Your search keyword '"real-time pcr"' showing total 40 results

1. Validation of the NAT Chagas IVD Kit for the Detection and Quantification of Trypanosoma cruzi in Blood Samples of Patients with Chagas Disease.

Author

Moreira, Otacilio C., Fernandes, Alice Gomes, Gomes, Natalia Lins da Silva, dos Santos, Carolina Messias, Jacomasso, Thiago, Costa, Alexandre Dias Tavares, Nascimento, Lucas de O. Rossetti, Hasslocher-Moreno, Alejandro Marcel, do Brasil, Pedro Emmanuel Alvarenga Americano, Morello, Luis Gustavo, Marchini, Fabricio Klerynton, Krieger, Marco Aurelio, and Britto, Constança

Subjects

*CHAGAS' disease, *TRYPANOSOMA cruzi, *BLOOD sampling, *SATELLITE DNA, *CURRENT good manufacturing practices, *DIAGNOSTIC reagents & test kits

Abstract

In the absence of validated biomarkers to control the cure of Chagas disease, PCR-based diagnosis is being used as the main tool for an early indication of therapeutic failure. However, since it is considered a technique of complex reproducibility, mainly due to difficulties in establishing accurate controls to guarantee the quality of the reaction, the use of PCR for Chagas disease diagnosis is restricted to specialized centers. In an effort to disseminate the molecular diagnosis of Chagas disease and its applications, new diagnostic kits based on qPCR have been made available in the market in recent years. Here, we show the results of the validation of the NAT Chagas kit (Nucleic Acid Test for Chagas Disease) for the detection and quantification of T. cruzi in blood samples of patients suspected of Chagas disease infection. The kit, composed of a TaqMan duplex reaction targeting the T. cruzi satellite nuclear DNA and an exogenous internal amplification control, presented a reportable range from 104 to 0.5 parasite equivalents/mL and a limit of detection (LOD) of 0.16 parasite equivalents/mL of blood. In addition, the NAT Chagas kit detected T. cruzi belonging to all six discrete typing units (DTUs—TcI to TcVI), similarly to the in-house real-time PCR performed with commercial reagents, which has been selected as the best performance assay in the international consensus for the validation of qPCR for Chagas disease. In the clinical validation presented here, the kit showed 100% sensitivity and 100% specificity when compared to the consensus in-house real-time PCR assay. Thus, the NAT Chagas kit, which is produced entirely in Brazil under the international standards of good manufacturing practices (GMP), appears as an excellent alternative to enable the molecular diagnosis of Chagas disease in public and private diagnostic centers, as well as to facilitate the monitoring of patients under etiological treatment participating in clinical trials. [ABSTRACT FROM AUTHOR]

Published

2023

2. Trichilia catigua against Helicobacter pylori: An in vitro, molecular and in silico approach.

Author

Ritter MR, Oliveira MT, Ardisson JS, Gonçalves RCR, Kitagawa RR, Lima DS, Seixas FAV, Nakamura CV, and Mello JCP

Subjects

Brazil, Virulence Factors, Meliaceae chemistry, Clarithromycin pharmacology, Urease, Drug Synergism, Antigens, Bacterial, Helicobacter pylori drug effects, Anti-Bacterial Agents pharmacology, Anti-Bacterial Agents chemistry, Microbial Sensitivity Tests, Molecular Docking Simulation, Plant Extracts pharmacology, Plant Extracts chemistry, Plant Bark chemistry, Bacterial Proteins

Abstract

Helicobacter pylori is a bacterium that is present in the stomach of about 50% of the global population and is associated with several gastric disorders, including cancer. Natural products with antimicrobial activity have been tested against H. pylori, among them Trichilia catigua (catuaba), which is widely distributed in Brazil. This study aimed to evaluate extracts of T. catigua bark against H. pylori via determination of the minimum inhibitory and bactericidal concentrations (MIC and MBC); evaluation of virulence factors by real-time PCR, synergism with standard antimicrobials and morphology by scanning electron microscopy and simulations of the mechanism of action by molecular docking. The ethyl acetate fraction provided the best results, with an MIC 50 of 250 μg/mL and a 42.34% reduction in urease activity, along with reduced expression of the CagA and VacA genes, which encode for the main virulence factors. This fraction presented synergistic activity with clarithromycin, reducing the MIC of the drug by four-fold. Docking simulations suggested that the extracts inhibit fatty acid synthesis by the FAS-II system, causing damage to the cell membrane. Therefore, T. catigua extracts have potential as an adjuvant to treatment and are promising for the development of new anti-H. pylori drugs., Competing Interests: Declaration of competing interest The authors declare no conflicts of interest., (Copyright © 2023. Published by Elsevier B.V.)

Published

2024

3. Prevalence of Leishmania infection in 205 cats from a referral hospital population in Brazil (2021-2022).

Author

Paiva BL, Sousa-Paula LC, Sales KGDS, Costa KMV, Venuto AM, Oriente VND, Cavalcante FRA, Brito RLL, Santos JMLD, and Dantas-Torres F

Subjects

Animals, Cats, Brazil epidemiology, Prevalence, Female, Male, Leishmania isolation & purification, Leishmaniasis, Visceral veterinary, Leishmaniasis, Visceral epidemiology, Leishmaniasis, Visceral parasitology, Real-Time Polymerase Chain Reaction veterinary, Hospitals, Animal, Leishmania infantum isolation & purification, Cat Diseases epidemiology, Cat Diseases parasitology, Leishmaniasis veterinary, Leishmaniasis epidemiology, Leishmaniasis parasitology

Abstract

Leishmaniases are a group of neglected diseases of significant public health concern, with Brazil being the primary focus of this disease in the Americas. The municipality of Sobral, in the state of Ceará, is a historical focus of visceral leishmaniasis in both humans and dogs, but data on Leishmania spp. infections in cats are limited. Between April 2021 and February 2022, 205 cats from a referral hospital population were sampled and tested for Leishmania spp. by real-time PCR. Eight cats (3.9%; 95% CI: 1.7-7.5%) tested positive. Among these, three (37.5%) displayed clinical signs compatible with feline leishmaniosis. Non-domiciled cats showed significantly higher positivity compared to domiciled ones (Fisher's exact test, P = 0.0124). Considering their potential role as reservoirs of L. infantum, it is crucial to conduct further studies to understand the Leishmania spp. circulating among cats in Sobral and to implement measures for reducing their exposure to phlebotomine sand fly vectors in this important focus of leishmaniases., Competing Interests: Declaration of competing interest The authors declare no conflicts of interest., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

4. A Real-Time PCR Assay for the Diagnosis of Intestinal Schistosomiasis and Cure Assessment After the Treatment of Individuals With Low Parasite Burden.

