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Microvesicle release is associated with extensive protein tyrosine dephosphorylation in platelets stimulated by A23187 or a mixture of thrombin and collagen.

机译：微囊泡释放与A23187或凝血酶和胶原蛋白混合物刺激的血小板中广泛的蛋白酪氨酸脱磷酸作用有关。

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Phosphatidylserine exposure and microvesicle release give rise to procoagulant activity during platelet activation. We have previously shown that whereas the Ca2+ ionophore and 2,5-di-(t-butyl)-1, 4-benzohydroquinone, a Ca2+-ATPase inhibitor, induce phosphatidylserine exposure, only the former triggers microvesicle release. We now report that microvesicle formation with ionophore is specifically associated with mu-calpain activation, increased protein tyrosine phosphatase (PTP) activity and decreased tyrosine phosphorylation. The degree to which calpain and individual PTPs were activated in response to depended on the extent of bivalent cation chelation in the external medium. EGTA (2 mM) blocked or severely retarded their activation, and addition of extracellular Ca2+ in excess (2 mM) resulted in virtually immediate tyrosine dephosphorylation. Dephosphorylation was correlated with an increase in total PTP activity in platelet lysates. In platelets stimulated by a combination of thrombin and collagen, only the subpopulation undergoing microvesicle release and isolated by their binding to annexin-V-coated magnetic beads exhibited protein tyrosine dephosphorylation. Detection of PTP activity in an 'in-gel' assay showed the Ca2+-dependent appearance of active low-molecular-mass bands at 38, 36 and 27 kDa. Individual PTPs varied in their protease sensitivity to changes in intracellular Ca2+ levels. For example, PTP1B was a more sensitive substrate than SH2-domain-containing tyrosine phosphatase-1 for mu-calpain cleavage. Incubation of platelets with the PTP inhibitors, phenylarsine oxide and benzylphosphonic acid acetoxymethyl ester, led to increased tyrosine phosphorylation and the surface expression of aminophospholipids but little microvesicle formation. Furthermore, microvesicle release in response to ionophore was inhibited. We conclude that platelet microvesicle formation is associated with extensive protein tyrosine dephosphorylation.

机译：磷脂酰丝氨酸的暴露和微囊泡的释放在血小板活化过程中引起促凝活性。先前我们已经表明，尽管Ca2 +离子载体和2,5-二-（叔丁基）-1、4-苯并氢醌（一种Ca2 + -ATPase抑制剂）诱导磷脂酰丝氨酸暴露，但只有前者会触发微囊泡释放。我们现在报道，具有离子载体的微泡形成与mu-钙蛋白酶激活，蛋白质酪氨酸磷酸酶（PTP）活性增加和酪氨酸磷酸化降低特别相关。钙蛋白酶和各个PTP响应的激活程度取决于外部介质中二价阳离子螯合的程度。 EGTA（2 mM）阻断或严重阻碍了它们的活化，过量添加细胞外Ca2 +（2 mM）导致酪氨酸立即脱磷酸。去磷酸化与血小板裂解物中总PTP活性的增加有关。在凝血酶和胶原蛋白组合刺激的血小板中，只有经历微泡释放并通过与膜联蛋白-V包被的磁珠结合而分离的亚群才表现出蛋白酪氨酸去磷酸化。在“凝胶中”测定法中检测PTP活性表明，在38、36和27 kDa处，活跃的低分子质谱带呈Ca2 +依赖性出现。各个PTP对细胞内Ca2 +水平变化的蛋白酶敏感性各不相同。例如，对于mu-钙蛋白酶裂解，PTP1B是比含SH2结构域的酪氨酸磷酸酶-1更敏感的底物。将血小板与PTP抑制剂，苯ar氧化物和苄基膦酸乙酰氧基甲基酯一起孵育，会导致酪氨酸磷酸化增加，氨基磷脂的表面表达增加，但微囊泡的形成却很少。此外，微泡释放响应离子载体被抑制。我们得出结论，血小板微囊泡形成与广泛的蛋白质酪氨酸脱磷酸有关。

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期刊名称 Biochemical Journal
作者
J M Pasquet; J Dachary-Prigent; A T Nurden;
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年(卷),期 1998(333),Pt 3
年度 1998
页码 591–599
总页数 9
原文格式 PDF
正文语种
中图分类分子生物学;
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专利

1. Microvesicle release is associated with extensive protein tyrosine dephosphorylation in platelets stimulated by A23187 or a mixture of thrombin and collagen. [J] . Pasquet JM, Dachary-Prigent J, Nurden AT The Biochemical Journal . 1998,第Pta3期

机译：微囊泡释放与A23187或凝血酶和胶原蛋白混合物刺激的血小板中大量蛋白酪氨酸脱磷酸作用有关。
2. Microvesicle release is associated with extensive protein tyrosine dephosphorylation in platelets stimulated by A23187 or a mixture of thrombin and collagen [J] . Pasquet JM., Nurden AT., Dachary-Prigent J. The Biochemical Journal . 1998,第Pta3期

机译：微囊泡释放与A23187或凝血酶和胶原蛋白混合物刺激的血小板中大量蛋白酪氨酸脱磷酸作用有关
3. Sustained stimulation of platelet thrombin receptor is associated with tyrosine dephosphorylation of a novel p67 peptide in a manner regulated by extracellular calcium [J] . Karim ZA, Mukhopadhyay S, Ramars ASS, Biochimica et biophysica acta. Molecular cell research . 2004,第2期

机译：持续刺激血小板凝血酶受体与新型p67肽的酪氨酸去磷酸化作用有关，这种抑制作用受细胞外钙调节
4. Label-free detection of protein released during platelet activation by CNT-enhanced love mode SAW sensors [C] . Wu Huiyan, Zu Hongfei, Wang Qing-Ming, IEEE International Ultrasonics Symposium . 2014

机译：通过CNT增强的Love模式SAW传感器对血小板活化过程中释放的蛋白质进行无标记检测
5. Platelet-derived growth factor receptor-beta mediates the tyrosine phosphorylation of the low-density lipoprotein receptor-related protein throughout the endocytic process. [D] . Newton, Christopher S. 2007

机译：在整个内吞过程中，血小板衍生的生长因子受体-β介导低密度脂蛋白受体相关蛋白的酪氨酸磷酸化。
6. The GPIIbIIIa antagonist drugs eptifibatide and tirofiban do not induce activation of apoptosis executioner caspase-3 in resting platelets but inhibit caspase-3 activation in platelets stimulated with thrombin or calcium ionophore A23187 [O] . Valery Leytin, Asuman Mutlu, Sergiy Mykhaylov, 2009

机译：GPIIbIIIa拮抗剂药物eptifibatide和tirofiban不会在静息血小板中诱导凋亡执行者caspase-3活化但会抑制凝血酶或钙离子载体A23187刺激的血小板中caspase-3活化。
7. Microvesicle release is associated with extensive protein tyrosine dephosphorylation in platelets stimulated by A23187 or a mixture of thrombin and collagen. [O] . Pasquet, J M, Dachary-Prigent, J, Nurden, A T 1998

机译：微囊泡释放与A23187或凝血酶和胶原蛋白混合物刺激的血小板中广泛的蛋白酪氨酸脱磷酸作用有关。

Microvesicle release is associated with extensive protein tyrosine dephosphorylation in platelets stimulated by A23187 or a mixture of thrombin and collagen.

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