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利用脂质交换和天然质谱法测量膜蛋白周围脂质环境的重塑。

Measuring Remodeling of the Lipid Environment Surrounding Membrane Proteins with Lipid Exchange and Native Mass Spectrometry.

出版信息

Anal Chem. 2020 Apr 21;92(8):5666-5669. doi: 10.1021/acs.analchem.0c00786. Epub 2020 Apr 7.

Abstract

Due to their crucial biochemical roles, membrane proteins are important drug targets. Although it is clear that lipids can influence membrane protein function, the chemistry of lipid binding remains difficult to study because protein-lipid interactions are polydisperse, competitive, and transient. Furthermore, detergents, which are often used to solubilize membrane proteins in micelles, may disrupt lipid interactions that occur in bilayers. Here, we present two new approaches to quantify protein-lipid interactions in bilayers and understand how membrane proteins remodel their surrounding lipid environment. First, we used mass spectrometry (MS) to measure the exchange of lipids between lipoprotein nanodiscs with and without an embedded membrane protein. Shifts in the lipid distribution toward the membrane protein nanodiscs revealed lipid binding, and titrations allowed measurement of the optimal lipid composition for the membrane protein. Second, we used native or nondenaturing MS to ionize membrane protein nanodiscs with heterogeneous lipids. Ejecting the membrane protein complex with bound lipids in the mass spectrometer revealed enrichment of specific lipids around the membrane protein. Both new approaches showed that the ammonium transporter AmtB prefers phosphatidylglycerol lipids overall but has a minor affinity for phosphatidylcholine lipids.

摘要

由于其关键的生化作用,膜蛋白是重要的药物靶点。尽管很明显脂质可以影响膜蛋白的功能,但脂质结合的化学性质仍然难以研究,因为蛋白质-脂质相互作用是多分散的、竞争的和瞬间的。此外,去污剂常用于将膜蛋白溶解在胶束中,但可能会破坏双层中发生的脂质相互作用。在这里,我们提出了两种新的方法来定量双层中蛋白质-脂质相互作用,并了解膜蛋白如何重塑其周围的脂质环境。首先,我们使用质谱(MS)测量脂蛋白纳米盘与嵌入其中的膜蛋白之间的脂质交换。脂质分布向膜蛋白纳米盘的转移揭示了脂质结合,而滴定允许测量膜蛋白的最佳脂质组成。其次,我们使用天然或非变性 MS 对具有异质脂质的膜蛋白纳米盘进行离子化。在质谱仪中喷射带有结合脂质的膜蛋白复合物,揭示了特定脂质在膜蛋白周围的富集。这两种新方法都表明铵转运蛋白 AmtB 总体上更喜欢磷脂酰甘油脂质,但对磷脂酰胆碱脂质有较小的亲和力。

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