腺病毒E1B 55kD癌蛋白与hDaxx的相互作用

为了探讨腺病毒(adenovirus,Ad)E1B 55kD癌蛋白(Ad E1B 55kD)打破hDaxx和PML共定 位细胞核的作用机制,本文利用体内外共免疫沉淀反应研究Ad E1B 55kD与hDaxx的结合反应 ,并通过酵母双杂交体系测定两种蛋白质的相互作用及其作用的氨基酸残基序列.结果显示 Ad2 E1B 55kD通过C端58个氨基酸(aa)与hDaxx结合并发生相互作用.Ad12 E1B 5 5kD与hDaxx结合需全序列aa及其构象.共免疫沉淀反应和Western blot结果证实Ad2/5或Ad1 2 E1B 55kD能在体内外与hDaxx直接结合.     

腺病毒E1B55ku癌蛋白打破hDaxx与PML在细胞核的共定位

利用间接免疫荧光试验,通过Confocal激光扫描生物荧光显微镜和图像软件分析腺病毒(adenovirus,Ad)E1B 55 ku癌蛋白(Ad E1B 55 ku)与人Daxx(human Daxx,hDaxx)在细胞核的定位关系,研究它对早幼粒细胞性白血病蛋白(promyelocytic leukemia protein,PML)与hDaxx在细胞核定位关系的影响.实验结果表明,Ad E1B 55 ku与hDaxx共定位细胞核,并打破hDaxx与PML共定位于细胞核PML致癌结构域(PML oncogenic domams,PODs).     

hDaxx与细胞肿瘤抑制子p53在体内外的相互作用

与急性早幼粒细胞性白血病蛋白(promyelocytic leukemia protein,PML)在体内相互作用共定位于细胞核PML致癌结构城(PML oncogenic domains,PODs)的人Daxx(human Daxx,hDaxx),能结合Fas死亡结构域诱导细胞凋亡.细胞肿瘤抑制子p53抑制细胞及病毒转录,提高细胞内Fas的表达并调节细胞凋亡.为了探索hDaxx与p53在诱导细胞凋亡中有无相互作用及其作用效果,利用酵母双杂交体系测定发现p53通过C端与hDaxx结合,共免疫沉淀反应及Western blot结果显示hDaxx与p53能在体内外直接结合.hDaxx与p53结合并发生相互作用可能对细胞周期有一定的调节作用.     

PES1与雌激素受体存在相互作用

雌激素(E2)和雌激素受体(ER)在E2诱发的肿瘤中起着极其重要的作用.ER共调节因子通过与ER相互作用调节其生物学功能.PES1主要表达于E2的重要靶器官如乳腺、卵巢等组织中,并在乳腺癌细胞中高表达.用PCR技术构建HA标签的PES1全长以及1～322aa、312 ～588aa和414～588aa三个不同功能区片段的重组质粒.将不同的重组质粒与FLAG-ERα和或FLAGC-ERβ共转染293T细胞后进行免疫共沉淀,以验证PES1与ER是否有相互作用以及相互作用的区域.用含雌激素受体作用元件的荧光素酶报告基因( ERE-LUC)检测PES1对ERα和ERβ转录激活活性的影响.结果表明,PES1与ERα和ERβ均相互作用,且PES1的1～ 322aa区域与ERα和ERβ相结合.PES1能特异地、E2非依赖性抑制ERβ的转录激活活性.实验结果显示,PES1是一个新的ER共调节因子,需要进一步研究其在ERβ信号通路及其在E2诱发的肿瘤的作用.     

