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利用15N弛豫测量分析人类免疫缺陷病毒逆转录酶核糖核酸酶H结构域的主链动力学。

Analysis of the backbone dynamics of the ribonuclease H domain of the human immunodeficiency virus reverse transcriptase using 15N relaxation measurements.

作者信息

Powers R, Clore G M, Stahl S J, Wingfield P T, Gronenborn A

机构信息

Laboratory of Chemical Physics, National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, Bethesda, Maryland 20892.

出版信息

Biochemistry. 1992 Sep 29;31(38):9150-7. doi: 10.1021/bi00153a006.

DOI:10.1021/bi00153a006
PMID:1382587
Abstract

The backbone dynamics of the uniformly 15N-labeled ribonuclease H (RNase H) domain of human immunodeficiency virus (HIV-1) reverse transcriptase have been investigated using two-dimensional inverse-detected heteronuclear 15N-1HNMR spectroscopy. 15N T1, T2, and nuclear Overhauser enhancement (NOE) data were obtained for 107 out of a total of 134 backbone amide groups. The overall rotational correlation time (tau R) for the protein at 26 degrees C is 10.4 ns. The backbone N-H vectors for all the measurable residues exhibit very fast motions on a time scale of less than or equal to 20 ps. The 15N relaxation data for only 14 residues can be explained by this single internal motion alone. A further 39 residues display a second motion on a time scale ranging from 28.8 ps to 3.9 ns, while another 15 residues are characterized by an additional motion on the 170-ns to 2.25-ms time scale resulting in 15N T2 exchange line broadening. There are 39 residues that exhibit both the additional 15N T2 exchange line broadening and the slow (28.8 ps-3.9 ns) internal motion. Thus, the RNase H domain experiences extensive mobility throughout its structure as evidenced by the 93 residues which exhibit multiple modes of motion. Distinctly mobile regions of the protein are identified by large decreases in the overall order parameter (S2) and correspond to the C-terminal residues and the loop regions between beta-strands beta 1 and beta 2 and between alpha-helix alpha B and beta-strand beta 4.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

利用二维反向检测异核15N-1H NMR光谱,对人免疫缺陷病毒(HIV-1)逆转录酶的均匀15N标记核糖核酸酶H(RNase H)结构域的主链动力学进行了研究。在总共134个主链酰胺基团中,获得了107个的15N T1、T2和核Overhauser增强(NOE)数据。该蛋白质在26摄氏度时的整体旋转相关时间(tau R)为10.4纳秒。所有可测量残基的主链N-H向量在小于或等于20皮秒的时间尺度上表现出非常快速的运动。仅14个残基的15N弛豫数据可仅由这种单一内部运动来解释。另外39个残基在28.8皮秒至3.9纳秒的时间尺度上表现出第二种运动,而另外15个残基的特征是在170纳秒至2.25毫秒的时间尺度上有额外运动,导致15N T2交换线加宽。有39个残基既表现出额外的15N T2交换线加宽又表现出缓慢(28.8皮秒 - 3.9纳秒)的内部运动。因此,RNase H结构域在其整个结构中经历广泛的流动性,这由93个表现出多种运动模式的残基所证明。通过整体序参数(S2)的大幅下降确定了蛋白质中明显可移动的区域,这些区域对应于C末端残基以及β链β1和β2之间以及α螺旋αB和β链β4之间的环区域。(摘要截断于250字)

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