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Optimising the transient expression of GABA(A) receptors in adherent HEK293 cells

机译:优化粘附HEK293细胞中GABA(A)受体的瞬时表达

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Owing to their therapeutic relevance, considerable efforts are devoted to the structural characterisation of membrane proteins. Such studies are limited by the availability of high quality protein due to the difficulty of overexpression in recombinant mammalian systems. We sought to systematically optimise multiple aspects in the process of transiently transfecting HEK293 cells, to allow the rapid expression of membrane proteins, without the lengthy process of stable clone formation. We assessed the impact of medium formulation, cell line, and harvest time on the expression of GABA(A) receptors, as determined by [H-3]muscimol binding in cell membranes. Furthermore, transfection with the use of calcium phosphate/polyethyleneimine multishell nanoparticles was optimised, and a dual vector system utilising viral enhancing elements was designed and implemented. These efforts resulted in a 40-fold improvement in GABA(A) alpha(1)beta(3) receptor expression, providing final yields of 22 fmol/cm(2). The findings from this work provide a guide to the optimisation of transient expression of proteins in mammalian cells and should assist in the structural characterisation of membrane proteins.
机译:由于其治疗相关性,大量努力致力于膜蛋白的结构表征。由于重组哺乳动物系统中过度表达的难度,这些研究受到高质量蛋白质的可用性。我们寻求系统地优化在瞬时转染HEK293细胞的过程中的多个方面,以允许膜蛋白的快速表达,而无需稳定的克隆形成的冗长过程。我们评估了培养基配方,细胞系和收获时间对GABA(A)受体表达的影响,通过在细胞膜中的[H-3] Muscimol结合而确定。此外,优化了使用磷酸钙/聚乙烯亚胺MultiShell纳米粒子的转染,并设计并实施了利用病毒增强元件的双载体系统。这些努力导致GABA(A)α(1)β(3)受体表达中的40倍改善,提供了22 fmol / cm(2)的最终产率。本作作品的发现提供了哺乳动物细胞中蛋白质瞬态表达的指导,并应有助于膜蛋白的结构表征。

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