Purification and characterization of the respiratory arsenate reductase of Chrysiogenes arsenatis

Chrysiogenes arsenatis is the only bacterium known that respires anaerobically using arsenate as the terminal electron acceptor and the respiratory substrate acetate as the electron donor. During growth, the arsenate is reduced to arsenite; the reduction is catalyzed by an arsenate reductase. This study describes the purification and characterization of a respiratory arsenate reductase (Arr). The enzyme consists of two subunits with molecular masses of 87 kDa (ArrA) and 29 kDa (ArrB), and is a heterodimer alpha(1)beta(1) with a native molecular mass of 123 kDa, The arsenate reductase contains molybdenum, iron, acid-labile sulfur and zinc as cofactor constituents. The K-m of the enzyme for arsenate is 0.3 mM and the V-max is 7013 mu mol arsenate reduced.min(-1).mg protein(-1). Nitrate, sulfate, selenate and fumarate cannot serve as alternative electron accepters for the arsenate reductase. Synthesis of the protein is regulated, as arsenate must be present during growth for the enzyme to be fully induced. The N-terminus of ArrA is similar to a number of procaryotic molybdenum-containing polypeptides (e.g. the formate dehydrogenases H and N of Escherichia coli). The N-terminus of ArrB is similar to iron-sulfur proteins. The respiratory arsenate reductase of C. arsenatis is different from the non-respiratory arsenate reductases of E, coli and Staphylococcus aureus.