Pronuclear Injection-Based Targeted Transgenesis

Current Protocols in Human Genetics Pub Date : 2018-02-13 DOI:10.1002/cphg.23

Samantha L.P. Schilit, Masato Ohtsuka, Rolen M. Quadros, Channabasavaiah B. Gurumurthy

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引用次数: 10

Abstract

Microinjection of DNA expression cassettes into fertilized zygotes has been a standard method for generating transgenic animal models. While efficient, the injected DNA integrates randomly into the genome, leading to potential disruption of endogenous genes or regulatory elements, variation in copy number, or integration into heterochromatic regions that inhibit transgene expression. A recently developed method addresses such pitfalls of traditional transgenesis by targeting the transgene to predetermined sites in the genome that can safely harbor exogenous DNA. This method, called Pronuclear Injection-based Targeted Transgenesis (PITT), employs an enzymatic transfer of exogenous DNA from a donor vector to a previously created landing-pad site in the mouse genome. DNA transfer is achieved using molecular tools such as the Cre-LoxP recombinase and PhiC31-attB/P integrase systems. Here, we provide protocols for performing PITT and an overview of the current PITT tools available to the research community. © 2016 by John Wiley & Sons, Inc.

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基于原核注射的靶向转基因

将DNA表达盒微量注射到受精卵中已成为建立转基因动物模型的标准方法。虽然有效，但注入的DNA随机整合到基因组中，导致内源基因或调控元件的潜在破坏，拷贝数的变化，或整合到抑制转基因表达的异色区域。最近开发的一种方法通过将转基因靶向基因组中可以安全地容纳外源DNA的预定位点来解决传统转基因的这些缺陷。这种方法被称为基于原核注射的靶向转基因(PITT)，利用酶将外源DNA从供体载体转移到小鼠基因组中先前创建的着陆点。DNA转移是使用分子工具，如Cre-LoxP重组酶和PhiC31-attB/P整合酶系统实现的。在这里，我们提供了执行PITT的协议，并概述了目前研究界可用的PITT工具。©2016 by John Wiley &儿子,Inc。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Current Protocols in Human Genetics Biochemistry, Genetics and Molecular Biology-Genetics

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期刊介绍： Current Protocols in Human Genetics is the resource for designing and running successful research projects in all branches of human genetics.