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硬脂酸与牛血清白蛋白结合的电子自旋共振研究。

ESR studies of stearic acid binding to bovine serum albumin.

作者信息

Ge M T, Rananavare S B, Freed J H

机构信息

Department of Chemistry, Baker Laboratory, Cornell University, Ithaca, NY 14853.

出版信息

Biochim Biophys Acta. 1990 Dec 6;1036(3):228-36. doi: 10.1016/0304-4165(90)90039-y.

DOI:10.1016/0304-4165(90)90039-y
PMID:2175216
Abstract

The ESR spectra of a series of chain-labelled doxyl stearic acids (5-, 7-, 12- and 16-DSA) and doxyl methyl stearates (5-, 7-, 12- and 16-DMS) bound to the high-affinity binding sites of bovine serum albumin (BSA) have been analyzed using nonlinear least-squares fitting of slow-motional ESR stimulation. The motional analysis reveals that the rotational diffusion of these stearates around the axis perpendicular to the long hydrocarbon chain is greatly hindered, suggesting that they are held tightly in a channel of the protein. Comparison of the isotropic hyperfine splitting, A0, among each series shows that 5- and 16-DSA and 16-DMS have larger A0 values than the other spin labels. In addition, labels at the 16-C position of both DSA and DMS exhibit significantly increased motion relative to the other positions. These observations suggest that the channel starts at 5-C of the chain and ends somewhere between 13-C and 15-C, leading to an estimate of 11 +/- 1 A for the length of the channel. The methyl stearate labels exhibit significantly faster rotation around the chain axis than the analogous stearic acid labels, suggesting a double hydrogen-bonding mechanism for fatty acid binding to BSA. The ability of the acid to form two hydrogen bonds apparently fixes it more rigidly in the protein, preventing rotation about either single hydrogen bond. A double-hydrogen bonding mechanism is most consistent with the formation of a salt bridge between the negatively charged carboxylate of the acid and either a positively charged guanidino group of arginine, or the positively charged omega-amino groups of two lysine residues. An ESR study of the pH dependence of DSA binding indicates that salt bridge formation with lysine is responsible for at least some of the long chain fatty acid binding sites of BSA.

摘要

通过对慢运动电子自旋共振(ESR)刺激进行非线性最小二乘法拟合,分析了一系列与牛血清白蛋白(BSA)高亲和力结合位点结合的链标记硬脂酸多昔(5-、7-、12-和16-DSA)和硬脂酸甲酯多昔(5-、7-、12-和16-DMS)的ESR谱。运动分析表明,这些硬脂酸盐围绕垂直于长烃链的轴的旋转扩散受到极大阻碍,这表明它们被紧密地固定在蛋白质的通道中。每个系列中各向同性超精细分裂A0的比较表明,5-和16-DSA以及16-DMS的A0值比其他自旋标记物的A0值更大。此外,DSA和DMS的16-C位置的标记相对于其他位置表现出显著增加的运动。这些观察结果表明,通道从链的5-C开始,在13-C和15-C之间的某个位置结束,由此估计通道长度为11±1埃。硬脂酸甲酯标记物围绕链轴的旋转明显比类似的硬脂酸标记物快,这表明脂肪酸与BSA结合存在双氢键机制。酸形成两个氢键的能力显然使其在蛋白质中固定得更牢固,阻止了围绕任何一个单氢键的旋转。双氢键机制与酸带负电荷的羧酸盐与精氨酸带正电荷的胍基或两个赖氨酸残基带正电荷的ω-氨基之间形成盐桥最为一致。对DSA结合的pH依赖性的ESR研究表明,与赖氨酸形成盐桥至少是BSA一些长链脂肪酸结合位点的原因。

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