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Clinical and Diagnostic Laboratory Immunology, September 1999, p. 751-755, Vol. 6, No. 5
Department of
Pediatrics1 and Department of Laboratory
Medicine,2 University of California, San
Francisco, California 94143
Received 15 March 1999/Returned for modification 22 April
1999/Accepted 24 June 1999
The host's immune response to cervical human papillomavirus (HPV)
infection is poorly understood. In a longitudinal cohort of women with
cervical HPV infections, defined by PCR-based HPV DNA testing, we used
exfoliated cervical cells and reverse transcription-PCR to examine the
cervical mucosal mRNA expression of cytokines involved in regulating
cell-mediated immunity. We identified seven HPV-positive subjects who
were found to have cleared their HPV infections 4 months later. In all
seven, a T-helper type 1 (Th1) cytokine pattern (expression of gamma
interferon and absence of interleukin-4) preceded clearance. The more
variable cytokine patterns seen in HPV-negative subjects suggest that
the Th1 pattern in the women with subsequent clearance was a response
to the HPV infection. This contention is supported by additional
cross-sectional data showing a Th1 pattern in a majority of
HPV-positive women. This study establishes a feasible means for
assessing local cytokine expression in the cervical milieu and
demonstrates that a Th1 cytokine response is associated with subsequent
clearance of cervical HPV infection.
Cervical infection with human
papillomavirus (HPV) usually results in a transient infection, with 70 to 90% of individuals showing clearance, as defined by repeated HPV
DNA testing, within 12 to 24 months of detection (6, 9, 16).
The importance of persistence of HPV in the remaining 10 to 30%,
specifically with oncogenic types, is its strong association with the
development of high-grade squamous intraepithelial lesions (9, 10,
16). Factors which contribute to viral persistence have not been
elucidated but appear to have little or no association with sexual
behavior (16). Evidence is accumulating that the host immune
responses may be among the most influential factors in defining the
natural history of HPV infection.
Although the immune response to cervical HPV infection is not well
understood, evidence from murine and human infections by various
intracellular pathogens has highlighted the roles of T-cell- and
accessory-cell-derived cytokines in the initiation and maintenance of
effective immune responses to such pathogens (17, 20, 21). In particular, a model of immune regulation by T helper (Th) cells has
evolved in which antigen-experienced Th cells differentiate into
phenotypically distinct cells which differ in the combinations of
immunoregulatory cytokines they produce (18). The dichotomy between Th type 1 (Th1) cells, which promote cell-mediated immune (CMI)
responses to intracellular pathogens and inhibit humoral immunity, and
Th2 cells, which promote humoral responses and inhibit CMI responses,
has provided insight into the natural history of leprosy,
leishmaniasis, and other diseases (15, 22). This model may
provide insight into HPV infection which, like leprosy and
leishmaniasis, involves localization of infection by an intracellular pathogen to squamous epithelium.
The objective of the present study was to examine the association
between cervical mucosal cytokine expression and the clearance of
cervical HPV infection. Four cytokines were studied. Two cytokines produced principally by T cells (a Th1 cytokine, gamma interferon [IFN- (This work was presented as an abstract at the 17th International
Papillomavirus Conference, January 1999, Charleston, S.C.)
Study population and HPV detection by PCR.
Women
participating in an ongoing natural history study of HPV were asked to
participate in this study under the guidelines set forth by the
Committee for Research on Human Subjects, University of California, San
Francisco. Recruitment procedures for the longitudinal study have been
described in detail elsewhere (16). Briefly, women aged 13 to 20 years who were attending one of two family planning clinics were
screened for cervical HPV infection. Women found to be initially
positive for HPV and who agreed to participate in the natural history
study were seen at baseline and at 4-month intervals which included
cervical testing for HPV. Cervical testing for Chlamydia
trachomatis and Neisseria gonorrhoeae was also
performed at the baseline and annual examinations and on women who had
symptoms of lower genital tract infections at the interval visits. In
addition, a random sample of women who had a negative screen for HPV
were asked to participate as controls. These subjects were seen at baseline and at 6-month intervals unless they became HPV positive during follow-up, at which time they were asked to return every 4 months. HPV detection in this study was performed using the PCR
technique described previously (25). The presence of
amplified HPV product was separately sought in a dot blot format using
an enhanced chemiluminescence method. A generic probe mix that
determined the presence of one or more of 25 different HPV types
nonspecifically was used. Samples were also probed for HPV types 6, 11, 16, 18, 31, 33, 35, 42, 43, 45, 51, 52, 56, and 58. For samples that
were not typeable by these probes, additional typing was performed with
a strip-based HPV detection kit kindly provided by Roche Diagnostics,
Inc. (Alameda, Calif.).