雌激素通过LRP16基因5′侧翼GC富含区上调其转录的分子机制

LRP16是一个明确的雌激素(E2)反应性靶基因,已往研究在LRP16基因上游调控区鉴定了一个E2反应性1/2ERE/GC富含的ERα作用位点(-676bp到-214bp;命名为A区).为进一步鉴定雌激素上调LRP16基因表达的最大化反应区域,对LRP16基因上游调控区进行缺失突变,通过相对荧光素酶活性分析观察到LRP16基因的一段5′近端侧翼序列(-213bp到-24bp;命名为B区)具有明显的E2反应性.通过与A区比较,认为B区最大化的呈递了E2对LRP16基因的转激活效应.序列分析表明,B区缺乏经典的ERE元件,而包含多个富含GC序列.针对Sp1的siRNA实验结果提示,Sp1参与了E2对该区域的转激活.针对GC富含区进一步的缺失突变,及荧光素酶活性分析,识别了一段30bp(-213bp到-184bp)的序列在B区呈递E2反应活性中发挥核心作用.超级凝胶电泳实验结果表明,Sp1蛋白与这段30bp的DNA序列在体外存在直接结合作用.染色质免疫共沉淀实验结果证实,ERα、Sp1与B区存在E2依赖性相互作用.本文在LRP16的5′-侧翼区识别了一段最大化呈递E2活性的DNA片段.机制研究表明,在E2存在条件下,ERα通过Sp1与该区域的直接作用上调LRP16基因的表达.     

我国新分离森林脑炎病毒E基因特征分析

为了解分离自黑龙江省大兴安岭林区全沟硬蜱中的DXAL-5、12、13、16、18,21共6株森林脑炎(TBE)病毒E蛋白基因特征并确定病毒基因型,应用RT-PCR技术对6株病毒E蛋白基因进行体外扩增、克隆、测序.结果发现,6株病毒E蛋白基因的核苷酸序列长均为1 488 bp,推导的氨基酸序列长均为496 aa.与TBE参考毒株E蛋白基因进行比较,这6株病毒与远东亚型同源性最高,其次是西伯利亚亚型,与欧洲亚型同源性最差;在决定亚型特征的氨基酸位点多数属于TBE病毒远东亚型.E蛋白基因推导的氨基酸种系发生树分析表明,6株病毒均在远东亚型分枝内.因此就E蛋白基因而言,DXAL-5、12、13、16、18、21株均属于TBE病毒的远东亚型.新分离毒株与Senzhang株同源性较高,种系发生关系也比较接近,推测疫苗株对新分离毒株仍具有很好的保护作用.但是在E蛋白的A、B和C抗原决定区内,6株病毒均有不同程度的氨基酸改变,这些突变有可能影响E蛋白的功能.     

HIV-1膜蛋白在甲醇型酵母中的表达和抗原性的研究

通过计算机辅助分析了中国广西B/C重组亚型HIV-1病毒株的Env蛋白(共851氨基酸残基)氨基酸的疏水性、潜在的抗原表位,与其它亚型的Env蛋白在氨基酸组成的保守性方面进行了比较,选择了env基因的469-511aa,538-674aa和700-734aa三段保守性及抗原性都较强的氨基酸序列构建成嵌合基因,将嵌合基因构建到毕赤酵母Pichia pastoris表达载体pPICZαB中,利用甲醇诱导表达,对表达的蛋白进行了Wester blot和SDS-PAGE分析,结果表明,三段基因能在毕赤酵母Pichia pastoris中表达,产物为40kD的特异性诱导糖蛋白,通过Ni-sepharose 4B金属Ni螯合层析柱分离纯化表达蛋白,酶联免疫检测结果表明,纯化的抗原有很强的抗原特异性,可以用于HIV检测试剂的研制和开发。     

四份中国HCV阳性血清中包膜蛋白E1/E2准种基因的序列分析及新型插入突变的发现

为分析四份中国丙型肝炎病毒（HCV）阳性血清中包膜蛋白E1/E2基因的准种特征。本研究对从4份中国HCV阳性血清（1b亚型：274、366、383;2a亚型：283）中提取的HCV核酸,采用逆转录-聚合酶反应扩增编码全长E1/E2蛋白（191～764aa）的基因片段,随机挑取多个克隆测序。根据E1/E2基因核苷酸的序列与其他相关序列（来自于GenBank）构建亲缘性关系进化树,进行核苷酸与氨基酸同源性分析并对重要的基因位点进行分析。共获得阳性克隆序列43个（274株10个,283株12个,366株13个,383株8个）,发现高变区HVR1、HVR2的基因异质性高,而其他抗体中和表位及跨膜区I、II及N末端糖基化位点相对保守。并首次发现在HCV 2a亚型（283血清）中多个准种序列存在1279nt（E1区,313aa）处单碱基插入优势基因突变,导致HCV包膜蛋白编码突变与中断（E2区,398aa）。本研究对中国HCV代表株包膜蛋白E1/E2编码基因的准种多样性及一种新型插入突变进行了描述,可为进一步研究HCV免疫逃避与慢性化机制提供重要信息。关键词：丙型肝炎病毒;包膜蛋白;序列分析;准种;插入突变     

