Real-Time PCR Improves Detection ofTrichomonas vaginalisInfection Compared With Culture Using Self-Collected Vaginal swabs

A M Green,A M Caliendo,R J Diclemente,G M Wingood,J Ingersoll,J A Jordan

doi:10.1080/10647440500068248

Abstract

OBJECTIVE: To compare a real-time polymerase chain reaction (PCR) assay with broth culture for the detection of Trichomonas vaginalis using self-collected vaginal swabs. METHODS: Self-collected vaginal swabs were obtained from adolescent and young adult African-American women participating in HIV-1 prevention programs. T. vaginalis culture was performed using the InPouch TV System. Samples for the real-time PCR assay were collected using the BDProbeTec ET Culturette Direct Dry Swab system and tested in a laboratory-developed assay which targeted a repeated sequence of the genome. Discrepant samples that were culture negative and positive in the real-time PCR assay were tested in a confirmatory PCR which targeted a different region of the T. vaginalis genome, the18S ribosomal DNA gene. RESULTS: Of the 524 specimens tested by both culture and real-time PCR, 36 were culture positive and 54 were positive in the real-time PCR assay; 16 of the 18 discrepant specimens were also positive in the confirmatory PCR assay. Using a modified gold standard of positive by culture or positive in both PCR assays, the sensitivity of the real-time PCR assay was 100% and the specificity was 99.6%, whereas culture had a sensitivity of 69.2% and a specificity of 100%. CONCLUSIONS: The real-time PCR assay was sensitive and specific for the detection of T. vaginalis DNA from self-collected vaginal swab specimens. The ability to use the BDProbeTec dry swab system for the real-time PCR testing allowed for the detection of Chlamydia trachomatis, Neisseria gonorrhoeae, and T. vaginalis from a single specimen.

Highlights

Trichomonas vaginalis is one of the most common sexually transmitted diseases, with an estimated 5 million cases per year in the United States [1] and as many as 200 million cases annually worldwide
The 18 specimens that were positive by real-time polymerase chain reaction (PCR) and culture negative, as well as 36 specimens that were negative by real-time PCR and culture, were tested in a confirmatory PCR assay, which targeted a different region of the T. vaginalis genome
We developed a real-time PCR assay for the detection of T. vaginalis that was both sensitive and specific

Summary

Introduction

Trichomonas vaginalis is one of the most common sexually transmitted diseases, with an estimated 5 million cases per year in the United States [1] and as many as 200 million cases annually worldwide. Common symptoms of T. vaginalis infection include vaginal discharge and vulval irritation. Complications of T. vaginalis infection can occur in untreated women and include endometritis, infertility and cervical erosion [2,3]. T. vaginalis infections can lead to severe complications including premature rupture of membranes [4], preterm deliveries and low-birth-weight infants [4]. T. vaginalis infection is a cause of nongonococcal urethritis, [5] and if untreated may lead to complications including chronic prostatitis, urethral strictures, epididymitis and/or infertility [2,3]. It has been estimated that between 10% and 50% of T. vaginalis infections are asymptomatic [10], supporting the need for more intensive screening for T. vaginalis infections in sexually active men and women as well as pregnant women

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