基因抑制的早熟转录终止鉴定突变的基本亚单位的分裂酵母切割和聚腺苷酸化机制。

IF 5 3区生物学 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY

RNA Pub Date : 2025-09-04 DOI:10.1261/rna.080664.125

Aleksei Innokentev, Ana M Sanchez, Lauren Bednor, Jill Babor, Beate Schwer, Stewart Shuman

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引用次数: 0

摘要

在磷酸盐充满的条件下，裂变酵母磷酸盐获取（PHO）调控被上游lncrna介导的转录干扰所抑制。肌醇-1焦磷酸通过其作为早熟PHO lncRNA 3'加工/终止的激动剂的作用来控制磷酸盐稳态。肌醇焦磷酸酶失活突变增加肌醇-1焦磷酸酶可引起PHO基因的抑制和YES培养基中严重的生长缺陷。先前的研究表明，通过对裂变酵母切割和聚腺苷化因子（CPF）复合物的非必需的Ssu72、Ppn1、Swd22和Ctf1亚基的靶向缺失或功能缺失突变，可以抑制肌醇焦磷酸中毒。在这里，我们筛选了抑制asp1-STF焦磷酸酶突变体发病的PHO lncRNA过早终止的自发突变。因此，我们在五个重要的CPF亚基中恢复并鉴定了新的亚形态错义突变：Ysh1（裂解内切酶）、Pta1（犰狳/热重复蛋白）、Pfs2 （WD重复蛋白）、Cft1 （WD重复蛋白）和Msi2（串联RRM rna结合蛋白）。筛选还在编码CPF必需亚基Iss1的基因中产生了内含子分支点突变。此外，我们发现asp1-STF中毒是由CPF必需的聚(a)聚合酶亚基Pla1活性位点的错义突变抑制的。遗传杂交揭示了必需CPF亚基、非必需CPF亚基、终止因子Rhn1、RNA聚合酶II CTD编码的Thr4“字母”和合成肌醇-1焦磷酸的Asp1激酶之间的突变协同作用的层次结构。Msi2 - g252e与ctf1∆、swd22∆、ppn1∆、ssu72-C13S、rpb1-CTD-T4A和asp1∆的合成致死性表明，Msi2是3'-加工/终止的中心剂，与肌醇-1焦磷酸平行起作用。

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Genetic suppression of precocious transcription termination identifies mutations in essential subunits of the fission yeast cleavage and polyadenylation machinery.

The fission yeast phosphate acquisition (PHO) regulon is repressed under phosphate-replete conditions by upstream lncRNA-mediated transcriptional interference. Inositol-1-pyrophosphates control phosphate homeostasis via their action as agonists of precocious PHO lncRNA 3'-processing/termination. Inositol pyrophosphatase-inactivating mutations that increase inositol-1-pyrophosphates elicit derepression of the PHO genes and a severe growth defect in YES medium. Previous studies demonstrated suppression of inositol pyrophosphate toxicosis by targeted deletion or loss-of-function mutations in the nonessential Ssu72, Ppn1, Swd22, and Ctf1 subunits of the fission yeast Cleavage and Polyadenylation Factor (CPF) complex. Here we conducted a screen for spontaneous mutations that suppress the precocious PHO lncRNA termination underlying the sickness of asp1-STF pyrophosphatase mutants. We thereby recovered and characterized novel hypomorphic missense mutations in five essential CPF subunits: Ysh1 (the cleavage endonuclease), Pta1 (an Armadillo/HEAT-repeat protein), Pfs2 (a WD repeat protein), Cft1 (a WD repeat protein), and Msi2 (a tandem RRM RNA-binding protein). The screen also yielded an intron branchpoint mutation in the gene encoding essential CPF subunit Iss1. In addition, we found that asp1-STF toxicosis was suppressed by a missense mutation in the active site of Pla1, the essential poly(A) polymerase subunit of CPF. Genetic crosses revealed a hierarchy of mutational synergies between the essential CPF subunits, the inessential CPF subunits, termination factor Rhn1, the Thr4 "letter" of the RNA polymerase II CTD code, and the Asp1 kinase that synthesizes inositol-1-pyrophosphates. The synthetic lethality of msi2-G252E with ctf1∆, swd22∆, ppn1∆, ssu72-C13S, rpb1-CTD-T4A, and asp1∆ establishes Msi2 as a central agent of 3'-processing/termination, functioning in parallel to inositol-1-pyrophosphates.

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来源期刊

RNA 生物-生化与分子生物学

CiteScore

8.30

自引率

2.20%

发文量

101

审稿时长

2.6 months

期刊介绍： RNA is a monthly journal which provides rapid publication of significant original research in all areas of RNA structure and function in eukaryotic, prokaryotic, and viral systems. It covers a broad range of subjects in RNA research, including: structural analysis by biochemical or biophysical means; mRNA structure, function and biogenesis; alternative processing: cis-acting elements and trans-acting factors; ribosome structure and function; translational control; RNA catalysis; tRNA structure, function, biogenesis and identity; RNA editing; rRNA structure, function and biogenesis; RNA transport and localization; regulatory RNAs; large and small RNP structure, function and biogenesis; viral RNA metabolism; RNA stability and turnover; in vitro evolution; and RNA chemistry.