高分化及低分化鼻咽癌细胞株中Epstein—Barr病毒潜伏感染膜蛋白（LMP…

应用染色原位杂交、ＰＣＲ扩增、克隆及核苷酸序列分析等方面,分析了ＣＮＥ１和ＮＥ３细胞株中的潜伏感染膜蛋白（ＬＭＰ１）基因。ＣＮＥ１是来自我国东北的高分化鼻咽癌细胞株。ＣＮＥ３是来自广西的低分化鼻咽癌细胞株。染色体原位杂交结果表明,ＣＮＥ１细胞中的ＬＭＰ１基因存在于细胞核内,整合在第一号染色体上,ＣＮＥ３中ＬＭＰ１２基因则随机存在于细胞核内及多条染色体上。用ＰＣＲ方法分别从ＣＮＥ１及ＣＮＥ３中扩增到     

EB病毒与促癌物协同作用诱发人鼻咽恶性淋巴瘤和未分化癌的研究

将ＥＢ病毒感染的人胎儿鼻咽粘膜移植于２２只Ｂａｌｂ／ｃ裸鼠皮下,每周一次皮下注射丁酸和佛波醇二酯（ＴＰＡ）,约１０天后肿物逐渐增大,１５周内行病理学检查,诊断为恶性淋巴瘤４例（其中Ｔ淋巴细胞型３例）,未分化癌３例,ＰＣＲ和原位杂交显示,两种肿瘤组织和细胞中均含有ＥＢ病毒ＬＭＰ１基因,核苷酸序列分析表明,与Ｂ９５－８细胞ＬＭＰ１基因相应序列的同源性约为９６％和９９％,说明ＥＢ病毒感染人胎儿新鲜鼻咽上     

鼻咽癌组织中Epstein—Barr病毒潜伏感染膜蛋白基因片段的克隆及分析

从两例鼻咽癌（ＮＰＣ）病人的活检组织切片中,用ＰＣＲ方法扩增出ＥＢ病毒潜伏感染膜蛋白（ＬＭＰ）基因的Ｅｘｏｎｌ、Ｉｎｔｒｏｌ ＥｘｏｎΠ和ＩｎｔｒｏｎΠ共５００ｂｐ的片段,克隆入载体ｐＧＥＭ－３ｚｆ（＋）′,测定核苷酸序列,其中有一个样品所测序列段与台湾析相似,另一个样品则与Ｂ９５－８极为相似。由此可知。中国陆南方的ＮＰＣ组织中ＥＢＶ－ＬＭＰ基因存在不同的变异。     

鼻咽癌组织中Epstein－Barr病毒潜伏感染膜蛋白基因片段的克隆及分析

从两例鼻咽癌（ＮＰＣ）病人的活检组织切片中,用ＰＣＲ方法扩增出ＥＢ病毒潜伏感染膜蛋白（ＬＭＰ）基因的ＥｘｏｎⅠ、ＩｎｔｒｏｎⅠ、ＥｘｏｎⅡ和ＩｎｔｒｏｎⅡ共５００ｂｐ的片段,克隆入载体ｐＧＥＭ－３ｚｆ（＋）′,测定核苷酸序列,其中有一个样品所测序列段与台湾株相似,另一个样品则与Ｅ９５－８极为相似。由此可知,中国大陆南方的ＮＰＣ组织中ＥＢＶ－ＬＭＰ基因存在不同的变异。     

猪瘟病毒糖蛋白E0基因的克隆及及表达研究

用ＲＴ－ＰＣＲ方法扩增分别获得了中国猪瘟病毒强毒石门株和兔化弱毒株糖蛋白Ｅ０基因ｃＤＮＡ,并克隆到ｐＧＥＭ Ｔ载体中测定其核苷酸序列和推导出其对应氨基酸序列,结果表明这两个毒 间的Ｅ０基因核苷酸序列同源性为９５．３％,氨基酸序列同源性为９４％,有１４个殖基的差异;与几个代表毒株ＡＬＤ株、ＧＰＥ株、Ｂｒｅｓｃｉａ株、Ａｌｆｏｒｔ株和国外测得的兔化弱毒Ｃ株相应序列进行比较,所测石门病毒核苷酸序列与上述     