Author

Siqueira, Liliane Maria Vidal, Senra, Carolina, de Oliveira, Áureo Almeida, Carneiro, Nidia Francisca de Figueiredo, Gomes, Luciana Inácia, Rabello, Ana, Coelho, Paulo Marcos Zech, and Oliveira, Edward

Subjects

INTESTINES, SCHISTOSOMIASIS, DIAGNOSIS, INFECTIOUS disease transmission, INTERNAL auditing

Abstract

The laboratorial diagnosis of the intestinal schistosomiasis is always performed using Kato-Katz technique. However, this technique presents low sensitivity for diagnosis of individuals with low parasite burden, which constitutes the majority in low endemicity Brazilian locations for the disease. The objective of this study was developed and to validate a real-time PCR assay (qPCR) targeting 121 bp sequence to detect Schistosoma spp. DNA for the diagnosis of intestinal schistosomiasis and a sequence of the human β-actin gene as internal control. Firstly, the qPCR was standardized and next it was evaluated for diagnosis and cure assessment of intestinal schistosomiasis in the resident individuals in Tabuas and Estreito de Miralta, two locations in Brazil endemic for intestinal schistosomiasis. The qPCR assay results were compared with those of the Kato-Katz (KK) test, examining 2 or 24 slides, Saline Gradient (SG) and "reference test" (24 KK slides + SG). The cure assessment was measured by these diagnostic techniques at 30, 90, and 180 days post-treatment. In Tabuas, the positivity rates obtained by the qPCR was 30.4% (45/148) and by "reference test" was of 31.0% (46/148), with no statistical difference (p = 0.91). The presumed cure rates at 30, 90, and 180 days post-treatment were 100, 94.4, and 78.4% by the analysis of 24 KK slides, 100, 94.4, and 78.4% by the SG, and 100, 83.3, and 62.1% by the qPCR assay. In Estreito de Miralta, the positivity obtained by qPCR was 18.3% (26/142) and with "reference test" was 24.6% (35/142), with no statistical difference (p = 0.20). The presumed cure rates were 93.3, 96.9, and 96.5% by the KK, 93.3, 96.9, and 100% by the SG, and 93.3, 93.9, and 96.5% by the qPCR at 30, 90, and 180 days post-treatment, respectively. This study showed that the diagnostic techniques presented different performance in the populations from the two districts (Tabuas and Estreito de Miralta) and reinforces the need of combining techniques to improve diagnosis accuracy, increasing the detection of individuals with low parasite burden. This combination of techniques consists an important strategy for controlling the disease transmission. [ABSTRACT FROM AUTHOR]

Published

2021

5. Fast multiplex real-time PCR assay for simultaneous detection of dog and human blood and Leishmania parasites in sand flies.

Author

Sales, Kamila Gaudêncio da Silva, Miranda, Débora Elienai de Oliveira, Paiva, Marcelo Henrique Santos, Figueredo, Luciana Aguiar, Otranto, Domenico, and Dantas-Torres, Filipe

Subjects

*SAND flies, *BLOOD parasites, *DETECTOR dogs, *CYTOCHROME b, *CYTOCHROME oxidase, *CYTOCHROME c, *HUMAN DNA

Abstract

Background: The blood-feeding behaviour of female sand flies may increase their likelihood of acquiring and transmitting Leishmania parasites. Studies on the host usage by these insects may thus improve our understanding of the Leishmania transmission risk in leishmaniasis-endemic areas. Here, we developed a fast multiplex real-time PCR assay for simultaneous detection of dog, human and Leishmania DNA in sand flies. Methods: Primers and TaqMan probes targeting the mitochondrial cytochrome c oxidase subunit 1 and cytochrome b genes of dog and human, respectively, were combined in a multiplex assay, which also includes primers and a TaqMan probe targeting the Leishmania minicircle kinetoplast DNA. Results: The multiplex assay was 100% specific, with analytical sensitivities of 103 fg/reaction for dog and human and 1 fg for Leishmania. By testing field-collected engorged female sand flies (95 Migonemyia migonei and two Nyssomyia intermedia), 50 M. migonei were positive for one or two targets (positivity rates: 45.4% for human, 4.1% for dog and 12.4% for Leishmania DNA). Conclusions: This multiplex real-time PCR assay represents a novel fast assay for detecting dog, human and Leishmania DNA in female sand flies and therefore a tool for assessing the risk of Leishmania transmission to these hosts in areas of active transmission. [ABSTRACT FROM AUTHOR]

Published

2020

6. Prevalence of hepatitis E virus infection in multiple transfused Brazilian patients with thalassemia and sickle cell disease.

Author

Slavov, Svetoslav N., Maçonetto, Juliana D. M., Martinez, Edson Z., Silva‐Pinto, Ana Cristina, Covas, Dimas T., Eis‐Hübinger, Anna Maria, and Kashima, Simone

Subjects

HEPATITIS E virus, SICKLE cell anemia, VIRUS diseases, IMMUNOGLOBULIN G, BLOOD transfusion

Abstract

Hepatitis E virus (HEV) is a leading cause of acute hepatitis worldwide. The virus is acquired by fecal‐oral route; however, it can also be transmitted by blood transfusion. The objective of the study was to examine anti‐HEV immunoglobulin G and HEV RNA prevalence in multiple transfused patients with thalassemia and sickle cell disease (SCD), and in blood donors. The HEV seroprevalence in the patients was 13% (20% in thalassemics; 7.7% in SCD), and 11% in blood donors. No positive result for HEV RNA was obtained. This is a pioneer study examining HEV circulation in Brazilian patients with hemoglobinopathies. Highlight: The prevalence of HEV in Brazil among multiple‐transfused patients is unknown.We detected HEV seroprevalence of 20% in the patients with thalassemia and 7.7% in the patients with Sickle‐Cell Disease.No patient was positive for HEV RNA.Different routes for HEV transmission might be suspected in Brazil. [ABSTRACT FROM AUTHOR]

Published

2019

7. Occurrence of the colistin resistance mcr‐1 gene in soils from intensive vegetable production and native vegetation.

Author

Oliveira, Camila C., Lopes, Eliene S., Barbosa, Daniele R., Pimenta, Ramon L., Sobrinho, Nelson M. B. A., Coelho, Shana M. O., Souza, Miliane M. S., and Coelho, Irene S.

