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Comparison of Human Papillomavirus Messenger RNA and DNA Detection: A Cross-sectional Study of 4,136 Women >30 Years of Age with a 2-Year Follow-up of High-Grade Squamous Intraepithelial Lesion

¹ Institute of Pathology, National University Hospital; ² Cancer Registry of Norway, Institute of Population-based Cancer Research, Oslo, Norway; and ³ NorChip AS, Klokkarstua, Norway

Requests for reprints: Tor Molden, Institute of Pathology, National University Hospital, Sognsveien 20, 0027 Oslo, Norway. Phone: 47-40403484; Fax: 011-47-32798801. E-mail: t.e.f.molden{at}labmed.uio.no

	Abstract

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The purpose of this study was to compare the detection of human papillomavirus (HPV) DNA with detection of mRNA. The study included 4,136 women >30 years of age. E6/E7 mRNA expression from the carcinogenic HPV types 16, 18, 31, 33, and 45 was detected by the PreTect HPV-Proofer assay, whereas the presence of HPV DNA was detected by Gp5+/6+ consensus PCR followed by type-specific PCR. A total of 4.0% had an abnormal cytologic diagnosis, 3.0% were positive by PreTect HPV-Proofer, 4.4% by type-specific PCR, and 10.4% by consensus PCR. For detection of HPV in high-grade squamous intraepithelial lesion (HSIL), no significant difference was observed between PreTect HPV-Proofer and consensus PCR. For women with a cytologic normal, atypical squamous cell of uncertain significance, and low-grade SIL diagnosis, the detection rate of HPV was significantly higher by Gp5+/6+ consensus PCR (P < 0.005) than by PreTect HPV-Proofer. Histology confirmed 14 of 23 cytologic HSIL as cervical intraepithelial neoplasia grade >2. Of these women, PreTect HPV-Proofer and type-specific PCR detected 12, whereas consensus PCR detected 13. In conclusion, for HSIL, detection of E6/E7 transcripts from HPV types 16, 18, 31, 33, and 45 are present to the same degree as DNA detected by consensus PCR. Equally important, only a small proportion of the HPV DNA–positive women with a normal, atypical squamous cell of uncertain significance or low-grade SIL diagnosis had a detectable mRNA expression. HPV E6/E7 mRNA detection by PreTect HPV-Proofer represents a new promising test as an adjunct to cytology.

	Introduction

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In some developed countries cytologic screening programs using Papanicolaou (Pap) smears have reduced cervical cancer incidence and mortality. Yet, cervical cancer is one of the most common malignant diseases and leading causes of morbidity and mortality among women worldwide (1). Single Pap tests suffer from suboptimal sensitivity, limited reproducibility, and many equivocal results (2, 3) and to compensate for these deficiencies a screening program with repeated testing combined with follow-up of positive cases is necessary. Furthermore, difficulties predicting which cervical lesion will progress, and the high rate of regression of low-grade lesion detected in cytologic screening, emphasize the need for additional prognostic and diagnostic markers for detection of cervical cancer precursors.

Infection with high-risk HPV is the main cause of cervical intraepithelial and invasive neoplasias (4, 5) and HPV DNA has been detected in >90% of cervical carcinomas, with the most common HPV types identified as HPV 16, 18, 31, 33, and 45⁴ (6-9). HPV is a common virus among women, particularly in younger age groups, and most infections are transient and asymptomatic (10, 11). Patients with persistent infection with these HPV types have a clearly enhanced risk of developing cervical carcinoma (12).

Large-scale screening studies have shown HPV testing as more sensitive than cytology for the detection of high-grade cervical lesions (13-16). However, low specificity of current assays and commercial kits hampers the use of HPV testing in screening. The combination of HPV DNA detection and cytology is more suitable for risk assessment of progression to cervical intraepithelial neoplasia (CIN) grade 3 and carcinoma than cytology alone (17, 18).

Viral infection is targeted at the parabasal keratinocytes, but with a relatively low level of viral E6/E7 mRNA expression (19). However, in the upper spinous and granular layers of the epithelium of squamous intraepithelial lesion (SIL) and cervical carcinoma, an increasing expression of the viral oncogenes E6 and E7 occurs. This expression is necessary for conversion to and maintenance of malignancy (20-22), and hence the detection of the E6/E7 transcripts of high-risk HPV types might serve as a better risk evaluation factor than mere DNA detection for the development of HSIL. The same would be true for the progression to cervical carcinoma (23).

The aim of the present study was to compare the detection of HPV mRNA from the carcinogenic HPV types 16, 18, 31, 33, and 45 with the detection of HPV DNA in an outpatient screening population in Norway with a 2-year follow-up of HSIL.

