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1.
Development of a PCR test to diagnose Haemophilus parasuis infections. 总被引:30,自引:0,他引:30
A polymerase chain reaction (PCR) test was developed in order to improve the accuracy and speed of diagnosis of Haemophilus parasuis, an economically important respiratory pathogen that affects swine. The gene sequence of the 16S small subunit ribosomal RNA of H. parasuis (GenBank M75065) was compared with 56 16S sequences of related bacteria, including those frequently isolated from pig tissues. Two species-specific primers were designed: HPS forward and HPS reverse. The predicted size of the amplified PCR product was 821 bp. The PCR test could detect a minimum of 102 bacteria and 0.69 pg of DNA. Thirty-one H. parasuis isolates, including 12 different serovars and 19 field isolates, were positive using the PCR test. No amplification was observed when the test was run using DNA from 15 other bacterial species commonly isolated from swine tissues. A weak band was observed when the PCR test was performed using Actinobacillus indolicus DNA as template. Clinical samples tested by PCR included tissues and swabs from 5 animals naturally infected with H. parasuis and 1 experimentally infected animal. The PCR was positive in 26 of 30 clinical samples. Four samples showed weak bands, and these results were not considered positive. Haemophilus parasuis was isolated from 18 of 30 of these samples. Tissues from specific pathogen-free (SPF) pigs and from unrelated species were negative for H. parasuis isolation and PCR. The developed PCR was successfully used in the diagnosis of H. parasuis infection, especially when compared with traditional microbiology techniques. 相似文献
2.
副猪嗜血杆菌PCR快速诊断方法的建立 总被引:7,自引:0,他引:7
副猪嗜血杆菌营养要求比较苛刻,常规生化试验检测方法比较烦琐,本研究针对副猪嗜血杆菌16SrRNA基因特异性PCR引物序列,合成一对PCR引物,建立相应的PCR检测方法,同时对该方法的灵敏性、特异性等实验。结果显示可检测出浓度为2.8×10^3CFU/mL的副猪嗜血杆菌表明该方法灵敏度高;对大肠杆菌、链球菌、巴氏杆菌、沙门氏杆菌、金黄色葡萄球菌进行PCR扩增均不获得任何条带,表明该方法特异性较强。所以该方法对于临床快速检测副猪嗜血杆菌具有重要意义。 相似文献
3.
副猪嗜血杆菌分离鉴定及药敏试验 总被引:1,自引:0,他引:1
副猪嗜血杆菌能够引起猪的多发性浆膜炎、关节炎和脑膜炎等,是影响猪的最重要细菌之一,目前在所有的主要养猪国家均有存在。为了弄清河南省副猪嗜血杆菌病流行情况,2012年-2015年,从河南不同地区猪场送检的疑似病料,进行副猪嗜血杆菌分离和鉴定,共分离到5株细菌,通过细菌形态观察、培养特征鉴定、生化试验、PCR检测,鉴定为副猪嗜血杆菌,分别命名为A6-fei、C3-xin、C12-xin、D2-fei和E1-fei。采用纸片扩散法,对分离5株副猪嗜血杆菌进行药敏试验,其结果表明所分离的5株副猪嗜血杆菌的药物敏感性不尽相同,各分离菌株对头孢噻肟、氟苯尼考星最敏感,对复方新诺明敏感性最差,其中菌株C3-xin对复方新诺明、庆大霉素、卡那霉素、青霉素完全耐药。表明副猪嗜血杆菌病在河南省依然存在,并且不同地区菌株对常用药物的敏感性各不相同,应当引起养猪场重视。 相似文献
4.
根据GenBank公布的大肠杆菌O157∶H7的Flic(H7)基因序列进行同源性比较分析,选择保守序列设计一对特异性扩增引物,通过优化反应条件,建立一个用于大肠杆菌O157∶H7快速定量检测的实时定量PCR方法。该方法的最低检测极限是103CFU/mL,敏感性比常规PCR提高10倍。方法重复性好、特异性强,重复性检测的变异系数均小于2%;只能检测大肠杆菌O157∶H7,对非大肠杆菌O157∶H7血清型细菌、猪链球菌2型、副猪嗜血杆菌无反应。利用此方法对模拟样本进行定量检测,其结果与平板细菌计数基本一致,表明此方法可作为大肠杆菌O157∶H7快速诊断和疫情监测的一种快速、准确、简便的检测工具。 相似文献
5.
