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Ty1 in vitro integration: effects of mutations in cis and in trans.

机译:Ty1体外整合:顺式和反式突变的影响。

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摘要

Mutations within the TYB gene of Ty1 encoding integrase (IN) as well as alterations in its substrate, a linear DNA molecule, were examined for their effects on in vitro IN activity, using a recently developed physical assay. Five different codon-insertion mutations, two frameshift mutations, and one missense mutation, previously identified as transposition-deficient mutations, were tested. Virus-like particles, the source of IN, from two different protease mutants and a reverse transcriptase mutant exhibited near-normal to normal IN activity. Two frameshift mutations mapping within the phylogenetically variable C-terminal domain of IN resulted in significant in vitro IN activity. In contrast, three mutations within the amino-terminal conserved domain of IN completely abolished IN activity. When the substrate termini were mutated, we found that substrates with as few as 4 bp of Ty1 termini were capable of efficiently generating integration products. Surprisingly, certain substrates that lacked obvious similarity to Ty1 termini were also readily integrated into both linear and circular targets, whereas others were not used as substrates at all. Termini rich in adenosine residues were among the more active substrates; however, certain substrates lacking terminal adenosine residues can form small quantities of integration products, including complete integration reactions.
机译:使用最近开发的物理检测方法,检查了编码整合酶(IN)的Ty1的TYB基因中的突变及其底物(线性DNA分子)的变化对体外IN活性的影响。测试了五个不同的密码子插入突变,两个移码突变和一个错义突变(先前确定为转座缺陷突变)。来自两个不同蛋白酶突变体和逆转录酶突变体的病毒样颗粒(IN的来源)表现出接近正常的正常IN活性。 IN的系统发育可变的C-末端结构域内的两个移码突变定位导致显着的体外IN活性。相反,IN的氨基末端保守结构域内的三个突变完全消除了IN活性。当底物末端被突变时,我们发现具有低至4 bp的Ty1末端的底物能够有效地产生整合产物。出人意料的是,某些与Ty1末端缺乏明显相似性的底物也很容易整合到线性和圆形靶标中,而其他底物根本没有用作底物。富含腺苷残基的Termmini是活性更高的底物之一。但是,某些缺少末端腺苷残基的底物会形成少量的整合产物,包括完整的整合反应。

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