SARS冠状病毒NS融合蛋白的重组表达纯化与免疫学性质分析(英文)

刺突蛋白(S)和核心蛋白(N)是SARS冠状病毒的主要结构蛋白.在病毒细胞受体结合和病毒包装过程起重要作用.重组融合表达这2种蛋白具有较高的诊断学价值.对SARS病毒N蛋白和S蛋白氨基酸序列进行计算机分析,选择含有优势抗原表位的N蛋白1～227位氨基酸片段和S蛋白450～650位氨基酸片段,采用序列重叠延伸策略(sequenceoverlappingextension,SOE)构建编码N1227LinkerS450650新型融合蛋白的基因片段,导入原核表达载体,实现融合蛋白在大肠杆菌的高效表达.利用组氨酸标签亲和层析的方法纯化,获得高纯度的融合蛋白.对该融合蛋白的结构特征模拟分析的结果显示,其免疫化学性质均无显著改变.采用ELISA和Western印迹方法对其识别SARS冠状病毒特异性抗体的能力进行初步鉴定,显示该融合蛋白具有较好的抗原性和特异性,可有效特异性地检测恢复期SARS病人血清中抗SARS冠状病毒结构蛋白的抗体,可以作为SARS冠状病毒感染的辅助诊断手段.     

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。     

重组杆状病毒表达尼帕病毒融合蛋白和受体结合蛋白的研究

构建了表达尼帕病毒(Nipah virus,NiV)囊膜功能糖蛋白F和G的重组杆状病毒rBac-NF、rBac-NG。Western-blot证实大小分别为61kD和66kD的重组融合蛋白(rNF)和受体结合蛋白(rNG)分别在rBac-NF、rBac-NG感染的昆虫细胞中获得表达,并且rNF前体F0可在昆虫细胞内进一步有效裂解为F1(~49kD)和F2;采用兔抗NiV病毒高免血清间接免疫荧光检测重组杆状病毒表达F和G蛋白显示出良好的特异免疫反应原性。以rBac-NF、rBac-NG感染的昆虫细胞裂解液稀释后直接包被ELISA板,间接ELISA检测兔抗灭活NiV全病毒高免血清中的F和G蛋白特异性抗体,同样具有良好的敏感性和特异性;以rBac-NF和rBac-NG感染昆虫细胞培养物直接免疫BALB/c小鼠,可诱导显著的NiVF和G蛋白特异体液免疫反应,产生的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,杆状病毒表达重组F和G蛋白抗原具有替代NiV全病毒,作为安全、经济、敏感和特异的诊断抗原的潜力,并为重组病毒亚单位疫苗防制尼帕病毒性脑炎的探索研究奠定了基础。     

表达猪瘟病毒石门株E0基因重组鸡痘病毒的构建及动物免疫试验

应用PCR从质粒pMD18-T-E0中扩增编码CSFV E0蛋白的基因片段,定向克隆到重组鸡痘病毒表达载体FPV-P11上,进一步构建出重组鸡痘病毒转移载体FPV-pSY-E0.用脂质体将该质粒转染至鸡痘病毒感染的鸡胚成纤维细胞(CEF)后,通过蓝斑纯化实验筛选出重组鸡痘病毒FV282-CSFV-E0.PCR证实E0基因已整合至鸡痘病毒基因组中,Western blot检测到重组病毒感染CEF细胞中E0蛋白的表达.重组病毒3次腹腔接种小鼠,ELISA检测血清抗体滴度高达1∶4 096.重组病毒免疫猪3次之后,接种猪瘟病毒强毒进行攻毒试验,结果对免疫组产生75%的保护率,为研制猪瘟活载体疫苗奠定了基础.     