为了解山东地区副猪嗜血杆菌病的流行情况和流行菌株的生物学特性及致病性,将2016-2018年山东省12个地区送检的103个发病猪的病料进行细菌分离,并对疑似菌株进行形态学观察、PCR鉴定及血清型鉴定,对两株流行菌株进行了培养特性观察、生化特性鉴定、药敏试验及致病性研究。最终分离获得29株副猪嗜血杆菌,分离率为28.16%,其中血清型4型和5型最为流行,其次是1型和12型。该病多发于春秋两季,31~50日龄的仔猪感染率最高。两株流行菌株LZ株和LC株均对青霉素类、头孢类等药物高度敏感,LZ株对庆大霉素、卡那霉素等中度敏感,对林可霉素、链霉素不敏感,LC株对庆大霉素、林可霉素等中度敏感,对卡那霉素、链霉素不敏感;生化特性试验结果显示,LC株和LZ株的硝酸盐还原试验、接触酶试验、葡萄糖发酵试验以及果糖发酵试验的结果均为阳性,吲哚试验、氧化酶试验、甘露醇发酵试验的结果均为阴性;动物致病性试验表明LZ株和LC株均具有较强的毒力,最小发病剂量分别为4.5×10^9 CFU和6.0×10^9 CFU。该研究为副猪嗜血杆菌病的防治提供了重要的参考依据。 相似文献
6.
猪胸膜肺炎放线杆菌、多杀性巴氏杆菌和副猪嗜血杆菌复合PCR检测方法的建立 总被引:2,自引:0,他引:2
目的建立可以同时检测猪胸膜肺炎放线杆菌、多杀性巴氏杆菌和副猪嗜血杆菌的快速而可靠的PCR检测方法。方法和结果根据胸膜肺炎放线杆菌的Apx-VIA基因序列、多杀性巴氏杆菌和副猪嗜血杆菌的16SrRNA基因序列设计5条引物。猪胸膜肺炎放线杆菌、多杀性巴氏杆菌和副猪嗜血杆菌模板的PCR扩增产物大小分别为342bp,485bp和1258bp。复合PCR对1~12型猪胸膜肺炎放线杆菌标准株,6株多杀性巴氏杆菌标准株,1~15型副猪嗜血杆菌以及25株经生化鉴定确认为上述三种细菌的分离株的基因组DNA作为模板进行检测,均获得预期大小的扩增产物。以猪放线杆菌、吲哚放线杆菌等14种常见细菌作为阴性对照进行PCR检测,结果仅有支气管败血波氏杆菌产生了可以和上述三个特异性条带明显区分的PCR产物。复合PCR针对胸膜肺炎放线杆菌、多杀性巴氏杆菌和副猪嗜血杆菌的敏感性分别为14pg、34pg和37pg。结论本研究建立的复合PCR特异性好,敏感性高,可以用于猪胸膜肺炎放线杆菌、多杀性巴氏杆菌和副猪嗜血杆菌的快速检测。 相似文献
7.
《Veterinary microbiology》1998,61(3):153-163
We compared a gB-ELISA, a gE-ELISA and a Danish test system (consisting of a blocking and an indirect ELISA) for their specificity and sensitivity to detect antibodies against BHV1. The Danish test system showed the highest sensitivity and the gE-ELISA the lowest; the gB-ELISA showed an intermediate sensitivity. If the doubtful zone (25–50% blocking) of the gB-ELISA was considered as positive (gB-ELISA+), the sensitivity almost reached that of the Danish test system. The specificity of all tests appeared to be very high, 99.7, 96.7 100, 99.7% for the gB-ELISA, gB-ELISA+, gE-ELISA and the Danish test system, respectively. Seroconversion was detected in the gE-ELISA up to 3 weeks later than in the gB-ELISA and the Danish test system. It is concluded that the combination of a gB-ELISA (for screening) and the Danish test (for confirmation) system used in the BHV1 eradication programme in the Netherlands, provides for very high sensitivity (>99.0%) (Kramps et al., 1994) and a very high specificity (>99.9%). 相似文献
8.
