Hee-Kyoung Lee, Yi Feng Zheng, Xiao-Yi Xiao, Mei Bai, Jun Sakakibara, Teruo Ono, Glenn D Prestwich
Index: Biochem. Biophys. Res. Commun. 315(1) , 1-9, (2004)
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Squalene epoxidase (SE) catalyzes the conversion of squalene to (3S)-2,3-oxidosqualene. Photolabeling and site-directed mutagenesis were performed on recombinant rat SE (rrSE) in order to identify the location of the substrate-binding site and the roles of key residues in catalysis. Truncated 50-kDa rrSE was purified and photoaffinity labeled by competitive SE inhibitor (Ki=18.4 microM), [(3)H]TNSA-Dza. An 8-kDa CNBr/BNPS-skatole peptide was purified and the first 24 amino acids were sequenced by Edman degradation. The sequence PASFLPPSSVNKRGVLLLGDAYNL corresponded to residues 388-411 of the full-length rat SE. Three nucleophilic residues (Lys-399, Arg-400, and Asp-407) were labeled by [(3)H]TNSA-Dza. Triple mutants were prepared in which bulky groups were used to replace the labeled charged residues. Purified mutant enzymes showed lower enzymatic activity and reduced photoaffinity labeling by [(3)H]TNSA-Dza. This constitutes the first evidence as to the identity of the substrate-binding site of SE.
Structure | Name/CAS No. | Molecular Formula | Articles |
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BNPS-SKATOLE
CAS:27933-36-4 |
C15H11BrN2O2S |
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Photoaffinity labeling of human serum vitamin D binding prot...
1991-07-30 [Biochemistry 30(30) , 7638-42, (1991)] |
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1986-04-01 [Anal. Biochem. 154(1) , 171-82, (1986)] |
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