Measurements of the G-/F-actin equilibrium in ADP-stimulated human platelets.

Acta histochemica. Supplementband Pub Date : 1991-01-01
P Spangenberg, S Heptinstall, J Crawford, U Till
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Abstract

The amounts of the different forms of actin (G-actin, F-actin) can be measured biochemically following lysis of the cells by the DNase I inhibition assay. The existing methodology for studying G-actin in unstimulated platelets was found to be inappropriate for studies during ADP-induced platelet activation. However, this problem was overcome by a simple modification of the procedure in which formaldehyde was added to the buffer used to lyse the activated platelets. Using this modification the G-actin values obtained immediately after lysis did not change during storage of the lysates on ice for more than 30 minutes. The results show rapid conversion of G-actin to F-actin in association with the shape change during ADP-stimulated activation. Examination of unstimulated platelets using the modified procedure enabled identification of a pool of actin that is rapidly dissociated to G-actin in the absence of formaldehyde, the existence of which had not previously been recognised.

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adp刺激的人血小板中G-/ f -肌动蛋白平衡的测量。
不同形式的肌动蛋白(g -肌动蛋白,f -肌动蛋白)的数量可以通过dna酶I抑制实验在细胞裂解后进行生化测量。研究未刺激血小板中g -肌动蛋白的现有方法被发现不适合研究adp诱导的血小板活化过程。然而,这个问题是克服了一个简单的修改程序,其中甲醛添加到缓冲液用于裂解活化血小板。使用这种修饰,裂解后立即获得的g -肌动蛋白值在裂解物在冰上储存超过30分钟时没有变化。结果表明,在adp刺激激活过程中,g -肌动蛋白向f -肌动蛋白的快速转化与形状变化有关。使用改进的程序检查未刺激的血小板,可以识别在没有甲醛的情况下迅速解离为g -肌动蛋白的肌动蛋白池,甲醛的存在以前没有被认识到。
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