Molecular Properties of the Dissimilatory Sulfite Reductase from Desulfovibrio Desulfuricans (Essex) and Comparison with the Enzyme from Desulfovibrio Vulgaris (Hildenborough)

Abstract

The dissimilatory sulfite reductase desulfoviridin was purified from the membrane (mSiR) and the soluble fraction (sSiR) of the sulfate‐reducing bacterium Desulfovibrio desulfuricans (Essex). Molecular and spectroscopic properties were determined and compared with the properties of the soluble desulfoviridin from Desulfovibrio vulgaris (Hildenborough). The enzymes were isolated as α2β2γn (n=1–3) multimers with a relative molecular mass of 200±10 (gel filtration). Both mSiR and sSiR from D. desulfuricans contained 24±3 Fe and 18±3 labile sulfide/200 kDa, respectively, and showed identical EPR spectra. Quantification of the high‐spin Fe(III) heme resonances at g of approximately 6 indicated that close to 80% of the siroheme moiety in the enzyme from D. desulfuricans was demetallated. D. desulfuricans sulfite reductase showed S=9/2 EPR signals with the highest apparent g value at g=17 as reported for SiR from D. vulgaris. Antibodies raised against the α, β and γ subunit of the D. vulgaris enzyme exhibited cross‐reactivity with the subunits of mSiR and sSiR from D. desulfuricans. N‐terminal sequences of α, β and γ subunits of both mSiR and sSiR from D. desulfuricans were identical and showed a high degree of similarity with the sequences of the corresponding subunits obtained from the D. vulgaris enzyme. During gel filtration of sSiR from D. desulfuricans, under non‐denaturing conditions, a small protein (molecular mass ≈ 11 kDa) was separated. This 11‐kDa protein exhibited cross‐reactivity with the antibody raised against the γ subunit of D. vulgaris sulfite reductase. In the case of D. desulfuricans sulfite reductase, the 11‐kDa γ subunit seems not to be an integral part of the protein and can be obtained from the soluble fraction and during purification of the soluble enzyme. Copyright © 1995, Wiley Blackwell. All rights reserved