Subjects

*NATIVE plants, *SOILS, *ANTIBIOTICS, *ORGANIC fertilizers, *COLISTIN, *FERTILIZERS

Abstract

Colistin, currently regarded as the last‐resort antibiotic for the treatment of infections caused by multidrug‐resistant bacteria, is used in poultry production to treat and prevent infection, and as a growth promoter. Poultry litter is commonly used as organic fertilizer; however, there are no reports on the effect of its application regarding colistin resistance in soils. Thus, the objective of the present study was to compare the abundance of the colistin resistance gene (mcr‐1) in soils from vegetable production areas that received non‐composted poultry litter as organic fertilizer and native vegetation areas. The mcr‐1 gene was detected in all soil samples from both areas. A significant difference (p < 0.05) was observed in the relative abundance of the mcr‐1 gene between soils pertaining to the vegetable production area and the native vegetation area in six of those 10 properties. This is the first report of the presence of the colistin resistance gene in soils from Brazil. The vast majority of antibiotic resistance genes acquired by human pathogens originated in natural environments. Thus, the presence of the mcr‐1 gene in soils treated with poultry litter and from native vegetation areas reinforces the need for studies that minimize potential risks of the development of colistin resistance. Highlights: Poultry litter usually is employed as fertilizer; however, there are no reports of its impact in colistin resistance in soils.The mcr‐1 gene was detected in soils from both native vegetation and vegetable production.This is the first report of the presence of colistin resistance gene in soils from Brazil.The presence of mcr‐1 gene in soils can increase risks of the development and spread of colistin resistance. [ABSTRACT FROM AUTHOR]

Published

2019

8. Prevalence of Zika Virus (Zikv) in blood donors from a hemotherapy service of the southern region of Brazil.

Author

Diefenbach, C. F., Slavov, S. N., Kashima, S., Ferreira, A. R., Hespanhol, M. R., Bandeira, B. S., Vizzotto, B. S., Krause, L. M. F., and Martins, J. S.

Subjects

*ZIKA virus, *BLOOD donors, *BLOOD transfusion, *HERD immunity, *OPACITY (Optics)

Abstract

Background and objectives: Zika virus is a flavivirus transmitted by Aedes mosquitos. A discussed transmission route is by blood transfusion due to the large number of ZIKV asymptomatic cases. The objective of the study was to estimate the ZIKV IgG seroprevalence and RNA presence in blood donors from a Hemotherapy Service in Southern Brazil due to the fact that until the end of 2016, 851 ZIKV suspected cases, 51.2% of which were with autochthons transmission were reported in this Brazilian region. Materials and methods: Five hundred blood samples were collected from blood donors between 5 December 2016 and 6 January 2017 in the Hemotherapy Service of Santa Maria, Rio Grande do Sul, Brazil. All samples were tested for the presence of ZIKV RNA by the use of TaqMan® real‐time PCR and 182 of these were serologically assessed for ZIKV IgG. Results: No samples showed positive results for ZIKV RNA. However, the serological survey detected one positive sample for ZIKV IgG and four samples with optical density values in the grey zone (consequently three of them confirmed as Dengue IgG‐positive). This indicates a 0.55% seroprevalence of ZIKV IgG among volunteer blood donors in the city of Santa Maria, Rio Grande do Sul State, Brazil. Conclusion: Our results demonstrate that although the transfusion risk of ZIKV in the south part of the country can be currently considered as low, further outbreaks cannot be excluded due to lack of herd immunity to ZIKV. Our study adds to the national and global prevalence of ZIKV among blood donors and its implications for the transfusion safety. [ABSTRACT FROM AUTHOR]

Published

2019

9. Distribution and Genetic Diversity of Genes from Brazilian Bacillus thuringiensis Strains Toxic to Agricultural Insect Pests Revealed by Real-Time PCR.

Author

Berçot MR, Queiroz PRM, Grynberg P, Togawa R, Martins ÉS, Rocha GT, and Monnerat RG

Subjects

Animals, Endotoxins genetics, Endotoxins chemistry, Real-Time Polymerase Chain Reaction, Bacillus thuringiensis Toxins, Brazil, Bacterial Proteins genetics, Bacterial Proteins chemistry, Insecta, Genetic Variation, Hemolysin Proteins genetics, Hemolysin Proteins chemistry, Bacillus thuringiensis genetics

Abstract

Bacillus thuringiensis is a Gram-positive aerobic bacterium and the most used biopesticide worldwide. Given the importance of B. thuringiensis strain characterization for the development of new bioinsecticides or transgenic events and the identification and classification of new B. thuringiensis genes and strains to understand its distribution and diversity, this work is aimed at creating a gene identification system based on qPCR reactions utilizing core B. thuringiensis genes cry1, cry2, cry3, cry4, cry5, app6, cry7, cry8, cry9, cry10, cry11, vpb1, vpa2, vip3, cyt1, and cyt2 for the characterization of 257 strains of B. thuringiensis. This system was based on the Invertebrate Bacteria Collection from Embrapa Genetic Resources and Biotechnology and analyzed (a) the degree of correlation between the distribution of these strains and the origin of the substrate from which the strain was isolated and (b) between its distribution and geoclimatic conditions. This study made it possible to observe that the cry1, cry2, and vip3A/B genes occur homogeneously in the Brazilian territory, and some genes are found in specific regions. The biggest reservoir of variability is within B. thuringiensis strains in each region, and it is suggested that both geoclimatic conditions and regional crops interfere with the genetic diversity of the B. thuringiensis strains present in the region, and B. thuringiensis strains can constantly exchange genetic information., (© 2023. The Author(s), under exclusive licence to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2023

10. Human Platelet Antigens in Brazilian Multiethnic Populations: Occurrence of Regional Variation and Frequency in a Large Urban Center (Belo Horizonte).

Author

Silva-Malta, Maria Clara Fernandes, de Oliveira, Lucas Gabriel Tavares, Barreiros, Luísa Ferreira, do amaral, Dilson Rocha, and Martins, Marina Lobato

Subjects

*AUTOIMMUNE diseases, *ALLOIMMUNITY, *THROMBOPENIC purpura, *ANTIGENS, *BLOOD platelets

Abstract

Background: The frequency of human platelet antigens (HPA) varies according to ethnicity, which causes differences in the morbidity of alloimmune and autoimmune thrombocytopenic disorders in different populations. Studies on HPA frequencies in Brazil have reported differences among Brazilian populations produced by the diverse degrees of admixture throughout the country. Methods: In the present study, we investigated the variation of HPA distribution in Brazil, compared with worldwide populations, and describe the frequencies of HPA-1, -2, -3, -5, and -15 in a large urban center in Southern Brazil (Belo Horizonte) based on a sample of blood donors. Results: The principal component analysis and the dendrogram based on genetic distance revealed a clear relationship between Brazilian populations and the groups formed by European and African populations. The coefficients of variation for HPA allele frequencies suggest that Brazilian populations presented variations for HPA alleles comparable with the populations from continental groups. In Belo Horizonte, the allele a frequencies for HPA-1, -2, -3, -5 and -15 were 0.8575, 0.8400, 0.6225, 0.8525 and 0.5825 respectively. The genotypes with higher frequencies were a/a (72-74%), except for HPA-3 and -15, whose heterozygous a/b genotypes were shown to be more prevalent (43.5 and 44.5%, respectively). Conclusion: We confirmed the heterogeneity of HPA antigens in Brazilian populations, reinforcing the importance of HPA panels composed of regional blood donors, or a national panel that contemplates the specificities of the different regions of the country, in order to provide support in platelet transfusions and to minimize the risks associated with HPA alloimmunization. The evaluation of HPA data from Belo Horizonte represents the initial step toward the development of a genotyped platelet donor registry in order to treat HPA alloimmunized patients in this region. [ABSTRACT FROM AUTHOR]

