中国动物检疫
中國動物檢疫
중국동물검역
CHINA ANMAL QUARANTINE
2012年
4期
32-36
,共5页
曹军平%胡新岗%吴双%胡顺林%赵国%王晓泉%刘晓文%陈长春%刘秀梵
曹軍平%鬍新崗%吳雙%鬍順林%趙國%王曉泉%劉曉文%陳長春%劉秀梵
조군평%호신강%오쌍%호순림%조국%왕효천%류효문%진장춘%류수범
新城疫病毒%中、强毒株%荧光定量RT-PCR%建立%验证
新城疫病毒%中、彊毒株%熒光定量RT-PCR%建立%驗證
신성역병독%중、강독주%형광정량RT-PCR%건립%험증
Newcastle disease virus%mesogenic and virulent strains%RRT-PCR%development%validation
根据新城疫病毒F基因的裂解位点序列,设计合成一对引物和TaqMan探针,以本室构建并保存的鹅源新城疫病毒ZJ1株F基因阳性重组质粒作为中、强毒力新城疫病毒RNA定量检测的标准品,建立检测方法。结果表明本试验建立的标准曲线循环阈值(Ct值)与模板浓度具有良好的线性关系,相关系数为0.999,灵敏度约为3拷贝/μL,对禽流感病毒和其他禽病病毒无交叉反应,特异性好、重复性佳,为中、强毒力新城疫病毒检测提供了一种快速高效的定量检测方法。对28株标准分离株强弱毒力的检测与经典病毒分离方法符合率达100%,对187份临床样品的检测,二者结果符合率接近90.0%。在新城疫病毒临床样品快速检测、流行病学监测等方面显示良好的应用前景。
根據新城疫病毒F基因的裂解位點序列,設計閤成一對引物和TaqMan探針,以本室構建併保存的鵝源新城疫病毒ZJ1株F基因暘性重組質粒作為中、彊毒力新城疫病毒RNA定量檢測的標準品,建立檢測方法。結果錶明本試驗建立的標準麯線循環閾值(Ct值)與模闆濃度具有良好的線性關繫,相關繫數為0.999,靈敏度約為3拷貝/μL,對禽流感病毒和其他禽病病毒無交扠反應,特異性好、重複性佳,為中、彊毒力新城疫病毒檢測提供瞭一種快速高效的定量檢測方法。對28株標準分離株彊弱毒力的檢測與經典病毒分離方法符閤率達100%,對187份臨床樣品的檢測,二者結果符閤率接近90.0%。在新城疫病毒臨床樣品快速檢測、流行病學鑑測等方麵顯示良好的應用前景。
근거신성역병독F기인적렬해위점서렬,설계합성일대인물화TaqMan탐침,이본실구건병보존적아원신성역병독ZJ1주F기인양성중조질립작위중、강독력신성역병독RNA정량검측적표준품,건립검측방법。결과표명본시험건립적표준곡선순배역치(Ct치)여모판농도구유량호적선성관계,상관계수위0.999,령민도약위3고패/μL,대금류감병독화기타금병병독무교차반응,특이성호、중복성가,위중、강독력신성역병독검측제공료일충쾌속고효적정량검측방법。대28주표준분리주강약독력적검측여경전병독분리방법부합솔체100%,대187빈림상양품적검측,이자결과부합솔접근90.0%。재신성역병독림상양품쾌속검측、류행병학감측등방면현시량호적응용전경。
According to the cleavge site sequence of Newcastle disease virus(NDV) F gene, a pair of primers and a T aqMan probe were designed and synthesized. A serial 10 fold dilutions positive plasmid was prepared and used for standard. The standard curve revealed the linear relationship between CT (cycle threshold) and template concentration with a good correlation (R2=0.999). The RRT-PCR method was highly specific and sensitive and could be used for rapid quantitative detection of mesogenic and virulent NDV. No cross-reaction was detected against other avian disease viruses. Sensitivity was 3 copies ofNDV genome. The total meet rate with traditional virus isolation method was about 90.0% in detecting 187 clinical samples as well as 100% in 28 standard isolated strains. It showed that a real-time RT- PCR method for quick, specific sensitive and quantitativedetection of mesogenic and virulent NDV had been established in this study and it displayed good prospects in the rapid screening of clinical samples and epidemiological monitoring of NDV.
