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本文对延边部分地区送检的病死猪、疑似大肠杆菌感染的腹泻病猪采集病料,分别接种在营养琼脂平板、麦康凯琼脂培养基、伊红美兰培养基上,进行分离培养及纯培养,对可疑菌落革兰氏染色,涂片镜检。对初步鉴定的细菌进行生化试验及血清型鉴定。结果从48份样本中,共分离出符合大肠杆菌生长特性的菌株40株。将培养后的40株大肠杆菌菌液分别接种小鼠。结果表明,其中36株为高致病性大肠杆菌、4株呈低致病性。本试验验中对分离得到的大肠杆菌菌株进行血清型分型,结果共分离出37个血清型。其中O6(4/37),O78(5/37)、O90(7/37)、O107(7/37)为优势血清型。 相似文献
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奶水牛牛分枝杆菌的分离与鉴定 总被引:1,自引:1,他引:1
从患疑似结核病的广西奶水牛群中进行牛分枝杆菌的分离和鉴定。共收集了238份临床样品(鼻黏液及牛奶),病料经1.25 mol/mL NaOH溶液预处理后,接种罗氏培养基进行细菌分离。分离菌经进一步纯化后进行抗酸性染色并镜检,镜检后判为阳性的细菌再接种到鉴别培养基上进行鉴别培养,同时,应用PCR方法对镜检为阳性的细菌进行进一步的鉴别检验。结果收集的所有临床样品,经37℃培养后共获得细菌12株。这12株菌经抗酸性染色后镜检都为分枝杆菌阳性,进一步经鉴别培养基鉴定12株菌中有2株为牛分枝杆菌,其余均为非典型分枝杆菌。2株牛分枝杆菌经PCR方法鉴定得以确诊。 相似文献
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《云南畜牧兽医》2016,(2)
巍山县某山羊养殖户,出生15 d内的羔羊出现共济失调等神经症状,死亡率高达85%。样品经阿卡班(AKA)、山羊病毒性关节炎-脑炎(CAE)、梅迪-威斯纳病(MV)、蓝舌病(BTV)real-time PCR及普通PCR检测均为阴性。样品(脑组织)划线接种于5%的绵羊血琼脂、营养琼脂及麦康凯琼脂培养基上,37℃培养24 h。结果:在5%的绵羊血琼脂、营养琼脂平板上生长出直径2~3 mm、稍凸、圆形、湿润、灰白色、边缘整齐、不透明的菌落;在麦康凯琼脂平板上菌落呈粉红色。经革兰氏染色镜检、细菌生化鉴定为大肠埃希氏菌,血清型鉴定为O78型。昆明小白鼠致病性试验显示,致病性较强,实验组25只小白鼠接种后48 h内全部死亡,并从死亡小白鼠肝脏和心血内成功回收到该株细菌。 相似文献
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《中国家禽》2017,(10)
从扬州大学动物医院收集送检病鸡的病料,无菌采集病死鸡的肝脏、肺脏等组织接种于麦康凯平板和血琼脂平板上进行细菌分离与培养,并对分离菌进行生化试验、16 S r RNA基因序列分析和荚膜分型PCR鉴定,同时用12种抗菌药物对分离菌株进行药敏试验。细菌分离结果显示,分离菌在麦康凯平板上未见菌落生长,在血琼脂平板上呈光滑、湿润的露滴样小菌落;革兰氏染色镜检结果为革兰氏阴性小杆菌,瑞氏染色镜检可见大量两极浓染的短杆菌;生化试验结果表明分离菌株能够发酵葡萄糖、果糖、蔗糖等糖类,不能发酵乳糖和麦芽糖;同时,16 S r RNA基因序列和荚膜分型PCR测定结果显示分离菌为荚膜A型多杀性巴氏杆菌。药敏试验结果表明,分离菌株对痢特灵、左氟沙星、强力霉素的敏感性较高,而对氯霉素、美洛西林、卡那霉素等高度耐药。 相似文献
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采集关节肿胀、关节囊内有浆液性渗出物患病鸡肝脏及骨髓进行细菌分离,对分离菌进行形态学观察、革兰氏染色、生理生化试验、PCR鉴定、16S rDNA序列测定和药敏试验。结果从病鸡样品中分离出一株在普通琼脂平板上形成湿润、表面光滑、隆起的圆形菌落,菌落在血琼脂平板上能产生β溶血;分离菌为革兰氏阳性,符合金黄色葡萄球菌生化培养特性;PCR检测结果显示金黄色葡萄球菌的耐热核酸酶基因呈阳性,细菌16S rDNA核酸序列Blast比对结果显示为金黄色葡萄球菌;分离菌对阿莫西林、四环素、青霉素G、氯霉素、复方新诺明和氨苄西林具有耐药性。结果为云南鸡源金黄色葡萄球菌病的临床诊断和防治提供了依据。 相似文献
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《青海畜牧兽医杂志》2021,51(5)
从发生腺疫的青海毛驴中采集样品进行染色镜检、分离纯化、PCR鉴定,并对纯化后的菌株进行药敏试验。研究结果表明:美兰染色结果观察到长链状球菌; 5%绵羊血平板培养出现透明的露珠样小菌落,且呈现β型溶血; PCR鉴定为马链球菌马亚种;药敏试验表明马链球菌马亚种对β内酰胺类抗生素敏感。 相似文献
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【目的】了解西藏拉萨地区牦牛链球菌的感染情况、致病性及其耐药性,为牦牛源链球菌的研究提供新的数据。【方法】对55份牦牛鼻拭子进行细菌分离培养、菌落形态观察、革兰氏染色镜检、生化鉴定、16S rRNA序列PCR扩增以鉴定分离菌的种属特性。通过人工感染试验小鼠评价分离菌的致病性,采用药敏纸片扩散法检测分离菌的耐药性。【结果】分离菌在血平板上长出灰白色、表面光滑的α溶血圆形菌落,革兰氏染色镜检呈链状排列的阳性球菌。分离菌可发酵葡萄糖、乳糖、海藻糖和山梨醇,不发酵麦芽糖和甘油,硝酸盐还原试验、靛基质试验、V-P试验和MR试验均呈阴性。经16S rRNA基因序列比对分析,确定有25株链球菌(Tibet-1~Tibet-25),检出率为45.46%(25/55),其中17株多动物链球菌,8株马链球菌。分离菌16S rRNA基因序列与NCBI上已发布的链球菌相似性在97.04%~99.77%之间,其中Tibet-1、Tibet-2、Tibet-3、Tibet-5、Tibet-9、Tibet-10、Tibet-11、Tibet-14、Tibet-15、Tibet-16、Tibet-17共11株牦牛源多... 相似文献
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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
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猪附红细胞体PCR诊断方法的建立及应用 总被引:1,自引:0,他引:1
