Verification of a method using magnetic bead enrichment and nucleic acid extraction to improve the molecular detection of bacterial contamination in blood components

Byungjoon Na; Jinyeop Lee; Ho Eun Chang; Eunseon Park; Sojin Park; Jiyoung Lee; Sujin Oh; Dong Woo Shin; Yun Ji Hong; Kyoung Un Park

doi:10.1128/spectrum.02760-23

Verification of a method using magnetic bead enrichment and nucleic acid extraction to improve the molecular detection of bacterial contamination in blood components

Microbiol Spectr. 2024 Feb 6;12(3):e0276023. doi: 10.1128/spectrum.02760-23. Online ahead of print.

Authors

Byungjoon Na¹, Jinyeop Lee¹, Ho Eun Chang², Eunseon Park¹, Sojin Park¹, Jiyoung Lee², Sujin Oh³, Dong Woo Shin⁴, Yun Ji Hong^{3

4}, Kyoung Un Park^{3

4}

Affiliations

¹ KingoBio Inc. Research Center, Seoul, South Korea.
² PHiCS Institute, Seoul, South Korea.
³ Department of Laboratory Medicine, Seoul National University College of Medicine, Seoul, South Korea.
⁴ Department of Laboratory Medicine, Seoul National University Bundang Hospital, Seongnam, South Korea.

Abstract

Bacterial contamination of blood products poses a significant risk in transfusion medicine. Platelets are particularly vulnerable to bacterial growth because they must be stored at room temperature with constant agitation for >5 days. The limitations of bacterial detection using conventional methods, such as blood cultures and lateral flow assays, include the long detection times, low sensitivity, and the requirement for substantial volumes of blood components. To address these limitations, we assessed the performance of a bacterial enrichment technique using antibiotic-conjugated magnetic nanobeads (AcMNBs) and real-time PCR for the detection of bacterial contamination in plasma. AcMNBs successfully captured >80% of four bacterial strains, including Staphylococcus aureus, Bacillus cereus, Escherichia coli, and Klebsiella pneumoniae, in both plasma and phosphate-buffered saline. After 24-h incubation with bacterial enrichment, S. aureus and B. cereus were each detected at 10¹ CFU/mL in all trials (5/5), E. coli at 10¹ CFU/mL in 1/5 trials, and K. pneumoniae at 10² CFU/mL in 4/5 trials. Additionally, without incubation, the improvement was also achieved in samples with bacterial enrichment, S. aureus at 10² CFU/mL and B. cereus at 10¹ CFU/mL in 1/5 trials each, E. coli at 10³ CFU/mL in 3/5 trials, and K. pneumoniae at 10¹ CFU/mL in 2/5 trials. Overall, the findings from this study strongly support the superiority of bacterial enrichment in detecting low-level bacterial contamination in plasma when employing AcMNBs and PCR.IMPORTANCEThe study presents a breakthrough approach to detect bacterial contamination in plasma, a critical concern in transfusion medicine. Traditional methods, such as blood cultures and lateral flow assays, are hampered by slow detection times, low sensitivity, and the need for large blood sample volumes. Our research introduces a novel technique using antibiotic-conjugated magnetic nanobeads combined with real-time PCR, enhancing the detection of bacteria in blood products, especially platelets. This method has shown exceptional efficiency in identifying even low levels of four different species of bacteria in plasma. The ability to detect bacterial contamination rapidly and accurately is vital for ensuring the safety of blood transfusions and can significantly reduce the risk of infections transmitted through blood products. This advancement is a pivotal step in improving patient outcomes and elevating the standards of care in transfusion medicine.

Keywords: bacterial contamination; bacterial enrichment; magnetic nanobeads; platelets; real-time PCR.