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Efficient recombinant protein production and secretion from nuclear transgenes in Chlamydomonas reinhardtii

机译:莱茵衣藻中高效重组蛋白的生产和核转基因的分泌

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Microalgae are diverse photosynthetic microbes which offer the potential for production of a number of high value products (HVP) such as pigments, oils, and bio-active compounds. Fast growth rates, ease of photo-autotrophic cultivation, unique metabolic properties and continuing progress in algal transgenics have raised interest in the use of microalgae systems for recombinant protein (RP) production. This work demonstrates the development of an advanced RP production and secretion system for the green unicellular model alga Chlamydomonas reinhardtii. We generated a versatile expression vector that employs the secretion signal of the native extracellular C reinhardtii carbonic anhydrase for efficient RP secretion into the culture medium. Unique restriction sites were placed between the regulatory elements to allow fast and easy sub-cloning of sequences of interest. Positive transformants can rapidly be identified by high-throughput plate-level screens via a coupled Gaussia luciferase marker. The vector was tested in Chlamydomonas wild type CC-1883 (WT) and in the transgene expression transformant UVM4. Compared to the native secretion signal of the Gaussia luciferase, up to 84% higher RP production could be achieved. With this new expression system we could generate transformants that express up to 10 mg RP per liter culture without further optimization. The target RP is found exclusively in culture medium and can therefore easily be isolated and purified. We conclude that this new expression system will be a valuable tool for many heterologous protein expression applications from C. reinhardtii in the future
机译:微藻是多种光合微生物,它们具有生产多种高价值产品(HVP)的潜力,例如颜料,油和生物活性化合物。快速的生长速度,易于光合自养的培养,独特的代谢特性以及藻类转基因技术的持续发展引起了人们对使用微藻系统生产重组蛋白(RP)的兴趣。这项工作演示了绿色单细胞模型藻衣藻的先进RP产生和分泌系统的开发。我们生成了一种多功能表达载体,该载体利用天然细胞外C莱茵碳碳酸酐酶的分泌信号将RP有效地分泌到培养基中。独特的限制性酶切位点位于调控元件之间,可快速,轻松地亚克隆目标序列。可通过偶联的高斯荧光素酶标记物,通过高通量板级筛选快速鉴定出阳性转化子。在衣藻CC-1883野生型(WT)和转基因表达转化体UVM4中测试了该载体。与高斯荧光素酶的天然分泌信号相比,可以实现高达84%的更高的RP产量。使用这种新的表达系统,我们无需进一步优化即可生成每升培养物中表达最高10 mg RP的转化体。目标RP仅存在于培养基中,因此可以轻松分离和纯化。我们得出的结论是,这个新的表达系统将是将来在莱茵衣藻中许多异源蛋白质表达应用的有价值的工具

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