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A phosphorylation assay using (y- P)ATP: A highly sensitive detection of protein kinase C

机译:使用(Y-P)ATP的磷酸化测定:蛋白激酶C的高敏感性检测

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摘要

The involvement of protein kinase C (PKC) in many biological processes such as development, memory, cell differentiation and proliferation, and carcinogenesis has been demonstrated. Using the mep45 gene encoding the 45-kDa major envelope protein (Mep45) of Selenomonas ruminantium, a protein-fused substrate (neurogranin-Mep45, MFS-PKC) was cloned, which is a highly selective substrate for PKC. The recombinant protein-fused substrate can be constantly produced in reasonable quantities with a small outlay. In this study, a suitable strategy for the detection of the phosphorylation of a peptide-type substrate and a Mep45-fused substrate catalyzed by PKC by using a sensitive radiodetection is described. This strategy can be applicable to the development of protein microarray, which can be a useful tool for high-throughput screening in biological and medical research.
机译:蛋白激酶C(PKC)在许多生物学过程中参与诸如显影,记忆,细胞分化和增殖和致癌作用。 使用编码Selenomonas硒的45-KDA主要包络蛋白(MEP45)的MEP45基因,克隆蛋白质稠合的基质(神经蛋白-MEP45,MFS-PKC),这是PKC的高度选择性底物。 重组蛋白稠合的基材可以以合理的数量不断地生产,具有小的支出。 在该研究中,描述了通过使用使用敏感的无线电通过PKC催化的肽型衬底的磷酸化和MEP45稠合基材的磷酸化的合适策略。 该策略可以适用于蛋白质微阵列的开发,这可以是生物学和医学研究中的高通量筛选的有用工具。

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