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HIV-1逆转录酶与模型RNA-DNA双链体的相互作用。

HIV-1 reverse transcriptase interaction with model RNA-DNA duplexes.

作者信息

Gorshkova I I, Rausch J W, Le Grice S F, Crouch R J

机构信息

Laboratory of Molecular Genetics, National Institute of Child Health and Human Development, NIH, Bethesda, Maryland 20892, USA.

出版信息

Anal Biochem. 2001 Apr 15;291(2):198-206. doi: 10.1006/abio.2001.5053.

DOI:10.1006/abio.2001.5053
PMID:11401293
Abstract

HIV-1 reverse transcriptase (HIV-1 RT) is a multifunctional enzyme responsible for converting viral RNA into preintegrative DNA during the early stages of viral infection. DNA polymerase and RNase H activities are required, and several conformationally distinct primer-templates must be accommodated by the enzyme during the process. Parameters of interaction between model substrates (ligands) and HIV-1 RT (wild type p66/p51 and the RNase H-deficient mutant p66(E478Q)/p51) (analytes) were estimated by surface plasmon resonance at 25 degrees C, pH 8.0. Binding of RT to the ligands is specific and can be analyzed using a conventional 1:1 binding algorithm. RNA-DNA hybrids with 5'-template overhangs of 6 and 12 nucleotides bind to RT approximately one order of magnitude stronger than the corresponding 36-mer with blunt ends due to slower dissociation. Immobilization of the latter through either the 5'-end of RNA or DNA strand does not change the equilibrium constant (K(D)) for wild-type RT but the values of kinetic constants of association and dissociation differ significantly. For the p66(E478Q)/p51 enzyme, orientation effects are notable even altering the K(D) value. Binding of the p66(E478Q)/p51 to any RNA-DNA hybrids is slightly stronger compared with wild type. Data can be interpreted in terms of the mechanism of reverse transcription.

摘要

HIV-1逆转录酶(HIV-1 RT)是一种多功能酶,在病毒感染早期负责将病毒RNA转化为整合前DNA。这一过程需要DNA聚合酶和核糖核酸酶H的活性,并且该酶在过程中必须适应几种构象不同的引物模板。在25摄氏度、pH 8.0条件下,通过表面等离子体共振估计了模型底物(配体)与HIV-1 RT(野生型p66/p51和核糖核酸酶H缺陷型突变体p66(E478Q)/p51)(分析物)之间的相互作用参数。RT与配体的结合具有特异性,可使用传统的1:1结合算法进行分析。由于解离较慢,具有6个和12个核苷酸5'模板突出端的RNA-DNA杂交体与RT的结合力比相应的平端36聚体强约一个数量级。通过RNA或DNA链的5'端固定后者不会改变野生型RT的平衡常数(K(D)),但结合和解离的动力学常数的值有显著差异。对于p66(E478Q)/p51酶,方向效应很明显,甚至会改变K(D)值。与野生型相比,p66(E478Q)/p51与任何RNA-DNA杂交体的结合略强。数据可以根据逆转录机制进行解释。

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