HEK 293细胞
重组DNA
转染
绿色荧光蛋白
融合蛋白
膜蛋白
细胞生物学
蛋白质纯化
膜
化学
异位表达
生物
生物化学
基因
作者
Joanna Pieprzyk,Samuel Pažický,Christian Löw
标识
DOI:10.1007/978-1-4939-8730-6_2
摘要
Membrane proteins play important roles in many biological processes and are a major drug target. However, only a limited number of structures of eukaryotic membrane proteins have been determined so far. Besides the challenges in crystallizing these proteins, one of the main bottlenecks in structure determination is their recombinant expression. The mammalian HEK293 cell line provides a natural environment for expression of eukaryotic membrane proteins but optimization of transfection and cultivation time is often necessary to yield amounts of protein suitable for structural studies.Here we describe a detailed protocol for expression and purification of membrane proteins from HEK293 cells with an example of the human peptide transporter, PepT2. In the first part, we focus on the expression optimization by changing transfection protocol and cultivation time. In the second part, we describe a robust protocol for large-scale expression and purification of membrane proteins based on affinity chromatography and gel filtration.
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