Sample collection and RNA isolation.
Cervical cells were
collected from study subjects via cervical cytology brush prior to all
other samples to minimize contamination with peripheral blood. The
cytology brush was immediately immersed in a 4 M guanidine
thiocyanate-based denaturing solution (2). The lysates were
stored at 4°C at the collection sites and sent to the laboratory for
processing within 1 week of collection. Total RNA was isolated from the
samples using the acid-phenol method (3) and quantified by
measuring optical density at 260 nm.
Cytokine and CD4 RT-PCR.
RT was performed by using
random-hexamer (Promega, Madison, Wis.) priming and Moloney murine
leukemia virus reverse transcriptase (Promega) as previously described
(1). Omission of sample RNA from one RT reaction in each
test provided a negative control for the RT reactions and PCRs. PCR
amplification was performed as previously described (11),
using Taq DNA polymerase and primer sequences derived from
the literature. The primer sequences, chosen so that amplified
sequences span at least one intron, were as follows: IFN- Data analysis.
Rates of cytokine expression between groups
of subjects were compared by chi-square or two-sided Fisher's exact
test, where appropriate.
Detection of cytokine mRNA expression in exfoliated cervical
cells.
To examine in vivo cytokine expression in exfoliated
cervical cells, we opted to perform our assessment on unstimulated
cells. Cells were collected by cervical cytology brush and immersed
immediately into a lysing and denaturing medium. Total cellular RNA was
isolated from the samples, and RT-PCR was used to detect cytokine mRNA expression. All samples examined showed expression of the housekeeping gene for GAPDH, confirming sample and cDNA integrity. Figure
1 shows a typical cytokine RT-PCR result
from two subjects.
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Copyright © 1999, American Society for Microbiology. All rights reserved.
Th1 Cytokine Patterns in Cervical Human
Papillomavirus Infection
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
], and a Th2 cytokine, interleukin-4 [IL-4]) were chosen for their roles in promoting or inhibiting CMI responses, respectively. We hypothesized that a Th1 cytokine response, defined as a pattern of
cytokine production characterized by the expression of IFN- coupled
with the absence of IL-4 expression, would be necessary for clearance
of HPV infection and that failure to express and maintain this pattern
would be associated with a persistent infection. Two other cytokines
with important roles in promoting CMI responses were also examined:
tumor necrosis factor (TNF), produced by a wide variety of cell types,
and IL-12, produced by antigen-presenting cells. Using exfoliated cells
collected by cervical cytology brush, we assessed cytokine expression
at the mRNA level by reverse transcription (RT)-PCR in specimens
collected from women with current or cleared cervical HPV infections.
