Estudo de comunidades fúngicas em arquivos: implicações na conservação e na saúde

A influência da contaminação fúngica para a saúde ambiental e para a conservação do património é o tema premente e actual que suscitou a hipótese de estudo aqui apresentada. Os fungos, dada a sua extrema capacidade de adaptação, podem colonizar diversos materiais - orgânicos ou não - e a sua acção pode ser mecânica, por intermédio das suas hifas, ou química, através dos seus metabolitos. Em termos de conservação do património, os estudos sobre fungos têm suscitado grande interesse dada a sua elevada capacidade de biodeterioração. Tendo inicialmente assentado em técnicas tradicionais de cultura, os estudos mais recentes já incluem tecnicas modernas de biologia molecular. O estudo aqui apresentado utiliza ambas as técnicas: a convencional, recorrendo a meios de cultura específicos para o crescimento de fungos e a mais recente, utilizando o DNA fúngico e a amplificação genómica dos mesmos para conseguir identificá-los até ao nível da espécie. Para conseguir realizar este intuito, foi desenvolvida a aplicação da recente técnica de cromatografia líquida desnaturante de alta resolução (DHPLC) à análise de amostras complexas de fungos filamentosos e leveduriformes.

CONTRIBUIÇÃO PARA O DIAGNÓSTICO MOLECULAR DAS ONICOMICOSES

Resumo Onicomicose ou infecção fúngica das unhas das mãos ou dos pés pode ser provocada por fungos que invadem primariamente a lâmina ungueal saudável. Embora existam outros agentes, como por exemplo bactérias, que podem causar infecções ungueais, as infecções causadas por fungos são mais frequentes e são consideradas uma das principais onicopatias do homem. Os efeitos psicológicos e emocionais que resultam dos aspectos clínicos da onicomicose podem ser marcantes e ter um impacto significativo na qualidade de vida dos portadores. É uma doença com grande potencial crónico associada a uma séria dificuldade terapêutica, sendo estes os principais factores agravantes do seu prognóstico. Conforme a extensão do comprometimento e a porção da unha envolvida na onicomicose, a infecção causada por fungos pode ser classificada em 5 tipos: onicomicose subungueal distal e lateral, onicomicose superficial leitosa, onicomicose subungueal proximal, onicomicose com distrofia total e onicomicose por candidose. São causadas por diferentes agentes etiológicos sendo que os mais comuns são os fungos dermatófitos (80 a 90%), seguidos pelas leveduras (5 a 17%) e fungos filamentosos não dermatófitos (2 a 12%). Neste trabalho foram estudadas 54 amostras recolhidas de unhas de doentes com hipótese clínica de onicomicose, das quais 25,93% (14/54) pertenciam a indivíduos do sexo masculino e 74,07% (40/54) a indivíduos do sexo feminino. As técnicas convencionais de diagnóstico são morosas e muitas vezes de difícil caracterização a nível fenotipico, o que condiciona grandemente a implementação da terapêutica adequada. O presente trabalho teve como principal objectivo a aquisição de conhecimentos que permitissem um correcto diagnóstico micológico das onicomicoses, através do isolamento e identificação das espécies de fungos causadoras de infecção. De uma forma global, consistiu inicialmente no isolamento e posteriormente na identificação dos agentes etiológicos de onicomicoses, utilizando para tal metodologias convencionais e moleculares. Foi realizado o diagnóstico laboratorial baseado no exame directo e na cultura de fragmentos de unhas provenientes de doentes com infecção. Paralelamente, foi extraído o DNA fúngico das mesmas amostras clínicas que, após amplificação da região ITS dos genes ribossómicos foi utilizado para confirmação e comparação dos resultados. Foi igualmente estudada a ocorrência de fungos não dermatófitos responsáveis por onicomicose. Os métodos moleculares de diagnóstico podem não só constituir uma alternativa mais rápida de diagnóstico micológico como também, por serem mais sensíveis, permitir a detecção de espécies que, por serem de crescimento fastidioso, não se desenvolvem em cultura.

