Clustered Genes Encoding the Methyltransferases of Methanogenesis from Monomethylamine

Author:

Burke Stephen A.1,Lo Sam L.1,Krzycki Joseph A.1

Affiliation:

1. Department of Microbiology, Ohio State University, Columbus, Ohio 43210

Abstract

ABSTRACT Coenzyme M (CoM) is methylated during methanogenesis from monomethyamine in a reaction catalyzed by three proteins. Using monomethylamine, a 52-kDa polypeptide termed monomethylamine methyltransferase (MMAMT) methylates the corrinoid cofactor bound to a second polypeptide, monomethylamine corrinoid protein (MMCP). Methylated MMCP then serves as a substrate for MT2-A, which methylates CoM. The genes for these proteins are clustered on 6.8 kb of DNA in Methanosarcina barkeri MS. The gene encoding MMCP ( mtmC ) is located directly upstream of the gene encoding MMAMT ( mtmB ). The gene encoding MT2-A ( mtbA ) was found 1.1 kb upstream of mtmC , but no obvious open reading frame was found in the intergenic region between mtbA and mtmC . A single monocistronic transcript was found for mtbA that initiated 76 bp from the translational start. Separate transcripts of 2.4 and 4.7 kb were detected, both of which carried mtmCB . The larger transcript also encoded mtmP , which is homologous to the APC family of cationic amine permeases and may therefore encode a methylamine permease. A single transcriptional start site was found 447 bp upstream of the translational start of mtmC . MtmC possesses the corrinoid binding motif found in corrinoid proteins involved in dimethylsulfide- and methanol-dependent methanogenesis, as well as in methionine synthase. The open reading frame of mtmB was interrupted by a single in-frame, midframe, UAG codon which was also found in mtmB from M. barkeri NIH. A mechanism that circumvents UAG-directed termination of translation must operate during expression of mtmB in this methanogen.

Publisher

American Society for Microbiology

Subject

Molecular Biology,Microbiology

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