Immunogenicity of plant‐produced porcine circovirus‐like particles in mice

Porcine circovirus type 2 (PCV‐2) is the main causative agent associated with a group of diseases collectively known as porcine circovirus‐associated disease (PCAD). There is a significant economic strain on the global swine industry due to PCAD and the production of commercial PCV‐2 vaccines is expensive. Plant expression systems are increasingly regarded as a viable technology to produce recombinant proteins for use as pharmaceutical agents and vaccines. However, successful production and purification of PCV‐2 capsid protein (CP) from plants is an essential first step towards the goal of a plant‐produced PCV‐2 vaccine candidate. In this study, the PCV‐2 CP was transiently expressed in Nicotiana benthamiana plants via agroinfiltration and PCV‐2 CP was successfully purified using sucrose gradient ultracentrifugation. The CP self‐assembled into virus‐like particles (VLPs) resembling native virions and up to 6.5 mg of VLPs could be purified from 1 kg of leaf wet weight. Mice immunized with the plant‐produced PCV‐2 VLPs elicited specific antibody responses to PCV‐2 CP. This is the first report describing the expression of PCV‐2 CP in plants, the confirmation of its assembly into VLPs and the demonstration of their use to elicit a strong immune response in a mammalian model.     

应用高效体积排阻色谱偶联多角度激光散射鉴定猪圆环病毒2型灭活疫苗及病毒样颗粒疫苗抗原

本文旨在建立基于高效体积排阻色谱(high-performance size-exclusion chromatography,HPSEC)偶联多角度激光散射仪(multi-angle laser light scattering,MALLS)的猪圆环病毒2型(porcine circovirus type 2,PCV2)疫苗抗原检测方法。以纯化的PCV2灭活病毒及病毒样颗粒(virus-like particles,VLP)为参照,对4家生产企业的2种PCV2灭活病毒疫苗(a、b)及VLP疫苗(c、d)破乳后进行HPSEC-MALLS检测及分子量分析;结合PCV2抗原检测卡、Western blotting和透射电子显微镜(transmission electron microscope,TEM),鉴定了特征色谱峰;考察了方法的重复性和检测线性。结果表明,两家企业生产的PCV2灭活病毒疫苗破乳液水相经HPSEC分离,在保留时间约13.3 min处出现抗原特征峰;MALLS计算该色谱峰分子量分别为2.61×10⁶(±4.34%) Da和2.40×10⁶(±2.51%) Da。两种VLP疫苗也在13.3 min处出现抗原特征峰,分子量分别为2.09×10⁶(±2.94%) Da和2.88×10⁶(±11.85%) Da,接近PCV2的理论分子量;同时在保留时间约11.4 min处也出现色谱峰,经检测分子量为4.37×10⁶(±0.42%) Da,TEM表征显示为VLP二聚体。取疫苗d和PCV2 VLP纯品进行重复检测,抗原色谱峰面积的RSD(n=3)均小于1.5%,重复性好;将PCV2 VLP纯品梯度稀释检测,VLP及其多聚体的色谱峰面积与浓度均呈良好的线性关系,R²分别为0.999及0.997,能够满足定量及多聚体含量分析。该方法有望成为一种准确、高效的PCV2疫苗的体外评价方法,用于质量评价与提升。     

Solution structure, divalent metal and DNA binding of the endonuclease domain from the replication initiation protein from porcine circovirus 2

Circoviruses are the smallest circular single-stranded DNA viruses able to replicate in mammalian cells. Essential to their replication is the replication initiator, or Rep protein that initiates the rolling circle replication (RCR) of the viral genome. Here we report the NMR solution three-dimensional structure of the endonuclease domain from the Rep protein of porcine circovirus type 2 (PCV2), the causative agent of postweaning multisystemic wasting syndrome in swine. The domain comprises residues 12-112 of the full-length protein and exhibits the fold described previously for the Rep protein of the representative geminivirus tomato yellow leaf curl Sardinia virus. The structure, however, differs significantly in some secondary structure elements that decorate the central five-stranded beta-sheet, including the replacement of a beta-hairpin by an alpha-helix in PCV2 Rep. The identification of the divalent metal binding site was accomplished by following the paramagnetic broadening of NMR amide signals upon Mn(2+) titration. The site comprises three conserved acidic residues on the exposed face of the central beta-sheet. For the 1:1 complex of the PCV2 Rep nuclease domain with a 22mer double-stranded DNA oligonucleotide chemical shift mapping allowed the identification of the DNA binding site on the protein and aided in constructing a model of the protein/DNA complex.     

Development of a Loop-Mediated Isothermal Amplification Assay for Porcine Circovirus Type 2

In this study, the loop-mediated isothermal amplification (LAMP) method was used to develop a rapid and simple detection system for porcine circovirus type 2 (PCV2). According to the PCV2 sequences published in GenBank, multiple LAMP primers were designed targeting conserved sequences of PCV2. Using the DNA extracted from PCV2 isolates HUN-09 and SD-09 as the template, LAMP reactions in a PCV2 LAMP system was performed, the amplification products were detected by adding SYBR Green I and could be observed di...     

