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使用在丰富培养基中生长的细胞,用15N氨基酸对膜肽进行选择性标记。

Selective labeling of a membrane peptide with 15N-amino acids using cells grown in rich medium.

作者信息

Englander Jacqueline, Cohen Leah, Arshava Boris, Estephan Racha, Becker Jeffrey M, Naider Fred

机构信息

Department of Chemistry and the Macromolecular Assemblies Institute, The College of Staten Island of the City University of New York, Staten Island, NY 10314, USA.

出版信息

Biopolymers. 2006;84(5):508-18. doi: 10.1002/bip.20546.

DOI:10.1002/bip.20546
PMID:16741986
Abstract

Nuclear magnetic resonance spectra of membrane proteins containing multiple transmembrane helices have proven difficult to resolve due to the redundancy of aliphatic and Ser/Thr residues in transmembrane domains and the low chemical shift dispersity exhibited by residues in alpha-helical structures. Although (13)C- and (15)N-labeling are useful tools in the biophysical analysis of proteins, selective labeling of individual amino acids has been used to help elucidate more complete structures and to probe ligand-protein interactions. In general, selective labeling has been performed in Escherichia coli expression systems using minimal media supplemented with a single labeled amino acid and nineteen other unlabeled amino acids and/or by using auxotrophs for specific amino acids. Growth in minimal media often results in low yields of cells or expression products. We demonstrate a method in which one labeled amino acid is added to a rich medium. These conditions resulted in high expression (> or =100 mg/L) of a test fusion protein and milligram quantities of the selectively labeled membrane peptide after cyanogen bromide cleavage to release the peptide from the fusion protein. High levels of (15)N incorporation and acceptable levels of cross-labeling into other amino acid residues of the peptide were achieved. Growth in rich media is a simple and convenient alternative to growth in supplemented minimal media and is readily applicable to the expression of proteins selectively labeled with specific amino acids.

摘要

由于跨膜结构域中脂肪族和丝氨酸/苏氨酸残基的冗余性,以及α-螺旋结构中残基表现出的低化学位移分散性,含有多个跨膜螺旋的膜蛋白的核磁共振谱已被证明难以解析。尽管碳-13和氮-15标记是蛋白质生物物理分析中的有用工具,但单个氨基酸的选择性标记已被用于帮助阐明更完整的结构并探测配体-蛋白质相互作用。一般来说,选择性标记是在大肠杆菌表达系统中进行的,使用补充有单一标记氨基酸和其他19种未标记氨基酸的基本培养基,和/或使用特定氨基酸的营养缺陷型菌株。在基本培养基中生长往往会导致细胞或表达产物产量较低。我们展示了一种方法,即在丰富培养基中添加一种标记氨基酸。这些条件导致了测试融合蛋白的高表达(≥100mg/L),并且在溴化氰裂解以从融合蛋白中释放肽后,获得了毫克量的选择性标记膜肽。实现了高水平的氮-15掺入以及肽的其他氨基酸残基中可接受水平的交叉标记。在丰富培养基中生长是在补充基本培养基中生长的一种简单方便的替代方法,并且很容易应用于用特定氨基酸选择性标记的蛋白质的表达。

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