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神经节苷脂生物合成。大鼠肝脏高尔基体中尿苷二磷酸半乳糖:GM2 半乳糖基转移酶的特性

Ganglioside biosynthesis. Characterization of uridine diphosphate galactose: GM2 galactosyltransferase in golgi apparatus from rat liver.

作者信息

Wilkinson F E, Morré D J, Keenan T W

出版信息

J Lipid Res. 1976 Mar;17(2):146-53.

PMID:5567
Abstract

An enzyme that transfers galactose from UDP-Gal to ganglioside GM2 (Tay-Sachs ganglioside) was concentrated 50 times in Golgi apparatus from rat liver relative to total homogenates. This enzyme required detergents or phospholipids as dispersing agents. Of the numerous detergents tested, sodium taurocholate and Triton CF-54 were most effective in stimulating the reaction. Cardiolipin alone was more effective than any of the detergents tested in stimulating enzyme activity. The pH optimum for the reaction varied with the nature of the dispersing agent. With sodium taurocholate, Triton CF-54 and cardiolipin, the pH optima were 6.2, 5.9, and 5.6, respectively. The enzyme had a nearly absolute requirement for Mn2+, with maximum activity being attained at a concentration of 15 mM Mn2+. Other divalent or trivalent cations were either less effective than Mn2+ or inhibited the transferase reaction. The Km values calculated for UDP-Gal and GM2 were 1.1 X 10(-4) M and 9.9 X 10(-5) M, respectively. The enzyme could not be dissociated from Golgi apparatus fractions by treatment with ultrasound, indicating that it is tightly associated with the membrane and not part of the luminal contents. The newly synthesized GM2, the product of the reaction, was incorporated into or became tightly associated with the membranes of the Golgi apparatus.

摘要

一种将半乳糖从尿苷二磷酸半乳糖(UDP - Gal)转移至神经节苷脂GM2(泰 - 萨克斯神经节苷脂)的酶,在大鼠肝脏的高尔基体中相对于总匀浆被浓缩了50倍。这种酶需要去污剂或磷脂作为分散剂。在测试的众多去污剂中,牛磺胆酸钠和Triton CF - 54在刺激该反应方面最有效。单独的心磷脂在刺激酶活性方面比所测试的任何去污剂都更有效。反应的最适pH值随分散剂的性质而变化。对于牛磺胆酸钠、Triton CF - 54和心磷脂,最适pH值分别为6.2、5.9和5.6。该酶对Mn2 +几乎有绝对需求,在15 mM Mn2 +浓度时达到最大活性。其他二价或三价阳离子要么比Mn2 +效果差,要么抑制转移酶反应。计算得出的UDP - Gal和GM2的Km值分别为1.1×10(-4) M和9.9×10(-5) M。用超声处理不能使该酶从高尔基体组分中解离,这表明它与膜紧密结合,而不是腔内容物的一部分。反应产物新合成的GM2被整合到高尔基体膜中或与高尔基体膜紧密结合。

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