Investigation of NADPH and acyl-binding sites on avian fatty acid synthase
- 8 June 1982
- journal article
- research article
- Published by American Chemical Society (ACS) in Biochemistry
- Vol. 21 (12), 2863-2870
- https://doi.org/10.1021/bi00541a009
Abstract
The binding of reduced NADPH to chicken liver fatty acid synthase was studied by using both fluorescence titrations and the direct bindng method of forced dialysis. Four apparently identical sites are found per enzyme molecule, with an intrinsic Kd of 0.6 .mu.M at pH 7.0, 23.degree. C. The acyl-binding sites on the enzyme were studied with a fluorescent analog of acetyl-CoA, .beta.-[N-(7-nitro-2,1,3-benzoxadiazol-4-yl)]alanyl CoA (NBDA-CoA). The enzyme slowly transfers NBDA to acyl-binding sites. Analysis of the kinetics of binding and of the stability and hydroxylamine sensitivity of the acyl-enzyme at pH 7.5 suggests that binding occurs predominantly at 2 classes of SH sites, with 2 sites of each class per enzyme molecule. Up to 1 NBDA/enzyme molecule is bound to a nonsulfhydryl site after overnight incubation of enzyme with NBDA-CoA. The acyl linkage at one class of SH sites appears to be hydrolyzed by the thioesterase activity of the enzyme. This hydrolysis can be prevented by modifying the enzyme with tosyl fluoride. The binding of NBDA is inhibited by acetyl-CoA, malonyl-CoA, and NADPH. The NBDA-enzyme adduct is inactive, although activity can be partially restored by incubation at 35.degree. C. The binding of NADPH to the enzyme is not significantly altered by the binding of NBDA. Fluorescence resonance energy transfer between enzyme-bound NADPH and enzyme-bound NBDA suggests that the acyl-binding sites are 30-40 .ANG. from the NADPH-binding sites. This distance can only be defined approximately because of the presence of multiple energy donors and acceptors and the uncertainty in the dipole-dipole orientations of the energy acceptors and donors.This publication has 14 references indexed in Scilit:
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