Establishment of Multi-Site Infection Model in Zebrafish Larvae for Studying Staphylococcus aureus Infectious Disease

Zebrafish(Danio rerio) is an ideal model for studying the mechanism of infectious disease and the interaction between host and pathogen.As a teleost,zebrafish has developed a complete immune system which is similar to mammals.Moreover,the easy acquirement of large amounts of transparent embryos makes it a good candidate for gene manipulation and drug screening.In a zebrafish infection model,all of the site,timing,and dose of the bacteria microinjection into the embryo are important factors that determine the bacterial infection of host.Here,we established a multi-site infection model in zebrafish larvae of 36 hours post-fertilization(hpf) by micro-injecting wild-type or GFP-expressing Staphylococcus aereus(5.aureus) with gradient burdens into different embryo sites including the pericardial cavity(PC),eye,the fourth hindbrain ventricle(4V),yolk circulation valley(YCV),caudal vein(CV),yolk body(YB),and Duct of Cuvier(DC) to resemble human infectious disease.With the combination of GFP-expressing S.aureus and transgenic zebrafish Tg(corola:eGFP;lyz:Dsred) and Tg(lyz:Dsred) lines whose macrophages or neutrophils are fluorescent labeled,we observed the dynamic process of bacterial infection by in vivo multicolored confocal fluorescence imaging.Analyses of zebrafish embryo survival, bacterial proliferation and myeloid cells phagocytosis show that the site- and dose-dependent differences exist in infection of different bacterial entry routes.This work provides a consideration for the future study of pathogenesis and host resistance through selection of multi-site infection model.More interaction mechanisms between pathogenic bacteria virulence factors and the immune responses of zebrafish could be determined through zebrafish multi-site infection model.     

PCR快速检测伪狂犬病病毒野毒感染

根据已发表的伪狂犬病病毒(PrV)gE、gI基因的序列,设计并合成了一对引物,以PrV容A株细胞培养毒为模板,筛选最佳反应条件和试剂工作浓度,建立了区分PrV野毒株和疫苗弱毒的鉴别PCR方法.该方法能从PrV容A株(RA)、上海株(SH)、鲁A株(LA)中扩增出一条848bp的片段,但Bartha-K61株没有扩增出该片段.测序结果表明PCR扩增产物和方法的特异性.对正常细胞与其它6种引起猪病毒性疫病相关病毒进行检测,结果均为阴性,没有出现交叉反应.对PrV容A株细胞毒提取物DNA进行检测,其最低检出量为5pg.PCR对感染野毒的发病猪不同组织器官检测发现,淋巴结检出率最高,依次为脾、脑(海马角)、肺、肾、肝等.对2003～2004年期间江苏、浙江、安徽、福建、上海等省市的37个大中型猪场送检的172份病料进行PCR检测病料阳性率为20.34%(35/172),猪场阳性率为40.54%(15/37).实验结果表明所建立的PCR技术可用于伪狂犬病野毒感染的快速鉴定和流行病学调查.     

SHIV-KB9感染中国恒河猴动物模型的建立

目的为了进一步确证SHIV-KB9感染中国恒河猴的病毒浓度范围,测试动物对病毒的适应性,明确该动物模型的可重复性。方法实验前采集猴血清并进行血清学检查。选出4只无SIV、STLV、SRV/D和B病毒感染的恒河猴,分别用10倍系列稀释的病毒液静脉感染实验猴,使用流氏细胞术、血常规、病毒分离、DNA-PCR和RT-PCR等方法确定实验猴是否被感染,以及感染后恒河猴体内病毒复制和免疫细胞损伤情况。结果实验猴的血浆病毒载量、病毒分离结果、CD4＋/CD8＋比值和CD4＋T细胞数等证实,4.8×105 copies/mL以上浓度的SHIV-KB9病毒液能成功感染中国恒河猴。结论本研究进一步明确了SHIV-KB9感染中国恒河猴的有效病毒浓度范围,确定了SHIV-KB9病毒感染中国恒河猴的病毒学、免疫学的测定指标,成功的建立了SHIV-KB9/中国恒河猴动物模型。     

