Cre-mediated site-specific cassette exchange in erythroid cell.

Xing-Guo Li, Hao-Heng Yan, De-Pei Liu, De-Long Hao, Chih-Chuan Liang
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Abstract

Cre-mediated cassette exchange has been developed to perform site-specific chromosomal integration using Cre recombinase. Here, site-specific integration with inverted Lox sites was used to investigate the erythroid cis-acting DNA element in specific chromatin contexts in mouse erythroleukemia cells. Single hygromycin-resistant clones were obtained from the selective semi-solid medium containing hygromycin post-electroporation. PCR and Southern blotting analysis showed single-copy integration of target vector in clones A, B and D. Site-specific cassette exchange was performed in clone A with exchange vector and Cre expression plasmid, followed by gancyclovir selection. Flow cytometry was used for analysis of EGFP gene expression. A 732-bp fragment of human beta-globin gene cluster 5' DNase I hypersensitive site 2 (HS2) was exchanged and integrated into clone A in an anti-genomic orientation. The low EGFP expression in clone A-HS may be due to the orientation-dependent gene silencing caused by integration of HS2 in a non-permissive orientation.

红细胞中cre介导的位点特异性盒体交换。
Cre介导的盒式交换已被开发用于使用Cre重组酶进行位点特异性染色体整合。本研究利用位点特异性整合倒置的Lox位点来研究小鼠红细胞白血病细胞中特定染色质背景下红系顺式作用DNA元件。电穿孔后,在含潮霉素的选择性半固体培养基中获得了单株耐潮霉素克隆。PCR和Southern blotting分析显示,A、B和d克隆中目标载体单拷贝整合,克隆A与交换载体和Cre表达质粒进行位点特异性的盒式交换,然后进行更昔洛韦选择。流式细胞术检测EGFP基因表达。人β -珠蛋白基因簇5' DNase I超敏位点2 (HS2)的732bp片段被交换并以抗基因组取向整合到克隆A中。克隆a - hs中EGFP的低表达可能是由于HS2在非允许取向上的整合导致定向依赖基因沉默。
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