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首页> 外文期刊>Journal of Virological Methods >Development of an antigen-capture ELISA for detection of H7 subtype avian influenza from experimentally infected chickens.
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Development of an antigen-capture ELISA for detection of H7 subtype avian influenza from experimentally infected chickens.

机译:抗原捕获ELISA的开发,用于从实验感染的鸡中检测H7亚型禽流感。

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摘要

Emergence of highly pathogenic avian influenza H7N1 was due to mutation of low pathogenic avian influenza H7N1 strain, which caused outbreaks in Italy between 1999 and 2000, and resulted in complete mortality of infected poultry. This outbreak places increased importance on the early detection of H7N1 AIV. Here we describe the development of a detection method for H7N1 virus from infected chickens using a specific antigen-capture-ELISA (AC-ELISA). A panel of mAbs was developed against the surface antigen HA of H7N1 AIV strain A/chicken/Singapore/94. The mAbs were screened by immunoflouorescence assays, ELISA and immunoblotting. Selected mAbs 5E5 and 8F10 were of isotypes IgM and IgG and were conformation- or linear epitope-specific, respectively. These mAbs were used as capture antibodies for AC-ELISA development. The detection limit was as little as 10(2)-10(3) TCID(50) units of virus derived from tissue culture supernatants. Virus from the tracheal swab samples of experimentally infected chickens wasdetected from days 3 to 7 post-infection using the AC-ELISA, with results being confirmed by RT-PCR. AIV subtypes H4N1, H5N3 H9N2 and H10N5 did not react in the AC-ELISA but were RT-PCR positive, indicating that this AC-ELISA is specific for H7N1 strains.
机译:高致病性禽流感H7N1的出现是由于低致病性禽流感H7N1株的突变所致,该突变在1999年至2000年间在意大利引起暴发,并导致被感染家禽完全死亡。此次爆发对H7N1 AIV的早期发现越来越重要。在这里,我们描述了一种使用特异性抗原捕获ELISA(AC-ELISA)从感染鸡中检测H7N1病毒的方法的发展。针对H7N1 AIV株A /鸡/新加坡/ 94的表面抗原HA研发了一组单克隆抗体。通过免疫荧光测定,ELISA和免疫印迹筛选mAb。选定的单克隆抗体5E5和8F10具有同型IgM和IgG,分别具有构象特异性或线性表位特异性。这些单克隆抗体用作AC-ELISA开发的捕获抗体。从组织培养上清液衍生的病毒的检出限低至10(2)-10(3)TCID(50)单位。使用AC-ELISA,从感染后第3天到第7天检测到来自实验感染鸡的气管拭子样品中的病毒,并通过RT-PCR确认了结果。 AIV亚型H4N1,H5N3,H9N2和H10N5在AC-ELISA中不发生反应,但RT-PCR呈阳性,表明该AC-ELISA对H7N1菌株具有特异性。

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