	Materials and Methods

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Study Design
The present study was a cross-sectional outpatient population–based screening study conducted in 2001, supplemented with follow-up data from the Cancer Registry of Norway. Cytology was compared with mRNA detection (PreTect HPV-Proofer) and DNA detection by type-specific and consensus PCR. Women with cytologic HSIL were subjected to follow-up for histologic confirmation according to guidelines for the Norwegian cervical cancer screening program (NCCSP). Results were compared with mRNA and DNA detection. The sensitivity, specificity, and positive and negative predictive values of HPV testing for detecting HSIL and of HPV testing in detecting CIN2+ in cytologic HSIL were calculated. McNemar's test was used for comparison of PCR and nucleic acid sequence–based amplification (NASBA). Student's t test was used for comparison of the differences in the mean follow-up time of women with HSIL and confirmed CIN2+ in contrast to those women with an unconfirmed CIN2+. The PCR and NASBA reactions were done independently. Cytology, NASBA, and PCR results were compared after all tests were done.

Study Subjects
In the NCCSP, women are encouraged to take a Pap smear every third year if the preceding Pap test is normal. Women with HSIL should be followed by immediate colposcopy and biopsy unless other medical reasons would indicate otherwise (e.g. pregnancy in which case close, cytologic surveillance might be preferred if there are no indication of invasiveness). A detailed description of the NCCSP is published elsewhere (24). In this study, women age 30 to 69 years (n = 4,154) were included, attending selected specialist gynecological clinics in Oslo in the period from February to May 2001. Of 4,154 women tested, 118 women were found negative for the U1A mRNA sample control. These samples were tested again and this time only 18 were negative for U1A, which were excluded from the study. The total number of women included in the study was 4,136. Gynecologists at 12 different clinics in Oslo performed the Pap smears, which were then screened by experienced cytotechnologists at two different laboratories. In the NCCSP, a hybrid classification with both dysplasia (WHO's classification) and CIN are used. In this article, the cytologic diagnoses HPV condyloma, CIN1, and mild dysplasia are defined as low-grade SIL (LSIL), whereas CIN2, CIN3, atypical glandular cell of uncertain significance, atypical squamous cell–cannot rule out high-grade lesion (ASC-H), moderate dysplasia, severe dysplasia, carcinoma in situ, and cervical cancer are defined as HSIL. Patients diagnosed with HSIL are referred to biopsy. For histopathologic evaluation, the WHO nomenclature and criteria are used.

Collection of Sample Material
The cervical samples were collected with a Cervex Brush (Rovers Medical Devices, Oss, the Netherlands) that was immersed in 9 mL of Nuclisens lysis buffer [5 mol/L guanidine thiocyanate, 0.1 mol/L Tris (pH 6.4), 20 mmol/L EDTA, and 1.2% (w/v) Triton X-100; BioMérieux, Boxtel, the Netherlands] directly after a cytologic smear was done. The samples in lysis buffer were stored at –70°C.

Automated DNA/RNA Isolation
The isolation of DNA/RNA was done according to Boom's isolation method (25) using the Nuclisens Extractor (BioMérieux) and the protocol for automated isolation. DNA/RNA was isolated from 1 mL of the 9 mL cervical smear sample in lysis buffer. DNA/RNA was eluted in 40 to 50 µL elution buffer [1 mmol/L Tris-HCl (pH 8.5)] and stored at –70°C.

PCR
Isolated DNA, stored at –70°C for no more than 6 months, was subjected to PCR using the consensus GP5+/6+ primers (26). Gp5+/6+ PCR was carried out in a 50-µL reaction volume containing 75 mmol/L Tris-HCl (pH 8.8 at 25°C), 20 mmol/L (NH₄)₂SO₄, 0.01% Tween 20, 200 µmol/L each of deoxynucleotide triphosphate, 1.5 mmol/L MgCl₂, 1 unit recombinant Taq DNA Polymerase (Fermentas Inc., Hanover, MD), 50 pmol of each primer, and 3 µL DNA. A 2-minute denaturation step at 94°C was followed by 40 cycles of amplification in a PCR processor (Primus 96, HPL block, MWG, Ebersberg, Germany). Each cycle included a denaturation step at 94°C for 1 minute, a primer annealing step at 40°C for 2 minutes, and a chain elongation step at 72°C for 1.5 minutes. The final elongation step was prolonged by 4 minutes to ensure a complete extension of the amplified DNA.