在昆虫细胞中表达能自聚成病毒样颗粒的兔出血症病毒衣壳蛋白

将兔出血症病毒衣壳蛋白VP60基因插入杆状病毒转移载体pBLUEBAC 4,获得重组转移载体pBLUEBAC4-VP60.在脂质体转染试剂介导下,将重组杆状病毒转移载体pBLUEBAC4-VP60 与线性化的野生型杆状病毒基因组DNA共转染对数生长期的Sf9昆虫细胞,经过三轮蚀斑纯化后,获得了克隆化的重组杆状病毒pBLUEBAC4-VP60.以重组杆状病毒感染Sf9细胞后,收获细胞培养上清和细胞裂解液上清,SDS-PAGE电泳分析显示,重组病毒pBLUEBAC4-VP60表达一分子量各为60kD左右的特异性重组蛋白,并且该重组蛋白经Western blot检测,皆可被兔抗RHDV高免血清所识别,表明VP60蛋白基因在重组杆状病毒感染的Sf9昆虫细胞中得到了表达,并且具有与天然VP60相似的抗原性.血凝试验表明,表达的重组蛋白具有血凝特性,可以凝集人"O"型红细胞,血凝价为213.同时,该血凝性可被抗RHDV的高免血清所抑制.经电镜观察,重组病毒表达的衣壳蛋白可以在没有其他任何成分存在的条件下,在昆虫细胞内也能自然聚合成不包裹核酸的、与天然RHDV病毒粒子在物理形态上类似的病毒样颗粒(VLPs).在与兔抗RHDV高免血清37℃作用1h后,该病毒样颗粒于电镜下观察可出现凝集成团的现象,表明该VLPs与天然RHDV在抗原性上也极为相似.     

共表达HIV-1中国流行株gp120与IL-18重组鸡痘病毒的构建及其免疫原性观察

为筛选我国的HIV-1疫苗候选株,以鸡痘病毒282E4中国疫苗株为载体,构建了共表达中国流行株HIV-1外膜蛋白gp120和IL-18的重组鸡痘病毒,并将该重组鸡痘病毒免疫BALB/c小鼠,检测免疫小鼠脾特异性CTL杀伤活性和血清抗体水平。结果显示,HIV_1外膜蛋白gp120和IL-18不但可在重组鸡痘病毒感染的鸡胚成纤维细胞中表达,而且可在重组鸡痘病毒感染的哺乳动物细胞中表达。重组病毒具有良好的免疫原性,可诱导小鼠产生特异性抗体和脾特异性CTL反应,且IL_18发挥了免疫佐剂的作用。本研究结果为制备安全、有效的HIV-1基因工程活载体疫苗奠定了基础。     

N端融合外源蛋白的兔出血症病毒衣壳蛋白自聚能力的研究

将兔出血症病毒衣壳蛋白VP6 0基因插入杆状病毒转移载体pBLUEBACHIS2_B的 6 HIS表达标签下游 ,与线性化野生型杆状病毒基因组DNA共转染Sf9昆虫细胞 ,经蚀斑纯化后获克隆化重组杆状病毒pBLUEBACHIS2B_VP6 0。以重组杆状病毒感染Sf9细胞 ,经SDS_PAGE和Westernblot检测显示高效表达一分子量为 6 9kD的重组蛋白 ,并且该蛋白可被兔抗RHDV高免血清识别。血凝试验表明 ,该重组蛋白可以凝集人“O”型红细胞 ,血凝价达 2 1 6 ,同时 ,该血凝性可被抗RHDV的高免血清所抑制。经电镜观察 ,重组病毒表达的融合有 6 HIS表达标签的衣壳蛋白仍可在昆虫细胞内自聚成不包裹核酸的、与天然RHDV病毒粒子在物理形态上相似的病毒样颗粒 (VLPs) ,并且该VLPs与兔抗RHDV高免血清作用后于电镜下可见凝集成团的现象 ,表明其与天然RHDV病毒粒子在抗原性上也极为相似     

尼帕病毒融合蛋白、受体结合蛋白的表达及特异性高免血清制备

尼帕病毒膜融合蛋白F和受体结合蛋白G在病毒感染和诱导机体产生保护性免疫中起重要的作用。通过PCR扩增获得尼帕病毒F1和G基因片段(均去掉信号肽和跨膜区),克隆至原核表达载体,IPTG诱导大肠杆菌表达目的蛋白,Western blot表明重组F1、G蛋白与兔抗尼帕病毒血清具有良好的反应原性;同时将F1和G基因克隆至经改造过的杆状病毒表达载体,获得了含有目的基因的重组杆状病毒,接种sf9单层细胞,间接免疫荧光检测表明F1、G蛋白在杆状病毒中正确表达,并与抗尼帕病毒血清具有良好的反应原性。以纯化原核表达的F1、G蛋白免疫兔获得了抗F1和抗G重组蛋白的特异血清,Western blot和间接免疫荧光检测表明所制备的血清具有特异性。试验所表达的抗原和制备的特异血清可用于尼帕病的诊断。     

