首页> 外文期刊>Acta Virologica: International Journal >Detection of beet yellows virus by RT-PCR and immunocapture RT-PCR in Tetragonia expansa and Beta vulgaris.
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Detection of beet yellows virus by RT-PCR and immunocapture RT-PCR in Tetragonia expansa and Beta vulgaris.

机译:通过RT-PCR和免疫捕获RT-PCR检测甜菜黄斑球菌和普通贝塔甜菜黄病毒。

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摘要

Two sensitive methods, RT-PCR with phenol-extracted RNA or Triton X-100-released RNA and immunocapture RT-PCR (IR-RT-PCR) were used for the detection of Beet yellows virus (BYV) in young and old leaves of Tetragonia expansa and sugar beet (Beta vulgaris) and in sugar beet roots. Four oligonucleotide primer pairs proved suitable for the detection of BYV. The release of BYV RNA with Triton X-100 was shown to be a very effective and easy as compared to isolation of total RNA by phenol extraction with the same or higher sensitivity of subsequent PCR. Using the Triton X-100 release of RNA and IC-RT-PCR the sensitivity of detection was so high that pg amounts of BYV RNA occurring in dilutions up to 10(-6) of saps from young Tetragonia and sugar beet leaves could be detected.
机译:两种敏感的方法,即使用苯酚提取的RNA或Triton X-100释放的RNA的RT-PCR和免疫捕获RT-PCR(IR-RT-PCR)分别用于检测甜菜黄叶中的甜菜黄病毒(BYV)。扩张性的Tetragonia expansa和甜菜(Beta vulgaris)以及甜菜根中。四对寡核苷酸引物被证明适合检测BYV。与通过酚提取分离总RNA相比,使用Triton X-100释放BYV RNA非常有效且容易,与后续PCR的灵敏度相同或更高。使用Triton X-100释放的RNA和IC-RT-PCR,检测的灵敏度非常高,以至于可以检测到从小满的破壁草和甜菜叶中提取到10(-6)汁液中的稀释液中所含的pg量的BYV RNA。 。

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