Bode J, Schlake T, Iber M, Schübeler D, Seibler J, Snezhkov E, Nikolaev L
German Center for Biotechnological Research (GBF), RDIF/Epigenetic Regulation, Braunschweig.
Biol Chem. 2000 Sep-Oct;381(9-10):801-13. doi: 10.1515/BC.2000.103.
Classical techniques for gene transfer into mammalian cells involve tedious screening procedures to identify transgenic clones or animals with the appropriate level and stability of expression or with the correct developmental patterns. These first generation technologies are clearly inadequate for complex genetic strategies by which gene regulation can be studied in its entire complexity. While site-specific insertions can principally be achieved by homologous recombination or by adapting the recombination apparatus from phages or yeast, these methods usually lack the required efficiency or they perturb expression patterns by the co-insertion of prokaryotic vector parts. Virtually all of these problems can be overcome by recombinase-mediated cassette exchange (RMCE) techniques which cleanly replace a resident cassette that is flanked by two hetero-specific recombination target sites for a second cassette with the analogous design, presented on a targeting vector. After illustrating the fundamentals of site-specific recombination by selected experiments, the authors (arranged in the chronological order of their contribution) will describe their efforts to develop RMCE into a method of wide applicability. Further developments that have been initiated utilizing the particular potential of the RMCE principle will be outlined.
将基因导入哺乳动物细胞的经典技术需要繁琐的筛选程序,以鉴定具有适当表达水平和稳定性或具有正确发育模式的转基因克隆或动物。这些第一代技术显然不足以用于研究基因调控全部复杂性的复杂遗传策略。虽然位点特异性插入原则上可以通过同源重组或通过改造噬菌体或酵母的重组装置来实现,但这些方法通常缺乏所需的效率,或者会因原核载体部分的共插入而干扰表达模式。几乎所有这些问题都可以通过重组酶介导的盒式交换(RMCE)技术来克服,该技术可以干净利落地将一个位于两个异源特异性重组靶位点侧翼的驻留盒式结构替换为第二个具有类似设计的盒式结构,该盒式结构存在于靶向载体上。在通过选定的实验阐述位点特异性重组的基本原理之后,作者(按照他们贡献的时间顺序排列)将描述他们为将RMCE发展成为一种广泛适用的方法所做的努力。还将概述利用RMCE原理的特殊潜力所启动的进一步发展。
