We report an extensive advanced paramagnetic resonance
characterization of the mixed-valence dinuclear
Fe center of methane monooxygenase hydroxylase (MMOHmv)
from Methylococcus capsulatus (Mc) (Bath) and
of
binding to it by the exogenous ligand DMSO. We employ continuous
wave and pulsed electron nuclear double
resonance (ENDOR) spectroscopy, both at Q-band microwave frequencies,
to examine 14,15N, 1,2H, 13C, and
57Fe
nuclei. Preliminary 1H ENDOR results were communicated
previously (DeRose, V. J.; Liu, K. E.; Hoffman,
B.
M.; Lippard, S. J. J. Am. Chem. Soc.
1993,
115, 6440−6441). ENDOR-derived 14,15N
hyperfine tensors are interpreted
in terms of the spin distribution on histidyl ligands bound to the
dinuclear center. Determination of the 57Fe
hyperfine
tensors gives a complete picture of the spin-coupled Fe2+
and Fe3+ ions. The 1,2H ENDOR results
disclose the
presence of a bridging hydroxide and an aqua ligand in both native and
DMSO-treated enzyme. A novel procedure
for describing the 1H hyperfine tensor of the bridge gives
the orientation of the g-tensor relative to the cluster
framework
in both enzyme forms, information that is normally obtained only from
full single-crystal EPR studies. DMSO is
found to cause small perturbations of both histidyl ligands, and little
change in the 57Fe hyperfine tensors.
However,
Q-band pulsed 2H and 13C ENDOR measurements of
labeled DMSO show that this exogenous ligand binds in a
distinct site with a well-ordered structure, and further indicate that
it is O-bound to the Fe3+ ion of the mixed-valence cluster. The analysis, coupled with 2H X-band
electron spin−echo envelope modulation data, places
limitations
on the possible orientation of the bound DMSO. These geometric
restrictions have been used to guide molecular
modeling of DMSO bound to the MMOHmv diiron active site.
The results reported here provide a basis with which
to study other dinuclear Fe−carboxylate proteins.
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