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Pap test

The Pap test, also known as the Papanicolaou test or Pap smear, is a cytological screening procedure that detects precancerous or cancerous cellular abnormalities in the uterine by microscopically examining exfoliated cells collected from the transformation zone using a spatula, brush, or broom-like device. Developed by Greek-American physician and cytopathologist Georgios Nicholas Papanicolaou in the late 1920s while studying vaginal smears at and Medical College, the method was first reported in a 1928 article co-authored with gynecologist Howard C. Taylor Jr., with its efficacy for early detection demonstrated through clinical trials by 1941. Introduced as the first widely implemented test, the Pap test revolutionized preventive gynecology by enabling detection of and , stages amenable to curative intervention, leading to at least an 80% reduction in incidence and mortality in screened populations through population-based programs established from the onward. Its success stems from the causal link between persistent high-risk human papillomavirus (HPV) —responsible for nearly all cancers—and detectable cytological changes in the squamous of the transformation zone, allowing empirical validation via longitudinal studies showing of low-grade lesions in many cases but progression in untreated high-grade ones. Despite its proven impact, the Pap test faces limitations including false-negative rates from sampling errors or obscured cells (up to 30% in some audits) and false-positive rates of 1-10%, often prompting and for benign or regressive lesions like CIN1, which modeling estimates contribute to 55-75% depending on grade thresholds. Overscreening persists in low-risk groups, exacerbating iatrogenic harm from unnecessary procedures, though empirical data affirm net benefits when guidelines limit testing to ages 21-65 at 3-5 year intervals, increasingly co-tested or replaced by primary HPV assays for superior in detecting persistent oncogenic types.

Overview

Definition and mechanism

The Pap test, also known as the Papanicolaou test or Pap smear, is an exfoliative procedure that collects and examines cells from the to identify precancerous or cancerous changes, infections, inflammatory conditions, and hormonal influences. Developed by Georgios Papanicolaou and first detailed in a 1943 monograph, it relies on the principle that abnormal cells shed or can be mechanically dislodged from the for microscopic analysis. Cell collection targets the transformation zone—the junction between squamous ectocervical epithelium and columnar endocervical epithelium—where most cervical dysplasia arises, often due to persistent human papillomavirus infection. A cytobrush rotates within the endocervical canal to sample glandular cells and mucus, while a plastic spatula scrapes the ectocervix to gather squamous cells; for conventional smears, samples are immediately smeared onto labeled glass slides and fixed in 95% ethanol or aerosol fixative to preserve morphology and prevent autolysis. Liquid-based cytology variants suspend cells in preservative fluid, reducing obscuring factors like blood or mucus through automated thin-layer preparation. Stained slides undergo Papanicolaou staining, a polychromatic technique using hematoxylin to basophilically stain nuclei dark blue-purple for chromatin detail assessment, followed by acidophilic counterstains like (OG-6) for keratinized cytoplasm (orange) and eosin-azure (EA) for non-keratinized elements (pink, blue, green), enabling differentiation of mature squamous cells, endocervical cells, and metaplastic intermediates. Under light microscopy at magnifications from 10x to 40x, cytotechnologists screen for cytologic —such as nuclear enlargement, hyperchromasia, irregular nuclear membranes, increased nuclear-to-cytoplasmic ratio, or cytoplasmic vacuolization—while pathologists confirm diagnoses using standardized systems like , which classifies findings from negative for intraepithelial lesion or to high-grade . This visual detection of dysplastic changes exploits causal cellular responses to oncogenic insults, prioritizing empirical morphology over molecular assays in primary screening.

Primary purpose and target population

The Pap test, formally known as the Papanicolaou test, functions primarily as a cytological screening tool to identify atypical squamous or glandular cells in cervical samples, which may indicate precancerous dysplasias such as or early invasive carcinoma, thereby facilitating timely diagnostic follow-up and treatment to avert progression to . This screening detects cellular abnormalities caused predominantly by persistent high-risk human papillomavirus (HPV) infection, though it is not diagnostic for HPV itself nor intended for active disease surveillance or symptomatic evaluation. The target population comprises asymptomatic women with an intact who are at average risk for , typically those aged 21 to 65 years, excluding individuals with prior total for non-cancerous conditions or those adequately screened previously without high-grade lesions. Screening initiation occurs at age 21 regardless of sexual history, with cytology alone recommended every 3 years for ages 21–29 to balance detection benefits against risks in this low-prevalence group. For ages 30–65, while primary high-risk HPV testing every 5 years is increasingly preferred due to superior sensitivity for detecting persistent infections, Pap cytology remains a viable standalone option every 3 years or in co-testing with HPV every 5 years, per guidelines from the U.S. Preventive Services Task Force (USPSTF, reaffirmed December 2024 draft) and American College of Obstetricians and Gynecologists (ACOG). Discontinuation after age 65 is advised for those with three consecutive negative cytology results or two negative co-tests within the prior 10 years, absent high-risk history. The advocates starting at age 25 with primary HPV testing to 65, reflecting evolving evidence favoring HPV-led strategies in vaccinated cohorts, though Pap cytology retains utility where HPV assays are unavailable. Screening is not routinely recommended before age 21 or after in low-risk cases, as benefits do not outweigh procedural harms.

Procedure

Sample collection techniques

The standard Pap test sample collection begins with the insertion of a speculum into the to visualize the , allowing access to the ectocervix and endocervical . This step ensures unobstructed sampling of the transformation zone, where precancerous changes most commonly arise. Providers typically collect endocervical cells first using a cytobrush or endocervical brush, which is gently inserted into the external os until the bristles are no longer visible, then rotated 360 degrees clockwise for 5-10 seconds to dislodge cells without causing trauma. Ectocervical sampling follows with an Ayre's or wooden , inserted parallel to the and rotated firmly 360 degrees around the exocervix to scrape squamous epithelial cells, particularly from the squamocolumnar junction. Alternative devices include a single broom-like sampler for non-pregnant individuals with an , where the device is inserted into the endocervical os and rotated five full turns to capture cells from both endocervical and ectocervical regions simultaneously. In () methods, such as ThinPrep or SurePath, collected cells are rinsed directly into a solution vial rather than smeared on a , reducing obscuring factors like or mucus; the and are swirled or broken off into the vial and discarded. Conventional smear techniques, though less common today, involve spreading the endocervical sample along one long axis and the sample perpendicularly on the same or a second , immediately fixed with 95% spray or solution to preserve . Collection should avoid menses, recent douching (within 24-48 hours), vaginal medications, or lubricants, as these can contaminate or degrade samples; sampling may be used post-hysterectomy if indicated. Self-collection techniques, primarily validated for HPV testing rather than cytology, involve tampon-like devices or swabs but yield lower cellularity for Pap interpretation and are not standard for routine screening. Adequate sampling requires the presence of endocervical or squamous metaplastic cells in the final preparation to confirm transformation representation.

