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An optimized growth medium for increased recombinant protein secretion titer via the type III secretion system

机译:通过III型分泌系统增加重组蛋白分泌滴度的优化生长培养基

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Protein secretion in bacteria is an attractive strategy for heterologous protein production because it retains the high titers and tractability of bacterial hosts while simplifying downstream processing. Traditional intracellular production strategies require cell lysis and separation of the protein product from the chemically similar cellular contents, often a multi-step process that can include an expensive refolding step. The type III secretion system of Salmonella enterica Typhimurium transports proteins from the cytoplasm to the extracellular environment in a single step and is thus a promising solution for protein secretion in bacteria. Product titer is sensitive to extracellular environmental conditions, however, and T3SS regulation is integrated with essential cellular functions. Instead of attempting to untangle a complex web of regulatory input, we took an “outside-in” approach to elucidate the effect of growth medium components on secretion titer. We dissected the individual and combined effects of carbon sources, buffers, and salts in a rich nutrient base on secretion titer. Carbon sources alone decreased secretion titer, secretion titer increased with salt concentration, and the combination of a carbon source, buffer, and high salt concentration had a synergistic effect on secretion titer. Transcriptional activity measured by flow cytometry showed that medium composition affected secretion system activity, and prolonged secretion system activation correlated strongly with increased secretion titer. We found that an optimal combination of glycerol, phosphate, and sodium chloride provided at least a fourfold increase in secretion titer for a variety of proteins. Further, the increase in secretion titer provided by the optimized medium was additive with strain enhancements. We leveraged the sensitivity of the type III secretion system to the extracellular environment to increase heterologous protein secretion titer. Our results suggest that maximizing secretion titer via the type III secretion system is not as simple as maximizing secreted protein expression—one must also optimize secretion system activity. This work advances the type III secretion system as a platform for heterologous protein secretion in bacteria and will form a basis for future engineering efforts.
机译:细菌中的蛋白质分泌是异源蛋白质产生的一种有吸引力的策略,因为它保留了细菌宿主的高滴度和易腐蚀性,同时简化了下游加工。传统的细胞内生产策略需要细胞裂解和分离蛋白质产品从化学上类似的细胞内容物,通常是可以包括昂贵的重折叠步骤的多步骤。 Salmonella肠毒蕈金的III型分泌系统在单一步骤中将蛋白质从细胞质转移到细胞外环境中,因此是细菌中蛋白质分泌的有希望的解决方案。产品滴度对细胞外环境条件敏感,然而,T3SS调节与必要的细胞功能集成。我们不是试图解开一个复杂的监管投入网络,我们采取了“外面的”方法,以阐明生长培养基组分对分泌滴度的影响。我们解释了碳源,缓冲液和盐在分泌滴度的富含营养碱中的个体和综合影响。单独碳源降低分泌滴度,分泌滴度随盐浓度而增加,碳源,缓冲液和高盐浓度的组合对分泌滴度具有协同作用。通过流式细胞术测量的转录活性显示培养基组合物影响分泌系统活性,并且延长分泌系统激活与分泌滴度增加的分泌强烈相关。我们发现甘油,磷酸盐和氯化钠的最佳组合提供了各种蛋白质的分泌滴度的至少四倍增加。此外,优化介质提供的分泌滴度的增加是菌株增强的添加剂。我们利用III型分泌系统对细胞外环境的敏感性来增加异源蛋白质分泌滴度。我们的研究结果表明,通过III型分泌系统最大化分泌滴度并不像最大化分泌的蛋白表达一样简单,也必须优化分泌系统活性。这项工作将III型分泌系统推进作为细菌中异源蛋白质分泌的平台,并将成为未来工程努力的基础。

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