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外源DNA整合到小鼠、大鼠、兔和猪基因组中的比较研究。

A comparative study on the integration of exogenous DNA into mouse, rat, rabbit, and pig genomes.

作者信息

Hirabayashi M, Takahashi R, Ito K, Kashiwazaki N, Hirao M, Hirasawa K, Hochi S, Ueda M

机构信息

YS New Technology Inst., Inc., 519 Shimoishibashi, Ishibashi-machi, Shimotsuga-gun, Tochigi 329-0512, Japan.

出版信息

Exp Anim. 2001 Apr;50(2):125-31. doi: 10.1538/expanim.50.125.

Abstract

Transgenic mammals, from small laboratory rodents to domestic animals, have been successfully produced to date, but their production efficiency within or across species has been variable. This is probably due to the differences in the type of injected DNA and/or technical procedures employed in each laboratory, as well as the reproductive characteristics of the species. Here we report the direct comparison of the efficiencies of producing transgenic mice, rats, rabbits and pigs by one technician using a fusion gene composed of the bovine alpha S1-casein promoter and human growth hormone (hGH) gene. Before the fusion gene was injected into the zygotes, high magnitude centrifugation to visualize the pronuclei was necessary for all of the pig zygotes and one-third of the rabbit zygotes, but not for mouse and rat zygotes. Post-injection survival of the mouse zygotes (67.1%) was lower than those of the rat, rabbit and pig zygotes (89.6 to 100%). The volume change of the pronucleus following DNA injection was the lowest in mice (50% increase), moderate in rabbits (148% increase), and the most prominent in rats (238% increase). The data from only 1 pig zygote indicated a 22% increase in the pronucleus volume by DNA injection. The PCR analyses of the tail DNA of new born offspring indicated that 0.8% (4/493), 4.8% (22/463), 0.8% (3/367) and 0.9% (2/221) of the injected eggs in mice, rats, rabbits and pigs, respectively, developed into transgenic offspring. Some of the founder animals in all four species expressed the transgene in the mammary gland which was confirmed in hGH mRNA by RT-PCR and/or hGH peptide in Witch's milk with ELISA. These results suggest that the maximum volume of DNA solution injectable into the pronucleus is a possible factor explaining the species differences in the production of transgenic animals.

摘要

迄今为止,已经成功培育出从小型实验啮齿动物到家畜的转基因哺乳动物,但其在种内或种间的生产效率各不相同。这可能是由于每个实验室所使用的注射DNA类型和/或技术程序不同,以及物种的繁殖特性所致。在此,我们报告了一位技术人员使用由牛αS1-酪蛋白启动子和人生长激素(hGH)基因组成的融合基因生产转基因小鼠、大鼠、兔子和猪的效率的直接比较。在将融合基因注射到受精卵之前,对所有猪受精卵和三分之一的兔子受精卵进行高强度离心以观察原核是必要的,但对小鼠和大鼠受精卵则不需要。小鼠受精卵注射后的存活率(67.1%)低于大鼠、兔子和猪受精卵(89.6%至100%)。DNA注射后原核的体积变化在小鼠中最小(增加50%),在兔子中适中(增加148%),在大鼠中最显著(增加238%)。仅来自1个猪受精卵的数据表明,DNA注射后原核体积增加了22%。对新生后代尾巴DNA的PCR分析表明,小鼠、大鼠、兔子和猪中分别有0.8%(4/493)、4.8%(22/463)、0.8%(3/367)和0.9%(2/221)的注射卵发育成了转基因后代。所有四个物种的一些奠基动物在乳腺中表达了转基因,这通过RT-PCR检测hGH mRNA和/或用ELISA检测初乳中的hGH肽得到了证实。这些结果表明,可注射到原核中的DNA溶液的最大体积可能是解释转基因动物生产中物种差异的一个因素。

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