脑微粒体的磷酸盐结合与三磷酸腺苷酶活性的关系。

Phosphate binding by cerebral microsomes in relation to adenosine-triphosphatase activity.

作者信息

Rodnight R, Hems D A, Lavin B E

出版信息

Biochem J. 1966 Nov;101(2):502-15. doi: 10.1042/bj1010502.

DOI:10.1042/bj1010502

PMID:4226016

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1270134/

Abstract

Microsomes prepared from guinea-pig and ox brain were incubated for periods of a few seconds with low concentrations of Mg-[(32)P]ATP, the reaction was stopped with trichloroacetic acid and determinations were made of the phosphate bound to the acid-washed, and in some cases solvent-extracted, residue. 2. At 20 mum-ATP, at 37 degrees and in the presence of Na(+) ions, 30-50 mumumoles of phosphate/mg. of microsomal protein were bound by the preparation within 1 sec. of starting the reaction; little further change in level occurred until hydrolysis of ATP exceeded 50%, when the bound phosphate began to decline fairly rapidly to the zero-time value. 3. At 20mum-ATP without Na(+) ions present or in the presence of K(+) ions, the level of bound phosphate increased gradually and did not decline as ATP hydrolysis approached completion. 4. Potassium ions either inhibited the formation of Na(+)-dependent bound phosphate or, when added during the course of the reaction, rapidly reduced its level. 5. At 200 mum-ATP the bound phosphate formed in the presence of Na(+) ions appeared to consist of a mixture of the unstable Na(+)-dependent type and the stable type requiring only Mg(2+) ions for its formation. 6. Non-radioactive ATP added during the course of the reaction at 20 mum-ATP with Na(+)ions present rapidly discharged virtually all the bound (32)P counts; at 200 mum-ATP only a proportion of the label was similarly discharged. The Na(+)-dependent bound phosphate is therefore turning over, in contrast with that formed in the absence of Na(+)ions, which proved more stable. 7. The Na(+)-dependent bound phosphate was not in the form of ATP; experiments with [(14)C]ATP instead of [(32)P]ATP showed a small and invariable binding of ATP by the preparation unaffected by Na(+) ions or time of incubation. 8. Under the usual conditions employed in this work ouabain stimulated formation of Na(+)-dependent bound phosphate when Na(+) ions were suboptimum and inhibited it when optimum Na(+) ions were present. 9. The Na(+)-dependent binding reaction under present conditions did not involve incorporation into phosphorylserine groups. 10. The relation of the findings to the (Na(+),K(+))-ATPase of the preparation, and to observations in brain slices appearing to implicate phosphorylserine groups in cation transport, is discussed.

摘要

用豚鼠和牛脑制备的微粒体与低浓度的Mg - [(32)P]ATP孵育数秒，反应用三氯乙酸终止，然后测定与酸洗后的残渣（在某些情况下为溶剂萃取后的残渣）结合的磷酸盐。2. 在20 μmol - ATP、37℃且存在Na⁺离子的条件下，反应开始后1秒内，制剂每毫克微粒体蛋白结合30 - 50纳摩尔的磷酸盐；在ATP水解超过50%之前，结合水平几乎没有进一步变化，当ATP水解超过50%时，结合的磷酸盐开始迅速下降至零时刻值。3. 在不存在Na⁺离子或存在K⁺离子的情况下，20 μmol - ATP时，结合磷酸盐的水平逐渐升高，并且在ATP水解接近完成时不会下降。4. 钾离子要么抑制Na⁺依赖性结合磷酸盐的形成，要么在反应过程中加入时迅速降低其水平。5. 在200 μmol - ATP时，在Na⁺离子存在下形成的结合磷酸盐似乎由不稳定的Na⁺依赖性类型和仅需Mg²⁺离子形成的稳定类型的混合物组成。6. 在20 μmol - ATP且存在Na⁺离子的反应过程中加入非放射性ATP，几乎能迅速释放所有结合的(32)P计数；在200 μmol - ATP时，只有一部分标记物以类似方式被释放。因此，与在不存在Na⁺离子时形成的更稳定的结合磷酸盐相比，Na⁺依赖性结合磷酸盐在周转。7. Na⁺依赖性结合磷酸盐不是ATP的形式；用[(14)C]ATP代替[(32)P]ATP进行的实验表明，制剂对ATP的结合量小且恒定，不受Na⁺离子或孵育时间的影响。8. 在本研究通常采用的条件下，当Na⁺离子浓度不足时，哇巴因刺激Na⁺依赖性结合磷酸盐的形成，而当存在最佳Na⁺离子浓度时则抑制其形成。9. 在当前条件下，Na⁺依赖性结合反应不涉及掺入磷酸丝氨酸基团。10. 讨论了这些发现与制剂的(Na⁺,K⁺)-ATP酶的关系，以及与脑切片中似乎表明磷酸丝氨酸基团参与阳离子转运的观察结果的关系。