用套式PCR方法检出腹泻及健康犬粪中的犬冠状病毒

自2003年夏至2004年初的8个月内收集犬粪样112份,其中南京地区家庭单养的腹泻犬粪便43份,某养犬场群养健康犬粪便30份,沈阳地区某养犬基地群养健康犬粪便 39 份,用套式 PCR方法检测犬冠状病毒(CCV)。结果显示,南京家庭单养腹泻病犬 CCV阳性率为 40.9%(18/43),CCV检出率与季节相关,冬季的检出率较高。健康犬阳性率为84.1%(58/69),其中沈阳某场健康犬CCV的感染率(87.2%)高于南京某犬场(80.0%)。取南京腹泻犬和沈阳健康犬阳性样本各2份测序,结果表明,4个样本 M基因 212bp的序列与 GenBank登录的中国大熊猫源的CCV同源性最高(94.8~96.7),并且南京和沈阳CCV毒株之间存在一定序列差异。所有阳性样本用 CCV基因型鉴别PCR鉴定,均为CCVⅡ型。     

从健康狐狸、貉粪中检出犬冠状病毒的两种基因型

取某养殖场健康狐狸 (6 1份 )、貉 (2 4份 )粪样 ,用套式PCR(RT-nPCR)方法检测犬冠状病毒 (CCV)并进行基因型鉴定。结果显示 :狐狸粪样中有 4 3份 (70 . 5 % )为CCVⅡ型阳性 ,2 9份 (47. 5 % )为CCVⅠ型阳性 ,两型混合感染2 5份 ,占 4 1 0 % ,两型总感染率为 77 .0 %。 2 4份貉粪样中 ,2 2份为CCVⅡ型阳性 (91 .7% ) ,其中 16份为CCVⅠ型、Ⅱ型混合感染 (6 6 . 7% )。分别取狐狸和貉粪样中CCVⅠ、Ⅱ型阳性PCR产物各 2份 (共 8份 )进行测序 ,均与CCV的M基因序列相符 ,证实PCR结果非假阳性。序列及系统进化分析表明 ,CCVⅠ型与源于意大利腹泻犬的CCVⅠ型 (AF5 0 2 5 83)同源性最高 (96 . 7%～ 98. 1% ) ;CCVⅠ、Ⅱ两种基因型同源性为 88. 3%～ 89. 7% ,在进化树中处于两个大的分支上 ;同为CCVⅡ型 ,狐狸源与貉源序列也存在多个位点差异。首次在貉粪中检出CCV ,证实在健康狐狸、貉群体中存在CCV流行 ,且CCVⅠ、Ⅱ型并存。     

猕猴逆转录病毒多重套式PCR检测方法的建立

分别针对编码STLV-1和SRV/D-1两种逆转录病毒膜蛋白的env基因进行引物设计,通过优化、调整PCR条件,建立一种能同时检测猕猴STLV-1和SRV/D-1两种逆转录病毒的多重PCR方法,用于猕猴种群逆转录病毒的常规监测。结果显示多重套式PCR产物片段大小与预期结果一致,进一步测序证实为目的产物,说明建立的多重套式PCR方法能同时检测出猕猴体内可能存在的STLV-1和SRV/D-1两种逆转录病毒。这种方法具有灵敏度高、特异性强、省时、试剂用量少和检测费用低等优点,因此可以作为一种新方法用于猕猴种群逆转录病毒的定性监测。     

绵羊肺腺瘤病特异性PCR及套式PCR诊断方法的建立

绵羊肺腺瘤是由外源性反转录病毒JSRV引起的接触性传染的肺肿瘤性疾病。感染羊没有针对JSRV的循环抗体,但在感染羊的肺肿瘤组织、淋巴网状系统及外周血单核细胞中可检测到外源性前病毒exJSRV及JSRV转录产物。健康羊基因组中存在15~20拷贝的内源性前病毒enJSRV,内外源性前病毒的结构基因高度相似,而在U3区存在差别,因而,设计了针对exJSRVU3区的特异性引物并在国内首次建立了一步法特异性PCR检测法及套式PCR检测法。以700ng健康羊基因组DNA为背景,梯度稀释阳性质粒pJSRV-LTR作为模板,比较两种方法的敏感性,结果表明套式法的敏感性是一步法的10倍以上,套式法也是目前可用于检测感染羊血液样品的唯一方法,可望在绵羊肺腺瘤病的流行病学调查及防控方面起重要作用。     

