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High-Level Expression of Single-Chain Fv-Fc Fusion Protein in Serum and Egg White of Genetically Manipulated Chickens by Using a Retroviral Vector

机译:逆转录病毒载体在转基因鸡的血清和蛋白中高表达单链Fv-Fc融合蛋白

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摘要

We report here the generation of transgenic chickens using a retroviral vector for the production of recombinant proteins. It was found that the transgene expression was suppressed when a Moloney murine leukemia virus-based retroviral vector was injected into chicken embryos at the blastodermal stage. When a concentrated viral solution was injected into the heart of developing embryos after 50 to 60 h of incubation, transgene expression was observed throughout the embryo, including the gonads. For practical production, a retroviral vector encoding an expression cassette of antiprion single-chain Fv fused with the Fc region of human immunoglobulin G1 (scFv-Fc) was injected into chicken embryos. The birds that hatched stably produced scFv-Fc in their serum and eggs at high levels (∼5.6 mg/ml). We obtained transgenic progeny from a transgenic chicken generated with this procedure. The transgene was stably integrated into the chromosomes of transgenic progeny. The transgenic progeny also expressed scFv-Fc in the serum and eggs.
机译:我们在这里报告了使用逆转录病毒载体生产重组蛋白产生的转基因鸡。发现在胚泡阶段将基于莫洛尼鼠白血病病毒的逆转录病毒载体注射到鸡胚中时,转基因表达受到抑制。孵育50至60小时后,将浓缩的病毒溶液注入发育中的胚胎的心脏,可在整个胚胎(包括性腺)中观察到转基因表达。为了实际生产,将编码与人类免疫球蛋白G1的Fc区(scFv-Fc)融合的抗pr病毒单链Fv表达盒的逆转录病毒载体注射到鸡胚中。稳定孵化的家禽在血清和卵中高水平(约5.6 mg / ml)产生scFv-Fc。我们从通过该程序产生的转基因鸡获得了转基因后代。转基因被稳定整合到转基因后代的染色体中。转基因子代还在血清和卵中表达scFv-Fc。

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