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Rapid and sensitive techniques for identification and analysis of 'reactive-centre' mutants of C1-inhibitor proteins contained in type II hereditary angio-oedema plasmas.

机译:快速和灵敏的技术,用于鉴定和分析II型遗传性血管性水肿血浆中C1抑制剂蛋白的“反应中心”突变体。

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摘要

Novel procedures for structural analysis of the 'reactive-centre' residues, particularly the P1 residue, of the dysfunctional C1-inhibitor proteins found in the plasmas of type II hereditary angio-oedema (HAE) patients are described. C1-inhibitor is adsorbed directly from plasma on to Sepharose-anti-(C1 inhibitor) beads. The P1 residue of C1 inhibitor is arginine and hence a potential cleavage site for trypsin. Thus trypsin digestion of the immobilized protein, followed by SDS/PAGE of the released fragments, identifies P1 residue mutations. Pseudomonas aeruginosa elastase digestion of the immobilized protein, followed by purification of the released C-terminal peptide (by h.p.l.c.) and N-terminal sequence analysis defines the new P1 residue (or other mutations in the reactive-centre region). The techniques are both rapid and highly sensitive, requiring only 400 microliters of plasma. In addition, they permit accurate assessment of the level of normal (functional) inhibitor in a subclass of type II HAE plasmas, those containing P1-residue mutant proteins.
机译:描述了用于II型遗传性血管性水肿(HAE)患者血浆中功能失调的C1抑制剂蛋白的“反应中心”残基,特别是P1残基的结构分析的新方法。 C1抑制剂直接从血浆中吸附到Sepharose-anti-(C1抑制剂)珠上。 C1抑制剂的P1残基是精氨酸,因此可能是胰蛋白酶的切割位点。因此,胰蛋白酶消化固定的蛋白质,然后对释放的片段进行SDS / PAGE,可以鉴定P1残基突变。铜绿假单胞菌弹性蛋白酶消化固定的蛋白质,然后纯化释放的C末端肽(通过h.p.l.c.)和N末端序列分析确定新的P1残基(或反应中心区域的其他突变)。该技术既快速又高度敏感,仅需要400微升血浆。此外,它们允许准确评估II型HAE血浆亚类中正常(功能性)抑制剂的水平,这些血浆中含有P1残基突变蛋白。

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  • 作者

    Aulak, K S; Harrison, R S;

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  • 年度 1990
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  • 原文格式 PDF
  • 正文语种 en
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