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PITT: Pronuclear Injection-Based Targeted Transgenesis, a Reliable Transgene Expression Method in Mice

机译:PITT:基于核前注射的靶向转基因,一种可靠的小鼠转基因表达方法

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Transgenic (Tg) mice have been extensively used as valuable tools for analyses of gene function and have also served as models for many human diseases. Typically, a transgenic mouse is created by microinjection of DNA into pronuclei in which the DNA gets integrated at random locations in the genome. Frequently however, the random integration of multiple copies of a transgene results in transgene silencing, probably because of a positional effect and/or repeat-induced gene silencing. The transgene silencing issue has been overcome by single-copy transgene integration into a predetermined locus through ES cell-mediated transgenesis, despite it being expensive and more time-consuming compared with pronuclear injection (PI)-mediated transgenesis. Recently, several groups have reported novel approaches that employ PI for targeted transgenesis. They are based on site-specific recombination catalyzed by a recombinase or an integrase or homologous recombination enhanced by a zinc-finger nuclease via PI. These next-generation transgenesis methods, which we termed as PI-based Targeted Transgenesis (PITT), are more convenient and faster than ES cell-based transgenesis. Furthermore, the Tg mice generated by these newer methods contain a single-copy transgene and exhibit reliable expression of the transgene. The objective of this review is to present the recent progress in mouse targeted transgenesis.
机译:转基因(Tg)小鼠已被广泛用作分析基因功能的有价值的工具,并已成为许多人类疾病的模型。通常,通过将DNA显微注射到前核中创建转基因小鼠,其中DNA在基因组中的随机位置整合。然而,经常可能由于位置效应和/或重复诱导的基因沉默,导致转基因多个拷贝的随机整合导致转基因沉默。通过单拷贝转基因通过ES细胞介导的转基因整合到预定位点已克服了转基因沉默的问题,尽管与原核注射(PI)介导的转基因相比它昂贵且耗时。最近,几个小组报告了采用PI进行靶向转基因的新方法。它们基于重组酶催化的位点特异性重组,或基于锌指核酸酶通过PI增强的整合酶或同源重组。这些下一代转基因方法,我们称为基于PI的靶向转基因(PITT),比基于ES细胞的转基因方法更方便,更快捷。此外,通过这些较新方法生成的Tg小鼠包含单拷贝转基因,并表现出可靠的转基因表达。这篇综述的目的是介绍小鼠靶向转基因的最新进展。

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