首页> 美国卫生研究院文献>Biochemical Journal >5-Nucleotidase activities in human erythrocytes. Identification of a purine 5-nucleotidase stimulated by ATP and glycerate 23-bisphosphate.
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5-Nucleotidase activities in human erythrocytes. Identification of a purine 5-nucleotidase stimulated by ATP and glycerate 23-bisphosphate.

机译:人红细胞中的5-核苷酸酶活性。鉴定由ATP和23-双磷酸甘油酯刺激的嘌呤5-核苷酸酶。

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摘要

A purine 5'-nucleotidase has been separated by DEAE-Trisacryl chromatography from other 5'-nucleotidase activities present in human haemolysates and purified approx. 30,000-fold by subsequent chromatography on Blue Sepharose. The enzyme has an Mr of around 250,000, displays hyperbolic substrate-saturation kinetics and hydrolyses preferentially IMP, GMP and their deoxy counterparts. It is much less active with AMP and dAMP. The purine 5'-nucleotidase is inhibited by Pi, and is strongly stimulated by ATP, dATP and GTP, and by glycerate 2,3-bisphosphate. Stimulators decrease Km and increase Vmax. Glycerate 2,3-bisphosphate is the most potent stimulator of the enzyme and, under physiological conditions, over-rides the influence of the other effectors. Glycerate 2,3-bisphosphate also influences the binding of the enzyme to DEAE-Trisacryl, as evidenced by the different elution profile obtained with fresh as compared with outdated blood. It is concluded that the glycerate 2,3-bisphosphate-stimulated purine 5'-nucleotidase is responsible for the dephosphorylation of IMP and GMP, but not of AMP, in human erythrocytes.
机译:嘌呤5'-核苷酸酶已通过DEAE-Trisacryl色谱法与人溶血产物中存在的其他5'-核苷酸酶活性分离,并进行了纯化。通过随后在蓝色琼脂糖凝胶上的色谱法纯化30,000倍。该酶的Mr约为250,000,显示双曲线底物饱和动力学,并优先水解IMP,GMP及其脱氧对应物。对于AMP和dAMP,它的活性要弱得多。嘌呤5'-核苷酸酶被Pi抑制,并被ATP,dATP和GTP和2,3-双磷酸甘油酯强烈刺激。刺激器降低Km并增加Vmax。甘油2,3-二磷酸甘油酯是该酶最有效的刺激剂,在生理条件下,其作用超过了其他效应物。 2,3-二磷酸甘油酯也影响酶与DEAE-Trisacryl的结合,这与新鲜血液与过时血液相比具有不同的洗脱特性所证明。结论是,甘油2,3-二磷酸刺激的嘌呤5'-核苷酸酶负责人红细胞中IMP和GMP而不是AMP的去磷酸化。

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