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利用慢病毒载体在小鼠中皮肤特异性转基因表达具有生物活性的人细胞毒性 T 淋巴细胞相关抗原 4-免疫球蛋白(hCTLA4Ig)。

Skin-specifically transgenic expression of biologically active human cytoxic T-lymphocyte associated antigen4-immunoglobulin (hCTLA4Ig) in mice using lentiviral vector.

机构信息

Department of Laboratory Animal Science, College of Basic Medical Sciences, Third Military Medical University, Gao Tan-yan Street, Shapingba District, Chongqing 400038, China.

出版信息

Transgenic Res. 2012 Jun;21(3):579-91. doi: 10.1007/s11248-011-9559-x. Epub 2011 Oct 8.

Abstract

Xenogeneic skin, especially porcine skin, has already been used to cover large wounds in clinic practice of wound care. Our previous data showed that transgenic expression of human cytoxic T-lymphocyte associated antigen4-immunoglobulin (hCTLA4Ig) in murine skin graft remarkably prolonged its survival in xenogeneic burn wounds without extensive immunosuppression in recipients, suggesting that transgenic hCTLA4Ig expression in skin graft may be an effective and safe method to prolong its survival in xenogeneic wounds for coverage. Lentiviral transgenesis provides an extremely efficient and cost-effective method to produce transgenic animals. However, tissue-targeted transgenic expression of biologically functional protein by lentiviral transgenesis is rarely reported. In this work, a recombinant lentiviral vector (LV), named FKCW in this article, was constructed by inserting a skin-specific hCTLA4Ig expression cassette consisting of keratin 14 (K14) promoter, hCTLA4Ig coding sequence and an intronic fragment. Its efficacy for transgenesis and skin-specific expression of bio-active hCTLA4Ig protein was tested using mice as models. The LV FKCW was readily to be packaged and concentrated to high titres (1.287-6.254 × 10(9) TU/ml) by conventional lentivirus package system. Using eggs collected from only five mated females having been subjected to conventional super-ovulation treatment, 8 hCTLA4Ig transgenic founder mice were generated with the concentrated FKCW vector, and transgenic founder per injected and transferred egg was 6.3%, which was nearly 9-fold higher than that for DNA micro-injection with a similar transgene construct in our previous work. The lentiviral transgenic hCTLA4Ig exhibited strictly skin-specific expression at a level comparable to or even slightly higher than that of transgenic hCTLA4Ig delivered by micro-injection in a similar cassette. Lentiviral transgenic hCTLA4Ig protein remarkably suppressed human lymphocyte proliferation in vitro to a degree comparable to that of commercially purchased purified hCTLA4Ig protein with defined activity at similar concentrations. Besides, lentiviral hCTLA4Ig transgenic mouse skin grafted into rat burn wounds exhibited remarkably extended survival compared to wild-type skin of the same strain (13.8 ± 3.8 vs. 6.8 ± 3.0 days), indicating that lentiviral transgenic hCTLA4Ig did inhibit immune rejection against xenogeneic skin graft in vivo. These results laid down the foundation to further efficiently generate transgenic pigs skin-specifically expressing bio-active hCTLA4Ig by lentiviral transgenesis, and provided a demonstration that transgenic animals with tissue-targeted expression of biologically functional protein can be efficiently produced using LV.

摘要

异种皮肤,特别是猪皮,已被用于临床创伤护理中覆盖大面积伤口。我们之前的数据表明,在接受者中没有广泛免疫抑制的情况下,转基因表达人细胞毒性 T 淋巴细胞相关抗原 4 免疫球蛋白(hCTLA4Ig)在鼠皮移植物中显著延长了其存活时间,这表明转基因 hCTLA4Ig 在皮移植物中的表达可能是一种有效且安全的方法,可以延长其在异种伤口中的存活时间以进行覆盖。慢病毒转基因提供了一种极其高效和具有成本效益的方法来产生转基因动物。然而,通过慢病毒转基因进行组织靶向的生物活性蛋白的转基因表达很少有报道。在这项工作中,构建了一种重组慢病毒载体(LV),本文中命名为 FKCW,它是通过插入一个由角蛋白 14(K14)启动子、hCTLA4Ig 编码序列和内含子片段组成的皮肤特异性 hCTLA4Ig 表达盒而构建的。使用小鼠作为模型,测试了它用于转基因和生物活性 hCTLA4Ig 蛋白的皮肤特异性表达的功效。LV FKCW 很容易通过常规慢病毒包装系统进行包装和浓缩至高滴度(1.287-6.254×10(9)TU/ml)。使用仅接受过常规超排卵处理的五只交配雌性收集的卵,使用浓缩的 FKCW 载体产生了 8 只 hCTLA4Ig 转基因创始鼠,每注射和转移的卵中产生转基因创始鼠的比例为 6.3%,这几乎比我们之前使用类似转基因构建体进行 DNA 微注射的比例高 9 倍。慢病毒转基因 hCTLA4Ig 表现出严格的皮肤特异性表达,其水平与微注射类似盒中递送的转基因 hCTLA4Ig 相当,甚至略高。慢病毒转基因 hCTLA4Ig 蛋白在体外显著抑制人淋巴细胞增殖,抑制程度与具有相似活性的商业购买的纯化 hCTLA4Ig 蛋白在相似浓度下相当。此外,与同一品系的野生型皮肤(13.8±3.8 天)相比,转基因 hCTLA4Ig 转基因鼠皮移植到大鼠烧伤创面后存活时间显著延长,表明慢病毒转基因 hCTLA4Ig 确实抑制了异种皮肤移植物的免疫排斥反应。这些结果为进一步通过慢病毒转基因高效产生皮肤特异性表达生物活性 hCTLA4Ig 的转基因猪皮奠定了基础,并证明了使用 LV 可以高效地产生具有组织靶向表达生物功能蛋白的转基因动物。

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