根据基因库中已登录的猪附红细胞体新的基因组DNA序列设计引物,从疑似猪附红细胞体(Mycoplasma suis)感染猪全血样品基因组DNA中扩增出了预期长度666 bp的目的DNA片段,通过对24份临床疑似病例样品的PCR扩增及其他病原微生物基因组DNA的特异性扩增试验,建立了E.suis的PCR诊断方法;进一步对PCR产物克隆、测序分析表明,与国外已报道的AJ504999株相关区域核苷酸、氨基酸序列同源性分别为98.19%和96.85%,表明我国分离株与国外株基因组存在差异。 相似文献
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上海地区31株2型猪链球菌的分离鉴定及其耐药性分析 总被引:1,自引:0,他引:1
猪链球菌病是由猪链球菌引起的一种重要人畜共患病,尤其是猪链球菌2型,不仅对猪的致病性最强,而目可感染特定人群并致死,给人类公共卫生和养猪业带来巨大影响。本研究采集临床症状疑似2型猪链球菌感染猪的全血及内脏器官,通过观察菌落形态及培养特征,筛选出可疑样品,纯化培养并进行PCR鉴定,筛选到31株2型猪链球菌,最后用纸片扩散法对临床分离到的2型猪链球菌菌株测定其耐药性,结果显示对5种药物耐药率分别为:80%(AM)、68%(GM)、84%(CHL)、52%(SXT)、55%(CIP)。试验结果表明分离的31株2型猪源性链球菌,均为多重耐药株,且青霉素类药物的耐药性较为严重,这为临床在治疗2型猪链球菌病提供了合理的指导作用。 相似文献
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通过细胞培养板法研究了猪链球菌2型生物被膜的生物学特性。结果显示:大部分猪链球菌均具有不同程度形成生物被膜的能力,其中3株(3/15)形成能力较强;猪链球菌生物被膜的成熟约需60 h,培养基中葡萄糖浓度是影响生物被膜形成的重要因素;生物被膜中的多糖含量显著高于浮游菌;氨苄青霉素钠和阿莫西林对这3株猪链球菌生物被膜的最低抑菌浓度(MIC)和最低杀菌浓度(MBC)均高于游离菌约2 500倍;扫描电镜观察发现,生物被膜内猪链球菌彼此黏连,形成致密的三维立体结构。对猪链球菌生物被膜生物学特性的研究为进一步揭示生物被膜的形成机制、耐药机理,以及清除生物被膜等提供理论依据。 相似文献
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Detection of virulent strains of Streptococcus suis type 2 and highly virulent strains of Streptococcus suis type 1 in tonsillar specimens of pigs by PCR. 总被引:17,自引:0,他引:17
H J Wisselink F H Reek U Vecht N Stockhofe-Zurwieden M A Smits H E Smith 《Veterinary microbiology》1999,67(2):143-157
We developed a PCR assay for the rapid and sensitive detection of virulent Streptococcus suis type 2 and highly virulent S. suis type 1 in tonsillar specimens from pigs. The PCR primers were based on the sequence of the gene encoding the EF-protein of virulent S. suis type 2 strains (MRP+EF+) and highly virulent S. suis type 1 strains (MRP(s)EF+) and of the EF protein of weakly virulent S. suis type 2 strains (MRP+EF). The latter strains give rise to larger PCR products than the virulent strains of S. suis type 1 and 2. A positive control template was included in the assay to identify false negative results. The PCR was evaluated using tonsillar specimens from herds known (or suspected) to be infected and herds without an S. suis history. The results obtained with the PCR assay were compared with the results obtained with a newly developed bacteriological examination. In this bacteriological examination we were able to identify the EF-positive strains directly in the tonsillar specimens. From the 99 tonsils examined, 48 were positive in the PCR and 51 negative. All specimens from which EF-positive S. suis strains were isolated were also positive in the PCR assay. Three samples were positive in the PCR, but negative by bacteriological examination. The results demonstrated that the PCR is a highly specific and sensitive diagnostic tool for the detection of pigs carrying virulent strains of S. suis type 2 and highly virulent strains of type 1. Application of the assay may contribute to the control of S. suis infections. 相似文献