SARS-CoV核衣壳蛋白的表达与免疫研究

依据GenBank中SARS基因组序列,采用人工合成的方法合成编码SARS病毒N蛋白的全基因(1296bp)序列,再与设计的CTL特异性表位基因(195bp)重组后,克隆到pET-28a(+)质粒中,重组质粒转化到大肠杆菌BL21(DE3)中诱导表达.利用SARS患者恢复期阳性血清,鉴定表达蛋白.进一步纯化后免疫马,并用ELISA方法检测血清抗体效价.结果显示SDS-PAGE表明所表达的蛋白相对分子质量约为55000 Da,与预计大小相符;Westernblot显示表达的蛋白具有良好的抗原性和特异性.对表达蛋白形成的包涵体进行洗涤,得到的蛋白纯度可达到70.1%.切胶纯化免疫马后,获得的抗SARS抗体滴度达12560.为亚单位疫苗研制和精制抗SARS抗体免疫制剂提供基础.     

一种展示SARS冠状病毒受体结合区的重组枯草杆菌芽孢的制备及免疫原性分析

目的：利用枯草杆菌芽孢呈递技术制备表达SARS冠状病毒S蛋白受体结合区（RBD）的重组芽孢。方法：将枯草杆菌 CotB 基因构建到基因组整合质粒pDG1664中,再将 RBD 基因连接到 CotB 基因的下游,构建成重组质粒pDG1664-CotB-RBD,通过同源重组整合到PY-79枯草杆菌基因组中;利用红霉素抗性筛选重组菌并进行PCR和DNA测序鉴定,Western印迹鉴定重组菌芽孢表面RBD蛋白的表达情况;用表达RBD的重组芽孢以口服方式免疫小鼠,通过ELISA和流式细胞术检测重组芽孢的免疫原性。结果：制备出枯草杆菌基因组整合了RBD抗原基因的重组菌株RS1931,形成的重组芽孢表达相对分子质量约62×103的CotB-RBD融合蛋白;重组芽孢免疫的小鼠血清RBD抗原特异性IgG抗体滴度在末次免疫后2周可达1∶10880,重组芽孢初免后18周的小鼠脾细胞中IFN-γ＋CD4^＋、IL-4＋CD4^＋和IFN-γ＋CD8^＋T细胞比例上调,表明重组芽孢经口服免疫产生良好的体液免疫和细胞免疫应答。结论：针对SARS冠状病毒S蛋白RBD建立了枯草杆菌芽孢呈递技术方法,制备出在枯草杆菌芽孢表面稳定表达外源RBD蛋白的重组株,获得的重组芽孢具有良好的免疫原性,为开发芽孢呈递型SARS疫苗奠定了基础。     

Antigenicity and receptor-binding ability of recombinant SARS coronavirus spike protein

Severe acute respiratory syndrome (SARS) is an emerging infectious disease associated with a novel coronavirus and causing worldwide outbreaks. SARS coronavirus (SARS-CoV) is an enveloped RNA virus, which contains several structural proteins. Among these proteins, spike (S) protein is responsible for binding to specific cellular receptors and is a major antigenic determinant, which induces neutralizing antibody. In order to analyze the antigenicity and receptor-binding ability of SARS-CoV S protein, we expressed the S protein in Escherichia coli using a pET expression vector. After the isopropyl-beta-D-thiogalactoside induction, S protein was expressed in the soluble form and purified by nickel-affinity chromatography to homogeneity. The amount of S protein recovered was 0.2-0.3mg/100ml bacterial culture. The S protein was recognized by sera from SARS patients by ELISA and Western blot, which indicated that recombinant S protein retained its antigenicity. By biotinylated ELISA and Western blot using biotin-labeled S protein as the probe, we identified 130-kDa and 140-kDa proteins in Vero cells that might be the cellular receptors responsible for SARS-CoV infection. Taken together, these results suggested that recombinant S protein exhibited the antigenicity and receptor-binding ability, and it could be a good candidate for further developing SARS vaccine and anti-SARS therapy.     