SARS病毒受体ACE2的克隆、原核表达及其功能区鉴定

ACE2(angiotensin-converting enzyme 2,ACE2)是SARS冠状病毒(severe acute respiratory syndrome associatedcoronavirus,SARS-CoV)的主要受体。此研究旨在鉴定ACE2的SARS-CoV受体功能区,为进一步阐明SARS-CoV与细胞间的相互作用机制及研制抗病毒药物等提供理论依据。利用RT-PCR从Vero-E6细胞的mRNA中分两段扩增ACE2基因,其中N端片段ACE2A1-367(102~1 210nt)不包括ACE2的酶活性位点(1 223~1 237nt,或374~378aa),而C端片段ACE2B335-805(1 101~2 524nt)包括ACE2的酶活性位点。扩增片段克隆入pMD-18T,并进行测序鉴定。进一步构建与GST基因融合表达的原核表达质粒pGEX-ACE2A与pGEX-ACE2B,IPTG诱导表达。表达的融合蛋白分子量为65kD和77kD,主要以包涵体形式存在。Western blot证实表达产物具有免疫学活性。将纯化的包涵体蛋白质复性后进行Western blot分析,证实pGEX-ACE2A表达的蛋白(~65kD)能与SARS-CoV S1蛋白特异结合,而pGEX-ACE2B表达的蛋白(~77kD)不能与S1蛋白结合。结果表明,ACE2的受体活性与酶活性位点无关,受体功能区在ACE2 N端367个氨基酸内。     

雌激素通过LRP16基因5′侧翼GC富含区上调其转录的分子机制

LRP16是一个明确的雌激素(E2)反应性靶基因,已往研究在LRP16基因上游调控区鉴定了一个E2反应性1/2ERE/GC富含的ERα作用位点（-676 bp到-214 bp;命名为A区）.为进一步鉴定雌激素上调LRP16基因表达的最大化反应区域,对LRP16基因上游调控区进行缺失突变,通过相对荧光素酶活性分析观察到LRP16基因的一段5′近端侧翼序列（-213 bp到-24 bp;命名为B区）具有明显的E2反应性.通过与A区比较,认为B区最大化的呈递了E2对LRP16基因的转激活效应.序列分析表明,B区缺乏经典的ERE元件,而包含多个富含GC序列.针对Sp1的siRNA实验结果提示,Sp1参与了E2对该区域的转激活.针对GC富含区进一步的缺失突变,及荧光素酶活性分析,识别了一段30 bp（-213 bp到-184 bp）的序列在B区呈递E2反应活性中发挥核心作用.超级凝胶电泳实验结果表明,Sp1蛋白与这段30 bp的DNA序列在体外存在直接结合作用.染色质免疫共沉淀实验结果证实,ERα、Sp1与B区存在E2依赖性相互作用.本文在LRP16的5′侧翼区识别了一段最大化呈递E2活性的DNA片段.机制研究表明,在E2存在条件下,ERα通过Sp1与该区域的直接作用上调LRP16基因的表达.     

The p21(WAF1) cyclin-kinase inhibitor: in vivo interaction with E1A adenoviral Ad2 and Ad12 oncoproteins

The capability of adenoviral oncoproteins E1A Ad2 and Ad12 to form complexes in vivo with cyclin-kinase inhibitor p21Waf1 has been analysed. The published data confirming direct interaction between E1A and p21Waf1 are insufficient. In the present work, a yeast two-hybrid SRS system was used to investigate the binding of different fragments of E1A Ad2 and Ad12 polypeptides with p21Waf1. We have shown that the full length product of 12S mRNA E1A Ad2 interacts weekly with p21Waf1, whereas the protein corresponding to 13S mRNA E1A Ad12 does not bind to cyclin-kinase inhibitor protein. Moreover, fragments 1-80 (Ad2), 1-29 (Ad12), 1-79 (Ad12), and 105-194 (Ad12) were able to interact with p21Waf1 to some extent. The difference between interacting regions of adenoviral proteins E1A Ad2/5 and Ad12 gives a new information about the mechanism of p21Waf1 functional inactivation and different transforming activity of Ad2/5 and Ad12.     