为建立副猪嗜血杆菌(Hps)的感染动物模型,本试验用Hps血清5型标准菌株(Nagasaki),以2.0×10~9CFU剂量腹腔感染豚鼠,观察豚鼠发病及死亡情况.取死亡豚鼠的主要器官组织,观察其病理和组织病理变化,与猪Classer's病痛变进行比较.并同时对死亡豚鼠进行细茵分离,分离菌经PCR鉴定.实验结果显示:在接种14 h后试验组豚鼠(5/8)出现死亡,死亡豚鼠剖检时出现了与猪Classer's病相似的病变;主要组织器官组织学变化以炎性细胞浸润、纤维蛋白和红细胞渗出等变化;并通过细茵分离培养,在豚鼠大脑、心血、肺、肝、脾和肾主要器官中分离到Hps血清5型茵.实验结果表明豚鼠可以作为Hps的感染动物模型.这一结果为研究其致病机制、诊断和免疫研究奠定基础. 相似文献
9.
本研究于2009年5月至2010年11月调查了广西南宁、桂林、玉林、钦州4个市60个猪场发生副猪嗜血杆菌病的情况。采集病猪组织样品共86份进行副猪嗜血杆菌分离;对疑似菌株进行形态学观察、培养特性、生化特性和PCR鉴定;最终分离鉴定到26株副猪嗜血杆菌,分离率为30.2%;对分离菌株进行血清型鉴定、致病性和药敏试验。结果表明26株分离株中血清4型有5株,5型3株,9、11、13、14、15型各1株,有1株与2、9、10、11型血清均有凝集,其余12株未能鉴定出血清型。血清型5、13、14菌株和5个未能定型的菌株能引起小白鼠全部死亡,其他菌株对小白鼠致病性不强。药敏试验结果表明70%以上的菌株除对恩诺沙星和氟苯尼考高度敏感外,对其他药物敏感性不高。本调查结果将对广西副猪嗜血杆菌病的防治提供指导。 相似文献
10.
猪传染性胸膜肺炎放线杆菌PCR检测试剂盒的研制 总被引:1,自引:1,他引:0
根据GenBank中猪传染性胸膜肺炎放线杆菌apxⅣA基因序列,设计了1对引物,通过对PCR反应条件进行优化,研制了检测猪传染性胸膜肺炎放线杆菌的PCR试剂盒。该试剂盒扩增的阳性条带为600 bp,特异性与敏感性结果显示,该PCR检测试剂盒的最低核酸检测量为50 CFU/mL,而对金黄色葡萄球菌、链球菌、多杀性巴氏杆菌、鼠伤寒沙门氏菌、副猪嗜血杆菌、大肠杆菌的扩增结果均为阴性。-20℃至少可保存12个月,且重复性良好。应用该PCR试剂盒对41份临床样本进行了检测,其PCR检测结果与细菌学检测结果相一致。结果表明,猪传染性胸膜肺炎放线杆菌PCR检测试剂盒能够对APP临床样品进行快捷、灵敏、准确的检测。 相似文献
11.
de la Puente Redondo VA Navas Méndez J García del Blanco N Ladrón Boronat N Gutiérrez Martín CB Rodríguez Ferri EF 《Veterinary microbiology》2003,92(3):253-262
On the basis of a species-specific PCR assay, a RFLP analysis for typing of Haemophilus parasuis strains was developed and evaluated. Amplification was based on the gene tbpA, encoding a transferrin-binding protein. RFLP analysis of the 1.9-kb tbpA-amplicon using TaqI, AvaI and RsaI endonucleases produced 12 different patterns for the reference strains of the 15 known H. parasuis serovars, and showed a high heterogeneity (33 RFLP groups) for 101 H. parasuis clinical isolates tested. The sensitivity, typeability (100% versus 65% for immunodiffusion), high degree of discrimination (0.93 versus 0.84 for immunodiffusion), simplicity and low cost per test make this PCR-RFLP assay a useful method for typing H. parasuis and, therefore, for studying the epidemiology of outbreaks of Gl?sser's disease. 相似文献
12.
13.
2011年从辽宁省采集以多发性纤维素性浆膜炎为主要特征的病猪肺脏、心包液、血液等病料,通过分离培养、生化试验和PCR检测等方法确认分离到1株副猪嗜血杆菌Hps LN111013,同时应用多种药物对该菌株进行了药物敏感性试验及分析;结果表明该菌株在形态、培养特性和生化试验等方面与国内其他地区所分离到的菌株基本一致,纸片法药敏试验证明本菌对氟苯尼考、头孢噻呋、洛美沙星最为敏感。本研究为进一步确认辽宁省副猪嗜血杆菌流行菌株的血清型和基因型,查明其传染来源和遗传变异情况奠定了基础,为制定辽宁省副猪嗜血杆菌病防控措施提供依据。 相似文献
14.
