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AS-30D腹水肝癌细胞膜中钙转运与(Ca2+,Mg2+)-ATP酶之间偶联状态的改变

Altered coupling states between calcium transport and (Ca2+, Mg2+)-ATPase in the AS-30D ascites hepatocarcinoma plasma membrane.

作者信息

Mas-Oliva J, Pérez-Montfort R, Cárdenas-García M, Rivas-Duro M

机构信息

Departamento de Bioenergética, Universidad Nacional Autónoma de México.

出版信息

Mol Cell Biochem. 1991 Jan 16;100(1):39-50. doi: 10.1007/BF00230808.

Abstract

Plasma membrane fractions from normal, regenerating liver and the AS-30D ascites hepatocarcinoma exhibited a high degree of enrichment when a set of plasma membrane enzyme markers were studied in comparison to the ones associated to the mitochondrial and cytosolic compartments. While the (Ca2+, Mg2+)-ATPase observed for the plasma membrane fraction isolated from normal liver showed an activity of 1.2 mumoles/mg/min, the regenerating liver and the AS-30D plasma membrane fractions presented a much lower ATPase activity (0.3 and 0.22 mumoles/mg/min respectively). Despite the differences in ATPase activity observed between models, the plasma membrane fraction from the AS-30D hepatocarcinoma presented a calcium transport activity similar to the value observed for the normal system (5.9 and 5.5 nmoles Ca2+/mg/10 min, respectively). Interestingly, the ATP in equilibrium with Pi exchange experiments carried out with the different plasma membrane fractions revealed that the (Ca2+, Mg2+)-ATPase contained in the plasma membrane from the AS-30D cells shows an exchange activity of 26 nmoles ATP in equilibrium with Pi/mg/min, similar to the one observed fo the enzyme from normal liver (30 nmoles ATP in equilibrium with Pi/mg/min). Our results suggest that the plasma membrane from the transformed model presents a more efficient mechanism to regulate the movement of calcium through the calcium pump, with an optimum expenditure of energy.

摘要

当研究一组质膜酶标记物,并与线粒体和胞质区室相关的标记物进行比较时,来自正常肝脏、再生肝脏和AS - 30D腹水肝癌的质膜组分表现出高度富集。从正常肝脏分离的质膜组分中观察到的(Ca2 +,Mg2 +)-ATP酶活性为1.2微摩尔/毫克/分钟,而再生肝脏和AS - 30D质膜组分的ATP酶活性则低得多(分别为0.3和0.22微摩尔/毫克/分钟)。尽管在不同模型中观察到ATP酶活性存在差异,但AS - 30D肝癌的质膜组分呈现出与正常系统相似的钙转运活性(分别为5.9和5.5纳摩尔Ca2 +/毫克/10分钟)。有趣的是,用不同质膜组分进行的ATP与Pi交换平衡实验表明,AS - 30D细胞的质膜中所含的(Ca2 +,Mg2 +)-ATP酶显示出与Pi平衡的ATP交换活性为26纳摩尔ATP/毫克/分钟,与正常肝脏中该酶的观察值相似(与Pi平衡的ATP为30纳摩尔ATP/毫克/分钟)。我们的结果表明,转化模型的质膜呈现出一种更有效的机制,通过钙泵调节钙的移动,且能量消耗最优。

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