首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Dissociation and reassociation of immobilized porphobilinogen synthase: use of immobilized subunits for enzyme isolation.
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Dissociation and reassociation of immobilized porphobilinogen synthase: use of immobilized subunits for enzyme isolation.

机译:固定化的胆色素原合酶的解离和重新结合:使用固定化的亚基进行酶分离。

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摘要

The dissociation and association of an immobilized preparation of the octameric enzyme porphobilinogen synthase [5-aminolevulinate hydro-lyase (adding 5-aminolevulinate and cyclizing), EC 4.2.1.24] is described. On treatment of the immobilized preparation with 4 M urea, four subunits per octamer are removed which can be reassociated into a soluble octameric enzyme. The tetrameric bound residual protein can also be reassembled into an octameric structure, with the same initial enzyme activity, by exposing the residual bound protein to a soluble pure enzyme preparation or to a crude liver extract in the presence of urea. The dissociation of the reconstituted bound enzyme releases subunits that again can be reassembled into a soluble octameric pure protein even when the crude liver preparation is used as the donor of the subunits. Thus, a pure enzyme can be isolated in a reassociation-dissociation cycle. The use of immobilized preparations of oligomeric proteins is considered for intra- and interspecies hybridization studies and for the ready preparation of purified enzyme preparations from different species and is suggested as a model for study of the formation of an oligomeric enzyme in the presence of other polypeptides.
机译:描述了八聚体酶胆色素原合酶[5-氨基乙酰丙酸酯水解酶(添加5-氨基乙酰丙酸酯并环化),EC 4.2.1.24)的固定制剂的解离和缔合。用4M尿素处理固定的制剂时,每个八聚体除去四个亚基,它们可以重新缔合成可溶性八聚体酶。通过将残留的结合蛋白暴露于可溶性纯酶制剂或在尿素存在下暴露于粗制肝提取物中,也可以将四聚体结合的残留蛋白重新组装成具有相同初始酶活性的八聚体结构。重组结合酶的解离释放出亚基,即使将粗肝制备物用作亚基的供体,亚基也可以再次组装成可溶性八聚体纯蛋白。因此,可以在再结合-解离循环中分离纯酶。考虑使用固定化的寡聚蛋白制剂进行种内和种间杂交研究,以及准备制备不同物种的纯化酶制剂,并被建议作为研究存在其他多肽时寡聚酶形成的模型。

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