Babler Kristina M, Solo-Gabriele Helena M, Sharkey Mark E, Amirali Ayaaz
Department of Chemical, Environmental and Materials Engineering, University of Miami, Coral Gables, FL, USA.
Department of Medicine, University of Miami Miller School of Medicine, Miami, FL, USA.
Bio Protoc. 2025 Feb 20;15(4):e5189. doi: 10.21769/BioProtoc.5189.
Wastewater-based surveillance (WBS) can provide a wealth of information regarding the health status of communities from measurements of nucleic acids found in wastewater. Processing workflows for WBS typically include sample collection, a primary concentration step, and lysis of the microbes to release nucleic acids, followed by nucleic acid purification and molecular-based quantification. This manuscript provides workflows from beginning to end with an emphasis on filtration-based concentration approaches coupled with specific lysis and nucleic acid extraction processes. Here, two WBS processing approaches are presented, one focusing on RNA-specific pathogens and the other focused on DNA-specific pathogens found within wastewater: 1) The RNA-specific approach, employed for analyzing RNA viruses like severe acute respiratory syndrome coronavirus-2 (SARS-CoV-2) couples electronegative filtration of wastewater with the placement of the filter within a lysis buffer followed by direct RNA extraction. 2) The DNA-specific approach, employed for analyzing DNA pathogens like , uses size selection membranes during filtration, subsequently followed by a lysis buffer, bead-beating, and DNA extraction. Separate workflows for RNA versus DNA isolations have the advantage of improving the detection of the target pathogen. A novel aspect of the RNA-specific workflow is the direct extraction of nucleic acids from filter lysates, which shows enhanced recoveries, whereas the DNA-specific approach requires bead beating prior to extraction. Novelty is also provided in a new qPCR approach called Volcano 2nd Generation (V2G), which uses a polymerase capable of using RNA as a template, bypassing the reverse transcriptase step normally required for qPCR. Key features • Membrane filtration approaches for concentrating suspended solids from wastewater. After concentration, workflows are optimized for separate recovery of RNA and DNA. • Unique polymerase utilized to perform qPCR analysis, foregoing reverse transcription, for RNA. • Sample products for use with other molecular techniques (e.g., sequencing) as workflow approaches generate high-quality, concentrated nucleic acid extracts with minimal inhibitors. • Validated through COVID-19 surveillance where >1,000 samples of wastewater and >3,000 filter concentrates produced from these samples have been created and analyzed, with published results. J Biomol Tech (2023), DOI: 10.7171/3fc1f5fe.dfa8d906.
基于废水的监测(WBS)可以通过测量废水中发现的核酸来提供有关社区健康状况的丰富信息。WBS的处理流程通常包括样本采集、初步浓缩步骤以及微生物裂解以释放核酸,随后进行核酸纯化和基于分子的定量分析。本手稿提供了从始至终的工作流程,重点是基于过滤的浓缩方法以及特定的裂解和核酸提取过程。这里介绍了两种WBS处理方法,一种侧重于RNA特异性病原体,另一种侧重于废水中发现的DNA特异性病原体:1)RNA特异性方法,用于分析严重急性呼吸综合征冠状病毒2(SARS-CoV-2)等RNA病毒,将废水的负电过滤与将过滤器放置在裂解缓冲液中相结合,随后直接进行RNA提取。2)DNA特异性方法,用于分析诸如 等DNA病原体,在过滤过程中使用尺寸选择膜,随后加入裂解缓冲液、珠磨法和DNA提取。针对RNA与DNA分离的单独工作流程具有提高目标病原体检测的优势。RNA特异性工作流程的一个新颖之处是直接从过滤器裂解物中提取核酸,这显示出更高的回收率,而DNA特异性方法在提取之前需要珠磨法。一种名为火山第二代(V2G)的新型定量聚合酶链反应(qPCR)方法也具有新颖性,它使用一种能够以RNA为模板的聚合酶,绕过了qPCR通常所需的逆转录步骤。关键特性 • 用于从废水中浓缩悬浮固体的膜过滤方法。浓缩后,工作流程针对RNA和DNA的单独回收进行了优化。 • 用于对RNA进行qPCR分析的独特聚合酶,无需逆转录。 • 可用于其他分子技术(如测序)的样本产物,因为工作流程可产生高质量、浓缩的核酸提取物,且抑制剂最少。 • 通过新冠病毒监测进行了验证,已创建并分析了超过1000份废水样本以及由这些样本产生的超过3000份过滤器浓缩物,且结果已发表。《生物分子技术杂志》(2023年),DOI:10.7171/3fc1f5fe.dfa8d906 。
