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猫免疫缺陷病毒gag-pol核糖体移码位点的鉴定与分析

Identification and analysis of the gag-pol ribosomal frameshift site of feline immunodeficiency virus.

作者信息

Morikawa S, Bishop D H

机构信息

AIDS Research Center, National Institute of Health, Tokyo, Japan.

出版信息

Virology. 1992 Feb;186(2):389-97. doi: 10.1016/0042-6822(92)90004-9.

Abstract

The pol genes of retroviruses are translated as gag-pol fusion proteins by ribosomal frameshifting within the gag-pol overlap region. During the ribosomal frameshift event, the gag open reading frame is shifted -1 nt to allow in-phase reading of the pol open reading frame. A consensus frameshift signal sequence of GGGAAAC within the gag-pol overlap region of feline immunodeficiency virus (FIV) has been identified followed by a sequence that has the potential for a pseudoknot tertiary structure. Using recombinant baculoviruses in which the frameshift occurs efficiently, the consensus sequence has been shown to be the site of the frameshift event. A mutation creating a termination codon just downstream of the putative frameshift signal sequence but upstream of the potential pseudoknot structure made a shorter gag product, but did not affect the efficiency of frameshifting. A mutation creating a termination codon just upstream of the putative frameshift signal made a shorter product and essentially abrogated frameshifting. Mutations in the first stem or the second stem in the potential pseudoknot structure severely reduced the frameshifting efficiency. Mutations which altered the length between the frameshift signal and the pseudoknot structure (the so-called spacer region) also reduced the frameshift efficiency. The insertion of a palindromic sequence, which could form a hairpin structure just upstream of the frameshift signal sequence, also affected the frameshifting. These results support the view that the ribosomal frameshift event in the FIV gag-pol region involves the identified signal sequence and appears to require the precisely positioned downstream sequence and indicated pseudoknot structure for efficient frameshifting.

摘要

逆转录病毒的pol基因通过gag-pol重叠区域内的核糖体移码被翻译为gag-pol融合蛋白。在核糖体移码事件中,gag开放阅读框发生-1个核苷酸的移位,以使pol开放阅读框能以同相位进行阅读。在猫免疫缺陷病毒(FIV)的gag-pol重叠区域内已鉴定出一个共有移码信号序列GGGAAAC,其后面跟着一个具有假结三级结构潜力的序列。使用移码能有效发生的重组杆状病毒,已证明该共有序列是移码事件的位点。在假定的移码信号序列下游但在潜在假结结构上游产生一个终止密码子的突变产生了较短的gag产物,但不影响移码效率。在假定的移码信号上游产生一个终止密码子的突变产生了较短的产物,并基本上消除了移码。潜在假结结构中第一个茎或第二个茎的突变严重降低了移码效率。改变移码信号与假结结构之间长度(即所谓的间隔区)的突变也降低了移码效率。在移码信号序列上游插入一个可形成发夹结构的回文序列也影响了移码。这些结果支持这样一种观点,即FIV gag-pol区域中的核糖体移码事件涉及已鉴定的信号序列,并且似乎需要精确定位的下游序列和所示的假结结构才能实现高效移码。

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