慢性蜜蜂麻痹病毒半套式PCR检测方法的建立

参考NCBI(National Center of Biotechnology Information)已发表的慢性蜜蜂麻痹病毒(Chronic bee paralysis virus,CBPV)的全基因序列,设计3条检测CBPV的特异性引物,建立CBPV半套式PCR(Polymerase Chain Reaction)检测方法,对其外引物退火温度(52、54、56和58℃)、内引物退火温度(48、50、52和54℃)、引物浓度(0.1、0.2和0.4mmol/L)和ExTaq酶体积(0.25、0.5和1μL)进行优化,并对优化后的方法进行了特异性、敏感性验证,同时,利用该方法对20份临床样品进行检测。结果表明,该半套式PCR最佳外引物退火温度、内引物退火温度、引物浓度和ExTaq酶体积分别为56℃、50℃、0.2mmol/L和0.25μL;感染CBPV与健康蜜蜂、急性蜜蜂麻痹病毒(Acute paralysis virus,ABPV)、中蜂囊状幼虫病病毒(Chinese sacbrood bee virus,CSBV)、黑蜂王台病毒(Black queen cell virus,BQCV)、蜜蜂残翼病毒(Deformed wing virus,DWV)的cDNA均无交叉反应,检出最低下限为10-3pg;从20份临床样品中检出4份阳性。说明建立的CBPV半套式PCR检测方法具有快捷、敏感、特异等优点,可用于CBPV感染的临床诊断和流行病学调查。     

RT套式PCR检测血浆HCV RNA及与抗HCV检测的比较

应用微量血清热变性法提取核酸,逆转录套式聚合酶链反应(RT-nest PCR)检测血浆HCV RNA,并与抗HCV ELISA检测结果比较,对HCV RNA阳性标本进行HGV RNA的筛查.结果在32例抗HCV阳性和20例抗HCV阴性血浆中,HCV RNA分别检出18例和2例,总符合率为70%,20例HCV RNA阳性者中有2例合并感染HBV,1例合并感染HGV.证明血浆样本中抗HCV与HCV RNA间存在很大的相关性.     

采用套式PCR检测水库产毒微囊藻

根据所测定的微囊藻毒素合成酶mcyB基因的部分核苷酸序列,设计并筛选出两对特异性引物,用于产毒微囊藻的套式PCR检测。套式PCR针对毒素基因的检测结果与ELISA针对微囊藻毒素的检测结果相一致,但灵敏度更高。套式PCR的检测下限达1—10个微囊藻细胞/反应。采用套式PCR对广东12个主要供水水库的247份水样进行了产毒微囊藻检测,共检出阳性水样82份,阳性率为33.2%。这些阳性水样分布于除深圳水库以外的其他11个水库;其中汤溪水库水样套式PCR检出阳性率最高,达67.4%,其水样一步PCR的检出阳性率亦达25.6%,值得引起水文部门重视,并进行进一步跟踪监测。     

逆转录套式PCR检测粪便样本中的SARS冠状病毒

为了观察SARS冠状病毒在SARS患者粪便中的存在规律,建立了检测SARS冠状病毒RNA的逆转录-聚合酶链反应(RT-PCR)方法,并应用该方法检测了241份SARS患者粪便样本。部分PCR产物应用测序技术进行验证。RT-PCR的灵敏度为10^-10稀释度的病毒原液(原液为10^8TCID50／ml)。241份粪便样本的总体检出率为24．1％(58／241),其中发病后的前10d和20d的检出率均为50．0％。随着发病时间的延长,阳性检出率呈下降趋势。应用RT-PCR从粪便中检测SARS冠状病毒是可行的,在发病50d以后仍有17．0％左右的阳性检出率,提示SARS恢复期患者具有排毒的可能性,给后续的卫生防疫措施提供了一定的参考数据。     

