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Expression of tissue factor procoagulant activity: regulation by cytosolic calcium.

机译:组织因子促凝活性的表达:由胞质钙调节。

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摘要

Intact bovine fibroblasts, pericytes, and kidney cells manifested significantly less tissue factor procoagulant activity than their disrupted counterparts. Addition of calcium ionophore A23187 rapidly and reversibly enhanced the cell-surface expression of tissue factor in intact cells up to the level achieved by disruption. Inhibitors of calmodulin blocked the ionophore-dependent enhancement of procoagulant activity. Similar kinetic parameters were obtained for factor X hydrolysis by tissue factor-factor VIIa on unperturbed pericytes and phosphatidylcholine vesicles. Increase in Vmax and decrease in apparent Km for this reaction were seen after either disruption or ionophore stimulation of the pericytes. Addition of phosphatidylserine to the reconstituted phospholipid vesicles also increased the Vmax and decreased the apparent Km for factor X hydrolysis. These data agree with the hypothesis that the expression of tissue factor procoagulant activity on cell surfaces is modulated by calcium-mediated changes in the asymmetric distribution of phosphatidylserine in plasma membrane.
机译:完整的牛成纤维细胞,周细胞和肾细胞表现出的组织因子促凝活性明显低于其破坏的对应因子。钙离子载体A23187的添加快速可逆地增强了完整细胞中组织因子在细胞表面的表达,直至达到破坏水平。钙调蛋白的抑制剂阻断了离子载体对促凝活性的增强。对于组织X因子VIIa在不受干扰的周细胞和磷脂酰胆碱囊泡上水解X因子获得了相似的动力学参数。在破坏或离子载体刺激周细胞后,可见该反应的Vmax增加和表观Km降低。向重构的磷脂囊泡中添加磷脂酰丝氨酸也增加了Vmax并降低了X因子水解的表观Km。这些数据符合这样的假设,即细胞表面组织因子促凝活性的表达受到钙介导的磷脂酰丝氨酸在质膜中不对称分布的改变的调节。

著录项

  • 作者

    Bach, R; Rifkin, D B;

  • 作者单位
  • 年度 1990
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  • 原文格式 PDF
  • 正文语种 en
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