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首页> 外文期刊>Virology >Combining mutations in HIV-1 reverse transcriptase with mutations in the HIV-1 polypurine tract affects RNase H cleavages involved in PPT utilization.
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Combining mutations in HIV-1 reverse transcriptase with mutations in the HIV-1 polypurine tract affects RNase H cleavages involved in PPT utilization.

机译:HIV-1逆转录酶中的突变与HIV-1多嘌呤区中的突变相结合会影响PPT利用中涉及的RNase H裂解。

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摘要

The RNase H cleavages that generate and remove the polypurine tract (PPT) primer during retroviral reverse transcription must be specific to generate linear viral DNAs that are suitable substrates for the viral integrase. To determine if specific contacts between reverse transcriptase (RT) and the PPT are a critical factor in determining the cleavage specificity of RNase H, we made HIV-1 viruses containing mutations in RT and the PPT at the locations of critical contacts between the protein and the nucleic acid. The effects on titer and RNase H cleavage suggest that combining mutations in RT with mutations in the PPT affect the structure of the protein of the RTucleic acid complex in ways that affect the specificity and the rate of PPT cleavage. In contrast, the mutations in the PPT (alone) and RT (alone) affect the specificity of PPT cleavage but have much less effect on the overall rate of cleavage.
机译:在逆转录病毒逆转录过程中产生和去除聚嘌呤束(PPT)引物的RNase H裂解必须特异于产生线性病毒DNA,这些线性DNA是病毒整合酶的合适底物。为了确定逆转录酶(RT)和PPT之间的特异性接触是否是决定RNase H裂解特异性的关键因素,我们制备了在RT和PPT的关键接触点处含有RT和PPT突变的HIV-1病毒。核酸。对滴度和RNase H裂解的影响表明,将RT中的突变与PPT中的突变相结合会以影响PPT裂解的特异性和速率的方式影响RT /核酸复合物的蛋白质结构。相反,PPT(单独)和RT(单独)中的突变影响PPT切割的特异性,但对总切割速率的影响要小得多。

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