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利用 Sf9 昆虫细胞中的翻转酶介导盒式交换进行稳定的基因表达。

Flipase-mediated cassette exchange in Sf9 insect cells for stable gene expression.

机构信息

Instituto de Biologia Experimental e Tecnológica, Oeiras, Portugal.

出版信息

Biotechnol Bioeng. 2012 Nov;109(11):2836-44. doi: 10.1002/bit.24542. Epub 2012 May 19.

Abstract

Site-specific DNA integration allows predictable heterologous gene expression and circumvents extensive clone screening. Herein, the establishment of a Flipase (Flp)-mediated cassette exchange system in Sf9 insect cells for targeted gene integration is described. A tagging cassette harboring a reporter dsRed gene was randomly introduced into the cell genome after screening different transfection protocols. Single-copy integration clones were then co-transfected with both Flp-containing plasmid and an EGFP-containing targeting cassette. Successful cassette exchange was suggested by emergence of G418-resistant green colonies and confirmed by PCR analysis, showing the absence of the tagging cassette and single integration of the targeting cassette in the same locus. Upon cassette exchange, uniform EGFP expression between clones derived from the same integration site was obtained. Moreover, the resulting cell clones exhibited the expression properties of the parental cell line. EGFP production titers over 40 mg/L were of the same order of magnitude as those achieved through baculovirus infection. This Sf9 master cell line constitutes a versatile and re-usable platform to produce multiple recombinant proteins for fundamental and applied research.

摘要

位点特异性 DNA 整合可实现可预测的异源基因表达,并避免广泛的克隆筛选。本文描述了一种在 Sf9 昆虫细胞中利用翻转酶(Flp)介导的盒式交换系统进行靶向基因整合的方法。在筛选不同的转染方案后,带有报告基因 dsRed 的标记盒随机引入细胞基因组。然后,将含有 Flp 的质粒和含有 EGFP 的靶向盒共转染单拷贝整合克隆。出现 G418 抗性绿色菌落表明成功进行了盒式交换,并通过 PCR 分析进一步证实,标记盒已缺失且靶向盒在同一基因座中进行了单整合。进行盒式交换后,可从同一整合位点获得克隆间均匀的 EGFP 表达。此外,所得细胞克隆表现出亲本细胞系的表达特性。EGFP 的产量超过 40mg/L,与杆状病毒感染相当。该 Sf9 主细胞系构成了一个多功能且可重复使用的平台,可用于生产用于基础和应用研究的多种重组蛋白。

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