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首页> 外文期刊>Biochemistry >CHARACTERIZATION OF MG2+-DEPENDENT 3'-PROCESSING ACTIVITY FOR HUMAN IMMUNODEFICIENCY VIRUS TYPE 1 INTEGRASE IN VITRO - REAL-TIME KINETIC STUDIES USING FLUORESCENCE RESONANCE ENERGY TRANSFER
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CHARACTERIZATION OF MG2+-DEPENDENT 3'-PROCESSING ACTIVITY FOR HUMAN IMMUNODEFICIENCY VIRUS TYPE 1 INTEGRASE IN VITRO - REAL-TIME KINETIC STUDIES USING FLUORESCENCE RESONANCE ENERGY TRANSFER

机译:荧光共振能量转移体外实时运动学研究人免疫缺陷病毒1型整合酶MG2 +依赖性3'加工活性

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摘要

Human immunodeficiency virus type 1 integrase (HIV-1 IN) catalyzes the integration of HIV-1 DNA into the host chromosome. In vitro reactions with endogenous viral DNA require Mg2+ as the metal cofactor, whereas in vitro studies performed with short oligonucleotide substrates utilize Mn2+. In this study, we report that the donor processing activity of HIV-1 IN alters depending on the structure and length of the oligonucleotide substrates. Increases in the length of the substrate cause alterations in the efficiency of Mg2+-dependent donor processing activity, thereby reconciling this discrepancy between the in vivo and in vitro HIV-1 IN mediated reactions. We have also found that the 3'-processing activity of HIV-IN is responsible for cleaving the junction between the viral and target sequences of the recombination intermediate. Its mechanism differs from the previously described disintegration reaction in that the donor strands are regenerated without a joining reaction of the target strands. Kinetic studies of 3'-processing activity suggest that the k(cat) (0.24/h) is very low. This implies that HIV-1 IN remains as a complex with the processed DNA prior to the strand transfer reaction.
机译:人类免疫缺陷病毒1型整合酶(HIV-1 IN)催化HIV-1 DNA整合入宿主染色体。与内源性病毒DNA的体外反应需要Mg2 +作为金属辅因子,而使用短寡核苷酸底物进行的体外研究则利用Mn2 +。在这项研究中,我们报告说,HIV-1 IN的供体加工活性根据寡核苷酸底物的结构和长度而改变。底物长度的增加导致Mg2 +依赖性供体加工活性效率的改变,从而调和了体内和体外HIV-1 IN介导的反应之间的这种差异。我们还发现,HIV-IN的3'加工活性负责裂解重组中间体的病毒和靶序列之间的连接。其机理与先前描述的崩解反应的不同之处在于,供体链在没有靶链的连接反应的情况下得以再生。 3'加工活性的动力学研究表明k(cat)(0.24 / h)非常低。这意味着在链转移反应之前,HIV-1 IN与加工过的DNA保持为复合物。

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