PCR快速检测伪狂犬病病毒野毒感染

根据已发表的伪狂犬病病毒(PrV)gE、gI基因的序列,设计并合成了一对引物,以PrV容A株细胞培养毒为模板,筛选最佳反应条件和试剂工作浓度,建立了区分PrV野毒株和疫苗弱毒的鉴别PCR方法。该方法能从PrV容A株(RA)、上海株(SH)、鲁A株(LA)中扩增出一条848bp的片段,但Bartha-K61株没有扩增出该片段。测序结果表明PCR扩增产物和方法的特异性。对正常细胞与其它6种引起猪病毒性疫病相关病毒进行检测,结果均为阴性,没有出现交叉反应。对PrV容A株细胞毒提取物DNA进行检测,其最低检出量为5pg。PCR对感染野毒的发病猪不同组织器官检测发现,淋巴结检出率最高,依次为脾、脑(海马角)、肺、肾、肝等。对2003～2004年期间江苏、浙江、安徽、福建、上海等省市的37个大中型猪场送检的172份病料进行PCR检测病料阳性率为20．34％(35／172),猪场阳性率为40.54％(15／37)。实验结果表明所建立的PCR技术可用于伪狂犬病野毒感染的快速鉴定和流行病学调查。     

树鼩呼吸道合胞病毒感染动物模型的建立

探讨用灵长类动物树鼠句建立呼吸道合胞病毒(RSV)感染动物模型的可行性。28只树鼠句随机分为7组,每组4只,鼻内滴入106PFU RSV,感染后每24h检测1组。另取7只树鼠句鼻内滴入100μl Hep-2细胞培养液,滴鼻后每24h检测1只作对照。无菌取树鼠句肺组织进行病毒分离、空斑形成实验检测病毒滴度、病理检查和RT-PCR检测肺组织内RSV mRNA表达。结果显示:树鼠句感染RSV后,无明显呼吸道感染症状;树鼠句肺组织匀浆接种于Hep-2细胞上,第3、4、5实验组出现细胞病变效应(CPE);树鼠句感染RSV后肺部病理改变在3~7d较为明显,主要为间质改变;在106PFU感染浓度下树鼠句肺组织内RSV处于低水平复制,复制的高峰期在3~5d,峰值在第4d。提示:树鼠句可以用来建立RSV感染的动物模型。     

雪貂感染流感病毒H3N2动物模型的建立

目的建立甲型流感病毒H3N2感染的雪貂动物模型。方法按实验要求筛选出流感抗体反应阴性的雪貂,经兽用氯胺酮轻度麻醉后进行滴鼻感染H3N2流感病毒株A/Brisbane/10/07,设立两个稀释度106和107 TCID50,每个稀释度接种3只雪貂,感染后第5天安乐处死。感染前采集鼻甲骨活检,感染后1～5 d鼻甲骨活检检测病毒载量,每天记录雪貂一般临床变化。处死时取雪貂肺、肝、脾、小肠、脑组织作病毒滴度检测,肺组织做病理检查。结果 106和107TCID50的H3N2病毒分别感染雪貂,没有雪貂死亡。雪貂感染后都出现一过性的体温升高,体重的下降,流涕、打喷嚏等症状。在鼻甲骨活检物中可测到病毒载量,肠组织可分离到病毒。肺组织以轻度性间质性肺炎为主要病理变化。结论雪貂感染H3N2病毒株A/Brisbane/10/07后,临床表现、病毒学、分子生物学、病理学方面的检测都可以证实雪貂感染H3N2病毒动物模型已建立,其中106 TCID50病毒滴度的是一个建立感染动物模型比较合适的剂量。     

