Template-binding site of AMV reverse transcriptase and inactivation of the enzyme by N-ethylmaleimide

Veena K. Parnaik, M.R. Das
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引用次数: 5

Abstract

N-Ethylmaleimide, a sulfhydryl-specific reagent, strongly inhibits AMV reverse transcriptase by specifically interfering with the template-binding site of the enzyme. However, the kinetics of inhibition differ widely with the composition and structure of the templates employed. The copying of templates with multiple 3′-hydroxyl termini appeared to be more susceptible to N-ethylmaleimide treatment, suggesting that the reagent may interfere with initiation of DNA synthesis. The ability of a template bound to enzyme prior to N-ethylmaleimide treatment to protect against inactivation of copying of other templates also, implies a common binding site for the different templates. Template exchange experiments demonstrated competition between activated calf thymus DNA and rAn · dT12–18 for binding to the enzyme. Thus, templates varying widely in composition and conformation appear to bind at a common site on reverse transcriptase. The experimental data also show suggestive evidence for small but finite differences in the requirements for optimal binding for templates of different structures.

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AMV逆转录酶的模板结合位点及n -乙基马来酰亚胺对该酶的失活作用
n -乙基马来酰亚胺是一种巯基特异性试剂,通过特异性干扰AMV逆转录酶的模板结合位点,强烈抑制AMV逆转录酶。然而,抑制的动力学与所用模板的组成和结构有很大的不同。具有多个3 ' -羟基末端的模板的复制似乎更容易受到n -乙基马来酰亚胺处理,这表明该试剂可能干扰DNA合成的起始。在n -乙基马来酰亚胺处理之前,模板与酶结合以防止其他模板复制失活的能力也意味着不同模板有一个共同的结合位点。模板交换实验表明,激活的小牛胸腺DNA和rAn·dT12-18之间存在竞争,以与酶结合。因此,在组成和构象上差异很大的模板似乎在逆转录酶的共同位点结合。实验数据还表明,不同结构的模板在最佳结合要求上存在微小但有限的差异。
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