Published

2018

11. Duffy blood group system: New genotyping method and distribution in a Brazilian extra-Amazonian population.

Author

Martins, Marina Lobato, da Silva, Adão Rogerio, Santos, Hadassa Campos, Alves, Michelle Teodoro, Schmidt, Luciana Cayres, Vertchenko, Stela Brener, Dusse, Luci Maria SantAna, and Silva Malta, Maria Clara Fernandes da

Subjects

*BLOOD groups, *GENOTYPES, *BLOOD transfusion, *IMMUNOLOGY, *GENETIC polymorphisms

Abstract

Duffy blood group system is of interest in several fields of science including transfusion medicine, immunology and malariology. Although some methods have been developed for Duffy polymorphism genotyping, not all of them have been sufficiently described and validated, and all present limitations. At the same time, the frequency of Duffy alleles and antigens in some densely populated regions of the world are still missing. In this study we present new tests for genotyping the major alleles of the Duffy blood system and describe Duffy alleles and antigens in blood donors and transfusion-dependent patients in Minas Gerais, Brazil. A simple and reproducible strategy was devised for Duffy genotyping based on real-time PCR that included SNPs rs12075 and rs2814778. No significant differences between the allele frequencies were observed comparing blood donors and patients. Among the blood donors, the phenotype Fy(a−b+) was the most common and the Fy(a−b−) phenotype, associated with populations of African descent, was remarkably less common among subjects who self-identified as black in comparison to other ethnoracial categories. However, the African ancestry estimated by molecular markers was significantly higher in individuals with the allele associated to the Duffy null phenotype. The genotyping method presented may be useful to study Duffy genotypes accurately in different contexts and populations. The results suggest a reduced risk of alloimmunization for Duffy antigens and increased susceptibility for malaria in Minas Gerais, considering the high frequency of Duffy-positive individuals. [ABSTRACT FROM AUTHOR]

Published

2017

12. High levels of benzimidazole resistance and β-tubulin isotype 1 SNP F167Y in Haemonchus contortus populations from Ceará State, Brazil.

Author

Santos, Jessica Maria Leite dos, Monteiro, Jomar Patrício, Ribeiro, Wesley Lyeverton Correia, Macedo, Iara Tersia Freitas, Araújo Filho, José Vilemar de, Andre, Weibson Paz Pinheiro, Araújo, Paulo Ricardo Monteiro, Vasconcelos, Janaelia Ferreira, Freitas, Edilson Pereira de, Camurça-Vasconcelos, Ana Lourdes Fernandes, Vieira, Luiz da Silva, and Bevilaqua, Claudia Maria Leal

Subjects

*HAEMONCHUS contortus, *ALBENDAZOLE, *SINGLE nucleotide polymorphisms, *BENZIMIDAZOLES, *TUBULINS, *POLYMERASE chain reaction, *DRUG resistance, *PUBLIC health, *THERAPEUTICS

Abstract

Haemonchus contortus is the most prevalent parasitic nematode in tropical areas, and anthelmintic resistance is a global problem. Our objective was to characterize benzimidazole (BZ) resistance in gastrointestinal nematode populations in Ceará State, Brazil, using the egg hatch test (EHT) and in H. contortus populations using quantitative real-time polymerase chain reaction (qPCR). Twenty locations were surveyed, and fecal samples were collected from a minimum of 40 animals from each farm and pooled. Five thousand L3 from each farm were used to infect single animals at Embrapa (Brazilian Agricultural Research Company) to provide a source of eggs for both phenotypical and molecular tests. The mean EHT was 2.46 μg/ml (±0.58 μg/ml), and BZ resistance was detected at all surveyed locations. The mean resistant allelic frequencies at positions F200Y and F167Y were 34.16% (±12.13%) and 58.31% (±18.89%), respectively. The resistant allelic frequencies at F167Y were higher than those at F200Y in most studied locations. We also investigated the possibility that specific BZ utilization may influence resistant allelic frequencies. We selected three nematode populations based on the resistant SNP prevalence at F200Y and F167Y as follows: higher frequency at SNP F200Y, higher frequency at SNP F167Y and similar frequencies at both positions. Anthelmintic treatments included two BZs (oxfendazole and albendazole) and ivermectin. Three animals per population per treatment were infected with 5000 L3, and nematode eggs were collected for molecular test before and after anthelmintic treatments. The results showed preferential selection of SNP F167Y in response to oxfendazole, an increase in resistant SNP frequencies in general in response to albendazole and little change in relation to pre-treatment situations in response to ivermectin. Our results confirm that BZ resistance is common. The resistant allele at SNP F167Y in H. contortus prevails in Ceará State, and we provide evidence that this result may be due to the utilization of oxfendazole in recent years. [ABSTRACT FROM AUTHOR]

Published

2017

13. Outbreak of Chagas disease in Brazil: Validation of a molecular diagnostic method.

Author

Costa-Oliveira, Cíntia Nascimento da, Paiva-Cavalcanti, Milena de, Barros, Michelle da Silva, Nakazawa, Mineo, Melo, Maria Gabriella Nunes de, Pessoa-e-Silva, Rômulo, Torres, Diego José Lira, Oliveira, Kamila Kássia dos Santos, Moreira, Leyllane Rafael, Morais, Rayana Carla Silva de, Goes, Tayná Correia de, Oliveira, Gênova Maria de Azevedo, Júnior, Wilson de Oliveira, Silva, Milena Maria de Morais E., Batista, Filipe Prohaska, Montenegro, Demetrius, and Lorena, Virginia Maria Barros de

Subjects

*CHAGAS' disease, *NUCLEAR DNA, *DISEASE outbreaks, *TRYPANOSOMA cruzi, *ACUTE diseases, *DNA primers

