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白细胞弹性蛋白酶增强组织蛋白酶G诱导的血小板活化:对中性粒细胞介导的血小板活化的影响。

Enhancement of cathepsin G-induced platelet activation by leukocyte elastase: consequence for the neutrophil-mediated platelet activation.

作者信息

Renesto P, Chignard M

机构信息

Unité de Pharmacologie Cellulaire, Unité Associée Institut Pasteur/INSERM 285, Institut Pasteur, Paris, France.

出版信息

Blood. 1993 Jul 1;82(1):139-44.

PMID:8324217
Abstract

We have focused our interest on the platelet-activating properties of two polymorphonuclear neutrophil (PMN)-derived proteinases, namely elastase (HLE) and cathepsin G (Cat.G). First of all, we observed that whereas HLE was unable to trigger platelet activation by itself, it enhanced platelet activation induced by Cat.G when both proteinases were added simultaneously. It has been recently described that, upon stimulation, PMN released Cat.G, which in turn activated surrounding platelets. Thus, we looked for a combined effect of Cat.G and HLE during this cell-to-cell interaction. When PMN (5 x 10(6)/mL) were stimulated by 0.5 mumol/L N-formyl-Met-Leu-Phe, they released 237.9 +/- 49.1 nmol/L Cat.G and 381.7 +/- 28.0 nmol/L HLE. Such a concentration of purified Cat.G (240 nmol/L) induced only a moderate platelet activation when added to a PMN-platelet mixture. However, when Cat.G (240 nmol/L) and HLE (380 nmol/L) were added together, the resulting platelet activation was strictly comparable to that corresponding to the addition of N-formyl-Met-Leu-Phe (P > .05) in terms of aggregation, dense and alpha granule secretion, and thromboxane B2 production. In fact, Elafin, a specific HLE inhibitor, when added to the PMN-platelet cooperation system triggered by N-formyl-Met-Leu-Phe, prevented platelet activation within the same range of concentrations as for inhibition of HLE activity. In conclusion, we now show that not only Cat.G, but also HLE is involved in the PMN-mediated platelet activation.

摘要

我们将研究兴趣集中在两种多形核中性粒细胞(PMN)衍生的蛋白酶,即弹性蛋白酶(HLE)和组织蛋白酶G(Cat.G)的血小板激活特性上。首先,我们观察到,虽然HLE自身无法触发血小板激活,但当两种蛋白酶同时添加时,它会增强Cat.G诱导的血小板激活。最近有报道称,受到刺激时,PMN会释放Cat.G,进而激活周围的血小板。因此,我们探究了在这种细胞间相互作用过程中Cat.G和HLE的联合作用。当用0.5 μmol/L的N-甲酰甲硫氨酰亮氨酰苯丙氨酸刺激PMN(5×10⁶/mL)时,它们释放出237.9±49.1 nmol/L的Cat.G和381.7±28.0 nmol/L的HLE。将如此浓度的纯化Cat.G(240 nmol/L)添加到PMN-血小板混合物中时,仅诱导了适度的血小板激活。然而,当将Cat.G(240 nmol/L)和HLE(380 nmol/L)一起添加时,就聚集、致密颗粒和α颗粒分泌以及血栓素B2产生而言,所产生的血小板激活与添加N-甲酰甲硫氨酰亮氨酰苯丙氨酸时的激活情况严格相当(P>0.05)。事实上,特异性HLE抑制剂Elafin添加到由N-甲酰甲硫氨酰亮氨酰苯丙氨酸触发的PMN-血小板协作系统中时,在与抑制HLE活性相同的浓度范围内可阻止血小板激活。总之,我们现在表明,不仅Cat.G,而且HLE也参与了PMN介导的血小板激活。

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Enhancement of cathepsin G-induced platelet activation by leukocyte elastase: consequence for the neutrophil-mediated platelet activation.白细胞弹性蛋白酶增强组织蛋白酶G诱导的血小板活化:对中性粒细胞介导的血小板活化的影响。
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