針對淋巴細胞脈絡(luò)叢腦膜炎病毒(lymphocytic choriomeningitis virus���,LCMV)基因保守序列,設(shè)計特異性引物和熒光探針�����,建立了LCMV實時重組聚合酶等溫擴增(real-time recombinasepolymerase amplification�����,real-time RPA)檢測方法���。該檢測方法具有良好的特異性���,與LCMV同步檢測的其他鼠病毒均未出現(xiàn)交叉反應(yīng);該檢測方法具有與RT-PCR一樣的高敏感性���;通過對LCMV感染鼠組織樣本和LCMV陰性鼠血清樣本的檢測�����,證實建立的實時熒光RPA方法具有良好的穩(wěn)定性和可靠性����。與現(xiàn)有的核酸檢測方法相比��,該實時熒光RPA檢測方法在核酸上樣20 min內(nèi)即可判讀結(jié)果�,可滿足嚙齒類動物L(fēng)CMV快速檢疫需要。
Establishment of a Real-time RPA Method for Rapid Detection ofLymphocytic Choriomeningitis Virus
In this paper����,specificprimers and fluorescent probes were designed according to the conservativesequence of lymphocytic choriomeningitis virus(LCMV),and a real-time recombinase polymerase amplification assay(real-time RPA)was established. Resultsshowed that the specificity of the assay was good���,andno any cross reaction with other murine viruses detected by LCMV was shown. Thesensitivity of established assay was as high as the RT-PCR method. Otherwise����,based on detection of LCMV infected murine tissues and negativeserums�,the real-time RPA showed good stability andreliability. Compared with current detection methods of nucleic acids,the test results could be interpreted within 20 minutes after loadingthe nucleic buffer using the real-time RPA����,which couldsatisfy the need of rapid LCMV inspection in rodent animals.
全文下載鏈接:http://kns.cnki.net/KCMS/detail/37.1246.S.20190605.1615.042.html
當前位置: