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Increasing protein production by directed vector backbone evolution

机译:通过定向载体主链进化提高蛋白质产量

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摘要

Recombinant protein production in prokaryotic and eukaryotic organisms was a key enabling technology for the rapid development of industrial and molecular biotechnology. However, despite all progress the improvement of protein production is an ongoing challenge and of high importance for cost-effective enzyme production. With the epMEGAWHOP mutagenesis protocol for vector backbone optimization we report a novel directed evolution based approach to increase protein production levels by randomly introducing mutations in the vector backbone. In the current study we validate the epMEGAWHOP mutagenesis protocol for three different expression systems. The latter demonstrated the general applicability of the epMEGAWHOP method. Cellulase and lipase production was doubled in one round of directed evolution by random mutagenesis of pET28a(+) and pET22b(+) vector backbones. Protease production using the vector pHY300PLK was increased ~4-times with an average of ~1.25 mutations per kb vector backbone. The epMEGAWHOP does not require any rational understanding of the expression machinery and can generally be applied to enzymes, expression vectors and related hosts. epMEGAWHOP is therefore from our point of view a robust, rapid and straight forward alternative for increasing protein production in general and for biotechnological applications.
机译:原核生物和真核生物中重组蛋白的生产是工业和分子生物技术快速发展的关键技术。然而,尽管取得了所有进展,但是蛋白质生产的改进仍是一个持续的挑战,并且对于具有成本效益的酶生产具有高度重要性。使用用于载体主链优化的epMEGAWHOP诱变方案,我们报道了一种新颖的基于定向进化的方法,通过在载体主链中随机引入突变来增加蛋白质的生产水平。在当前的研究中,我们验证了epMEGAWHOP诱变方案可用于三种不同的表达系统。后者证明了epMEGAWHOP方法的普遍适用性。通过随机诱变pET28a(+)和pET22b(+)载体骨架,在定向进化的一轮中,纤维素酶和脂肪酶的产量增加了一倍。使用载体pHY300PLK产生的蛋白酶增加了约4倍,每kb载体主链平均有1.25个突变。 epMEGAWHOP不需要对表达机制有任何合理的了解,并且通常可以应用于酶,表达载体和相关宿主。因此,从我们的角度来看,epMEGAWHOP是一种健壮,快速而直接的替代方案,可用于提高蛋白质的生产量以及用于生物技术领域。

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