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首页> 外文期刊>Virology >Mutagenesis of the dimer interface residues of tethered and untethered HIV-1 protease result in differential activity and suggest multiple mechanisms of compensation.
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Mutagenesis of the dimer interface residues of tethered and untethered HIV-1 protease result in differential activity and suggest multiple mechanisms of compensation.

机译:系留和未系留的HIV-1蛋白酶二聚体界面残基的诱变导致活性差异,并提示多种补偿机制。

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摘要

As is the case for all retroviruses, the protease of HIV-1 is only functional as a homodimer; dimerization of two protease monomers results in the formation of the enzyme active site. This dimer structure is supported primarily by interactions between the first four amino-terminal and the last four carboxy-terminal amino acids. These eight amino acids form a beta-sheet in which hydrophobic residues are oriented towards the core of the molecule and polar residues are directed towards the solvent. Although the structure of the dimer interface has been determined, the forces that support dimerization have not been fully characterized. Here, we describe a tethered construct in which two protease monomers are joined by a 5 amino acid linker. We evaluate the relative role of each dimer interface residue in functional homo- and heterodimers. Our studies indicate that the hydrophobic residues of the dimer interface are particularly important in maintaining enzyme activity and that enzyme activity is more sensitive to substitutions of the C-terminal amino acids. Further, we demonstrate that the presence of the tether is able to compensate for mutations within the dimer interface that inactivate the enzyme.
机译:与所有逆转录病毒一样,HIV-1的蛋白酶仅起同型二聚体的作用。两种蛋白酶单体的二聚化导致酶活性位点的形成。该二聚体结构主要由前四个氨基末端氨基酸和后四个羧基末端氨基酸之间的相互作用支持。这八个氨基酸形成一个β-折叠,其中疏水残基指向分子的核心,极性残基指向溶剂。尽管已经确定了二聚体界面的结构,但尚未完全表征支持二聚化的力。在这里,我们描述了其中两个蛋白酶单体通过一个5个氨基酸的接头相连的拴系结构。我们评估功能同型和异型二聚体中每个二聚体界面残基的相对作用。我们的研究表明,二聚体界面的疏水残基在维持酶活性方面特别重要,并且酶活性对C端氨基酸的取代更敏感。此外,我们证明系链的存在能够补偿使酶失活的二聚体界面内的突变。

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