西北民族大学学报:自然科学版
西北民族大學學報:自然科學版
서북민족대학학보:자연과학판
Journal of Northwest Minorities University:Natural Science Edition
2012年
1期
47-52
,共6页
李倬%田镔%李明生%平玲
李倬%田鑌%李明生%平玲
리탁%전빈%리명생%평령
牛病毒性腹泻病毒%反转录聚合酶链反应%建立%应用
牛病毒性腹瀉病毒%反轉錄聚閤酶鏈反應%建立%應用
우병독성복사병독%반전록취합매련반응%건립%응용
Bovine viral diarrhea virus%RT - PCR%Establishment%Application
根据GenBank中登录的牛病毒性腹泻病毒(BVDV)5'非编码区基因序列,设计合成了1对特异性引物,建立了检测BVDV的反转录PCR快速检测方法.通过对该方法的特异性、敏感性和重复性进行试验,结果显示,该方法从BVDV标准毒株Oregon C24V中扩增出267 bp的特异性片段,该方法重复性好,反应批内检测结果相同.与牛轮状病毒、牛冠状病毒、猪瘟病毒和F4新生牛肾传代正常细胞无交叉反应,具有高度的特异性,而且敏感性高,最低检出限为10~1.84 TCID50/mL.利用该方法对42份临床腹泻病牛疑似粪便样品进行了检测,结果检出7份阳性,而同时利用IDEXX公司抗原检测试剂盒检出阳性只有6份.表明,建立的该方法具有快速、敏感、特异等优点,是牛病毒性腹泻病毒病的临床诊断和流行病学调查的有力工具.
根據GenBank中登錄的牛病毒性腹瀉病毒(BVDV)5'非編碼區基因序列,設計閤成瞭1對特異性引物,建立瞭檢測BVDV的反轉錄PCR快速檢測方法.通過對該方法的特異性、敏感性和重複性進行試驗,結果顯示,該方法從BVDV標準毒株Oregon C24V中擴增齣267 bp的特異性片段,該方法重複性好,反應批內檢測結果相同.與牛輪狀病毒、牛冠狀病毒、豬瘟病毒和F4新生牛腎傳代正常細胞無交扠反應,具有高度的特異性,而且敏感性高,最低檢齣限為10~1.84 TCID50/mL.利用該方法對42份臨床腹瀉病牛疑似糞便樣品進行瞭檢測,結果檢齣7份暘性,而同時利用IDEXX公司抗原檢測試劑盒檢齣暘性隻有6份.錶明,建立的該方法具有快速、敏感、特異等優點,是牛病毒性腹瀉病毒病的臨床診斷和流行病學調查的有力工具.
근거GenBank중등록적우병독성복사병독(BVDV)5'비편마구기인서렬,설계합성료1대특이성인물,건립료검측BVDV적반전록PCR쾌속검측방법.통과대해방법적특이성、민감성화중복성진행시험,결과현시,해방법종BVDV표준독주Oregon C24V중확증출267 bp적특이성편단,해방법중복성호,반응비내검측결과상동.여우륜상병독、우관상병독、저온병독화F4신생우신전대정상세포무교차반응,구유고도적특이성,이차민감성고,최저검출한위10~1.84 TCID50/mL.이용해방법대42빈림상복사병우의사분편양품진행료검측,결과검출7빈양성,이동시이용IDEXX공사항원검측시제합검출양성지유6빈.표명,건립적해방법구유쾌속、민감、특이등우점,시우병독성복사병독병적림상진단화류행병학조사적유력공구.
A reverse transcription- coupled PCR(RT- PCR) assay for quick detection of bovine viral diarrhea virus(BVDV) was established using a pair of specific primers based on the 5"UTR gene of BVDV published in GenBank. The results showed that this method could specifically amplify a 267 bp fragment from BVDV Oregon C24 V strain, reproducibility of this assay were reliable and the results were fully consistent. The specificity test proved that this assay had a high specificity which had no cross- reaction with bovine rotavirus, bovine coronavirus, classical swine fever virus and normal F4 NBPC cells. The assay also had good sensitivity, and the detection limit was up to 10-- 1.84 TCID50/mL. 7 positive of 42 samples from clinical diarrhea bovine were detected by RT- PCR and only 6 positive were detected by IDEXX diagnostic kit test at the same time. The results revealed that established RT - PCR assay possessed some advantages such as fast, sensitive and specific. It may be used for clinical diagnosis and the epidemiologic survey of bovine viral diarrhea/mucosal disease as a powerful tool.
