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来自荚膜甲基球菌(巴斯德菌株)的甲烷单加氧酶羟化酶的晶体结构:对底物门控和组分相互作用的影响。

Crystal structures of the methane monooxygenase hydroxylase from Methylococcus capsulatus (Bath): implications for substrate gating and component interactions.

作者信息

Rosenzweig A C, Brandstetter H, Whittington D A, Nordlund P, Lippard S J, Frederick C A

机构信息

Department of Biological Chemistry and Molecular Pharmacology, Harvard Medical School, Boston, MA 02115, USA.

出版信息

Proteins. 1997 Oct;29(2):141-52.

PMID:9329079
Abstract

The crystal structure of the nonheme iron-containing hydroxylase component of methane monooxygenase hydroxylase (MMOH) from Methylococcus capsulatus (Bath) has been solved in two crystal forms, one of which was refined to 1.7 A resolution. The enzyme is composed of two copies each of three subunits (alpha 2 beta 2 gamma 2), and all three subunits are almost completely alpha-helical, with the exception of two beta hairpin structures in the alpha subunit. The active site of each alpha subunit contains one dinuclear iron center, housed in a four-helix bundle. The two iron atoms are octahedrally coordinated by 2 histidine and 4 glutamic acid residues as well as by a bridging hydroxide ion, a terminal water molecule, and at 4 degrees C, a bridging acetate ion, which is replaced at -160 degrees C with a bridging water molecule. Comparison of the results for two crystal forms demonstrates overall conservation and relative orientation of the domain structures. The most prominent structural differences identified between the two crystal forms is in an altered side chain conformation for Leu 110 at the active site cavity. We suggest that this residue serves as one component of a hydrophobic gate controlling access of substrates to and products from the active site. The leucine gate may be responsible for the effect of the B protein component on the reactivity of the reduced hydroxylase with dioxygen. A potential reductase binding site has been assigned based on an analysis of crystal packing in the two forms and corroborated by inhibition studies with a synthetic peptide corresponding to the proposed docking position.

摘要

来自荚膜甲基球菌(巴斯)的甲烷单加氧酶羟化酶(MMOH)的非血红素含铁羟化酶组分的晶体结构已通过两种晶体形式解析出来,其中一种已精修至1.7埃分辨率。该酶由三个亚基(α2β2γ2)各两个拷贝组成,并且所有三个亚基几乎完全是α螺旋结构,α亚基中有两个β发夹结构除外。每个α亚基的活性位点包含一个双核铁中心,位于一个四螺旋束中。两个铁原子由2个组氨酸和4个谷氨酸残基以及一个桥连氢氧根离子、一个末端水分子八面体配位,在4℃时还有一个桥连乙酸根离子,在-160℃时被一个桥连水分子取代。两种晶体形式结果的比较表明了结构域结构的总体保守性和相对取向。两种晶体形式之间最显著的结构差异在于活性位点腔中Leu 110的侧链构象改变。我们认为该残基作为疏水门控的一个组分,控制底物进入活性位点和产物从活性位点出来。亮氨酸门控可能是B蛋白组分对还原型羟化酶与双氧反应性影响的原因。基于对两种形式晶体堆积的分析确定了一个潜在的还原酶结合位点,并通过与对应于提议对接位置的合成肽的抑制研究得到证实。

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