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山羊地方性鼻内肿瘤病毒(ENTV-2)SYBR-Green Ⅰ 实时荧光定量PCR检测方法的建立与应用

张靖鹏 江锦秀 林裕胜 游伟 刘道泉 毛坤明 江斌 胡奇林

张靖鹏,江锦秀,林裕胜,等. 山羊地方性鼻内肿瘤病毒(ENTV-2)SYBR-Green Ⅰ 实时荧光定量PCR检测方法的建立与应用 [J]. 福建农业学报,2021,36(7):779−784 doi: 10.19303/j.issn.1008-0384.2021.07.007
引用本文: 张靖鹏,江锦秀,林裕胜,等. 山羊地方性鼻内肿瘤病毒(ENTV-2)SYBR-Green Ⅰ 实时荧光定量PCR检测方法的建立与应用 [J]. 福建农业学报,2021,36(7):779−784 doi: 10.19303/j.issn.1008-0384.2021.07.007
ZHANG J P, JIANG J X, LIN Y S, et al. A SYBR-Green Ⅰ RT-qPCR Assay for Detecting Enzootic Nasal Tumor Virus in Goats [J]. Fujian Journal of Agricultural Sciences,2021,36(7):779−784 doi: 10.19303/j.issn.1008-0384.2021.07.007
Citation: ZHANG J P, JIANG J X, LIN Y S, et al. A SYBR-Green RT-qPCR Assay for Detecting Enzootic Nasal Tumor Virus in Goats [J]. Fujian Journal of Agricultural Sciences,2021,36(7):779−784 doi: 10.19303/j.issn.1008-0384.2021.07.007

山羊地方性鼻内肿瘤病毒(ENTV-2)SYBR-Green Ⅰ 实时荧光定量PCR检测方法的建立与应用

doi: 10.19303/j.issn.1008-0384.2021.07.007
基金项目: 福建省科技重大专项(2019NZ09007);福建省科技计划公益类专项(2018R1023-1)
详细信息
    作者简介:

    张靖鹏(1988−),男,硕士,研究实习员,主要从事动物传染病研究(E-mail:870063543@qq.com)

    通讯作者:

    胡奇林(1963−),男,研究员,主要从事动物传染病学和免疫学研究(E-mail:hql562713@163.com

  • 中图分类号: S 852.62

A SYBR-Green RT-qPCR Assay for Detecting Enzootic Nasal Tumor Virus in Goats

  • 摘要:   目的  建立一种快速、敏感的ENTV-2检测方法,用于ENT的早期诊断与流行病学调查。  方法  通过生物信息学的方法将ENTV-2与ENTV-1、ERVs、JSRV进行比对,寻找ENTV-2的保守序列并设计1对特异性引物,建立SYBR-Green Ⅰ 实时荧光定量PCR检测方法,对所建立的PCR反应条件进行优化,将PCR扩增产物连接T载体构建的阳性质粒作为标准品,对SYBR-Green Ⅰ 实时荧光定量PCR检测方法的特异性、敏感性和重复性进行验证。  结果  建立的检测ENTV-2 qPCR 方法标准曲线呈现良好的线性关系(R2 =0.992);该方法的特异性良好,对ENTV-2可以产生特异性扩增曲线,与ENTV-2高度同源的ERVs没有交叉反应,也无法扩增羊口疮病毒(ORFV)、绵羊肺炎支原体(Mo)、丝状支原体山羊亚种(Mmc)等常见病原;敏感性良好,最低检测限度为7.5×102 copies·μL−1,敏感性可达常规PCR检测方法的100倍;批内、批间的变异系数CV<1%,重复性良好;对81份临床样品的阳性检出率为17.3%。  结论  建立的SYBR-Green Ⅰ 实时荧光定量PCR方法特异性良好,敏感性较高,重复性良好,为山羊地方性鼻内肿瘤的早期、快速检测提供了技术支持。
  • 图  1  ENTV-2 荧光定量PCR标准曲线

    Figure  1.  Standard curve of ENTV-2 detected by SYBR-Green Ⅰ RT-qPCR

    图  2  ENTV-2荧光定量PCR熔解曲线

    Figure  2.  Melting curve of ENTV-2 detected by SYBR-Green Ⅰ RT-qPCR

    图  3  ENTV-2 SYBR Green Ⅰ qPCR的特异性

    注:1:ENTV-2; 2:羊肾1;3:羊肾2;4:羊肾3;5:羊肾4;6:羊肾5;7:山羊皮细胞;8:绵羊肺细胞;9:ORFV; 10:BCV;11:Mo;12:Mmc;13:Mccp;14:H2O。

    Figure  3.  Specificity of SYBR Green Ⅰ RT-qPCR in detecting ENTV-2

    Note: 1: ENTV-2; 2: kidney cell of goat No. 1; 3: kidney cell of goat No. 2; 4: kidney cell of goat No. 3; 5: kidney cell of goat No. 4; 6: kidney cell of goat No. 5; 7: goat skin cells; 8: sheep lung cells; 9: ORFV; 10: BCV; 11: MO; 12: Mmc; 13: Mccp; 14: H2O.

    图  4  部分临床样品检测结果

    注: 1为阳性样品,2~17均为临床样品,18为H2O。

    Figure  4.  Partial results of detection by SYBR-Green Ⅰ RT-qPCR on clinical samples

    Note: 1: positive sample; 2-7: clinical samples; 18: H2O.

    表  1  ENTV-2 荧光定量PCR的重复性

    Table  1.   Repeatability of SYBR-Green I RT-qPCR in detecting ENTV-2

    Entv阳性质粒含量/
    (copies·μL−1
    批内重复
    Intra-assay reproducibility
    批间重复
    Inter-assay reproducibility
    Ct±SDCV/%Ct±SDCV/%
    7.51×10325.25±0.150.5925.53±0.160.63
    7.51×10518.78±0.110.5819.11±0.170.89
    7.51×10712.44±0.120.9612.89±0.120.93
    下载: 导出CSV

    表  2  SYBR Green I荧光定量PCR和传统PCR法临床样品检测ENTV-2结果比较

    Table  2.   Detections by SYBR-Green Ⅰ RT-qPCR and conventional PCR on clinical samples

    检测方法
    Detecting method
    荧光定量PCR
    SYBR-Green Ⅰ qPCR
    总计
    Sum
    阳性数量
    Positive
    number
    阴性数量
    Negative
    number
    常规PCR
    Convenional PCR
    阳性数量
    Positive number
    10 0 10
    阴性数量
    Negative number
    46771
    总计 Sum146781
    下载: 导出CSV
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出版历程
  • 收稿日期:  2020-12-04
  • 修回日期:  2021-03-25
  • 网络出版日期:  2021-07-13
  • 刊出日期:  2021-07-28

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