The Na+, K+-ATPase activation energy of the embryos of a cold-blooded loach

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Abstract

The Na + , K + -ATPase is an ubiquitously expressed P-type of ATPase. Its main role is to maintain Na + and K + gradients across the plasma membrane by ATP-driven active transport. The Na + , K + -ATPase was one of the first ion pumps studied because of its importance in main-taining osmotic and ionic balances between intracellular and extracellular environments. Ad-ditional extracellular stimuli have been shown to induce internalization of the Na in the incubation medium, including the loss of endogenous phosphorus Pi in the membrane preparation, expressed in μmoles Pi per minutes per milligram of protein. The amount of endogenous phosphorus has been identified by the modified Fiske-Subbarow method, the quanti-tation of protein in the membrane preparation has been determined by Lowry method and the activation energy – in the Arrhenius coordinates. The activity of ouabain-sensitive ATPase under the change in the incubation medium temperature gradually increased at the stages of embryos development by an average of 23.4 ± 1.6% as compared with the control group. The maximum value of the enzymatic activity of Na + , K + pump of the embryos has been defined at the 8-stage of blastomers division (270 min). At the 6th hour of the development, no significant changes in the activity of Na + , K + -ATPase has been observed in comparison with the previous stage of the development. The results have shown that with the temperature change (10 o C) of the incubation medium, the Na + , K + -ATPase activity increased significantly at the investigated stages of the development. For Na + , K + -ATPase, a nonlinear dependence of the enzymatic activity on the temperature in the Arrhenius coordinates was found; the activation energy is 10.6 ÷ 20.8 kJ / mol. The calculated values of the Na + , K + -ATPase activation energy of the loach embryos during embryogenesis are consistent with the existing data and are likely due to the binding strength of the investigated ATP-hydrolase to membrane lipids during the embryonal cell division.
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冷血泥鳅胚胎的Na+, K+- atp酶活化能
Na +, K + - atp酶是一种普遍表达的p型atp酶。其主要作用是通过atp驱动的主动转运维持Na +和K +在质膜上的梯度。Na +, K + - atp酶是最早被研究的离子泵之一,因为它在维持细胞内和细胞外环境之间的渗透和离子平衡方面具有重要意义。额外的细胞外刺激已被证明可以诱导培养液中Na的内化,包括在膜制备中内源性磷Pi的损失,以μ摩尔Pi每分钟每毫克蛋白质表示。用改进的Fiske-Subbarow法测定了内源磷的量,用Lowry法测定了膜制备过程中蛋白质的定量,并在Arrhenius坐标系下测定了活化能。在胚胎发育阶段,随着培养液温度的变化,瓦巴因敏感atp酶的活性逐渐升高,平均较对照组升高23.4±1.6%。胚胎的Na +、K +泵酶活性在囊胚分裂第8期(270 min)达到最大值。在发育第6小时,Na +, K + - atp酶的活性与发育前阶段相比没有明显变化。结果表明,随着培养温度(10℃)的变化,Na +, K + - atp酶活性在发育阶段显著升高。对于Na +, K + - atp酶,在Arrhenius座标下,酶活性与温度呈非线性关系;泥鳅胚胎在胚胎发生过程中Na +、K + - atp酶的活化能计算值与已有数据一致,可能与胚胎细胞分裂过程中所研究的atp水解酶与膜脂的结合强度有关。
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