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Dimers and Trimers of Chondroitin in Molecular Docking of Bovine Testicular Hyaluronidase

机译:牛睾丸透明质酸酶分子对接中软骨素的二聚体和三聚体

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摘要

Molecular docking of a 3D model of bovine testicular hyaluronidase was performed with dimers and trimers of chondroitin. On the molecular surface of a hyaluronidase globule, eight sites for ligand binding were established. Sites 6, 3, and 1 of the enzyme structure were found to be the most important sites since chondroitin binding therewith distorts the protein 3D structure. The interactions of enzyme structure with chondroitin ligands are mainly determined by electrostatic forces. For free hyaluronidase molecule (without ligands) at temperatures above 300 K conformational transfers leading to the enzyme inactivation were noted. The inactivation was mainly manifested through irreversible attraction of the protein fragment surrounding the Glu-105 residue and the one between Arg-59 and Arg-96, where a temperature decrease did not induce the restoration of the initial view of 3D structure of the enzyme molecule. Binding of chondroitin ligands to the enzyme structure at positions 6, 3, and 1 increased its denaturation temperature by approximately 10 degrees. The most significant effect of enzyme structure stabilization was provided by chondroitin ligand binding with hyaluronidase at site 6. This effect of protein structure stabilization exceeded the one of chondroitin sulfate trimers against the enzyme inhibition by heparin tetramers, which required binding of four to five chondroitin sulfate ligands on the molecular surface of the enzyme.
机译:用软骨素的二聚体和三聚体进行牛睾丸透明质酸酶3D模型的分子对接。在透明质酸酶小球的分子表面上,建立了8个配体结合的8位点。发现酶结构的遗址6,3和1是最重要的位点,因为蛋白质3D结构扭曲了蛋白质3D结构。酶结构与软骨素配体的相互作用主要由静态力决定。对于游离的透明质酸酶分子(无配体)在300k以上的温度下,注意到导致酶失活的一致转移。灭活主要是通过围绕Glu-105残基的蛋白质片段的不可逆吸引和Arg-59和Arg-96之间的不可逆吸引,其中温度降低未诱导酶分子的3D结构的初始视图恢复。软骨素配体与酶结构的结合在6,3和1的位置,增加其变性温度约10度。酶结构稳定化的最显着效果是在部位的透明质酸酶的含有酸软配体的情况下提供的。这种蛋白质结构稳定的这种效果超过了肝素四聚体抑制酶抑制的软骨素抑制剂中的一种,这需要硫酸四到五个软骨素的结合所需的结合在酶的分子表面上的配体。

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