A large, population-based study of age-related associations between vaginal pH and human papillomavirus infection

Vaginal pH was measured during enrollment and follow-up screening visits of a population-based cohort study of cervical neoplasia in Guanacaste, Costa Rica. Detailed methods of recruitment, screening, and follow-up have been reported elsewhere [15, 16]. Briefly, a random sample of about 20% of Guanacaste census tracts identified 11,742 women, of whom 10,769 were eligible for the study (Figure 1). Of these eligible women, 10,049 agreed to participate and were interviewed after giving informed consent. A pelvic examination was offered to women who reported previous sexual intercourse in the interview and of the 9,466 eligible, 9,175 (97%) had the exam performed. At enrollment, vaginal pH measurements were obtained from 9,165 women. A subcohort of women (n = 3,065) who were at risk of developing CIN3 or cancer (CIN3+) based on enrollment screening results and reported sexual behavior, as well as a group of women who had negative screening results (referent group) were actively followed at intervals of 6 or 12 months for up to 7 years. The remaining 6,029 women, who were considered (and subsequently proven) to be at very low risk of cervical cancer based on completely negative multimodal screening, were included in the passive follow-up cohort that was screened again at 5-7 years after enrollment [16]. Among the 9,094 women followed, 8,080 (88.8%) had at least one follow-up visit. Of the active cohort, 87.4% had greater than one follow up visit whereas 98% of the passive cohort had at least one follow up visit. The median follow-up times in both cohorts were equivalent (6-7 years), although the screening intensity was clearly higher in the active cohort. The study protocol was reviewed and reapproved annually by the National Cancer Institute and a Costa Rican Institutional Review Board.

Exfoliated cervical cells for split-sample conventional Pap smear and ThinPrep cytology (Cytyc Corp., Boxborough, MA) were collected using a Cervex broom-like collection device (Unimar, Wilton, CT) during the pelvic exam. Additional cervical cells were collected using a Dacron swab and stored in Specimen Transport medium (Qiagen, previously Digene Corp., Gaithersburg, MD) for HPV testing. Cervical abnormalities were identified by visual inspection, cytology, or cervicography. Cervical cytologic abnormalities were classified as cancer and/or high-grade squamous intraepithelial lesions (HSIL+), low-grade squamous intraepithelial lesions (LSIL), atypical squamous cells of undetermined significance (ASCUS), reactive changes, or normal. As the current analysis focused on HPV-related cytomorphologic changes, a woman's cytology was interpreted as LSIL if her conventional smear and/or ThinPrep results met the criteria for LSIL and the diagnosis of the alternative method was either ASCUS or LSIL.

Specimens from the enrollment visit were tested initially in the United States by the Hybrid Capture Tube test (Qiagen, previously Digene Corp., Gaithersburg, MD). However, because this method had limited sensitivity (10 pg/mL) and only detected 11 of the carcinogenic HPV types, all specimens were retested using a polymerase chain reaction (PCR) test. As previously described [17, 18], DNA extracted from exfoliated cells in a 100-μL aliquot of the specimen was amplified using the MY09/MY11 L1 degenerate primer PCR system with AmpliTaq Gold polymerase (TaqGold; Perkin-Elmer-Cetus, Norwalk, CT). After amplification, PCR products were analyzed by electrophoresis and hybridized with radiolabeled generic HPV DNA probes. Type specific oligonucleotide hybridization was used for HPV typing: Probes were specific for types 2, 6, 11, 13, 16, 18, 26, 31-35, 39, 40, 42-45, 51-59, 61, 62, 64, 66-74, 81-85, and 89. We considered the following HPV types as carcinogenic: HPV16, 18, 31, 33, 35, 39, 45, 51, 52, 56, 58, and 59 [19]. The HPV testing lab was masked to clinical outcomes. All PCR testing and genotyping were done in the United States, at the Albert Einstein College of Medicine in New York.

Vaginal pH was measured with a pHydrion strip (Micro Essential Laboratories, Brooklyn, NY). After insertion of a sterile speculum the pHydrion strip was placed on the left lateral vaginal wall between the speculum blades until moistened and color change was immediately compared with the colorimetric scale and the measurement was recorded across a range of 3.0-5.5 in increments of 0.5 pH units.

Detection of C. trachomatis was measured with an assay for C. trachomatis DNA as previously described [20] in an age-stratified subsample (N = 1,216). Briefly, C. trachomatis DNA was detected in enrollment samples using a C. trachomatis PCR-DEIA assay (Labo Biomedical Products BV, Rijswijk, the Netherlands). After the PCR, C. trachomatis DNA was detected by C. trachomatis--specific probe hybridization in a DNA enzyme immunoassay that used 10 μL of the PCR product. The mixture of probes present in the C. trachomatis DNA enzyme immunoassay can recognize all C. trachomatis serovars and genovariants that have been deposited in GenBank.

The unit of analysis was the study visit. Based on their age at each visit, women were stratified into the following categories: < 25 years, 25-34 years, 35-44 years, 45-54 years, 55-64 years and 65+ years. To standardize frequency of visits by time, each clinic visit was assigned to a bin defined by years after enrollment. Bins for each woman began with bin 0 (enrollment date), continued for every year until they were censored (for suspicion of HSIL+ or completion of the follow-up, i.e., at least 6 years and 9 months from enrollment) or they were lost to follow-up. If a woman was tested more than once in a bin and her HPV results were discordant on positivity, the result from the positive visit was taken to acknowledge the possibility of HPV measurement error. Similarly, if pH was tested more than once in a bin, the visit with the highest vaginal pH recorded was chosen. Regarding cytology, if more than one result was available, the more severe reading was chosen.

Our main analyses focused on risk of HPV positivity with vaginal pH as the primary independent variable. We calculated the odds of testing HPV positive vs. testing negative and the odds of testing positive for multiple HPV types vs. a single HPV type. For all of the above-mentioned analyses, we used the method of generalized estimating equations (GEE) with an independent correlation structure [21]. This approach accounted for repeated visits resulting in possible auto-correlation and reduced overall variance, but it made few assumptions regarding the nature of the intra-individual correlations [22]. To determine if elevated vaginal pH was also related to HPV-induced cytological abnormalities, we calculated the odds of concurrent LSIL cytology, vs. a result of normal or reactive changes and we looked at the relationship between vaginal pH and high grade lesions(HSIL) compared to ≤ LSIL among HPV positive women.