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通过核糖体移码在体外合成推测的红三叶草坏死花叶病毒RNA聚合酶。

Synthesis of the putative red clover necrotic mosaic virus RNA polymerase by ribosomal frameshifting in vitro.

作者信息

Xiong Z, Kim K H, Kendall T L, Lommel S A

机构信息

Department of Plant Pathology, North Carolina State University, Raleigh 27695-7616.

出版信息

Virology. 1993 Mar;193(1):213-21. doi: 10.1006/viro.1993.1117.

DOI:10.1006/viro.1993.1117
PMID:8438566
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7131720/
Abstract

The red clover necrotic mosaic virus (RCNMV) genome is split between two single-stranded RNA species termed RNA-1 and RNA-2. RNA-1 directs the synthesis of 88-kDa (p88), 57-kDa (p57), 37-kDa (p37), and 27-kDa (p27) polypeptides and RNA-2 a 35-kDa (p35) polypeptide in vitro. The coding order of the RNA-1 products was determined to be 5'-p27-p57-p37-3'. Antibodies to synthetic peptides representing the carboxyl terminal portions of p27 and p57 immunoprecipitated their respective polypeptides in addition to p88, suggesting that p88 is a fusion protein. A frameshift heptanucleotide sequence element has been identified in RCNMV RNA-1. In addition, a stable stem-loop secondary structure adjacent to the heptanucleotide sequence is predicted. Together, these sequence elements suggest that a ribosomal frameshifting event occurs which allows translational readthrough of the p27 open reading frame into the p57 open reading frame, generating the observed p88 product. An RNA-1 expression construct fusing the p57 and the CP open reading frame was engineered to investigate the ribosomal frameshifting event. CP antibodies immunoprecipitated a fusion protein of the predicted size containing the carboxyl portion of CP. Site-directed mutagenesis of the frameshift element indicates that in vitro, p88 can also be expressed alternatively by suppression of an amber termination codon. Based on these data, we propose that the putative RCNMV RNA polymerase is an 88-kDa polypeptide expressed by a ribosomal frameshifting mechanism similar to those utilized by retroviruses.

摘要

红三叶草坏死花叶病毒(RCNMV)的基因组分布在两个单链RNA分子上,分别称为RNA - 1和RNA - 2。RNA - 1在体外指导合成88 kDa(p88)、57 kDa(p57)、37 kDa(p37)和27 kDa(p27)的多肽,RNA - 2指导合成35 kDa(p35)的多肽。RNA - 1产物的编码顺序确定为5'-p27-p57-p37-3'。针对代表p27和p57羧基末端部分的合成肽的抗体,除了p88外,还免疫沉淀了它们各自的多肽,这表明p88是一种融合蛋白。在RCNMV RNA - 1中鉴定出一个移码七核苷酸序列元件。此外,预测在七核苷酸序列附近有一个稳定的茎环二级结构。这些序列元件共同表明发生了核糖体移码事件,该事件允许p27开放阅读框的翻译通读进入p57开放阅读框,从而产生观察到的p88产物。构建了一个融合p57和CP开放阅读框的RNA - 1表达构建体,以研究核糖体移码事件。CP抗体免疫沉淀了预测大小的融合蛋白,该融合蛋白包含CP的羧基部分。对移码元件的定点诱变表明,在体外,p88也可以通过抑制琥珀终止密码子以另一种方式表达。基于这些数据,我们提出假定的RCNMV RNA聚合酶是一种88 kDa的多肽,其通过类似于逆转录病毒所利用的核糖体移码机制表达。

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