广东、四川两省规模化肉鸭养殖场病原菌调查研究

采取流行病学、临床症状、病理解剖、病原分离与墼定系列方法,对2008年5月至2008年11月之间,从广东和四川两省抽样调查的鸭病病原菌进行了研究。从2省6个市县的11个规模化养殖场,采集病死鸭头、肝等病料,接种巧克力LB平板和麦康凯培养基,共获得20株细菌。通过生化反应等系统鉴定,判为大肠杆菌的9株,占42．8％;鸭疫里默氏杆菌的11株,占57．2％。采用玻板凝集实验检测,11株鸭疫里默氏杆菌属于AF型的5株（占45．5％）、DZ型1株（占9．1％）、5株（45．5％）未能定型。     

Identification of Yersinia enterocolitica in minced meat: a comparative analysis of API 20E, Yersinia identification kit and a 16S rRNA-based PCR method

The isolation and identification of Yersinia enterocolitica from minced meat on CIN agar medium is still one of the major problems in food microbiology because of the low selectivity of cefsulodin-irgasan-novobiocin (CIN) agar. A total of 198 minced meat samples were collected from commercial establishments (butcher shops and supermarkets) in seven German cities in order to investigate the sensitivity and specificity of three identification techniques suitable for the differentiation of Y. enterocolitica within the rich background flora on CIN agar plates. As expected isolation of Y. enterocolitica from minced meat on CIN agar medium after 72 h enrichment in peptone, sorbitol and bile salts (PSB) broth was difficult because all plates were abundantly covered with numerous 'typical'Yersinia-like colonies of bull's eye appearance as well as with atypical colonies. Based on the phenotype of the colonies it was possible to detect colonies showing Yersinia-like growth on CIN agar in 52 samples (26%). For identification of Y. enterocolitica the API 20E system (bioMerieux, Nürtingen, Germany), the Yersinia identification kit (Merlin, Bornheim-Hersel, Germany) and a 16S rRNA based PCR assay were compared. Only in one sample (0.5%) a Y. enterocolitica strain was detected by all methods. Of the three identification systems tested for routine laboratory diagnostics the API 20E system was found to be the most suitable tool to identify Y. enterocolitica colonies within the rich background flora from minced meat samples on CIN agar plates.     

人工诱发鸡大肠杆菌病的接种规律

采用鸡大肠杆菌 O2标准强毒株 ,对 4 80羽宝万斯 -高兰蛋雏鸡颈部皮下注射进行人工发病 ,研究了细菌培养时间、接种量与致病力之间的关系和规律。结果表明 ,在同一毒株条件下 ,细菌致病力强弱 ,主要取决于接种感染菌数 ,只要接种菌数适宜 ,4～ 2 4 h细菌培养液均可成功发病 ,不必受普遍采用 1 8h细菌培养液接种的时间约束。这一试验结果可为灵活、合理安排抗菌新兽药试验中人工病例复制提供参考     

猪致病性链球菌的分离鉴定

采集33例临床症状疑似猪链球菌感染猪的全血及内脏器官进行涂(触)片染色镜检,取有球菌感染的样品16份进行血琼脂平板分离纯化试验;根据血琼脂平板上菌落形态、溶血情况及对单个菌落涂片染色镜检结果,共筛选出12份可疑样品,进一步采用液体培养基对12份样品进行增菌及纯化培养;选取纯化培养菌进行链球菌生化试验,结果共鉴定出11株纯化的猪链球菌;11株猪链球菌均对小鼠表现出高致病力.     

Evaluation of matrix-assisted laser desorption ionization-time of flight mass spectrometry (MALDI-TOF MS) for species identification of bacteria of genera Arcanobacterium and Trueperella

In the present study matrix-assisted laser desorption ionization-time of flight mass spectrometry (MALDI-TOF MS) was evaluated for species identification of 98 bacteria previously classified phenotypically and genotypically to genera Arcanobacterium and Trueperella. Species identification was carried out by comparing the main spectra of each strain with the main spectra of reference strains of both genera and 3740 database entries included in the MALDI Biotyper 2.0 software package (Bruker Daltonik GmbH, Bremen, Germany). MALDI-TOF MS correctly identified (log (score) values ≥ 2.0) all investigated strains of the species A. (T.) bialowiezense (n=3), A. (T.) bonasi (n=7), A. haemolyticum (n=10), A. pluranimalium (n=1) and A. (T.) pyogenes (n=77). According to the present results MALDI-TOF MS had a comparable discriminating power than previously conducted tests on DNA level. Further studies with strains isolated from human infections would show the robustness of MALDI-TOF MS for identification of bacteria of these genera.     

