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利用 BAC 衍生的全长基因和胞质内精子注射介导的基因转移技术创建表达人蛋白的转基因猪。

The creation of transgenic pigs expressing human proteins using BAC-derived, full-length genes and intracytoplasmic sperm injection-mediated gene transfer.

机构信息

Nakauchi Stem Cell and Organ Regeneration Project, Japan Science and Technology Agency (JST), ERATO, 4-6-1 Shirokanedai, Minato-ku, Tokyo 108-8639, Japan.

出版信息

Transgenic Res. 2012 Jun;21(3):605-18. doi: 10.1007/s11248-011-9561-3. Epub 2011 Oct 25.

DOI:10.1007/s11248-011-9561-3
PMID:22038447
Abstract

In most transgenic (Tg) animals created to date, a transgene consisting of the minimum promoter region linked to a cDNA has been used. However, transgenes on small plasmids are susceptible to the position effect, increasing the difficulty of controlling transgene expression. In this study, we attempted to create Tg pigs by intracytoplasmic sperm injection-mediated gene transfer (ICSI-MGT) using two large genomic transgenes derived from a bacterial artificial chromosome (BAC) containing the full genomic region encoding two human proteins, type I collagen and albumin. The production efficiencies (Tg piglets/live offspring) of type I collagen and albumin Tg pigs were 11.8% (6/51) and 18.2% (2/11), respectively. In all of the Tg pigs examined by real-time PCR analysis, tissue-specific expression of the transgene was confirmed (type I collagen: skin, tendon, vessels, genitalia; albumin: liver). The production of human proteins derived from BAC transgenes was also confirmed. Fluorescence in situ hybridization analysis indicated that the BAC transgenes transferred into porcine oocytes by ICSI-MGT were integrated into single or multiple sites on the host chromosomes. These data demonstrate that Tg pigs expressing human proteins in a tissue-specific manner can be created using a BAC transgenic construct and the ICSI-MGT method.

摘要

在迄今为止创建的大多数转基因 (Tg) 动物中,使用的是由最小启动子区域与 cDNA 连接而成的转基因。然而,小质粒上的转基因易受位置效应的影响,增加了控制转基因表达的难度。在这项研究中,我们尝试通过胞质内精子注射介导的基因转移 (ICSI-MGT) 使用来自包含编码两种人类蛋白质(I 型胶原和白蛋白)的全长基因组区域的细菌人工染色体 (BAC) 的两个大型基因组转基因来创建 Tg 猪。I 型胶原和白蛋白 Tg 猪的生产效率(Tg 仔猪/活产仔数)分别为 11.8%(6/51)和 18.2%(2/11)。通过实时 PCR 分析检查的所有 Tg 猪中,均证实了转基因的组织特异性表达(I 型胶原:皮肤、肌腱、血管、生殖器官;白蛋白:肝脏)。还证实了源自 BAC 转基因的人类蛋白的产生。荧光原位杂交分析表明,通过 ICSI-MGT 转入猪卵母细胞的 BAC 转基因被整合到宿主染色体的单个或多个位点上。这些数据表明,使用 BAC 转基因构建体和 ICSI-MGT 方法可以创建以组织特异性方式表达人类蛋白的 Tg 猪。

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