Immunoelectrophoretic analysis of C4 split products expressing D but not C epitopes: influence of storage, Ca2+ and Ca2+-chelating agents.

N E Petersen, J Folkersen, B Teisner, S E Svehag
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引用次数: 2

Abstract

Based on immunoelectrophoretic methods a heterogeneity in the electrophoretic mobility of C4d was observed. C4d was defined immunochemically as C4 molecules expressing D but lacking C epitopes. A beta-mobile form was observed when EDTA or heparin was not added to the sample prior to electrophoretic analysis. This component was generated during electrophoresis. Another C4d component migrating to the post-albumin region probably represented an in vivo generated split product. However, this C4d form was also produced during storage of serum or plasma at room temperature and its formation was enhanced in the presence of EDTA. Based on these findings standard conditions for collection and storage of clinical samples for quantification of C4d by electroimmunoassay are suggested.

表达D而不表达C表位的C4分裂产物的免疫电泳分析:储存、Ca2+和Ca2+螯合剂的影响。
基于免疫电泳方法,观察到C4d的电泳迁移率存在异质性。免疫化学将C4d定义为表达D但缺乏C表位的C4分子。当EDTA或肝素未添加到电泳分析之前的样品时,观察到β -移动形式。该成分是在电泳过程中产生的。另一个迁移到白蛋白后区域的C4d成分可能代表了体内产生的分裂产物。然而,在室温下血清或血浆中也会产生这种C4d形式,并且在EDTA存在下其形成增强。在此基础上,提出了电免疫法定量C4d临床样品采集和储存的标准条件。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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