双重套式PCR对不同取样胚胎性别鉴定灵敏度测试

目的:测定双重套式PCR微量扩增体系的灵敏度,为附植前遗传学诊断 (PGD)、家畜胚胎性别鉴定等提供技术保障。方法:以桑椹胚卵裂球为模板进行扩增,建立昆明白小鼠特异的SRY ZFX双重套式PCR性别鉴定体系。按卵裂球数量的不同分为五组,对应的卵裂球个数分别为 1、2、3、4、5及以上。根据有效扩增结果得出双重套式PCR的灵敏度。结果:第 1组 (卵裂球个数为 1 ),有效检出率为 85 % ( 34 /40 ),污染率为 7 5 % ( 3 /40 ),漏检率为 7 .5 % ( 3 /40 )。随着卵裂球个数的增多,有效检出率逐渐升高,而污染率和漏检率则呈逐渐下降趋势。第 5组 (卵裂球达到 5及以上 ),有效检出率达到 1 0 0 %,漏检率为 0。对于第 2、3、4、5组而言,有效检出率及漏检率各组间并无显著差异 (P >0 . 0 5 );而第一组与其它各组间,有效检出率及漏检率存在显著差异 (P <0 .0 5 )。结论:双重套式PCR可以有效扩增基因组DNA量约为 1 2pg的模板,且扩增片段为单拷贝片段。     

运用套式PCR检测传染性喉气管炎病毒核酸

选择鸡传染性喉气管炎病毒保守TK基因的蛋白编码区域,设计并合成了一对外引物和一对内引物,建立并优化了检测鸡传染性喉气管炎病毒DNA的套式PCR法。通过检测ILTV感染的鸡胚绒毛尿囊膜,实验室病料和临床病料,结果表明,套式PCR法能检测出ILTV感染后的非免疫鸡胚和SPF鸡绒毛膜研磨液中的被稀释了10^5倍的病毒（约1fg的ILTV DNA）,攻毒后第10天还能从非免疫鸡和SPF鸡气管拭子中检出ILTV,第10天非免疫鸡气管拭子中ILTV的最大检出率为7／10,第10天SPF鸡气管拭子中ILTV的最大检出率为8／10。对非免疫鸡和SPF鸡的气管拭中ILTV最佳检出时间均在攻毒后第5天。对临床样品中的ILTV的最大检出率为7／7。经过核酸杂交验证,套式PCR法具有很高的特异性和敏感性,为从分子水平探讨ILTV的发病机理、临床早期快速诊断提供了新的研究手段。     

PCR Detection and Molecular Characterization of Pentatrichomonas hominis from Feces of Dogs with Diarrhea in the Republic of Korea

Pentatrichomonas hominis is considered a commensal protozoan in the large intestine of a number of mammalian hosts, such as cats, dogs, and non-human primates. The resulting infections, which can induce diarrhea, have been attributed to opportunistic overgrowth of P. hominis. This study was performed to confirm the P. hominis infection and its molecular characterization from the feces of puppies with diarrhea. Fecal samples were obtained from 14 German shepherd puppies with diarrhea over 1 week (7 females and 7 males, 2-9 months of age) residing on a dog farm in August 2007. Species-specific PCR assay identified P. hominis 18S rRNA genes in 3 of the 14 puppies (1 female and 2 males; 1 aged 2 months and 2 aged 9 months). This phylogenetic analysis established that P. hominis belonged to the 1st clade, which is comprised of Bos taurus and Felines.     

