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一种使用疏水相互作用色谱法对脂质结合蛋白进行联合亚分级分离和脱脂的方案。

A protocol for the combined sub-fractionation and delipidation of lipid binding proteins using hydrophobic interaction chromatography.

作者信息

Velkov Tony, Lim Maria L R, Capuano Benjamin, Prankerd Richard

机构信息

Medicinal Chemistry and Drug Action, Monash Institute of Pharmaceutical Sciences, Monash University (Parkville Campus), 381 Royal Parade, Parkville 3052 Victoria, Australia.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2008 May 15;867(2):238-46. doi: 10.1016/j.jchromb.2008.04.011. Epub 2008 Apr 15.

Abstract

Cellular lipids frequently co-purify with lipid binding proteins isolated from tissue extracts or heterologous host systems and as such hinder in vitro ligand binding approaches for which the apo-protein is a prerequisite. Here we present a technique for the complete removal of unesterified fatty acids, phospholipids, steroids and other lipophilic ligands bound to soluble proteins, without protein denaturation. Peroxisome proliferator activated receptor gamma ligand binding domain and intracellular fatty acid binding proteins were expressed in an Escherichia coli host and completely delipidated by hydrophobic interaction chromatography using phenyl sepharose. The delipidation procedure operates at room temperature with complete removal of bound lipids in a single step, as ascertained by mass spectrometry analysis of organic solvent extracts from purified protein samples. The speed and capacity of this method makes it amenable to scale-up and high-throughput applications. The method can also easily be adapted for other lipid binding proteins that require delipidation under native conditions.

摘要

细胞脂质常常与从组织提取物或异源宿主系统中分离出的脂质结合蛋白共同纯化,因此会妨碍以脱辅基蛋白为前提条件的体外配体结合方法。在此,我们介绍一种在不使蛋白质变性的情况下,完全去除与可溶性蛋白结合的未酯化脂肪酸、磷脂、类固醇及其他亲脂性配体的技术。过氧化物酶体增殖物激活受体γ配体结合结构域和细胞内脂肪酸结合蛋白在大肠杆菌宿主中表达,并通过使用苯基琼脂糖的疏水相互作用色谱法完全脱脂。脱脂过程在室温下进行,一步即可完全去除结合的脂质,这通过对纯化蛋白样品的有机溶剂提取物进行质谱分析得以确定。该方法的速度和容量使其适用于扩大规模和高通量应用。此方法也可轻松适用于其他需要在天然条件下进行脱脂的脂质结合蛋白。

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