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Recombinase-Mediated Cassette Exchange (RMCE)-in Reporter Cell Lines as an Alternative to the Flp-in System

机译:重组酶介导的盒式磁带交换(RMCE)的Reporter细胞系作为Flp导入系统的替代品

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摘要

Recombinase mediated cassette exchange (RMCE) is a powerful tool for targeted insertion of transgenes. Here we describe non-proprietary 'RMCE-in' cell lines as an alternative to the 'Flp-in' system and cell lines. RMCE-in cell lines offer a number of advantages including increased efficiency of integration of the genetic element of interest (GEI) at a single docking site, lack of bacterial backbone at the docking site both before and after GEI integration, removal of selection and visual markers initially present at the docking site upon GEI integration and the possibility to validate GEI integration by loss of a red fluorescence reporter. Moreover, the RMCE-in cell lines are compatible with GEI donors used for the Flp-in system. We demonstrate a three-step procedure for generating RMCE-in cell lines, (I) RMCE-in transposon and SB10 transposase transfection, (II) clone isolation, and (III) selecting single integrated clones with highest RFP level, which could in principle be used to turn any cell line into an RMCE-in cell line. The RMCE-in system was used as a proof of concept to produce three new RMCE-in cell lines using HEK293, HeLa, and murine embryonic stem (mES) cells. The established RMCE-in cell lines and vector are freely available from the ATCC cell bank and Addgene respectively.
机译:重组酶介导的盒交换(RMCE)是靶向插入转基因的强大工具。在这里,我们将非专有的“ RMCE-in”细胞系描述为“ Flp-in”系统和细胞系的替代品。 RMCE-in细胞系具有许多优势,包括在单个停靠位点整合感兴趣的遗传元件(GEI)的效率提高,GEI整合前后,停靠位点细菌骨架均缺乏,选择和视觉去除标记最初在GEI整合后出现在对接位点,并且可能通过丢失红色荧光报告基因来验证GEI整合。此外,RMCE-in细胞系与用于Flp-in系统的GEI供体兼容。我们演示了生成RMCE-in细胞系的三步过程,(I)RMCE-in转座子和SB10转座酶转染,(II)克隆分离,以及(III)选择具有最高RFP水平的单个整合克隆,原则上可以用于将任何细胞系转化为RMCE-in细胞系。使用RMCE-in系统作为概念证明,可使用HEK293,HeLa和鼠类胚胎干(mES)细胞生产三种新的RMCE-in细胞系。建立的RMCE-in细胞系和载体可分别从ATCC细胞库和Addgene免费获得。

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