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Rrp5 binding at multiple sites coordinates pre-rRNA processing and assembly.

Molecular cell | 2013

In vivo UV crosslinking identified numerous preribosomal RNA (pre-rRNA) binding sites for the large, highly conserved ribosome synthesis factor Rrp5. Intramolecular complementation has shown that the C-terminal domain (CTD) of Rrp5 is required for pre-rRNA cleavage at sites A0-A2 on the pathway of 18S rRNA synthesis, whereas the N-terminal domain (NTD) is required for A3 cleavage on the pathway of 5.8S/25S rRNA synthesis. The CTD was crosslinked to sequences flanking A2 and to the snoRNAs U3, U14, snR30, and snR10, which are required for cleavage at A0-A2. The NTD was crosslinked to sequences flanking A3 and to the RNA component of ribonuclease MRP, which cleaves site A3. Rrp5 could also be directly crosslinked to several large structural proteins and nucleoside triphosphatases. A key role in coordinating preribosomal assembly and processing was confirmed by chromatin spreads. Following depletion of Rrp5, cotranscriptional cleavage was lost and preribosome compaction greatly reduced.

Pubmed ID: 24239293 RIS Download

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Associated grants

  • Agency: NIGMS NIH HHS, United States
    Id: R01 GM063952
  • Agency: Wellcome Trust, United Kingdom
    Id: 077248
  • Agency: Wellcome Trust, United Kingdom
    Id: 092076
  • Agency: Wellcome Trust, United Kingdom
    Id: 091020
  • Agency: NIGMS NIH HHS, United States
    Id: GM63952
  • Agency: Wellcome Trust, United Kingdom
    Id: 084229

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Cluster (tool)

RRID:SCR_013505

Software R package. Methods for Cluster analysis. Performs variety of types of cluster analysis and other types of processing on large microarray datasets.

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