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Regulation of the interaction of purified human erythrocyte AMP deaminase and the human erythrocyte membrane.

机译:纯化的人红细胞AMP脱氨酶与人红细胞膜相互作用的调节。

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摘要

The binding of purified human erythrocyte AMP deaminase to human erythrocyte membranes and the effect of binding on enzyme catalytic activity was investigated. AMP deaminase binds preferentially and specifically to the cytoplasmic surface of the erythrocyte membrane. The binding is saturable, reversible, and responsive to alterations of pH, of ionic strength, and of ATP and AMP concentrations. A limited number (approximately equal to 2.2 X 10(4) per erythrocyte) of apparently homogeneous high affinity (Ka approximately equal to 2.6 X 10(7) M-1) binding sites is present. The stability of purified and endogenously bound AMP deaminase is markedly improved by the interaction with the membrane, whereas the catalytic activity of AMP deaminase is sharply reduced. AMP deaminase displaces membrane bound glyceraldehyde 3-phosphate dehydrogenase in roughly a dose-response manner. No evidence for binding of AMP deaminase to spectrin or band 3 (the G3PD binding protein) was found in sucrose gradients, however. The interaction of AMP deaminase with the erythrocyte membrane may play an important role in the regulation of cellular adenine nucleotide metabolism.
机译:研究了纯化的人红细胞AMP脱氨酶与人红细胞膜的结合以及结合对酶催化活性的影响。 AMP脱氨酶优先且特异性地与红细胞膜的细胞质表面结合。结合是可饱和的,可逆的,并且对pH,离子强度以及ATP和AMP浓度的变化有反应。存在有限数量(大约等于每个红细胞2.2 X 10(4))的表观均一的高亲和力(Ka大约等于2.6 X 10(7)M-1)结合位点。纯化的和内源结合的AMP脱氨酶的稳定性通过与膜的相互作用而显着提高,而AMP脱氨酶的催化活性急剧降低。 AMP脱氨酶以剂量反应的方式取代了膜结合的3-磷酸甘油醛脱氢酶。然而,在蔗糖梯度中没有发现AMP脱氨酶与血影蛋白或条带3(G3PD结合蛋白)结合的证据。 AMP脱氨酶与红细胞膜的相互作用可能在调节细胞腺嘌呤核苷酸代谢中起重要作用。

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