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亲环蛋白和蛋白质二硫键异构酶基因在秀丽隐杆线虫中以功能相关的方式共同转录。

Cyclophilin and protein disulfide isomerase genes are co-transcribed in a functionally related manner in Caenorhabditis elegans.

作者信息

Page A P

机构信息

Wellcome Unit of Molecular Parasitology, The Anderson College, The University of Glasgow, Scotland.

出版信息

DNA Cell Biol. 1997 Nov;16(11):1335-43. doi: 10.1089/dna.1997.16.1335.

DOI:10.1089/dna.1997.16.1335
PMID:9407005
Abstract

The ubiquitous enzymes peptidyl prolyl cis-trans isomerase (PPI, EC 5.2.1.8) and protein disulfide isomerase (PDI, EC 5.3.4.1) are important rate-limiting catalysts of protein-folding events in the cell. In the free-living nematode Caenorhabditis elegans, two genes encoding these enzymes (cyp-9 and pdi-1, respectively) are clustered together on chromosome III. In work described elsewhere, the encoded enzymes have been expressed as recombinant proteins and have been determined to possess in vitro PPI and PDI activity. Taken together, this organization of the two genes and the related functions of their transcripts indicate that they may be cotranscribed as a polycistronic unit, similar to bacterial operons. This study details the very close linkage of pdi-1 and cyp-9, which are in the same orientation. pdi-1 is the upstream gene, and the putative polyadenylation cleavage signal of this gene is separated from the trans-splice acceptor site of cyp-9 by only 103 bp. pdi-1 is trans-spliced by the ubiquitous nematode trans-spliced leader SL1, whereas cyp-9 was found to be predominantly trans-spliced by the "operon-specific" trans-spliced leader SL2. Similar trends in relative transcript abundance were demonstrated with synchronously produced mRNA for both genes during larval development, supporting the contention that the genes are co-expressed. Finally, reporter gene analysis provides strong evidence that both genes are controlled by a single upstream regulatory element, which directs expression of both enzymes in the hypodermal cells that synthesize the cuticle.

摘要

普遍存在的肽基脯氨酰顺反异构酶(PPI,EC 5.2.1.8)和蛋白质二硫键异构酶(PDI,EC 5.3.4.1)是细胞中蛋白质折叠事件的重要限速催化剂。在自由生活的线虫秀丽隐杆线虫中,编码这两种酶的两个基因(分别为cyp-9和pdi-1)在第三条染色体上聚集在一起。在其他地方描述的研究中,编码的酶已被表达为重组蛋白,并已确定具有体外PPI和PDI活性。综合来看,这两个基因的这种组织方式及其转录本的相关功能表明它们可能作为一个多顺反子单元共转录,类似于细菌操纵子。本研究详细阐述了处于相同方向的pdi-1和cyp-9的紧密连锁。pdi-1是上游基因,该基因的推定聚腺苷酸化切割信号与cyp-9的反式剪接受体位点仅相隔103 bp。pdi-1通过普遍存在的线虫反式剪接前导序列SL1进行反式剪接,而cyp-9主要通过“操纵子特异性”反式剪接前导序列SL2进行反式剪接。在幼虫发育过程中,这两个基因同步产生的mRNA显示出相对转录本丰度的相似趋势,支持了这两个基因共表达的观点。最后,报告基因分析提供了强有力的证据,表明这两个基因都受单个上游调控元件控制,该元件指导这两种酶在合成角质层的皮下细胞中表达。

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