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AMP激活的蛋白激酶使谷氨酰胺:果糖-6-磷酸酰胺转移酶1的丝氨酸243位点磷酸化,以调节其酶活性。

AMP-activated protein kinase phosphorylates glutamine : fructose-6-phosphate amidotransferase 1 at Ser243 to modulate its enzymatic activity.

作者信息

Eguchi Satoshi, Oshiro Noriko, Miyamoto Takafumi, Yoshino Ken-Ichi, Okamoto Sumiko, Ono Takamasa, Kikkawa Ushio, Yonezawa Kazuyoshi

机构信息

Biosignal Research Center, Kobe University, Japan.

出版信息

Genes Cells. 2009 Feb;14(2):179-89. doi: 10.1111/j.1365-2443.2008.01260.x. Epub 2008 Jan 6.

DOI:10.1111/j.1365-2443.2008.01260.x
PMID:19170765
Abstract

Glutamine : fructose-6-phosphate amidotransferase 1 (GFAT1) was identified as a protein phosphorylated in glucose-deprived cells by immunoprecipitation using the anti-phospho Akt substrates (PAS) antibody, which recognizes the phosphorylation motif site by AMP-activated protein kinase (AMPK), followed by mass fingerprinting analysis. Glucose depletion-induced phosphorylation of endogenous GFAT was potentiated by 2-deoxyglucose (2-DG), an AMPK activator, and the 2-DG-stimulated phosphorylation of FLAG-tagged GFAT1 in transfected cells was suppressed by Compound C, an AMPK inhibitor. The 2-DG induced phosphorylation of GFAT1 was attenuated by the introduction of the kinase-negative mutant of AMPK, and the phosphorylation was observed in the cells expressing the constitutively active mutant of AMPK even in the absence of 2-DG. Subsequent analysis revealed that the PAS antibody recognized GFAT1 phosphorylated at Ser243, which is conserved among different species. The assay of the GFAT enzymatic activity in the cell lysates indicated that the 2-DG-treatment inhibited the enzymatic activity, and Compound C-preincubation partially prevented the 2-DG-induced decrease of the activity. Furthermore, the mutant replacing Ser243 by alanine partially prevented the decrease of GFAT activity by 2-DG treatment. These results indicate that the phosphorylation of GFAT1 at Ser243 by AMPK has an important role in the regulation of the GFAT1 enzymatic activity.

摘要

谷氨酰胺

果糖-6-磷酸酰胺转移酶1(GFAT1)被鉴定为在葡萄糖缺乏的细胞中通过使用抗磷酸化Akt底物(PAS)抗体进行免疫沉淀而被磷酸化的一种蛋白质,该抗体识别由AMP激活的蛋白激酶(AMPK)的磷酸化基序位点,随后进行质谱指纹分析。AMPK激活剂2-脱氧葡萄糖(2-DG)增强了葡萄糖耗竭诱导的内源性GFAT磷酸化,而AMPK抑制剂Compound C抑制了转染细胞中2-DG刺激的FLAG标记的GFAT1磷酸化。引入AMPK的激酶阴性突变体减弱了2-DG诱导的GFAT1磷酸化,并且即使在没有2-DG的情况下,在表达AMPK组成型活性突变体的细胞中也观察到了磷酸化。随后的分析表明,PAS抗体识别在Ser243处磷酸化的GFAT1,该位点在不同物种中保守。细胞裂解物中GFAT酶活性的测定表明,2-DG处理抑制了酶活性,而Compound C预孵育部分阻止了2-DG诱导的活性降低。此外,用丙氨酸替代Ser243的突变体部分阻止了2-DG处理导致的GFAT活性降低。这些结果表明,AMPK使GFAT1在Ser243处磷酸化在调节GFAT1酶活性中起重要作用。

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