HPV type-specific PCR for HPV type 16, 31, and 33 were done according to Karlsen et al. (27), and HPV types 18 and 45 according to the following PCR protocol (NorChip AS, Klokkarstua, Norway). Only Gp5+/6+ PCR-positive samples were tested by type-specific PCR. The HPV 18 PCR reagent mixtures were similar to the Gp5+/6+ PCR reagent mixture, except for the inclusion of 2.0 mmol/L MgCl₂ rather than 1.5 mmol/L. The HPV 45 PCR was carried out without (NH₄)₂SO₄ and Tween 20, but included 10 mmol/L Tris-HCl (pH 8.3 at 25°C), 50 mmol/L KCl, and 0.001% gelatin. HPV type-specific PCR used 25 pmol of each primer. A 2-minute denaturation step at 94°C was followed by 35 cycles of amplification. Each cycle included a denaturation step at 94°C for 0.5 minute, a primer-annealing step at 57°C for 0.5 minute, and a chain elongation step at 72°C for 1 minute. The final elongation step was prolonged by 10 minutes to ensure a complete extension of the amplified DNA.

A ß-globin primer set was used to assess specimen adequacy (Operating procedure, University Hospital Vrije Universiteit, Amsterdam, the Netherlands). HeLa cells were used as positive controls for HPV 18, whereas SiHa or CaSki were used as positive control for HPV 16. No positive controls for HPV 31, 33, and 45 were run, due to lack of cell lines containing these HPV types. Water was used as negative control. Visualization of the PCR products was done on a DNA 500 chip according to the manufacturer's protocol (Agilent Technologies, Palo Alto, CA). The DNA chip uses a microscale gel electrophoresis with an optimal detection limit of 0.5 to 50 ng/µL. The results were interpreted using the Bioanalyzer 2100 software.

PreTect HPV-Proofer
The PreTect HPV-Proofer assay uses real-time multiplex NASBA, which amplifies mRNA in a DNA background with real-time detection of the products by molecular beacon probes. The PreTect HPV-Proofer assay was done according to the manufacturers instructions (NorChip) and automatically using RoboRead (MWG): Briefly, three premixes were made by reconstitution of reagent sphere (nucleotides, dithiotreitol and MgCl₂) in reagent sphere diluent (Tris-HCl, 45% DMSO), followed by addition of either U1A/HPV 16, HPV 33/45, or HPV 18/31 primer/molecular beacon mixes and KCl stock solution; 10 µL of this premix were distributed to each well in a reaction plate, followed by addition of 5 µL RNA (diluted 1:5) before incubation for 4 minutes at 65°C to destabilize secondary structures of RNA, followed by cooling down to 41°C. The reaction was started by addition of enzymes (AMV-RT, RNase H, T7 RNA polymerase, and bovine serum albumin) and measured in real-time using the Lambda FL 600 fluorescence reader (Bio-Tek, Winooski, VT) at 41°C for 2 hours and 30 minutes. Total reaction volume was 20 µL.

The RNA was stored for 1 year at –70°C before they were tested by NASBA. RNA isolated from CaSki cells was used as positive control for HPV 16. Artificial and standardized oligo's, corresponding to the viral sequence, were used as positive control for HPV 18, 31, 33, and 45. Water was used as negative control. The U1A serve as mRNA quality control.

A newly developed software package (PreTect Analysis Software, NorChip) was used for analysis of the experimental data. The excitation (nm) filters for FAM and Texas Red are 485/20 and 590/20, and the emission (nm) filters are 530/25 and 645/40, respectively.

	Results

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Cytologic Findings
The age distribution of women having a normal smear, HSIL smear, and HPV test positive results is given in Table 1. The age distribution was 24.7% in the group age 30 to 39 years, 29.3% in the group age 40 to 49 years, 29.2% in the group age 50 to 59 years, and 16.8% in the group age >60+ years. The mean age was 48.9 years (range = 30-91 years). A total of 98.2% of the 4,136 women included had taken at least one Pap smear with an average number of 5.3 during the previous 10-year period. The average number of Pap smears for PreTect HPV-Proofer negative women was 5.2 and 5.8 for the positive women (not significantly different).

HPV Detection in Relation to Cytology
The HPV DNA and E6/E7 mRNA prevalence from the five carcinogenic HPV types 16, 18, 31, 33, and 45 was in the range of 2.4% in cytologic normal to 52% in HSIL (Table 2). The HPV DNA prevalence detected by consensus PCR, was in the range of 9.3% to 64%. The detection of HPV in cytologically normal and LSIL women was significantly higher by type-specific PCR (McNemar's P < 0.05) than for PreTect HPV-Proofer. For the cytologically normal, ASCUS, and LSIL women, but not for HSIL women, the frequency of HPV DNA positive women detected by Gp5+/6+ consensus PCR was significantly higher than by mRNA detection (McNemar's P < 0.005). Furthermore, for the women having an unsatisfactory smear, no mRNA expression was observed, whereas type-specific PCR and consensus PCR detected 3.1% and 4.7%, respectively.

