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来自巴氏甲烷八叠球菌的甲醇:辅酶M甲基转移酶——游离的钴胺素(I)替代含类咕啉的亚基MtaC

Methanol:coenzyme M methyltransferase from Methanosarcina barkeri -- substitution of the corrinoid harbouring subunit MtaC by free cob(I)alamin.

作者信息

Sauer K, Thauer R K

机构信息

Max-Planck-Institut für terrestrische Mikrobiologie, Philipps- Universität, Marburg, Germany.

出版信息

Eur J Biochem. 1999 May;261(3):674-81. doi: 10.1046/j.1432-1327.1999.00355.x.

DOI:10.1046/j.1432-1327.1999.00355.x
PMID:10215883
Abstract

Methyl-coenzyme M formation from coenzyme M and methanol in Methanosarcina barkeri is catalysed by an enzyme system composed of three polypeptides MtaA, MtaB and MtaC, the latter of which harbours a corrinoid prosthetic group. We report here that MtaC can be substituted by free cob(I)alamin which is methylated with methanol in an MtaB-catalysed reaction and demethylated with coenzyme M in an MtaA-catalysed reaction. Methyl transfer from methanol to coenzyme M was found to proceed at a relatively high specific activity at micromolar concentrations of cob(I)alamin. This finding was surprising because the methylation of cob(I)alamin catalysed by MtaB alone and the demethylation of methylcob(III)alamin catalysed by MtaA alone exhibit apparent Km for cob(I)alamin and methylcob(III)alamin of above 1 mm. A possible explanation is that MtaA positively affects the MtaB catalytic efficiency and vice versa by decreasing the apparent Km for their corrinoid substrates. Activation of MtaA by MtaB was methanol-dependent. In the assay for methanol:coenzyme M methyltransferase activity cob(I)alamin could be substituted by cob(I)inamide which is devoid of the nucleotide loop. Substitution was, however, only possible when the assays were supplemented with imidazole: approximately 1 mm imidazole being required for half-maximal activity. Methylation of cob(I)inamide with methanol was found to be dependent on imidazole but not on the demethylation of methylcob(III)inamide with coenzyme M. The demethylation reaction was even inhibited by imidazole. The structure and catalytic mechanism of the MtaABC complex are compared with the cobalamin-dependent methionine synthase.

摘要

巴氏甲烷八叠球菌中辅酶M和甲醇形成甲基辅酶M的过程由一种由三种多肽MtaA、MtaB和MtaC组成的酶系统催化,其中MtaC含有一个类咕啉辅基。我们在此报告,MtaC可以被游离的钴胺素(I)替代,其在MtaB催化的反应中被甲醇甲基化,并在MtaA催化的反应中被辅酶M去甲基化。发现在微摩尔浓度的钴胺素(I)下,从甲醇到辅酶M的甲基转移以相对较高的比活性进行。这一发现令人惊讶,因为单独由MtaB催化的钴胺素(I)甲基化和单独由MtaA催化的甲基钴胺素(III)去甲基化对钴胺素(I)和甲基钴胺素(III)的表观Km值均高于1 mM。一种可能的解释是,MtaA通过降低其类咕啉底物的表观Km值对MtaB的催化效率产生正向影响,反之亦然。MtaB对MtaA的激活依赖于甲醇。在甲醇:辅酶M甲基转移酶活性测定中,钴胺素(I)可以被不含核苷酸环的钴胺素(I)酰胺替代。然而,只有当测定中补充咪唑时才可能进行替代:半最大活性大约需要1 mM咪唑。发现钴胺素(I)酰胺与甲醇的甲基化依赖于咪唑,但不依赖于甲基钴胺素(III)酰胺与辅酶M的去甲基化。去甲基化反应甚至被咪唑抑制。将MtaABC复合物的结构和催化机制与钴胺素依赖性甲硫氨酸合酶进行了比较。

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