首页> 美国卫生研究院文献>Journal of Virology >Monoclonal and polyclonal antibodies against Epstein-Barr virus nuclear antigen 5 (EBNA-5) detect multiple protein species in Burkitts lymphoma and lymphoblastoid cell lines.
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Monoclonal and polyclonal antibodies against Epstein-Barr virus nuclear antigen 5 (EBNA-5) detect multiple protein species in Burkitts lymphoma and lymphoblastoid cell lines.

机译:针对爱泼斯坦-巴尔病毒核抗原5(EBNA-5)的单克隆和多克隆抗体可检测Burkitt淋巴瘤和淋巴母细胞系中的多种蛋白质。

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摘要

The Epstein-Barr virus nuclear antigen 5 (EBNA-5) is encoded by highly spliced mRNA from the major IR1 (BamHI-W) repeat region of the virus genome. A mouse monoclonal antibody, JF186, has been raised against a synthetic 18-amino-acid peptide deduced from the EBNA-5 message of B95-8 and Raji cells. The antibody showed characteristic coarse nuclear granules by indirect immunofluorescence and revealed multiple EBNA-5 species by immunoblotting and immunoprecipitation. The B95-8 line itself and all B95-8 virus-carrying cells, whether lymphoblastoid cell lines or in vitro-converted sublines of Epstein-Barr virus (EBV)-negative Burkitt's lymphoma (BL) lines, were EBNA-5 positive. Among 36 cell lines carrying different EBV strains, only 10 expressed the B95-8-Raji-prototype EBNA-5 recognized by JF186; this was probably due to genetic variation in the epitope recognized by JF186, as shown for P3HR-1. Human antibodies, affinity purified against EBNA-5-JF186 immunoprecipitates, detected EBNA-5 in the majority of EBV-positive BL lines and in all lymphoblastoid cell lines containing the BL-derived viruses. Thus, EBNA-5 can be expressed by all virus isolates examined, but is down-regulated, together with other latent gene products, in a minority of BL lines which have a particular cellular phenotype. EBNA-5 was detected as a ladder of protein species of 20 to 130 kilodaltons (kDa), with a regular spacing of 6 to 8 kDa, consistent with the coding capacity of the combined BamHI-W 66- and 132-base-pair exons, together with shifts of 2 to 4 kDa, consistent with the size of the separate 66- and 132-base-pair exons. Multiple EBNA-5 proteins can be expressed by the single cell as shown by cloning of newly infected cells.
机译:爱泼斯坦巴尔病毒核抗原5(EBNA-5)由来自病毒基因组主要IR1(BamHI-W)重复区域的高度剪接的mRNA编码。已针对从B95-8和Raji细胞的EBNA-5信息推导的合成18-氨基酸肽产生了小鼠单克隆抗体JF186。该抗体通过间接免疫荧光显示出特征性的粗核颗粒,并通过免疫印迹和免疫沉淀显示出多种EBNA-5种类。 B95-8系本身和所有携带B95-8病毒的细胞,无论是淋巴母细胞系还是体外转化的爱泼斯坦-巴尔病毒(EBV)阴性的伯基特淋巴瘤(BL)系,都是EBNA-5阳性。在携带不同EBV株的36个细胞系中,只有10个表达被JF186识别的B95-8-Raji原型EBNA-5。如P3HR-1所示,这可能是由于JF186识别的表位的遗传变异所致。针对EBNA-5-JF186免疫沉淀物亲和纯化的人抗体在大多数EBV阳性BL系和所有包含BL衍生病毒的淋巴母细胞系中检测到EBNA-5。因此,EBNA-5可以在所有具有特定细胞表型的BL系中被检测到的所有病毒分离株表达,但与其他潜在基因产物一起被下调。 EBNA-5被检测为20至130千道尔顿(kDa)的蛋白质物种的阶梯,规则间距为6至8 kDa,与结合的BamHI-W 66和132个碱基对外显子的编码能力一致,以及2至4 kDa的位移,与单独的66和132个碱基对外显子的大小一致。如克隆新感染的细胞所示,单个细胞可以表达多种EBNA-5蛋白。

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