Nitrile hydratase from Rhodococcus sp. N-771 is an alpha beta heterodimer w
ith a nonheme ferric iron in the catalytic center. In the catalytic center,
alpha Cys112 and alpha Cys114 are modified to a cysteine sulfinic acid (Cy
s-SO2H) and a cysteine sulfenic acid (Cys-SOH), respectively. To understand
the function and the biogenic mechanism of these modified residues, we rec
onstituted the nitrile hydratase from recombinant unmodified subunits. The
alpha beta complex reconstituted under argon exhibited no activity. However
, it gradually gained the enzymatic activity through aerobic incubation. ES
I-LC/MS analysis showed that the anaerobically reconstituted alpha beta com
plex did not have the modification of alpha Cys112-SO2H and aerobic incubat
ion induced the modification. The activity of the reconstituted alpha beta
complex correlated with the amount of alpha Cys112-SO2H. Furthermore, ESI-L
C/MS analyses of the tryptic digest of the reconstituted complex. removed o
f ferric iron at low pH and carboxamidomethylated without reduction, sugges
ted that alpha Cys114 is modified to Cys-SOH together with the sulfinic aci
d modification of alpha Cys112. These results suggest that alpha Cys112 and
alpha Cys114 are spontaneously oxidized to Cys-SO2H and Cys-SOH, respectiv
ely, and alpha Cys112-SO2H is responsible for the catalytic activity solely
or in combination with alpha Cys114-SOH.