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Cwf16p与19S复合体结合确保裂殖酵母组成型前体mRNA剪接中有序的外显子连接。

Cwf16p Associating with the Nineteen Complex Ensures Ordered Exon Joining in Constitutive Pre-mRNA Splicing in Fission Yeast.

作者信息

Sasaki-Haraguchi Noriko, Ikuyama Takeshi, Yoshii Shogo, Takeuchi-Andoh Tomoko, Frendewey David, Tani Tokio

机构信息

Department of Biological Sciences, Graduate School of Science and Technology, Kumamoto University, Kumamoto, Japan.

Regeneron Pharmaceuticals, Inc., Tarrytown, New York, United States of America.

出版信息

PLoS One. 2015 Aug 24;10(8):e0136336. doi: 10.1371/journal.pone.0136336. eCollection 2015.

Abstract

Exons are ligated in an ordered manner without the skipping of exons in the constitutive splicing of pre-mRNAs with multiple introns. To identify factors ensuring ordered exon joining in constitutive pre-mRNA splicing, we previously screened for exon skipping mutants in Schizosaccharomyces pombe using a reporter plasmid, and characterized three exon skipping mutants named ods1 (ordered splicing 1), ods2, and ods3, the responsible genes of which encode Prp2/U2AF59, U2AF23, and SF1, respectively. They form an SF1-U2AF59-U2AF23 complex involved in recognition of the branch and 3' splice sites in pre-mRNA. In the present study, we identified a fourth ods mutant, ods4, which was isolated in an exon-skipping screen. The ods4+ gene encodes Cwf16p, which interacts with the NineTeen Complex (NTC), a complex thought to be involved in the first catalytic step of the splicing reaction. We isolated two multi-copy suppressors for the ods4-1 mutation, Srp2p, an SR protein essential for pre-mRNA splicing, and Tif213p, a translation initiation factor, in S. pombe. The overexpression of Srp2p suppressed the exon-skipping phenotype of all ods mutants, whereas Tif213p suppressed only ods4-1, which has a mutation in the translational start codon of the cwf16 gene. We also showed that the decrease in the transcriptional elongation rate induced by drug treatment suppressed exon skipping in ods4-1. We propose that Cwf16p/NTC participates in the early recognition of the branch and 3' splice sites and cooperates with the SF1-U2AF59-U2AF23 complex to maintain ordered exon joining.

摘要

在外显子组成型剪接过程中,外显子按顺序连接,不会跳过多个内含子的前体mRNA中的外显子。为了确定确保组成型前体mRNA剪接中外显子有序连接的因素,我们之前使用报告质粒在粟酒裂殖酵母中筛选外显子跳跃突变体,并鉴定了三个外显子跳跃突变体,分别命名为ods1(有序剪接1)、ods2和ods3,其相关基因分别编码Prp2/U2AF59、U2AF23和SF1。它们形成一个SF1-U2AF59-U2AF23复合物,参与前体mRNA中分支位点和3'剪接位点的识别。在本研究中,我们鉴定了第四个ods突变体ods4,它是在一次外显子跳跃筛选中分离得到的。ods4+基因编码Cwf16p,它与九蛋白复合物(NTC)相互作用,NTC被认为参与剪接反应的第一步催化过程。我们在粟酒裂殖酵母中分离出了ods4-1突变的两个多拷贝抑制子,即Srp2p(一种前体mRNA剪接所必需的SR蛋白)和Tif213p(一种翻译起始因子)。Srp2p的过表达抑制了所有ods突变体的外显子跳跃表型,而Tif213p仅抑制ods4-1,ods4-1在cwf16基因的翻译起始密码子处有一个突变。我们还表明,药物处理诱导的转录延伸率降低抑制了ods4-1中的外显子跳跃。我们提出,Cwf16p/NTC参与分支位点和3'剪接位点的早期识别,并与SF1-U2AF59-U2AF23复合物协同作用以维持外显子的有序连接。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1db7/4547733/49e3cf088afe/pone.0136336.g001.jpg

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