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Streptococcus suis isolated from pigs in Finland 总被引:6,自引:0,他引:6
A total of 58 Streptococcus suis strains were isolated from deceased pigs submitted to the National Veterinary Institute, Regional Laboratory in Kuopio, Finland, over a 3 1/2 year period, most frequently from cases of pneumonia. The bacteria were isolated from cases of meningitis, sepsis, rhinitis, endocarditis and abortion. S. suis was also isolated from nasal cavity, lung and brain of some sick piglets without signs of inflammation. Further S. suis was detected in 12 out of 107 tonsils of healthy fatteners tested. S. suis strains were identified by biochemical methods followed by typing. The most common capsular types were 7, 3 and 2, respectively. Only one type 1 strain and no types 6 and 9 strains were found. All S. suis strains tested were sensitive to penicillin and ampicillin.S. suis is not uncommon in Finnish pig herds. S. suis may be regarded as a potentially pathogenic organism which under certain predisposing conditions may cause serious disease. 相似文献
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为了解9型猪链球菌广东分离株毒力因子基因型、基因变异和进化情况,本试验采集发病猪脑脊液、关节液、脾脏、肝脏、淋巴结进行细菌分离培养和生化鉴定,采用PCR方法鉴定其血清型及部分毒力基因,对cps9D、gdh、gapdh与orf2基因进行序列测定和分析,并构建系统发育树。结果显示,分离菌镜检为革兰氏阳性链状球菌,在鲜血琼脂平板中呈β溶血,可发酵大多数糖类,能成功扩增cps9D基因,含重要的保守基因gdh及毒力基因gapdh和orf2,表明分离菌株为9型猪链球菌。分离菌株cps9D、gdh、gapdh、orf2基因核苷酸序列与GenBank上国内外参考菌株的同源性分别为95.9%~100.0%、98.6%~99.8%、98.7%~99.6%和95.5%~99.9%,说明分离菌株与国内外其他9型猪链球菌毒株核苷酸同源性都较高,且与国内外的流行毒株基本一致,未发生太大的变异。系统发育树表明,分离株与国内外来源不同的猪链球菌分离株同源性高,亲缘关系密切。 相似文献
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To investigate the epidemics of Streptococcus suis in Guangdong province, 228 samples from infected pigs,and 698 samples from healthy pigs including 243 samples from tonsils of slaughtered pigs and 455 nasal swabs of healthy pigs were analyzed.The results showed that the positive rate of Streptococcus suis of infected,healthy and slaughtered pigs were 82.02%(187/228),42.20%(192/455) and 32.10%(78/243),respectively.187 strains of Streptococcus suis were isolated from infected pigs and serotyped in 11 serotypes,including serotype SS1,SS2,SS3,SS4,SS7,SS8,SS9,SS16,SS19,SS29 and SS31, in which serotype SS2(16.58%),SS3(9.63%) and SS19 (7.49%) were dominant,flowed by SS7(6.95%)and SS9(5.34%),and 48.66% strains were non-typabled.Meanwhile,154 strains of Streptococcus suis from healthy swine(including farms and slaughter houses) were classified into 17 serotypes,including serotype SS2,SS3,SS4,SS5,SS7,SS8,SS9,SS10,SS12,SS15,SS16,SS17,SS19,SS21,SS23,SS29 and SS30,in which SS2(18.83%) and SS29(14.94%)were dominant,flowed by SS16(6.50%) and 31.82% strains were non-typabled. 相似文献