苜蓿根瘤菌绿色荧光蛋白标记株的构建及对菌株结瘤固氮能力的影响

以苜蓿中华根瘤菌Sinorhizobium meliloti12531,Sinorhizobium meliloti343和苜蓿根瘤菌Rhizobium meliloti GN5为受体菌,以Escherichia coli pRK2073为辅助菌及绿色荧光蛋白GFP104为供体菌,采用三亲本杂交法进行结合转导。以Winogradsky无氮培养基和TY培养基对标记菌株进行荧光表达及固氮特性的遗传稳定性检测,再对选出的荧光标记菌株以甘农5号紫花苜蓿和WL.343紫花苜蓿为宿主进行回接验证,测定了回接植物的生物量,结瘤数和标记菌的占瘤率等指标。结果表明:(1)三亲本杂交法适用于苜蓿根瘤菌GFP荧光标记菌株的构建,能以S.meliloti 343、R.meliloti GN5和S.meliloti 12531为出发菌株成功构建荧光标记菌株;(2)传代筛选后得到的荧光标记菌株中,S.meliloti 343-gfp2、R.meliloti GN5-gfp4和S.meliloti12531-gfp4遗传稳定性好,荧光表达量高;(3)含抗生素Winogradsky无氮培养基平板筛选与现有含抗生素平板分离筛选法相比,能显著提高荧光标记根瘤菌株的筛选效率;(4)获得的苜蓿根瘤菌荧光标记菌株间无显著差异,对标记菌株形成根瘤的固氮能力,及标记菌株对苜蓿植株生物量的影响进行比较,GFP荧光标记根瘤菌具有较高的遗传稳定性。     

Identification of Yersinia enterocolitica in Minced Meat: A Comparative Analysis of API 20E,Yersinia Identification Kit and a 16S rRNA‐based PCR Method

The isolation and identification of Yersinia enterocolitica from minced meat on CIN agar medium is still one of the major problems in food microbiology because of the low selectivity of cefsulodin–irgasan–novobiocin (CIN) agar. A total of 198 minced meat samples were collected from commercial establishments (butcher shops and supermarkets) in seven German cities in order to investigate the sensitivity and specificity of three identification techniques suitable for the differentiation of Y. enterocolitica within the rich background flora on CIN agar plates. As expected isolation of Y. enterocolitica from minced meat on CIN agar medium after 72 h enrichment in peptone, sorbitol and bile salts (PSB) broth was difficult because all plates were abundantly covered with numerous ‘typical’Yersinia‐like colonies of bull's eye appearance as well as with atypical colonies. Based on the phenotype of the colonies it was possible to detect colonies showing Yersinia‐like growth on CIN agar in 52 samples (26%). For identification of Y. enterocolitica the API 20E system (bioMerieux, Nürtingen, Germany), the Yersinia identification kit (Merlin, Bornheim‐Hersel, Germany) and a 16S rRNA based PCR assay were compared. Only in one sample (0.5%) a Y. enterocolitica strain was detected by all methods. Of the three identification systems tested for routine laboratory diagnostics the API 20E system was found to be the most suitable tool to identify Y. enterocolitica colonies within the rich background flora from minced meat samples on CIN agar plates.     

Antibiotic resistance among indicator bacteria isolated from healthy pigs in New Zealand