Nested-PCR检测恒河猴泡沫病毒

目的用nested-PCR检测恒河猴泡沫病毒SFV的前病毒形式。方法从SFV-1的pol区域选择两对引物分别对原代猴肾细胞（rhesus monkey kidney,RMK）及猴外周血淋巴细胞（peripheral blood lymphocytes,PBLs）进行体外扩增,扩增产物经1.0%的琼脂糖凝胶电泳,证实其特异性。阳性对照使用具有典型泡沫样病变的RMK377细胞株的前病毒DNA,阳性对照的PCR扩增产物经测序证实,阴性对照为恒河猴的SRV-1cDNA。结果nested-PCR能快速灵敏的直接从猴外周血淋巴细胞检出SFV的前病毒形式,与RMK细胞培养结果基本相一致。结论本实验所建立的检测SFV的nested-PCR法能快速准确的检测猴群中的SFV的带毒情况,对于提高实验猴的质量具有重要意义。     

Feline Coronavirus Type II Strains 79-1683 and 79-1146 Originate from a Double Recombination between Feline Coronavirus Type I and Canine Coronavirus

Recent evidence suggests that the type II feline coronavirus (FCoV) strains 79-1146 and 79-1683 have arisen from a homologous RNA recombination event between FCoV type I and canine coronavirus (CCV). In both cases, the template switch apparently took place between the S and M genes, giving rise to recombinant viruses which encode a CCV-like S protein and the M, N, 7a, and 7b proteins of FCoV type I (K. Motowaka, T. Hoh- datsu, H. Hashimoto, and H. Koyama, Microbiol. Immunol. 40:425–433, 1996; H. Vennema, A. Poland, K. Floyd Hawkins, and N. C. Pedersen, Feline Pract. 23:40–44, 1995). In the present study, we have looked for additional FCoV-CCV recombination sites. Four regions in the pol gene were selected for comparative sequence analysis of the type II FCoV strains 79-1683 and 79-1146, the type I FCoV strains TN406 and UCD1, the CCV strain K378, and the TGEV strain Purdue. Our data show that the type II FCoVs have arisen from double recombination events: additional crossover sites were mapped in the ORF1ab frameshifting region of strain 79-1683 and in the 5′ half of ORF1b of strain 79-1146.     

The Skin Microbiome in Healthy and Allergic Dogs

Background

Changes in the microbial populations on the skin of animals have traditionally been evaluated using conventional microbiology techniques. The sequencing of bacterial 16S rRNA genes has revealed that the human skin is inhabited by a highly diverse and variable microbiome that had previously not been demonstrated by culture-based methods. The goals of this study were to describe the microbiome inhabiting different areas of the canine skin, and to compare the skin microbiome of healthy and allergic dogs.

Methodology/Principal Findings

DNA extracted from superficial skin swabs from healthy (n = 12) and allergic dogs (n = 6) from different regions of haired skin and mucosal surfaces were used for 454-pyrosequencing of the 16S rRNA gene. Principal coordinates analysis revealed clustering for the different skin sites across all dogs, with some mucosal sites and the perianal regions clustering separately from the haired skin sites. The rarefaction analysis revealed high individual variability between samples collected from healthy dogs and between the different skin sites. Higher species richness and microbial diversity were observed in the samples from haired skin when compared to mucosal surfaces or mucocutaneous junctions. In all examined regions, the most abundant phylum and family identified in the different regions of skin and mucosal surfaces were Proteobacteria and Oxalobacteriaceae. The skin of allergic dogs had lower species richness when compared to the healthy dogs. The allergic dogs had lower proportions of the Betaproteobacteria Ralstonia spp. when compared to the healthy dogs.

Conclusions/Significance

The study demonstrates that the skin of dogs is inhabited by much more rich and diverse microbial communities than previously thought using culture-based methods. Our sequence data reveal high individual variability between samples collected from different patients. Differences in species richness was also seen between healthy and allergic dogs, with allergic dogs having lower species richness when compared to healthy dogs.     

