流行性感冒病毒重组的研究——Ⅰ.高产株和表面抗原重组株的选育

本文报告了甲型流感病毒重组高产株、血凝素单价抗原重组株及神经氨酸酶单价抗原重组株的选育和鉴定方法。实验证明利用灭活病毒和活病毒两株亲本株混合感染,在鸡胚系统中重组,经过抗血清中和选择,再经终末纯化,可以简便、快速而又准确地获得重组株。     

中国口蹄疫病毒同源重组研究

从GenBank数据库中获得在我国分离的16株口蹄疫病毒全基因组序列,进而运用常规的系统发生方法分析了这16株病毒的同源重组情况,发现5株重组毒株．这些重组病毒主要来源于亚洲Ⅰ型(Asia1)和O型病毒间的重组．这些重组事件的鉴定也表明口蹄疫病毒间的交叉感染在我国比较常见．另外,在我国还出现了由于Asia1型和O型病毒重组后导致病毒血清型发生转化的现象．这些结果解释了我国口蹄疫病毒(FMDV)遗传多样性和抗原多变性的成因,提示了我国在口蹄疫预防、治疗方面所面临的复杂局面．     

表达HIV-I CN54株gagpol基因重组痘苗病毒疫苗株的构建

为研制不带筛选标记的HIV活载体疫苗,首先构建含有neo基因和lacZ基因双重筛选标记的pV175转移质粒,并将HIV—I中国主要流行株B’／C重组株CN54 gagpol基因置于pV175的启动子pE／L下,构建重组质粒pVl75—Gagpol。重组质粒与痘苗病毒天坛株共转染鸡胚细胞。前三轮通过G418加压,噬斑纯化,得到既含目的基因又含筛选标记的蓝色重组痘苗病毒;后三轮在无G418选择压力下,筛选只含目的基因而缺失了筛选标记的白色重组痘苗病毒。结果表明筛选到了一株重组病毒,经PCR和Dot blot检测确认该株重组痘苗病毒的neo基因和lacZ基因已丢失;PCR鉴定表明目的基因已插入重组痘苗病毒中;抗体染色和Westem blot结果证实该重组病毒能很好地表达目的蛋白。     

小鼠对重组痘苗病毒表达流感病毒血凝素的免疫反应

实验比较了小鼠对表达流感病毒A/NJ/11/76(H1N1)和A/Jap/305/57(H2N2)血凝素基因的痘苗病毒重组株HSW2和VInf1的免疫反应,两株重组病毒经静脉或静脉加鼻腔免疫小鼠后都产生相应血凝抑制抗体;用不同剂量的痘苗病毒重组株HSW2皮内接种家兔也产生相应抗体,且抗体滴度与接种的病毒量成正比关系,但用痘苗病毒野毒株免疫的家兔未测到抗体,这两株痘苗病毒重组株免疫的小鼠,能保护小鼠对流感病毒母株的攻击,HSW2和VInf1的保护指数分别为3.3和3.9个对数,但这两株病毒未能诱导细胞毒性T细胞反应。     

猪口蹄疫病毒与猪肠道病毒在细胞培养中的基因重组——病毒重组及一个重组株的初步鉴定

利用两株不同理化和生物学特性的不同属小RNA病毒,即口蹄疫病毒(FMDV)与猪肠道病毒(EV),建立了病毒基因重组,克隆筛选和鉴定的方法,初步证实,在实验室条件下它们可以进行基因重组,本文为研究自然界病毒变异机理,不同属病毒的基因重组提供了依据。     

表达HIV-I CN54株gagpol基因重组痘苗病毒疫苗株的构建

为研制不带筛选标记的HIV活载体疫苗,首先构建含有neo基因和lacZ基因双重筛选标记的pVI75转移质粒,并将HIV-I中国主要流行株B'/C重组株CN54 gagpol基因置于pVI75的启动子pE/L下,构建重组质粒pVI75-Gagpol.重组质粒与痘苗病毒天坛株共转染鸡胚细胞.前三轮通过G418加压,噬斑纯化,得到既含目的基因又含筛选标记的蓝色重组痘苗病毒;后三轮在无G418选择压力下,筛选只含目的基因而缺失了筛选标记的白色重组痘苗病毒.结果表明筛选到了一株重组病毒,经PCR和Dot blot检测确认该株重组痘苗病毒的neo基因和lacZ基因已丢失;PCR鉴定表明目的基因已插入重组痘苗病毒中;抗体染色和Western blot结果证实该重组病毒能很好地表达目的蛋白.     