Large E1B proteins of adenovirus types 5 and 12 have different effects on p53 and distinct roles in cell transformation.

The formation of complexes between oncoproteins of DNA tumor viruses and the cellular protein p53 is thought to result in inactivation of the growth suppressor function of p53. In cells transformed by nononcogenic human adenovirus type 5 (Ad5), the 55-kDa protein encoded by E1B forms a stable complex with p53 and sequesters it in the cytoplasm. However, the homologous 54-kDa protein of highly oncogenic Ad12 does not detectably associate with p53. Yet in Ad12-transformed cells, p53 is metabolically stable, is present at high levels in the nucleus, and contributes to the oncogenicity of the cells. Such properties have previously been described for mutant forms of p53. Here, we show that stable p53 in Ad12-transformed cells is wild type rather than mutant and that stabilization of p53 is a direct consequence of the expression of the Ad12 E1B protein. We also compared the effects of the E1B proteins on transformation of rodent cells by different combinations of oncogenes. A synergistic interaction was observed for the gene encoding the 54-kDa E1B protein of Ad12 with myc plus ras oncogenes, resembling the effect of mutant p53 on myc plus ras. In contrast, the Ad5 55-kDa E1B protein strongly inhibited transformation by myc plus ras but stimulated transformation by E1A plus ras. The data are explained in terms of different interactions of the two E1B proteins with endogenous p53. The results suggest that in cultured rat cells, endogenous wild-type p53 plays an essential role in cell proliferation, even in the presence of myc plus ras. The dependence on p53 is lost, however, when the adenovirus E1A oncogene is present.     

转染E1B55K基因提高Hep2细胞包装肠腺病毒Ad41的能力

人F组腺病毒Ad40、Ad41难以在体外培养的细胞中传代,被称为难养腺病毒(Fastidious adenovirus).本研究观察了在Hep2细胞表达Ad41 E1B55K基因对Ad41复制的促进作用.从Ad41阳性粪便标本中用PCR的方法获得E1B55K基因,构建真核表达载体,转染Hep2细胞,筛选单克隆,用RT-PCR检测了E1B55K基因的表达.用引起293细胞完全CPE比较产毒量的方法对所得细胞克隆进行初步筛选,获得一株产毒相对较强的细胞Hep2-E1B#4.与对照细胞Hep2、Hep2-DNA3相比,等量Ad41接种Hep2-E1B#4产生的细胞病变效应(CPE)程度明显加深.用免疫细胞化学的方法测定产毒的感染滴度,等量Ad41接种后,Hep2-E1B#4产生的子代腺病毒滴度大于对照的9倍;半定量PCR测得Hep2-E1B#4子代病毒基因组拷贝数约为对照细胞的4倍.结果说明转染E1B55K基因促进了Ad41在Hep2细胞的复制,获得的Hep2-E1B#4细胞株可用于Ad41的分离、培养和体外扩增.     

Downregulation of MHC class I expression due to interference with p105-NF kappa B1 processing by Ad12E1A.

We have previously demonstrated that expression of major histocompatibility complex (MHC) class I genes is repressed in baby rat kidney cells transformed by early region 1 of oncogenic adenovirus type 12 (Ad12E1). Reduced expression of MHC class I antigens contributes to the escape of Ad12-transformed cells from T-cell-mediated immune surveillance and to tumour induction. In this study, we show that repression of MHC class I expression by Ad12E1A is mediated via the H2TF1 element of the MHC class I promoter. This element binds NF kappa B and KBF1, two factors which play a major role in the regulation of MHC class I expression in vivo. In extracts from Ad12E1-transformed cells, binding of KBF1 and NF kappa B to the H2TF1 element is decreased. This is caused by reduced production of p50-NF kappa B1, the 50 kDa subunit shared by KBF1 and NF kappa B, due to interference with p105-NF kappa B1 processing by Ad12-13S-E1A protein. Overexpression of the p105-NF kappa B1 cDNA, or of a truncated p105-NF kappa B1 cDNA that codes for p50-NF kappa B1, restores MHC class I expression in Ad12E1-transformed cells. These data demonstrate that downregulation of MHC class I expression in Ad12E1-transformed cells is due to interference with processing of p105-NF kappa B1 by the Ad12-13S-E1A protein.     

