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Dicistronic expression of human proinsulin-protein A fusion in tobacco chloroplast

机译:人胰岛素原蛋白A融合蛋白在烟草叶绿体中的双顺反子表达

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Different expression systems such as bacteria and mammalian cells have been used to produce pharmaceutical proteins. In recent years, the use of plants as bioreactors offers efficient and economical systems in recombinant protein production. Furthermore, because of the large number of plastid copies in plants, chloroplast engineering functions as an effective method to increase recombinant protein expression. Because the commercially available insulin for treatment does not contain C-peptide, which is of great importance for type 1 diabetic patients, the current study introduces the human proinsulin gene fused with protein A into the tobacco chloroplast genome using the biolistic method. To achieve homoplasmy, three rounds of selection and regeneration of transforming cells were performed on the medium that contained spectinomycin antibiotic and hormones. The PCR analysis indicated the presence of the proinsulin gene in transplastomic plants. The reverse-transcription PCR analysis confirmed the expression of the proinsulin-proteinA fusion at the transcription level. Immunoblot assays of leaf-derived protein extracts confirmed that the target gene expression is up to 0.2% of the total soluble protein. Our study showed that protein A fusion is not as efficient as other reported fusions. The transplastomic plants were also confirmed for homoplasmy using Southern blot analysis.
机译:已经使用诸如细菌和哺乳动物细胞的不同表达系统来产生药物蛋白。近年来,将植物用作生物反应器在重组蛋白生产中提供了有效而经济的系统。此外,由于植物中大量的质体拷贝,叶绿体工程作为增加重组蛋白表达的有效方法。因为市售的治疗用胰岛素不包含C肽,这对1型糖尿病患者而言非常重要,所以本研究使用生物弹射法将与蛋白A融合的人胰岛素原基因引入到烟草叶绿体基因组中。为了实现同质性,在包含壮观霉素抗生素和激素的培养基上进行了三轮转化细胞的选择和再生。 PCR分析表明在转质体植物中存在胰岛素原基因。逆转录PCR分析在转录水平上证实了胰岛素原-蛋白A融合蛋白的表达。叶衍生蛋白提取物的免疫印迹分析证实,靶基因表达高达总可溶性蛋白的0.2%。我们的研究表明,蛋白A融合不如其他报道的融合有效。还使用Southern印迹分析确认了转质体植物的同质性。

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