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大鼠肝脏中嘌呤补救途径的调节

Regulation of the purine salvage pathway in rat liver.

作者信息

Kim Y A, King M T, Teague W E, Rufo G A, Veech R L, Passonneau J V

机构信息

Laboratory of Metabolism and Molecular Biology, National Institute of Alcohol Abuse and Alcoholism, Rockville, Maryland 20852.

出版信息

Am J Physiol. 1992 Mar;262(3 Pt 1):E344-52. doi: 10.1152/ajpendo.1992.262.3.E344.

DOI:10.1152/ajpendo.1992.262.3.E344
PMID:1372483
Abstract

The regulation of purine metabolism in rat liver has been examined under conditions that alter the flux through the pathway. Rats were given intraperitoneal injections of ethanol, sodium acetate, or sodium phosphate to attain body water concentrations of approximately 70, 20, and 10 mM, respectively. The livers were freeze-clamped after 30 min, and extracts were made for the analysis of metabolites, cofactors, purine bases, and nucleosides; homogenates were made for the measurement of the activities and kinetic parameters of seven enzymes that participate in purine salvage. The values of the equilibrium constants of nine reactions were determined in vitro and compared with the ratios of the reactants measured in liver. The changes in phosphoribosylpyrophosphate (PRPP), a key intermediate in both the de novo and salvage pathways of purine metabolism, were directly correlated with the changes in ribose 5-phosphate (ribose-5-P); ([PRPP] = 1.7[ribose-5-P] - 7.4 mumol/kg). Ribose-5-P concentrations in turn could be predicted from the liver content of fructose 6-phosphate and glyceraldehyde 3-phosphate by calculation from the known equilibria. The maximum velocities in the tissue of the seven enzymes measured were calculated from the measured substrate values in the liver and with consideration of other effectors of enzyme activity. PRPP synthetase was the least active of the enzymes measured, indicating a possible rate-limiting step. The delta G of the enzyme steps differed from equilibrium values by factors ranging from 4 (nucleoside phosphorylase) to 10(5) (PRPP synthetase and purine transferase reactions). The regulation of purine salvage appeared to depend on the levels of PRPP and ribose-5-P.

摘要

在改变嘌呤代谢途径通量的条件下,对大鼠肝脏中嘌呤代谢的调节进行了研究。分别给大鼠腹腔注射乙醇、醋酸钠或磷酸钠,使体内水浓度分别达到约70、20和10 mM。30分钟后将肝脏速冻夹闭,制备提取物用于分析代谢物、辅因子、嘌呤碱和核苷;制备匀浆用于测定参与嘌呤补救途径的七种酶的活性和动力学参数。在体外测定了九个反应的平衡常数,并与肝脏中测得的反应物比率进行比较。嘌呤代谢从头合成途径和补救途径的关键中间产物磷酸核糖焦磷酸(PRPP)的变化与5-磷酸核糖(核糖-5-P)的变化直接相关;([PRPP]=1.7[核糖-5-P]-7.4 μmol/kg)。根据已知平衡计算,核糖-5-P浓度又可由6-磷酸果糖和3-磷酸甘油醛的肝脏含量预测。根据肝脏中测得的底物值并考虑酶活性的其他效应物,计算出所测七种酶在组织中的最大反应速度。PRPP合成酶在所测酶中活性最低,表明可能是限速步骤。酶促反应的ΔG与平衡值的差异系数范围为4(核苷磷酸化酶)至10⁵(PRPP合成酶和嘌呤转移酶反应)。嘌呤补救途径的调节似乎取决于PRPP和核糖-5-P的水平。

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