Cholera toxin stimulates human B-cell DR antigen biosynthesis at the level of translation

被引:3
作者
Papadimitriou, E [1 ]
Mintzas, A [1 ]
Skoutari, M [1 ]
Dimitracopoulos, G [1 ]
Anastassiou, ED [1 ]
机构
[1] UNIV PATRAS,SCH MED,DEPT MICROBIOL,GR-26110 PATRAS,GREECE
关键词
D O I
10.1006/cimm.1997.1167
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Cholera toxin (CT) exerts many diverse regulatory effects on cells of the immune system and is considered a potent adjuvant on gut mucosal immune responses to orally presented antigens. It has been previously described that CT induces surface DR expression in human resting B-cells. As a further step toward understanding this phenomenon, the molecular mechanisms underlying the regulation of DR expression were investigated. By the use of Western analysis, it is shown that CT increases the total levels of DR protein in highly purified human tonsillar cells. [S-35]Methionine incorporation studies show that the aforementioned increase is due to de novo biosynthesis of DR protein at as early as 6 hr after CT stimulation and is completed by 24 hr. [H-3]Uridine uptake experiments, nuclear transcription runoff assays, and Northern analysis show that CT does not exert its effect at a transcriptional level, indicating translational regulation. Anti-IgM, which mimics B-cell antigen binding, behaves in a manner similar to CT. The B subunit of CT (B-CT) and prostaglandin E-2, either alone or in combination, do not induce DR protein biosynthesis nor do they exert any effect on the transcription of DR beta 1 gene. These results show that cAMP elevation as well as binding of B-CT to GM-1 ganglioside, by themselves, do not lead to DR protein biosynthesis suggesting that other activation pathways may be involved. (C) 1997 Academic Press.
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页码:176 / 184
页数:9
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