重组痘苗病毒表达人免疫缺陷病毒中国株B'亚型Gag蛋白及免疫效果观察

为筛选用于我国HIV疫苗的候选基因,利用痘苗病毒载体构建表达HIV-1 B′亚型中国流行株RL42的Gag蛋白的重组病毒rVV-RL42gag,并免疫BALB/c小鼠,检测其诱导的特异性抗体及中和抗体,同时检测其诱导的特异性CTL及与中国流行株C(B′/C重组)亚型和国际流行株A亚型之间的CTL交叉反应.结果显示:重组病毒能很好地表达Gag蛋白,它具有与7株单克隆抗体结合的抗体表位;电镜下可观察到Gag蛋白形成的颗粒.rVV-RL42gag免疫小鼠后能诱导产生高滴度的特异性抗体和CTL,抗体具一定的中和活性,且检测到与C(B′/C重组)亚型和国际流行株A亚型之间的CTL交叉反应.这些结果表明,rVV-RL42gag具有良好的免疫原性,可进一步构建表达HIV B′亚型中国流行株RL42的Gag蛋白的重组痘苗病毒作为候选疫苗.     

表达HIV多价抗原的重组痘苗病毒的构建及免疫效果研究

为了构建适用于中国的HIV候选疫苗,利用痘苗病毒天坛株表达中国HIV-1主要流行毒株CN54的gagpol△和gpl40TM基因。实验结果显示,重组痘苗病毒能正确表达Gag和gpl40TM蛋白。获得的重组痘苗病毒与DNA疫苗、重组腺病毒联合免疫Balb／c小鼠,并检测不同免疫程序在小鼠中诱导的细胞和体液免疫。免疫实验表明,DNA疫苗初始免疫,重组腺病毒与重组痘苗病毒依次加强所诱导的CTL应答、T淋巴细胞增殖以及中和抗体均高于其他免疫方案。DNA疫苗与两种活载体疫苗的联合运用,在小动物模型中取得了较好的免疫效果,这将为艾滋病疫苗的研究增加新的免疫策略。     

一株新的狂犬病重组痘苗病毒某些生物学性质的研究

对表达狂犬病毒糖蛋白的重组痘苗病毒ＶＶＭ１１ＫＲＧ株生物学性质进行了研究,该重组病毒的特点是：（１）糖蛋白基因插入到痘苗病毒天坛株基因组ＨｉｎｄⅢＭ片段中;（２）启动子为痘苗病毒天坛株Ｐ１１晚期启动子;（３）不含外源ｌａｃ基因。该重组病毒在ＣＶ－１细胞和鸡胚细胞上繁殖滴渡略高于另一株重组痘苗病毒ＶＶＴＫ１１ＫＲＧ,在鸡胚细胞中繁殖滴度第三天达到最高,在ＣＶ－１细胞中第二天达到最高。温度稳定性与天坛株相比没有明显改变。重组病毒在家兔皮内的毒力比亲本株（天坛株）低。间接免疫荧光和Ｗｅｓｔｅｒｎｂｌｏｔ都证明了狂犬病毒糖蛋白有良好的表达。通过Ｓｏｕｔｈｅｒｎｂｌｏｔ证实糖蛋白基因准确地插入到ＨｉｎｄⅢＭ片段中。重组痘苗病毒启动子与部分糖蛋白基因克隆到ｐＧＥＭ３ｚｆ（－）质粒上,对该段ＤＮＡ序列分析表明不会产生移码和融合蛋白,从而为该重组病毒的使用提供了明确的基因背景资料。     

表达尼帕病毒G囊膜糖蛋白重组牛痘病毒的研究

采用牛痘病毒WR株,构建了表达哺乳动物密码子优化的NiV G蛋白基因的重组病毒rWR-NiV-G。Westernblot证实大小为66kDa的重组G蛋白在rWR-NiV-G感染的Hela细胞中获得表达;采用兔抗NiV高免血清间接免疫荧光检测重组痘病毒表达G蛋白显示出良好的特异免疫反应原性。rWR-NiV-G感染NiV敏感的BHK细胞系,并与NiV融合蛋白F共同表达,可形成强烈细胞融合现象。rWR-NiV-G感染免疫BALB/c小鼠,可诱导显著的NiV G蛋白特异体液免疫反应。以原核表达NiV G蛋白片段为包被抗原,间接ELISA检测rWR-NiV-G感染免疫小鼠血清中的G蛋白特异抗体,具有良好的敏感性和特异性。同时,rWR-NiV-G感染免疫小鼠血清中的G蛋白特异抗体可有效中和NiV囊膜蛋白F和G介导的伪型VSV重组病毒侵入NiV易感宿主细胞的感染性。结果表明,重组牛痘病毒表达的NiV G蛋白有良好的免疫原性和生物学活性功能,为进一步深入研究NiV G蛋白生物学功能、免疫原性及重组活载体疫苗研究奠定了重要基础。     