Laboratory processing and types

Laboratory processing of Pap test samples involves preparing cervical cells for microscopic evaluation to detect abnormalities indicative of precancerous or cancerous changes. Following collection, specimens are transported to a cytology laboratory where they are accessioned, stained, and mounted for examination by cytotechnologists or pathologists. The Papanicolaou (Pap) stain, a polychromatic method using hematoxylin for nuclear staining, Orange G 6 for keratinized cytoplasm, and modified eosin azure for non-keratinized elements, is standard for highlighting cellular morphology, nuclear details, and cytoplasmic features. Two main types of Pap test preparations exist: conventional smears and (LBC). In conventional processing, cells are directly smeared onto a glass slide using a or , immediately fixed with 95% or a cytologic spray to preserve and prevent air-drying artifacts, then allowed to dry before transport. Upon lab receipt, slides undergo hydration if needed, followed by the Pap staining sequence: immersion in Harris hematoxylin for nuclear counterstaining, differentiation in acid-alcohol, bluing in alkaline solution, staining with and eosin azure mixtures, dehydration through graded alcohols, clearing in , and coverslipping. This method, while cost-effective, can result in overlapping cells, obscuring elements like blood or , leading to higher rates of unsatisfactory specimens in some studies, reported at up to 5-10% compared to LBC. Liquid-based cytology, introduced in the 1990s and now predominant in many settings, collects cells into a preservative liquid medium (e.g., methanol-based for ThinPrep or ethanol-based for SurePath), which disperses and preserves cells while allowing removal of debris. Processing entails vortexing or agitating the vial, then automated deposition of a thin, uniform cell layer onto a slide via (ThinPrep) or (SurePath), followed by the same staining protocol. reduces unsatisfactory rates by minimizing artifacts—studies show 1-2% inadequacy versus 3-5% for conventional—and enables ancillary testing like HPV DNA detection from residual liquid, but randomized trials indicate no significant improvement in sensitivity or specificity for high-grade lesions over conventional methods. Quality assurance in processing includes evaluating specimen adequacy, requiring at least 10-12 well-preserved squamous cells or presence of endocervical or transformation zone cells to confirm representative sampling. Automated screening aids like the ThinPrep Imaging System review pre-selected fields to enhance efficiency, though manual review remains essential for final interpretation. Variations such as ultrafast Pap staining adapt the for rapid intraoperative but are not routine for screening.

Reporting and interpretation standards

, first developed in 1988 and revised in 2014, provides the standardized framework for interpreting and reporting results from cervicovaginal cytologic specimens, including Pap tests. This system ensures uniform terminology across laboratories to facilitate consistent communication between pathologists, clinicians, and patients. Reports must include specimen type (e.g., conventional smear or liquid-based preparation), adequacy assessment, general categorization, automated review if applicable, cellular interpretation, ancillary testing results, and optional educational notes. Specimen adequacy is evaluated first and is mandatory for reporting. A specimen is deemed satisfactory for evaluation if it contains at least 5,000 nucleated squamous cells in liquid-based preparations (or 8,000–12,000 in conventional smears), with the presence of endocervical or squamous metaplastic cells indicating adequate sampling of the transformation zone; lower cell counts may still qualify if abnormal cells are identified. Unsatisfactory specimens, defined by fewer than 2,000 evaluable cells or obscuration of more than 75% of cells by , , or other factors, require repeat collection and must specify the reason for inadequacy. Interpretation proceeds only on satisfactory specimens, with quality indicators such as transformation zone component noted to assess sampling reliability. General categorization divides reports into "Negative for Intraepithelial Lesion or Malignancy" (NILM) or "Epithelial Cell Abnormality," with the latter subdivided by squamous or glandular origin. NILM encompasses non-neoplastic findings, such as reactive cellular changes from inflammation or infection (e.g., , , ), atrophy, , or endometrial cells in women over 40 (which warrant clinical correlation for risk). Epithelial abnormalities are interpreted based on cytomorphologic criteria, including nuclear size, hyperchromasia, irregular nuclear membranes, and cytoplasmic changes. Squamous epithelial abnormalities are classified as: Glandular epithelial abnormalities include:

Clinical Effectiveness

Evidence from randomized trials and observational data

Observational studies, including population-based analyses and case-control designs, provide the strongest evidence for the effectiveness of Pap test screening in reducing incidence and mortality, as large randomized controlled trials directly comparing cytology to no screening have not been feasible in high-income settings due to established practice and ethical constraints. In countries implementing organized cytology programs, such as , , and , mortality declined by 50%, 34%, and 80%, respectively, over periods spanning decades following program initiation, with reductions attributed to early detection and of precancerous lesions. Case-control studies further corroborate these findings, showing that unscreened women face 3- to 10-fold higher risks of invasive compared to regularly screened women, with protective effects increasing with screening frequency and recency. A and of observational data confirmed that is associated with reductions in invasive incidence, with odds ratios indicating 40% to 90% lower risk among screened versus unscreened populations, though effect estimates vary by screening coverage and interval. studies, such as one analyzing U.S. surveillance data, estimated that smear screening averted between 105,000 and 492,000 cases from 1975 to 2009 by preventing progression from , after adjusting for pre-screening era baselines. In , an analysis of screening-attributable mortality calculated a 53% reduction (95% : 23–72%) linked to program participation. Randomized trials exist primarily for comparative purposes, such as HPV versus cytology arms, where cytology serves as an active demonstrating baseline ; for instance, in trials like the Swedish Malmo study, cytology screening yielded cumulative reductions in grade 3 or higher, though HPV arms showed superior long-term outcomes. Attendance at screening episodes in observational audits, such as Finland's program, correlates with 41%–92% mortality reductions among participants, underscoring dose-response relationships but highlighting gaps for non-attenders, who account for disproportionate cancer deaths. These data collectively support causal attribution to screening via temporal associations, biological plausibility of interrupting HPV-driven , and consistency across diverse populations, despite potential confounders like concurrent improvements in healthcare access.

