Harisdangkul V, McDougal J S, Knapp M, Christian C L
J Immunol. 1975 Jul;115(1):216-22.
A method for purification of low molecular weight IgM (LMW IgM) which utilized salt precipitation, gel filtration, and insoluble immunoadsorbents is described. The yield from pathologic sera containing LMW IgM in the range of 15 to 36 mg% was approximately 20%. Antisera prepared against LMW IgM, IgM, and reduced-alkylated IgM recognized common determinants. Purified LMW IgM from seropositive rheumatoid subjects did not have rheumatoid factor activity in agglutination tests but demonstrated binding to 125I-labeled aggregated IgG. LMW IgM from a patient with SLE and vasculitis had anti-nuclear factor activity and anti-native DNA activity. When complexed with reduced-alkylated aggregated IgG, LMW IgM and IgM with anti-IgG activity were essentially equivalent on a weight basis in complement fixation. The source and function of LMW in biologic processes remain unknown.
本文描述了一种利用盐沉淀、凝胶过滤和不溶性免疫吸附剂纯化低分子量IgM(LMW IgM)的方法。从含有15至36mg%范围内LMW IgM的病理血清中获得的产量约为20%。针对LMW IgM、IgM和还原烷基化IgM制备的抗血清识别共同的决定簇。来自血清阳性类风湿性疾病患者的纯化LMW IgM在凝集试验中没有类风湿因子活性,但显示出与125I标记的聚集IgG结合。来自一名系统性红斑狼疮和血管炎患者的LMW IgM具有抗核因子活性和抗天然DNA活性。当与还原烷基化聚集IgG复合时,LMW IgM和具有抗IgG活性的IgM在补体固定方面按重量计基本相当。LMW在生物过程中的来源和功能仍然未知。