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一种用于多用途敲除优先等位基因的可靠lacZ表达报告盒。

A reliable lacZ expression reporter cassette for multipurpose, knockout-first alleles.

作者信息

Testa Giuseppe, Schaft Julia, van der Hoeven Frank, Glaser Stefan, Anastassiadis Konstantinos, Zhang Youming, Hermann Thomas, Stremmel Wolfgang, Stewart A Francis

机构信息

Biotec, Technische Universität Dresden, c/o Max Planck Institute of Molecular cell Biology and Genetics, Dresden, Germany.

出版信息

Genesis. 2004 Mar;38(3):151-8. doi: 10.1002/gene.20012.

Abstract

Alteration of the mouse genome through homologous recombination in embryonic stem (ES) cells is the most accurate and versatile way to dissect gene function in a vertebrate model. Most often, a selectable marker is used to create a knockout allele by replacing an essential part of the gene. However, knockout strategies are limited because the mutation is present constitutively. Conditional approaches based on the Cre-loxP site-specific recombination (SSR) system address this limitation; however, it requires that all parts of the targeted gene remain in ES cells. Here we report success with a "knockout-first" strategy that ablates gene function by insertion of RNA processing signals without deletion of any of the target gene. Incorporation of site-specific recombination target sites creates a multipurpose allele for both knockout and conditional applications.

摘要

通过胚胎干细胞(ES细胞)中的同源重组来改变小鼠基因组,是在脊椎动物模型中剖析基因功能最准确且最通用的方法。最常见的情况是,使用一个可选择标记通过替换基因的关键部分来创建一个敲除等位基因。然而,敲除策略存在局限性,因为突变是组成性存在的。基于Cre-loxP位点特异性重组(SSR)系统的条件性方法解决了这一局限性;然而,它要求目标基因的所有部分都保留在ES细胞中。在此,我们报告了一种“敲除优先”策略的成功,该策略通过插入RNA加工信号来消除基因功能,而不删除任何目标基因。整合位点特异性重组靶位点可创建一个用于敲除和条件性应用的多功能等位基因。

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