中国动物检疫
中國動物檢疫
중국동물검역
CHINA ANMAL QUARANTINE
2013年
10期
57-60
,共4页
唐梦君%高玉时%张小燕%陆俊贤%施祖灏%唐修君%陈大伟
唐夢君%高玉時%張小燕%陸俊賢%施祖灝%唐脩君%陳大偉
당몽군%고옥시%장소연%륙준현%시조호%당수군%진대위
空肠弯曲杆菌%ERIC-PCR%分型
空腸彎麯桿菌%ERIC-PCR%分型
공장만곡간균%ERIC-PCR%분형
Campylobacter jejuni%ERIC-PCR%typing
目的:建立空肠弯曲杆菌肠杆菌科基因间重复一致序列PCR(ERIC-PCR)的分子分型技术,快速分析空肠弯曲杆菌指纹谱。方法本研究提取空肠弯曲杆菌ATCC33560的基因组DNA作为模板,采用对优化项目设置梯度其它条件不变的方法,对ERIC-PCR反应中的模板量、引物浓度和退火温度等进行优化,建立空肠弯曲杆菌的ERIC-PCR分型技术,并采用该技术对20株空肠弯曲杆菌的指纹图谱进行了分析。结果 ERIC-PCR反应体系中DNA模板量96ng/25μL,ERIC1、ERIC2引物浓度各0.8μmol/L,退火温度40℃时,指纹图谱条带清晰、明亮;20株空肠弯曲杆菌临床分离株ERIC-PCR指纹图谱差异较大,可在160bp~32000bp范围内出现2条~13条条带,分为14型。结论研究显示成功建立了空肠弯曲杆菌ERIC-PCR指纹图谱分型技术,应用该方法可从分子水平上对空肠弯曲杆菌基因组DNA进行快速指纹图谱分析,具有简便和快速等优点,能够为空肠弯曲杆菌流行病学调查提供科学依据。
目的:建立空腸彎麯桿菌腸桿菌科基因間重複一緻序列PCR(ERIC-PCR)的分子分型技術,快速分析空腸彎麯桿菌指紋譜。方法本研究提取空腸彎麯桿菌ATCC33560的基因組DNA作為模闆,採用對優化項目設置梯度其它條件不變的方法,對ERIC-PCR反應中的模闆量、引物濃度和退火溫度等進行優化,建立空腸彎麯桿菌的ERIC-PCR分型技術,併採用該技術對20株空腸彎麯桿菌的指紋圖譜進行瞭分析。結果 ERIC-PCR反應體繫中DNA模闆量96ng/25μL,ERIC1、ERIC2引物濃度各0.8μmol/L,退火溫度40℃時,指紋圖譜條帶清晰、明亮;20株空腸彎麯桿菌臨床分離株ERIC-PCR指紋圖譜差異較大,可在160bp~32000bp範圍內齣現2條~13條條帶,分為14型。結論研究顯示成功建立瞭空腸彎麯桿菌ERIC-PCR指紋圖譜分型技術,應用該方法可從分子水平上對空腸彎麯桿菌基因組DNA進行快速指紋圖譜分析,具有簡便和快速等優點,能夠為空腸彎麯桿菌流行病學調查提供科學依據。
목적:건립공장만곡간균장간균과기인간중복일치서렬PCR(ERIC-PCR)적분자분형기술,쾌속분석공장만곡간균지문보。방법본연구제취공장만곡간균ATCC33560적기인조DNA작위모판,채용대우화항목설치제도기타조건불변적방법,대ERIC-PCR반응중적모판량、인물농도화퇴화온도등진행우화,건립공장만곡간균적ERIC-PCR분형기술,병채용해기술대20주공장만곡간균적지문도보진행료분석。결과 ERIC-PCR반응체계중DNA모판량96ng/25μL,ERIC1、ERIC2인물농도각0.8μmol/L,퇴화온도40℃시,지문도보조대청석、명량;20주공장만곡간균림상분리주ERIC-PCR지문도보차이교대,가재160bp~32000bp범위내출현2조~13조조대,분위14형。결론연구현시성공건립료공장만곡간균ERIC-PCR지문도보분형기술,응용해방법가종분자수평상대공장만곡간균기인조DNA진행쾌속지문도보분석,구유간편화쾌속등우점,능구위공장만곡간균류행병학조사제공과학의거。
Objective To generate an efifcient enterobacterial repetitive intergenic consensus sequence (ERIC-PCR) typing and analyze molecular type of different food-borne Campylobacter jejuni.Method Genomic DNA of Campylo-bacter jejuni reference strain ATCC33560 was used as the template for PCR. Target sequences in Campylobacter jejuni genomic DNA were amplified with the primers designed according to the reference. To obtain optimum fingerprint maps,template and primer concentration of the reaction system and annealing temperature of PCR,the factors to be optimized were designed in different concentration grads and other factors were ifxed. Then 20 Campylobacter jejuni isolates were classiifed by PCR.Result The optimal concentration of template DNA was 96ng/25mL,the concentration of primers was 0.8mmol/L each primer and annealing temperature of PCR was 40 ℃.The ERIC-PCR ifngerprint maps of different isolates were different. The ampliifcation products contained 2 to 13 bands in length were ranging between 160bp and 32000bp. The 20 Campylobacter jejuni isolates were classiifed into 14 types according to ifngerprint maps. Conclusion The optimum ERIC-PCR molecular classiifcation method of Campylobacter jejuni was established. ERIC-PCR system is an efficient method for identification,typing and tracking analysis. It will be a promising method in studying molecular epidemiology of. Campylobacter jejuni.
