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C3b、Bb衰变解离后Bb所表达的残余溶血和蛋白水解活性。

Residual hemolytic and proteolytic activity expressed by Bb after decay-dissociation of C3b,Bb.

作者信息

Fishelson Z, Müller-Eberhard H J

出版信息

J Immunol. 1984 Mar;132(3):1425-9.

PMID:6229580
Abstract

Bb (Mr = 63,000) is the catalytic site-bearing subunit of the C3 convertase of the alternative complement pathway, C3b,Bb, which is dissociated from the complex upon decay of the enzyme. Because purified Bb induced certain leukocyte activities, we examined whether it expresses residual hemolytic or proteolytic activity. Hemolytic activity of Bb was tested by using Factor B- or Factor D-depleted normal human serum and rabbit or sheep erythrocytes. Proteolytic activity of Bb was assessed by using purified C3 or C5 as substrates and SDS-PAGE to detect protein cleavage. Bb expressed metal-dependent hemolytic activity that was approximately 100-fold lower than that of Factor B. This activity could be inhibited by Factor H and enhanced by properdin. Low but statistically significant binding of 125I-labeled Bb to C3b on erythrocytes was demonstrated. Monoclonal antibodies that bind to Bb but not to intact Factor B inhibited the Bb hemolytic activity. Purified Bb cleaved C3 to C3a and C3b, as evidenced by the appearance of the alpha'-chain of C3b. It also cleaved C5 to C5a and C5b when cobra venom factor was present in the reaction mixture. Metal ions were required for expression of proteolytic activity, and Ni supported the activity better than Mg. These results indicate that decayed Bb has residual C3 and C5 cleaving activity and hemolytic activity, expression of which appears to require its association with C3b, C3(H2O), or cobra venom factor. These observations may aid in explaining the mechanism of action of Bb on leukocytes.

摘要

Bb(分子量63,000)是替代补体途径C3转化酶C3b,Bb中带有催化位点的亚基,该酶在衰变时会从复合物中解离。由于纯化的Bb可诱导某些白细胞活性,我们研究了它是否具有残余的溶血或蛋白水解活性。通过使用缺乏B因子或D因子的正常人血清以及兔或羊红细胞来检测Bb的溶血活性。通过使用纯化的C3或C5作为底物并采用SDS-PAGE检测蛋白裂解来评估Bb的蛋白水解活性。Bb表现出金属依赖性溶血活性,其活性比B因子低约100倍。该活性可被H因子抑制,并被备解素增强。已证实125I标记的Bb与红细胞上的C3b存在低水平但具有统计学意义的结合。与Bb结合但不与完整B因子结合的单克隆抗体可抑制Bb的溶血活性。纯化的Bb将C3裂解为C3a和C3b,C3b的α'链的出现证明了这一点。当反应混合物中存在眼镜蛇毒因子时,它还可将C5裂解为C5a和C5b。蛋白水解活性的表达需要金属离子,镍比镁更能支持该活性。这些结果表明,衰变的Bb具有残余的C3和C5裂解活性以及溶血活性,其表达似乎需要与C3b、C3(H2O)或眼镜蛇毒因子结合。这些观察结果可能有助于解释Bb对白细胞的作用机制。

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