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Protein kinase activity in Cucumis sativus cotyledons: Effect of calcium and light

机译:黄瓜子叶中的蛋白激酶活性:钙和光的影响

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Light signals received by phytochromes in plants may be transduced through protein phosphorylation. Ca(2+) as second messenger was involved in phytochrome-mediated cellular events. Our experiments with Cucumis sativus cotyledons, treated with red (R) and far-red (FR) light, showed a stimulatory effect on in vitro protein phosphorylation of histone, added as exogenous substrate to the cotyledon extracts, and also modified the phosphorylation of endogenous polypeptides. The effect of light treatments was mimicked by the addition of Ca(2+) to the phosphorylation buffer, indicating phytochrome- and Ca(2+)-dependence on activity of some protein kinases (PKs). In-gel kinase assays were performed to characterize the PKs involved at the cotyledon stage of cucumber plants. Three proteins of about 75, 57 and 47kDa with PK activity were detected between M(r) markers of 94 and 45kDa. All three were able to phosphorylate histone and undergo autophosphorylation. However, only the 75 and 57kDa proteins autophosphorylated and phosphorylated the substrate in a Ca(2+)-dependent manner, and were inhibited when calmodulin (CaM) antagonists were added to the incubation buffer. Western-blot analysis with polyclonal antibodies directed against calcium-dependent protein kinase of rice (OsCDPK11) or Arabidopsis (AtCPK2) recognised 57 and 75kDa polypeptides, respectively. These results indicate the presence in cucumber cotyledons of at least two proteins (ca. 75 and 57kDa) with activity of PKs that could be calcium-dependent protein kinases (CDPKs). Both CDPKs could be modulated by phytochromes throughout FR-HIR and VLFR responses.
机译:植物中植物色素所接收的光信号可通过蛋白质磷酸化进行转导。 Ca(2+)作为第二信使参与植物色素介导的细胞事件。我们用红色(R)和远红色(FR)光处理的黄瓜黄瓜子叶的实验显示出对组蛋白的体外蛋白质磷酸化的刺激作用,作为外源底物添加到子叶提取物中,并且还修饰了内源性磷酸化。多肽。通过将Ca(2+)添加到磷酸化缓冲液中来模拟光处理的效果,表明植物色素和Ca(2+)对某些蛋白激酶(PKs)活性的依赖性。进行凝胶内激酶测定以表征黄瓜植株子叶期所涉及的PK。在94和45kDa的M(r)标记之间检测到具有PK活性的约75、57和47kDa的三种蛋白质。这三个都能够磷酸化组蛋白并进行自磷酸化。但是,只有75和57kDa的蛋白质以Ca(2+)依赖性方式自磷酸化和磷酸化底物,并且在将钙调蛋白(CaM)拮抗剂添加到孵育缓冲液中时被抑制。用针对水稻(OsCDPK11)或拟南芥(AtCPK2)的钙依赖性蛋白激酶的多克隆抗体进行的蛋白质印迹分析分别识别了57和75kDa多肽。这些结果表明在黄瓜子叶中存在至少两种具有PK活性的蛋白(约75kDa和57kDa),其可能是钙依赖性蛋白激酶(CDPK)。在整个FR-HIR和VLFR反应中,两种CDPK均可被植物色素调节。

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