Abstract

Chagas disease (CD), caused by the protozoan Trypanosoma cruzi (T. cruzi), affects millions of people worldwide. Polymerase Chain Reaction (PCR) and real-time quantitative PCR (qPCR) have been used as tools to monitor parasitic levels in the bloodstream of individuals exposed to infection, thus enabling the monitoring of relapses and the effectiveness of therapy, for example. The aim of this study was to evaluate the TcSAT-IAM system, developed by our research group, on samples from patients with suspected Chagas disease infection. Initially, primer systems were developed for the detection of the nuclear DNA (SAT-DNA) from T. cruzi (TcSAT-IAM). The Cruzi system, predicted in the literature, and TcSAT-IAM were then evaluated in relation to their analytical sensitivity, specificity and efficiency. Afterwards, the applicability of the qPCR technique using both systems (separately) for the diagnosis of acute CD was evaluated in samples from 77 individuals exposed to the outbreak that occurred in Pernambuco-Brazil, relating the results obtained to those of the classical diagnostic methods recommended for this stage of the infection. TcSAT-IAM and Cruzi had a detection limit of 1 fg of target DNA (0,003 parasites). Thirty-eight cases were recorded, 28 by laboratory criteria and 10 by clinical and epidemiological criteria. Blood samples from 77 subjects were submitted to qPCR by both systems, reaching an agreement of 89.61% between them. After analyzes between systems and diagnostic criteria, the TcSAT-IAM showed sensitivity and specificity of 52.36% (CI 37.26–67.52) and 92.31% (CI 79.68–97.35), respectively, accuracy of 72.73% and moderate agreement. The TcSAT-IAM showed an accuracy of 72.58% and 75% in relation to parasitological and serological tests (IgM anti- T. cruzi), respectively. Therefore, quantitative PCR should be incorporated into the diagnosis of suspected acute cases of Chagas disease. [Display omitted] • QPCR as a diagnostic method for the detection of T. cruzi DNA in acute Chagas disease. • TcSAT-IAM proved to be applicable as a complementary technique for acute Chagas disease. • Samples targeted for qPCR should be collected prior to etiologic treatment. [ABSTRACT FROM AUTHOR]

Published

2023

14. Mitochondrial and satellite real time-PCR for detecting T. cruzi DTU II strain in blood and organs of experimentally infected mice presenting different levels of parasite load.

Author

Ferreira Filho, Júlio César Rente, Braz, Lucia Maria Almeida, Andrino, Marcos Luiz Alves, Yamamoto, Lidia, Kanunfre, Kelly Aparecida, and Okay, Thelma Suely

Subjects

*SATELLITE DNA, *CHAGAS' disease, *MOLECULAR pathology, *PARASITES, *MICE

Abstract

The choice of cost-effective molecular methods for diagnosing and monitoring of Chagas disease before and after treatment is crucial in endemic countries with high patients' demand and limited financial resources. To this end, a kDNA was compared to a satellite real-time quantitative PCR (sat-qPCR), both amplifications using Sybr Green instead of Taqman hydrolysis probes. Non-isogenic Swiss albino mice were infected with a small inoculum of the highly virulent and partially resistant to benznidazole Y strain, belonging to T. cruzi discrete typing unit II (DTU-II) that predominates in Atlantic and Central Brazil. DNA from EDTA-blood samples and 10 organs of mice containing high, moderate and low parasite load levels were extracted by a highly used commercial kit and tested in triplicate, showing no disagreements between the two qPCRs. The melting temperature of positive samples was 79.8 °C ± 1 °C for satellite-DNA and 78.1 °C ± 1 °C for kDNA. DNA from genetically-related parasites such as Leishmania sp. showed no cross-reactions, but the sympatric T. rangeli was detected by both qPCRs, more effectively by kDNA than the satellite system, which required the equivalent of 50 parasites to give a positive result. Samples from infected mice, regardless of the type of biological matrix (blood or organ samples) or the parasite load gave positive results by both qPCRs. The sensitivity of sat-qPCR was 2 × 10−3 parasite or 240 target copies, and for kDNA, 2 × 10−4 parasite or 24 target copies. Regarding repeatability and reproducibility, the coefficient of variation (CV) was always < 25% in both assays; linearity of sat-qPCR was 0.991 (±0.002) and 0.991 (±0.008) for kDNA qPCR. In most collection times, the median Ct values found in blood and organs provided by sat-DNA and kDNA qPCRs were similar. In conclusion, although kDNA qPCR achieved a better analytical sensitivity, sat-qPCR gave better specificity results. Nevertheless, further research is intended to test other T. cruzi DTUs and chagasic patients' samples before these cost-effective techniques are incorporated into diagnostic routines. • kDNA and satellite DNA Sybr Green real-time PCR were similar to T. cruzi detection. • kDNA qPCR achieved a better analytical sensitivity. • sat-qPCR gave better specificity results. [ABSTRACT FROM AUTHOR]

Published

2019

15. Arbovirus detection in synanthropic mosquitoes from the Brazilian Amazon and in mosquito saliva using Flinders Technology Associates cards.

Author

Rios, Flávia Geovana Fontineles, Alves do Nascimento, Valdinete, Naveca, Felipe Gomes, Vieira, Deusilene Souza, and Julião, Genimar Rebouças

Subjects

*ARBOVIRUSES, *MOSQUITOES, *AEDES aegypti, *SALIVA, *ZIKA virus infections, *CULEX quinquefasciatus, *ZIKA virus

Abstract

Although arbovirus transmission and identifying target vectors may provide a baseline for planning disease control strategies, there are many gaps in knowledge regarding these mosquitoes and viral species in urban, rural, or sylvatic habitats in the Brazilian Amazon. Our goal was to screen for dengue, chikungunya, and Zika viruses in synanthropic mosquitoes and with Flinders Technology Associates (FTA) cards using insect saliva. Mosquitoes were caught using ovitraps and aspirators in the city of Porto Velho, Rondônia, Brazil. Honey-baited FTA cards were placed in mosquito cages for 15 days; whole mosquitoes and FTA cards were analysed for viral RNA using RT-qPCR assays. One pool of Aedes aegypti females was found to be infected with the Zika virus and one male mosquito was infected with dengue-4, suggesting natural vertical/venereal transmission. Our study also reported evidence of vertical/venereal transmission of ZIKV in Culex quinquefasciatus males for the first time in the Brazilian Amazon, and the feasibility of using FTA cards to detect arboviruses in the saliva of field-collected mosquitoes. Vertical/venereal transmission of viruses by atypical mosquito species reinforces the need for combined viral and entomological screening in arbovirus surveillance programs. [ABSTRACT FROM AUTHOR]

Published

2023

16. Salmonella and other Enterobacteriaceae in conventional and organic vegetables grown in Brazilian farms.

Author

Padovani NFA, Santos TS, Almeida P, Dias M, Mendes MA, Cesar ASM, and Maffei DF

Subjects

Farms, Brazil, Salmonella, Food Microbiology, Colony Count, Microbial, Food Contamination analysis, Enterobacteriaceae genetics, Vegetables microbiology

