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In vitro analysis of the HIV-1 second strand-transfer reaction

机译:HIV-1第二链转移反应的体外分析

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Two strand-transfer reactions arc required during the retroviral reverse transcription. The second strand-transfer is believed to occur at the primer binding site (PBS). By using an in vitro model system derived from the human immunodeficiency virus type-1 (HIV-1), molecular events related to die second strand-transfer reaction were examined. The RNA-directed DNA synthesis catalyzed by the HIV-1 reverse tran.seriptase (RT) appears to pause twice, around the 2nd and the 11th bases downstream into the HIV-1 PBS. In either ease, pausing seems lo be caused by local sequence effects. From both these pause sites the nascent DNA strands can undergo transfer to PBS-homologous templates. The results confirm that pausing favors the internal strand-transfer, They also indicate that PBS-mediated transfers proceed through displacement of the DNA strands from RNA donor molecules by the acceptor template, as in one of the models proposed by DeStefano et al. (DeStefano, J.J., Bambara, R.A. and Fay, P.J. (1994) J. Biol. Chem. 269, 161-168). Whereas no hydrolysis by the ribonuclease II activity of HIV-1 RT seemed to occur within the HIV-1 PBS, specific cleavage was observed outside of this sequence and noticeably 5 bases upstream from its .V end relative to the DNA primer growing point. This particular cleavage event remained essentially unchanged when the second pause site downstream into the PBS, located 16 bases beyond, was removed by mutation. The experiments suggest that this prominent RNA degradation event could precede the PBS-mediated strand-transfers.
机译:在逆转录病毒逆转录过程中需要两个链转移反应。据信第二条链转移发生在引物结合位点(PBS)。通过使用源自人类1型免疫缺陷病毒(HIV-1)的体外模型系统,检查了与第二条链转移反应有关的分子事件。 HIV-1逆转录酶(RT)催化的RNA定向的DNA合成似乎在HIV-1 PBS下游的第2个和第11个碱基附近停顿了两次。无论哪种情况,暂停似乎都是由局部序列效应引起的。从这两个停顿位点,新生的DNA链可以转移到PBS同源模板中。结果证实暂停有利于内部链转移,它们还表明PBS介导的转移是通过受体模板置换RNA供体分子的DNA链进行的,如DeStefano等人提出的模型之一。 (DeStefano,J.J.,Bambara,R.A。和Fay,P.J。(1994)J.Biol.Chem.269,161-168)。尽管在HIV-1 PBS中似乎没有发生HIV-1 RT的核糖核酸酶II活性水解,但在该序列之外观察到了特异性切割,并且相对于DNA引物生长点,在其.V末端上游明显有5个碱基。当通过突变除去位于PBS下游下游的第二个停顿位点时,该特定的裂解事件基本上保持不变,位于PBS之外的16个碱基。实验表明,这种显着的RNA降解事件可以先于PBS介导的链转移。

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