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Optimization of the expression of the HIV fusion inhibitor cyanovirin?¢????N from the tobacco plastid genome

机译:烟草质体基因组中HIV融合抑制剂cyanovirin?N?N的表达优化

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Plants with transgenic plastid (chloroplast) genomes represent a promising production platform in molecular farming, mainly because of the plastids?¢???? potential to accumulate foreign proteins to very high levels and the increased biosafety conferred by the maternal mode of plastid inheritance. Although some transgenes can be expressed to extraordinarily high levels, the expression of others has been unsuccessful. Lack of detectable transgene expression is usually attributable to either RNA instability or protein instability. Here, we have investigated the possibilities to improve the production of a pharmaceutical protein that is difficult to express in chloroplasts: the HIV?¢????1 fusion inhibitor cyanovirin?¢????N (CV?¢????N). Testing various N?¢????terminal and C?¢????terminal fusions to peptide sequences from two proteins known to accumulate to high levels in transgenic plastids (GFP and the protein antibiotic PlyGBS), we show that both low mRNA stability and low protein stability contribute to the lack of detectable CV?¢????N expression in chloroplasts. Both problems can be alleviated by N?¢????terminal fusions to the CV?¢????N coding region, thus highlighting a suitable strategy for optimization of plastid transgene expression.
机译:具有转基因质体(叶绿体)基因组的植物代表了分子农业中一个有希望的生产平台,这主要是由于质体的原因。潜在地将外来蛋白质积累到很高的水平,并通过母体质体遗传方式提高了生物安全性。尽管某些转基因可以高水平表达,但其他表达却不成功。缺乏可检测的转基因表达通常归因于RNA不稳定或蛋白质不稳定。在这里,我们研究了改善难以在叶绿体中表达的药物蛋白的生产的可能性:HIV-1融合抑制剂cyanovirin 1 N(CV 2? N)。从已知在转基因质体中积累到高水平的两种蛋白质(GFP和蛋白质抗生素PlyGBS)测试肽序列的各种Nα-β-末端和Cα-β-末端融合,我们发现这两种mRNA均低稳定性和较低的蛋白质稳定性导致叶绿体中缺乏可检测的CV→N→N表达。这两个问题都可以通过与CV 3 -N N编码区的N 2 -C 3末端融合而得到缓解,因此突出了优化质体转基因表达的合适策略。

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