猪瘟病毒糖蛋白E0基因的克隆及其表达研究*

用ＲＴ－ＰＣＲＡ法扩增分别获得了中国猪瘟病毒强毒石门株和免化弱毒株糖蛋白Ｅ０基因ｃＤＮＡ,并克隆到ｐＧＥＭ Ｔ载体中测定其核着酸序列和推导出其对应氨基酸序列;结果表明这两个毒株间的Ｅ０基因核着酸序列同源性为９５．３％,氨基酸序列同源性为９４％,有１４个残基的差异;与几个代表毒株ＡＬＤ株、ＧＰＥ株、Ｂｒｅｓｃｉａ株、Ａｌｆｏｒｔ株和国外测得的免化弱毒Ｃ株相应序列进行比较,所测石门病毒核苷酸序列与上述各株对应序列的同源性分别为９８．０％、９７．１％、９２．７％、８６．８％和９５．４％;氨基酸序列同源性分别为９     

EB病毒胸苷激酶基因的定向克隆

采用异硫氰酸胍（ＧｕＳＣＮ）和硅藻从Ｂ９５－８细胞中快速抽摸板ＤＮＡ。根据ＥＢ病毒（ＥＢＶ）Ｂ９５－８株ＤＮＡ全序列及编码ＥＢＶ胸苷激酶（ＴＫ）的开放读框ＢＸＬＦ１的结构,设计合成一对引物,并在引物的５′一端分别引入ＥｃｏＲＩ和ＰｓｔＩ切点,用ＰＣＲ技术扩增出一含完整的ＥＢＶＴＫ基因的１．８４３ＫｂＤＮＡ片段,ＮｃｏＩ酶切分析鉴定,ＥｃｏＲＩ／ＰｓｔＩ双酶切ＰＣＲ产物和载体,使目的基因定向克隆至选     

葡萄扇叶病毒外壳蛋白基因的克隆,序列分析及其在大肠杆菌中…

通过ＲＴ－ＰＣＲ方法把葡萄扇叶病毒（ＧＦＬＶ）外壳蛋白基因（ＣＰ ｇｅｎｅ）分成两部分扩增,扩增产物克隆入ｐｇＥＭ－５Ｚｆ（＋）载体,并通过ＢｇｌⅡ位点连接成一完整的外壳蛋白基因,通过序列分析测得全长外壳蛋白基因为１５１２ｂｐ,编码５０４个ＡＡ＇ｓ与国外株系ＧＦＬＶ－Ｆ１３相比,核苷酸同源性为８８．４％,氨基酸同源性为９５．８％。并且这一外壳蛋白基因在大肠杆菌Ｅ． ｃｏｌｉＤＨ－５α中得到了表达。     

番茄花叶病毒外壳蛋白基因及3′端非编码区的克隆、序列分析及其表达

根据已报道的番茄花叶病毒Ｌ株系（ＴｏＭＶＬ）序列人工合成引物,经ＲＴＰＣＲ扩增并克隆了我国番茄花叶病毒分离物（ＴｏＭＶＳ１）的外壳蛋白ＣＰ基因及３′端非编码区。序列测定结果表明,所得ｃＤＮＡ共长６８２个核苷酸,其中ＣＰ基因含４８０个核苷酸,编码１５８个氨基酸,３′端非编码区含２０２个核苷酸,其核苷酸序列与ＴｏＭＶＬ株系具有９９．５％的同源率。将该基因片段克隆到ｐＧＥＭＥＸ１载体中,转入Ｅ．ｃｏｌｉ后诱导表达,经Ｗｅｓｔｅｒｎｂｌｏｔ检测证明,该基因已在大肠杆菌中正确表达。这是我国首次报道ＴｏＭＶＣＰ基因序列。     

