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人乳中乳糖合成酶A蛋白的巯基及尿苷二磷酸半乳糖与该酶结合的研究。

Studies on the thiol group of lactose synthetase A protein from human milk and on the binding of uridine diphosphate galactose to the enzyme.

作者信息

Kitchen B J, Andrens P

出版信息

Biochem J. 1974 Jul;141(1):173-8. doi: 10.1042/bj1410173.

Abstract

The lactose synthetase activity of A protein from human milk was much decreased but not abolished by reaction with thiol-group reagents. Protection experiments indicated that a free thiol group on the enzyme is situated near the UDP-galactose binding site and inactivation of the enzyme with p-hydroxymercuribenzoate was probably due to prevention of UDP-galactose binding. Affinity chromatography showed that the mercuribenzoate substituent also decreased the affinity of A protein for N-acetylglucosamine but complex-formation between A protein-N-acetylglucosamine and alpha-lactalbumin was relatively unaffected. UDP-galactose appears to be bound to the enzyme mainly through its pyrophosphate group with Mn(2+) ion and through the cis hydroxyls of ribose, whereas its hexose moiety has little if any affinity for the enzyme. Lactose synthetase activity remaining after the reaction with thiol-group reagents indicates that a free thiol group is not an essential part of the A protein active site.

摘要

人乳中A蛋白的乳糖合成酶活性在与巯基试剂反应后大幅降低,但并未完全消除。保护实验表明,酶上的一个游离巯基位于UDP-半乳糖结合位点附近,对羟基汞苯甲酸使酶失活可能是由于阻止了UDP-半乳糖的结合。亲和层析显示,汞苯甲酸取代基也降低了A蛋白对N-乙酰葡糖胺的亲和力,但A蛋白-N-乙酰葡糖胺与α-乳白蛋白之间的复合物形成相对未受影响。UDP-半乳糖似乎主要通过其焦磷酸基团与Mn(2+)离子以及核糖的顺式羟基与酶结合,而其己糖部分对该酶的亲和力很小(如果有的话)。与巯基试剂反应后剩余的乳糖合成酶活性表明,游离巯基不是A蛋白活性位点的必需部分。

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本文引用的文献

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Tissue sulfhydryl groups.组织巯基
Arch Biochem Biophys. 1959 May;82(1):70-7. doi: 10.1016/0003-9861(59)90090-6.
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Chemical coupling of proteins to agarose.蛋白质与琼脂糖的化学偶联。
Nature. 1967 Sep 30;215(5109):1491-2. doi: 10.1038/2151491a0.
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Purification and properties of bovine milk glyco-alpha-lactalbumin.牛乳糖基-α-乳白蛋白的纯化及性质
Biochim Biophys Acta. 1970 Jul 27;214(1):242-4. doi: 10.1016/0005-2795(70)90094-2.
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The role of alpha-lactalbumin in lactose synthetase.
Biochem Biophys Res Commun. 1970 Jun 5;39(5):833-41. doi: 10.1016/0006-291x(70)90398-0.

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