Quantitative metrics: sensitivity, specificity, and predictive values

The of conventional Pap tests for detecting grade 2 or higher (CIN2+), a common endpoint for high-grade lesions, is typically reported in the range of 50% to 70% across studies, reflecting variability due to factors such as protocols, reader experience, and verification bias in evaluations against or . A 2024 review of screening strategies found conventional cytology at 59% for CIN2+, lower than alternatives like HPV testing, while shows marginally higher rates, around 60-65% in comparative analyses. for CIN3+ or invasive cancer is somewhat higher, with pooled estimates from individual patient data reaching 76% at an atypical squamous cells of undetermined significance (ASC-US) or worse threshold, though this drops to 45-50% for stricter high-grade squamous intraepithelial lesion (HSIL) cutoffs in primary screening contexts. Specificity for CIN2+ is consistently higher, often exceeding 90%, as the test effectively rules out disease in most negative cases but suffers from trade-offs with sensitivity due to heterogeneous study designs and thresholds. In the same 2024 review, conventional Pap specificity reached 94%, outperforming HPV-based methods in avoiding false positives, while a Latin American evaluation reported 97.5% specificity for cytology versus 91.7% for HPV testing. Earlier meta-analyses confirm this pattern, with specificities from 84% to 97%, negatively correlated with sensitivity estimates due to diagnostic verification issues where only abnormal results prompt . Liquid-based methods yield similar specificity, around 92-95%, but real-world performance can decline with high-volume screening due to subtle cytologic changes being missed. Positive predictive value (PPV) for CIN2+ following an abnormal Pap result varies with the cytologic and underlying , typically 20-40% for low-grade abnormalities like LSIL (reflecting in many cases) and rising to 60-80% for HSIL referrals. In low- screening populations (e.g., <1% CIN2+ rate), PPV for ASC-US is often below 10%, necessitating triage, whereas negative predictive value (NPV) exceeds 99% for negative cytology, providing reassurance against high-grade disease for 3-5 years. These values underscore the test's role in interval cancer prevention despite modest PPV, with combined cytology-HPV strategies enhancing overall accuracy in recent evaluations.
MetricTypical Range for CIN2+ DetectionKey Influencing FactorsExample Pooled Estimate
Sensitivity50-70%Cutoff threshold (ASC-US vs. HSIL), cytology type (conventional vs. liquid-based)59% (conventional)
Specificity90-97%Population prevalence, verification bias94% (conventional)
PPV20-40% (abnormal result)Cytologic grade, HPV co-testing37% (LSIL/HSIL referrals)
NPV>99% (negative result)Low disease prevalence in screened cohorts99.8% (with )

Impact on cervical cancer incidence and mortality

The introduction of widespread Pap test screening in the mid-20th century correlated with marked declines in incidence and mortality across multiple populations. , incidence and mortality rates have decreased by over 50% in the four decades leading up to 2020, primarily due to the uptake of Pap smear screening programs that enable early detection and treatment of precancerous lesions. Similarly, population-based studies in and elsewhere attribute reductions of 41% to 92% in mortality to participation in screening, with organized systems yielding 17% to 79% lower mortality compared to non-invited groups. Quantitative evidence from and observational underscores the screening's causal role in averting advanced . Regular Pap screening has been associated with at least an 80% reduction in both cervical cancer incidence and mortality, as evidenced by long-term follow-up in screened versus unscreened women. For instance, screened individuals exhibited a 38% lower risk of cervical cancer death overall, with reductions of 59%, 35%, and 38% for localized, regional, and unknown-stage cancers, respectively, independent of stage at . Ecological analyses further estimate that Pap smears prevented 105,000 to 492,000 cervical cancer deaths in the U.S. from 1975 to 2010 by shifting detection toward early-stage , evidenced by a halving of early-stage incidence from 9.8 to 4.9 cases per 100,000 women between 1976 and 2009, alongside declines in late-stage cases. These impacts are most pronounced in settings with high screening coverage, such as organized programs in , where a 53% reduction in mortality (95% CI: 23-72%) was directly attributable to screening after adjusting for pre-screening trends. The International Agency for Research on Cancer concludes that reduces mortality by 80% or more among adherent women, primarily through prevention of progression from to invasive via colposcopy-guided interventions. However, residual mortality persists in under-screened subgroups, highlighting coverage as a key limiter, while recent U.S. data show sustained precancer declines (79-80% from 2008-2022 in young women), reinforcing ongoing benefits despite HPV vaccination's emergence.

Limitations and Associated Harms

Sources of inaccuracy: false positives and negatives

False-negative results in Pap tests occur when precancerous or cancerous lesions are present but not detected, primarily due to sampling errors where inadequate collection misses abnormal cells from the transformation zone, endocervical canal, or submucosal lesions, accounting for up to 81% of false negatives in some analyses. Obscuring factors such as , , , or inflammatory can mask abnormal cells on the slide, while douching or vaginal medications may dilute or wash away atypical cells prior to sampling. Screening errors involve overlooking subtle abnormalities during initial review by cytotechnologists, and interpretive errors stem from subjective misclassification of cells as benign, with interobserver reproducibility limited (kappa=0.46 for low-grade lesions) and rescreening reclassifying over 50% of normal slides as abnormal in certain studies. These issues contribute to Pap test ranging from 30% to 87% for detecting high-grade lesions, with false-negative rates of 13% to 70% reported across reviews. False-positive results arise when benign cellular alterations are misinterpreted as dysplastic or malignant, often leading to unnecessary or . Reactive inflammatory changes from non-neoplastic causes, such as or irritation, frequently mimic high-grade squamous intraepithelial lesions through nuclear enlargement, hyperchromasia, and irregular contours. Reparative processes following epithelial injury, including those from infections like or , produce streaming sheets of cells with atypical features that challenge distinction from true . Atrophic changes in postmenopausal women cause squamous cells to exhibit enlarged, hyperchromatic nuclei resembling , while immature or follicular can further confound interpretation. Benign conditions overall represent a common source of false-positive reports, as evidenced by high rates of negative follow-up biopsies after atypical squamous cells of undetermined significance (ASC-US) designations.