Expression cloning of functional receptor used by SARS coronavirus

We have expressed a series of truncated spike (S) glycoproteins of SARS-CoV and found that the N-terminus 14-502 residuals were sufficient to bind to SARS-CoV susceptible Vero E6 cells. With this soluble S protein fragment as an affinity ligand, we screened HeLa cells transduced with retroviral cDNA library from Vero E6 cells and obtained a HeLa cell clone which could bind with the S protein. This cell clone was susceptible to HIV/SARS pseudovirus infection and the presence of a functional receptor for S protein in this cell clone was confirmed by the cell-cell fusion assay. Further studies showed the susceptibility of this cell was due to the expression of endogenous angiotensin-converting enzyme 2 (ACE2) which was activated by inserted LTR from retroviral vector used for expression cloning. When human ACE2 cDNA was transduced into NIH3T3 cells, the ACE2 expressing NIH3T3 cells could be infected with HIV/SARS pseudovirus. These data clearly demonstrated that ACE2 was the functional receptor for SARS-CoV.     

SARS冠状病毒S受体结合区蛋白片段在杆状病毒载体中的表达及其抗原性研究

目的:利用Bac-to-Bac1杆状病毒系统,在sf9昆虫细胞中表达严重急性呼吸综合征(SARS)冠状病毒(SARS-CoV)的S受体结合区蛋白片段,并对其免疫原性进行研究。方法:将S蛋白的受体结合区基因片段定向克隆至转座载体pFast-Bac1,转化大肠杆菌DH10Bac感受态细胞,用抗生素平板筛选重组杆粒。脂质体介导重组杆粒转染sf9昆虫细胞,待细胞形态明显改变后收获细胞和培养上清液。利用SARS病人恢复期抗血清做ELISA和Western印迹,分析重组蛋白的抗原性。结果:ELISA和Western印迹表明,在sf9昆虫细胞中表达的SARS-CoVS受体结合区重组蛋白可与SARS病人恢复期抗血清发生特异反应。结论:获得了在昆虫细胞内表达的SARS-CoVS受体结合区重组蛋白,并证明该蛋白有可能用于SARS感染的抗体检测,为SARS-CoV免疫机制及其疫苗的进一步研究奠定了基础。     

Functional analysis of the receptor binding domain of SARS coronavirus S1 region and its monoclonal antibody

Severe acute respiratory syndrome (SARS) is caused by the SARS coronavirus (CoV). The spike protein of SARS-CoV consists of S1 and S2 domains, which are responsible for virus binding and fusion, respectively. The receptor-binding domain (RBD) positioned in S1 can specifically bind to angiotensin-converting enzyme 2 (ACE2) on target cells, and ACE2 regulates the balance between vasoconstrictors and vasodilators within the heart and kidneys. Here, a recombinant fusion protein containing 193-amino acid RBD (residues 318–510) and glutathione S-transferase were prepared for binding to target cells. Additionally, monoclonal RBD antibodies were prepared to confirm RBD binding to target cells through ACE2. We first confirmed that ACE2 was expressed in various mouse cells such as heart, lungs, spleen, liver, intestine, and kidneys using a commercial ACE2 polyclonal antibody. We also confirmed that the mouse fibroblast (NIH3T3) and human embryonic kidney cell lines (HEK293) expressed ACE2. We finally demonstrated that recombinant RBD bound to ACE2 on these cells using a cellular enzyme-linked immunosorbent assay and immunoassay. These results can be applied for future research to treat ACE2-related diseases and SARS.     

SARS-CoV核衣壳蛋白的表达与免疫研究

依据GenBank中SARS基因组序列,采用人工合成的方法合成编码SARS病毒N蛋白的全基因(1296bp)序 列,再与设计的CTL特异性表位基因(195bp)重组后,克隆到pET-28a( )质粒中,重组质粒转化到大肠杆菌BL21 (DE3)中诱导表达。利用SARS患者恢复期阳性血清,鉴定表达蛋白。进一步纯化后免疫马,并用ELISA方法检 测血清抗体效价。结果显示SDS-PAGE表明所表达的蛋白相对分子质量约为55000 Da,与预计大小相符;Western blot显示表达的蛋白具有良好的抗原性和特异性。对表达蛋白形成的包涵体进行洗涤,得到的蛋白纯度可达到 70．1％。切胶纯化免疫马后,获得的抗SARS抗体滴度达1:2560。为亚单位疫苗研制和精制抗SARS抗体免疫制 剂提供基础。     

An exposed domain in the severe acute respiratory syndrome coronavirus spike protein induces neutralizing antibodies

Exposed epitopes of the spike protein may be recognized by neutralizing antibodies against severe acute respiratory syndrome (SARS) coronavirus (CoV). A protein fragment (S-II) containing predicted epitopes of the spike protein was expressed in Escherichia coli. The properly refolded protein fragment specifically bound to the surface of Vero cells. Monoclonal antibodies raised against this fragment recognized the native spike protein of SARS CoV in both monomeric and trimeric forms. These monoclonal antibodies were capable of blocking S-II attachment to Vero cells and exhibited in vitro antiviral activity. These neutralizing antibodies mapped to epitopes in two peptides, each comprising 20 amino acids. Thus, this region of the spike protein might be a target for generation of therapeutic neutralizing antibodies against SARS CoV and for vaccine development to elicit protective humoral immunity.     

