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荧光激活细胞分选后通过直接质粒回收进行功能富集

Functional enrichment by direct plasmid recovery after fluorescence activated cell sorting.

作者信息

Ramesh Balakrishnan, Frei Christopher S, Cirino Patrick C, Varadarajan Navin

机构信息

Department of Chemical and Biomolecular Engineering, University of Houston, Houston, TX.

出版信息

Biotechniques. 2015 Sep 1;59(3):157-61. doi: 10.2144/000114329. eCollection 2015 Sep.

DOI:10.2144/000114329
PMID:26345509
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5173293/
Abstract

Iterative screening of expressed protein libraries using fluorescence-activated cell sorting (FACS) typically involves culturing the pooled clones after each sort. In these experiments, if cell viability is compromised by the sort conditions and/or expression of the target protein(s), rescue PCR provides an alternative to culturing but requires re-cloning and can introduce amplification bias. We have optimized a simple protocol using commercially available reagents to directly recover plasmid DNA from sorted cells for subsequent transformation. We tested our protocol with 2 different screening systems in which <10% of sorted cells survive culturing and demonstrate that >60% of the sorted cell population was recovered.

摘要

使用荧光激活细胞分选(FACS)对表达蛋白文库进行迭代筛选通常涉及在每次分选后培养汇集的克隆。在这些实验中,如果分选条件和/或目标蛋白的表达损害了细胞活力,挽救PCR提供了一种替代培养的方法,但需要重新克隆并且可能引入扩增偏差。我们优化了一个简单的方案,使用市售试剂直接从分选的细胞中回收质粒DNA用于后续转化。我们用2种不同的筛选系统测试了我们的方案,在这些系统中,<10%的分选细胞在培养后存活,并证明>60%的分选细胞群体被回收。

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