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人肥大细胞类胰蛋白酶从人C3生成C3a过敏毒素。

Generation of C3a anaphylatoxin from human C3 by human mast cell tryptase.

作者信息

Schwartz L B, Kawahara M S, Hugli T E, Vik D, Fearon D T, Austen K F

出版信息

J Immunol. 1983 Apr;130(4):1891-5.

PMID:6339618
Abstract

Tryptase, the dominant neutral protease of human pulmonary mast cell secretory granules, has the capacity in vitro to generate C3a anaphylatoxin from purified human C3. Only the alpha-chain of C3 is cleaved, and major fragments with apparent m.w. of 105,000, 39,500, 34,000, 29,000, and 9000 are detected by sodium dodecyl sulfate (SDS) polyacrylamide gel electrophoresis under reducing conditions. Fragments of 34,000 and 9000 m.w. are detected without reduction. A portion of the 9000 m.w. protein corresponds to C3a by virtue of its co-migration in SDS polyacrylamide gels with purified C3a and with trypsin-generated C3a, by its detection in a radioimmunoassay for C3a, and by its contractile activity on the guinea pig ileum bioassay. In the presence of heparin, another component of the mast cell secretory granule, the rate of appearance and the distribution of C3 cleavage fragments as assessed in SDS polyacrylamide gels are not appreciably changed with the exception that no C3a material can be detected in the SDS polyacrylamide gels or by radioimmunoassay and bioassay of the unresolved reaction mixture. Enhanced catabolism of authentic C3a by tryptase occurs in the presence of heparin and by analogy when C3a is generated from C3 by tryptase in the presence of heparin. Whereas tryptase secreted by activated human mast cells may generate C3a, a potentially important additional mediator of immediate hypersensitivity events, the concomitant release of heparin may serve to down-regulate C3a irrespective of its mechanism of generation.

摘要

类胰蛋白酶是人类肺肥大细胞分泌颗粒中的主要中性蛋白酶,在体外有能力从纯化的人C3生成C3a过敏毒素。只有C3的α链被切割,在还原条件下通过十二烷基硫酸钠(SDS)聚丙烯酰胺凝胶电泳检测到表观分子量为105,000、39,500、34,000、29,000和9000的主要片段。在非还原条件下检测到分子量为34,000和9000的片段。9000分子量的蛋白质的一部分通过其在SDS聚丙烯酰胺凝胶中与纯化的C3a和胰蛋白酶生成的C3a共迁移、通过其在C3a放射免疫测定中的检测以及通过其在豚鼠回肠生物测定中的收缩活性而对应于C3a。在肥大细胞分泌颗粒的另一种成分肝素存在的情况下,SDS聚丙烯酰胺凝胶中评估的C3切割片段的出现速率和分布没有明显变化,只是在SDS聚丙烯酰胺凝胶中或通过未解析反应混合物的放射免疫测定和生物测定无法检测到C3a物质。在肝素存在的情况下,类胰蛋白酶对真实C3a的分解代谢增强,并且类推,当在肝素存在的情况下类胰蛋白酶从C3生成C3a时也是如此。虽然活化的人类肥大细胞分泌的类胰蛋白酶可能生成C3a,C3a是速发型超敏反应事件的潜在重要额外介质,但肝素的伴随释放可能有助于下调C3a,无论其生成机制如何。

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