Hironaka T, Nagasaki M, Morikawa S, Hirai K
Department of Cell Regulation, Tokyo Medical and Dental University, Japan.
J Virol Methods. 1993 Oct;44(2-3):141-54. doi: 10.1016/0166-0934(93)90050-2.
We report a simple procedure for the detection of Epstein-Barr virus (EBV) by in situ DNA-RNA hybridization with an alkaline phosphatase-linked oligonucleotide probe. EBV-producing cell lines P3HR-1 and Akata were treated with phorbol ester and n-butyrate, and anti-human IgG, respectively. This treatment resulted in highly increased populations of cells with EBV transcripts of the latent membrane protein 1 (LMP1) and envelop glycoprotein gp350/220, but not of EBV-encoded small nuclear RNAs (EBERs). Synthesis of the LMP1 protein, which was encoded by the induced mRNA, was mostly dependent on viral DNA synthesis, as shown by double or single labeling for in situ DNA-DNA hybridization with the oligo-nucleotide probe, and immunoperoxidase staining with a monoclonal antibody against LMP1. In situ hybridization of the null cell line HLN-STL-C established from an adult T-cell leukemia patient showed that 100% of the cells contained both EBERs and LMP1 mRNA and about 0.1% of the cells contained gp350/220 mRNA, indicating that a few of the null cells which carried the EBV genome spontaneously entered the late EBV replication cycle.
我们报告了一种通过用碱性磷酸酶连接的寡核苷酸探针进行原位DNA-RNA杂交来检测爱泼斯坦-巴尔病毒(EBV)的简单方法。产生EBV的细胞系P3HR-1和Akata分别用佛波酯和丁酸盐以及抗人IgG处理。这种处理导致具有潜伏膜蛋白1(LMP1)和包膜糖蛋白gp350/220的EBV转录本的细胞群体大量增加,但EBV编码的小核RNA(EBERs)的细胞群体未增加。如用寡核苷酸探针进行原位DNA-DNA杂交的双重或单一标记以及用抗LMP1单克隆抗体进行免疫过氧化物酶染色所示,由诱导的mRNA编码的LMP1蛋白的合成主要依赖于病毒DNA合成。从一名成人T细胞白血病患者建立的空细胞系HLN-STL-C的原位杂交显示,100%的细胞同时含有EBERs和LMP1 mRNA,约0.1%的细胞含有gp350/220 mRNA,这表明少数携带EBV基因组的空细胞自发进入了EBV晚期复制周期。
