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Lewis大鼠对偶氮苯胂酸-N-乙酰-L-酪氨酸的半抗原特异性T细胞应答。II. 经TNP-半抗原化的ABA-肽-菲可诱导辅助活性的证明

Hapten-specific T cell response to azobenzenearsonate-N-acetyl-L-tyrosine in the Lewis rat. II. Induction of helper activity demonstrated by TNP-haptenated ABA-peptide-Ficoll.

作者信息

Komatsu T, Amsden A, Lawn C Y, Leskowitz S

出版信息

J Immunol. 1983 Feb;130(2):579-85.

PMID:6336767
Abstract

In an effort to study T cell functions in Lewis rats immunized with ABA-N-acetyl-L-tyrosine (ABA-tyr), we developed an antigen that provides a sensitive assay of ABA-specific helper function that is read as an increase in TNP-specific plaque-forming cells (PFC). This antigen has ABA coupled to AECM-Ficoll by virtue of a tripeptide (tyr-ala-ala) spacer and TNP coupled to the AECM side chains. At subimmunogenic doses, this antigen induced 400 anti-TNP PFC/10(6) spleen cells in ABA-tyr-immunized rats. As many as 8000 PFC/10(6) spleen cells were induced with larger doses of antigen (200 micrograms). By contrast, only 490 PFC/10(6) spleen cells could be induced with 1 mg of the conventional doubly haptenated protein carriers such as ABA-BSA-TNP. Both direct and indirect PFC were induced by this antigen in primed rats. The use of this antigen and passive transfer techniques to study ABA-specific helper activity revealed some differences from ABA-specific delayed-type hypersensitivity (DTH) and in vitro proliferation, which were studied previously. Cells responsible for helper activity appeared sooner after immunization and were found most prominently in peritoneal exudates but also significantly in spleen where the cells responsible for DTH or in vitro proliferative responses were never found. By contrast, helper cells were not seen in lymph nodes, where some proliferative activity could be found. Of these three ABA-specific T cell functions, helper activity was least easily suppressed by the previously used regimens of ABA-tyr in incomplete freunds adjuvant (IFA). Moreover, helper activity appears after injection of ABA-tyr in IFA, a method that has never in our hands yielded detectable DTH or in vitro proliferative responses. Despite these differences, phenotyping with monoclonal antibodies indicated that cells responsible for helper and proliferative activities were both W3/25+ and OX8-.

摘要

为了研究用ABA-N-乙酰-L-酪氨酸(ABA- tyr)免疫的Lewis大鼠的T细胞功能,我们开发了一种抗原,该抗原可提供对ABA特异性辅助功能的灵敏检测,通过TNP特异性空斑形成细胞(PFC)的增加来读取结果。这种抗原通过三肽(tyr-ala-ala)间隔物将ABA与AECM-菲可耦合,并且将TNP耦合到AECM侧链上。在亚免疫原剂量下,这种抗原在ABA-tyr免疫的大鼠中诱导出400个抗TNP PFC/10⁶脾细胞。用较大剂量的抗原(200微克)可诱导出多达8000个PFC/10⁶脾细胞。相比之下,用1毫克传统的双半抗原化蛋白载体如ABA-BSA-TNP只能诱导出490个PFC/10⁶脾细胞。这种抗原在致敏大鼠中诱导了直接和间接PFC。使用这种抗原和被动转移技术来研究ABA特异性辅助活性,发现与之前研究的ABA特异性迟发型超敏反应(DTH)和体外增殖存在一些差异。负责辅助活性的细胞在免疫后出现得更早,最显著地存在于腹腔渗出物中,但在脾中也有显著发现,而负责DTH或体外增殖反应的细胞在脾中从未被发现。相比之下,在淋巴结中未发现辅助细胞,而在淋巴结中可发现一些增殖活性。在这三种ABA特异性T细胞功能中,辅助活性最难被之前在不完全弗氏佐剂(IFA)中使用的ABA-tyr方案所抑制。此外,辅助活性在IFA中注射ABA-tyr后出现,而在我们手中,这种方法从未产生可检测到的DTH或体外增殖反应。尽管存在这些差异,但用单克隆抗体进行表型分析表明,负责辅助和增殖活性的细胞均为W3/25⁺和OX8⁻。

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