Designing specific bacterial 16S primers to sequence and quantitate plant endo-bacteriome

底漆(化妆品) 放大器 生物 聚合酶链反应 细菌 DNA测序 遗传学 16S核糖体RNA 计算生物学 DNA 基因 化学 有机化学
作者
Liying Chen,Mengting Zhang,Da Liu,Hongbo Sun,Jianxiang Wu,Yan Huo,Xiaoying Chen,Rongxiang Fang,Lili Zhang
出处
期刊:Science China-life Sciences [Springer Nature]
卷期号:65 (5): 1000-1013 被引量:30
标识
DOI:10.1007/s11427-021-1953-5
摘要

Plant endophytic bacteria colonize the internal tissues of plants and interact with plants closely. The past two decades have witnessed the increasing application of next-generation 16S rRNA gene sequencing in the investigation of bacterial communities. However, deciphering plant endo-bacterial communities by this method is difficult because of the co-amplification of massive plant organellar DNAs with bacterial 16S. Here, we designed polymerase chain reaction (PCR) primer sets, including 799F/1107R, 322F/796R, and 322F-Dr/796Rs (primer pair 322F/796R with a penultimate-base substitution in 322F), that can specifically amplify bacterial 16S from plant total DNAs. We computationally and experimentally evaluated the specificity, coverage, and accuracy of the newly designed primer sets. Both 799F/1107R and 322F-Dr/796Rs produced plant DNA-free 16S amplicon libraries or reduced plant DNA contamination to lower than 5% for the plant materials with extremely-low-abundance bacterial communities. The primer set 322F-A/796R was used through absolute quantitative PCR to quantitate the population size of rice leaf or root endo-bacteriome, which revealed 106-107 and 109-1010 bacteria per gram fresh weight, respectively. These 16S primer sets and amplification methods enable the simple and inexpensive next-generation sequencing and quantification of plant endo-bacteriome, which will significantly advance studies on the plant-related microbiome.
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