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人阳离子胰蛋白酶原在酪氨酸154处发生硫酸化。

Human cationic trypsinogen is sulfated on Tyr154.

作者信息

Sahin-Tóth Miklós, Kukor Zoltán, Nemoda Zsófia

机构信息

Department of Molecular and Cell Biology, Boston University, Goldman School of Dental Medicine, Boston, MA, USA.

出版信息

FEBS J. 2006 Nov;273(22):5044-50. doi: 10.1111/j.1742-4658.2006.05501.x.

Abstract

The crystal structure of human pancreatic cationic trypsin showed the chemical modification of Tyr154, which was originally described as phosphorylation [Gaboriaud C, Serre L, Guy-Crotte O, Forest E & Fontecilla-Camps JC (1996) J Mol Biol259, 995-1010]. Here we report that Tyr154 is sulfated, not phosphorylated. Cationic and anionic trypsinogens were purified from human pancreatic juice and subjected to alkaline hydrolysis. Modified tyrosine amino acids were separated on a Dowex cation-exchange column and analyzed by thin layer chromatography. Both human cationic and anionic trypsinogens contained tyrosine sulfate, but no tyrosine phosphate, whereas bovine trypsinogen contained neither. Furthermore, incorporation of [(35)S]SO(4) into human cationic trypsinogen transiently expressed by human embryonic kidney 239T cells was demonstrated. Mutation of Tyr154 to Phe abolished radioactive sulfate incorporation, confirming that Tyr154 is the site of sulfation in cationic trypsinogen. Sulfated pancreatic cationic trypsinogen exhibited faster autoactivation than a nonsulfated recombinant form, suggesting that tyrosine sulfation of trypsinogens might enhance intestinal digestive zymogen activation in humans. Finally, sequence alignment revealed that the sulfation motif is only conserved in primate trypsinogens, suggesting that typsinogen sulfation is absent in other vertebrates.

摘要

人胰阳离子胰蛋白酶的晶体结构显示了Tyr154的化学修饰,最初认为该修饰为磷酸化修饰[Gaboriaud C, Serre L, Guy-Crotte O, Forest E & Fontecilla-Camps JC (1996) J Mol Biol259, 995 - 1010]。在此我们报道Tyr154是硫酸化的,而非磷酸化的。从人胰液中纯化出阳离子和阴离子胰蛋白酶原,并进行碱性水解。在Dowex阳离子交换柱上分离修饰的酪氨酸氨基酸,并通过薄层色谱法进行分析。人阳离子和阴离子胰蛋白酶原均含有硫酸酪氨酸,但不含磷酸酪氨酸,而牛胰蛋白酶原两者均不含。此外,还证实了[(35)S]SO(4)掺入到人胚肾239T细胞瞬时表达的人阳离子胰蛋白酶原中。将Tyr154突变为苯丙氨酸消除了放射性硫酸盐的掺入,证实Tyr154是阳离子胰蛋白酶原硫酸化的位点。硫酸化的胰阳离子胰蛋白酶原比未硫酸化的重组形式表现出更快的自身激活,这表明胰蛋白酶原的酪氨酸硫酸化可能增强人类肠道消化酶原的激活。最后,序列比对显示硫酸化基序仅在灵长类胰蛋白酶原中保守,这表明其他脊椎动物中不存在胰蛋白酶原硫酸化。

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