Overall Agreement between PreTect HPV-Proofer and PCR
A total of 98 (2.4%) women were positive for HPV by both Gp5+/6+ consensus PCR and PreTect HPV-Proofer, whereas 331 (8.0%) women were positive only by consensus PCR. Twenty-eight (0.7%) women were positive only by PreTect HPV-Proofer. For type-specific PCR, the corresponding numbers were 101 (2.4%), 82 (2.0%), and 25 (0.6%), respectively.

Comparison of HPV Type-Specific mRNA and DNA Detection Related to Cytology
In women with a cytologically normal diagnosis (n = 3,970), E6/E7 mRNA was expressed in only 30% of the HPV 16, 56% of the HPV 18 and 75% of the HPV 31 DNA–positive women (Table 3). This difference was significant (McNemar's P < 0.05). For HPV 33 and 45, no significant differences were found. In the cytologic ASCUS, LSIL, and HSIL women, no significant differences between DNA and mRNA detection were observed for HPV types 16, 18, 31, 33, and 45. An overall higher prevalence of HPV was detected in the women with cervical cell abnormalities, with HPV 16 as the most common type.

HPV Distribution and Subsequent Patient Histology within 2 Years
Women diagnosed with cytologic HSIL were followed up for any histology within 2 years (Table 4). Of the 25 cytologic HSIL women (including one squamous cell carcinoma), 14 were confirmed as CIN2+ by histology. In these 14 women, the index cytology was HSIL/CIN2 (n = 1), HSIL/CIN3 (n = 11), HSIL/ASC-H (n = 1), and HSIL/squamous cell carcinoma (n = 1). One woman with HSIL/CIN3 index cytology was not confirmed by histology. Two women in the cytologic HSIL group lacked follow up. From the 14 women confirmed by histology, the PreTect HPV-Proofer assay identified E6/E7 mRNA in 12 women in the index cytology test, which was identical to type-specific PCR. Gp5+/6+ consensus PCR identified 13 women positive for HPV DNA. The one CIN2+ woman positive for Gp5+/6+ PCR, but negative by PreTect HPV-Proofer, was typed to be HPV 35 by PCR.

	Discussion

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The women recruited for this study, older than 30 years of age, had several previous Pap tests. This may explain the low percentage of women with a cytologic HSIL diagnosis and therefore the low prevalence of histologic CIN2+. In addition, some women with a CIN2+ lesion may not have been detected due to a negative cytology result or due to an ASCUS or LSIL diagnosis, and hence not tested by histology.

For women with a cytologic HSIL diagnosis, the prevalence of HPV detected by PreTect HPV-Proofer and PCR was not significantly different. When excluding women not confirmed as CIN2+ on the histologic follow-up within 2 years, the detection rate for PreTect HPV-Proofer and type-specific PCR was 86%, whereas consensus PCR detected 93%. This difference is due to one HPV 35 infection, which is not detected by the PreTect HPV-Proofer assay. A high detection rate for E6 and E7 transcripts in CIN and cervical carcinomas has also been observed by Nakagawa et al. (28). In studies of histologically proven CIN3 and invasive cervical carcinoma, it has been shown that DNA and mRNA detection is practically identical⁴ (29). The low prevalence of cytologic HSIL explains the relatively low positive predictive values, since predictive values are dependent on the prevalence. Among the cytologic HSIL women, however, the prevalence of histologic CIN2+ was much higher and therefore also the positive predictive values.

In women with normal cytology, consensus PCR detected almost four times as many HPV positive and more than twice as many women with an ASCUS and LSIL diagnosis than PreTect HPV-Proofer. This difference was also observed between type-specific PCR and PreTect HPV-Proofer, with the most noticeable difference seen among cytologically normal women, where HPV 16 and 18 DNA was detected in respectively thrice and twice as many women as with RNA. For HPV 31, a similar result was observed. Sotlar et al. detected E6/E7 spliced transcripts in 50% of the HPV 16 infected normal and mildly dysplastic epithelia (23), whereas Falcinelli et al. did not observe any E6 mRNA expression in cytologically normal women but in 50% of the cytologically abnormal women (30).