Overdiagnosis of precancerous lesions

Overdiagnosis in cervical screening refers to the detection of precancerous lesions, such as cervical intraepithelial neoplasia (CIN), that would spontaneously regress or remain subclinical without progressing to invasive cancer, thereby subjecting asymptomatic individuals to unnecessary diagnostic follow-up and potential treatment. This phenomenon arises because Pap tests identify cellular abnormalities across a spectrum of CIN grades, many of which exhibit high rates of natural regression, particularly in younger women. The natural history of CIN1 (low-grade squamous intraepithelial lesion, LSIL) is characterized by spontaneous in approximately 80% of cases, often within 2 years, with progression to higher-grade s or cancer occurring rarely. For CIN2 (a borderline high-grade lesion), rates range from 40% to 60% over 24 months, especially among HPV-negative or young patients, while or progression is less predictable but lower than for CIN3. 00542-2/fulltext) CIN3 s show lower , with complete resolution to in about 14% of observed cases and partial to CIN1 or CIN2 in another 9-17%, though most persist or progress without intervention. In population screening, Pap cytology contributes to overdiagnosis by flagging these regressive lesions for and , amplifying detection of non-progressive abnormalities; randomized trials and observational data indicate that screening in adolescents and women under 21 yields minimal benefits but increases of transient precancers by up to 50-fold compared to older s. Longitudinal studies confirm that many CIN2+ diagnoses represent , as and untreated data reveal that only a fraction of such lesions would evolve into invasive within lifetimes, with regression favored by immune clearance of transient HPV infections underlying most low-grade changes. This underscores the need for risk-stratified management, such as observation for CIN1 and select CIN2 cases, to mitigate harms from interventions like excision, which carry risks of cervical incompetence and .

Overtreatment risks and downstream complications

Overtreatment in cervical screening arises from the excision or ablation of precervical lesions, particularly (CIN) grades 1 and 2, many of which spontaneously without progressing to invasive cancer. Studies indicate rates of approximately 60% for CIN1 lesions and 40-70% for CIN2, with higher rates (up to 60%) observed in women under 30 years old during short-term follow-up. For instance, in a of untreated CIN2 cases, 44.1% regressed within 12 months, and cumulative reached 55.4% by 24 months. Immediate intervention thus exposes women to procedural risks without averting disease in a substantial proportion of cases, particularly when triggered by abnormal Pap results that prompt and . Common overtreatment procedures include loop electrosurgical excision procedure (LEEP) and cold knife cone biopsy, performed for confirmed CIN2 or higher to remove potentially precancerous tissue. These interventions, while effective for high-grade lesions, carry downstream complications such as , , and , which can impair menstrual flow or . More critically, excisional treatments increase the risk of adverse obstetric outcomes in subsequent pregnancies, including and . A meta-analysis linked LEEP conization to elevated preterm delivery risk, with odds ratios heightened among women without prior preterm history. The association with preterm birth stems from removal of cervical tissue, which may compromise structural integrity and lead to cervical incompetence. Reviews of conization effects report consistent increases in preterm delivery rates, influenced by factors like specimen volume and procedure type, with second-trimester cervical shortening as a predictor. Although one recent study found comparable preterm risks between surveillance and immediate LEEP for CIN2, broader evidence supports a small but significant elevation in adverse outcomes post-procedure, affecting a minority of women but underscoring the harm of unnecessary treatment. These complications highlight the trade-off in screening programs, where detection of transient abnormalities prompts interventions that, for regressing lesions, yield net harm rather than benefit.

Complementary and Alternative Screening Methods

Integration with HPV DNA testing

The integration of human papillomavirus (HPV) DNA testing with the Pap test addresses limitations in cytology sensitivity by detecting high-risk HPV types responsible for nearly all cervical cancers. In co-testing, both and or hybrid capture assays for high-risk HPV (hrHPV) are performed concurrently on the same sample, allowing for risk stratification: negative results on both confer low risk, while hrHPV positivity prompts further evaluation regardless of cytology, and abnormal cytology with negative HPV may warrant observation. This approach, applicable to women aged 30–65 years, extends screening intervals to 5 years for dual negatives, as endorsed by the Preventive Services (USPSTF) in its 2018 guidelines and reaffirmed in the December 2024 draft recommendation. Randomized controlled trials, including pooled analyses from European studies, demonstrate that co-testing yields higher sensitivity for detecting grade 3 or greater (CIN3+)—approximately 95–100% versus 60–80% for cytology alone—while providing comparable long-term protection against invasive to primary HPV testing. A of three such trials found co-testing reduced CIN3+ detection at subsequent rounds compared to cytology, though with marginally lower specificity (around 90% versus 95% for HPV alone), leading to more referrals. Observational data from U.S. implementation corroborate these findings, showing co-testing detects persistent hrHPV infections causal to precancerous lesions earlier than cytology, which primarily identifies downstream morphologic changes that may regress spontaneously in up to 50% of cases. HPV testing also serves as triage for equivocal Pap results, such as atypical squamous cells of undetermined significance (ASC-US), where hrHPV negativity identifies over 90% of low-risk cases for routine rescreening, avoiding unnecessary procedures and improving efficiency over repeat cytology. The College of Obstetricians and Gynecologists (ACOG) and American Cancer Society (ACS) guidelines from 2021 and 2023, respectively, position co-testing as an acceptable alternative to primary hrHPV screening every 5 years, particularly where standalone HPV assays are unavailable, though they emphasize primary HPV's superior negative predictive value (over 99% for CIN3+ at 5–6 years). Integration has contributed to declining U.S. cervical cancer incidence, with hrHPV-positive cases triaged to reducing missed precancers by 30–50% relative to cytology-only protocols in cohort studies. Despite enhanced detection, co-testing's dual thresholds can amplify over-referral for transient HPV infections in women under 30, where prevalence exceeds 20% but cancer risk remains low; thus, guidelines restrict it to ages 30 and older to minimize harms. Cost-effectiveness analyses indicate co-testing is comparable to primary HPV in high-resource settings, with quality-adjusted life years gained similar to cytology alone but at higher upfront costs due to expenses, estimated at $50–100 per test in U.S. implementations. Ongoing refinements, informed by HPV vaccination reducing hrHPV prevalence by 80–90% in vaccinated cohorts, prioritize de-intensification for low-risk dual negatives to balance benefits against procedural risks like anxiety and complications.