Ⅲ型登革病毒在THP-1细胞上的ADE模型建立

登革热(dengue fever,DF)是由Ⅰ、Ⅱ、Ⅲ和Ⅳ型登革病毒(dengue virus,DENV)引起的急性传染病,抗体依赖增强感染(antibody-dependent enhancement,ADE)是自限性的登革热以及危及生命的登革出血热(dengue hemorrhagic fever,DHF)或登革休克综合症(dengue shock syndrome,DSS)等重症的主要原因。采用不同稀释度的Ⅱ型登革病毒prM前膜抗体与分离自云南西双版纳重症病人的Ⅲ型登革病毒复合感染THP-1细胞,通过实时荧光定量PCR发现亚中和浓度prM前膜抗体诱发THP-1细胞液中更高浓度的病毒载量。在THP-1细胞系上的研究可为后续研究登革病毒ADE打下坚实的基础。     

A Recombinant Measles Vaccine Virus Expressing Wild-Type Glycoproteins: Consequences for Viral Spread and Cell Tropism

Wild-type, lymphotropic strains of measles virus (MV) and tissue culture-adapted MV vaccine strains possess different cell tropisms. This observation has led to attempts to identify the viral receptors and to characterize the functions of the MV glycoproteins. We have functionally analyzed the interactions of MV hemagglutinin (H) and fusion (F) proteins of vaccine (Edmonston) and wild-type (WTF) strains in different combinations in transfected cells. Cell-cell fusion occurs when both Edmonston F and H proteins are expressed in HeLa or Vero cells. The expression of WTF glycoproteins in HeLa cells did not result in syncytia, yet they fused efficiently with cells of lymphocytic origin. To further investigate the role of the MV glycoproteins in virus cell entry and also the role of other viral proteins in cell tropism, we generated recombinant vaccine MVs containing one or both glycoproteins from WTF. These viruses were viable and grew similarly in lymphocytic cells. Recombinant viruses expressing the WTFH protein showed a restricted spread in HeLa cells but spread efficiently in Vero cells. Parental WTF remained restricted in both cell types. Therefore, not only differential receptor usage but also other cell-specific factors are important in determining MV cell tropism.     

Development of a Hamster Model for Chikungunya Virus Infection and Pathogenesis

Chikungunya virus is transmitted by mosquitoes and causes severe, debilitating infectious arthritis in humans. The need for an animal model to study the disease process and evaluate potential treatments is imminent as the virus continues its spread into novel geographic locations. Golden hamsters (Mesocricetus auratus) are often used as outbred laboratory animal models for arboviral diseases. Here we demonstrate that hamsters inoculated with chikungunya virus developed viremia and histopathologic lesions in their limbs and joints similar to those seen in human patients. The virus disseminated rapidly and was found in every major organ, including brain, within a few days of infection. Hamsters did not manifest overt clinical signs, and the virus was generally cleared within 4 days, followed by a strong neutralizing antibody response. These results indicate that hamsters are highly susceptible to chikungunya virus infection and develop myositis and tenosynovitis similar to human patients followed by a complete recovery. This animal model may be useful for testing antiviral drugs and vaccines.     

Zebrafish Egg Infection Model for Studying Candida albicans Adhesion Factors

Disseminated candidiasis is associated with 30–40% mortality in severely immunocompromised patients. Among the causal agents, Candida albicans is the dominant one. Various animal models have been developed for investigating gene functions in C. albicans. Zebrafish injection models have increasingly been applied in elucidating C. albicans pathogenesis because of the conserved immunity, prolific fecundity of the zebrafish and the low costs of care systems. In this study, we established a simple, noninvasive zebrafish egg bath infection model, defined its optimal conditions, and evaluated the model with various C. albicans mutant strains. The deletion of SAP6 did not have significant effect on the virulence. By contrast, the deletion of BCR1, CPH1, EFG1, or TEC1 significantly reduced the virulence under current conditions. Furthermore, all embryos survived when co-incubated with bcr1/bcr1, cph1/cph1 efg1/efg1, efg1/efg1, or tec1/tec1 mutant cells. The results indicated that our novel zebrafish model is time-saving and cost effective.     

