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未刺激血小板α颗粒中β-血小板球蛋白、血小板因子4和纤维蛋白原免疫细胞化学显示的最佳技术。

Optimal techniques for the immunocytochemical demonstration of beta-thromboglobulin, platelet factor 4, and fibrinogen in the alpha granules of unstimulated platelets.

作者信息

Stenberg P E, Shuman M A, Levine S P, Bainton D F

出版信息

Histochem J. 1984 Sep;16(9):983-1001. doi: 10.1007/BF01003853.

Abstract

The distribution of beta-thromboglobulin, platelet factor 4, and fibrinogen in unstimulated platelets was investigated by several immunocytochemical techniques. All three substances were found to be localized in the majority of platelet alpha granules either by immunoperoxidase methods on saponin-treated platelets or by colloidal gold immunoconjugates on frozen thin sections. The optimal conditions for preparing and fixing platelets for immunocytochemistry were also determined. Platelets obtained from blood dripped directly into fixative or anticoagulated blood were compared systematically with respect to shape. Temperature was found to be the most important variable. Immediately fixed platelets were generally disc-shaped, regardless of the temperature of the fixative. Reducing the temperature of blood (stored with anticoagulant) before fixation resulted in more swollen and fewer disc-shaped platelets. However, if the blood was mixed with an anticoagulant and maintained at 37 degrees C for 1 h before fixation, the same number of disc-shaped platelets were present as in samples from blood fixed immediately. The intracellular localization of beta-thromboglobulin, platelet factor 4, and fibrinogen was consistent regardless of platelet preparatory procedure, but several technical problems were encountered with respect to plasma membrane labelling when control experiments were analysed. Immediately fixed, non-permeabilized platelet plasma membranes were always labelled, no matter which control substances or immunoperoxidase markers were used. However, when platelets were washed by centrifugation, the plasma membranes were negative. Exposure to saponin markedly diminished labelling of the plasma membranes. Optimal techniques for the immunocytochemical demonstration of these alpha granule proteins in platelets are presented in this report.

摘要

采用多种免疫细胞化学技术研究了β-血小板球蛋白、血小板第4因子和纤维蛋白原在未受刺激血小板中的分布情况。通过对皂素处理过的血小板进行免疫过氧化物酶法,或对冷冻薄片进行胶体金免疫缀合物法,发现这三种物质均定位于大多数血小板α颗粒中。还确定了用于免疫细胞化学的血小板制备和固定的最佳条件。系统比较了直接滴入固定剂中的血液或抗凝血液中获得的血小板的形状。发现温度是最重要的变量。立即固定的血小板通常呈盘状,与固定剂的温度无关。固定前降低血液(用抗凝剂储存)的温度会导致血小板肿胀加剧且盘状血小板减少。然而,如果血液与抗凝剂混合并在固定前于37℃保持1小时,则盘状血小板的数量与立即固定的血液样本中的数量相同。无论血小板的制备程序如何,β-血小板球蛋白、血小板第4因子和纤维蛋白原的细胞内定位都是一致的,但在分析对照实验时,在质膜标记方面遇到了几个技术问题。无论使用哪种对照物质或免疫过氧化物酶标记物,立即固定的、未通透的血小板质膜总是被标记。然而,当通过离心洗涤血小板时,质膜呈阴性。暴露于皂素会显著减少质膜的标记。本报告介绍了血小板中这些α颗粒蛋白免疫细胞化学显示的最佳技术。

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