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通过配体诱导无活性片段互补对Cre重组酶进行调控。

Regulation of Cre recombinase by ligand-induced complementation of inactive fragments.

作者信息

Jullien Nicolas, Sampieri François, Enjalbert Alain, Herman Jean-Paul

机构信息

ICNE-UMR 6544, CNRS-Université de la Méditerranée, IFR Jean-Roche, Faculté de Médecine Nord, 13916 Marseille Cedex 20, France.

出版信息

Nucleic Acids Res. 2003 Nov 1;31(21):e131. doi: 10.1093/nar/gng131.

Abstract

Cre recombinase is extensively used to engineer the genome of experimental animals. However, its usefulness is still limited by the lack of an efficient temporal control over its activity. To overcome this, we have developed DiCre, a regulatable fragment complementation system for Cre. The enzyme was split into two moieties that were fused to FKBP12 (FK506-binding protein) and FRB (binding domain of the FKBP12-rapamycin-associated protein), respectively. These can be efficiently heterodimerized by rapamycin. Several variants, based on splitting Cre at different sites and using different linker peptides, were tested in an indicator cell line. The fusion proteins, taken separately, had no recombinase activity. Stable transformants, co-expressing complementing fragments based on splitting Cre between Asn59 and Asn60, displayed low background activity affecting 0.05-0.4% of the cells. Rapamycin induced a rapid recombination, reaching 100% by 48-72 h, with an EC50 of 0.02 nM. Thus, ligand-induced dimerization can efficiently regulate Cre, and should be useful to achieve a tight temporal control of its activity, such as in the case of the creation of conditional knock-out animals.

摘要

Cre重组酶被广泛用于构建实验动物的基因组。然而,其效用仍受限于对其活性缺乏有效的时间控制。为克服这一问题,我们开发了DiCre,一种用于Cre的可调控片段互补系统。该酶被拆分为两个部分,分别与FKBP12(FK506结合蛋白)和FRB(FKBP12-雷帕霉素相关蛋白的结合结构域)融合。它们可通过雷帕霉素高效异源二聚化。基于在不同位点拆分Cre并使用不同连接肽的几种变体在指示细胞系中进行了测试。单独的融合蛋白没有重组酶活性。共表达基于在Asn59和Asn60之间拆分Cre的互补片段的稳定转化体显示出低背景活性,影响0.05 - 0.4%的细胞。雷帕霉素诱导快速重组,48 - 72小时达到100%,EC50为0.02 nM。因此,配体诱导的二聚化可有效调控Cre,对于实现对其活性的严格时间控制应该是有用的,例如在创建条件性基因敲除动物的情况下。

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