猪瘟病毒石门株与兔化弱毒株E0糖蛋白基因的克隆及序列分析

参考已发表的猪瘟病毒序列,设计并合成了一对引物,应用ＲＴＰＣＲ 技术,扩增了猪瘟兔化弱毒（Ｈｏｇ ｃｈｏｌｅｒａ ｖｉｒｕｓ ｌａｐｉｎｉｚｅｄ Ｃｈｉｎｅｓｅ ｓｔｒａｉｎ , ＨＣＬＶ） 和石门强毒株的Ｅ０ 糖蛋白基因,并将其克隆到ｐＧＥＭＴ 载体中,测定了其核苷酸序列,并推导了其氨基酸序列。结果表明我国这两株强弱不同毒株Ｅ０ 糖蛋白核苷酸序列同源性和推导的氨基酸序列同源性分别为９５－０ ％ 和９４－３ ％ ,有１３ 个氨基酸的差异,ＨＣＬＶ 比石门株多了一个潜在的Ｎ糖基化位点。将我国这两株病毒与国外已报导的ＨＣＶ 毒株Ｅ０ 基因序列进行了比较,发现石门株与日本的两株毒株ＡＬＤ 和ＧＰＥ－ 同源性较高,核苷酸序列同源性分别为９７－４ ％ 和９６－５ ％ ,氨基酸同源性分别为９７－４ ％ 和９６－０ ％ ,而与欧洲Ｂｒｅｓｃｉａ 株和Ａｌｆｏｒｔ 株同源性较低,核苷酸同源性分别为９２－２ ％ 和８６－５ ％ ,氨基酸同源性为９５－２ ％ 和９２－５ ％ , ＨＣＬＶ 与ＡＬＤ、ＧＰＥ－ 、Ｂｒｅｓｃｉａ、Ａｌｆｏｒｔ 株核苷酸同源性分别为９５－６ ％ 、９４－９ ％ 、９１－３ ％ 、８５－５ ％ …     

EB病毒LMP-1上调鼻咽癌细胞系AP-1的活性

为了探讨 EB病毒潜伏膜蛋白 1 ( LMP- 1 )通过信号传导途径介导的致瘤分子机制 ,由此首先构建了 AP- 1报告基因 ,用佛波酯诱导确定了其报道 AP- 1的功能 ;通过建立荧光素酶双报道系统 ,研究了 LMP- 1表达对 AP- 1和 NFκB活性的影响 .研究发现 :在 LMP- 1阴性鼻咽癌 ( NPC)细胞系 ,导入 LMP- 1表达质粒后 ,AP- 1和 NFκB的活性均升高 4～ 5倍 ;而在 LMP- 1阳性 NPC细胞系中 ,当导入 LMP- 1反义表达质粒 ,AP- 1和 NFκB的活性则受抑制 ,活性下调 3～ 4倍 .结果表明 ,LMP- 1能上调 NPC细胞系 AP- 1的活性 ,同时再次证实了 LMP- 1能活化 NFκB.     

Proteomics-based identification of proteins with altered expression induced by 12-O-tetradecanoylphorbol 13-acetate in nasopharyngeal carcinoma CNE2 cells

Nasopharyngeal carcinoma (NPC) is a malignancy with high incidence in Southern China and South-East Asia. Etiology studies indicate that chemical carcinogen promoters, such as 12-O-tetradecanoylphorbol-13-acetate (TPA), are important factors causing NPC development. However, the mechanism of the TPA effect on NPC remains unclear. In the present study, cells from a poorly differentiated squamous cell carcinoma NPC cell line, CNE2, were stimulated by TPA and proteomics technology was carried out to find protein discrepancies between control and TPA-treated cells. Results revealed that TPA treatment in CNE2 cells could upregulate the expression of ““““triosephosphate isomerase““““ and ““““14-3-3 protein sigma““““ and downregulate the expression of ““““reticulocalbin 1 precursor““““, ““““nucleophosmin““““, ““““mitochondrial matrix protein pl precursor““““, and ““““stathmin““““. The changes in the expression of these genes suggested that TPA induced CNE2 cells to antiproliferation and to apoptosis, which was confirmed by subsequent apoptosis detection. Therefore, the effects of TPA on nasopharyngeal carcinoma cells were distinct from the effects on primary epithelial cells and we suggest reasons for these differences.     

A positive autoregulatory loop of LMP1 expression and STAT activation in epithelial cells latently infected with Epstein-Barr virus

