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Comparison of various methods for periplasmic release of recombinant creatinase from Escherichia coli

机译:从大肠杆菌周质释放重组肌酐酶的各种方法的比较

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摘要

Various methods are compared for the periplasmic release of a recombinant creatinase from Escherichia coli. The examined methods include cell disruption (sonication and toluene/ethanol), chemical permeabilization (Triton X-100, guanidine-HCl, guanidine-HCl/ EDTA, chloroform, and glycine), and osmotic shock. It is found that methods involving the removal of lipopolysaccharide (such as guanidine-HCl/EDTA and osmotic shock) can achieve both excellent recovery and high purity. These findings indicate that the absence of lipopolysaccharide is closely related to the permeability for periplasmic release. Since it is based on diffusion, guanidine-HCl/EDTA achieves a much slower rate of periplasmic release than osmotic shock, which is based on shrinkage-and-swelling pumping. Osmotic shock can be further improved by using lysozyme or Ca2+-pretreatment, where the latter is seemingly the most suitable method for periplasmic release.
机译:比较了从大肠杆菌中周质释放重组肌酐酶的各种方法。检查的方法包括细胞破裂(超声处理和甲苯/乙醇),化学通透性(Triton X-100,胍盐酸盐,胍盐酸盐/ EDTA,氯仿和甘氨酸)和渗透压休克。已经发现,涉及去除脂多糖的方法(例如胍盐酸盐/ EDTA和渗透压休克)可以实现优异的回收率和高纯度。这些发现表明,脂多糖的缺乏与周质释放的渗透性密切相关。由于基于扩散,胍盐酸盐/ EDTA的周质释放速率比渗透压休克要慢得多,渗透压休克基于收缩和溶胀泵送。通过使用溶菌酶或Ca2 +预处理可以进一步改善渗透压休克,后者似乎是最适合周质释放的方法。

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