利用乙型肝炎病毒共价闭合环状DNA构建慢性乙型肝炎病毒感染的小鼠模型

目的通过水动力法注射乙型肝炎病毒(HBV)共价闭合环状DNA(cccDNA)构建C57BL/6小鼠慢性乙型肝炎病毒感染的模型。方法取29只C57BL/6小鼠,分为实验组、对照组和空白组,应用水动力法分别注射HBV cccDNA、pAAV-HBV1.2及等渗盐水,于注射后收集不同时间点的血清和肝组织。利用放射免疫法检测血清样本中乙型肝炎病毒表面抗原(HBsAg)和乙型肝炎病毒e抗原(HBeAg);荧光定量PCR检测血清和肝组织中HBV DNA拷贝数;免疫组织化学法检测肝组织中HBsAg和乙型肝炎病毒核心抗原(HBc Ag)的表达;苏木精-伊红(HE)染色观察肝组织病理变化;使用SPSS 17.0对数据进行统计学分析。结果实验组HBsAg和HBeAg表达均呈现4个上升-下降曲线:HBsAg峰值分别出现在第3天、第3周、第7周和第9周;HBeAg峰值分别出现在第1天、第1周、第4周和第10周。对照组HBsAg和HBeAg表达分别呈现2个或3个明显的峰:HBsAg峰值分别出现在第3天和第8周;HBeAg峰值分别出现在第1天、第3周和第10周。空白组未检测出HBsAg和HBeAg。实验组HBV DNA拷贝数高于对照组的拷贝数(P<0.01);肝组织中HBV DNA拷贝数高于同期血清中的拷贝数(P<0.01);实验组和对照组的肝组织中均有HBsAg和HBc Ag的表达;实验组与对照组出现肝脏细胞炎症、肝细胞纤维化、肝细胞坏死等病理变化,而空白组正常。结论利用水动力法向C57BL/6小鼠体内转入HBV cccDNA,成功建立了慢性乙型肝炎病毒感染的小鼠模型,与对照组比较,新建立的小鼠乙肝模型具有更高的HBV表达,动物模型为研究乙型肝炎病毒HBV cccDNA的感染及其引起肝损伤的机制奠定了基础。     

Comprehensive Analysis of Herpes Simplex Virus 1 (HSV-1) Entry Mediated by Zebrafish 3-O-Sulfotransferase Isoforms: Implications for the Development of a Zebrafish Model of HSV-1 Infection

Binding of herpes simplex virus 1 (HSV-1) envelope glycoprotein D (gD) to the receptor 3-O-sulfated heparan sulfate (3-OS HS) mediates viral entry. 3-O-Sulfation of HS is catalyzed by the 3-O-sulfotransferase (3-OST) enzyme. Multiple isoforms of 3-OST are differentially expressed in tissues of zebrafish (ZF) embryos. Here, we performed a comprehensive analysis of the role of ZF 3-OST isoforms (3-OST-1, 3-OST-5, 3-OST-6, and 3-OST-7) in HSV-1 entry. We found that a group of 3-OST gene family isoforms (3-OST-2, -3, -4, and -6) with conserved catalytic and substrate-binding residues of the enzyme mediates HSV-1 entry and spread, while the other group (3-OST-1, -5, and -7) lacks these properties. These results demonstrate that HSV-1 entry can be recapitulated by certain ZF 3-OST enzymes, a significant step toward the establishment of a ZF model of HSV-1 infection and tissue-specific tropism.     

乙型肝炎病毒急性感染小鼠模型的建立

采用高压水注射方法,通过尾静脉将具有复制能力的HBV质粒导入BABL/cJ小鼠体内,应用real-timePCR、ELISA、RIA、Southern Blot、Northern Blot,以及免疫组化等方法,检测小鼠病毒血症、血清和肝组织中HBV抗原表达动态变化、肝组织中HBV转录和复制情况,以及小鼠免疫应答状况.结果HBV基因可以在小鼠体内表达和复制,并诱导小鼠产生特异性免疫应答,其应答模式及HBV清除过程与人类的HBV急性感染类似.实验显示高压注射具有复制能力的HBV质粒可以在小鼠体内建立HBV急性感染模型,这种模型可以用于HBV病毒学、免疫学以及抗病毒药物筛选等方面的研究.     

