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Jurkat细胞中70千道尔顿的百日咳毒素结合蛋白。

The 70-kilodalton pertussis toxin-binding protein in Jurkat cells.

作者信息

Armstrong G D, Clark C G, Heerze L D

机构信息

Department of Medical Microbiology and Infectious Diseases, University of Alberta, Edmonton, Canada.

出版信息

Infect Immun. 1994 Jun;62(6):2236-43. doi: 10.1128/iai.62.6.2236-2243.1994.

Abstract

125I-ASD photoaffinity-labeling derivatives of pertussis toxin (125I-ASD-PT) or lipopolysaccharide (125I-ASD-LPS) labeled similar 70-kDa proteins in Jurkat cells, a cell line derived from human CD4+ T lymphocytes. Labeling of this 70-kDa protein by 125I-ASD-PT was inhibited by underivatized PT but not by underivatized LPS. However, an immunoglobulin M monoclonal antibody with specificity for the p73 LPS receptor in murine splenocytes (S. W. Bright, T.-Y. Chen, L. M. Flebbe, M.-G. Lei, and D. C. Morrison, J. Immunol. 145:1-7, 1990) inhibited 125I-ASD-PT labeling of the 70-kDa species in Jurkat cells. Our results suggested that PT may bind to the same 70-kDa protein as LPS does in Jurkat cells but that PT and LPS bind to different sites on this receptor candidate. 125I-ASD-PT photoaffinity labeling of the 70-kDa protein was also inhibited by underivatized glycoproteins to which PT has been shown to bind, and this inhibition correlated with the relative binding affinities of the glycoproteins for PT. 125I-ASD derivatives of two sialic acid-specific plant lectins, Maackia amurensis leukoagglutinin and Sambucus nigra agglutinin, with oligosaccharide binding specificities similar to those of PT also labeled a 70-kDa protein in Jurkat cells. This suggests that the 70-kDa PT receptor candidate in Jurkat cells likely contains sialooligosaccharide sequences to which PT, M. amurensis leukoagglutinin, and S. nigra agglutinin bind. The cross-reacting epitope recognized by monoclonal antibody 5D3 in this 70-kDa species might overlap the PT- and LPS-binding sites.

摘要

百日咳毒素(125I-ASD-PT)或脂多糖(125I-ASD-LPS)的125I-ASD光亲和标记衍生物在Jurkat细胞(一种源自人CD4 + T淋巴细胞的细胞系)中标记了相似的70 kDa蛋白质。125I-ASD-PT对这种70 kDa蛋白质的标记被未衍生化的PT抑制,但未被未衍生化的LPS抑制。然而,一种对鼠脾细胞中p73 LPS受体具有特异性的免疫球蛋白M单克隆抗体(S. W. Bright、T.-Y. Chen、L. M. Flebbe、M.-G. Lei和D. C. Morrison,《免疫学杂志》145:1-7,1990)抑制了Jurkat细胞中70 kDa物种的125I-ASD-PT标记。我们的结果表明,PT可能与Jurkat细胞中LPS结合的是同一种70 kDa蛋白质,但PT和LPS结合在该候选受体的不同位点上。125I-ASD-PT对70 kDa蛋白质的光亲和标记也被已证明PT能结合的未衍生化糖蛋白抑制,这种抑制与糖蛋白对PT的相对结合亲和力相关。两种具有与PT相似的寡糖结合特异性的唾液酸特异性植物凝集素——黑芥凝集素和接骨木凝集素的125I-ASD衍生物,也在Jurkat细胞中标记了一种70 kDa蛋白质。这表明Jurkat细胞中70 kDa的PT候选受体可能含有PT、黑芥凝集素和接骨木凝集素能结合的唾液酸寡糖序列。单克隆抗体5D3在这种70 kDa物种中识别的交叉反应表位可能与PT和LPS的结合位点重叠。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5ba7/186503/e2a55902d4bb/iai00006-0108-a.jpg

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