Serruya Raphael, Orlovetskie Natalie, Reiner Robert, Dehtiar-Zilber Yana, Wesolowski Donna, Altman Sidney, Jarrous Nayef
Department of Microbiology and Molecular Genetics, IMRIC, The Hebrew University-Hadassah Medical School, Jerusalem 91120, Israel.
Department of Molecular, Cellular and Developmental Biology, Yale University, New Haven, CT 06520, USA.
Nucleic Acids Res. 2015 Jun 23;43(11):5442-50. doi: 10.1093/nar/gkv447. Epub 2015 May 7.
Human RNase P is implicated in transcription of small non-coding RNA genes by RNA polymerase III (Pol III), but the precise role of this ribonucleoprotein therein remains unknown. We here show that targeted destruction of HeLa nuclear RNase P inhibits transcription of 5S rRNA genes in whole cell extracts, if this precedes the stage of initiation complex formation. Biochemical purification analyses further reveal that this ribonucleoprotein is recruited to 5S rRNA genes as a part of proficient initiation complexes and the activity persists at reinitiation. Knockdown of RNase P abolishes the assembly of initiation complexes by preventing the formation of the initiation sub-complex of Pol III. Our results demonstrate that the structural intactness, but not the endoribonucleolytic activity per se, of RNase P is critical for the function of Pol III in cells and in extracts.
人核糖核酸酶P(RNase P)与RNA聚合酶III(Pol III)转录小非编码RNA基因有关,但这种核糖核蛋白在其中的确切作用尚不清楚。我们在此表明,如果在起始复合物形成阶段之前进行,靶向破坏HeLa细胞核RNase P会抑制全细胞提取物中5S rRNA基因的转录。生化纯化分析进一步表明,这种核糖核蛋白作为有效起始复合物的一部分被招募到5S rRNA基因上,并且该活性在重新起始时持续存在。敲低RNase P可通过阻止Pol III起始亚复合物的形成来消除起始复合物的组装。我们的结果表明,RNase P的结构完整性而非核糖核酸内切酶活性本身对于Pol III在细胞和提取物中的功能至关重要。
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