CONTRIBUIÇÃO PARA O DIAGNÓSTICO MOLECULAR DAS ONICOMICOSES

Onicomicose ou infecção fúngica das unhas das mãos ou dos pés pode ser provocada por fungos que invadem primariamente a lâmina ungueal saudável. Embora existam outros agentes, como por exemplo bactérias, que podem causar infecções ungueais, as infecções causadas por fungos são mais frequentes e são consideradas uma das principais onicopatias do homem. Os efeitos psicológicos e emocionais que resultam dos aspectos clínicos da onicomicose podem ser marcantes e ter um impacto significativo na qualidade de vida dos portadores. É uma doença com grande potencial crónico associada a uma séria dificuldade terapêutica, sendo estes os principais factores agravantes do seu prognóstico. Conforme a extensão do comprometimento e a porção da unha envolvida na onicomicose, a infecção causada por fungos pode ser classificada em 5 tipos: onicomicose subungueal distal e lateral, onicomicose superficial leitosa, onicomicose subungueal proximal, onicomicose com distrofia total e onicomicose por candidose. São causadas por diferentes agentes etiológicos sendo que os mais comuns são os fungos dermatófitos (80 a 90%), seguidos pelas leveduras (5 a 17%) e fungos filamentosos não dermatófitos (2 a 12%). Neste trabalho foram estudadas 54 amostras recolhidas de unhas de doentes com hipótese clínica de onicomicose, das quais 25,93% (14/54) pertenciam a indivíduos do sexo masculino e 74,07% (40/54) a indivíduos do sexo feminino. As técnicas convencionais de diagnóstico são morosas e muitas vezes de difícil caracterização a nível fenotipico, o que condiciona grandemente a implementação da terapêutica adequada. O presente trabalho teve como principal objectivo a aquisição de conhecimentos que permitissem um correcto diagnóstico micológico das onicomicoses, através do isolamento e identificação das espécies de fungos causadoras de infecção. De uma forma global, consistiu inicialmente no isolamento e posteriormente na identificação dos agentes etiológicos de onicomicoses, utilizando para tal metodologias convencionais e moleculares. Foi realizado o diagnóstico laboratorial baseado no exame directo e na cultura de fragmentos de unhas provenientes de doentes com infecção. Paralelamente, foi extraído o DNA fúngico das mesmas amostras clínicas que, após amplificação da região ITS dos genes ribossómicos foi utilizado para confirmação e comparação dos resultados. Foi igualmente estudada a ocorrência de fungos não dermatófitos responsáveis por onicomicose. Os métodos moleculares de diagnóstico podem não só constituir uma alternativa mais rápida de diagnóstico micológico como também, por serem mais sensíveis, permitir a detecção de espécies que, por serem de crescimento fastidioso, não se desenvolvem em cultura.

Polymerase Chain Reaction Screening for Fungemia and/or Invasive Fungal Infections in Patients with Hematologic Malignancies

INTRODUCTION: Invasive fungal infections (IFIs) are a life-threatening complication in patients with hematologic malignancies, mainly in acute leukemia patients, following chemotherapy. IFI incidence is increasing, and associated mortality remains high due to unreliable diagnosis. Antifungal drugs are often limited by inadequate antimicrobial spectrum and side effects. Thus, the detection of circulating fungal DNA has been advocated as a rapid, more sensitive diagnostic tool. PATIENTS AND METHODS: Between June 01 and January 03, weekly blood samples (1,311) were screened from 193 patients undergoing intensive myelosuppressive or immunosuppressive therapy. IFI cases were classified according to European Organization for Research and Treatment of Cancer/Mycoses Study Group criteria. Fungal DNA was extracted from whole blood and amplified using polymerase chain reaction (PCR) published primers that bind to the conserved regions of the fungal 18S rRNA gene sequence. In our study, two or more consecutive positive samples were always associated with fungal disease. RESULTS: PCR screening predicted the development of IFI to be 17 days (median). This test had a specificity of 91.1% and a sensitivity of 75%. IFI incidence was 7.8%. DISCUSSION: Therefore, our results confirm the potential usefulness of PCR serial screening and the clinical applicability in everyday routine. PCR screening offers a noninvasive repeatable aid to the diagnosis of IFI.