We report here that this method can be used to successfully assess
cytokine production in exfoliated cervical cells and that our data
suggest that a local Th1 cytokine pattern is associated with the
clearance of cervical HPV infections and that its expression appears to
be a response to the HPV infection. Also, while analysis of the
cytokine patterns associated with viral persistence will require
longitudinal study, preliminary observations suggest that women with
persistent HPV infection may be unable to maintain a Th1 response.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
,
5'-AATGCAGGTCATTCAGATGTAGCGG-3' and
5'-GGATGAGTTCATGTATTGCTTTGCG-3' (13); TNF,
5'-TCTCGAACCCCGAGTGACAA-3' and
5'-TATCTCTCAGCTCCACGCCA-3' (26); and IL-4,
5'-CAACTTTGTCCACGGACAC-3' and
5'-TCCAACGTACTCTGGTTGG-3' (23). Primers for
the IL-12 p40 chain were a generous gift from Stan Wolf, Genetics
Institute, Boston, Mass.; the sequences were 5'-CCAAGAACTTGCAGCTGAAG-3' and
5'-TGGGTCTATTCCGTTGTGTC-3'. Amplification of message for CD4
was performed by using commercial primers (Clontech Laboratories, Inc.,
Palo Alto, Calif.). Positive control reactions were set up for each
target sequence, using an identical sequence, in each PCR run. Message
from the housekeeping gene for glyceraldehyde 3-phosphate dehydrogenase
(GAPDH) was also amplified from each sample to verify sample and cDNA
integrity. PCRs were performed in a total volume of 50 µl in a
reaction mix consisting of 2.5 µl of cDNA, deoxynucleoside
triphosphate (dNTP) mix (0.2 M each [final concentration] dATP, dCTP,
dGTP, and dTTP; Pharmacia, Uppsala, Sweden), 2.5 mM MgCl2,
primers at 0.5 µM final concentration (each), reaction buffer
(supplied with enzyme), and 1 U of Taq DNA polymerase (Promega). The enzyme was withheld until the reactions reached 94°C,
to minimize mispriming. Amplification was carried out using 40 (or, for
IL-4, 45) cycles of PCR in a Perkin-Elmer (Foster City, Calif.)
thermocycler. The cycling program was 94°C denaturation for 1 min (5 min for first cycle), 60°C primer annealing for 1 min, and a 72°C
extension for 2 min. Amplified product was resolved by electrophoresis
on a 1.5% agarose gel and visualized and photographed using ethidium
bromide staining. A DNA size marker (Pharmacia) was included on the gel
to aid interpretation of product size. Bands were recorded as either
present (positive result) or absent (negative result).
RESULTS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
View larger version (3K):
[in a new window]
FIG. 1.
Cytokine RT-PCR results for four cytokines from two
subjects (lanes 3 and 4) and a positive (lane 1) and negative (lane 2)
control for each cytokine. Gel photographs were scanned on a
Hewlett-Packard flatbed scanner and composited with Adobe Photoshop
4.0; labels were added with Adobe Illustrator 8.0 on a Power Macintosh
computer.
Cervical cytokine expression preceding clearance of HPV
infection.
To examine cytokine profiles associated with subsequent
clearance of infection, we identified seven subjects for whom we had RNA samples from a visit at which they were HPV positive, but who had
cleared their infections by the time of the following study visit, 4 months later. All seven subjects showed a Th1 pattern of cytokine
expression which preceded their clearance of HPV (Table 1). Samples from all seven subjects also
showed expression of CD4 mRNA.
|
and TNF but now had
expression of the CMI response-inhibiting cytokine IL-4 as well,
reflecting a loss of a Th1 pattern. Subject f was positive only for TNF
among the cytokines examined.
|
Cervical cytokine expression in HPV-negative subjects.
To
investigate whether a Th1 pattern is a response to the HPV infection,
as suggested by the longitudinal data from subjects b and f (described
above) or represents constitutive cytokine production in resident cells
of the cervical epithelium, we examined cytokine expression in 15 HPV-negative subjects (Table 3). All subjects had cleared a prior HPV infection at some time in the past and
had remained HPV negative for various periods, as shown in Table 3. In
contrast to the subjects in Table 1, of whom 100% had a Th1 cytokine
pattern, only 23% (3 of 13) of these subjects had a Th1 pattern
(P = 0.003; two subjects with incomplete data were
excluded). IFN- expression was seen in only 67% (10 of 15) of these
subjects compared with 100% in the group with subsequent clearance
(P = 0.1), while 69% (9 of 13) showed expression of IL-4 compared with 0% (P = 0.005). The percentages of
subjects expressing the accessory-cell products TNF and IL-12 were not significantly different between the two groups (P = 1
for both cytokines).
|
Cervical cytokine expression in subjects with HPV infections of
various duration.
