為探索適合臨床高通量雞傳染性喉氣管炎檢測的方法���,針對雞傳染性喉氣管炎病毒gB基因序列保守區(qū)域����,篩選1對特異性引物和1條特異性探針�����,建立了實(shí)時(shí)熒光PCR檢測方法,并對該方法進(jìn)行特異性�����、敏感性評估和臨床應(yīng)用檢測����。結(jié)果顯示:篩選出的引物和探針與其他禽類常見病毒無交叉反應(yīng)�����,檢測下限達(dá)到100拷貝/反應(yīng)�����;對來自13個(gè)場的480份臨床樣本進(jìn)行檢測���,檢測出17個(gè)陽性樣品��,與常規(guī)PCR檢測結(jié)果符合率為100%�����。結(jié)果表明�,此方法特異性強(qiáng)���,靈敏度高��、耗時(shí)少���,可用于雞傳染性喉氣管炎的快速檢測��。
Establishment and Application of a Real-time PCR for Detecting Infectious Laryngotracheitis Virus
In order to develop an appropriate method for high-throughput detection of avian infectious laryngotracheitis(AILT)��,a real-time PCR assay was established with a pair of specific primers and a probe based on the conservative zone of gB gene sequence of AILT�����,then its specificity and sensitivity were evaluated�����,and its clinical application was tested. The results showed that the selected primers and probe failed to cross-react with other common poultry viruses�,with the detection limit of 100 copies/reaction. 17 out of 480 clinical samples collected from 13 farms were positive. The results completely conformed to the test result by common PCR assay. As a conclusion�,AILT could be rapidly detected by the established method with high specificity,high sensitivity and less time-consuming.
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