Comparison of Pap test to primary HPV screening

Primary HPV screening detects high-risk human papillomavirus (hrHPV) DNA or RNA as the initial test for cervical cancer precursors, with reflex cytology or genotyping for positive results, whereas the Pap test relies on cytological examination of cervical cells to identify atypical or malignant changes. Randomized controlled trials, such as the New Technologies for Cervical Cancer (NTCC) trial in , have demonstrated that HPV testing exhibits substantially higher sensitivity for detecting grade 2 or worse (CIN2+), with a 39.2% relative increase over Pap cytology (HPV sensitivity approximately 96% vs. Pap 55-68%), though specificity is modestly lower (HPV 90-94% vs. Pap 93-97%). Meta-analyses of screening strategies confirm primary HPV testing's superior performance in identifying CIN2+, with pooled sensitivity exceeding 90% compared to 40-60% for cytology, enabling detection of persistent infections that precede cytological abnormalities by years; however, this advantage incurs higher rates of unnecessary colposcopies due to transient HPV infections that regress without progression, affecting specificity and increasing risks. In long-term follow-up from trials like NTCC and ARTISTIC, HPV-based screening reduced CIN3+ incidence by 50-60% over 6-10 years relative to cytology, with a 40% lower invasive cancer rate in meta-analyses, attributed to earlier intervention on high-risk cases, though cytology's higher specificity minimizes immediate procedural harms.
MetricPap Test (Cytology)Primary HPV Testing
Sensitivity for CIN2+40-68%90-96%
Specificity for CIN2+93-97%90-94%
CIN3+ Detection (relative)Baseline50-60% greater
Colposcopy ReferralsLower2-3x higher
Evidence from observational data in diverse settings reinforces these metrics, with HPV primary screening's reproducibility advantages stemming from molecular detection over subjective cytological , which varies by reader expertise and sample adequacy; nonetheless, in resource-limited contexts, Pap's lower needs sustain its despite inferior detection. Guidelines, including USPSTF recommendations updated in 2024, endorse primary HPV every 5 years as preferable for ages 30-65 due to optimized benefit-harm balance, with Pap every 3 years as an alternative where HPV is unavailable, reflecting of equivalent long-term mortality reduction but HPV's efficiency in risk stratification.

Emerging self-sampling and automated technologies

Self-sampling technologies enable individuals to collect vaginal or cervicovaginal specimens at home or in clinical settings without requiring a pelvic examination by a clinician, primarily for human papillomavirus (HPV) detection as a complement or alternative to traditional Pap cytology. A 2024 U.S. Food and Drug Administration (FDA) approval permits self-collection of vaginal samples for certain HPV tests in health care settings, demonstrating detection rates comparable to clinician-collected samples, with pooled sensitivity for high-risk HPV of approximately 92-95% in meta-analyses of randomized trials. These kits, often using brushes like the Evalyn Brush or Cervex-Brush, have shown higher screening uptake—up to 20-30% increases in participation rates among hard-to-reach populations—due to reduced barriers such as embarrassment, access, and discomfort associated with speculum-based Pap collection. However, direct self-sampling for cytological analysis (akin to Pap smears) yields lower adequacy and sensitivity for detecting squamous intraepithelial lesions, with clinician-collected samples outperforming self-collected by 10-15% in detecting high-grade lesions in comparative studies, limiting its standalone use for cytology-based screening. Automated technologies for Pap test interpretation leverage (AI) and to assist cytotechnologists in slide review, addressing inter-observer variability and workload burdens in manual microscopy. The Genius Digital Diagnostics System, FDA-cleared in 2023 as the first fully cytology platform, employs AI algorithms to scan slides, prioritize regions of interest, and reduce full slide review time by up to 33% while maintaining or improving abnormality detection rates. models, validated in 2024 studies on digitized whole-slide images, achieve AUC values exceeding 0.95 for classifying cervical cytology as negative, low-grade, or high-grade intraepithelial lesions, outperforming traditional manual screening in for precancerous changes by identifying subtle morphological features like irregularities. Collaborations such as and Techcyte's AI-based cytology digitize slides for remote review, enhancing in resource-limited settings, though prospective trials report false-negative reductions of 5-10% but require human oversight to mitigate AI errors in rare atypical cases. Low-cost AI-microscopy platforms, developed in 2025 prototypes, integrate for automated cell classification in conventional smears, achieving over 90% concordance with expert pathologists in pilot evaluations from low-resource contexts. These advancements prioritize empirical validation against gold-standard , yet ongoing concerns include from training datasets skewed toward high-prevalence populations and the need for regulatory standardization to ensure generalizability across diverse demographics.

Historical Development

Invention by George Papanicolaou

George Nicholas Papanicolaou, a Greek-born and researcher, developed the foundational technique of the Pap test through studies in exfoliative cytology beginning in the early . Arriving in the United States in 1913, he joined Medical College's Department of in 1914, where he initially investigated reproductive cycles in guinea pigs using vaginal smears to identify estrous phases via cellular changes observed under a . By 1916, this approach allowed precise timing of reproductive cycles, laying groundwork for applying similar cytological methods to humans. In 1920, Papanicolaou extended his research to human vaginal smears, starting with his wife as the initial subject to map variations through epithelial cell morphology. Examining smears from patients at Cornell Clinic and later in collaboration with Woman's Hospital from 1925, he noted atypical cellular features in cases of known uterine , including enlarged, irregular nuclei indicative of during routine cycle studies. This led to the core innovation: non-invasive sampling of exfoliated and vaginal cells via speculum insertion, followed by microscopic analysis to detect early cancerous or precancerous changes, distinct from invasive methods. Papanicolaou first publicly presented the cancer-detection potential of vaginal smears in 1928 at the Third Race Betterment Conference, describing it as "New Cancer " based on observations of abnormal cells in smears from affected patients; however, the largely overlooked these findings at the time. He refined the technique, including a specialized staining protocol—later termed the —using hematoxylin, , and EA (a mixture) to enhance and cytoplasmic detail for accurate classification of types. Mary Papanicolaou contributed extensively as lab technician and daily smear provider for calibration over two decades, enabling consistent methodological validation. Renewed efforts in 1939, spurred by Cornell's Dr. Joseph Hinsey and collaboration with gynecologist Herbert F. Traut, involved systematic testing on thousands of cases at New York Hospital, confirming the smear's diagnostic value for . In 1941, they published "The Diagnostic Value of Vaginal Smears in Carcinoma of the Uterus" in the American Journal of Obstetrics and Gynecology, analyzing smears from over 300 patients and demonstrating detection rates for early lesions. This culminated in their 1943 monograph, Diagnosis of Uterine Cancer by the Vaginal Smear, documenting over 3,000 cases and establishing the Pap test as a reproducible, low-cost screening tool reliant on cytological criteria rather than symptomatic presentation.

