首页> 外文OA文献 >Cellular origins of human polymeric and monomeric IgA: enumeration of single cells secreting polymeric IgA1 and IgA2 in peripheral blood, bone marrow, spleen, gingiva and synovial tissue.
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Cellular origins of human polymeric and monomeric IgA: enumeration of single cells secreting polymeric IgA1 and IgA2 in peripheral blood, bone marrow, spleen, gingiva and synovial tissue.

机译:人类聚合和单体IgA的细胞起源:在外周血,骨髓,脾,齿龈和滑膜组织中分泌聚合IgA1和IgA2的单个细胞的计数。

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摘要

Using modified ELISA and spot-ELISA, which permit the parallel determination of heavy chain subclass and the presence of covalently linked J chain, we analysed IgA found in cell culture supernatants or secreted by individual cells from peripheral blood, spleen, bone marrow, gingiva and synovial tissue, with respect to its polymeric or monomeric IgA form (pIgA, mIgA) and IgA1 or IgA2 subclass. The ELISA for determination of J chain in tissue culture supernatants was specific and highly sensitive (detection limit in pg). The results demonstrated that IgA1-producing cells predominated in the tissues examined, and that J chain could be detected in association with the majority of IgA1 and IgA2 secreted by individual cells. With respect to the frequency of cells secreting polymeric, J chain-containing IgA, only 20-30% of cells from the bone marrow were engaged in the synthesis of PIgA. In other tissues the frequency of cells secreting pIgA1 and pIgA2 was considerably higher. Peripheral blood mononuclear cells secreting pIgA2 were easily inducible during stimulation with T cell-dependent pokeweed mitogen, whereas Epstein-Barr virus-transformed cells secreted preferentially mIgA1. When the frequencies of pIgA-, pIgA1- or pIgA2-secreting cells (determined by spot-ELISA technique) from different tissues were correlated with the proportion of pIgA to mIgA (and IgA subclasses) secreted in tissue culture supernatants, data obtained suggest that many individual IgA-producing cells could be engaged in simultaneous secretion of mIgA and pIgA.
机译:我们使用改良的ELISA和定点ELISA方法,可以平行测定重链亚类和共价连接的J链的存在,我们分析了细胞培养上清液中发现的IgA或外周血,脾脏,骨髓,牙龈和皮肤中单个细胞分泌的IgA。滑膜组织,就其聚合或单体IgA形式(pIgA,mIgA)和IgA1或IgA2亚类而言。用于测定组织培养上清液中J链的ELISA具有特异性和高度敏感性(检测限以pg为单位)。结果表明,在检查的组织中占主导地位的是产生IgA1的细胞,并且可以与单个细胞分泌的大多数IgA1和IgA2相关联地检测到J链。关于分泌聚合的含J链的IgA的细胞的频率,仅20-30%的来自骨髓的细胞参与了PIgA的合成。在其他组织中,分泌pIgA1和pIgA2的细胞的频率要高得多。分泌pIgA2的外周血单核细胞在用T细胞依赖的商陆有丝分裂原刺激时很容易诱导,而爱泼斯坦-巴尔病毒转化的细胞优先分泌mIgA1。当来自不同组织的分泌pIgA-,pIgA1-或pIgA2的细胞的频率(通过斑点ELISA技术确定)与组织培养上清液中分泌的pIgA与mIgA(和IgA亚类)的比例相关时,获得的数据表明单个产生IgA的细胞可以同时分泌mIgA和pIgA。

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