贵州畜牧兽医
貴州畜牧獸醫
귀주축목수의
GUIZHOU ANIMAL SCIENCE AND VETERINARY MEDICINE
2014年
5期
1-5
,共5页
金静维%马保华%邱索平%凌彬冰%李贺%胡晓冰%曹永长%薛春宜
金靜維%馬保華%邱索平%凌彬冰%李賀%鬍曉冰%曹永長%薛春宜
금정유%마보화%구색평%릉빈빙%리하%호효빙%조영장%설춘의
口蹄疫病毒%逆转录解旋酶恒温扩增%检测
口蹄疫病毒%逆轉錄解鏇酶恆溫擴增%檢測
구제역병독%역전록해선매항온확증%검측
FMDV%RT-HAD%Detection
针对FMDV编码3D蛋白(RNA聚合酶)的保守序列设计特异性引物,利用逆转录解旋酶恒温扩增技术(Reverse Transcription helicase-dependent isothermal amplification,RT-HDA)建立了口蹄疫病毒( foot-and-mouth disease virus,FMDV)快速检测方法。该方法可在65℃下,120 min内实现对口蹄疫病毒保守序列的大量扩增。该方法可检测到0.2 ng的FMDV核酸量,比普通RT-PCR高10倍;具有极高的特异性,除了能对FMDV核酸进行扩增外,对其他临床症状与口蹄疫类似的病毒,如水泡病病毒(SVDV)、猪繁殖与呼吸综合症病毒(PRRSV)、猪瘟病毒(CSFV)、猪细小病毒(PPV)和水泡性口炎病毒( VSV)的核酸,则不能扩增出目的片段。 FMDV的RT-HDA检测方法灵敏度和特异性高,而且不需要昂贵的仪器设备,具有广阔的应用前景。
針對FMDV編碼3D蛋白(RNA聚閤酶)的保守序列設計特異性引物,利用逆轉錄解鏇酶恆溫擴增技術(Reverse Transcription helicase-dependent isothermal amplification,RT-HDA)建立瞭口蹄疫病毒( foot-and-mouth disease virus,FMDV)快速檢測方法。該方法可在65℃下,120 min內實現對口蹄疫病毒保守序列的大量擴增。該方法可檢測到0.2 ng的FMDV覈痠量,比普通RT-PCR高10倍;具有極高的特異性,除瞭能對FMDV覈痠進行擴增外,對其他臨床癥狀與口蹄疫類似的病毒,如水泡病病毒(SVDV)、豬繁殖與呼吸綜閤癥病毒(PRRSV)、豬瘟病毒(CSFV)、豬細小病毒(PPV)和水泡性口炎病毒( VSV)的覈痠,則不能擴增齣目的片段。 FMDV的RT-HDA檢測方法靈敏度和特異性高,而且不需要昂貴的儀器設備,具有廣闊的應用前景。
침대FMDV편마3D단백(RNA취합매)적보수서렬설계특이성인물,이용역전록해선매항온확증기술(Reverse Transcription helicase-dependent isothermal amplification,RT-HDA)건립료구제역병독( foot-and-mouth disease virus,FMDV)쾌속검측방법。해방법가재65℃하,120 min내실현대구제역병독보수서렬적대량확증。해방법가검측도0.2 ng적FMDV핵산량,비보통RT-PCR고10배;구유겁고적특이성,제료능대FMDV핵산진행확증외,대기타림상증상여구제역유사적병독,여수포병병독(SVDV)、저번식여호흡종합증병독(PRRSV)、저온병독(CSFV)、저세소병독(PPV)화수포성구염병독( VSV)적핵산,칙불능확증출목적편단。 FMDV적RT-HDA검측방법령민도화특이성고,이차불수요앙귀적의기설비,구유엄활적응용전경。
A rapid detection method of foot-and-mouth disease virus ( FMDV) was established based on reverse transcription helicase-dependent isothermal amplification ( RT-HAD) . Its sensitivity and specificity were assessed and compared with RT-PCR method. The results showed that target fragment of FMDV RNA could be amplified by incubating at 65℃ for 120 minutes using a pair of primers designed based on the conservative sequence of foot-and-mouth disease virus genome. The detection limit of this method was 0. 2 ng of RNA sample which was 10 fold higher than that of RT-PCR. The specificity of this method is also high. We couldn’ t detection swine vesicular disease virus( SVDV)、porcine reproductive and respiratory syndrome vi-rus ( PRRSV)、swine fever virus ( CSFV)、porcine parvo virus ( PPV) and vesicular stomatitis virus ( VSV) by this method with the primers of FMDV. RT-HDA detection method of FMDV not only has high sensitivity and specificity,but also does not require expensive equipment. These properties offer a great potential for the development of simple portable DNA diagnostic devices to be used in the field and at the point-of-care.