AIM: To determine the resistance to antibiotics among the indictor bacteria, Escherichia coli and Enterococcus spp, isolated from the faeces of healthy pigs on three conventional pig farms and one organic farm in the North Island of New Zealand. METHODS: Faecal samples, collected at intervals between March and October 2001, were plated onto MacConkey agar and Slanetz-Bartley agar and examined after 1-3 days incubation for colonies resembling E. coli and Enterococcus spp, respectively. Typical colonies were subcultured for further identification and storage. The isolates were tested for antibiotic resistance, using disc diffusion, to ampicillin, gentamicin, streptomycin, and tetracycline. Escherichia coli isolates were also tested for resistance to ciprofloxacin, cotrimoxazole and neomycin. Enterococcus spp isolates were also tested for resistance to vancomycin, erythromycin and virginiamycin. RESULTS: A total of 296 E. coli and 273 Enterococcus spp isolates were obtained from the three conventional farms, and 79 E. coli and 80 Enterococcus spp isolates were obtained from the organic farm. All the E. coli isolates from both the conventional and organic pig farms were susceptible to ciprofloxacin, and all the Enterococcus spp isolates were susceptible to ampicillin, gentamicin and vancomycin. Isolates of E. coli from conventional pig farms were resistant to gentamicin (0.7%), neomycin (0.7%), ampicillin (2.7%), cotrimoxazole (11%), streptomycin (25%) and tetracycline (60%). Enterococcus spp isolates from the same farms were resistant to erythromycin (68%), tetracycline (66%), streptomycin (54%) and virginiamycin (49%). By contrast, for the organic pig farm 相似文献   

牦牛大肠杆菌的分离鉴定及系统发育分析

本试验旨在研究牦牛源大肠杆菌的遗传进化关系,明确其与人和其他动物大肠杆菌的亲缘关系。采集来源于四川省甘孜州、阿坝州的60份临床健康成年牦牛肛门棉拭子样本,接种于麦康凯琼脂培养基上进行细菌的分离培养,通过常规形态学、培养特性、生化特征和16S rRNA PCR检测的研究,确定49株为大肠杆菌。对其中9株牦牛源大肠杆菌进行16S rRNA克隆、测序,经系统发育分析发现牦牛菌株组内同源性为98.8%~99.9%,与GenBank中其他菌株的同源性为94.0%~100%。结果表明,牦牛源大肠杆菌与牛源菌株的遗传距离最近,与羊源菌株的遗传距离最远,与人、猪、鸭、鸡源菌株的遗传距离较近,其中有2株菌与人肠出血性大肠杆菌(EHEC)O₁₅₇∶H₇和志贺氏菌聚为一支,从遗传进化的关系看其有可能成为人类的潜在病原菌。     

西藏牦牛大肠埃希氏菌生物学特性的研究

本文对西藏牦牛大肠埃希氏菌进行培养特性、形态染色、鞭毛检查、血凝性、生化试验、血清型鉴定、抗原性、致病性等生物学特性研究,同时用大肠埃希氏菌标准菌种C83907做对照试验.结果表明,西藏牦牛大肠埃希氏菌在普通琼脂平板上可形成光滑型和粗糙型两种类型的菌落,在5%绵羊鲜血琼脂平板上无溶血现象;具有运动性,对家兔红细胞表现出强凝集,而对牦牛、绵羊、马、鸡、猪、鸭的红细胞不凝集,能发酵大多数糖类;其0抗原血清型为026、0142、0148和0158混合型;牦牛大肠埃希氏菌的培养物对家兔具有致病性,用牦牛大肠埃希氏菌油乳剂疫苗2次免疫家兔14 d后检测抗体效价,抗体效价≥2<8>.     

Acid-induced autoagglutination found in chicken pathogenic Escherichia coli strain.

Chicken pathogenic Escherichia coli strains were found to autoagglutinate in a static culture of trypticase soy broth (TSB). One strain, designated PDI-386, was further studied for its autoagglutinating property. Acidity in the cultured medium caused by glucose degradation induced the autoagglutination. The bacterial cells grown in a glucose-free L-broth could be aggregated by adding acid, which suggests a potentiality of autoagglutination of the strain grown in the L-broth. The autoagglutinating parent (Agg) formed small colonies with irregular edges like rough colonies on the TS agar, whereas its non-autoagglutinating variant (Nag) formed larger smooth colonies with a perfectly round edge. The Nag colony was easily generated from the Agg colony on the TS agar. The autoagglutinating property was very unstable when the bacteria was passed in the TSB, but rather stable in the L-broth. Under electron microscope, the Agg were found to possess pili of more than 20 microns in length. However, the phenotypic expression of autoagglutination did not correlate with that of mannose-sensitive hemagglutination against guinea pig erythrocytes. Incubation of the Nag in the L-broth at room temperature for more than 10 days provoked the reversion of the autoagglutination. There was no difference between the Agg and the Nag in terms of surface hydrophobicity, sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) patterns of membrane proteins and LPS, and plasmid profiles. The virulence of the Agg was higher than that of the Nag. The autoagglutination property is, however, so unstable that the pathogenicity of E. coli isolates from chickens should be carefully evaluated.     

