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PKA 催化同工型的激活环在酿酒酵母中被 Pkh 蛋白激酶差异化磷酸化。

The activation loop of PKA catalytic isoforms is differentially phosphorylated by Pkh protein kinases in Saccharomyces cerevisiae.

机构信息

Department of Molecular Biology, University of Geneva CH-1211, Switzerland.

出版信息

Biochem J. 2012 Dec 15;448(3):307-20. doi: 10.1042/BJ20121061.

DOI:10.1042/BJ20121061
PMID:22957732
Abstract

PDK1 (phosphoinositide-dependent protein kinase 1) phosphorylates and activates PKA (cAMP-dependent protein kinase) in vitro. Docking of the HM (hydrophobic motif) in the C-terminal tail of the PKA catalytic subunits on to the PIF (PDK1-interacting fragment) pocket of PDK1 is a critical step in this activation process. However, PDK1 regulation of PKA in vivo remains controversial. Saccharomyces cerevisiae contains three PKA catalytic subunits, TPK1, TPK2 and TPK3. We demonstrate that Pkh [PKB (protein kinase B)-activating kinase homologue] protein kinases phosphorylate the activation loop of each Tpk in vivo with various efficiencies. Pkh inactivation reduces the interaction of each catalytic subunit with the regulatory subunit Bcy1 without affecting the specific kinase activity of PKA. Comparative analysis of the in vitro interaction and phosphorylation of Tpks by Pkh1 shows that Tpk1 and Tpk2 interact with Pkh1 through an HM-PIF pocket interaction. Unlike Tpk1, mutagenesis of the activation loop site in Tpk2 does not abolish in vitro phosphorylation, suggesting that Tpk2 contains other, as yet uncharacterized, Pkh1 target sites. Tpk3 is poorly phosphorylated on its activation loop site, and this is due to the weak interaction of Tpk3 with Pkh1 because of the atypical HM found in Tpk3. In conclusion, the results of the present study show that Pkh protein kinases contribute to the divergent regulation of the Tpk catalytic subunits.

摘要

PDK1(磷酸肌醇依赖性蛋白激酶 1)在体外磷酸化并激活 PKA(cAMP 依赖性蛋白激酶)。PKA 催化亚基 C 末端尾部的 HM(疏水性基序)与 PDK1 的 PIF(PDK1 相互作用片段)口袋对接是这种激活过程中的关键步骤。然而,PDK1 在体内对 PKA 的调节仍然存在争议。酿酒酵母含有三种 PKA 催化亚基,TPK1、TPK2 和 TPK3。我们证明 Pkh[PKB(蛋白激酶 B)激活激酶同源物]蛋白激酶在体内以不同的效率磷酸化每个 Tpk 的激活环。Pkh 失活减少了每个催化亚基与调节亚基 Bcy1 的相互作用,而不影响 PKA 的特异性激酶活性。Pkh1 对 Tpks 的体外相互作用和磷酸化的比较分析表明,Tpk1 和 Tpk2 通过 HM-PIF 口袋相互作用与 Pkh1 相互作用。与 Tpk1 不同,Tpk2 激活环位点的突变并不消除体外磷酸化,这表明 Tpk2 含有其他尚未表征的 Pkh1 靶位。Tpk3 在其激活环位点上的磷酸化程度较差,这是由于 Tpk3 与 Pkh1 的弱相互作用,因为 Tpk3 中存在非典型的 HM。总之,本研究的结果表明,Pkh 蛋白激酶有助于 Tpk 催化亚基的不同调节。

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