To further investigate cytokine patterns
associated with cervical HPV infection, we examined cross-sectional
cytokine data from women with current positive HPV tests of various
durations (Table 4) and compared them
with data from the HPV-negative subjects (Table 3). Overall, a Th1
pattern was seen in 60% (9 of 15) of HPV-positive subjects compared
with 23% (3 of 13) of subjects with cleared infections (P = 0.07). IFN- expression was seen in 80% (12 of 15) of
HPV-positive subjects compared with 67% (P = 0.7), and
IL-4 expression was seen in 20% (3 of 15) compared with 69%
(P = 0.02). The percentages of subjects expressing the accessory-cell products TNF and IL-12 were not significantly different between the two groups (P = 1 for both cytokines).
|
and TNF.
Additional testing for sexually transmitted diseases. To assess the possible influence of other genital tract infections on cervical cytokine expression, we examined the most recent annual tests for C. trachomatis and N. gonorrhoeae in the subjects. None of the subjects was positive for either infection.
Correlation of cytokine patterns with the date of the last menstrual period. To assess the possible influence of phases of the menstrual cycle on cervical cytokine expression, we evaluated cytokine patterns in those subjects who were HPV negative and not taking oral contraceptive pills. No apparent association was noted between cytokine patterns and the phases (proliferative, ovulatory, or follicular) of the cycle.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
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This study demonstrates the feasibility of using a sensitive
RT-PCR method for the examination of local cytokine expression in the
cervical milieu. The ease of sample collection and high sensitivity of
this method allow for the much-needed investigation of the role of
local cytokine expression in the natural history of cervical HPV
infection in a longitudinal cohort. The method does not require
invasive collection techniques, such as biopsy, nor extensive
postcollection manipulation, such as cloning or in vitro stimulation.
Furthermore, unlike immunoassays for detection of soluble protein, this
method detects actual cellular production of cytokines, at the level of
mRNA expression. The validity of this approach is affirmed by recent
work demonstrating a strong correlation between detection of cytokine
mRNA, by RT-PCR, and detection of protein secretion, by immunoassay
methods, for IFN- and IL-4 (8). This is consistent with
evidence that cytokine production is regulated principally at the level
of transcription (14, 24).
Using this method, we found that in all seven women who were shown to clear an HPV infection, a Th1 pattern of cytokine expression preceded their clearance (Table 1), supporting our hypothesis that clearance requires a Th1 response. Several lines of evidence indicate that the observed Th1 pattern was a response to the HPV infection. First, the contrast between this pattern and the more variable patterns in the HPV-negative subjects argues strongly that the Th1 pattern observed in the subjects with subsequent clearance was neither a random finding nor a constitutional pattern of the cervical epithelium. The most compelling evidence is provided by the longitudinal data for the two subjects described in Table 2, who each appear to have responded to a new HPV infection by mounting a Th1 response, followed by clearance of the new infection. Lastly, although limited by its cross-sectional nature and small sample number, our data from HPV-positive subjects also showed that women with HPV appeared more likely to show a Th1 response than HPV-negative subjects.
We had also hypothesized that viral persistence would be associated with failure to express and maintain a Th1 cytokine pattern. As expected, many of the patients with a history of HPV persistence (Table 4) lacked a Th1 response. However, there did not appear to be a simple causal relationship between expression of a Th1 pattern and clearance, since several subjects with a prolonged history of infection had Th1 cytokine patterns. This exemplifies the complexity and heterogeneity of the immune response and highlights the importance of longitudinal analysis. It may be that patients with persistent infection are unable to maintain a Th1 response over successive visits, as suggested by the two women (gg and ii) who had Th1 patterns on one visit but not the following visit, even though they remained HPV positive. Furthermore, even if a Th1 response is required for clearance, it may be insufficient without sustained and competent effector mechanisms and may be type specific. Evidence for this possibility comes from our longitudinal data on subject f, who appeared to mount a Th1 response to an intercurrent infection with HPV type 39 but not to her longstanding HPV 16 infection (Table 2). This may suggest that certain HPV types, such as HPV 16, somehow evade the immune system and go unrecognized. We anticipate that these issues will become clearer as more longitudinal data is collected from our study cohort.
