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High pressure homogenization and the separation of soluble protein from recombinant Escherichia coli lysate using crossflow membrane filtration.

机译:高压均质化,并使用错流膜过滤从重组大肠杆菌裂解物中分离可溶性蛋白。

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Recombinant Escherichia coli often accumulates the recombinant protein of interest as insoluble inclusion bodies. Removing the soluble proteins from the inclusion bodies following cell disruption is a difficult processing step. Pretreatment of recombinant E. coli with 1.5 M guanidine HCl and 1.5% Triton X-100 allowed for reductions in the number of passes required for cell disruption and in the number of downstream processing steps required for the recovery of protein from the inclusion bodies. The combination of guanidine HCl and Triton X-100 gave higher permeate fluxes than guanidine HCl alone during crossflow membrane filtration of E. coli cell lysates. Low concentrations of urea had less of an effect on permeate flux and protein transmission than cell lysate solutions containing guanidine HCl. Increasing cell disruption had no effect on permeate flux and protein transmission because of the release of macromolecules and small cell debris after one pass through the high pressure homogenizer. A constant volume diafiltration process was developed to remove 84% of the UV
机译:重组大肠杆菌通常将目的重组蛋白积累为不溶性包涵体。细胞分裂后从包涵体中去除可溶性蛋白是困难的加工步骤。用1.5 M盐酸胍和1.5%Triton X-100预处理重组大肠杆菌可以减少细胞破坏所需的通过次数,并减少从包涵体中回收蛋白质所需的下游加工步骤。在大肠杆菌细胞裂解液的错流膜过滤过程中,盐酸胍和Triton X-100的组合产生的通量比单独盐酸胍更高。与含有盐酸胍的细胞裂解液相比,低浓度的尿素对渗透通量和蛋白质传输的影响较小。细胞破裂的增加对渗透通量和蛋白质传输没有影响,因为在高压匀浆器中通过一次之后,大分子的释放和小细胞碎片的释放。开发了恒定体积的渗滤工艺以去除84%的紫外线

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