Composition of pathogenic microorganism in chronic osteomyelitis based on metagenomic sequencing and its application value in etiological diagnosis

Kang Zhang; Yu-Zhe Bai; Chang Liu; Shan-Shan Liu; Xin-Xin Lu; Run-Gong Yang

doi:10.1186/s12866-023-03046-x

Composition of pathogenic microorganism in chronic osteomyelitis based on metagenomic sequencing and its application value in etiological diagnosis

BMC Microbiol. 2023 Oct 28;23(1):313. doi: 10.1186/s12866-023-03046-x.

Authors

Kang Zhang^#¹, Yu-Zhe Bai^#², Chang Liu³, Shan-Shan Liu¹, Xin-Xin Lu⁴, Run-Gong Yang²

Affiliations

¹ Laboratory Medicine of Beijing Tongren Hospital affiliated to Capital Medical University, Beijing, China.
² Department of Tissue Repair and Regeneration, The First Medical Center of PLA General Hospital, Beijing, China.
³ Clinical Laboratory of Tsinghua University Hospital, Beijing, China.
⁴ Laboratory Medicine of Beijing Tongren Hospital affiliated to Capital Medical University, Beijing, China. luxinxin2009@126.com.

^# Contributed equally.

Abstract

Background: Traditionally, conventional microbiological culture methods have been used to detect pathogenic microorganisms in chronic osteomyelitis. However, these methods have been found to have a low detection rate, complicating the precise guidance of infection treatment. This study employed metagenomic next-generation sequencing (mNGS) to detect these microorganisms in chronic osteomyelitis with three main objectives: 1). Gain a deeper understanding of the composition of pathogenic microorganisms in chronic osteomyelitis. 2). Compare the microbial detection rates between mNGS and the standard culture methods used in laboratories to enhance the effectiveness of the traditional culture methods. 3). Explore the potential of mNGS in etiological diagnosis.

Methods: Fifty clinically confirmed intraoperative bone tissue samples of chronic osteomyelitis from January 2021 to December 2021 were collected and subjected to mNGS and microbiological testing, respectively. The orthopaedic surgeon combined clinical manifestations and related examinations to determine the causative pathogens.

Results: The culture method obtained 29 aerobic and parthenogenic anaerobic bacteria, 3 specific anaerobic bacteria, and 1 yeast-like fungus. Thirty-six aerobic and parthenogenic anaerobic bacteria, 11 specific anaerobic bacteria, and 1 yeast-like fungus were obtained by mNGS, and 2 Mycobacterium tuberculosis(MTB) strains were detected. However, there was no significant difference in the overall positive detection rate between mNGS and the culture method (P = 0.07), and the two were not statistically significant in detecting aerobic and partly anaerobic bacteria (P = 0.625). But, mNGS was significantly superior to culture in detecting anaerobic bacteria and Mycobacterium tuberculosis (P<0.05).

Conclusions: The mNGS method has enhanced our understanding of the distribution of pathogenic microorganisms in chronic osteomyelitis. Traditional culture methods help isolate and cultivate aerobic and facultative anaerobic bacteria, and fungi, and are also utilized for antibacterial drug sensitivity tests. However, mNGS has shown superior capabilities in detecting anaerobic bacteria, MTB, and mixed infection bacteria. This finding offers invaluable guidance for improving laboratory microbial culture and detection conditions. Hence, mNGS should be judiciously used for chronic osteomyelitis, and PCR can be implemented for certain difficult-to-culture microorganisms, such as MTB.

Keywords: Application value; Chronic osteomyelitis; Culture method; Microorganism; mNGS.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Anti-Bacterial Agents
Coinfection*
High-Throughput Nucleotide Sequencing
Humans
Metagenomics
Mycobacterium tuberculosis*
Osteomyelitis* / diagnosis
Saccharomyces cerevisiae
Sensitivity and Specificity

Substances

Anti-Bacterial Agents