Nova abordagem no diagnóstico de infecções invasivas por fungos do género Aspergillus

Nas últimas duas décadas tem-se verificado um aumento da incidência de aspergilose pulmonar invasiva, que se reflecte em taxas de mortalidade e morbilidade extremamente elevadas. Esta realidade resulta da elevada utilização de quimioterapia e de agentes imunossupressores, usados sobretudo em doentes imunocomprometidos, principalmente, em doentes hemato-oncológicos e receptores de transplante de medula óssea. Estas infecções fúngicas são provocadas por algumas espécies do género Aspergillus em que Aspergillus fumigatus é a espécie mais frequentemente isolada a partir de infecções humanas. Contudo, outras espécies como A. flavus, A. niger, A. glaucus, A. nidulans, A. terreus ou A. versicolor também podem ser responsáveis por infecções fúngicas no Homem. Um factor determinante para o aumento da incidência de aspergilose invasiva consiste na incapacidade de se estabelecer um diagnóstico precoce definitivo para que, em tempo útil, possa ser instituída terapêutica antifúngica que vá seguramente melhorar o prognóstico desses doentes. Actualmente, as técnicas convencionais (microbiológicas e histológicas) têm servido como linhas de orientação para o diagnóstico definitivo de micoses. No entanto, como se tratam técnicas morosas, o diagnóstico imunológico e molecular tem todas as potencialidades para oferecer uma abordagem promissora no diagnóstico de infecções fúngicas. Neste trabalho foram estudadas 37 amostras clínicas, das quais 45,9% pertenciam a indivíduos do sexo feminino, 54,1% do sexo masculino, maioritariamente com o diagnóstico clínico de leucemia mielóide aguda (75,7%). O principal objectivo deste trabalho consistiu na comparação dos resultados obtidos por uma técnica imunológica utilizada no diagnóstico de aspergilose pulmonar invasiva (pesquisa do antigénio GM) com uma nova técnica molecular de diagnóstico (nested-PCR), com o intuito de avaliar a sensibilidade e especificidade dos resultados obtidos. Dos 37 doentes do estudo, 35,1% revelaram presença do antigénio galactomanano e em 32,4% das amostras foi possível detectar DNA fúngico utilizando primers específicos numa reacção de nested-PCR. No final deste trabalho pode-se constatar que, em virtude do método molecular utilizando uma reacção de nested-PCR não se ter revelado mais sensível que a pesquisa do antigénio galactomanano, julgamos ser no entanto muito promissor no diagnóstico da aspergilose pulmonar invasiva, bastando apenas aperfeiçoar a sua optimização.

Dna Extraction From Filter-paper Spots Of Vaginal Samples Collected After Sexual Violence.

To detect the presence of male DNA in vaginal samples collected from survivors of sexual violence and stored on filter paper. A pilot study was conducted to evaluate 10 vaginal samples spotted on sterile filter paper: 6 collected at random in April 2009 and 4 in October 2010. Time between sexual assault and sample collection was 4-48hours. After drying at room temperature, the samples were placed in a sterile envelope and stored for 2-3years until processing. DNA extraction was confirmed by polymerase chain reaction for human β-globin, and the presence of prostate-specific antigen (PSA) was quantified. The presence of the Y chromosome was detected using primers for sequences in the TSPY (Y7/Y8 and DYS14) and SRY genes. β-Globin was detected in all 10 samples, while 2 samples were positive for PSA. Half of the samples amplified the Y7/Y8 and DYS14 sequences of the TSPY gene and 30% amplified the SRY gene sequence of the Y chromosome. Four male samples and 1 female sample served as controls. Filter-paper spots stored for periods of up to 3years proved adequate for preserving genetic material from vaginal samples collected following sexual violence.

Analysis Of The Dna Fourier Transform-infrared Microspectroscopic Signature Using An All-reflecting Objective.

The Fourier transform-infrared (FT-IR) signature of dry samples of DNA and DNA-polypeptide complexes, as studied by IR microspectroscopy using a diamond attenuated total reflection (ATR) objective, has revealed important discriminatory characteristics relative to the PO2(-) vibrational stretchings. However, DNA IR marks that provide information on the sample's richness in hydrogen bonds have not been resolved in the spectral profiles obtained with this objective. Here we investigated the performance of an all reflecting objective (ARO) for analysis of the FT-IR signal of hydrogen bonds in DNA samples differing in base richness types (salmon testis vs calf thymus). The results obtained using the ARO indicate prominent band peaks at the spectral region representative of the vibration of nitrogenous base hydrogen bonds and of NH and NH2 groups. The band areas at this spectral region differ in agreement with the DNA base richness type when using the ARO. A peak assigned to adenine was more evident in the AT-rich salmon DNA using either the ARO or the ATR objective. It is concluded that, for the discrimination of DNA IR hydrogen bond vibrations associated with varying base type proportions, the use of an ARO is recommended.

Prognostic Value Of Dna And Mrna E6/e7 Of Human Papillomavirus In The Evolution Of Cervical Intraepithelial Neoplasia Grade 2.

