从β -半乳糖苷酶(大肠杆菌)中提取大量α -互补肽的一种快速纯化方法。

Preparative biochemistry Pub Date : 1994-11-01 DOI:10.1080/10826069408010101
C N Gallagher, N J Roth, R E Huber
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引用次数: 5

摘要

将编码-半乳糖苷酶残基6-44的DNA片段连接到含有谷胱甘肽- s转移酶基因的载体上,该基因还含有编码凝血酶识别位点的序列。融合蛋白与载体编码的另外9个氨基酸,使用谷胱甘肽琼脂糖亲和柱纯化。然后用凝血酶从谷胱甘肽- s -转移酶上切割出由-半乳糖苷酶残基6-44和另外9个氨基酸组成的肽,并用凝胶过滤柱纯化。该肽的α -互补活性是野生型β -半乳糖苷酶CNBr酶切得到的α -肽的3-4倍。
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A rapid method for the purification of large amounts of an alpha-complementing peptide derived from beta-galactosidase (E. coli).

A DNA segment coding for residues 6-44 of beta-galactosidase was ligated to a vector with the glutathione-S-transferase gene which also contained a sequence coding for a thrombin recognition site. The fused protein, with an additional 9 amino acids coded for by the vector, was purified using a glutathione agarose affinity column. A peptide made up of residues 6-44 of beta-galactosidase and the 9 additional amino acids was then cleaved from the glutathione-S-transferase using thrombin and purified with a gel filtration column. The peptide was about 3-4 times as active for alpha-complementation as the alpha-peptide derived from CNBr digestion of wild type beta-galactosidase.

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Preparative biochemistry
Preparative biochemistry
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