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Effect of polymerase mutations on packaging of primer tRNAPro during murine leukemia virus assembly.

机译:聚合酶突变对鼠白血病病毒装配过程中引物tRNAPro包装的影响。

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摘要

The role of reverse transcriptase in selective encapsidation of the murine leukemia virus (MuLV) tRNA primer, tRNAPro, was investigated by examining the tRNA composition of several nonconditional pol mutants. One mutant, clone 23, which contains an altered polymerase about 40% smaller than the wild-type enzyme (B. I. Gerwin et al., J. Virol. 31:741-751, 1979) had a typical viral tRNA pattern, including normal levels of tRNAPro in free and 70S-associated 4S RNA. Another class of mutants, produced by Moloney murine leukemia virus-infected cell clone M13 and subclone M13/1, does not contain any detectable polymerase protein (A. Shields et al., Cell 14:601-609, 1978) and was found to have reduced amounts of tRNAPro in free 4S RNA. However, the level of tRNAPro associated with the genome was normal in the mutant virions. These results suggest that the reverse transcriptase protein is involved in the initial selection of tRNA primer during virus assembly, but not in the subsequent association of this tRNA with genomic RNA.
机译:通过检查几种无条件pol突变体的tRNA组成,研究了逆转录酶在鼠白血病病毒(MuLV)tRNA引物tRNAPro的选择性衣壳化中的作用。一个突变体,克隆23,其包含比野生型酶小约40%的改变的聚合酶(BI Gerwin等人,J。Virol。31:741-751,1979)具有典型的病毒tRNA模式,包括正常水平游离和70S相关的4S RNA中的tRNAPro片段。由莫洛尼氏鼠白血病病毒感染的细胞克隆M13和亚克隆M13 / 1产生的另一类突变体不含任何可检测的聚合酶蛋白(A. Shields等人,Cell 14:601-609,1978),并发现游离4S RNA中的tRNAPro含量降低。但是,与基因组相关的tRNAPro水平在突变病毒粒子中是正常的。这些结果表明,逆转录酶蛋白参与病毒装配过程中tRNA引物的初始选择,但不参与该tRNA与基因组RNA的后续结合。

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