肉牛屠宰线不同工序中沙门菌和大肠杆菌污染调查及分离鉴定

为了确定肉牛屠宰线沙门菌和大肠杆菌的污染情况,选取山西省2家屠宰厂(A、B),分别在屠宰线7道不同工序和屠宰刀具上进行采样,采用传统方法进行沙门菌和大肠杆菌的分离、培养,利用生化鉴定法和16SrDNA序列分析法对分离菌株进行鉴定。结果表明:A厂所有工序均未发现沙门菌和大肠杆菌污染情况;B厂所有工序均未检测出沙门菌,但在宰前皮毛和粪便中检测到8株疑似大肠杆菌,经生化鉴定法和16SrDNA序列分析法全部确定为大肠杆菌。综上表明,选取的2个肉牛屠宰加工企业屠宰线相关工序消毒、减菌措施到位,但应注重宰前动物的规范化管理,以减少宰前污染。     

Occurrence of the temperature-sensitive hemagglutinin among avian Escherichia coli

In this study, we determined the occurrence of the tsh gene among 305 Escherichia coli isolates from chickens by means of the polymerase chain reaction and agglutination of chicken erythrocytes; 200 of those isolates were obtained from chickens with colisepticemia, 52 isolates were from lesions of cellulitis, and 53 were from feces of normal chickens. The tsh gene was found in 79 (39.5%) isolates from colisepticemia, in 10 (19%) cellulitis-derived E. coli isolates, and in two (3.8%) fecal isolates. Among the tsh+ strains, 68 (86%) isolates from colisepticemia and nine (90%) from cellulitis agglutinated chicken erythrocytes in the presence of mannose, after growing the strains on colonization factor antigen agar plates at 26 C, which confirms a correlation between mannose-resistant hemagglutination and expression of hemagglutinin Tsh. These results show, for the first time, the presence of the gene tsh in cellulitis-derived E. coli isolates; the high frequency of this gene among avian pathogenic E. coli isolates in Brazil indicates that its putative role as a virulence factor should be studied more thoroughly.     

The rapid identification of Escherichia coli using Bactident E. coli

165 (93.7%) of 175 E. coli strains isolated from various materials of different animal species were correctly identified as E. coli with help of commercially available Bactident E. coli (E. Merck, D-6100 Darmstadt). Further 52 strains of the family of Enterobacteriaceae (2x Providencia sp., 2x Salmonella sp., 7 Citrobacter sp., 9 Proteus sp., 15 Klebsiella sp., 17 Enterobacter sp.) were correctly not identified as E. coli by this test. Bactident E. coli is a suitable test for rapid identification of E. coli in veterinary bacteriology.     

一对斑马“猝死综合症”的诊断

2003年3月31日,兰州市动物园1对斑马突然暴亡,经尸体剖检和实验室检验,从采取的脏器及组织分离出大量高致病力的大肠杆菌,经中国兽医药品监察所对2株大肠杆菌血型O、K抗原鉴定,结果一株为O2和O74混合型,另一株为O6;但K抗原血清鉴定未获结果。初步确诊该对斑马死亡是高致病力的大肠杆菌所致。     

规模化猪场母猪子宫内膜炎致病菌的分离鉴定

从福建省南平市6个种猪场采集52头猪子宫内膜炎病猪子宫分泌物,分别进行致病菌分离鉴定,从52例子宫内膜炎患病母猪的活体病料中共分离细菌72株,检出率为150%。全部细菌分属为大肠杆菌、链球菌、葡萄球菌、沙门氏菌、绿脓杆菌、化脓棒状杆菌和克雷伯氏菌,分离到的细菌以大肠杆菌、链球菌和葡萄球菌占较大比例,它们分别占总检出菌株的43.0%、23.6%和16.7%。患猪中有61.5%的母猪为单一细菌感染;其它为细菌混合感染,混合感染比例,达到38.5%,其中以大肠杆菌造成的混合感染占比较高的比例,占总感染头数的28.8%。     

