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Construction of a recombinant human insulin expression vector for mammary gland-specific expression in buffalo (Bubalus bubalis) mammary epithelial cell line

机译:用于在水牛乳腺上皮细胞系中乳腺特异性表达的重组人胰岛素表达载体的构建

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The aim of the present study was construction of mammary gland specific expression vector for high level of human insulin (hINS) expression in transgenic buffalo for therapeutic use. We have constructed mammary gland specific vector containing human insulin gene and there expression efficiency was checked into in vitro cultured buffalo mammary epithelial cells (BuMECs). Human pro-insulin coding region was isolated from human genomic DNA by intron skipping PCR primer and furin cleavage site was inserted between B-C and C-A chain of human insulin by overlap extension PCR. A mammary gland-specific buffalo beta-lactoglobulin promoter was isolated from buffalo DNA and used for human insulin expression in BuMEC cells. The construct was transfected into BuMECs by lipofection method and positive transgene cell clones were obtained by G418 selection after 3 weeks. Expression of hINS in transfected cells were confirmed by RT-PCR, Immunocytochemistry, Western Blotting and ELISA. The pAcISUBC insulin-expressing clones secreted insulin at varying levels between 0.18 - 1.43 ng/ml/24 h/2.0 x 10(6) cells.
机译:本研究的目的是构建用于在转基因水牛中高水平表达人胰岛素(hINS)的乳腺特异性表达载体,以进行治疗。我们构建了含有人胰岛素基因的乳腺特异性载体,并在体外培养的水牛乳腺上皮细胞(BuMEC)中检测了表达效率。通过内含子跳过PCR引物从人基因组DNA分离人胰岛素原编码区,并通过重叠延伸PCR将弗林蛋白酶切割位点插入人胰岛素的B-C和C-A链之间。从水牛DNA中分离出乳腺特异性水牛β-乳球蛋白启动子,并将其用于人胰岛素在BuMEC细胞中的表达。通过脂转染法将该构建体转染到BuMEC中,并在3周后通过G418选择获得阳性转基因细胞克隆。 hINS在转染细胞中的表达通过RT-PCR,免疫细胞化学,蛋白质印迹和ELISA来证实。表达pAcISUBC胰岛素的克隆以0.18-1.43 ng / ml / 24 h / 2.0 x 10(6)细胞之间的不同水平分泌胰岛素。

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