应用聚合酶链反应检测口蹄疫病毒的实验研究

聚合酶链反应用于直接检测口蹄疫病毒(FMDV),可快速、灵敏地检出乳鼠组织或细胞繁殖的病毒的核酸。其灵敏度可达0.062pg,整个检测过程可缩短至4～5个小时内完成,比其它检测方法都敏感和快速。本文还探讨了直接用PCR扩增合成生物素化核酸探针检测口蹄疫病毒核酸的存在。     

Antigenic structure of the foot-and-mouth disease virus. II. Synthesis of protective peptides from the major immunogenic region of VP1 protein of foot-and-mouth disease virus type A22

Earlier we found that the immune response and antiviral protection from FMDV can be achieved by immunization with uncoupled FMDV peptides. In a search of approaches to animal protection from FMDV A22 strain we prepared a series of peptides corresponding to the putative antigenic determinants. Synthetic 131-149 and 140-149 sequences afforded 50 to 80% protection, both in the free state and conjugated with keyhole limpet hemocyanin. We believe that the 140-149 segment is so far the smallest peptide capable of eliciting specific antiviral protection without conjugation with a high molecular carrier.     

口蹄疫病毒O/NY00株基因组L片段的克隆及其基因特征

采用RT—PCR方法对口蹄疫病毒O／NY00株基因组L片段进行了分子克隆和序列测定。结果表明：获得的O／NY00株基因组L片段长7805nt,其中包括715nt的5’非编码区和6999nt的多聚蛋白编码区。将O／NY00株与其它参考毒株进行序列比较,结果显示：O／NY00株与O／SKR／2000、O／1JKG／3／2001遗传关系最近,而与其它毒株遗传关系较远,属于0型口蹄疫ME-SA拓扑型Pan／ksia株的成员。与Cathay拓扑型的代表毒株O／TAW／97比较,两者在主要抗原位点1和位点3呈现出明显的以拓扑型为特征的氨基酸差别,提示两拓扑型毒株之间有较高的抗原差异。     

Immunity to avirulent enterovirus 71 and coxsackie A16 virus protects against enterovirus 71 infection in mice

In this study, we sought to determine whether intratypic and intertypic cross-reactivity protected against enterovirus 71 (EV71) infection in a murine infection model. We demonstrate that active immunization of 1-day-old mice with avirulent EV71 strain or coxsackie A16 virus (CA16) by the oral route developed anti-EV71 antibodies with neutralizing activity (1:16 and 1:2, respectively). Splenocytes from both EV71- and CA16-immunized mice proliferated upon EV71 or CA16, but not coxsackie B3 virus (CB3), antigen stimulation. Immunized mice became more resistant to virulent EV71 strain challenge than nonimmunized mice. There was an increase in the percentage of activated splenic T cells and B cells in the immunized mice 2 days after EV71 challenge. The CA16 immune serum reacted with EV71 antigens in an enzyme-linked immunosorbent assay and neutralized EV71 but not CB3 or poliovirus at a titer of 1:4. Passive immunization with the CA16 immune serum reduced the clinical score, diminished the organ viral load, and increased the survival rate of mice upon EV71 challenge. CB3 neither shared in vitro cross-reactivity with EV71 nor provided in vivo protection after both active and passive immunization. These results illustrated that live vaccine is feasible for EV71 and that intertypic cross-reactivity of enteroviruses may provide a way to determine the prevalence of EV71.     

Extensive cell heterogeneity during persistent infection with foot-and-mouth disease virus.

Coevolution of viruses and the host cells occurred in BHK-21 cell cultures persistently infected with foot-and-mouth disease virus (FMDV) (J. C. de la Torre, E. Martínez-Salas, J. Diez, A. Villaverde, F. Gebauer, E. Rocha, M. Dávila, and E. Domingo, J. Virol. 62:2050-2058, 1988). In the present report we provide evidence of an extreme phenotypic heterogeneity of the cells, which was generated in the course of persistence. A total of 248 stable cell clones isolated from FMDV carrier cultures at early or late passages were analyzed. At least six distinct cell phenotypes were distinguished with regard to cell morphology, resistance to FMDV strain C-S8c1, and cell growth characteristics. No infectious FMDV or viral RNA was detected in variant cell clones, suggesting that the altered phenotypes were caused by inheritable cell modifications, selected in the course of persistence. Thus, the FMDV-BHK-21 carrier cell system must be described as a dynamic interaction between an evolving heterogeneous population of virus and multiple cell variants. We suggest that cell heterogeneity confers a selective advantage for long-term virus and cell survival by providing the cell population with a range of responses toward FMDV.     

