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通过核转染技术使α1,3-半乳糖基转移酶基因失活和膜辅因子蛋白表达,用于猪到灵长类动物的异种移植。

Nucleofection-mediated α1,3-galactosyltransferase gene inactivation and membrane cofactor protein expression for pig-to-primate xenotransplantation.

机构信息

a Animal Biotechnology Division , National Institute of Animal Science , RDA , Suwon , South Korea.

出版信息

Anim Biotechnol. 2013;24(4):253-67. doi: 10.1080/10495398.2012.752741.

DOI:10.1080/10495398.2012.752741
PMID:23947662
Abstract

Xenotransplantation of pig organs into primates leads to hyperacute rejection (HAR). Functional ablation of the pig α 1,3-galactosyltransferase (GalT) gene, which abrogates expression of the Gal α 1-3Gal β 1-4GlcNAc-R (Gal) antigen, which inhibits HAR. However, antigens other than Gal may induce immunological rejection by their cognate antibody responses. Ultimately, overexpression of complement regulatory proteins reduces acute humoral rejection by non-Gal antibodies when GalT is ablated. In this study, we developed a vector-based strategy for ablation of GalT function and concurrent expression of membrane cofactor protein (MCP, CD46). We constructed an MCP expression cassette (designated as MCP-IRESneo) and inserted between the left and the right homologous arms to target exon 9 of the GalT gene. Nucleofection of porcine ear skin fibroblasts using the U-023 and V-013 programs resulted in high transfection efficiency and cell survival. We identified 28 clones in which the MCP-IRESneo vector had been successfully targeted to exon 9 of the GalT gene. Two of those clones, with apparent morphologically mitotic fibroblast features were selected through long-term culture. GalT gene expression was downregulated in these 2 clones. Importantly, MCP was shown to be efficiently expressed at the cell surface and to efficiently protect cell lysis against normal human complement serum attack in vitro.

摘要

猪器官异种移植到灵长类动物中会导致超急性排斥反应(HAR)。功能性敲除猪α1,3-半乳糖基转移酶(GalT)基因,可消除Gal α 1-3Gal β 1-4GlcNAc-R(Gal)抗原的表达,从而抑制 HAR。然而,除 Gal 之外的抗原可能会通过其同源抗体反应引起免疫排斥。最终,当 GalT 被敲除时,补体调节蛋白的过度表达可降低非 Gal 抗体引起的急性体液排斥反应。在这项研究中,我们开发了一种基于载体的策略来敲除 GalT 功能并同时表达膜辅因子蛋白(MCP,CD46)。我们构建了一个 MCP 表达盒(命名为 MCP-IRESneo),并将其插入 GalT 基因的左同源臂和右同源臂之间,以靶向外显子 9。使用 U-023 和 V-013 程序对猪耳皮成纤维细胞进行核转染,可获得高转染效率和细胞存活率。我们鉴定出 28 个成功靶向 GalT 基因外显子 9 的 MCP-IRESneo 载体克隆。其中 2 个克隆具有明显的有丝分裂成纤维细胞形态特征,通过长期培养筛选出来。这些克隆中 GalT 基因的表达下调。重要的是,MCP 在细胞表面得到有效表达,并在体外有效保护细胞免受正常人类补体血清的攻击。

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