Department of Integrative Biology, University of South Florida, Tampa, FL, USA.
Department of Civil & Environmental Engineering, University of South Florida, Tampa, FL, USA.
J Microbiol Methods. 2020 Aug;175:105990. doi: 10.1016/j.mimet.2020.105990. Epub 2020 Jun 27.
Steps in the global nitrogen cycle are mainly catalyzed by microorganisms. Accordingly, the activities of these microorganisms affect the health and productivity of ecosystems. Their activities are also used in wastewater treatment systems to remove reactive nitrogen compounds and prevent eutrophication events triggered by nutrient discharges. Therefore, tracking the activities of these microorganisms can provide insights into the functioning of these systems. The presence and abundance of genes encoding nitrogen-metabolizing enzymes can be traced via polymerase chain reaction (PCR); however, this requires primers that are sensitive to a heterogenous gene pool yet specific enough to the target biomarker. The ever-expanding diversity of sequences available from databases includes many sequences relevant to nitrogen metabolism that match poorly with primers previously designed to track their presence and/or abundance. This includes genes encoding ammonia monooxygenase (AMO) of ammonia oxidizing microorganisms, nitrite oxidoreductase (NXR) of nitrite oxidizing bacteria, and nitrous oxide reductase (NOS) of denitrifying bacteria. Some primers are also not designed to generate the short (~200 nucleotides) amplicons required for real-time quantitative PCR (qPCR) and reverse-transcriptase qPCR (qRT-PCR). In this study, genes collected from the Integrated Microbial Genomes database (IMG) were aligned to design PCR primers that could capture more sequence diversity than is possible using existing primers. Primers were designed to target three clades of AMO (Betaproteobacteria, Chrenarchaeota, and complete ammonia oxidizing Nitrospira), periplasmic NXR and two clades of NOS (Proteobacteria and Bacteroidetes/Firmicutes). These primers successfully amplified target sequences from two wastewater treatment plants with biological nitrogen removal (one with simultaneous nitrification/denitrification and one with distinct anoxic/oxic zones) and estuary sediment. Nucleotide sequences of the amplicons retrieved homologs when used to query GenBank by BLAST. While convincingly identified as target sequences for these primer pairs, these amplicons were divergent from each other, and quite divergent (as low as 73%) from those present in GenBank, suggesting these primers are capable of capturing a diverse range of sequences. A direct comparison showed that primers designed here are better suited to environmental samples, such as wastewater treatment facilities, by producing a greater number of amplicons from the same sample than primers currently established in literature.
全球氮循环的步骤主要由微生物催化。因此,这些微生物的活性影响着生态系统的健康和生产力。它们的活性也被用于废水处理系统中,以去除反应性氮化合物,并防止由营养物质排放引发的富营养化事件。因此,追踪这些微生物的活性可以深入了解这些系统的功能。可以通过聚合酶链反应 (PCR) 来追踪编码氮代谢酶的基因的存在和丰度;然而,这需要对异质基因库敏感且对目标生物标志物足够特异的引物。数据库中可用的序列不断扩展,其中包括许多与氮代谢相关的序列,这些序列与之前设计用于追踪其存在和/或丰度的引物匹配不佳。这包括氨氧化微生物的氨单加氧酶 (AMO)、亚硝酸盐氧化还原酶 (NXR) 的基因和反硝化细菌的亚硝酸盐还原酶 (NOS)。一些引物也不是为了生成实时定量 PCR (qPCR) 和逆转录 qPCR (qRT-PCR) 所需的短 (~200 个核苷酸) 扩增子而设计的。在这项研究中,从集成微生物基因组数据库 (IMG) 中收集的基因被用于设计 PCR 引物,这些引物可以捕获比现有引物更多的序列多样性。设计的引物针对 AMO 的三个分支 (β变形菌纲、泉古菌门和完整的氨氧化硝化螺旋菌)、周质 NXR 和 NOS 的两个分支 (变形菌门和拟杆菌门/厚壁菌门)。这些引物成功地从具有生物脱氮功能的两个废水处理厂 (一个具有同时硝化/反硝化功能,另一个具有明显的缺氧/好氧区) 和河口沉积物中扩增出目标序列。当使用 BLAST 通过 GenBank 对扩增子的核苷酸序列进行查询时,它们检索到了同源物。虽然这些扩增子被确认为这些引物对的目标序列,但它们彼此之间存在差异,并且与 GenBank 中的序列差异很大 (低至 73%),这表明这些引物能够捕获广泛的序列。直接比较表明,与目前文献中建立的引物相比,这里设计的引物更适合于废水处理厂等环境样本,因为它们可以从同一样本中产生更多的扩增子。
