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建立并鉴定了两种潜伏感染爱泼斯坦-巴尔病毒且源自鼻咽癌的上皮肿瘤细胞系(HNE-1和HONE-1)。

Establishment and characterization of two epithelial tumor cell lines (HNE-1 and HONE-1) latently infected with Epstein-Barr virus and derived from nasopharyngeal carcinomas.

作者信息

Yao K T, Zhang H Y, Zhu H C, Wang F X, Li G Y, Wen D S, Li Y P, Tsai C H, Glaser R

机构信息

Cancer Research Laboratory, Human Medical University, Changsha, People's Republic of China.

出版信息

Int J Cancer. 1990 Jan 15;45(1):83-9. doi: 10.1002/ijc.2910450116.

Abstract

Two epithelial tumor cell lines were established from biopsy specimens of 2 nasopharyngeal carcinomas (NPC) and designated HNE-1 and HONE-1. Uncloned HNE-1 cells were found to be Epstein-Barr virus (EBV) DNA-positive when examined by Southern blot analysis up to passage 35, after which the EBV genome could no longer be detected. A similar loss of EBV DNA took place in uncloned HONE-1 cells. However, HONE-1 clone 40 cells are still EBV DNA-positive up to passage 42 thus far and cell cultures contain 85-90% EBV nuclear antigen (EBNA)-positive cells. The HNE-1 cell line has been passaged more than 100 times and the uncloned HONE-1 cells more than 90 times. The tumorigenicity of the HNE-1 and HONE-1 cells was demonstrated by tumor induction in nude mice. Karyotypic analysis of the HNE-1 cells demonstrated an aneuploidy with a modal chromosomal number of 74 at passages 5 and 101 at passage 20; 18 marker chromosomes were identified. We have continued to map the EBV genome latently associated with the HNE-1 and HONE-1 cells using the Bam HI, EcoRI or Hind III restriction enzymes. Using EcoRI fragments A-K as probes, we found that HNE-1 EBV DNA is different from B95-8 and HR-1 EBV DNA in the EcoRI-C region. The Bam HI map for HONE-1 EBV DNA is very similar to the B95-8 map; it contains the Bam HI-Y fragment but without Bam HI B' and WI'. Differences were observed between HONE-1 EBV DNA and B95-8 DNA using the Hind III restriction enzyme. There was no evidence of spontaneous expression of the latent EBV genome in HNE-1 cells, and attempts to induce replication of the latent EBV genome and rescue infectious virus have failed, suggesting a tightly restricted virus genome.

摘要

从2例鼻咽癌活检标本中建立了两种上皮肿瘤细胞系,分别命名为HNE - 1和HONE - 1。通过Southern印迹分析检测,未克隆的HNE - 1细胞在传代至35代时发现Epstein - Barr病毒(EBV)DNA呈阳性,此后再也检测不到EBV基因组。未克隆的HONE - 1细胞也发生了类似的EBV DNA丢失。然而,HONE - 1克隆40细胞至今传代至42代时仍为EBV DNA阳性,细胞培养物中含有85 - 90%的EBV核抗原(EBNA)阳性细胞。HNE - 1细胞系已传代100多次,未克隆的HONE - 1细胞传代90多次。HNE - 1和HONE - 1细胞的致瘤性通过在裸鼠中诱导肿瘤得以证明。对HNE - 1细胞的核型分析显示,在第5代时为非整倍体,众数染色体数为74,在第20代传至101代时;鉴定出18条标记染色体。我们继续使用Bam HI、EcoRI或Hind III限制性内切酶对与HNE - 1和HONE - 1细胞潜在相关的EBV基因组进行定位。使用EcoRI片段A - K作为探针,我们发现HNE - 1 EBV DNA在EcoRI - C区域与B95 - 8和HR - 1 EBV DNA不同。HONE - 1 EBV DNA的Bam HI图谱与B95 - 8图谱非常相似;它包含Bam HI - Y片段,但没有Bam HI B'和WI'。使用Hind III限制性内切酶观察到HONE - 1 EBV DNA和B95 - 8 DNA之间存在差异。没有证据表明HNE - 1细胞中潜伏的EBV基因组有自发表达,并且诱导潜伏EBV基因组复制和拯救感染性病毒的尝试均失败,这表明病毒基因组受到严格限制。

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