Abstract

This study aimed to assess the microbiological profile of conventional and organic vegetables grown in Brazilian farms through the detection of Salmonella and other Enterobacteriaceae. A total of 200 samples (100 conventional and 100 organic), including leafy greens, spices/herbs, and other unusual vegetables, were submitted to the enumeration of Enterobacteriaceae by plating on VRBG agar. Moreover, colonies of Enterobacteriaceae were randomly selected and submitted to identification by MALDI-TOF MS. Samples were also tested for Salmonella, using culture-based and PCR-based enrichment methods. The mean counts of Enterobacteriaceae in conventional and organic vegetables were 5.1 ± 1.5 and 5.4 ± 1.4 log CFU/g, respectively (P > 0.05). A total of 18 genera (including 38 species) of Enterobacteriaceae were identified, and the most frequent ones found in samples from both farming systems were Enterobacter (76%) and Pantoea (68%). Salmonella was identified in 17 samples (8.5%): nine (4.5%) in conventional and eight (4.0%) in organic vegetables. These results indicate that the farming system had no impact on the Enterobacteriaceae populations and rates of Salmonella and revealed unsatisfactory microbiological safety of some samples, mainly due to the presence of Salmonella. These findings highlight the need for control measures during vegetable production, regardless of the farming system, to reduce microbial contamination and the risks of foodborne illnesses., (© 2023. The Author(s) under exclusive licence to Sociedade Brasileira de Microbiologia.)

Published

2023

17. Gene Expression Profile of Uterine Leiomyoma from Women Exposed to Different Air Pollution Levels in Metropolitan Cities of Sao Paulo, Brazil.

Author

Dos Anjos LG, de Almeida BC, Baracat EC, Al-Hendy A, Yang Q, and Carvalho KC

Subjects

Pregnancy, Humans, Female, Cities, Brazil epidemiology, Transcriptome, Air Pollutants toxicity, Air Pollutants analysis, Air Pollution adverse effects, Air Pollution analysis, Infertility, Leiomyoma etiology, Leiomyoma genetics

Abstract

Leiomyomas (LMs) are the most frequent uterine benign tumors, representing the leading cause of hysterectomy indications worldwide. They are highly associated with women's reproductive complications, and endocrine disruptors may influence their etiology. In this sense, air pollution represents a relevant hormonal disruptor that acts on key signaling pathways, resulting in tumor development and infertility. Our goal was to evaluate submucosal LM samples from patients living in the metropolitan and Sao Paulo city regions, focusing on genes involved in tumor development and infertility features. Twenty-four patients were selected based on their region of residence and clinical information availability. Several genes were differentially expressed between women living in metropolitan areas and Sao Paulo city. Significant associations were observed between BCL-2 , DVL1 , FGFR3 , and WNT5b downregulation and contraceptive use in the samples from women living in Sao Paulo city. ESR1 and HHAT downregulation was associated with ethnicity. WNT5b and GREM were associated with LM treatment and related pathologies, respectively. In the samples from women living in other cities of the metropolitan region, abortion occurrence was associated with BMP4 upregulation. Although further studies may be necessary, our results showed that air pollution exposure influences the expression of genes related to LM development and female reproductive features.

Published

2023

18. MOLECULAR INVESTIGATION OF HEMOTROPIC MYCOPLASMAS IN HUMAN BEINGS, DOGS AND HORSES IN A RURAL SETTLEMENT IN SOUTHERN BRAZIL.

Author

da Costa VIEIRA, Rafael Felipe, VIDOTTO, Odilon, Jayme VIEIRA, Thállitha Samih Wischral, Sá GUIMARAES, Ana Márcia, dos SANTOS, Andrea Pires, NASCIMENTO, Naíla Cannes, dos SANTOS, Nelson Jesse Rodrigues, MARTINS, Thiago Fernandes, LABRUNA, Marcelo Bahia, MARCONDES, Mary, BIONDO, Alexander Welker, and MESSICK, Joanne Belle

Subjects

MYCOPLASMATALES, RURAL geography, PUBLIC health, HAEMOBARTONELLA, MYCOPLASMA, LABORATORY dogs, FACTOR analysis

Abstract

Copyright of Revista do Instituto de Medicina Tropical de São Paulo is the property of Instituto de Medicina Tropical de Sao Paulo and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published

2015

19. Evaluation of conjunctival swab as a mass-screening tool for molecular diagnosis of canine visceral leishmaniasis.

Author

Leite, Rodrigo, Souza, Natalia, Barbosa, Amanda, Ferreira, Aline, and Andrade, Antero

Subjects

*DIAGNOSIS of dog diseases, *LEISHMANIASIS diagnosis, *MOLECULAR diagnosis, *LEISHMANIASIS, *POLYMERASE chain reaction, *PREVENTION

Abstract

The canine visceral leishmaniasis (CVL) diagnosis is an important step of visceral leishmaniasis control program in Brazil once the dog is the main reservoir host of the disease. The aim of this study was to evaluate the conjunctival swab (CS) as a mass-screening tool for CVL molecular diagnosis in an endemic area classified as priority for the Brazilian Ministry of Healthy for surveillance action. A total of 1350 domiciled dogs were screened. The animals were evaluated by serological tests (enzyme-linked immunosorbent assay (ELISA) as screening and immunofluorescence antibody test (IFAT) for confirmation) and by CS associated to real-time PCR, using primers addressed to kinetoplast DNA (kDNA) minicircles and SYBR Green. Canine β-globin gene amplification was used to evaluate the sample DNA integrity. A subgroup of 484 animals was also submitted to clinical evaluation. Among the 1350 dogs screened, 369 (27.3 %) were positive by CS real-time PCR and 126 (9.3 %) tested positive by ELISA. Thirty-one percent (39/126) of the ELISA-positive dogs were confirmed by IFAT. CS real-time PCR was able to detect infection in dogs independently of the symptomatology degree ( p > 0.05), while ELISA was more sensitive in the group of dogs that present three or more clinical signs related to CVL. The results demonstrated that CS real-time PCR was able to detect a higher number of infected dogs than ELISA and that the prevalence of canine infections has been underestimated by the serological assays. The use of sensitive molecular diagnostic methods like CS real-time PCR, mainly in endemic areas, could greatly contribute to disease control. [ABSTRACT FROM AUTHOR]

Published

2015

20. Detection of hantaviruses in Brazilian rodents by SYBR-Green-based real-time RT-PCR.

Author

Araujo, J., Pereira, A., Nardi, M., Henriques, D., Lautenschalager, D., Dutra, L., Ometto, T., Hurtado, R., Maués, F., Nava, A., Morais, F., Aires, C., Favorito, S., and Durigon, E.

