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Flow cytometric analysis of DNA binding and cleavage by cell surface-displayed homing endonucleases

机译:细胞表面展示的归巢核酸内切酶对DNA结合和裂解的流式细胞术分析

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摘要

LAGLIDADG homing endonucleases (LHEs) cleave 18–24 bp DNA sequences and are promising enzymes for applications requiring sequence-specific DNA cleavage amongst genome-sized DNA backgrounds. Here, we report a method for cell surface display of LHEs, which facilitates analysis of their DNA binding and cleavage properties by flow cytometry. Cells expressing surface LHEs can be stained with fluorescently conjugated double-stranded oligonucleotides (dsOligos) containing their respective target sequences. The signal is absolutely sequence specific and undetectable with dsOligos carrying single base-pair substitutions. LHE–dsOligo interactions facilitate rapid enrichment and viable recovery of rare LHE expressing cells by both fluorescence-activated cell sorting (FACS) and magnetic cell sorting (MACS). Additionally, dsOligos conjugated with unique fluorophores at opposite termini can be tethered to the cell surface and used to detect DNA cleavage. Recapitulation of DNA binding and cleavage by surface-displayed LHEs provides a high-throughput approach to library screening that should facilitate rapid identification and analysis of enzymes with novel sequence specificities.
机译:LAGLIDADG归巢核酸内切酶(LHEs)可以切割18-24bp的DNA序列,是需要在基因组大小的DNA背景中进行序列特异性DNA切割的应用中很有希望的酶。在这里,我们报告LHEs的细胞表面展示的方法,它有助于通过流式细胞仪分析其DNA结合和切割特性。表达表面LHE的细胞可用含有各自靶序列的荧光偶联双链寡核苷酸(dsOligos)染色。该信号绝对是序列特异性的,对于带有单个碱基对取代的dsOligos来说是不可检测的。 LHE-dsOligo相互作用可通过荧光激活细胞分选(FACS)和磁性细胞分选(MACS)促进稀有LHE表达细胞的快速富集和可行恢复。另外,在相反的末端与独特的荧光团缀合的dsOligos可以拴在细胞表面,并用于检测DNA裂解。表面展示的LHE对DNA结合和裂解的概括提供了一种高通量的文库筛选方法,该方法应有助于快速鉴定和分析具有新型序列特异性的酶。

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