4.5 Article

Functional definition of the tobacco protoporphyrinogen IX oxidase substrate-binding site

Journal

BIOCHEMICAL JOURNAL
Volume 402, Issue -, Pages 575-580

Publisher

PORTLAND PRESS LTD
DOI: 10.1042/BJ20061321

Keywords

enzyme kinetics; haem biosynthesis; protoporphyrin; protoporphyrinogen IX oxidase; stopped-flow fluorescence; variegate porphyria

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PPO (protoporphyrinogen IX oxidase) catalyses the flavin-dependent six-electron oxidation of protogen (protoporphyrinogen IX) to form proto (protoporphyrin IX), a crucial step in haem and chlorophyll biosynthesis. The apparent K value for wild-type tobacco PPO2 (mitochondrial PPO) was 1.17 mu M, with a V-max of 4.27 mu M center dot min(-1) center dot mg(-1) and a catalytic activity k(cat) of 6.0 s(-1). Amino acid residues that appear important for substrate binding in a crystal structure-based model of the substrate docked in the active site were interrogated by site-directed mutagenesis. PPO2 variant F392H did not reveal detectable enzyme activity indicating an important role of Phe(392) in substrate ring A stacking. Mutations of Leu(356), Leu(372) and Arg(98) increased k(cat) values up to 100-fold, indicating that the native residues are not essential for establishing an orientation of the substrate conductive to catalysis. Increased K values of these PPO2 variants from 2- to 100-fold suggest that these residues are involved in, but not essential to, substrate binding via rings B and C. Moreover, one prominent structural constellation of human PPO causing the disease variegate porphyria (N67W/S374D) was successfully transferred into the tobacco PPO2 background. Therefore tobacco PPO2 represents a useful model system for the understanding of the structure-function relationship underlying detrimental human enzyme defects.

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