Role of the proximal ligand in peroxidase catalysis. Crystallographic, kinetic, and spectral studies of cytochrome c peroxidase proximal ligand mutants.

K Choudhury,M Sundaramoorthy,A Hickman,T Yonetani,E Woehl,M.F Dunn,T.L Poulos

doi:10.1016/s0021-9258(17)31982-8

K Choudhury, M Sundaramoorthy + Show 5 more

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https://doi.org/10.1016/s0021-9258(17)31982-8

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Abstract

The role of the proximal histidine ligand in peroxidase function was studied by replacing the His side chain in cytochrome c peroxidase with Gln, Glu, or Cys. In addition, a double mutant was prepared where His-175 is converted to Gln and the site of free radical formation in Compound I, Trp-191 (Sivaraja, M., Goodin, D.B., Smith, M., and Hoffman, B. M. (1989) Science 245, 738-740), is converted to Phe. With the exception of the His-175-->Cys mutant, the proximal ligand mutants retain high levels of enzyme activity. Stopped flow studies show that replacing the His ligand with Gln has only a modest effect on the rate of Compound I formation demonstrating that the precise nature of the proximal ligand is not important in achieving a high rate of peroxide O-O bond cleavage. The double mutant, His-175-->Gln/Trp-191-->Phe, also forms Compound I rapidly but the initial product formed is very likely a long-lived porphyrin pi cation radical that slowly converts to a species more closely resembling the heme oxyferryl center of wild type Compound I. The relevance of these studies to the cytochrome c peroxidase-cytochrome c electron transfer system are discussed.

Highlights

The Glu-175 and Gln-175 side chains adopt slightly proximal ligand mutants exhibit a large decrease in the Soret different conformations,but both are close to the iron atom, 2.0 maximum indicating loss of heme or significant destabilization
With CCP, the His-175 + Cys mutant exhibits a Soret band nea3r 96 nm immediately after the apoenzyme is reconstituted with heme, but within several minutes this band shifts to400 nm
There is a slight increase in activity concomitantwith the spectral shift which plateaus at about 7% wild type activity

Summary

Present address

Pharmaceutical, 3401 Hillview Ave., Palo Alto, CA 94303, of Maryland) which has a mechanism for deleting uracil-encodedDNA. The efficiency of mutagenesis was about 80%.The His-175 + Gln and His-175 + Gln/Trp-lgl + Phe mutants were prepared according to Sundaramoorthy et al (1991)and Choudhuryet al. Bakers’ yeast CCP differs in sequencefrom the laboratory yeast strain used to construct our expression system at 2 amino acid positions: 53 and 152. Bakers’yeast CCP contains Thr andAsp at positions 53 and 152 (Takioet al., 1980),respectively, whilethe yeast strain has Ile and Gly at these positions (Kaput et al, 1982).

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1.87 A resolution

RESULTS

I I II

DISCUSSION