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通过表面等离子体共振方法评估未修饰天然脂质的脂质转移蛋白结合情况。

Lipid transfer protein binding of unmodified natural lipids as assessed by surface plasmon resonance methodology.

作者信息

Kernstock Robert M, Girotti Albert W

机构信息

Department of Biochemistry, Medical College of Wisconsin, Milwaukee WI 53226, USA.

出版信息

Anal Biochem. 2007 Jun 1;365(1):111-21. doi: 10.1016/j.ab.2007.02.018. Epub 2007 Feb 22.

DOI:10.1016/j.ab.2007.02.018
PMID:17376396
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1975857/
Abstract

A new approach for analyzing lipid-lipid transfer protein interactions is described. The transfer protein is genetically engineered for expression with a C-terminal biotinylated peptide extension (AviTag). This allows protein anchoring to a streptavidin-coated chip for surface plasmon resonance (SPR)-based assessment of lipid binding. Sterol carrier protein-2 (SCP-2), involved in the intracellular trafficking of cholesterol, fatty acids, and other lipids, was selected as the prototype. Biotinylated SCP-2 (bSCP-2) was expressed in Escherichia coli, purified to homogeneity by mutated streptavidin (SoftLink) affinity chromatography, and confirmed by mass spectrometry to contain one biotin group at the expected position. Intermembrane [(14)C]cholesterol transfer was strongly enhanced by bSCP-2, demonstrating that it was functional. Using bSCP-2 immobilized on a Biacore streptavidin chip, we determined on- and off-rate constants along with equilibrium dissociation constants for the following analytes: oleic acid, linoleic acid, cholesterol, and fluorophore (NBD)-derivatized cholesterol. The dissociation constant for NBD-cholesterol was similar to that determined by fluorescence titration for SCP-2 in solution, thereby validating the SPR approach. This method can be readily adapted to other transfer proteins and has several advantages over existing techniques for measuring lipid binding, including (i) the ability to study lipids in their natural states (i.e., without relatively large reporter groups) and (ii) the ability to measure on- and off- rate constants as well as equilibrium constants.

摘要

本文描述了一种分析脂质 - 脂质转移蛋白相互作用的新方法。将转移蛋白进行基因工程改造,使其表达带有C末端生物素化肽延伸(AviTag)的蛋白。这使得蛋白能够锚定到链霉亲和素包被的芯片上,用于基于表面等离子体共振(SPR)的脂质结合评估。选择参与胆固醇、脂肪酸和其他脂质细胞内运输的固醇载体蛋白2(SCP - 2)作为原型。生物素化的SCP - 2(bSCP - 2)在大肠杆菌中表达,通过突变链霉亲和素(SoftLink)亲和色谱法纯化至同质,并通过质谱确认在预期位置含有一个生物素基团。膜间[(14)C]胆固醇转移被bSCP - 2强烈增强,表明其具有功能。使用固定在Biacore链霉亲和素芯片上的bSCP - 2,我们测定了以下分析物的结合和解离速率常数以及平衡解离常数:油酸、亚油酸、胆固醇和荧光团(NBD)衍生的胆固醇。NBD - 胆固醇的解离常数与溶液中SCP - 2荧光滴定法测定的结果相似,从而验证了SPR方法。该方法可轻松应用于其他转移蛋白,并且与现有测量脂质结合的技术相比具有几个优点,包括(i)能够研究天然状态的脂质(即没有相对较大的报告基团)以及(ii)能够测量结合和解离速率常数以及平衡常数。

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