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登革病毒与柯萨奇病毒在通过巨噬细胞呈递给B细胞方面的抗原竞争。

Antigenic competition between dengue and Coxsackie viruses for presentation to B cells by macrophages.

作者信息

Rizvi N, Chaturvedi U C, Mathur A

机构信息

Postgraduate Department of Microbiology, K.G. Medical College, Lucknow, India.

出版信息

Int J Exp Pathol. 1990 Dec;71(6):761-70.

Abstract

Macrophages (M phi) pulsed with dengue type 2 (DV) and Coxsackie B4 (CoxB) viruses present antigen to B lymphocytes leading to their clonal expansion as detected by counting antigen-specific IgM antibody plaque-forming cells (PFC). The present study was undertaken to investigate the site for competition in M phi between the two heterologous antigens, DV and CoxB, for their presentation to B cells. It was observed that DV-pulsed M phi presented antigen to B cells in mice depleted of T cells by treatment with anti-Thy 1.2 monoclonal antibodies. The B cells could not be stimulated in absence of M phi in mice treated with silica. The PFC counts for both the antigens were inhibited when M phi were pulsed simultaneously with DV and CoxB. PFC counts were increased by 53-120% by predigesting the antigens by trypsin. Inhibition of DV-specific response by CoxB was abrogated by predigesting CoxB. A marked reduction in DV-specific PFC response was observed when CoxB was superimposed on M phi pulsed with DV 24 h earlier. CoxB-specific PFC counts were not affected by superimposing DV on M phi pulsed with CoxB 24 h earlier. PFC response to the antigen given to M phi before glutaraldehyde fixation was not affected while that for the antigen given to glutaraldehyde-fixed M phi was markedly depressed. It is concluded that the competition between DV and CoxB for antigen presentation to B cells occurs in M phi at the level of antigen processing.

摘要

用2型登革热病毒(DV)和柯萨奇B4病毒(CoxB)脉冲处理的巨噬细胞(M phi)将抗原呈递给B淋巴细胞,导致其克隆扩增,这可通过计数抗原特异性IgM抗体斑块形成细胞(PFC)来检测。本研究旨在调查在M phi中两种异源抗原DV和CoxB之间竞争向B细胞呈递抗原的位点。观察到,用抗Thy 1.2单克隆抗体处理使T细胞耗竭的小鼠中,经DV脉冲处理的M phi将抗原呈递给B细胞。在用二氧化硅处理的小鼠中,在没有M phi的情况下B细胞无法被刺激。当M phi同时用DV和CoxB脉冲处理时,两种抗原的PFC计数均受到抑制。通过用胰蛋白酶预先消化抗原,PFC计数增加了53% - 120%。预先消化CoxB可消除CoxB对DV特异性反应的抑制。当在24小时前用DV脉冲处理的M phi上叠加CoxB时,观察到DV特异性PFC反应显著降低。在24小时前用CoxB脉冲处理的M phi上叠加DV时,CoxB特异性PFC计数不受影响。对戊二醛固定前给予M phi的抗原的PFC反应不受影响,而对给予戊二醛固定的M phi的抗原的PFC反应则明显降低。结论是,DV和CoxB在向B细胞呈递抗原方面的竞争发生在M phi的抗原加工水平上。

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