Path to clinical adoption and standardization

Following the initial publication of the Papanicolaou method in and its validation through clinical studies by , adoption faced initial resistance due to skepticism among physicians regarding cytology's reliability for early cancer detection. A pivotal advancement occurred in 1943 with the publication of Diagnosis of Uterine Cancer by the Vaginal Smear by George Papanicolaou and Herbert Traut, which provided detailed protocols and case evidence, prompting demonstrations at institutions like Harlem Hospital in that year. These efforts led to rapid uptake in urban medical centers, as gynecologists observed high sensitivity in identifying precancerous lesions, reducing reliance on more invasive biopsies. By the late , the Pap test had become a standard component of women's , coinciding with post-World War II initiatives that emphasized preventive screening amid cervical cancer's status as a leading cause of female mortality. Nationwide programs expanded in the and , with clinical trials confirming efficacy in detecting squamous intraepithelial lesions, leading to routine integration into gynecological practice by the early . This era marked a shift from opportunistic testing to systematic screening, supported by organizations like the , which advocated for annual exams, though evidence later tempered frequency recommendations. Standardization of reporting lagged behind adoption, initially relying on the Papanicolaou classification system (Classes I–V, denoting normal to malignant cells), which suffered from inter-observer variability and inconsistent terminology across labs. In December 1988, the convened a workshop in , resulting in (TBS), a uniform framework for cervical cytology interpretation that emphasized descriptive diagnoses like atypical squamous cells of undetermined significance (ASC-US) and low-grade squamous intraepithelial lesion (LSIL). TBS revisions in 1991, 2001, and 2014 refined criteria to incorporate ancillary testing and reduce ambiguity, facilitating global comparability and quality control in screening programs. This system addressed prior inconsistencies, improving diagnostic reproducibility without altering the core smearing technique.

Post-adoption refinements amid HPV discoveries

The identification of high-risk human papillomavirus (HPV) types, particularly HPV-16 and HPV-18, as the primary causative agents of by in the mid-1980s prompted a reevaluation of cytological screening practices, revealing that most Pap test abnormalities represented transient HPV infections rather than inevitable progression to malignancy. This causal insight shifted focus from cytology alone to risk stratification, emphasizing persistent high-risk HPV infection as the key precursor to high-grade lesions. Early refinements included the introduction of for reporting cervical cytology, which standardized terminology such as atypical squamous cells of undetermined significance (ASC-US), low-grade (LSIL), and high-grade (HSIL), facilitating more consistent interpretation amid emerging virological data. Subsequent revisions in 1991, 2001, and 2014 incorporated nuances like HPV-related changes to refine diagnostic categories and reduce interpretive variability. Technological advancements in sample preparation paralleled these discoveries, with the U.S. (FDA) approving () methods, such as ThinPrep in 1996, as alternatives to conventional smears. minimized obscuring artifacts like blood and —common in up to 20% of conventional slides—improving cellular preservation and readability while enabling residual sample use for molecular HPV assays. This preparation technique increased sensitivity for detecting high-grade lesions by 5-10% compared to smears and laid the groundwork for integrated testing, addressing Pap test limitations such as 20-40% false-negative rates attributed to sampling errors and transient HPV-driven changes. HPV DNA testing emerged as a critical adjunct, with the Hybrid Capture 2 (HC2) receiving FDA approval in 1999 for triaging ASC-US results, identifying high-risk HPV to prioritize and averting unnecessary procedures in low-risk cases where cytology alone over-referred up to 70% of women with benign transient infections. The American Society for and Pathology (ASCCP) formalized this in 2001 consensus guidelines, recommending high-risk HPV testing for ASC-US management, which reduced referrals by 40-60% while maintaining detection of precancerous lesions. By 2003, FDA clearance extended HC2 use to co-testing with cytology for women aged 30 and older, enabling every-5-year screening intervals for double-negative results, as HPV negativity provided >99% negative predictive value for high-grade disease over 5-10 years. These protocols, validated in trials like ALTS (ASCUS/LSIL Triage Study), demonstrated superior efficiency over cytology alone, though implementation highlighted challenges like higher upfront costs and the need for triage algorithms to manage HPV-positive, cytology-negative findings.

Guidelines and Global Implementation

Major organizational recommendations (e.g., USPSTF, WHO, ACS)

The Preventive Services Task Force (USPSTF) recommends cervical cytology (Pap test) every 3 years for women aged 21-29; for ages 30-65, primary high-risk human papillomavirus (hrHPV) testing every 5 years is preferred, with cytology alone every 3 years or co-testing (cytology plus hrHPV) every 5 years as acceptable alternatives. Screening should cease after age 65 for those with adequate prior negative results and no high-risk history. The (ACS) advises against routine screening before age 25 due to low incidence in younger women; for ages 25-65 at average risk, primary hrHPV testing every 5 years is recommended as the preferred method, with cytology alone every 3 years acceptable only if hrHPV is unavailable. Co-testing is not routinely endorsed. Discontinue after 65 with three consecutive negative hrHPV tests or two negative co-tests in the prior decade, absent high risk. The (WHO) prioritizes hrHPV DNA testing as the primary screening modality globally, particularly in resource-limited settings, with cytology reserved for triage or where HPV testing is inaccessible; screening initiation at age 30 with HPV every 5 years (or 10 years if triage-negative) is suggested, extending to 49-65 based on context and HIV status. WHO endorses "screen-and-treat" or "screen-triage-treat" approaches to pre-cancer lesions, emphasizing equity and feasibility over cytology-alone strategies in low-income regions. The American College of Obstetricians and Gynecologists (ACOG) aligns closely with USPSTF, recommending cytology every 3 years from ages 21-29 (with optional hrHPV co-testing at 25-29 if preferred); for 30-65, options include primary hrHPV every 5 years, co-testing every 5 years, or cytology alone every 3 years. Cessation follows USPSTF criteria post-65.
OrganizationScreening Start AgeCytology (Pap) Frequency (Ages 21-29)Preferred Method (Ages 30-65)Cessation Criteria
USPSTF21Every 3 yearshrHPV every 5 years (cytology or co-test alternatives)Age 65+ with adequate negatives, no high risk
ACS25Not routine (use only if HPV unavailable)hrHPV every 5 years (cytology alternative if needed)Age 65+ with recent negatives, no high risk
WHO30 (contextual)Triage or limited usehrHPV every 5-10 yearsResource-dependent, post-65 if low risk
ACOG21Every 3 years (HPV optional 25+)hrHPV, co-test, or cytology every 3-5 yearsAligns with USPSTF post-65
These guidelines reflect a shift toward HPV-centric screening for superior in detecting high-grade precursors, reducing cytology's role amid evidence of its lower specificity and higher false-positive rates, though cytology persists in younger cohorts or transitional settings to balance accessibility and harm minimization.

International variations and access challenges

International cervical cancer screening programs exhibit significant variations in the utilization of the Pap test, influenced by resource availability, healthcare , and evolving on . In high-income countries with organized screening systems, such as those in , the Pap test is often integrated into cytology-based protocols or transitioned toward primary HPV testing with cytology triage, with screening intervals typically every 3–5 years for women aged 25–64. For instance, the employs an organized, invitation-based program limiting Pap-inclusive screening to ages 30–60, achieving higher compliance rates compared to opportunistic approaches elsewhere. In contrast, the relies more on opportunistic screening, with guidelines from the recommending Pap testing alone every 3 years for ages 21–29, shifting to co-testing or primary HPV for ages 30–65 at 3–5 year intervals. These differences stem from national priorities, with European programs emphasizing population coverage through centralized registries, while U.S. practices reflect decentralized healthcare delivery. In middle- and low-income countries, Pap test adoption varies widely, often constrained by opportunistic rather than organized systems. Countries like and have implemented national organized programs incorporating Pap cytology, targeting women aged 30–59 with 3–5 year intervals, yet coverage remains below 50% in many regions due to logistical hurdles. Eastern European nations, such as , predominantly use opportunistic Pap screening, resulting in lower participation rates compared to . The advocates for periodic Pap or alternative screening for all adult women where feasible, aiming for 70% coverage among ages 30–49 by 2030, but global data indicate only one-third of women in this group have ever been screened, with stark disparities: high coverage (>70%) in and versus <20% in and . Access challenges to Pap testing are pronounced in low-resource settings, where the method's reliance on trained cytotechnologists, quality-controlled laboratories, and follow-up limits scalability. In , insufficient infrastructure and personnel contribute to advanced-stage diagnoses, with screening uptake hindered by rural-urban divides and issues for reagents. Barriers include high costs relative to , lack of , cultural , and transportation difficulties, exacerbating inequities; for example, women in low-income households in and face 2–3 times lower screening rates than urban counterparts. Policy support exists in many low- and middle-income countries, but financial commitments are minimal, leading to fragmented programs and reliance on alternatives over Pap cytology. Despite evidence that Pap screening can reduce mortality by over 80% when systematically applied, implementation gaps in these regions perpetuate higher incidence, underscoring the need for adaptable, low-cost adaptations like self-sampling adjuncts.

Recent updates emphasizing risk stratification

In 2019, the American Society for and (ASCCP) introduced risk-based management consensus guidelines for abnormal results, marking a significant shift from traditional results-based algorithms to individualized risk stratification using current and prior test history, HPV genotyping, and cytology findings to estimate the immediate risk of grade 3 or higher (CIN3+). This approach draws on empirical data from large trials like the Atypical Squamous Cells of Undetermined Significance () Low-Grade Squamous Intraepithelial Lesion (LSIL) Triage Study (ALTS) and cohorts, establishing risk benchmarks: is recommended if CIN3+ risk is 4% or greater, repeat testing if between 0.55% and 4%, and return to routine screening if below 0.55%. HPV-16 or HPV-18 positivity elevates risk thresholds, prompting immediate even with negative cytology, while other high-risk HPV types allow for nuanced . Subsequent refinements in 2024 extended these guidelines to incorporate partial or extended for non-16/18 , enabling finer risk tiering; for instance, certain genotypes (e.g., HPV-31, 33, 45, 52, 58) confer intermediate risks that can defer when combined with negative tests like cytology or dual-stain (/Ki-67 ). The ASCCP also endorsed dual-stain cytology as a option for HPV-positive women in primary screening or co-testing, providing risk stratification comparable to or better than standalone cytology by identifying high-grade lesions with higher specificity and reducing unnecessary referrals. These updates prioritize causal factors like persistent high-risk HPV over isolated Pap test abnormalities, aiming to minimize overtreatment while maintaining detection of precancerous lesions. This risk-stratified framework aligns with broader guideline evolutions, such as the 2020 recommendation for HPV-primary screening starting at age 25, where subsequent management follows ASCCP risk thresholds for positives. A December 2024 U.S. Preventive Services Task Force draft similarly emphasizes HPV testing as optimal for ages 30-65, implicitly supporting by favoring its higher sensitivity for high-grade disease over cytology alone. Empirical validation shows these methods achieve CIN3+ detection rates equivalent to prior guidelines but with 30-50% fewer colposcopies in low-risk scenarios, reflecting a data-driven reduction in interventions driven by transient HPV infections rather than oncogenic persistence.

