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黄绿原矛头蝮蛇(哈布蛇)毒液中磷脂酶A2的晶体结构分析,分辨率为1.5埃

Crystal structure analysis of phospholipase A2 from trimeresurus flavoviridis (Habu snake) venom at 1.5 A resolution.

作者信息

Suzuki A, Matsueda E, Yamane T, Ashida T, Kihara H, Ohno M

机构信息

Department of Biotechnology, School of Engineering, Nagoya University, Aichi.

出版信息

J Biochem. 1995 Apr;117(4):730-40. doi: 10.1093/oxfordjournals.jbchem.a124770.

Abstract

The crystal structure of dimeric phospholipase A2 (PLA2) from the venom of Habu snake, Trimeresurus flavoviridis, has been determined by the molecular replacement method, and has been refined at 1.5 A resolution to an R-factor of 0.175. In the crystal, T. flavoviridis PLA2 forms a dimer using two 14 kDa subunits related by a pseudo 2-fold axis. Along the axis, the dimer has a narrow channel passing through it. Although no calcium ion is present in the calcium binding site, the peptide-chain folding of the subunits, the conformation of the catalytic residues, and the hydrogen-bonding network around the active sites are almost identical to those of the group I/II monomeric or dimeric PLA2s. The catalytic residues in both subunits are buried in the interior of the dimer and are inaccessible to substrate from the bulk solvent. In addition, the subunits of the dimer interact with each other at the hydrophobic region of the molecular surface where the entrance to the active site opens and where PLA2 is presumed to interact with the phospholipid of the substrate. Therefore, it is inferred that dimerization of T. flavoviridis PLA2 is the result of free-energy minimization by excluding the hydrophobic molecular surface from the aqueous solvent, rather than being required for the enzymatic function.

摘要

通过分子置换法测定了来自蝮蛇(竹叶青蛇)毒液的二聚体磷脂酶A2(PLA2)的晶体结构,并在1.5埃分辨率下进行了精修,R因子为0.175。在晶体中,竹叶青蛇PLA2利用两个通过伪二次轴相关的14 kDa亚基形成二聚体。沿着该轴,二聚体有一个狭窄的通道贯穿其中。尽管在钙结合位点不存在钙离子,但亚基的肽链折叠、催化残基的构象以及活性位点周围的氢键网络与I/II组单体或二聚体PLA2几乎相同。两个亚基中的催化残基都埋藏在二聚体内部,从本体溶剂中无法接触到底物。此外,二聚体的亚基在分子表面的疏水区域相互作用,该区域是活性位点的入口处,也是PLA2推测与底物磷脂相互作用的地方。因此,推断竹叶青蛇PLA2的二聚化是通过将疏水分子表面排除在水性溶剂之外使自由能最小化的结果,而不是酶功能所必需的。

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