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通过体内逆转录病毒转导雄性生殖系干细胞产生的转基因小鼠。

Transgenic mice produced by retroviral transduction of male germ line stem cells in vivo.

作者信息

Kanatsu-Shinohara Mito, Toyokuni Shinya, Shinohara Takashi

机构信息

Horizontal Medical Research Organization, Graduate School of Medicine, Kyoto University Yoshida-Konoe, Kyoto, Japan.

出版信息

Biol Reprod. 2004 Oct;71(4):1202-7. doi: 10.1095/biolreprod.104.031294. Epub 2004 Jun 9.

Abstract

Spermatogonial stem cells are the only stem cells in the postnatal body that can transmit parental genetic information to the offspring, making them an attractive target cell population for animal transgenesis. Although transgenic mice and rats were recently produced by retrovirus transduction of these cells in vitro, with transplantation of the transduced cells into infertile recipients, the difficulty of restoring fertility and preparing recipients using spermatogonial transplantation limits practical application of the technique. In this article, we describe a novel approach for producing transgenic animals by transducing spermatogonial stem cells in vivo using a retrovirus vector. Microinjection of retrovirus into immature seminiferous tubules resulted in the direct transduction of spermatogonial stem cells in situ, and the animals produced transgenic offspring after mating with females. Transgenic mice were produced in C57BL/6, BALB/C, A, and C3H backgrounds, with an average efficiency of 2.8%. The transgene was transmitted stably and expressed in the next generation. The technique overcomes the drawback of the in vitro-transduction approach, and will be useful as a novel method for producing transgenic animals as well as providing a means for analyzing the self-renewal and differentiation processes of spermatogonial stem cells in vivo.

摘要

精原干细胞是出生后体内唯一能够将亲代遗传信息传递给后代的干细胞,这使得它们成为动物转基因研究中极具吸引力的靶细胞群体。尽管最近通过体外逆转录病毒转导这些细胞并将转导后的细胞移植到不育受体中成功培育出了转基因小鼠和大鼠,但利用精原细胞移植恢复生育能力和制备受体的困难限制了该技术的实际应用。在本文中,我们描述了一种通过使用逆转录病毒载体在体内转导精原干细胞来生产转基因动物的新方法。将逆转录病毒显微注射到未成熟的生精小管中可导致精原干细胞原位直接转导,并且这些动物与雌性交配后产生了转基因后代。在C57BL/6、BALB/C、A和C3H背景下均成功培育出了转基因小鼠,平均效率为2.8%。转基因能够稳定遗传并在下一代中表达。该技术克服了体外转导方法的缺点,将作为一种生产转基因动物的新方法,同时也为体内分析精原干细胞的自我更新和分化过程提供了一种手段。

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