STAT3 and STAT5 are constitutively activated and nuclear in nasopharyngeal carcinoma (NPC) cells. In normal signaling, STATs are only transiently activated. To investigate whether Epstein-Barr virus (EBV), and in particular the protein LMP1, contributes to sustained STAT phosphorylation and activation in epithelial cells, we examined STAT activity in two sets of paired cell lines, HeLa, an EBV-converted HeLa cell line, HeLa-Bx1, the NPC-derived cell line CNE2-LNSX, and an LMP1-expressing derivative, CNE2-LMP1. EBV infection was associated with a significant increase in the tyrosine-phosphorylated forms of STAT3 and STAT5 in HeLa-Bx1 cells. This effect correlated with LMP1 expression, since phosphorylated STAT3 and STAT5 levels were also increased in CNE2-LMP1 cells relative to the control CNE2-LNSX cells. No change was observed in STAT1 or STAT6 phosphorylation in these cell lines, nor was there a significant change in the levels of total STAT3, STAT5, STAT1, or STAT6 protein. Tyrosine phosphorylation allows the normally cytoplasmic STAT proteins to enter the nucleus and bind to their recognition sequences in responsive promoters. The ability of LMP1 to activate STAT3 was further established by immunofluorescence assays in which coexpression of LMP1 in transfected cells was sufficient to mediate nuclear relocalization of Flag-STAT3 and by an electrophoretic mobility shift assay which showed that LMP1 expression in CNE2-LNSX cells was associated with increased endogenous STAT3 DNA binding activity. In addition, the activity of a downstream target of STAT3, c-Myc, was upregulated in HeLa-Bx1 and CNE2-LMP1 cells. A linkage was established between interleukin-6 (IL-6)- and LMP1-mediated STAT3 activation. Treatment with IL-6 increased phosphorylated STAT3 levels in CNE2-LNSX cells, and conversely, treatment of CNE2-LMP1 cells with IL-6 neutralizing antibody ablated STAT3 activation and c-Myc upregulation. The previous observation that STAT3 activated the LMP1 terminal repeat promoter in reporter assays was extended to show upregulated expression of endogenous LMP1 mRNA and protein in HeLa-Bx1 cells transfected with a constitutively activated STAT3. A model is proposed in which EBV infection of an epithelial cell containing activated STATs would permit LMP1 expression. This in turn would establish a positive feedback loop of IL-6-induced STAT activation, LMP1 and Qp-EBNA1 expression, and viral genome persistence.     

Regulation of survivin and CDK4 by Epstein-Barr virus encoded latent membrane protein 1 in nasopharyngeal carcinoma cell lines

Latent membrane protein 1 （LMP1）, an important protein encoded by Epstein Barr virus （EBV）, has been implied to link with the pathogenesis of nasopharyngeal carcinoma （NPC）. Its dual effects of increasing cell proliferation and inhibiting cell apoptosis have been confirmed. In this study, we showed that the expression of Survivin and CDK4 protein in CNE-LMP1, a LMP1 positive NPC epithelial cell line, is higher than in LMP1 negative NPC epithelial cell line- CNE1, and the expression is LMP1 dosage-dependent. Although it was reported that Survivin specifically expressed in cell cycle G2/M phase, our studies suggested that LMP1 could promote the expression of Survivin in G0/G1, S and G2/ M phase. It also showed that Survivin and CDK4 could be accumulated more in the nuclei triggered by LMP1. More interestingly, Survivin and CDK4 could form a protein complex in the nuclei of CNE-LMP1 rather than in that of CNE1, which demonstrated that the interaction between these two proteins could be promoted by LMPI. These results strongly suggested that the role of LMP1 in the regulation of Survivin and CDK4 may also shed some light on the mechanism research of LMP1 in NPC.     

Tx基因与Igk基因的同源性研究及其在不同细胞株的表达

本文对以前报道的Ｔｘ基因２．８ｋｂ片段的核苷酸序列与人免疫球蛋白ｋａｐｐａ链Ｃ区基因的核苷酸序列及其编码产物的氨基酸序列进行了同源性比较。结果表明,Ｔｘ基因与ｋａｐｐａ链Ｃ区基因的同源性高达９９．５％以上,编码区的同源性高达１００％。从而提示Ｔｘ基因与ｋａｐｐａ链Ｃ区基因可能是同一种基因。限制性内切酶图谱及Ｓｏｕｔｈｅｒｎ印迹杂交分析,也进一步支持这一观点。本文还报道了ｋａｐｐａ链Ｃ区基因在不同细     

Identification of differential proteins in nasopharyngeal carcinoma cells with p53 silence by proteome analysis

