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Journal Article

Citation

Abe I, Zheng YF, Prestwich GD. Biochemistry 1998; 37(17): 5779-5784.

Copyright

(Copyright © 1998, American Chemical Society)

DOI

10.1021/bi980366c

PMID

9558310

Abstract

A new orally active oxidosqualene:lanosterol cyclase (OSLC) inhibitor (Ro48-8071; Morand, O. H. et al. (1997) J. Lipid Res. 38, 373-390) showed potent noncompetitive inhibition of bacterial squalene:hopene cyclase (SHC) from Alicyclobacillus acidocaldarius (IC50 = 9.0 nM, KI = 6.6 nM) and OSLC (IC50 = 40 nM, KI = 22 nM for homogeneous rat liver OSLC). A tritium-labeled isotopomer (18.8 Ci/mmol) of this nonterpenoid inhibitor, which possesses a benzophenone (BP) photophore, was chemically synthesized as a photoaffinity label. Specific, efficient covalent modification of both OSLC and SHC enzymes was observed after UV irradiation at 360 nm. Labeling of both OSLC and SHC by [3H]Ro48-8071 was competitively displaced by coincubation with a 1000-fold molar excess of 18-thia-2, 3-oxidosqualene or the nonterpenoid inhibitor BIBX79. Displacement of labeling of OSLC was also achieved with the suicide substrate (3S)-29-methylidene-2,3-oxidosqualene. Thus, the nonsubstrate Ro48-8071 and both terpenoid and nonterpenoid inhibitors of these enzymes appear to share a common binding site.


Language: en

Keywords

Animals; Bacillaceae; Benzophenones; Binding, Competitive; Enzyme Inhibitors; Intramolecular Transferases; Kinetics; Lyases; Microsomes, Liver; Photoaffinity Labels; Protein Conformation; Rats; Substrate Specificity

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