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蛋白激酶C使大鼠脑中的MARCKS的丝氨酸152、丝氨酸156和丝氨酸163发生磷酸化,但不使丝氨酸160磷酸化。

Protein kinase C phosphorylates Ser152, Ser156 and Ser163 but not Ser160 of MARCKS in rat brain.

作者信息

Heemskerk F M, Chen H C, Huang F L

机构信息

Endocrinology and Reproduction Research Branch, National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, MD 20892.

出版信息

Biochem Biophys Res Commun. 1993 Jan 15;190(1):236-41. doi: 10.1006/bbrc.1993.1036.

Abstract

MARCKS is one of the major physiological substrates of PKC and was reported to be phosphorylated by PKC at 4 serine residues that are within the CaM-binding region (Graff et al., J. Biol. Chem. 264, 11912, 1989). Using MARCKS from rat brain and a synthetic peptide of 25 amino acids containing all 4 of the serine residues, we investigate the differences in phosphorylation by PKC isozymes I, II and III. Tryptic peptide analysis of PKC phosphorylated MARCKS or peptide, we found 32P was in peptides of (K)S152FK, (R)FS156FK and LS160GFS163FK. Further digestion of LSGFSFK with alpha-chymotrypsin revealed that 32P incorporation occurred only at Ser163 but not at Ser160. The initial rates and stoichiomatry of phosphorylation of Ser152 and Ser156 were twice as those of Ser163 using either one of the three PKC isozymes. These results indicate that in vitro, PKC phosphorylates MARCKS only at three sites, but not at Ser160 as that reported previously, and there was no preferential phosphorylation of MARCKS by either PKC isozyme I, II or III.

摘要

MARCKS是蛋白激酶C(PKC)的主要生理底物之一,据报道它在钙调蛋白结合区域内的4个丝氨酸残基处被PKC磷酸化(Graff等人,《生物化学杂志》264, 11912, 1989)。我们使用大鼠脑来源的MARCKS以及包含所有4个丝氨酸残基的25个氨基酸的合成肽,研究了PKC同工酶I、II和III在磷酸化方面的差异。通过对PKC磷酸化的MARCKS或肽进行胰蛋白酶肽段分析,我们发现32P存在于(K)S152FK、(R)FS156FK和LS160GFS163FK肽段中。用α-胰凝乳蛋白酶对LSGFSFK进一步消化后发现,32P仅掺入Ser163,而未掺入Ser160。使用三种PKC同工酶中的任何一种时,Ser152和Ser156的磷酸化初始速率和化学计量比是Ser163的两倍。这些结果表明,在体外,PKC仅在三个位点磷酸化MARCKS,而不是如先前报道的在Ser160位点,并且PKC同工酶I、II或III对MARCKS没有优先磷酸化作用。

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