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A high-throughput screening of genes that encode proteins transported into the endoplasmic reticulum in mammalian cells

机译:高通量筛选编码哺乳动物细胞内质网中转运蛋白的基因

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摘要

The compartments of eukaryotic cells maintain a distinct protein composition to perform a variety of specialized functions. We developed a new method for identifying the proteins that are transported to the endoplasmic reticulum (ER) in living mammalian cells. The principle is based on the reconstitution of two split fragments of enhanced green fluorescent protein (EGFP) by protein splicing with DnaE from Synechocystis PCC6803. Complementary DNA (cDNA) libraries fused to the N-terminal halves of DnaE and EGFP are introduced in mammalian cells with retroviruses. If an expressed protein is transported into the ER, the N-terminal half of EGFP meets its C-terminal half in the ER, and full-length EGFP is reconstituted by protein splicing. The fluorescent cells are isolated using fluorescence-activated cell sorting and the cDNAs are sequenced. The developed method was able to accurately identify cDNAs that encode proteins transported to the ER. We identified 27 novel proteins as the ER-targeting proteins. The present method overcomes the limitation of the previous GFP- or epitope-tagged methods, using which it was difficult to identify the ER-targeting proteins in a high-throughput manner.
机译:真核细胞的区室保持不同的蛋白质组成,以执行多种专门功能。我们开发了一种新的方法来鉴定在活的哺乳动物细胞中转运到内质网(ER)的蛋白质。该原理基于通过用蓝藻PCC6803的DnaE剪接蛋白质来增强绿色荧光蛋白(EGFP)的两个分裂片段的重组。通过逆转录病毒将与DnaE和EGFP的N端一半融合的互补DNA(cDNA)文库引入哺乳动物细胞。如果将表达的蛋白质转运到ER中,则EGFP的N端一半会在ER中遇到C端一半,并且全长EGFP通过蛋白剪接重构。使用荧光激活的细胞分选方法分离荧光细胞,并对cDNA进行测序。所开发的方法能够准确鉴定编码转运至ER的蛋白质的cDNA。我们确定了27种新型蛋白作为ER靶向蛋白。本方法克服了以前的GFP-或表位标记方法的局限性,使用该方法很难以高通量的方式鉴定靶向ER的蛋白。

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