ABSTRACT
The aim of this study was to investigate an outbreak caused by protozoa, which occurred in a municipality in the Brazil southern region. The investigations were carried out analyzing 47 fresh stool samples and 26 water samples by parasitological and molecular methods, as well as, direct immunofluorescence. After the filtrations of water samples and purification of stool samples, the concentrates were evaluated microscopically for presence of parasites. Molecular analyses were performed by polymerase chain reaction (PCR) for DNA detection of Giardia spp., Cryptosporidium parvum, C. hominis and Cyclospora cayetanensis. Out of 26 water samples, 30.8% (8/26) had waterborne protozoa and C. cayetanensis was the most prevalent (15.5%). Out of the 47 stool samples, 23.4% (11/47) were infected with C. cayetanensis and Giardia spp. The results showed that backwash water samples from filters of the Water Treatment Station were contaminated with C. cayetanensis, C. hominis and Giardia spp., suggesting the contamination of water sources with human waste brought by sewage. These results show the importance of protozoa investigation in water and stool samples by laboratory methodologies principally in outbreaks causing acute diarrheal disease (AU).
O objetivo do presente estudo foi investigar um surto causado por protozoários, ocorrido em um município da região sul do Brasil. As investigações foram realizadas analisando 47 amostras de fezes frescas e 26 amostras de água por métodos parasitológicos, moleculares e de imunofluorscência direta. Após as filtrações das amostras de água e purificação das amostras de fezes, os concentrados foram avaliados microscopicamente a procura de parasitas. A seguir, foram analisadas, pela reação em cadeia da polimerase (PCR), a detecção de DNA de Giardia spp., Cryptosporidium parvum, C. hominis e Cyclospora cayetanensis. Das 26 amostras de água, 30,8% (8/26) apresentaram protozoários de veiculação hídrica, sendo que, C. cayetanensis foi o mais prevalente (15,5%). Das 47 amostras de fezes, 23,4% (11/47) estavam infectadas por C. cayetanensis e Giardia spp. Os resultados mostraram que as águas de retrolavagem dos filtros da Estação de Tratamento de Água estavam contaminadas com C. cayetanensis, C. hominis e Giardia spp. sugerindo a contaminação dos mananciais com dejetos humanos trazidos pelo esgoto. Estes resultados mostram a importância da investigação de protozoários em água e fezes por metodologias laboratoriais, principalmente em surtos que causam doença diarreica aguda (AU).
Subject(s)
Protozoan Infections , Disease Outbreaks , Cryptosporidium , Cyclospora , Diarrhea , Waterborne Diseases , GiardiaABSTRACT
This study investigated the genetic features of T. gondii isolated directly in autopsies of HIV-infected patients who died with severe disseminated toxoplasmosis. This retrospective analysis was conducted in a cohort of 15 HIV-infected patients with clinical and laboratory data. They had previous cerebral toxoplasmosis at least 6 months before the disseminated toxoplasmosis episode. The hypothesis was that they were infected with highly virulent parasites due to the condition in which they died. T. gondii genotyping was done directly in DNA extracted from 30 autopsy brain and lung samples (2 per patient) and mutilocus PCR-RFLP genotyping was done using 12 molecular markers. The 30 clinical samples were genotyped successfully in 8 or more loci and six suggestive genotypes were identified. One of them was Toxo DB #11, previously identified in different domestic animals and virulent in experimental animals. The other five suggestive genotypes...(AU)
Subject(s)
Toxoplasma , Acquired Immunodeficiency Syndrome , DNA, A-FormABSTRACT
BACKGROUND: Cerebral toxoplasmosis (CT) continues to cause significant morbidity and mortality in human immunodeficiency virus (HIV)-infected patients in Brazil. In clinical practice, the initial diagnosis is usually presumptive and alternative diagnosis tools are necessary. Our objective was to evaluate whether the detection of high titers of IgG anti-Toxoplasma gondii and T. gondii DNA in blood samples are associated with the diagnosis of CT. METHODS: In this case-control study we included 192 patients with HIV-1 infection: 64 patients with presumptive CT (cases) and 128 patients with other diseases (controls). Blood samples to perform indirect immunofluorescense reaction (IFI) to detect anti-T. gondii IgG antibodies and polymerase chain reaction (PCR) were collected before or within the first three days of anti-Toxoplasma therapy. Two multivariate logistic regression models were performed: one including the variable qualitative serology and another including quantitative serology. RESULTS: In the first model, positive IgG anti-T. gondii (OR 4.7, 95 percent CI 1.2-18.3; p = 0.027) and a positive T. gondii PCR result (OR 132, 95 percent CI 35-505; p < 0.001) were associated with the diagnosis. In the second model, IgG anti-T. gondii titres > 1:1024 (OR 7.6, 95 percent CI 2.3-25.1; p = 0.001) and a positive T. gondii PCR result (OR 147, 95 percent CI 35-613; p < 0.001) were associated with the diagnosis. CONCLUSIONS: Quantitative serology and molecular diagnosis in peripheral blood samples were independently associated with the diagnosis of CT in HIV-infected patients. These diagnostic tools can contribute to a timely diagnosis of CT in settings where Toxoplasma infection is common in the general population.
