酿酒酵母中己糖激酶2的体内磷酸化位点。
In vivo phosphorylation site of hexokinase 2 in Saccharomyces cerevisiae.
作者信息
Kriegel T M, Rush J, Vojtek A B, Clifton D, Fraenkel D G
机构信息
Department of Microbiology and Molecular Genetics, Harvard Medical School, Boston, Massachusetts 02115.
出版信息
Biochemistry. 1994 Jan 11;33(1):148-52. doi: 10.1021/bi00167a019.
Yeast hexokinase 2 is known to be a phosphoprotein in vivo, prominently labeled from 32P-inorganic phosphate after a shift of cells to medium with low glucose concentration [Vojtek, A. B., & Fraenkel D. G. (1990) Eur. J. Biochem, 190, 371-375]. The principal and perhaps sole site of phosphorylation is now identified as residue serine-15, by observation of a single tryptic peptide difference, its sequencing and size determination by mass spectrometry, and by mutation to alanine, which prevents phosphorylation in vivo. Although protein kinase A was unlikely to accomplish the phosphorylation in vivo, serine-15 does belong to a protein kinase A consensus phosphorylation sequence, and in vitro phosphorylation by protein kinase A at serine-15 could be shown by labeling and by peptide determination. The alanine-15 mutant enzyme was not phosphorylated in vitro.
已知酵母己糖激酶2在体内是一种磷蛋白,当细胞转移到低葡萄糖浓度的培养基中后,它会被无机磷酸显著标记[沃伊捷克,A. B.,& 弗伦克尔,D. G.(1990年)《欧洲生物化学杂志》,190,371 - 375]。现在,通过观察单个胰蛋白酶肽段差异、其测序以及通过质谱法测定大小,并通过突变为丙氨酸(这可防止体内磷酸化),确定了磷酸化的主要位点,可能也是唯一位点为丝氨酸 - 15。尽管蛋白激酶A不太可能在体内完成磷酸化,但丝氨酸 - 15确实属于蛋白激酶A的共有磷酸化序列,并且通过标记和肽段测定可以证明蛋白激酶A在体外可使丝氨酸 - 15磷酸化。丙氨酸 - 15突变酶在体外未被磷酸化。
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