番木瓜环斑病毒PCR检测技术研究

建立了检测番木瓜环斑病毒(PRV)的免疫捕捉-PCR(IC-PCR)法、ELISA-PCR法和巢式-PCR法,它们分别能从10-4、10-7和10-14稀释度的番木瓜叶粗汁液(所含鲜叶组织的量分别0.5ug、0.5ng和5×10-6ng)中检测出PRV.     

应用PCR-RFLP和巢式PCR检测黄瓜尖镰孢菌

以3株黄瓜尖镰孢菌(Fusarium oxysporum f.sp.cucumarinum)、23株镰孢菌属(Fusariumspp.)真菌和分离自土壤的20株真菌、6株细菌和7株放线菌为材料,采用化学裂解法提取总DNA,进行PCR-RFLP和巢式PCR检测,试验证明PCR-RFLP程序不能完全区分Fusarium属内不同种,而巢式PCR对黄瓜尖镰孢菌具有特异性.运用优化的PCR-RFLP和巢式PCR检测程序对染病黄瓜组织进行了检测,结果表明,两种方法均可在接种发病早期(未显症时)检测出黄瓜枯萎病菌,PCR-RFLP在感病品种接种后3d即可检测到病原菌,而巢式PCR在接种后5d才能检测到病原菌.     

番木瓜环斑病毒PCR检测技术研究

建立了检测番木瓜环斑病毒 (PRV)的免疫捕捉 PCR (IC PCR)法、ELISA PCR法和巢式 PCR法 ,它们分别能从 10 - 4、10 - 7和 10 - 14 稀释度的番木瓜叶粗汁液 (所含鲜叶组织的量分别 0 .5ug、0 .5ng和 5× 10 - 6ng)中检测出PRV。     

Antimicrobial Susceptibility and rRNA Gene Restriction Patterns among Staphylococcus intermedins from Healthy Dogs and from Dogs Suffering from Pyoderma or Otitis Externa

A total of 60 Staphylococcus intermedins strains from dogs were investigated by their sensitivity to various antibiotics (50 strains) and by their rRNA gene restriction patterns (ribotyping) (60 strains). Fifteen isolates were from healthy dogs, 9 with otitis externa, and 36 with pyoderma, including 10 strains from a previous study. Sixty per cent of the 50 strains tested for antibiotic susceptibility demonstrated resistance to penicillin, 24% to spiramycin, 20% to tetracycline, 16% to chloramphenicol, and 2% to fucidic acid. All isolates were susceptible to amoxycillin with clavulanic acid, enrofloxacin, and sulphonamides with trimethoprim. There were no significant differences in antimicrobial susceptibility patterns observed among isolates from pyoderma, otitis externa or healthy dogs. Among the 60 strains studied by ribotyping, 10 different ribotypes were identified: 6 different ribotypes among isolates from otitis externa, 8 among isolates from pyoderma, and 5 among isolates from healthy dogs. One ribotype (profile C) was dominant among the isolates from healthy dogs while another ribotype (profile A) was dominant among strains from dogs suffering from pyoderma. This profile was not demonstrated in any of the strains from healthy dogs. From 5 different dogs suffering from pyoderma, 2 different clones were demonstrated based on their plasmid profile and antibiogram. In these dogs 1 of the clones always belonged to ribotype A. The results concerning strains of S. intermedins isolated from furunculosis suggest the existence of distinct subpopulations with different pathogenicity to dogs.     

猴血中SFV病毒基因PCR检测方法的建立及应用

针对猴泡沫病毒SFV（Simian Foany Virus）多聚酶区（pol区）设计两对引物,以猴血DNA为模板者嵌套式PCR扩增,得到500bp左右基因片段,克隆进入pUC-19载体,经测序鉴定为SFV465bp的pol区基因片段,将此段序列与SFV各型425bp的pol区基因片段进行同源性比较,它与SFV－1型的同源性最高,为92.00%。在此基础上,用这两对引物对158例猴血DNA进行检测,阳性54例,阳性率为34.2%,发现猴群中有较高的SFV病毒的感染。