Quantification of coenzyme F420analogues from methanogenic bacteria by HPLC and fluorimetry

An improved method for separating analogues of coenzyme F420 by isocratic reversed-phase high performance liquid chromatography is described. The method offers improved resolution, shorter chromatography runs and requires less complex apparatus.

Quantification of coenzymes and related compounds from methanogens was performed in extracts obtained from whole cells with aqueous ethanol at 80°C. By means of high-performance liquid chromatography the following compounds could be detected and quantified in extracts from Methanobacterium thermoaut

1. Introduction. the hydrocorphinoid nickel complex 1 (F430) [l] is the cofactor of methyl-coenzyme M reductase which catalyzes the last step of methane formation in methanogenic bacteria according to Scheme l a . The mechanism by which the enzyme

## Abstract A methylnickel(II) derivative of coenzyme F430 (1) was proposed as an intermediate in the enzymic process catalyzed by methyl‐CoM reductasc. Indirect evidence points to formation of CH~3~–F430M^II^ in the reaction of F30M^1^ (obtained from F430M^II^ (2)) with eleclrophilic methyl donors

## ~ ~~ F430M, the pentamethyl ester of coenzyme F430, can be oxidized reversibly by one electron. The oxidation potential has been determined, and the electrolytically prepared oxidation product was characterized by its UVjVIS and ESR spectrum. The strongly anisotropic and nearly axial ESR spectr