Controversies and Debates

Screening start , frequency, and cessation debates

Debates on the optimal to initiate screening with the Pap test center on balancing the rarity of invasive disease in younger women against the risks of false-positive results leading to invasive follow-up procedures. Prior to , some practices recommended screening as early as 18 for sexually active adolescents, but evidence from cohort studies showed that grade 3 (CIN3) lesions, precursors to cancer, rarely progress to before 25, with fewer than 0.1% of cases in women under 20 resulting in cancer. The American Society for Colposcopy and Cervical Pathology and others endorsed starting at 21 in 2006, formalized in by the American College of Obstetricians and Gynecologists (ACOG), citing high regression rates of low-grade lesions (over 90% for CIN1) and procedure-related harms like from excisional treatments. The U.S. Preventive Services (USPSTF) affirmed this in 2018, recommending Pap testing every 3 years from ages 21-29, as earlier screening yields minimal mortality reduction while increasing colposcopies by up to 50% in low-risk groups. The (ACS) updated in 2020 to delay primary HPV testing (preferred over Pap alone) until 25, arguing incidence under 25 is under 1 per 100,000, reducing unnecessary interventions without increasing risk. Critics of starting at 21, including some European models, advocate 25-30 based on randomized trials showing no survival benefit from earlier cytology, though U.S. adherence lags due to provider habits and patient expectations. Frequency recommendations have shifted from annual to triennial or quinquennial intervals following longitudinal data on lesion progression timelines. Pre-2003 annual screening stemmed from limited understanding of human papillomavirus (HPV) persistence, but natural history studies indicate CIN3 takes 10-20 years to become invasive, allowing safe extension to every 3 years with cytology for ages 21-29 and 30-65, or every 5 years with HPV testing, per USPSTF 2018 guidelines. This change averted an estimated 4.6 million procedure-related harms annually in the U.S., including bleeding and infection from 1-2% of colposcopies, alongside anxiety from 0.8 million false positives. Debates persist on overuse, with 2021 analyses showing 20-30% of women receiving annual Paps despite guidelines, correlating with higher preterm delivery risks from excisional therapies ( 1.5-2.0 for cone biopsy). Proponents of less frequent screening cite randomized trials like the ARTISTIC study, where 6-year intervals matched 3-year efficacy (95% sensitivity for CIN3), but opponents highlight disparities in high-risk groups, such as immunocompromised women, where annual cytology may outperform extended intervals by 10-15% in detection. Recent 2024 draft USPSTF updates favor primary HPV every 5 years from age 30, dismissing cytology-only as inferior (sensitivity 60% vs. 95% for HPV), though implementation faces resistance from cytology-focused labs. Cessation debates focus on and prior screening adequacy, with guidelines recommending discontinuation at age 65 for average-risk women with three consecutive negative Paps or two negative HPV tests in the prior decade, as lifetime risk post-65 drops below 0.7% with adequate history. This stems from modeling showing minimal benefit (number needed to screen 1,000 for one prevented cancer) versus harms like and in , where CIN3 exceeds 30%. However, 20-25% of U.S. cervical cancers occur post-65, often in underscreened women, with studies indicating those ceasing without criteria face doubled incidence by age 85. Observational data reveal sharp Pap rate drops at 66 (15-20% decline), disproportionately affecting and women with inconsistent histories, prompting calls for risk-based extensions to 70-75 using HPV testing for catch-up. European extensions to age 70 in low-incidence areas yield net benefits in models (life-years gained 50-100 per 1,000 screened), but U.S. critiques emphasize incentives, with 40% of seniors still screened unnecessarily per 2022 surveys. In vaccinated cohorts, earlier cessation (e.g., 50-55) is proposed but unproven, pending long-term data.

Net benefit assessment in vaccinated populations

In populations vaccinated against human papillomavirus (HPV), the incidence of high-risk HPV infections, precancerous (CIN) grades 2 and 3, and invasive has substantially declined, particularly for vaccine-targeted types such as HPV-16 and HPV-18, which account for approximately 70% of cases. A nationwide Swedish of women aged 10 to 30 found that quadrivalent HPV was associated with an 86% reduction in risk among those vaccinated at ages 12 to 13, and a 68% reduction for those vaccinated at ages 17 to 18, based on data through 2017. Similarly, real-world effectiveness analyses in reported an 86% lower incidence of in women vaccinated before age 17 compared to unvaccinated peers. These reductions imply a lower pretest probability of , decreasing the positive predictive value of Pap tests and potentially diminishing the net benefit by increasing the number needed to screen to prevent one cancer case while maintaining risks of false positives, anxiety, and unnecessary colposcopies. Despite these shifts, major guidelines, including those from the U.S. Preventive Services Task Force (USPSTF) and American Cancer Society (ACS), do not currently differentiate screening intervals or modalities by status, recommending or HPV-based screening from ages 25 to 65 for all women regardless of vaccination, as vaccines do not cover all oncogenic HPV types (e.g., 31, 33, 45, 52, 58) and uptake remains incomplete. Observational data from vaccinated cohorts show up to 60% fewer squamous cells of undetermined significance (ASC-US) or worse results on cytology compared to unvaccinated women, with corresponding drops in high-grade detection rates of 30-50% in programs with high vaccination coverage. Modeling studies project that lifetime CIN3+ risk under five-yearly HPV primary screening falls to very low levels (below 1%) in fully vaccinated birth cohorts, suggesting that of transient low-grade lesions could outweigh benefits if screening frequency is not adjusted. Debates center on whether risk-stratified approaches, such as extended intervals or delayed onset for confirmed individuals, could optimize net benefit by reducing harms without compromising prevention, especially as vaccinated cohorts enter screening age. For instance, analyses indicate that HPV reinforces recommendations for less frequent screening (e.g., every 5-10 years with HPV testing), but residual risks from non-vaccine HPV types and potential failures necessitate continued until population-level elimination thresholds are met. In high- settings like and the , early data show sustained screening efficacy but with lower lesion yields, prompting calls for genotype-specific triage to further minimize referrals in low-prevalence groups. Overall, while enhances primary prevention, Pap testing retains a role in secondary prevention, though its marginal per screen declines, favoring HPV-based over cytology-alone strategies for efficiency.

Critiques of overtreatment incentives and guideline shifts

Critics of cervical screening practices contend that reimbursement structures incentivize physicians to perform frequent tests and follow-up procedures, fostering overtreatment of transient (CIN) lesions that often regress without intervention. In particular, low-grade lesions like CIN1 regress spontaneously in 60% to 90% of cases among women aged 18 to 24 within two years, yet diagnostic colposcopies, biopsies, and excisional treatments such as loop electrosurgical excision procedure (LEEP) are commonly pursued, amplifying procedural volume and revenue. These interventions carry documented reproductive harms, including elevated risks of and mid-trimester loss; meta-analyses indicate that treatments for CIN increase preterm delivery odds by up to twofold compared to untreated cases, with each additional screening in young women associated with a 0.073 rise in preterm delivery risk. In the United States, more aggressive screening and management protocols—such as triennial Pap tests versus quinquennial cytology in the —yield 3.9 times more punch biopsies and 70% more CIN treatments per capita, contributing to an estimated 5,300 excess preterm births annually and 63% more overall health problems from screening-related care. Guideline evolutions, including the U.S. Preventive Services Task Force's 2018 recommendations for combined HPV-Pap co-testing every five years or primary HPV every three years starting at age 30, and cessation after age 65 for low-risk women, represent efforts to curb by prioritizing high-risk human papillomavirus strains and extending intervals from prior annual norms. These shifts acknowledge that excessive screening inflates false-positive rates—up to 4.88 on a 1-7 harm severity scale in patient surveys—and subsequent , particularly as HPV reduces precancer . Nonetheless, critiques persist that systemic incentives undermine adherence, with studies showing 10% to 20% of average-risk U.S. women still undergoing overscreening beyond guidelines, perpetuating unnecessary anxiety, costs, and iatrogenic harms without proportional mortality benefits. In resource-limited settings, "see-and-treat" approaches exacerbate this, overtreating 18% to 71% of screened women due to unverified positives, driven by provider priorities for reimbursable interventions over conservative monitoring.