Subject(s)
Adult , Female , Humans , Male , AIDS-Related Opportunistic Infections/diagnosis , Antibodies, Protozoan/blood , DNA, Protozoan/blood , Immunoglobulin G/blood , Toxoplasma/genetics , Toxoplasma/immunology , Toxoplasmosis, Cerebral/diagnosis , AIDS-Related Opportunistic Infections/parasitology , Case-Control Studies , Fluorescent Antibody Technique, Indirect , Polymerase Chain Reaction , Sensitivity and SpecificityABSTRACT
Objetivos: analisar experimentalmente a evolução da resposta imune humoral nas fases aguda e crônica recente da infecção por Toxoplasma gondii e sua correlação com o parasitismo sanguíneo. Métodos: foram analisados, por 60 dias, 10 camundongos fêmeas da linhagem AS/n infectados, por via oral, com 10 cistos por animal da cepa ME-49 de Toxoplasma gondii. As coletas de sangue foram feitas a cada 3-4 dias. O parasitismo sanguíneo foi avaliado pela reação em cadeia da polimerase e os títulos de anticorpos por enzimaimunoensaio e imunofluorescência indireta. Resultados: a reação em cadeia da polimerase foi positiva em amostras com intervalos de aproximadamente 7 dias até o 28º dia, e a seguir, negativas até o 60º dia. Os soros avaliados pela imunofluorescência indireta apresentaram anticorpos IgM após o 7º dia, com pico entre o 18º e 27º dia. Após o primeiro mês os títulos foram baixos até o 60º dia. Anticorpos IgG surgiram no 14º dia e persistiram em altos títulos até o 60º dia. A cinética dos anticorpos IgG, bem como a avidez destes, demonstrou que os níveis de anticorpos aumentaram a partir do 14º dia e as porcen-tagens de avidez evoluíram com pico máximo após 28 dias, estabelecendo-se então a fase crônica da infecção. Conclusões: os dados aqui demonstrados enfatizam que taquizoítos podem estar presentes na circulação sanguínea durante toda a fase aguda da toxoplasmose, mesmo que já se tenha instalado a resposta imune protetora.
Aims: To analyze experimentally the humoral immune response in acute and recent chronic infections by Toxoplasma gondii and its correlation with the blood parasitism. Methods: Ten female mice AS/n inbred strain orally infected with 10 cysts per animal from T. gondii ME-49 strain were evaluated during 60 days. Blood collections were made in each 3-4 days. Blood parasitism was evaluated by polymerase chain reaction, and antibody titres by enzyme-linked immunosorbent assay and indirect immunofluorescence. Results: Positive polymerase chain reaction was detected around seven day-intervals until the 28th day and was negative after the 30th day pos-infection. Sera assayed by immunofluorescence presented IgM antibodies after the 7th day of infection and high titers were found between the 18th and 27th day. After 30 days, IgM titers were low until the 60th day. IgG antibodies were produced around the 14th day and were high until the 60th day. The avidity and kinetic exhibited by IgG antibody levels increased from the 14th day and the avidity percents increased with maximum peak after 28 days, establishing the chronic infection. Conclusions: These data emphasize that tachyzoites can be detected in blood during the acute phase of toxoplasmosis, even though the protective immune response was already developed.