Although mutation of p53 tumor-suppressor gene is rare in nasopharyngeal carcinoma (NPC), NPC has a high frequency of overexpression of p53 protein. There seem to be complex mechanisms of inactivation and stabilization of p53 in NPC. To detect proteins associated with the function of p53 in high throughout screening, we succeeded in establishing p53 knockdown human NPC CNE2 cell line (CNE2sip53) using stable RNA interference, and compared the proteomic changes between CNE2sip53 and control cell line CNE2/pSUPER using two-dimensional gel electrophoresis. Twenty-two differentially expressed proteins between the two cell lines were identified by both matrix-assisted laser desorption/ionization time-of-flight mass spectrometry and electrospray ionization tandem mass spectrometry, some of which are known to be associated with the p53 function (HSP27, hnRNP K, 14-3-3sigma, etc.), and others may be novel proteins associated with p53 function (eIF4B, TPT1, hnRNP H3, SFRS1 etc.). Furthermore, several differential proteins including HSP27, HSP70, GRP75 and GRP78 were verified as p53 interacting proteins in NPC by immunoprecipitation and Western blot analysis, and the suppression of HSP27 expression by HSP27 antisense oligonucleotides could decrease the p53 protein level. Our data suggest that these differential proteins may be associated with the function of p53 in NPC, and provide new clues to elucidate the mechanisms of inactivation and stabilization of p53 in NPC.     

Lentivirus-mediated RNAi knockdown of LMP2A inhibits the growth of nasopharyngeal carcinoma cell line C666-1 in vitro

Latent membrane protein 2A (LMP2A) is found to play a key role in the development of nasopharyngeal carcinoma (NPC). However, the role of LMP2A silencing in the inhibition of cell growth of NPC has not been clarified. In this study, we inhibited LMP2A gene expression by lentivirus-mediated RNAi, to explore the effects of LMP2A silencing on the growth of NPC cell line in vitro. A lentivirus-mediated RNAi technology was employed to specifically knock down the LMP2A gene in NPC cell line C666-1. Quantitative real-time polymerase chain reaction, Western blot, flow cytometry and colony formation assays were performed to evaluate the expression of LMP2A and biological behavior of cell line C666-1 in vitro. We successfully construct a highly efficient and stable lentivirus vector, which efficiently downregulate the expression of LMP2A gene in infected cell line C666-1. Down-regulation of the expression of LMP2A significantly inhibits the proliferation and colony formation of C666-1 cells. In addition, the specific down-regulation of LMP2A arrests cells in G0/G1 phase of cell cycle and increases apoptosis rate. Our findings suggest that lentivirus-mediated RNAi knockdown of LMP2A inhibits the growth of NPC cell line C666-1 in vitro, and LMP2A may be a potential target for gene therapy in treatment of NPC.     

Variable expression of latent membrane protein in nasopharyngeal carcinoma can be related to methylation status of the Epstein-Barr virus BNLF-1 5''-flanking region.

Seven virus-coded proteins, the nuclear proteins EBNA-1 to EBNA-6 and the latent membrane protein (LMP), are regularly expressed in Epstein-Barr virus (EBV)-transformed lymphoblastoid cell lines. In nasopharyngeal carcinoma (NPC), only EBNA-1 is regularly expressed; LMP is detected in about 65% of the tumors. In Burkitt's lymphoma tumors only EBNA-1 is expressed. We have recently shown that the methylation patterns of the EBV genome varied between these cell types. In virally transformed lymphoblastoid cell lines of normal origin, the EBV DNA is completely unmethylated. In contrast, in the Burkitt's lymphoma-derived cell line Rael and in a nude mouse-passaged NPC tumor, C15, there was an extensive methylation of CpG pairs. The methylation extended into the coding regions of the two expressed genes, EBNA-1 (in both tumor types) and LMP (in C15). Two presumptive control regions were exempted from this overall methylation: the oriP that contains both an origin of DNA replication and an EBNA-1-dependent enhancer and the 5'-flanking region of the BNLF-1 open reading frame that codes for LMP. The latter was only exempted in the LMP expressing NPC. We have now investigated the relation between expression of LMP and methylation of DNA in the 5'-flanking 1 kb region of BNLF-1, coding for LMP. LMP was methylated in 3 of 12 NPC biopsies that did not express LMP but was partially or totally unmethylated in the remaining 9 that expressed the protein. The three BNLF-1 exons were highly methylated in all the tumors. The oriP region was unmethylated in all the tumors, as in the previously studied Rael cell line and nude mouse-passaged NPC. Also, the BamHI W enhancer region involved in the expression of EBNA nuclear proteins was methylated. None of the biopsies expressed EBNA-2. Our data show that the EBV genomes are highly methylated in NPC tumors. The strong reverse correlation between the methylation of the putative control region of the LMP gene and the expression of LMP suggests that methylation has a role in the regulation of this gene.