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半乳糖基转移酶的金属离子激活作用。

Metal ion activation of galactosyltransferase.

作者信息

Powell J T, Brew K

出版信息

J Biol Chem. 1976 Jun 25;251(12):3645-52.

PMID:932001
Abstract

Galactosyltransferase, which functions as the catalytic component of lactose synthase and in the glycosylation of glycoproteins, has been previously reported to have an absolute dependence on Mn2+ for activity, with a Kd for Mn2+ (10(-3) M) 2 to 3 orders of magnitude greater than the physiological range of Mn2+ concentrations (v 10(-6) M). Reinvestigation of the metal ion dependence of this enzyme has shown that Zn2+, Cd2+, Fe2+, Co2+, and Pr3+ also produce activation, although with lower activities at saturation than that attained with Mn2+. Velocity against metal ion concentration curves for all metals, including Mn2+, are sigmoid, suggesting the presence of two or more activating metal binding sites on the enzyme. The presence of two sites is confirmed by studies using both Mn2+ and Ca2+. While galactosyltransferase is inactive in the presence of Ca2+ alone, at low concentrations of Mn2+ (10(-5) M), enzyme activity is stimulated by Ca2+. A more detailed investigation by steady state kinetics has revealed that there is a tight binding site for Mn2+ (site I: Kd of 2 X 10(-6) M) from which Ca2+ is excluded, and a site at which Ca2+ can replace Mn2+ (site II: Kd for Ca2+ of 1.76 X 10(-3) M), to which metal binding has a specific synergistic effect on UDP-galactose binding, possibly as a result of the formation of an enzyme-Ca2+-UDP-galactose bridge complex. The site I Mn2+, site II Ca2+-activated enzyme has a maximum velocity similar to that of the Mn2+-activated enzyme, and is the enzyme form that must act in lactose synthesis in vivo. A trypsin-degraded form of galactose transferase (galactosyltransferase-T) (Powell, J.T., and Brew, K. (1974) Eur. J. Biochem. 48, 217-228) appears to lack site I and is activated by Ca2+ in the absence of Mn2+.

摘要

半乳糖基转移酶作为乳糖合酶的催化成分并参与糖蛋白的糖基化过程,此前有报道称其活性绝对依赖于Mn2+,其对Mn2+的解离常数(Kd为10(-3) M)比Mn2+浓度的生理范围(约10(-6) M)大2至3个数量级。对该酶金属离子依赖性的重新研究表明,Zn2+、Cd2+、Fe2+、Co2+和Pr3+也能产生激活作用,尽管饱和时的活性低于Mn2+所达到的活性。包括Mn2+在内的所有金属的速度-金属离子浓度曲线均为S形,这表明该酶上存在两个或更多个激活金属结合位点。使用Mn2+和Ca2+进行的研究证实了存在两个位点。虽然半乳糖基转移酶在单独存在Ca2+时无活性,但在低浓度Mn2+(10(-5) M)下,Ca2+会刺激酶活性。通过稳态动力学进行的更详细研究表明,存在一个Mn2+的紧密结合位点(位点I:Kd为2×10(-6) M),Ca2+被排除在外,还有一个位点Ca2+可以取代Mn2+(位点II:Ca2+的Kd为1.76×10(-3) M),金属结合对UDP-半乳糖的结合具有特定的协同作用,这可能是由于形成了酶-Ca2+-UDP-半乳糖桥复合物。位点I的Mn2+、位点II的Ca2+激活的酶具有与Mn2+激活的酶相似的最大速度,并且是体内乳糖合成中必须起作用的酶形式。一种经胰蛋白酶降解的半乳糖转移酶形式(半乳糖基转移酶-T)(鲍威尔,J.T.,和布鲁,K.(1974年)《欧洲生物化学杂志》48,217 - 228)似乎缺乏位点I,并且在没有Mn2+的情况下被Ca2+激活。

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