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从MSM/Ms品系建立具有种系能力的胚胎干细胞系。

Establishment of germline-competent embryonic stem cell lines from the MSM/Ms strain.

作者信息

Araki Kimi, Takeda Naoki, Yoshiki Atsushi, Obata Yuichi, Nakagata Naomi, Shiroishi Toshihiko, Moriwaki Kazuo, Yamamura Ken-ichi

机构信息

Department of Developmental Genetics, Institute of Molecular Embryology and Genetics, Kumamoto University, Honjo 2-2-1, Kumamoto, 860-0811, Japan.

出版信息

Mamm Genome. 2009 Jan;20(1):14-20. doi: 10.1007/s00335-008-9160-7. Epub 2008 Dec 12.

DOI:10.1007/s00335-008-9160-7
PMID:19082856
Abstract

MSM/Ms is an inbred mouse strain established from the Japanese wild mouse, Mus musculus molossinus, which has been phylogenetically distinct from common laboratory mouse strains for about 1 million years. The nucleotide substitution rate between MSM/Ms and C57BL/6 is estimated to be 0.96%. MSM/Ms mice display unique characteristics not observed in the commonly used laboratory strains, including an extremely low incidence of tumor development, high locomotor activity, and resistance to high-fat-diet-induced diabetes. Thus, functional genomic analyses using MSM/Ms should provide a powerful tool for the identification of novel phenotypes and gene functions. We report here the derivation of germline-competent embryonic stem (ES) cell lines from MSM/Ms blastocysts, allowing genetic manipulation of the M. m. molossinus genome. Fifteen blastocysts were cultured in ES cell medium and three ES lines, Mol/MSM-1, -2, and -3, were established. They were tested for germline competency by aggregation with ICR morulae and germline chimeras were obtained from all three lines. We also injected Mol/MSM-1 ES cells into blastocysts of ICR or C57BL/6 x BDF1 mice and found that blastocyst injection resulted in a higher production rate of chimeric mice than did aggregation. Furthermore, Mol/MSM-1 subclones electroporated with a gene trap vector were also highly efficient at producing germline chimeras using C57BL/6 x BDF1 blastocyst injection. This Mol/MSM-1 ES line should provide an excellent new tool allowing the genetic manipulation of the MSM/Ms genome.

摘要

MSM/Ms是一种从日本野生小家鼠(Mus musculus molossinus)培育而来的近交系小鼠品系,在系统发育上与常见的实验室小鼠品系已经分化了约100万年。MSM/Ms与C57BL/6之间的核苷酸替换率估计为0.96%。MSM/Ms小鼠表现出常用实验室品系中未观察到的独特特征,包括极低的肿瘤发生率、高运动活性以及对高脂饮食诱导的糖尿病具有抗性。因此,使用MSM/Ms进行功能基因组分析应该为鉴定新的表型和基因功能提供一个强大的工具。我们在此报告从MSM/Ms囊胚中获得具有生殖系能力的胚胎干细胞(ES)系,从而能够对小家鼠基因组进行遗传操作。将15个囊胚在ES细胞培养基中培养,建立了3个ES系,即Mol/MSM-

1、-2和-3。通过与ICR桑椹胚聚集来测试它们的生殖系能力,并且从所有3个系都获得了生殖系嵌合体。我们还将Mol/MSM-1 ES细胞注射到ICR或C57BL/6×BDF1小鼠的囊胚中,发现囊胚注射产生嵌合小鼠的效率高于聚集法。此外,用基因捕获载体电穿孔的Mol/MSM-1亚克隆在使用C57BL/6×BDF1囊胚注射产生生殖系嵌合体方面也非常高效。这个Mol/MSM-1 ES系应该提供一个出色的新工具,用于对MSM/Ms基因组进行遗传操作。

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