The interpretation of the varied cytokine responses seen in HPV-negative individuals (Table 3) is unclear but again highlights the heterogeneity of the immune response. The expression of IL-4 in several of the women with recent clearance of an HPV infection (Tables 2 and 3) may reflect a regulatory role for Th2 cytokines in inhibiting a prolonged inflammatory response and consequent immune-mediated tissue damage, following clearance of the pathogen. Also, it is possible that in some cases, the virus may actually be suppressed rather than eliminated, the suppression being associated with continued intermittent cytokine production. The intermittent HPV type 58 positivity observed in one subject underscores this possibility, since the recurrence at the visit for which we have cytokine data available was accompanied by a Th1 pattern and was followed by an HPV-negative visit.
A limitation of the RT-PCR method is the inability to determine the
cellular sources of cytokine production. The four cytokines chosen for
study include both T-cell products (IFN- and IL-4) and accessory
cell products (TNF and IL-12). While our most compelling findings
involve patterns of expression of IFN- and IL-4, it cannot be
determined by our method whether Th cells were the main sources of
these cytokines in our samples. The apparent exclusion of IL-4
production preceding viral clearance (Table 1) suggests that these
women's responses involved some degree of cross-regulation between
IFN- and IL-4, which is a central feature of Th-cell-mediated immunoregulation (18). To begin investigating this, we were able to show that all seven patients in Table 1 also had expression of
CD4 message, indicating the presence of Th cells in the samples. This
points to Th cells as likely sources of IFN- in these samples but
does not rule out a role for CD8+ cells and NK cells.
Elucidation of the exact cellular sources of these cytokines will
ultimately require single-cell-based assays. Still, it is apparent even
from our bulk assay that examining the local mRNA expression of
immunoregulatory cytokines, regardless of their cellular sources,
provides greater understanding of the natural history of infection.
Another limitation of this method is the inability to assess potential
contamination of the samples with peripheral blood, since cells are
lysed at the time of collection. Our prior experience, however, had
shown that the majority of samples collected with a cytology brush do
not contain erythrocytes on microscopic examination if the sample is
the first one collected during the patient visit. Moreover, detection
of IFN- and IL-4 production in unstimulated peripheral blood
leukocytes appears to be relatively uncommon, with some investigators
reporting no detection by RT-PCR (12, 19) and others
reporting that they did detect constitutive production of one or the
other of these cytokines (4, 5, 7).
In summary, we have shown a feasible means for assessing an important aspect of local immune function in cervical HPV infection. The cytokine patterns demonstrated are not random, and a strong association between a Th1 pattern and subsequent clearance of infection was found, supporting our hypothesis that clearance requires Th1 cytokine production. It is anticipated that the collection of longitudinal data will allow more extensive correlation of cytokine patterns with subsequent course of infection. An understanding of the immunoregulatory mechanisms involved in control of HPV infection will prove valuable in assessment of vaccine and other prevention and treatment strategies.
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ACKNOWLEDGMENTS |
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We thank Sepideh Farhat for her contribution in performing the HPV PCR testing.
This work was supported in part by National Cancer Institute grant R01CA51323 and National Institutes of Health grant M01RR01271.
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FOOTNOTES |
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* Corresponding author. Mailing address: University of California San Francisco, Department of Pediatrics, Division of Adolescent Medicine, Box 1374, 513 Parnassus Ave., San Francisco, CA 94143. Phone: (415) 476-3260. Fax: (415) 502-1222. E-mail: mscott{at}itsa.ucsf.edu.
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Abstract
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Materials and Methods
Results
Discussion
References
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Clinical and Diagnostic Laboratory Immunology, September 1999, p. 751-755, Vol. 6, No. 5
1071-412X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
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