Z/10/Z]
  9. European Research Council Advanced Grant [339270]
  10. Wellcome Trust [203141/Z/16/Z]

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Small nucleolar RNA (snoRNA) are conserved and essential non-coding RNA that are transcribed by RNA Polymerase II (Pol II). Two snoRNA classes, formerly distinguished by their structure and ribonucleoprotein composition, act as guide RNA to target RNA such as ribosomal RNA, and thereby introduce specific modifications. We have studied the 5'end processing of individually transcribed snoRNA in S. cerevisiae to define their role in snoRNA biogenesis and functionality. Here we show that pre-snoRNA processing by the endonuclease Rnt1 occurs co-transcriptionally with removal of the m7G cap facilitating the formation of box C/D snoRNA. Failure of this process causes aberrant 3'end processing and mislocalization of snoRNA to the cytoplasm. Consequently, Rnt1-dependent 5'end processing of box C/D snoRNA is critical for snoRNA-dependent methylation of ribosomal RNA. Our results reveal that the 5'end processing of box C/D snoRNA defines their distinct pathway of maturation.

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