新生牛血清中大肠杆菌噬菌体检测方法的建立

本研究用大肠杆菌标准噬菌体株选择确定的大肠杆菌C-3000作为宿主菌,采用增殖法和噬斑法与双层琼脂平板法,对多个厂家的新生牛血清进行了大肠杆菌噬菌体检测,建立了兽用生物制品细胞培养用新生牛血清中大肠杆菌噬菌体的检测方法。     

Rapid and specific differentiation of enterotoxin-producing Escherichia coli strains from other gram-negative enteric bacteria using multiplex PCR

Enterotoxigenic Escherichia coli (ETEC) may produce heat-labile (LT) and heat-stable (STI or STII) enterotoxins. Differentiation between ETEC and other pathogenic and non-pathogenic E. coli as well as other Gram-negative bacteria responsible for induction of diarrhoea, requires isolation, biochemical identification and determination of toxins (or their genes--elt, estI, estII). A multiplex polymerase chain reaction (PCR) system for the rapid and specific detection of enterotoxin-gene-positive E. coli was developed. The primers described by other authors, specific for the universal stress protein A (UspA) of E. coli and enterotoxin genes were used and allowed a simultaneous amplification of the E. coli-specific uspA and the respective toxin genes. The specificity of this multiplex PCR system was confirmed by testing ETEC, non-ETEC and other non-E. coli bacteria. The specific 884 bp uspA gene and 280 bp (eltI), 166 bp (estI) or 278 bp (estII) amplification products were generated with the respective ETEC strains whereas no amplification was detected with non-E. coli bacteria. The multiplex PCR developed allowed the rapid and specific identification of enterotoxin-producing E. coli colonies directly grown from faecal samples of pigs with diarrhoea. The test may be used as a method for the determination of ETEC among other pathogenic groups of E. coli and other Gram-negative enteric isolates.     

Effect of pooling bovine fecal samples on the sensitivity of detection of E. coli O157:H7

To assess the effect of pooling fecal samples on the sensitivity of detection of E. coli O157:H7, 12 calves, inoculated orally with 10(8)cfu per calf of nalidixic acid resistant E. coli O157:H7, were used to provide positive fecal samples. After inoculation, calves were sampled twice weekly. Negative fecal samples were from calves at a local dairy. Samples from inoculated calves were incubated without pooling or were mixed with known negative fecal samples in a 1:4 ratio or a 2:3 ratio (positive:negative) for detection of E. coli O157:H7. Samples were enriched 6h in Gram negative broth with vancomycin, cefixime, and cefsoludin, underwent immunomagnetic separation with Dynabeads, and were plated onto sorbitol MacConkey agar with cefixime, and tellurite (SMACct). Morphologically typical colonies were plated onto blood agar, incubated overnight at 37 degrees C and an indole test was performed on each colony. Indole positives colonies were plated on SMAC agar with 20 microg/ml nalidixic acid (SMACnal). Colonies that grew on SMACnal were confirmed by O157 agglutination. Sensitivity of detection in non-pooled samples was 77%. Samples pooled 1:4 and 2:3 with negative samples were 55 and 52% sensitive, respectively. Pooling decreased sensitivity of detection for E. coli O157:H7 in bovine fecal samples (P<0.01). A deterministic binomial probability model was developed to assess the probability of detecting pens of cattle shedding E. coli O157 using a pooling protocol or individual samples. Pooling decreased sensitivity of detection at low pen prevalence compared to individual samples but was similar at high prevalence.     

Multiplex polymerase chain reaction assay for identification of enterotoxigenic Escherichia coli strains.

A multiplex polymerase chain reaction (PCR) system was developed for identification of enterotoxigenic Escherichia coli (ETEC) strains and to differentiate them from other gram negative enteric bacteria. This test simultaneously amplifies heat-labile (LTI) and heat-stable (STI and STII) toxin sequences and the E. coli-specific universal stress protein (uspA). The specificity of the method was validated by single PCR tests performed with the reference E. coli and non-E. coli strains and with bacteria isolated from pig feces. The multiplex PCR allowed the rapid and specific identification of enterotoxin-positive E. coli and may be used as a method for direct determination of ETEC and to differentiate them from other E. coli and gram-negative enteric isolates.