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A novel technique for rapid determination of energy consumption in platelets. Demonstration of different energy consumption associated with three secretory responses

机译:快速测定血小板能量消耗的新技术。展示与三种分泌反应相关的不同能量消耗

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pA novel method has been developed for rapid and quantitative determination of the rate of energy consumption in platelets. In platelets suspended in a cyanide-containing medium. ATP resynthesis is abruptly blocked by addition of 2-deoxyglucose and D-glucono-1,5-lactone. We demonstrate that the subsequent changes in the levels of cytoplasmic ATP and ADP reflect the velocity of energy consumption in the platelets immediately before addition of the inhibitors. Despite the arrest in ATP resynthesis the platelets remain responsive to stimulation by thrombin (5 units x ml-1) which triggers the secretion of the contents of dense, alpha- and acid hydrolase granules. Unstimulated platelets were found to consume about 3.5 and 0.5 mumol of ATP equivalents x min-1 x (10(11) cells)-1 at 37 degrees C and 15 degrees C, respectively; the thrombin-treated platelets consumed respectively 16 and 2 mumol of ATP equivalents x min-1 x (10(11) cells)-1 at these temperatures. When the velocity of energy consumption was varied by (a) changing the temperature and (b) preincubation with glyco(geno)lytic inhibitors, it was found to be linearly related to the initial rate of secretion from the three types of granules. The precise nature of this relationship differed between the three types of secretion responses and indicated an increasing requirement for metabolic energy for secretion from the three types of granules in the order: dense granule less than alpha-granule less than acid hydrolase granule. The results obtained with changes in temperature were superimposable on those obtained with the glyco(geno)lytic inhibitors for dense granule secretion and alpha-granule secretion, suggesting an apparent coupling between energy consumption and the rate of these secretion responses. The rate of secretion of acid hydrolase was always higher when energy consumption was varied by temperature changes than when glyco(geno)lytic inhibitors were used, probably as a result of metabolic changes prior to induction of secretion. On the basis of these experiments, we calculated an incremental energy consumption during complete secretion of dense, alpha- and acid hydrolase granule contents of 2.5, 4.2 and 6.7 mumol of ATP equivalents x (10(11) platelets)-1, respectively./p
机译:已开发出一种新颖的方法,用于快速定量测定血小板中的能量消耗速率。在血小板中悬浮于含氰化物的介质中。加入2-脱氧葡萄糖和D-葡萄糖基1,5-内酯会突然阻止ATP的再合成。我们证明,随后添加抑制剂之前,细胞质ATP和ADP水平的后续变化反映了血小板中能量消耗的速度。尽管ATP重新合成被阻止,血小板仍然对凝血酶(5单位x ml-1)的刺激反应,这触发了致密,α-和酸性水解酶颗粒内容物的分泌。发现未刺激的血小板在37摄氏度和15摄氏度分别消耗约3.5和0.5摩尔摩尔的ATP当量x min-1 x(10(11)细胞)-1。在这些温度下,凝血酶处理的血小板分别消耗了16和2摩尔摩尔的ATP当量x min-1 x(10(11)细胞)-1。当通过(a)改变温度和(b)用糖(基因)分解抑制剂预温育改变能量消耗的速度时,发现这与三种类型颗粒的初始分泌速率呈线性关系。在三种类型的分泌反应之间,这种关系的精确性质有所不同,并且表明从以下三种类型的颗粒中分泌所需的代谢能量的增加顺序为:致密颗粒小于α-颗粒小于酸性水解酶颗粒。随着温度变化而获得的结果可与用糖(遗传)分解抑制剂获得的结果相叠加,从而获得密集的颗粒分泌和α-颗粒分泌,表明能量消耗与这些分泌反应的速率之间存在明显的耦合。当能量消耗随温度变化而变化时,酸水解酶的分泌率始终高于使用糖(基因)分解抑制剂时,这可能是诱导分泌之前代谢变化的结果。在这些实验的基础上,我们计算出完全分泌2.5、4.2和6.7摩尔摩尔ATP当量x(10(11)血小板)-1的致密,α-和酸性水解酶颗粒含量时的增量能耗。 / p>

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