Competition between Wild-Type and Recombinant Nucleopolyhedroviruses in a Greenhouse Microcosm

Wild-type Autographa californica nucleopolyhedrovirus (AcNPV or AcNPV.WT), AcNPV expressing a scorpion toxin (AcNPV.AaIT), and AcNPV expressing a mutated juvenile hormone esterase (AcJHE.SG) were compared in their capability to produce epizootics in larvae of Trichoplusia ni infesting collards in a greenhouse microcosm. Larvae treated in four different ways were released into 1.8-m² microplots in week 1. The four treatments included (1) uninfected larvae (control), (2) 100% AcNPV.WT-infected larvae (WT), (3) 100% AcNPV.AaIT-infected larvae (AaIT), and (4) 1:1 ratio of AcNPV.WT-infected and AcNPV.AaIT-infected larvae (WT+AaIT). On a weekly basis, larvae were sampled and new, uninfected larvae were added to all plots. Sampled larvae were reared until death and then subjected individually to DNA–DNA dot-blot hybridization assay to determine the proportion of insects infected with each virus in each plot. The entire experiment was repeated with AcJHE.SG in the place of AcNPV.AaIT. Epizootics of AcNPV.WT lasted 8 weeks after a single viral release in the replicated greenhouse microplots. AcJHE.SG epizootics also lasted 8 weeks after viral release, but this virus and AcNPV.AaIT were both out-competed by AcNPV.WT. AcNPV.AaIT was no longer detected in the T. ni population by the fourth week after release. AcNPV.WT also increased to greater numbers in soil than AcNPV.AaIT or AcJHE.SG after 8 weeks. Thus, it was possible to induce 8-week epizootics of AcNPV.WT in replicated microplots under artificial greenhouse conditions, and the wild-type virus out-competed the recombinant virus for a niche in this greenhouse microcosm, which reduces the probability that the recombinant virus will persist in an agroecosystem.     

乙型肝炎病毒急性感染小鼠模型的建立

采用高压水注射方法,通过尾静脉将具有复制能力的HBV质粒导入BABL/cJ小鼠体内,应用real-time PCR、ELISA、RIA、Southern Blot、Northern Blot,以及免疫组化等方法,检测小鼠病毒血症、血清和肝组织中HBV 抗原表达动态变化、肝组织中HBV转录和复制情况,以及小鼠免疫应答状况。结果HBV基因可以在小鼠体内表 达和复制,并诱导小鼠产生特异性免疫应答,其应答模式及HBV清除过程与人类的HBV急性感染类似。实验显 示高压注射具有复制能力的HBV质粒可以在小鼠体内建立HBV急性感染模型,这种模型可以用于HBV病毒 学、免疫学以及抗病毒药物筛选等方向的研究。     

恒河猴感染SARS病毒致病模型的建立

为建立恒河猴严重急性呼吸道综合征(SARS)的模型并对其致病特点进行观察,采用病毒分离、免疫荧光、光镜及RT-PCR方法对病毒感染组和非感染组恒河猴不同时间、不同组织或分泌物进行检测.结果显示从恒河猴不同组织中分离到病毒,而且在病毒感染后第2d和第5d的血液、第7、9d的鼻咽分泌物、第3d的粪、第5d的粪尿中均检测到SARS-CoV RNA.光镜观察到病毒感染组肺组织肺泡间隔增宽,有大量淋巴细胞、单核细胞浸润,肺泡腔有渗出,甚至形成透明膜样物;多个肺泡形成机化性肺炎的表现.感染组肝组织可见较大的坏死灶,并伴有大量炎性细胞浸润.结论认为已成功建立了恒河猴SARS模型,可用于评价抗SARS药物和疫苗的研究.