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用磷脂类似物混合物稳定和最小化膜蛋白的溶解。

Stable and Minimum Size Solubilization of Membrane Proteins with Cocktails of Phospholipid Analogues.

机构信息

Graduate School of Pharmaceutical Sciences, Kyoto University, Kyoto 606-8501, Japan.

School of Pharmacy, Hyogo Medical University, Kobe 650-8530, Japan.

出版信息

ACS Appl Mater Interfaces. 2024 Nov 20;16(46):63358-63367. doi: 10.1021/acsami.4c15697. Epub 2024 Nov 7.

DOI:10.1021/acsami.4c15697
PMID:39509591
Abstract

Membrane proteins (MPs) play important roles in various cellular processes and are major targets for drugs. Solubilization of MPs is often needed for structural and biophysical studies. For high-resolution nuclear magnetic resonance measurements, there is a size limit of the sample (<100 kDa), and a high thermal stability at an increased temperature is required. Furthermore, lipid bilayer-like environments are desirable to preserve the native states of MPs. However, existing solubilization techniques do not fulfill these requirements at the same time. In this study, we combined two phospholipid analogues as a solubilizer and stabilizer to isolate MPs. This method maintained bacteriorhodopsin (bR) extracted from purple membranes in its native state for 7 d at 40 °C. The solubility was comparable to that of conventional detergents for MPs, and the thermal stability of the solubilizate was the best among them. The increase in the molecular size caused by the solubilization of bR was only 20 kDa, indicating that 20 phospholipid analogue molecules were sufficient to solubilize one bR molecule. N-H heteronuclear single quantum coherence spectra of solubilized H- and N-labeled bR gave ∼80% of the expected peaks. In addition, the lysate of human neuropeptide Y receptor-expressing mammalian cells exhibited ligand recognition for 7 d at 37 °C, suggesting that this technique can be used for ligand screening. Moreover, the structure of the single membrane-spanning M2 protein of the influenza A virus expressed in was stably maintained for 7 d at 40 °C. Thus, our method is promising for various MP studies.

摘要

膜蛋白 (MPs) 在各种细胞过程中发挥重要作用,是药物的主要靶点。为了进行结构和生物物理研究,通常需要 MPs 的增溶。对于高分辨率的核磁共振测量,样品的大小有限制(<100 kDa),并且需要在升高的温度下具有高热稳定性。此外,希望 MPs 处于类似脂质双层的环境中以保持其天然状态。然而,现有的增溶技术无法同时满足这些要求。在这项研究中,我们将两种磷脂类似物组合在一起作为增溶剂和稳定剂来分离 MPs。这种方法将从紫色膜中提取的菌紫质 (bR) 以其天然状态在 40°C 下保持 7 天。其溶解度与 MPs 常用的去污剂相当,且增溶产物的热稳定性是其中最好的。bR 的增溶导致的分子大小增加仅为 20 kDa,表明 20 个磷脂类似物分子足以增溶一个 bR 分子。增溶的 H 和 N 标记 bR 的 N-H 异核单量子相干光谱给出了约 80%的预期峰。此外,在 37°C 下,表达人类神经肽 Y 受体的哺乳动物细胞的裂解液在 7 天内表现出配体识别,表明该技术可用于配体筛选。此外,在 40°C 下稳定表达的甲型流感病毒的单跨膜 M2 蛋白的结构在 7 天内保持稳定。因此,我们的方法有望用于各种 MPs 研究。

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