This study aimed at evaluating whether human papillomavirus (HPV) groups and E6/E7 mRNA of HPV 16, 18, 31, 33, and 45 are prognostic of cervical intraepithelial neoplasia (CIN) 2 outcome in women with a cervical smear showing a low-grade squamous intraepithelial lesion (LSIL). This cohort study included women with biopsy-confirmed CIN 2 who were followed up for 12 months, with cervical smear and colposcopy performed every three months. Women with a negative or low-risk HPV status showed 100% CIN 2 regression. The CIN 2 regression rates at the 12-month follow-up were 69.4% for women with alpha-9 HPV versus 91.7% for other HPV species or HPV-negative status (P < 0.05). For women with HPV 16, the CIN 2 regression rate at the 12-month follow-up was 61.4% versus 89.5% for other HPV types or HPV-negative status (P < 0.05). The CIN 2 regression rate was 68.3% for women who tested positive for HPV E6/E7 mRNA versus 82.0% for the negative results, but this difference was not statistically significant. The expectant management for women with biopsy-confirmed CIN 2 and previous cytological tests showing LSIL exhibited a very high rate of spontaneous regression. HPV 16 is associated with a higher CIN 2 progression rate than other HPV infections. HPV E6/E7 mRNA is not a prognostic marker of the CIN 2 clinical outcome, although this analysis cannot be considered conclusive. Given the small sample size, this study could be considered a pilot for future larger studies on the role of predictive markers of CIN 2 evolution.

Phylogenetics, Ancestral State Reconstruction, And A New Infrafamilial Classification Of The Pantropical Ochnaceae (medusagynaceae, Ochnaceae S.str., Quiinaceae) Based On Five Dna Regions.

Ochnaceae s.str. (Malpighiales) are a pantropical family of about 500 species and 27 genera of almost exclusively woody plants. Infrafamilial classification and relationships have been controversial partially due to the lack of a robust phylogenetic framework. Including all genera except Indosinia and Perissocarpa and DNA sequence data for five DNA regions (ITS, matK, ndhF, rbcL, trnL-F), we provide for the first time a nearly complete molecular phylogenetic analysis of Ochnaceae s.l. resolving most of the phylogenetic backbone of the family. Based on this, we present a new classification of Ochnaceae s.l., with Medusagynoideae and Quiinoideae included as subfamilies and the former subfamilies Ochnoideae and Sauvagesioideae recognized at the rank of tribe. Our data support a monophyletic Ochneae, but Sauvagesieae in the traditional circumscription is paraphyletic because Testulea emerges as sister to the rest of Ochnoideae, and the next clade shows Luxemburgia+Philacra as sister group to the remaining Ochnoideae. To avoid paraphyly, we classify Luxemburgieae and Testuleeae as new tribes. The African genus Lophira, which has switched between subfamilies (here tribes) in past classifications, emerges as sister to all other Ochneae. Thus, endosperm-free seeds and ovules with partly to completely united integuments (resulting in an apparently single integument) are characters that unite all members of that tribe. The relationships within its largest clade, Ochnineae (former Ochneae), are poorly resolved, but former Ochninae (Brackenridgea, Ochna) are polyphyletic. Within Sauvagesieae, the genus Sauvagesia in its broad circumscription is polyphyletic as Sauvagesia serrata is sister to a clade of Adenarake, Sauvagesia spp., and three other genera. Within Quiinoideae, in contrast to former phylogenetic hypotheses, Lacunaria and Touroulia form a clade that is sister to Quiina. Bayesian ancestral state reconstructions showed that zygomorphic flowers with adaptations to buzz-pollination (poricidal anthers), a syncarpous gynoecium (a near-apocarpous gynoecium evolved independently in Quiinoideae and Ochninae), numerous ovules, septicidal capsules, and winged seeds with endosperm are the ancestral condition in Ochnoideae. Although in some lineages poricidal anthers were lost secondarily, the evolution of poricidal superstructures secured the maintenance of buzz-pollination in some of these genera, indicating a strong selective pressure on keeping that specialized pollination system.

Diet Carotenoid Lutein Modulates The Expression Of Genes Related To Oxygen Transporters And Decreases Dna Damage And Oxidative Stress In Mice.

