Intraoral human herpes viruses detectable by PCR in majority of patients

Objectives To identify factors which influence the intraoral prevalence of human herpes viruses (HHVs) using mucosal swabs, saliva samples and qPCR analysis. Methodology In this cross‐sectional observational study, matched saliva and oral swabs were collected from a total of 115 subjects: 70 immunoc...

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Veröffentlicht in:Oral diseases 2021-03, Vol.27 (2), p.378-387
Hauptverfasser: Yap, Tami, Khor, Shuan, Kim, Jung Seo, Kim, Jaeyoung, Kim, Sung Yun, Kern, Johannes S., Martyres, Raymond, Varigos, George, Chan, Hiu Tat, McCullough, Michael J., Thomas, Melissa L, Scardamaglia, Laura
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Sprache:eng
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Zusammenfassung:Objectives To identify factors which influence the intraoral prevalence of human herpes viruses (HHVs) using mucosal swabs, saliva samples and qPCR analysis. Methodology In this cross‐sectional observational study, matched saliva and oral swabs were collected from a total of 115 subjects: 70 immunocompetent subjects with no mucosal abnormalities, 22 with mucosal abnormalities and 23 therapeutically immunocompromised individuals. Extracted DNA was analysed by multiplex qPCR for detection and quantification of HHVs 1–6. Results At least one human herpes virus was detected in 77.1% of immunocompetent individuals with no mucosal abnormalities, with EBV the most commonly detected at 61.4%. HHV‐6 was detected in 17.1%, HSV‐1 in 4.3% and CMV in 1.1%. Detection was higher in saliva than in oral swabs. There was no detection of HSV‐2 or VZV. Neither presence of oral mucosal abnormality nor therapeutic immunocompromise was related to increased detection of human herpes virus. Conclusion Commensal detection rates of EBV are high, and caution in clinical correlation of positive detection is warranted. Commensal CMV rates are low, and detection is likely to be clinically relevant. This study presents a comprehensive commensal detection rate of HHVs 1–6 by qPCR in saliva and swabs.
ISSN:1354-523X
1601-0825
DOI:10.1111/odi.13523