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A recombinant hybrid anaphylatoxin with dual C3a/C5a activity

机译:具有双重C3a / C5a活性的重组杂合过敏毒素

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pBy site-directed mutagenesis of a human complement factor C5a cDNA clone, we have designed a hybrid anaphylatoxin in which three amino acid residues in the C-terminal sequence of human C5a were exchanged to create the native C-terminal human C3a (hC3a) sequence Leu-Gly-Leu-Ala-Arg. This hybrid anaphylatoxin rC5a-(1-69)-LGLAR exhibited true C3a and C5a activity when tested in the guinea pig ileum contraction assay. Quantitative measurements of ATP release from guinea pig platelets revealed about 1% intrinsic C3a activity for this hybrid, while the C5a activity was essentially unchanged. Competitive binding assays confirmed that the rC5a-(1-69)-LGLAR mutant was able to displace radioiodinated rhC5a with a KI of approx. 40 nM and hC3a with a KI of approx. 3.7 microM from guinea pig platelets. Since the C-termini of both human C3a and C5a anaphylatoxins are known to interact with their respective receptors, we conclude that the same peptidic sequence, LGLAR, is able to bind to and activate two different receptors, the C3a receptor as well as the C5a receptor. This clone provides a novel tool for the identification of further receptor-binding residues in both anaphylatoxins, since any mutants may be tested for altered C3a and C5a activity simultaneously./p
机译:>通过人补体因子C5a cDNA克隆的定点诱变,我们设计了一种杂种过敏毒素,其中人C5a的C端序列中的三个氨基酸残基被交换以创建天然C端的人C3a( hC3a)序列Leu-Gly-Leu-Ala-Arg。当在豚鼠回肠收缩试验中进行测试时,这种杂合的过敏毒素rC5a-(1-69)-LGLAR表现出真正的C3a和C5a活性。从豚鼠血小板中释放的ATP的定量测量表明,该杂种的C3a固有活性约为1%,而C5a的活性基本未变。竞争性结合试验证实,rC5a-(1-69)-LGLAR突变体能够以KI约为KI取代放射性碘化的rhC5a。 40 nM和hC3a的KI约为1。来自豚鼠血小板的3.7 microM。由于已知人C3a和C5a过敏毒素的C末端均与它们各自的受体相互作用,因此我们得出结论,相同的肽序列LGLAR能够结合并激活两个不同的受体,即C3a受体和C5a受体。该克隆为鉴定两种过敏毒素中的其他受体结合残基提供了一种新颖的工具,因为可以同时测试任何突变体的C3a和C5a活性。

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