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Design Synthesis and Use of Novel Photoaffinity Probes in Measuring the Serum Concentration of Glycogen Phosphorylase

机译:新型光亲和探针的设计合成及其在测量糖原磷酸化酶血清浓度中的用途

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摘要

A procedure to measure the serum concentration of glycogen phosphorylase during acute myocardial infarction is presented. This method was based on the synthesis of photoaffinity probes, and used the semiquantitative protein electrophoretic mobility shift technique. Three novel photoaffinity probes bearing different secondary tags were synthesized. Their potency was evaluated in an enzyme inhibition assay against rabbit muscle glycogen phosphorylase a (RMGPa). The inhibitory activity of probe >1 was only 100-fold less potent than the mother compound CP-320626. The photoaffinity labeling experiments were also performed, and a protein with molecular weight (MW) of about 90–100 kDa, which was consistent with the MW of GP, was clearly labeled by probe >1. A semiquantitative evaluation of the GP level in serum with probe >1 was also performed. The results showed that the protein band with a MW of about 90–100 kDa was tagged, and the concentration of the protein in serum was found to be between 25 and 50 ng/mL. Mass spectrometric analysis revealed that alpha-1,4 glucan phosphorylase (GPMM) was well-preserved in the bands.
机译:提出了一种在急性心肌梗塞期间测量糖原磷酸化酶血清浓度的方法。该方法基于光亲和探针的合成,并使用了半定量蛋白质电泳迁移率迁移技术。合成了三种带有不同二级标签的新型光亲和探针。在针对兔肌肉糖原磷酸化酶a(RMGPa)的酶抑制试验中评估了它们的效力。探针> 1 的抑制活性仅比母体化合物CP-320626低100倍。还进行了光亲和标记实验,并用探针> 1 清楚地标记了分子量(MW)约为90–100 kDa的蛋白质,该蛋白质与GP的MW一致。还用探针> 1 对血清中的GP水平进行了半定量评估。结果表明,分子量约为90–100 kDa的蛋白带被标记,血清中的蛋白浓度在25至50 ng / mL之间。质谱分析表明α-1,4葡聚糖磷酸化酶(GPMM)在条带中保存完好。

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