An important issue in detection of HPV mRNA is the differentiation specific expression levels and the type of epithelium sampled by a routine swab. All infections have a controlled expression of E6/E7 at some time interval in the normal viral life cycle, as they are necessary viral proteins to carry out the viral life cycle (19). This may reflect the lack of detectable mRNA in LSIL and cytologically normal DNA–positive infections. Normal E2-induced down-regulation of E6 and E7 is followed by epithelial differentiation. Nontransforming HPV infections would not be as likely to express E6/E7 in the differentiated exfoliating epithelial cells that are sampled, whereas a dedifferentiated neoplasia would be expressing more E6/E7 in the surface epithelium. In terms of sensitivity for dysplastic lesions, mRNA detection hence will not have a lower sensitivity than DNA detection.

The use of HPV DNA testing for the triage of ASCUS and LSIL smears has been investigated by the ASCUS-LSIL Triage Study group (31-33). They found that a very high percentage of women with cytological diagnosis of LSIL were positive for HPV with the Hybrid Capture II assay, and for that reason, they concluded that there is limited potential for HPV testing in the clinical management of these women. In our study, however, for cytologically normal and LSIL women the E6/E7 mRNA prevalence found by the PreTect HPV-Proofer assay was considerably lower than by consensus PCR and also by type-specific PCR, yet nearly identical in histologically confirmed CIN2+.

An important issue in screening for cervical carcinoma is to keep the number of women referred to costly follow-up at a minimum, without substantially decreasing the sensitivity. For women with a cytologic ASCUS and LSIL diagnosis, the detection of E6/E7 transcripts may be more relevant than detection of DNA as a prognostic tool for risk evaluation regarding the development of CIN and its progression to cervical cancer (23). This minimizes unnecessary concern among HPV DNA positive women with a low risk for progression to HSIL. Consequently, a combination of HPV RNA testing and cytology done in a primary screening context may give the most optimal sensitivity and specificity. However, longer follow-up of women with cytologically normal, ASCUS, and LSIL diagnosis is needed.

Based on this study, as well as other studies done on dysplasia and carcinomas, a natural question is the number of different HPV types needed for efficient screening as an adjunct to cytology. Type-specific identification is important for monitoring possible persistent infections, which is a major risk factor for development of severe dysplasia (34). However including additional HPV types makes the testing procedure more complicated and also increases the detection rate for cervical carcinomas merely marginally. Today, 15 HPV types have been classified as high risk and sorted according to decreasing prevalence in cancer samples worldwide (8, 35). Detecting the five high-risk HPV types 16, 18, 31, 33, and 45 will identify most of the carcinoma cases worldwide, but regional differences have to be taken into regard. The choice of test procedure also depends on the local strategy; whether all women at risk for CIN2+ should be identified no matter the cost, or whether some women can be missed by screening to keep the costs down.

A limitation of our study is the testing by type-specific PCR only on the Gp5+/6+ consensus PCR positive samples and hence sensitivity, specificity, and predictive values cannot be calculated for type-specific PCR. However, performing type-specific PCR on all samples was considered too labor intensive in relation to a possible gain in information. In addition, the PCR products were detected by gel electrophoresis, and not by hybridization probes, which would have optimized the procedure and enhanced the sensitivity. Also, according to Norwegian guidelines, confirmation by histology has only been done on cytologic HSIL and consequently, some histologic CIN2+ may have been missed. Hence, the sensitivity and specificity values reported may be inflated due to verification bias.

In conclusion, for HSIL and CIN2+, E6/E7 transcripts from HPV types 16, 18, 31, 33, and 45 are present to the same degree as DNA detected by consensus PCR. Equally important, only a small proportion of the HPV DNA positive women with a cytologically normal, ASCUS, or LSIL diagnosis had a detectable mRNA expression. Introduction of carcinogenic HPV E6/E7 mRNA detection by PreTect HPV-Proofer represents a new promising technology in HPV diagnostics work as adjunct to cytology.

	Acknowledgments

 
We thank participating gynecologists for the collection of sample material; staff at the Department of Pathology, Norwegian National Hospital; staff at the Pathology Laboratory; and everybody at NorChip AS for their valuable help, especially Siri Hovland, Marit Øder Øye, Inger Marie Falang, Petter Grønn, Trine Nordstrøm, and Anders Aak for technical assistance and Einar Morland for help with the database.

	Footnotes

 
Grant support: Research Council of Norway grant 145316/213.

The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

⁴ I. Kraus and T. Molden et al. Investigation of 204 cervical squamous cell carcinomas; comparison of a novel HPV E6/E7 mRNA detection assay with various HPV DNA detection systems.

Received 6/ 4/04; revised 8/27/04; accepted 9/22/04.

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