Assembly of human severe acute respiratory syndrome coronavirus-like particles

Viral particles of human severe acute respiratory syndrome coronavirus (SARS CoV) consist of three virion structural proteins, including spike protein, membrane protein, and envelope protein. In this report, virus-like particles were assembled in insect cells by the co-infection with recombinant baculoviruses, which separately express one of these three virion proteins. We found that the membrane and envelope proteins are sufficient for the efficient formation of virus-like particles and could be visualized by electron microscopy. Sucrose gradient purification followed by Western blot analysis and immunogold labeling showed that the spike protein could be incorporated into the virus like particle also. The construction of engineered virus-like particles bearing resemblance to the authentic one is an important step towards the development of an effective vaccine against infection of SARS CoV.     

Mass spectrometric characterization of proteins from the SARS virus: a preliminary report

A new coronavirus has been implicated as the causative agent of severe acute respiratory syndrome (SARS). We have used convalescent sera from several SARS patients to detect proteins in the culture supernatants from cells exposed to lavage another SARS patient. The most prominent protein in the supernatant was identified by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF MS) as a approximately 46-kDa species. This was found to be a novel nucleocapsid protein that matched almost exactly one predicted by an open reading frame in the recently published nucleotide sequence of the same virus isolate (>96% coverage). A second viral protein corresponding to the predicted approximately 139-kDa spike glycoprotein has also been examined by MALDI-TOF MS (42% coverage). After peptide N-glycosidase F digestion, 12 glycosylation sites in this protein were confirmed. The sugars attached to four of the sites were also identified. These results suggest that the nucleocapsid protein is a major immunogen that may be useful for early diagnostics, and that the spike glycoprotein may present a particularly attractive target for prophylactic intervention in combating SARS.     

严重急性呼吸道综合征冠状病毒疫苗研究现状

冠状病毒被认为是新近爆发的严重急性呼吸道综合征的病原体.迄今公共数据库中已发表了不同国家和地区分离的12个SARS病毒株基因组完整序列.突起蛋白是冠状病毒的主要抗原,包含许多抗原决定簇.SARS冠状病毒突起蛋白的相对保守性为有效疫苗的开发奠定了很好的研究基础.灭活或减毒的冠状病毒疫苗存在一定的局限性和危险性.开展基因工程疫苗和核酸疫苗的制备研究以及相关候选疫苗的联合应用研究将是一个切实可行的途径.     

Identification and antigenic epitope mapping of immunodominant region amino residues 510 to 672 on the spike protein of the severe acute respiratory syndrome coronavirus

The severe acute respiratory syndrome (SARS) is a newly emerging human infectious disease caused by the severe acute respiratory syndrome coronavirus (SARS-CoV). The spike (S) protein of SARS-CoV is a major virion structural protein. It plays an important role in the interaction with receptors and neutralizing antibodies. In this study, the S1 domain of the spike protein and three truncated fragments were expressed by fusion with GST in a pGEX-6p-1 vector. Western blot results demonstrated that the 510-672 fragment of the S1 domain is a linear epitope dominant region. To map the antigenic epitope of this linear epitope dominant region, a set of 16 partially overlapping fragments spanning the fragment were fused with GST and expressed. Four antigenic epitopes S1C3 (539-559), S1C4 (548-567), S1C7/8 (583-606), and S1C10/11 (607-630) were identified. Immunization of mice with each of the four antigenic epitope-fused proteins revealed that all four proteins could elicit spike protein specific antisera. All of them were able to bind to the surface domain of the whole spike protein expressed by recombinant baculovirus in insect cells. Identification of antigenic epitopes of the spike protein of SARS-CoV may provide the basis for the development of immunity-based prophylactic, therapeutic, and diagnostic clinical techniques for the severe acute respiratory syndrome.