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超长链脂肪酰辅酶A酯与过氧化物酶体非特异性脂质转运蛋白(固醇载体蛋白-2)的高亲和力结合。

High-affinity binding of very-long-chain fatty acyl-CoA esters to the peroxisomal non-specific lipid-transfer protein (sterol carrier protein-2).

作者信息

Dansen T B, Westerman J, Wouters F S, Wanders R J, van Hoek A, Gadella T W, Wirtz K W

机构信息

Centre for Biomembranes and Lipid Enzymology, Institute of Biomembranes, Utrecht University, Padualaan 8, 3584 CH Utrecht, The Netherlands.

出版信息

Biochem J. 1999 Apr 1;339 ( Pt 1)(Pt 1):193-9.

Abstract

Binding of fluorescent fatty acids to bovine liver non-specific lipid-transfer protein (nsL-TP) was assessed by measuring fluorescence resonance energy transfer (FRET) between the single tryptophan residue of nsL-TP and the fluorophore. Upon addition of pyrene dodecanoic acid (Pyr-C12) and cis-parinaric acid to nsL-TP, FRET was observed indicating that these fatty acids were accommodated in the lipid binding site closely positioned to the tryptophan residue. Substantial binding was observed only when these fatty acids were presented in the monomeric form complexed to beta-cyclodextrin. As shown by time-resolved fluorescence measurements, translocation of Pyr-C12 from the Pyr-C12-beta-cyclodextrin complex to nsL-TP changed dramatically the direct molecular environment of the pyrene moiety: i.e. the fluorescence lifetime of the directly excited pyrene increased at least by 25% and a distinct rotational correlation time of 7 ns was observed. In order to evaluate the affinity of nsL-TP for intermediates of the beta-oxidation pathway, a binding assay was developed based on the ability of fatty acyl derivatives to displace Pyr-C12 from the lipid binding site as reflected by the reduction of FRET. Hexadecanoyl-CoA and 2-hexadecenoyl-CoA were found to bind readily to nsL-TP, whereas 3-hydroxyhexadecanoyl-CoA and 3-ketohexadecanoyl-CoA bound poorly. The highest affinities were observed for the very-long-chain fatty acyl-CoA esters (24:0-CoA, 26:0-CoA) and their enoyl derivatives (24:1-CoA, 26:1-CoA). Binding of non-esterified hexadecanoic acid and tetracosanoic acid (24:0) was negligible.

摘要

通过测量非特异性脂质转运蛋白(nsL-TP)的单个色氨酸残基与荧光团之间的荧光共振能量转移(FRET),评估了荧光脂肪酸与牛肝非特异性脂质转运蛋白(nsL-TP)的结合情况。向nsL-TP中添加芘十二烷酸(Pyr-C12)和顺式-十八碳四烯酸后,观察到FRET,表明这些脂肪酸被容纳在与色氨酸残基紧密相邻的脂质结合位点中。仅当这些脂肪酸以与β-环糊精复合的单体形式存在时,才观察到大量结合。如时间分辨荧光测量所示,Pyr-C12从Pyr-C12-β-环糊精复合物向nsL-TP的转移极大地改变了芘部分的直接分子环境:即直接激发的芘的荧光寿命至少增加了25%,并观察到明显的7 ns旋转相关时间。为了评估nsL-TP对β-氧化途径中间体的亲和力,基于脂肪酰基衍生物从脂质结合位点取代Pyr-C12的能力(通过FRET的降低反映)开发了一种结合测定法。发现十六烷酰辅酶A和2-十六碳烯酰辅酶A很容易与nsL-TP结合,而3-羟基十六烷酰辅酶A和3-酮基十六烷酰辅酶A结合较差。观察到超长链脂肪酰辅酶A酯(24:0-CoA、26:0-CoA)及其烯酰衍生物(24:1-CoA、26:1-CoA)具有最高的亲和力。未酯化的十六烷酸和二十四烷酸(24:0)的结合可忽略不计。

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