Classical swine fever virus: a second ring test to evaluate RT-PCR detection methods 总被引:5,自引:0,他引:5
Paton DJ McGoldrick A Bensaude E Belak S Mittelholzer C Koenen F Vanderhallen H Greiser-Wilke I Scheibner H Stadejek T Hofmann M Thuer B 《Veterinary microbiology》2000,77(1-2):71-81
Six laboratories participated in a study to compare the sensitivity and specificity of RT-PCR tests for the detection of classical swine fever virus (CSFV). Sets of coded samples were prepared by serial dilution of positive samples and then distributed to each of the laboratories. One set comprised 25 samples of random primed cDNA, synthesised from viral RNA representative of different pestiviruses. The other set comprised samples of blood and serum obtained from virus-free or CSFV-infected pigs. Each laboratory tested the samples using PCR/RT-PCR according to a set of standardised protocols that specified the exact conditions and requirements for inclusion of control samples. Two types of test were evaluated. One amplified a part of the 5'-non coding region of the pestivirus genome by means of a closed, one-tube RT-nested PCR. The other amplified a part of the NS5B gene using non-nested RT-PCR. The results of the laboratories were compared with one another, and with those obtained earlier when similar samples were tested by the same laboratories using non-standardised methods [Paton et al., Classical swine fever virus: a ring test to evaluate RT-PCR detection methods, Vet. Microbiol., in press]. Standardisation of the protocols resulted in a more consistent test sensitivity. Three laboratories avoided significant false positive results. Others that did not, could nevertheless recognise that test specificity was inadequate from the results obtained with the control samples. Minimum requirements for the inclusion of adequate controls and periodic proficiency testing are proposed. 相似文献
15.
Haemophilus parasuis: new trends on diagnosis, epidemiology and control 总被引:35,自引:0,他引:35
Haemophilus parasuis is a commensal organism of the upper respiratory tract of conventional pigs, but under appropriate conditions can invade and cause severe systemic disease, characterized by fibrinous polyserositis, arthritis and meningitis. Factors involved in systemic invasion by H. parasuis remain largely unknown. However, major advances in our knowledge of H. parasuis include (1) development of a species-specific PCR test to detect H. parasuis in clinical samples, (2) study of molecular epidemiology within and between herds, by use of a repetitive element-based PCR, (3) the proposal of an alternative serotyping technique, (4) development and testing of a new in vivo model for pathogenesis and virulence studies, and (5) use of controlled exposure of young pigs to low doses of live, virulent H. parasuis strains to reduce nursery mortality in affected swine herds. 相似文献
16.
A Mycoplasma bovis species-specific PCR assay has been developed with improvement of a previously described method (Ghadersohi et al., 1997). This test and its semi-nested version (Hayman and Hirst, 2003) did not function at all in our hands. A new reverse primer (Mbr2) was designed using previously published sequence data. For testing specificity, DNA was extracted from the most frequently occurring mycoplasma species and bacteria of bovine origin. The new PCR detected only Mycoplasma bovis. Moreover, no cross-reaction was observed with the genetically closest relative species, M. agalactiae. The target organism could be detected in a dose as low as 150 CFU ml(-1) in broth cultures using ethidium-bromide-stained agarose gels. 相似文献
17.
Haemophilus parasuis belongs to opportunistic microorganisms of undefined virulence. The purpose of the studies was to compare suitability of PCR/RFLP in our modification and ERIC PCR for epidemiological study of domestic strains of H. parasuis. The results were evaluated taking into account two different aspects: suitability of the tests for isolating the highest possible number of clone groups and subjective evaluation of the method judged with respect to the following criteria: difficulty, availability of equipment and reagents as well as time and cost of the study. The results obtained in the present study show that the two methods used for typing of H. parasuis had high discriminatory power. Taking into account this parameter it can be concluded that ERIC PCR is more suitable than PCR/RFLP. This justifies the use of ERIC PCR for routine epidemiological analyses of mentioned pathogen. Taking into account the complexity of method used, ERIC-PCR based on random amplification of DNA, proved to be comparable to PCR/RFLP. The last mentioned technique is relatively less expensive and labour-consuming, especially when diagnostic PCR method is used for the epidemiological studies. 相似文献
18.