Subjects

*HANTAVIRUSES, *REVERSE transcriptase polymerase chain reaction, *RODENTS as carriers of disease, *DIAGNOSTIC microbiology, *PATHOGENIC microorganisms, *DNA primers, *DIAGNOSTIC virology

Abstract

Current knowledge of the pathogenic hantavirus indicates that wild rodents are its primary natural reservoir. Specific primers to detect the presence of viral genomes were developed using an SYBR-Green-based real-time RT-PCR protocol. One hundred sixty-four rodents native to the Atlantic Forest biome were captured in São Paulo State, Brazil, and their tissues were tested. The presence of hantavirus RNA was detected in sixteen rodents: three specimens of Akodon montensis, three of Akodon cursor, two of Necromys lasiurus, one of Juliomys sp., one of Thaptomys nigrita, five of Oligoryzomys nigripes, and one of Oryzomys sp. This SYBR Green real-time RT-PCR method for detection of hantavirus may be useful for surveying hantaviruses in Brazil. [ABSTRACT FROM AUTHOR]

Published

2011

21. The best algorithm to confirm the diagnosis of HTLV-1 and HTLV-2 in at-risk individuals from São Paulo, Brazil

Author

Costa, Emanuela A.S., Magri, Mariana C., and Caterino-de-Araujo, Adele

Subjects

*HTLV-I, *HTLV-II (Virus), *POLYMERASE chain reaction, *ENZYME-linked immunosorbent assay, *ALGORITHMS, *OPACITY (Optics), *VIRAL disease diagnosis

Abstract

Abstract: The ability to confirm the diagnosis of human T-lymphotropic virus types 1 and 2 (HTLV-1 and HTLV-2) in at-risk individuals in São Paulo, Brazil by Western blotting (WB), conventional polymerase chain reaction (tax and pol PCR) and real-time PCR (pol) is compared. Seventy-three blood samples that were reactive in HTLV-1/2 serological screening enzyme immunoassays (EIAs) were evaluated. HTLV-1/2 was confirmed in 53 blood samples: 48 were positive by WB, 41 were positive by PCR and 42 scored positive by real-time PCR assays (37 of 48 WB-positive samples plus five WB-indeterminate samples that were further confirmed by sequencing). Although WB was able to detect more cases of HTLV-1/2 infection, the real-time PCR assay was able to discriminate between these two viruses and confirm an individual HTLV-1/HTLV-2 diagnosis in two HTLV WB-untyped samples and five WB-indeterminate samples. Because of the large number of WB-indeterminate samples and the cost of the WB assay in Brazil, it is proposed an algorithm that employs two EIAs for screening and then real-time PCR to confirm the infection, followed by testing any PCR-negative samples with the WB assay. This strategy reduces costs and improves the accuracy of the diagnosis of HTLV-1/2. [Copyright &y& Elsevier]

Published

2011

22. Survey of compliance with labeling legislation in food containing GMOs in Brazil

Author

Branquinho, Maria Regina, Ferreira, Renata T.B., and Cardarelli-Leite, Paola

Subjects

*FOOD labeling laws, *TRANSGENIC organisms, *FOOD chemistry, *FOOD composition, *QUANTITATIVE research, *POLYMERASE chain reaction, *FOOD safety, *RECOMBINANT DNA

Abstract

Abstract: Analysis of food products consisting of, or produced from, genetically modified organisms (GMOs) is required to verify compliance with labeling legislation and to detect any possible unauthorized transgenic crops. With these goals, 240 samples of soy-derived foodstuffs and 25 samples of maize-derived foodstuffs were analyzed from 2004 to 2007. All samples positive for Roundup Ready® soybean were quantitatively examined using the TaqMan® GMO 35S Soy kit. In food containing soy, 68 (28.3%) were shown to contain GM soy, whereas in food containing maize, neither Bt 176 nor MON 810 maize were found. Quantitative analysis revealed GMO contents ranging from 0.05 to 1% in 43 (63.2%) samples, and more than 1% in 25 (36.8%) samples. The absolute and relative limits of detection (LODs) were approximately 10 copies and 0.0125%, respectively, and the absolute and relative limits of quantification (LOQs) were approximately 40 copies and 0.05%, respectively, suggesting sufficient sensitivity to quantify genetically modified (GM) materials below and above the legal threshold of 1%. The presence of GM material in these samples was not indicated on their labels, indicating that none of these food products had been appropriately labeled. These results clearly demonstrate the need for a monitoring program of food products by the Brazilian regulatory authorities. [Copyright &y& Elsevier]

Published

2010

23. Monitoring of GMO in Brazilian processed meat and soy-based products from 2007 to 2008

Author

Dinon, Andréia Zilio, Treml, Diana, de Mello, Carla Souza, and Arisi, Ana Carolina Maisonnave

Subjects

*FOOD chemistry, *TRANSGENIC organisms, *MEAT, *SOYBEAN products, *POLYMERASE chain reaction, *RECOMBINANT DNA, *FOOD composition

Abstract

Abstract: Roundup Ready™ (RR) soybean is the first genetically modified organism (GMO) approved in Brazil. In this country, the labeling of foodstuffs containing GMOs is mandatory if the GMO content exceeds 1% (10gkg−1). In order to monitor and quantify the presence of RR soybean in soy-based and processed meat products on the Brazilian food market, DNA was extracted from 59 food samples and analyzed by polymerase chain reaction (PCR) to amplify the soybean lectin gene, and by nested PCR to amplify the recombinant DNA present in RR soybean. Positive samples for the presence of RR soybean were subjected to a real-time quantification of GMO using a duplex real-time PCR. The results showed that out of 59 samples, 54 were positive for lectin gene and six were positive for RR soybean, 5 samples contained less than10gkg−1 GMO and one sample contained more than 10gkg−1 GMO. [Copyright &y& Elsevier]

Published

2010

24. Real-time PCR assay to identify variants of Vaccinia virus: Implications for the diagnosis of bovine vaccinia in Brazil

Author

Trindade, Giliane de Souza, Li, Yu, Olson, Victoria A., Emerson, Ginny, Regnery, Russell L., Fonseca, Flavio Guimaraes da, Kroon, Erna Geessien, and Damon, Inger

Subjects

*VACCINIA, *POLYMERASE chain reaction, *CLINICAL pathology

Abstract

Abstract: Naturally occurring infections of Vaccinia virus (VACV) have been recognized in Brazil during the past 10 years. Human Brazilian Vaccinia virus (BVV) infections typically occur as a zoonosis transferred from affected dairy cows to their handlers. Outbreaks have caused notable economic losses to the rural community in the region. The origins of BVV are unclear but previous analyses have shown that at least two distinct clades of BVV exist. The aim of this study was to develop a rapid and inexpensive process for identification and differentiation of BVV that should facilitate epidemiological and ecological investigations including the improved diagnosis of Brazilian Orthopoxvirus infections. A SYBR green quantitative real-time polymerase chain reaction (PCR) targeting the hemagglutinin gene was developed to identify different populations of BVV, VACV vaccine strains used in Brazil during the smallpox eradication campaign (Vaccinia Lister (VACV-LIS) and New York City Board of Health (VACV-NYCBH)), and currently available vaccines (VACV-NYCBH DRYVAX and VACV-NYCBH Acambis 2000). Three primer combinations (one to amplify many orthopoxviruses including all vaccinia viruses described so far; one to differentiate BVV from vaccine strains (VACV-LIS, VACV-NYCBH DRYVAX and VACV-NYCBH Acambis 2000); and one to differentiate BVV clades) were designed to work at the same annealing temperature and reaction conditions. In addition, these methods were able to detect orthopoxvirus viral DNA in lesion biopsy material without the need for DNA extraction. [Copyright &y& Elsevier]

Published

2008

25. Frequency of human metapneumovirus infection in hematopoietic SCT recipients during 3 consecutive years.

Author

Oliveira, R. R., Machado, A. F., Tateno, A. F., Vilas Boas, L. S., Pannuti, C. S., and Machado, C. M.

