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Simultaneous synthesis and degradation of rat liver glycogen. An in vivo nuclear magnetic resonance spectroscopic study.

机译:大鼠肝糖原的同时合成和降解。体内核磁共振波谱研究。

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摘要

Using 13C nuclear magnetic resonance spectroscopic methods we examined in vivo the synthesis of liver glycogen during the infusion of D-[1-13C]glucose and the turnover of labeled glycogen during subsequent infusion of D-[1-13C]glucose. In fasted rats the processes of glycogen synthesis and degradation were observed to occur simultaneously with the rate of synthesis much greater than degradation leading to net glycogen synthesis. In fed rats, incorporation of infused D-[1-13C]glucose occurred briskly; however, over 2 h there was no net glycogen accumulated. Degradation of labeled glycogen was greater in the fed versus the fasted rats (P less than 0.001), and the lack of net glycogen synthesis in fed rats was due to degradation and synthesis occurring at similar rates throughout the infusion period. There was no indication that suppression of phosphorylase a or subsequent activation of glycogen synthase was involved in modulation of the flux of tracer into liver glycogen. We conclude that in both fed and fasted rats, glycogen synthase and phosphorylase are active simultaneously and the levels of liver glycogen reached during refeeding are determined by the balance between ongoing synthetic and degradative processes.
机译:使用13 C核磁共振波谱方法,我们在体内检查了D- [1-13C]葡萄糖输注过程中肝糖原的合成以及在随后的D- [1-13C]葡萄糖输注过程中标记糖原的周转率。在禁食的大鼠中,观察到糖原合成和降解的过程同时发生,其合成速率远大于导致净糖原合成的降解。在进食的大鼠中,注入的D- [1-13C]葡萄糖反应迅速。但是,超过2小时没有累积糖原。与禁食的大鼠相比,进食的大鼠中标记糖原的降解更大(P小于0.001),并且由于在整个输液期间降解和合成的发生速率相似,因此进食的大鼠中缺乏净糖原合成。没有迹象表明磷酸化酶α的抑制或随后糖原合酶的激活与示踪剂通入肝糖原的通量的调节有关。我们得出的结论是,在进食和禁食的大鼠中,糖原合酶和磷酸化酶同时具有活性,并且在进食期间肝糖原的水平取决于正在进行的合成和降解过程之间的平衡。

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