Lutein (LT) is a carotenoid obtained by diet and despite its antioxidant activity had been biochemically reported, few studies are available concerning its influence on the expression of antioxidant genes. The expression of 84 genes implicated in antioxidant defense was quantified using quantitative reverse transcription polymerase chain reaction array. DNA damage was measured by comet assay and glutathione (GSH) and thiobarbituric acid reactive substances (TBARS) were quantified as biochemical parameters of oxidative stress in mouse kidney and liver. cDDP treatment reduced concentration of GSH and increased TBARS, parameters that were ameliorated in treatment associated with LT. cDDP altered the expression of 32 genes, increasing the expression of GPx2, APC, Nqo1 and CCs. LT changed the expression of 37 genes with an induction of 13 mainly oxygen transporters. In treatments associating cDDP and LT, 30 genes had their expression changed with a increase of the same genes of the cDDP treatment alone. These results suggest that LT might act scavenging reactive species and also inducing the expression of genes related to a better antioxidant response, highlighting the improvement of oxygen transport. This improved redox state of the cell through LT treatment could be related to the antigenotoxic and antioxidant effects observed.

Changes In Liver Cell Dna Methylation Status In Diabetic Mice Affect Its Ft-ir Characteristics.

Lower levels of cytosine methylation have been found in the liver cell DNA from non-obese diabetic (NOD) mice under hyperglycemic conditions. Because the Fourier transform-infrared (FT-IR) profiles of dry DNA samples are differently affected by DNA base composition, single-stranded form and histone binding, it is expected that the methylation status in the DNA could also affect its FT-IR profile. The DNA FT-IR signatures obtained from the liver cell nuclei of hyperglycemic and normoglycemic NOD mice of the same age were compared. Dried DNA samples were examined in an IR microspectroscope equipped with an all-reflecting objective (ARO) and adequate software. Changes in DNA cytosine methylation levels induced by hyperglycemia in mouse liver cells produced changes in the respective DNA FT-IR profiles, revealing modifications to the vibrational intensities and frequencies of several chemical markers, including νas -CH3 stretching vibrations in the 5-methylcytosine methyl group. A smaller band area reflecting lower energy absorbed in the DNA was found in the hyperglycemic mice and assumed to be related to the lower levels of -CH3 groups. Other spectral differences were found at 1700-1500 cm(-1) and in the fingerprint region, and a slight change in the DNA conformation at the lower DNA methylation levels was suggested for the hyperglycemic mice. The changes that affect cytosine methylation levels certainly affect the DNA-protein interactions and, consequently, gene expression in liver cells from the hyperglycemic NOD mice.

A Modified Acidic Approach For Dna Extraction From Plant Species Containing High Levels Of Secondary Metabolites.

Purified genomic DNA can be difficult to obtain from some plant species because of the presence of impurities such as polysaccharides, which are often co-extracted with DNA. In this study, we developed a fast, simple, and low-cost protocol for extracting DNA from plants containing high levels of secondary metabolites. This protocol does not require the use of volatile toxic reagents such as mercaptoethanol, chloroform, or phenol and allows the extraction of high-quality DNA from wild and cultivated tropical species.

Human Herpesvirus-6 And Cytomegalovirus Dna In Liver Donor Biopsies And Their Correlation With Hla Matches And Acute Cellular Rejection.

Herpesvirus reactivation is common after liver transplantation. Analyze the presence of cytomegalovirus (HCMV) and human herpesvirus-6 (HHV-6) DNA in liver donor biopsies, seeking to better understand issues involving human donor leukocyte antigens (HLA)-A, B and DR, as well as correlations with acute cellular rejection. Fifty-nine liver transplantation patients were investigated for the presence of HCMV and HHV-6 DNA in liver donor biopsies, using the Nested-PCR technique. The clinical donor information and HLA matches were obtained from the São Paulo State Transplant System. The recipients' records regarding acute cellular rejection were studied. Seven (11.8%) biopsies were positive for HCMV DNA and 29 (49%) were positive for HHV-6 DNA. In 14 donors with HLA-DR 15 nine had HHV-6 DNA positive liver biopsy with a tendency for significant association (p=0.09), 22 recipients developed acute cellular rejection and 9/22 were positive for HLA-DR 15 (p=0.03; χ(2)=4.51), which was statistically significant in univariate analysis and showed a tendency after multivariate analysis (p=0.08). HHV-6 DNA was prevalent in liver donors studied as well as HLA-DR 15. These findings suggest that patients with HLA-DR 15 in liver donor biopsies develop more rejection after liver transplantation.

