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宏基因组下一代测序、桑格测序和传统培养法在临床样本中检测引起下呼吸道感染的常见病原体的比较分析

Comparative Analysis of Metagenomic Next-Generation Sequencing, Sanger Sequencing, and Conventional Culture for Detecting Common Pathogens Causing Lower Respiratory Tract Infections in Clinical Samples.

作者信息

Yi Qiaolian, Zhang Ge, Wang Tong, Li Jin, Kang Wei, Zhang Jingjia, Liu Yali, Xu Yingchun

机构信息

Department of Laboratory Medicine, Peking Union Medical College Hospital, Chinese Academy of Medical Sciences and Peking Union Medical College, Beijing 100730, China.

Graduate School, Chinese Academy of Medical Sciences and Peking Union Medical College, Beijing 100730, China.

出版信息

Microorganisms. 2025 Mar 18;13(3):682. doi: 10.3390/microorganisms13030682.

Abstract

Metagenomic next-generation sequencing (mNGS) has emerged as a revolutionary tool for infectious disease diagnostics. The necessity of mNGS in real-world clinical practice for common Lower Respiratory Tract Infections (LRTI) needs further evaluation. A total of 184 bronchoalveolar lavage fluid (BALF) samples and 322 sputa associated with LRTI were fully examined. The detection performance was compared between mNGS and standard microbiology culture, using Sanger sequencing as the reference method. 52.05% (165/317) of sputa showed identical results for all three methods. Compared to Sanger sequencing, the same results obtained by mNGS were 88.20% (284/322). In 2.80% (9/322) of cases, Sanger sequencing detected more microorganisms, while mNGS detected more in 9% (29/322) of cases. For BALF, 49.41% (85/172) of cases showed identical results for all three methods. In 91.30% (168/184) of cases, identical results were produced by both mNGS and Sanger sequencing. mNGS detected more species in 7.61% (14/184) of cases, whereas in 2.80% (2/184) instances, the Sanger sequencing detected more microorganisms than mNGS. In the 184 BALF samples, 66 samples were identified as having co-infections by mNGS, Sanger sequencing identified 64 samples, and cultures identified 22 samples. Our study demonstrates that mNGS offers a significant advantage over conventional culture methods in detecting co-infections. For common bacterial pathogens, conventional culture methods are sufficient for detection. However, mNGS provides comprehensive pathogen detection and is particularly useful for identifying rare and difficult-to-culture pathogens.

摘要

宏基因组下一代测序(mNGS)已成为传染病诊断的一项革命性工具。mNGS在常见下呼吸道感染(LRTI)的实际临床实践中的必要性需要进一步评估。对总共184份支气管肺泡灌洗液(BALF)样本和322份与LRTI相关的痰液进行了全面检测。以桑格测序作为参考方法,比较了mNGS与标准微生物培养的检测性能。52.05%(165/317)的痰液样本在三种方法下结果相同。与桑格测序相比,mNGS获得相同结果的比例为88.20%(284/322)。在2.80%(9/322)的病例中,桑格测序检测到更多微生物,而在9%(29/322)的病例中,mNGS检测到更多微生物。对于BALF样本,49.41%(85/172)的病例在三种方法下结果相同。在91.30%(168/184)的病例中,mNGS和桑格测序产生相同结果。在7.61%(14/184)的病例中,mNGS检测到更多菌种,而在2.80%(2/184)的病例中,桑格测序检测到的微生物比mNGS更多。在184份BALF样本中,mNGS鉴定出66份样本存在混合感染,桑格测序鉴定出64份样本,培养鉴定出22份样本。我们的研究表明,在检测混合感染方面,mNGS比传统培养方法具有显著优势。对于常见细菌病原体,传统培养方法足以进行检测。然而,mNGS可提供全面的病原体检测,尤其有助于识别罕见和难以培养的病原体。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/26f4/11944894/dbf8fe32eb83/microorganisms-13-00682-g001.jpg

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