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去污剂和磷脂在人红细胞阴离子交换膜结构域结晶中的重要性。

Importance of detergent and phospholipid in the crystallization of the human erythrocyte anion-exchanger membrane domain.

作者信息

Lemieux M Joanne, Reithmeier Reinhart A F, Wang Da-Neng

机构信息

Skirball Institute of Biomolecular Medicine and Department of Cell Biology, New York University School of Medicine, 540 First Avenue, New York 10016, USA.

出版信息

J Struct Biol. 2002 Mar;137(3):322-32. doi: 10.1016/s1047-8477(02)00010-2.

Abstract

Three-dimensional crystals were obtained for the membrane domain of the human erythrocyte anion exchanger (AE1, Band 3). Protein homogeneity and stability and the delicate balance between the detergent used and the amount of phospholipids copurifying are critical to the formation of three-dimensional crystals of the AE1 membrane domain. While deglycosylation improved the protein homogeneity, its stability was significantly increased by inhibitor binding. Size-exclusion chromatography showed that the protein was monodisperse in detergents with acyl chains of 10-12 carbons over a pH range of 5.5-10.0. This pH range and the detergents that retained the protein's monodispersity were used for crystallization screening. Crystals were obtained with the protein purified in C(12)E(8), dodecylmaltoside, decylthiomaltoside, and cyclohexyl-hexylmaltoside. Five to 13 lipid molecules per protein were required for the protein crystal formation. Those crystals grown in dodecylmaltoside diffracted X-rays to 14 A. With these factors taken into consideration, ways to further improve the crystal quality are suggested.

摘要

获得了人红细胞阴离子交换蛋白(AE1,带3)膜结构域的三维晶体。蛋白质的均一性和稳定性以及所用去污剂与共纯化磷脂量之间的微妙平衡对于AE1膜结构域三维晶体的形成至关重要。去糖基化虽提高了蛋白质的均一性,但其稳定性通过抑制剂结合显著增加。尺寸排阻色谱显示,在pH值5.5 - 10.0范围内,该蛋白质在具有10 - 12个碳的酰基链的去污剂中呈单分散状态。此pH范围以及能保持蛋白质单分散性的去污剂被用于结晶筛选。用在C(12)E(8)、十二烷基麦芽糖苷、癸基硫代麦芽糖苷和环己基己基麦芽糖苷中纯化的蛋白质获得了晶体。蛋白质晶体形成需要每个蛋白质有5至13个脂质分子。在十二烷基麦芽糖苷中生长的那些晶体将X射线衍射至14 Å。考虑到这些因素,提出了进一步提高晶体质量的方法。

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