On The Consistency Of Monte Carlo Track Structure Dna Damage Simulations.

Monte Carlo track structures (MCTS) simulations have been recognized as useful tools for radiobiological modeling. However, the authors noticed several issues regarding the consistency of reported data. Therefore, in this work, they analyze the impact of various user defined parameters on simulated direct DNA damage yields. In addition, they draw attention to discrepancies in published literature in DNA strand break (SB) yields and selected methodologies. The MCTS code Geant4-DNA was used to compare radial dose profiles in a nanometer-scale region of interest (ROI) for photon sources of varying sizes and energies. Then, electron tracks of 0.28 keV-220 keV were superimposed on a geometric DNA model composed of 2.7 × 10(6) nucleosomes, and SBs were simulated according to four definitions based on energy deposits or energy transfers in DNA strand targets compared to a threshold energy ETH. The SB frequencies and complexities in nucleosomes as a function of incident electron energies were obtained. SBs were classified into higher order clusters such as single and double strand breaks (SSBs and DSBs) based on inter-SB distances and on the number of affected strands. Comparisons of different nonuniform dose distributions lacking charged particle equilibrium may lead to erroneous conclusions regarding the effect of energy on relative biological effectiveness. The energy transfer-based SB definitions give similar SB yields as the one based on energy deposit when ETH ≈ 10.79 eV, but deviate significantly for higher ETH values. Between 30 and 40 nucleosomes/Gy show at least one SB in the ROI. The number of nucleosomes that present a complex damage pattern of more than 2 SBs and the degree of complexity of the damage in these nucleosomes diminish as the incident electron energy increases. DNA damage classification into SSB and DSB is highly dependent on the definitions of these higher order structures and their implementations. The authors' show that, for the four studied models, different yields are expected by up to 54% for SSBs and by up to 32% for DSBs, as a function of the incident electrons energy and of the models being compared. MCTS simulations allow to compare direct DNA damage types and complexities induced by ionizing radiation. However, simulation results depend to a large degree on user-defined parameters, definitions, and algorithms such as: DNA model, dose distribution, SB definition, and the DNA damage clustering algorithm. These interdependencies should be well controlled during the simulations and explicitly reported when comparing results to experiments or calculations.

Post Hoc Analysis Of The Patricia Randomized Trial Of The Efficacy Of Human Papillomavirus Type 16 (hpv-16)/hpv-18 As04-adjuvanted Vaccine Against Incident And Persistent Infection With Nonvaccine Oncogenic Hpv Types Using An Alternative Multiplex Type-specific Pcr Assay For Hpv Dna.

The efficacy of the human papillomavirus type 16 (HPV-16)/HPV-18 AS04-adjuvanted vaccine against cervical infections with HPV in the Papilloma Trial against Cancer in Young Adults (PATRICIA) was evaluated using a combination of the broad-spectrum L1-based SPF10 PCR-DNA enzyme immunoassay (DEIA)/line probe assay (LiPA25) system with type-specific PCRs for HPV-16 and -18. Broad-spectrum PCR assays may underestimate the presence of HPV genotypes present at relatively low concentrations in multiple infections, due to competition between genotypes. Therefore, samples were retrospectively reanalyzed using a testing algorithm incorporating the SPF10 PCR-DEIA/LiPA25 plus a novel E6-based multiplex type-specific PCR and reverse hybridization assay (MPTS12 RHA), which permits detection of a panel of nine oncogenic HPV genotypes (types 16, 18, 31, 33, 35, 45, 52, 58, and 59). For the vaccine against HPV types 16 and 18, there was no major impact on estimates of vaccine efficacy (VE) for incident or 6-month or 12-month persistent infections when the MPTS12 RHA was included in the testing algorithm versus estimates with the protocol-specified algorithm. However, the alternative testing algorithm showed greater sensitivity than the protocol-specified algorithm for detection of some nonvaccine oncogenic HPV types. More cases were gained in the control group than in the vaccine group, leading to higher point estimates of VE for 6-month and 12-month persistent infections for the nonvaccine oncogenic types included in the MPTS12 RHA assay (types 31, 33, 35, 45, 52, 58, and 59). This post hoc analysis indicates that the per-protocol testing algorithm used in PATRICIA underestimated the VE against some nonvaccine oncogenic HPV types and that the choice of the HPV DNA testing methodology is important for the evaluation of VE in clinical trials. (This study has been registered at ClinicalTrials.gov under registration no. NCT00122681.).