鹅圆环病毒感染性克隆的构建及其转染试验

设计带BamHⅠ酶切标记位点的引物,PCR扩增鹅圆环病毒(Goose circovirus,GoCV)全长基因组,将2个基因组顺式连接插入到pGEM-T Easy载体中,获得GoCV全长基因组头尾串联二聚体感染性克隆质粒pGEMT-2GoCV。EcoRⅠ酶切线性化pGEMT-2GoCV,与脂质体混合转染GoCV阴性鹅胚和雏鹅,常规PCR检测发现GoCV在转染鹅体内增殖,鹅胚转染组于孵出第2周和第4周检出血清阳性,且其中一个个体于4周龄扑杀时检出法氏囊阳性,雏鹅转染组于转染后2周检出血清阳性。试验进一步对扩增片段进行了BamHⅠ标记位点的检测,并应用GoCV实时荧光定量PCR方法对转染阳性样品进行了定量,结果显示阳性法氏囊组织中病毒含量为1.57×106拷贝/mg,阳性血清含病毒拷贝数在3.52×104～5.92×105拷贝/μL。综上,本试验构建的GoCV全长基因组头尾串联二聚体感染性克隆DNA可以转染鹅胚和雏鹅并增殖出带标记的GoCV克隆。     

Mapping of the nuclear localization signals in open reading frame 2 protein from porcine circovirus type 1

Porcine circovirus type 1 （PCV1） contains two major open reading frames encoding the replication-associated proteins and the major structural capsid （Cap） protein. PCV1 Cap has an N-terminus carrying several potential monopartite or bipartite nuclear localization signals （NLS）. The contribution of these partially overlapping motifs to nuclear importing was identified by expression of mutated PCVI Cap versions fused to enhanced green fluorescent protein （EGFP）. The Cterminus truncated PCV1 Cap-EGFP was localized in nuclei of PK-15 cells similar to the wild-type PCV1 Cap-EGFP, whereas truncation of the N-terminus rendered the fusion protein distributed into cytoplasm, indicating that the nuclear import of PCV1 Cap was efficiently mediated by its N-terminal region. Substitutions of basic residues in stretches 9RR- RR12 or the right part of 25RRPYLAHPAFRNRYRWRRK43 resulted in a diffused distribution of the fusion protein in both nuclei and cytoplasm, indicating that the two NLSs were responsible for restricted nuclear targeting of PCV1 Cap.     

II型猪圆环病毒检测试剂盒的研制

猪圆环病毒(Porcine circovirus, PCV)属圆环病毒科圆环病毒属成员[1]。PCV分两种血清型,即PCV 1 和 PCV 2,其中 PCV 1 由 Tischer 等[2] 于1974年检测到,对猪没有致病性;PCV 2 可引起部分断奶仔猪和育肥猪的断奶仔猪多系统综合征( postweaning multisystemic wasting syndrome,PMWS)[3]。目前,该病呈世界分布,给养猪业造成巨大的经济损失。本研究通过分析已发表的 PCV 2的基因序列,找出 PCV 2 的特异性片段,研制了检测PCV 2的试剂盒。检测临床疑似病料,结果表明该试剂盒使用方便、快速、敏感、特异,符合国内的养殖场…     

猪圆环病毒II型ORF2基因在酵母中的高效分泌表达

为了建立一种简便的检测猪圆环病毒2型(PCV2)的方法,本实验将PCV2 的ORF2 基因片段整合到巴斯德毕赤酵母(Pichia pastoris)菌株X 33染色体上,构建了X 33(pPICZa ORF2)重组工程菌。经甲醇诱导后,成功的表达出ORF2基因片段。经过Bradford 蛋白质总含量测定和凝胶薄层扫描结果表明,表达产物占重组工程菌培养上清总蛋白的58%,表达量可达47mg/ L。间接ELISA结果初步表明重组表达产物具有良好的抗原性,能够有效地区分PCV2型病毒标准阳性与阴性血清。     

猪圆环病毒2型ORF2基因在昆虫细胞中的表达及其特性

利用Bac-to-Bac杆状病毒表达系统将圆环病毒2型的ORF2全基因克隆到杆状病毒转移载体pFastBac^TM1中,获得重组转移载体pFast-OFR2,再将其转化进含穿梭载体Bacmid的感受态细胞DH10Bac中,发生转座作用,经蓝白菌落筛选得到含ORF2基因的重组穿梭载体Bac-ORF2,以脂质体介导的方法将重组穿梭载体转染sf9细胞,获得重组病毒,命名为Ac-ORF2。间接免疫荧光分析表明,PCV2阳性血清能使Ac-ORF2感染的sf9昆虫细胞呈强的荧光着色; SDS-PAGE与Western-blotting分析可见大小约为28kD的特异性带,表明Ac.ORF2在sf9细胞中成功表达了PCV2-ORF2蛋白。将该表达蛋白纯化并经磷钨酸负染后,通过电镜观察可见形态与PCV2病毒粒子相似的病毒样颗粒(VLPs),其中某些颗粒由于中心浓染而似空衣壳,其直径也为17nm左右。