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成骨细胞靶向性Cre重组酶转基因在小鼠骨骼组织中的表达及活性

Expression and activity of osteoblast-targeted Cre recombinase transgenes in murine skeletal tissues.

作者信息

Liu Fei, Woitge Henning W, Braut Alen, Kronenberg Mark S, Lichtler Alexander C, Mina Mina, Kream Barbara E

机构信息

Department of Medicine, University of Connecticut Health Center, Farmington, Connecticut 06030, USA.

出版信息

Int J Dev Biol. 2004 Sep;48(7):645-53. doi: 10.1387/ijdb.041816fl.

DOI:10.1387/ijdb.041816fl
PMID:15470637
Abstract

The Cre/loxP recombination system can be used to circumvent many of the limitations of generalized gene ablation in mice. Here we present the development and characterization of transgenic mice in which Cre recombinase has been targeted to cells of the osteoblast lineage with 2.3 kb (Col 2.3-Cre) and 3.6 kb (Col 3.6-Cre) fragments of the rat Col1a1 promoter. Cre mRNA was detected in calvaria and long bone of adult Col 2.3-Cre and Col 3.6-Cre mice, as well as in tendon and skin of Col 3.6-Cre mice. To obtain a historical marking of the temporal and spatial pattern of Cre-mediated gene rearrangement, Col-Cre mice were bred with ROSA26 (R26R) mice in which Cre-mediated excision of a floxed cassette results in LacZ expression. In Col 2.3-Cre;R26R and Col 3.6-Cre;R26R progeny, calvarial and long bone osteoblasts showed intense beta-gal staining at embryonic day 18 and postnatal day 5. The spatial pattern of beta-gal staining was more restricted in bone and in bone marrow stromal cultures established from Col 2.3-Cre;R26R mice. Similar differences in the spatial patterns of expression were seen in transgenic bone carrying Col1a1-GFP visual reporters. Our data suggest that Col 2.3-Cre and Col 3.6-Cre transgenic mice may be useful for conditional gene targeting in vivo or for obtaining osteoblast populations for in vitro culture in which a gene of interest has been inactivated.

摘要

Cre/loxP重组系统可用于克服小鼠中广泛基因敲除的许多局限性。在此,我们展示了转基因小鼠的构建及特性,在这些小鼠中,Cre重组酶已通过大鼠Col1a1启动子的2.3 kb(Col 2.3-Cre)和3.6 kb(Col 3.6-Cre)片段靶向成骨细胞谱系细胞。在成年Col 2.3-Cre和Col 3.6-Cre小鼠的颅骨和长骨中检测到Cre mRNA,在Col 3.6-Cre小鼠的肌腱和皮肤中也检测到了Cre mRNA。为了获得Cre介导的基因重排的时间和空间模式的历史标记,将Col-Cre小鼠与ROSA26(R26R)小鼠杂交,在R26R小鼠中,Cre介导的对一个loxP侧翼盒的切除导致LacZ表达。在Col 2.3-Cre;R26R和Col 3.6-Cre;R26R后代中,颅骨和长骨成骨细胞在胚胎第18天和出生后第5天显示出强烈的β-半乳糖苷酶染色。在从Col 2.3-Cre;R26R小鼠建立的骨和骨髓基质培养物中,β-半乳糖苷酶染色的空间模式限制更大。在携带Col1a1-GFP视觉报告基因的转基因骨中也观察到了类似的表达空间模式差异。我们的数据表明,Col 2.3-Cre和Col 3.6-Cre转基因小鼠可能有助于体内条件性基因靶向,或用于获得其中感兴趣基因已失活的体外培养的成骨细胞群体。

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