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大肠杆菌鸟苷三磷酸环化水解酶I的纯化。在亲和色谱中使用竞争性抑制剂与底物作为配体。

Purification of guanosine triphosphate cyclohydrolase I from Escherichia coli. The use of competitive inhibitors versus substrate as ligands in affinity chromatography.

作者信息

Ferre J, Yim J J, Jacobson K B

出版信息

J Chromatogr. 1986 May 2;357(2):283-92. doi: 10.1016/s0021-9673(01)95830-3.

Abstract

Different affinity chromatography ligands have been compared for the purification of guanosine triphosphate (GTP) cyclohydrolase I, an enzyme that catalyses the transformation of GTP into formate and dihydroneopterin triphosphate, the first metabolite in the biosynthetic pathway of the pterins. When this enzyme is purified by affinity chromatography on GTP-Sepharose a major fraction of the activity is lost and the yield of enzyme decreases as the amount of enzyme applied to the column decreases. The use of nucleotide competitive inhibitors (UTP and ATP) as ligands in the affinity column has shown that the extent of inactivation of the enzyme is related to the affinity of the enzyme for the ligand. Further, the extent of inactivation was reduced by reducing the length of the columns when using the same volume of GTP-Sepharose. Dihydrofolate-Sepharose gave consistently higher yields of GTP cyclohydrolase I regardless of the amount of enzyme applied, but several other proteins were also obtained. For a high purification of GTP cyclohydrolase I the best yield may be obtained with UTP as the affinity ligand and with the shortest length possible of the affinity column, and the purity of enzyme is comparable with that obtained with GTP-Sepharose.

摘要

人们比较了不同的亲和层析配体用于纯化鸟苷三磷酸(GTP)环化水解酶I的效果。该酶催化GTP转化为甲酸和二氢新蝶呤三磷酸,后者是蝶呤生物合成途径中的首个代谢产物。当用GTP-琼脂糖亲和层析法纯化该酶时,随着上样量减少,大部分活性丧失,酶的产量也降低。在亲和柱中使用核苷酸竞争性抑制剂(UTP和ATP)作为配体表明,酶的失活程度与酶对配体的亲和力有关。此外,在使用相同体积的GTP-琼脂糖时,缩短柱长可降低失活程度。无论上样量多少,二氢叶酸-琼脂糖都能始终如一地获得较高产量的GTP环化水解酶I,但同时也会得到其他几种蛋白质。对于GTP环化水解酶I的高度纯化,以UTP作为亲和配体并使用尽可能短的亲和柱可获得最佳产量,且酶的纯度与用GTP-琼脂糖获得的相当。

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