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大鼠体内血小板激活因子和血小板溶解因子的免疫生成

The immunological generation of a platelet-activating factor and a platet-lytic factor in the rat.

作者信息

Valone F H, Whitmer D I, Pickett W C, Austen K F, Goetzl E J

出版信息

Immunology. 1979 Aug;37(4):841-8.

Abstract

Antigen challenge of the rat peritoneal cavity which had been prepared with IgGa-rich antiserum generated activities which released [14C]-serotonin from pre-labelled human platelets. After adsorption of these activities onto Amberlite XAD-8 and elution in 80% ethanol, two factors of differing polarity were resolved by chromatography on diethylaminoethyl cellulose in organic solvents. The activity eluting in the 7:1 chloroform:methanol solvent contained a platelet-lytic factor (PLF) assessed by the parallel release of lactic acid dehydrogenase and [14C]-serotonin; the cytotoxicity of this fraction was confirmed by phase-contrast microscopy examination which demonstrated fragmentation of the exposed platelets. The activity eluting in the 1:1 methanol: aqueous 1.0 M ammonium carbonate solvent was a platelet-activating factor (PAF) as defined by release of [14C]-serotonin without lactic acid dehydrogenase. Both the lytic and the activating principles were separable from slow reacting substance of anaphylaxis and polymorphonuclear leucocyte chemotactic activity, and each presented a single activity peak of differing mobility when chromatographed on silica gel H plates. Human eosinophil phospholipase D inactivated the lytic factor by more than 85% in 2 h at 37 degrees without affecting the activity of the activating factor. The release of [14C]-serotonin induced by the PAF was not affected by the absence of calcium from the medium or by elevations in the platelet concentrations of cyclic AMP or cyclic GMP that resulted from pre-incubation of platelets with prostaglandin D2 or sodium ascorbate, respectively.

摘要

用富含IgGa的抗血清预处理大鼠腹腔后进行抗原激发,产生的活性物质可使预先标记的人血小板释放[14C] - 5 -羟色胺。这些活性物质吸附到Amberlite XAD - 8上,并用80%乙醇洗脱后,通过在有机溶剂中用二乙氨基乙基纤维素进行色谱分离,得到了两种极性不同的因子。在氯仿:甲醇为7:1的溶剂中洗脱的活性物质含有一种血小板溶解因子(PLF),通过乳酸脱氢酶和[14C] - 5 -羟色胺的平行释放来评估;通过相差显微镜检查证实了该组分的细胞毒性,该检查显示暴露的血小板发生了破碎。在甲醇:1.0 M碳酸铵水溶液为1:1的溶剂中洗脱的活性物质是一种血小板激活因子(PAF),其定义为释放[14C] - 5 -羟色胺而不释放乳酸脱氢酶。溶解和激活原理均与过敏反应慢反应物质及多形核白细胞趋化活性可分离,并且在硅胶H板上进行色谱分析时,每种都呈现出一个迁移率不同的单一活性峰。人嗜酸性粒细胞磷脂酶D在37℃下2小时内使溶解因子失活超过85%,而不影响激活因子的活性。PAF诱导的[14C] - 5 -羟色胺释放不受培养基中无钙的影响,也不受血小板分别与前列腺素D2或抗坏血酸钠预孵育导致的血小板环磷酸腺苷(cAMP)或环磷酸鸟苷(cGMP)浓度升高的影响。

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