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一种快速、高灵敏度的基于双重嵌套 PCR 的鱼类免疫组库筛选方法。

A fast, highly sensitive double-nested PCR-based method to screen fish immunobiomes.

机构信息

Institut de Biologie Intégrative et des Systèmes (IBIS), Département de Biologie, Université Laval, Québec, QC, Canada.

出版信息

Mol Ecol Resour. 2012 Nov;12(6):1027-39. doi: 10.1111/j.1755-0998.2012.03166.x. Epub 2012 Jul 17.

Abstract

Efficient methods for constructing 16S tag amplicon libraries for pyrosequencing are needed for the rapid and thorough screening of infectious bacterial diversity from host tissue samples. Here we have developed a double-nested PCR methodology that generates 16S tag amplicon libraries from very small amounts of bacteria/host samples. This methodology was tested for 133 kidney samples from the lake whitefish Coregonus clupeaformis (Salmonidae) sampled in five different lake populations. The double-nested PCR efficiency was compared with two other PCR strategies: single primer pair amplification and simple nested PCR. The double-nested PCR was the only amplification strategy to provide highly specific amplification of bacterial DNA. The resulting 16S amplicon libraries were synthesized and pyrosequenced using 454 FLX technology to analyse the variation of pathogenic bacteria abundance. The proportion of the community sequenced was very high (Good's coverage estimator; mean = 95.4%). Furthermore, there were no significant differences of sequence coverage among samples. Finally, the occurrence of chimeric amplicons was very low. Therefore, the double-nested PCR approach provides a rapid, informative and cost-effective method for screening fish immunobiomes and most likely applicable to other low-density microbiomes as well.

摘要

需要高效的方法来构建焦磷酸测序的 16S 标签扩增子文库,以便快速、彻底地筛选宿主组织样本中的感染性细菌多样性。在这里,我们开发了一种双重嵌套 PCR 方法,可从少量细菌/宿主样本中生成 16S 标签扩增子文库。该方法已在五个不同湖泊种群中采集的 133 个湖白鲑(鲑科)肾脏样本中进行了测试。将双重嵌套 PCR 效率与另外两种 PCR 策略进行了比较:单对引物扩增和简单嵌套 PCR。只有双重嵌套 PCR 提供了细菌 DNA 的高度特异性扩增。使用 454 FLX 技术合成了所得的 16S 扩增子文库,并进行了焦磷酸测序,以分析病原菌丰度的变化。测序的群落比例非常高(Good's coverage estimator;平均值=95.4%)。此外,样品之间的序列覆盖率没有显著差异。最后,嵌合扩增子的发生率非常低。因此,双重嵌套 PCR 方法为筛选鱼类免疫生物群提供了一种快速、信息丰富且具有成本效益的方法,并且很可能适用于其他低密度微生物群。

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