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优化从模拟血液培养标本中进行牛津纳米孔非靶向鸟枪法宏基因组测序的真菌DNA提取和纯化方法。

Optimizing fungal DNA extraction and purification for Oxford Nanopore untargeted shotgun metagenomic sequencing from simulated hemoculture specimens.

作者信息

Langsiri Nattapong, Meyer Wieland, Irinyi Laszlo, Worasilchai Navaporn, Pombubpa Nuttapon, Wongsurawat Thidathip, Jenjaroenpun Piroon, Luangsa-Ard J Jennifer, Chindamporn Ariya

机构信息

Department of Microbiology, Faculty of Medicine, Chulalongkorn University, Bangkok, Thailand.

Westerdijk Fungal Biodiversity Institute, Utrecht, the Netherlands.

出版信息

mSystems. 2025 Jun 17;10(6):e0116624. doi: 10.1128/msystems.01166-24. Epub 2025 Apr 8.

Abstract

UNLABELLED

Long-read metagenomics provides a promising alternative approach to fungal identification, circumventing methodological biases, associated with DNA amplification, which is a prerequisite for DNA barcoding/metabarcoding based on the primary fungal DNA barcode (Internal Transcribed Spacer (ITS) region). However, DNA extraction for long-read sequencing-based fungal identification poses a significant challenge, as obtaining long and intact fungal DNA is imperative. Comparing different lysis methods showed that chemical lysis with CTAB/SDS generated DNA from pure fungal cultures with high yields (ranging from 11.20 ± 0.17 µg to 22.99 ± 2.22 µg depending on the species) while preserving integrity. Evaluating the efficacy of human DNA depletion protocols demonstrated an 88.73% reduction in human reads and a 99.53% increase in fungal reads compared to the untreated yeast-spiked human blood control. Evaluation of the developed DNA extraction protocol on simulated clinical hemocultures revealed that the obtained DNA sequences exceed 10 kb in length, enabling a highly efficient sequencing run with over 80% active pores. The quality of the DNA, as indicated by the 260/280 and 260/230 ratios obtained from NanoDrop spectrophotometer readings, exceeded 1.8 and 2.0, respectively. This demonstrated the great potential of the herein optimized protocol to extract high-quality fungal DNA from clinical specimens enabling long-read metagenomics sequencing.

IMPORTANCE

A novel streamlined DNA extraction protocol was developed to efficiently isolate high molecular weight fungal DNA from hemoculture samples, which is crucial for long-read sequencing applications. By eliminating the need for labor-intensive and shear-force-inducing steps, such as liquid nitrogen grinding or bead beating, the protocol is more user-friendly and better suited for clinical laboratory settings. The automation of cleanup and extraction steps further shortens the overall turnaround time to under 6 hours. Although not specifically designed for ultra-long DNA extraction, this protocol effectively supports fungal identification through Oxford Nanopore Technology (ONT) sequencing. It yields high molecular weight DNA, resulting in longer sequence fragments that improve the number of fungal reads over human reads. Future improvements, including adaptive sampling technology, could further simplify the process by reducing the need for human DNA depletion, paving the way for more automated, bioinformatics-driven workflows.

摘要

未加标签

长读长宏基因组学为真菌鉴定提供了一种有前景的替代方法,规避了与DNA扩增相关的方法学偏差,而DNA扩增是基于主要真菌DNA条形码(内转录间隔区(ITS)区域)的DNA条形码/元条形码分析的前提条件。然而,基于长读长测序的真菌鉴定的DNA提取面临重大挑战,因为获得长且完整的真菌DNA至关重要。比较不同的裂解方法表明,用CTAB/SDS进行化学裂解可从纯真菌培养物中高产获得DNA(根据物种不同,产量范围为11.20±0.17μg至22.99±2.22μg),同时保持完整性。评估人DNA去除方案的效果表明,与未处理的添加酵母的人血对照相比,人源读数减少了88.73%,真菌读数增加了99.53%。对在模拟临床血培养物上开发的DNA提取方案的评估表明,获得的DNA序列长度超过10kb,能够以超过80%的活性孔进行高效测序运行。从NanoDrop分光光度计读数获得的260/280和260/230比率表明,DNA质量分别超过1.8和2.0。这证明了本文优化方案从临床标本中提取高质量真菌DNA以实现长读长宏基因组学测序的巨大潜力。

重要性

开发了一种新颖简化的DNA提取方案,以从血培养样本中高效分离高分子量真菌DNA,这对于长读长测序应用至关重要。通过消除对劳动密集型和诱导剪切力步骤(如液氮研磨或珠磨)的需求,该方案更便于用户使用,更适合临床实验室环境。净化和提取步骤的自动化进一步将总周转时间缩短至6小时以内。尽管该方案并非专门为超长DNA提取设计,但它有效地支持通过牛津纳米孔技术(ONT)测序进行真菌鉴定。它产生高分子量DNA,从而产生更长的序列片段,提高真菌读数相对于人源读数的数量。未来的改进,包括自适应采样技术,可通过减少对人DNA去除的需求进一步简化流程,为更自动化、生物信息学驱动的工作流程铺平道路。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9aff/12172461/8009e73a8a8c/msystems.01166-24.f001.jpg

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