Cooperative effect of the attenuation determinants derived from poliovirus sabin 1 strain is essential for attenuation of enterovirus 71 in the NOD/SCID mouse infection model

Enterovirus 71 (EV71) is a causative agent of hand, foot, and mouth disease and is also associated with serious neurological disorders. An attenuated EV71 strain [EV71(S1-3′)] has been established in the cynomolgus monkey infection model; this strain contains the attenuation determinants derived from the type 1 poliovirus vaccine strain, Sabin 1 [PV1(Sabin)], in the 5′ nontranslated region (NTR), 3D polymerase, and 3′ NTR. In this study, we analyzed the effect of the attenuation determinants of PV1(Sabin) on EV71 infection in a NOD/SCID mouse infection model. We isolated a mouse-adapted EV71 strain [EV71(NOD/SCID)] that causes paralysis of the hind limbs in 3- to 4-week-old NOD/SCID mice by adaptation of the virulent EV71(Nagoya) strain in the brains of NOD/SCID mice. A single mutation at nucleotide 2876 that caused an amino acid change in capsid protein VP1 (change of the glycine at position 145 to glutamic acid) was essential for the mouse-adapted phenotype in NOD/SCID mice. Next, we introduced attenuation determinants derived from PV1(Sabin) along with the mouse adaptation mutation into the EV71(Nagoya) genome. In 4-week-old mice, the determinants in the 3D polymerase and 3′ NTR, which are the major temperature-sensitive determinants, had a strong effect on attenuation. In contrast, the effect of individual determinants was weak in 3-week-old NOD/SCID mice, and all the determinants were required for substantial attenuation. These results suggest that a cooperative effect of the attenuation determinants of PV1(Sabin) is essential for attenuated neurovirulence of EV71.     

Asia Ⅰ型口蹄疫病毒中和表位与羊IgG重链恒定区的融合表达及免疫原性测定

VP1蛋白是口蹄疫病毒(Foot-and-Mouth Disease Virus,FMDV)诱导机体产生抗病毒感染免疫的主要蛋白,含有病毒的若干中和表位.本研究设计和合成了由Asia Ⅰ型FMDV VP1蛋白136～160aa和198～211aa两个表位组成的重复串联表位的编码基因,并克隆了羊IgG重链恒定区编码基因.利用BamH I、EcoR I和Xho I位点将2个基因片段依次克隆到pPROExHTb载体,构建成重组质粒pPRO-FshIgG,将其转化大肠杆菌BL21(DE3)感受态细胞,以IPTG诱导表达得到融合蛋白FshIgG.100μg FshIgG蛋白免疫豚鼠后刺激豚鼠产生了高效价的FMDV中和抗体,而且使这些免疫豚鼠在用200 ID_(50)剂量FMDV攻击时得到了完全保护.由此证明,羊IgG重链恒定区蛋白能够作为FMDV表位肽的载体,而融合蛋白FshIgG可成为一种口蹄疫表位疫苗候选物用于口蹄疫的预防.     

Structures of EV71 RNA-dependent RNA polymerase in complex with substrate and analogue provide a drug target against the hand-foot-and-mouth disease pandemic in China

Enterovirus 71 (EV71), one of the major causative agents for hand-foot-and-mouth disease (HFMD), has caused more than 100 deaths among Chinese children since March 2008. The EV71 genome encodes an RNA-dependent RNA polymerase (RdRp), denoted 3D^pol, which is central for viral genome replication and is a key target for the discovery of specific antiviral therapeutics. Here we report the crystal structures of EV71 RdRp (3D^pol) and in complex with substrate guanosine-5'-triphosphate and analog 5-bromouridine-5'-triphosphate best to 2.4 ? resolution. The structure of EV71 RdRp (3D^pol) has a wider open thumb domain compared with the most closely related crystal structure of poliovirus RdRp. And the EV71 RdRp (3D^pol) complex with GTP or Br-UTP bounded shows two distinct movements of the polymerase by substrate or analogue binding. The model of the complex with the template:primer derived by superimposition with foot-and-mouth disease virus (FMDV) 3D/RNA complex reveals the likely recognition and binding of template:primer RNA by the polymerase. These results together provide a molecular basis for EV71 RNA replication and reveal a potential target for anti-EV71 drug discovery.