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用于定量针对T细胞和菠萝蛋白酶处理的小鼠红细胞自身抗原的B细胞和血清抗体的新型酶联免疫吸附测定(ELISA)和酶联免疫斑点测定。

Novel ELISA and ELISA-spot assays used to quantitate B cells and serum antibodies specific for T cell and bromelated mouse red blood cell autoantigens.

作者信息

Klinman D M, Steinberg A D

机构信息

National Institute of Arthritis and Musculoskeletal Diseases, Bethesda, MD 20892.

出版信息

J Immunol Methods. 1987 Sep 24;102(2):157-64. doi: 10.1016/0022-1759(87)90072-x.

Abstract

The frequency of splenic B cells producing antibodies reactive with bromelain-treated mouse red blood cells (BrMRBC) or T cell surface antigens was examined in autoimmune and normal mice. This was accomplished by fixing target cells to microtiter plates such that their membrane antigens could be detected in ELISA and ELISA-spot assays. This technique was rapid, sensitive, and permitted antibodies of both the IgG and IgM isotypes to be measured independently. Autoimmune NZB, BXSB male and MRL-lpr/lpr mice had 10-100-fold higher levels of serum anti-BrMRBC and anti-T cell antibodies than did control DBA/2 and CBA/J animals. The frequency of splenic B cells producing autoantibodies of these specificities was similarly increased among autoimmune mice. In general, the number of antibody-forming cells (AFC) reactive with BrMRBCs was 2-5 times higher than the number reactive with T cell surface determinants. In NZB mice these cells produced primarily IgM autoantibodies whereas in MRL-lpr/lpr animals they secreted primarily IgG. The concentration of serum autoantibody did not precisely correlate with AFC frequency, indicating that immunoglobulin catabolism and other factors play a role in regulating serum antibody concentration.

摘要

在自身免疫小鼠和正常小鼠中检测了产生与菠萝蛋白酶处理的小鼠红细胞(BrMRBC)或T细胞表面抗原反应的抗体的脾脏B细胞频率。这是通过将靶细胞固定在微量滴定板上来实现的,以便在ELISA和ELISA斑点试验中检测其膜抗原。该技术快速、灵敏,并且能够独立测量IgG和IgM同种型的抗体。自身免疫性NZB、BXSB雄性和MRL-lpr/lpr小鼠的血清抗BrMRBC和抗T细胞抗体水平比对照DBA/2和CBA/J动物高10-100倍。在自身免疫小鼠中,产生这些特异性自身抗体的脾脏B细胞频率同样增加。一般来说,与BrMRBC反应的抗体形成细胞(AFC)数量比与T细胞表面决定簇反应的细胞数量高2-5倍。在NZB小鼠中,这些细胞主要产生IgM自身抗体,而在MRL-lpr/lpr动物中,它们主要分泌IgG。血清自身抗体浓度与AFC频率并不精确相关,这表明免疫球蛋白分解代谢和其他因素在调节血清抗体浓度中起作用。

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