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首页> 美国卫生研究院文献>Journal of Virology >Identification of membrane antigen C33 recognized by monoclonal antibodies inhibitory to human T-cell leukemia virus type 1 (HTLV-1)-induced syncytium formation: altered glycosylation of C33 antigen in HTLV-1-positive T cells.
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Identification of membrane antigen C33 recognized by monoclonal antibodies inhibitory to human T-cell leukemia virus type 1 (HTLV-1)-induced syncytium formation: altered glycosylation of C33 antigen in HTLV-1-positive T cells.

机译:鉴定对人T细胞白血病病毒1型(HTLV-1)诱导的合胞体形成有抑制作用的单克隆抗体识别的膜抗原C33:改变HTLV-1阳性T细胞中C33抗原的糖基化。

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We isolated four monoclonal antibodies (MAbs), M38, M101, M104, and C33, which were capable of inhibiting syncytium formation induced in a human T-cell line, MOLT-4-#8, by coculture with human T-cell leukemia virus type 1 (HTLV-1)-positive human T-cell lines. The MAbs had, however, no inhibitory activity on syncytium formation induced in a human osteosarcoma line, HOS, by HTLV-1-positive T-cell lines. They also did not inhibit syncytium formation induced in MOLT-4-#8 by human immunodeficiency virus type 1-positive MOLT-4. All MAbs reacted with various human cell lines of lymphoid and nonlymphoid origins, including HTLV-1-positive T-cell lines. Furthermore, they all reacted with a murine A9 clone containing human chromosome 11 fragment q23-pter. Two MAbs, M104 and C33, immunoprecipitated a membrane antigen with the same molecular size. The antigen (henceforth called C33 antigen) was about 40 to 55 kDa in HTLV-1-negative Jurkat, CEM, MOLT-4, and normal peripheral blood CD4-positive human T cells and about 40 to 75 kDa in HTLV-1-positive C91/PL, TCL-Kan, MT-2, and in fresh HTLV-1-transformed CD4-positive human T-cell lines. Pulse-chase experiments revealed that C33 antigen was synthesized as a 35-kDa precursor that was then processed to 41 to 50 kDa in MOLT-4 and to 44 to 70 kDa in C91/PL. In the presence of tunicamycin, a 28-kDa protein was synthesized. The conversion from 35 kDa to 41 to 50 kDa in MOLT-4 and to 44 to 70 kDa in C91/PL was inhibited by monensin. Treatment with N-glycanase alone, but not with sialidase and O-glycanase in combination, completely removed the sugar moiety of C33 antigen from both HTLV-1-negative Jurkat and HTLV-1-positive C91/PL. Therefore, C33 antigen has only N-linked carbohydrates, the modification of which appears to be substantially altered in the presence of the HTLV-1 genome.
机译:我们分离了四种单克隆抗体(MAb)M38,M101,M104和C33,它们能够与人T细胞白血病病毒共培养,从而抑制人T细胞系MOLT-4-#8中诱导的合胞体形成1型(HTLV-1)阳性人类T细胞系。但是,单克隆抗体对HTLV-1阳性T细胞系在人骨肉瘤系HOS中诱导的合胞体形成没有抑制活性。他们也没有抑制人类免疫缺陷病毒1型阳性MOLT-4在MOLT-4-#8中诱导的合胞体形成。所有单克隆抗体都与各种人类淋巴和非淋巴来源的细胞系发生反应,包括HTLV-1阳性T细胞系。此外,它们都与含有人类11号染色体片段q23-pter的鼠A9克隆反应。两个单克隆抗体M104和C33免疫沉淀具有相同分子大小的膜抗原。 HTLV-1阴性Jurkat,CEM,MOLT-4和正常外周血CD4阳性人T细胞中的抗原(以下称为C33抗原)约为40至55 kDa,而HTLV-1阳性的抗原约为40至75 kDa。 C91 / PL,TCL-Kan,MT-2和新鲜的HTLV-1转化的CD4阳性人T细胞系。脉冲追踪实验表明,C33抗原被合成为35 kDa的前体,然后在MOLT-4中被加工成41至50 kDa,在C91 / PL中被加工成44至70 kDa。在衣霉素的存在下,合成了28kDa的蛋白质。莫能菌素抑制了MOLT-4中从35 kDa到41至50 kDa的转化和C91 / PL中的44至70 kDa的转化。单独用N-聚糖酶治疗,而不是用唾液酸酶和O-聚糖酶联合治疗,可完全从HTLV-1阴性Jurkat和HTLV-1阳性C91 / PL中完全去除C33抗原的糖部分。因此,C33抗原仅具有N-连接的碳水化合物,其修饰似乎在HTLV-1基因组的存在下被实质性改变。

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