Herpes simplex direct detection of genital lesions
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Editor-In-Chief: C. Michael Gibson, M.S., M.D. [1]; Associate Editor(s)-in-Chief: Lakshmi Gopalakrishnan, M.B.B.S.
Overview
The confirmation and characterization of the infection and its type by direct detection of herpes simplex virus in genital lesions is essential for diagnosis, prognosis, counseling, and management. Cell culture and PCR are the preferred HSV tests for people seeking medical treatment for genital ulcers or other mucocutaneous lesions. The sensitivity of viral culture is low, especially for recurrent lesions, and declines rapidly as lesions begin to heal. PCR assays for HSV DNA are more sensitive and are increasingly used in many settings.[1][2] PCR is the test of choice for detecting HSV in spinal fluid for diagnosis of HSV infection of the central nervous system. Viral culture isolates should be typed to determine which type of HSV is causing the infection. Failure to detect HSV by culture or PCR does not indicate an absence of HSV infection, because viral shedding is intermittent. The use of cytologic detection of cellular changes of HSV infection is an insensitive and nonspecific method of diagnosis, both for genital lesions (i.e., Tzanck preparation) and for cervical Pap smears and therefore should not be relied upon.
British Association for Sexual Health and HIV (BASHH) Recommendations[3]
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External Link
BASHH guidelines mentioned in National Guideline Clearinghouse
References
- ↑ Scoular A, Gillespie G, Carman WF (2002) Polymerase chain reaction for diagnosis of genital herpes in a genitourinary medicine clinic. Sex Transm Infect 78 (1):21-5. PMID: 11872854
- ↑ Wald A, Huang ML, Carrell D, Selke S, Corey L (2003) Polymerase chain reaction for detection of herpes simplex virus (HSV) DNA on mucosal surfaces: comparison with HSV isolation in cell culture. J Infect Dis 188 (9):1345-51. DOI:10.1086/379043 PMID: 14593592
- ↑ http://www.bashh.org/documents/59/59.pdf