Department of Renewable Resources, University of Alberta, 442 Earth Sciences Building, Edmonton, AB T6G 2E3 Canada.
Plant Methods. 2015 Jun 26;11:36. doi: 10.1186/s13007-015-0079-1. eCollection 2015.
Roots of different plant species are typically morphologically indistinguishable. Of the DNA-based techniques, fluorescent amplified-fragment length polymorphisms (FAFLPs) are considered reliable, high throughput, inexpensive methods to identify roots from mixed species samples. False-negatives, however, are not uncommon and their underlying causes are poorly understood. We investigated several sources of potential biases originating in DNA extraction and amplification. Specifically, we examined the effects of sample storage, tissue, and species on DNA yield and purity, and the effects of DNA concentration and fragment size on amplification of three non-coding chloroplast regions (trnT-trnL intergenic spacer, trnL intron, and trnL-trnF intergenic spacer).
We found that sample condition, tissue and species all affected DNA yield. A single freeze-thaw reduces DNA yield, DNA yield is less for roots than shoots, and species vary in the amount of DNA yielded from extractions. The effects of template DNA concentration, species identity, and their interaction on amplicon yield differed across the three chloroplast regions tested. We found that the effect of species identity on amplicon production was generally more pronounced than that of DNA concentration. Though these factors influenced DNA yield, they likely do not have a pronounced effect on detection success of fragments and only underscore the restriction on the use of FAFLPs for measuring species presence rather than their abundance. However, for two of the regions tested-the trnT-trnL intergenic spacer and the trnL intron-size-based fragment competition occurred and the likelihood of detection was higher for smaller than larger fragments. This result reveals a methodological bias when using FAFLPs.
To avoid potential bias with the use of FAFLPs, we recommend users check for the disproportionate absence of species detected belowground versus aboveground as a function of fragment size, and explore other regions, aside from the trnT-trnL intergenic spacer and trnL intron, for amplification.
不同植物物种的根通常在形态上无法区分。在基于 DNA 的技术中,荧光扩增片段长度多态性(FAFLP)被认为是一种可靠、高通量、低成本的方法,可以从混合物种样本中鉴定根。然而,假阴性并不少见,其潜在原因也知之甚少。我们研究了几种可能源自 DNA 提取和扩增的潜在偏倚来源。具体来说,我们检查了样品储存、组织和物种对 DNA 产量和纯度的影响,以及 DNA 浓度和片段大小对三个非编码叶绿体区域(trnT-trnL 基因间间隔区、trnL 内含子和 trnL-trnF 基因间间隔区)扩增的影响。
我们发现样品条件、组织和物种都影响 DNA 产量。一次冻融会降低 DNA 产量,根的 DNA 产量低于芽,而且不同物种从提取中产生的 DNA 量也不同。模板 DNA 浓度、物种身份及其相互作用对扩增子产量的影响在测试的三个叶绿体区域中有所不同。我们发现,物种身份对扩增产物的影响通常比 DNA 浓度的影响更为显著。尽管这些因素会影响 DNA 产量,但它们不太可能对片段检测成功率产生明显影响,只是强调了 FAFLP 用于测量物种存在而不是其丰度的限制。然而,对于测试的两个区域——trnT-trnL 基因间间隔区和 trnL 内含子,基于大小的片段竞争发生,较小的片段检测到的可能性更高。这个结果揭示了使用 FAFLP 时存在方法学偏差。
为了避免使用 FAFLP 时出现潜在偏差,我们建议用户检查由于片段大小而导致的地下物种检测不足与地上物种检测不足之间的不成比例情况,并探索 trnT-trnL 基因间间隔区和 trnL 内含子以外的其他区域进行扩增。
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