Abstract
Five hundred specimens (288 genital, 192 dermal, and 20 ocular) were extracted by technologists, and the DNA was assayed by LightCycler PCR (DNA polymerase and thymidine kinase [TK] gene targets) and by conventional tube and shell vial cell culture. One hundred fifty-eight confirmed (by cell culture and TK target PCR) positive and LightCycler-positive specimens were detected during the first 30 PCR cycles. LightCycler PCR-positive results for cycles 31 to 45 (39 of 67 [58.2%]) required confirmation by another PCR target (TK). LightCycler PCR is more sensitive (n = 197; 23.1%) than cell cultures (n = 150) for the routine laboratory detection of herpes simplex virus infections.
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CITATION STYLE
Espy, M. J., Ross, T. K., Teo, R., Svien, K. A., Wold, A. D., Uhl, J. R., & Smith, T. F. (2000). Evaluation of LightCycler PCR for implementation of laboratory diagnosis of herpes simplex virus infections. Journal of Clinical Microbiology, 38(8), 3116–3118. https://doi.org/10.1128/jcm.38.8.3116-3118.2000
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