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Design of experiments‐based high‐throughput strategy for development and optimization of efficient cell disruption protocols

机译:设计基于实验的高通量策略以开发和优化有效的细胞分裂方案

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摘要

Efficient and reproducible cell lysis is a crucial step during downstream processing of intracellular products. The composition of an optimal lysis buffer should be chosen depending on the organism, its growth status, the applied detection methods, and even the target molecule. Especially for high‐throughput applications, where sample volumes are limited, the adaptation of a lysis buffer to the specific campaign is an urgent need. Here, we present a general design of experiments‐based strategy suitable for eight constituents and demonstrate the strength of this approach by the development of an efficient lysis buffer for Gram‐negative bacteria, which is applicable in a high‐throughput format in a short time. The concentrations of four lysis‐inducing chemical agents EDTA, lysozyme, Triton X‐100, and polymyxin B were optimized for maximal soluble protein concentration and ß‐galactosidase activity in a 96‐well format on a Microlab Star liquid handling platform under design of experiments methodology. The resulting lysis buffer showed the same performance as a commercially available lysis buffer. The developed protocol resulted in an optimized buffer within only three runs. The established procedure can be easily applied to adapt the lysis buffer to other strains and target molecules.
机译:高效且可重现的细胞裂解是细胞内产物下游加工过程中的关键步骤。最佳裂解缓冲液的组成应根据生物体,其生长状态,应用的检测方法甚至目标分子进行选择。尤其是对于样品量有限的高通量应用,迫切需要使裂解缓冲液适应特定活动。在这里,我们介绍适用于八种成分的基于实验的策略的总体设计,并通过开发革兰氏阴性细菌的高效裂解缓冲液来证明这种方法的优势,该缓冲液可在短时间内以高通量形式应用。在Microlab Star液体处理平台上,根据实验设计,对四种裂解诱导化学试剂EDTA,溶菌酶,Triton X-100和多粘菌素B的浓度进行了优化,以在96孔形式下实现最大可溶性蛋白浓度和ß-半乳糖苷酶活性。方法。所得裂解缓冲液显示出与市售裂解缓冲液相同的性能。开发的协议仅在三个运行中就产生了优化的缓冲区。既定的程序可轻松应用于使裂解缓冲液适应其他菌株和目标分子。

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