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转基因果蝇眼睛中的膜蛋白表达。

Membrane protein expression in the eyes of transgenic flies.

作者信息

Panneels Valérie, Sinning Irmgard

机构信息

Heidelberg University Biochemistry Center, Germany.

出版信息

Methods Mol Biol. 2010;601:135-47. doi: 10.1007/978-1-60761-344-2_9.

Abstract

Eukaryotic membrane proteins are often difficult to obtain in sufficient amounts for structural studies using classical cell culture overexpression systems. This could be due to incomplete protein maturation and insufficient trafficking to the plasma membrane or to a cytotoxic effect of the recombinant membrane protein changing the overall metabolism. The method presented here takes advantage of the membrane stacks in the retina, where rhodopsin resides. The idea is to direct G protein-coupled receptors (GPCRs) and transporters to these membrane stacks and to express the target proteins in the retina of transgenic Drosophila melanogaster. Drosophila was chosen since fly genetics are well established and rather easily accessible. Metabotropic glutamate receptor mGluRa from Drosophila was among the first examples for GPCRs expressed in this system. It showed high expression yield, functionality and high homogeneity. When the same protein was expressed in Sf9 cells, however, contamination by immature protein was a problem. Encouraged by this success, the fly system is now successfully used for a larger variety of membrane proteins, including mammalian GPCRs and transporters.

摘要

真核膜蛋白通常难以通过经典的细胞培养过表达系统获得足够量用于结构研究。这可能是由于蛋白质成熟不完全、转运到质膜的量不足,或者是重组膜蛋白的细胞毒性作用改变了整体代谢。这里介绍的方法利用了视紫红质所在的视网膜中的膜堆叠。其思路是将G蛋白偶联受体(GPCRs)和转运蛋白导向这些膜堆叠,并在转基因黑腹果蝇的视网膜中表达目标蛋白。选择果蝇是因为果蝇遗传学已经很成熟且相当容易操作。果蝇的代谢型谷氨酸受体mGluRa是在该系统中表达的GPCRs的首批例子之一。它表现出高表达产量、功能性和高均一性。然而,当相同的蛋白在Sf9细胞中表达时,未成熟蛋白的污染是个问题。受此成功鼓舞,果蝇系统现在已成功用于更多种类的膜蛋白,包括哺乳动物的GPCRs和转运蛋白。

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