《Veterinary microbiology》1998,63(1):39-48
Based on the 16S rRNA sequences of a collection of well-characterized strains of Haemophilus somnus a set of primers was selected as candidates for a species-specific PCR test. All investigated H. somnus strains were found positive in the test, including 12 strains earlier found to represent H. somnus by DNA–DNA hybridization as well as representatives of the 16 ribotypes previously described within this species. The specificity of the test was evaluated on a broad collection of strains within the family Pasteurellaceae and on other Gram positive and negative species. None of these strains gave rise to an amplicon in the PCR test. The performance of the test on mixed cultures was evaluated by adding P. multocida to serial dilutions of H. somnus and incubating the agarplates for 1 and 2 days. This showed that the PCR test applied to the harvest from an agarplate can be expected to detect a single colony of H. somnus in the presence of 109 CFU of P. multocida even after 2 days of incubation. In conclusion, the present PCR test has been shown to represent a specific test for identification of H. somnus both in pure and mixed cultures. It represents a quick, sensitive and reliable method for identification of bacteria belonging to this phenotypically heterogeneous and often slow growing species. 相似文献
19.
为了建立猪链球菌(Streptococcus suis,SS)种与9型猪链球菌(SS9)的快速诊断方法,本研究根据GenBank已登录的SS种特异性基因gdh和SS9型特异性基因CPS9H设计引物,以标准SS9株基因组DNA为模板,建立了SS种和SS9的二重PCR检测方法,并进行了特异性、敏感性和重复性试验;利用所建立的方法对检测疑似猪链球菌感染猪临床样品,并与常规细菌分离鉴定方法进行了比对。结果表明成功建立SS种和SS9型猪链球菌二重PCR检测方法,该方法的检测灵敏度可达100个CFU,特异性和重复性好;利用该方法对34份临床分离自疑似猪链球菌感染样品的细菌培养物进行了应用检测试验,其中有11份样品为gdh阳性,11份gdh阳性样品中有3份样品同时为SS9阳性。本研究成功建立了SS种与SS9型猪链球菌二重PCR检测方法,可用于猪链球菌种和SS9型猪链球菌的快速诊断。 相似文献
20.
Chiers K Van Overbeke I Donné E Baele M Ducatelle R De Baere T Haesebrouck F 《Veterinary microbiology》2001,83(2):147-159
A PCR assay for the detection of Actinobacillus pleuropneumoniae was developed based on the amplification of a dsbE-like gene. All of 157 field isolates of A. pleuropneumoniae reacted in the PCR by the amplification of a 342bp product. No reaction was observed with related bacterial species or other bacterial species isolated from pigs, except for A. lignieresii. The lower detection limit of the PCR was 10(2) CFU per PCR test tube and was not affected by the addition of 10(6) CFU Escherichia coli. The PCR was evaluated on mixed bacterial cultures from nasal and tonsillar swabs as well as suspensions of nasal conchae and tonsils obtained from specific pathogen-free (SPF) pigs, experimentally infected pigs, and pigs from farrow-to-finish herds. The results of the new PCR were compared with a PCR based on the detection of the omlA gene coding for an outer membrane protein, with a commercially available PCR (Adiavet APP, Adiagène, Saint-Brieuc, France), and with conventional culturing. No positive reactions were observed with any of the PCR methods in samples of SPF animals. In samples of the other animals, no or low significant differences between nasal swabs and suspensions as well as tonsillar swabs and suspensions were observed in any method. In general, more positive results were obtained from tonsillar samples in comparison to nasal samples. Interassay sensitivity and specificity values were assessed for each test by pair wise comparisons between assays. The agreement between tests was evaluated by calculating Cohen's kappa coefficient. From these analyses the three PCR assays showed a good agreement. The dsbE-based PCR proved to be highly sensitive (95 and 93%) and specific (82 and 74%) in comparison to the omlA-based PCR and the commercially available PCR, respectively. It was concluded that the dsbE-like gene-based PCR is a reliable diagnostic assay for demonstration of A. pleuropneumoniae. Furthermore, it was demonstrated that tonsillar swabs can be used for the detection of the pathogen in healthy carrier animals. 相似文献