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Direct Refolding of Inclusion Bodies Using Reversed Micelles

机译:使用反向胶束直接折叠包涵体

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The protein refolding of inclusion bodies was investigated using reversed micelles formed by aerosol OT(AOT).Ribonuclease A(RNase A)was overexpressed in Escherichia coli and used as native inclusion bodies.The enzymatic activity of RNase A was completely regained from the inclusion bodies within 14 h by solubilization in reversed micelles.To further enhance the refolding rate,a molecular chaperone,GroEL,was incorporated into the refolding system.The resultant refolding system including GroEL showed better performance under optimized conditions for the refolding of RNase A inclusion bodies.The refolding rate was considerably improved by the addition of the molecular chaperone,and the refolding step was completed in 1 h.The protein refolding in the GroEL-containing refolding system was strongly dependent on the coexistence of ATP and Mg~(2+),suggesting that the GroEL hosted in the reversed micelles was biologically active and assisted in the renaturation of the inclusion bodies.The addition of cold acetone to the reversed micellar solution allowed over 90% recovery of the renatured RNase A.
机译:使用由气溶胶OT(AOT)形成的反向胶束研究包涵体的蛋白重折叠。核糖核酸酶A(RNase A)在大肠杆菌中过表达并用作天然包涵体,从包涵体完全恢复了RNase A的酶活性。为了进一步提高重折叠率,在重折叠系统中加入了分子伴侣GroEL。为了进一步提高重折叠速度,在最佳条件下,包括GroEL在内的重折叠系统在RNase A包涵体的重折叠条件下表现出更好的性能。分子伴侣的加入使重折叠率大大提高,重折叠步骤在1 h内完成。含GroEL的重折叠系统中的蛋白质重折叠强烈依赖于ATP和Mg〜(2+)的共存,这表明反向胶束中的GroEL具有生物活性,并有助于包涵体的复性。将冷的丙酮离子加到逆胶束溶液中,可使回收的RNase A回收率超过90%。

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