Takemura Yasuyuki, Sekiguchi Yuji, Syutsubo Kazuaki, Harada Hideki, Omura Tatsuo, Li Yu-You, Kubota Kengo
Department of Civil and Environmental Engineering, Tohoku Universitygrid.69566.3a, Sendai, Miyagi, Japan.
Regional Environment Conservation Division, National Institute for Environmental Studiesgrid.140139.e, Tsukuba, Ibaraki, Japan.
Appl Environ Microbiol. 2021 Sep 28;87(20):e0116721. doi: 10.1128/AEM.01167-21. Epub 2021 Jul 28.
A method named sequence-specific capture of oligonucleotide probes (SCOPE) was developed for quantification of microbial rRNA molecules in a multiplex manner. In this method, a molecular weight cutoff membrane (MWCOM) was used for the separation of fluorescence-labeled oligonucleotide probes hybridized with rRNA from free unhybridized probes. To demonstrate proof of concept, probes targeting bacteria or archaea at different taxonomic levels were prepared and were hybridized with rRNAs. The hybridization stringency was controlled by adjusting reaction temperature and urea concentration in the mixture. Then, the mixture was filtered through the MWCOM. The rRNA and hybridized probes collected on the MWCOM were recovered and quantified using a spectrophotometer and fluorospectrometer, respectively. The method showed high accuracy in detecting specific microbial rRNA in a defined nucleic acid mixture. Furthermore, the method was capable of simultaneous detection and quantification of multiple target rRNAs in a sample with sensitivity up to a single-base mismatch. The SCOPE method was tested and benchmarked against reverse transcription-quantitative PCR (RT-qPCR) for the quantification of , , and some key methanogens in anaerobic sludge samples. It was observed that the SCOPE method produced more reliable and coherent results. Thus, the SCOPE method allows simple and rapid detection and quantification of target microbial rRNAs for environmental microbial population analysis without any need for enzymatic reactions. Microorganisms play integral roles in the Earth's ecosystem. Microbial populations and their activities significantly affect the global nutrient cycles. Quantification of key microorganisms provides important information that is required to understand their roles in the environment. Sequence-based analysis of microbial population is a powerful tool, but it provides information only on relative abundance of microorganisms. Hence, the development of a simpler and quick method for the quantification of microorganisms is necessary. To address the shortcomings of a variety of molecular methods reported so far, we developed a simple, rapid, accurate, and multiplexed microbial rRNA quantification method to evaluate the abundance of specific microbial populations in complex ecosystems. This method demonstrated high specificity, reproducibility, and applicability to such samples. The method is useful for quantitative detection of particular microbial members in the environment.
一种名为寡核苷酸探针序列特异性捕获(SCOPE)的方法被开发出来,用于以多重方式定量微生物rRNA分子。在该方法中,使用分子量截止膜(MWCOM)将与rRNA杂交的荧光标记寡核苷酸探针与游离的未杂交探针分离。为了证明概念验证,制备了针对不同分类水平的细菌或古菌的探针,并使其与rRNA杂交。通过调节混合物中的反应温度和尿素浓度来控制杂交严谨性。然后,将混合物通过MWCOM过滤。收集在MWCOM上的rRNA和杂交探针分别使用分光光度计和荧光分光光度计进行回收和定量。该方法在检测特定核酸混合物中的特定微生物rRNA时显示出高准确性。此外,该方法能够同时检测和定量样品中的多个靶标rRNA,灵敏度高达单碱基错配。针对厌氧污泥样品中的 、 和一些关键产甲烷菌的定量,对SCOPE方法进行了测试并与逆转录定量PCR(RT-qPCR)进行了比较。观察到SCOPE方法产生了更可靠和一致的结果。因此,SCOPE方法允许对目标微生物rRNA进行简单快速的检测和定量,用于环境微生物种群分析,而无需任何酶促反应。微生物在地球生态系统中发挥着不可或缺的作用。微生物种群及其活动显著影响全球养分循环。关键微生物的定量提供了理解它们在环境中作用所需的重要信息。基于序列的微生物种群分析是一种强大的工具,但它仅提供有关微生物相对丰度的信息。因此,开发一种更简单快速的微生物定量方法是必要的。为了解决迄今为止报道的各种分子方法的缺点,我们开发了一种简单、快速、准确且多重的微生物rRNA定量方法,以评估复杂生态系统中特定微生物种群的丰度。该方法在这类样品中显示出高特异性、可重复性和适用性。该方法可用于环境中特定微生物成员的定量检测。