腺病毒4型E3区核苷酸序列测定及其基因结构与功能分析

本文将Ａｄ４基因组相当于７３．３－８９．２基因图谱单位的ＤＮＡ片段进行了序列测定及基因结构分析,它包括了Ａｄ４Ｅ３区全基因及该区两侧的部分序列。序列分析表明,Ａｄ４ Ｅ３区从ＴＡＴＡＡ ｂｏｘ起至该区基因结束共４７７８ｂｐ,编码１１个大于６ｋＤ的开放读码框架。对Ａｄ４ Ｅ３区ＯＲＦ分析结果表明,Ａｄ４ Ｅ３区编码的１９．３ｋ,１５ｋ,１０．４ｋ蛋白,分别与Ａｄ２ Ｅ３区的ｇｐ１９ｋ,１４．ｋ和１０     

The Replicative Capacities of Large E1B-Null Group A and Group C Adenoviruses Are Independent of Host Cell p53 Status

Recent reports suggest that an early region 1B (E1B) 55,000-molecular-weight polypeptide (55K)-null adenovirus type 5 (Ad5) mutant (dl1520) can replicate to the same extent as wild-type (wt) Ad5 in cells either deficient or mutated in p53, implicating p53 in limiting viral replication in vivo. In contrast, we show here that the replicative capacity of Ad5 dl1520 is wholly independent of host cell p53 status, as is the replicative capacity of comparable Ad12 E1B 54K-null adenoviruses (Ad12 dl620 and Ad12 hr703). Furthermore, we show that there is no requirement for complex formation between p53 and Ad5 E1B 55K or Ad12 E1B 54K for a productive infection, such that wt Ad5 and wt Ad12 will both replicate in cells which are null for p53. In addition, we find that these Ad5 and Ad12 mutant viruses induce S phase irrespective of the p53 status of the cell and that, therefore, S-phase induction does not correlate with the replicative capacity of the virus. Interestingly, the replicative capacities of the large E1B-null adenoviruses correlated positively with the ability to express E1B 19K and were related to the ability to repress premature adenovirus-induced apoptosis. Infection of primary human cells indicated that Ad5 dl1520, wt Ad5, and wt Ad12 replicated better in cycling normal human skin fibroblasts (HSFs) than in quiescent HSFs. Thus, the cell cycle status of the host cell, upon infection, also influences viral yield.     

Nuclear export of the E1B 55-kDa and E4 34-kDa adenoviral oncoproteins mediated by a rev-like signal sequence.

The E1B 55-kDa and E4 34-kDa oncoproteins of adenovirus type 5 (abbreviated here as E1B-55kD and E4-34kD) promote the export of viral mRNA and inhibit the export of most cellular mRNA species. We show that the intracellular complex containing E1B-55kD and E4-34kD continuously shuttles between the nucleus and the cytoplasm, and may thus serve as a nucleocytoplasmic transporter for viral mRNA. We present evidence that within this complex, it is the E4-34kD protein that directs both nuclear import and nuclear export. E4-34kD contains a functional nuclear export signal similar to corresponding sequences found in the retroviral proteins rev and rex. This sequence element is required for nuclear export of the complex, and it can function autonomously when fused to a carrier protein and microinjected in HeLa cell nuclei. When E4-34kD is expressed alone, a portion of the protein that contains a predicted arginine-rich amphipathic alpha-helical structure mediates nuclear retention of the protein. This retention, however, can be abolished by the association with E1B-55kD or by a specific point mutation within the arginine-rich motif. The export of E4-34kD can be blocked by an HTLV-rex derived competitive inhibitor and overexpressed E4-34kD inhibits rev-mediated transport, suggesting that the export pathways accessed by the adenoviral and retroviral proteins share components. The interplay between two polypeptides as well as the involvement of a dominant nuclear retention domain are novel features that might contribute to the efficiency and regulation of the adenovirus export system.