Molecular detection of oprL gene in Pseudomonas aeruginosa associated with surgical site infections in Bauchi, Nigeria

Molecular detection of oprL gene in Pseudomonas aeruginosa associated with surgical site infections in Bauchi, Nigeria

Background: Pseudomonas  aeruginosa  (P. aeruginosa) associated with surgical site infections (SSIs) is often multidrug-resistant and associated with delayed wound healing, morbidity, and deaths. Molecular detection of P. aeruginosa is often required for specific diagnosis for optimal care. Although...

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Bibliographic Details
Main Authors: Titus Onyi, Hassan DOKO, ELIJAH ELLA
Format: Article
Language:English
Published: Zagazig University, Faculty of Medicine 2025-08-01
Series:Microbes and Infectious Diseases
Subjects:
pseudomonas aeruginosa
surgical site infections
oprl gene
polymerase chain reaction
pcr
Online Access:https://mid.journals.ekb.eg/article_353189_8f24c66a5e40a87ee49fba96fcbf4bcf.pdf
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Summary:Background: Pseudomonas  aeruginosa  (P. aeruginosa) associated with surgical site infections (SSIs) is often multidrug-resistant and associated with delayed wound healing, morbidity, and deaths. Molecular detection of P. aeruginosa is often required for specific diagnosis for optimal care. Although SSIs are prevalent in North-East Nigeria, there is a lack of studies on molecular confirmation targeting virulence genes. This study aimed to isolate and characterize P. aeruginosa isolates from surgical wound swabs and then confirm them with PCR assay with the oprL target gene. Methods: The study was a cross-sectional study that analyzed 250 post-surgical wound swabs  (n = 250) from two hospitals in Bauchi State, Nigeria. The inclusion criteria include fever and purulent pus from the incision site within 30 days of surgery. The conventional analyses were bacterial colonial morphology on Cetrimide agar, Gram staining, and biochemical characterization. The PCR assay was conducted with oprL as the target gene. Results: aeruginosa was serially identified in 5 out of 250 swabs, with a prevalence of 2.0%. All the isolates had the oprL gene with an amplicon size of 504 bp. Conclusion: The prevalence of Pseudomonas aeruginosa isolates associated with SSIs was 2.0% from the traditional assays. The PCR assay of the isolates detected the oprL gene in all the isolates. The study confirms the increasing evidence of the specificity of the oprL  virulence factor for detecting Pseudomonas aeruginosa. associated with SSIs.It also recommends further studies on the   antibiogram assays associated with P.aeruginosa with the oprL gene  to optimize the treatment of SSIs.
ISSN:2682-4132
2682-4140

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