Subjects

*RESPIRATORY infections, *HEMATOPOIETIC agents, *POLYMERASE chain reaction, *GENOMES, *CLINICAL trials, *HEALTH outcome assessment

Abstract

Respiratory viruses can cause significant morbidity in immunocompromised hosts. Human metapneumovirus (hMPV) has been increasingly associated with lower respiratory tract infection in hematopoietic SCT (HSCT) recipients, with mortality rates up to 50%. No data on the occurrence of hMPV infection in HSCT recipients have been reported in the southern hemisphere. We conducted a retrospective study including 228 nasal wash samples from 153 HSCT recipients with respiratory symptoms during 2001, 2002 and 2003. hMPV was detected by real-time PCR with primers complementary to the nucleocapsid region of hMPV genome. Eleven of the 153 patients (7.2%) acquired hMPV infection during the study period (6.4% in 2001, 4.7% in 2002 and 11.1% in 2003). Among the 11 HSCT recipients with hMPV infection, 1 died 8 days after the diagnosis, but the role of hMPV in the patient's death could not be established. In 2001 and 2003, hMPV group A prevailed over group B. In 2002, both groups were detected equally. hMPV infections were diagnosed in late winter and spring. The frequency of hMPV infection in HSCT recipients living in Brazil was similar to those observed in the northern hemisphere. Sensitive techniques to detect hMPV should be included in the diagnostic assessment of HSCT recipients with respiratory symptoms.Bone Marrow Transplantation (2008) 42, 265–269; doi:10.1038/bmt.2008.153; published online 2 June 2008 [ABSTRACT FROM AUTHOR]

Published

2008

26. High prevalence of human Torque teno virus in streams crossing the city of Manaus, Brazilian Amazon.

Author

Diniz-Mendes, L., Paula, V. S. de, Luz, S. L. B., and Niel, C.

Subjects

*DNA viruses, *ADSORPTION (Chemistry), *GENOMICS, *POLYMERASE chain reaction

Abstract

Aims: Torque teno virus (TTV) is a human DNA virus chronically infecting most healthy individuals worldwide and can be transmitted by faecal–oral route. The occurrence of TTV was evaluated in the streams crossing the city of Manaus (Brazilian Amazon) over a 1-year period, four times a year. Methods and Results: Fifty-two water samples were collected from 13 different locations. Viruses were concentrated from two litres of water by adsorption to negative membrane filters followed by ultrafiltration. TTV DNA was detected by PCR assays designed to detect all five TTV genomic groups. By conventional PCR, 19/52 (37%) samples were positive. By real-time PCR, TTV DNA could be detected in 48/52 (92%) samples. Viral loads ranged from 1300 to 746 000 genome equivalent per 100 ml of river water. Eleven distinct nucleotide sequences were obtained. Conclusions: Our results show the wide distribution and diversity of TTV among Manaus urban micro basins. Significance and Impact of the Study: The data presented here may contribute to substantiate TTV as a sensitive indicator of human contamination. [ABSTRACT FROM AUTHOR]

Published

2008

27. Molecular detection of hepatitis A virus in urban sewage in Rio de Janeiro, Brazil.

Author

Villar, L. M., de Paula, V. S., Diniz-Mendes, L., Guimarães, F. R., Ferreira, F. F. M., Shubo, T. C., Miagostovich, M. P., Lampe, E., and Gaspar, A. M. C.

Subjects

*HEPATITIS A, *VIRAL hepatitis, *NUCLEIC acids, *POLYMERASE chain reaction, *GENETIC polymorphisms

Abstract

Aims: A one-year survey was conducted to examine hepatitis A virus (HAV) prevalence, distribution of genotypes and their relationship to bacterial indicators in raw and treated sewage samples. Methods and Results: Fifty sewage samples (raw = 25 and treated = 25) were collected twice monthly from one sewage treatment plant in Rio de Janeiro. Virus concentration was performed by adsorption to an electronegative membrane followed by ultrafiltration. Viral RNA was detected by nested reverse transcriptase-polymerase chain reaction (RT-PCR) and real-time PCR and positive products were directly sequenced. Total and faecal coliform concentrations were also determined. By nested RT-PCR, HAV RNA was detected in 16/50 (32%) and eight (16%) of them were found in treated sewage samples. By real-time PCR, HAV RNA was detected in 46/50 (92%) samples and 24 were from treated sewage. Phylogenetic analyses classified nine isolates (56%) as subgenotype IA and seven (44%) as IB. Conclusions: Real-time PCR was more sensitive than nested RT-PCR; the presence of subgenotypes IA and IB was described and bacterial indicators cannot be used to predict HAV presence in sewage. Significance and Impact of the Study: These results demonstrated that HAV still remains in the environment after sewage treatment and could play an important role in maintaining the endemicity of HAV infection. [ABSTRACT FROM AUTHOR]

Published

2007

28. A preliminary investigation of Ehrlichia species in ticks, humans, dogs, and capybaras from Brazil

Author

Labruna, Marcelo B., McBride, Jere W., Camargo, Luis Marcelo A., Aguiar, Daniel M., Yabsley, Michael J., Davidson, William R., Stromdahl, Ellen Y., Williamson, Phillip C., Stich, Roger W., Long, S. Wesley, Camargo, Erney P., and Walker, David H.

Subjects

*EHRLICHIA, *TICKS, *CAPYBARA

Abstract

Abstract: A molecular epidemiologic investigation in two Brazilian states (Rondônia and São Paulo) was undertaken to determine if Ehrlichia species responsible for human and animal ehrlichioses in North America could be found in Brazilian vectors, potential natural mammalian reservoirs and febrile human patients with a tick bite history. Samples, including 376 ticks comprising 9 Amblyomma species, 29 capybara (Hydrochaeris hydrochaeris) spleens, 5 canine blood, and 75 human blood samples from febrile patients with history of tick bites were tested by a real-time PCR assay targeting a fragment of the Ehrlichia dsb gene. Ehrlichia DNA was not detected in any tick, capybara or human samples. In contrast, 4 out of 5 dogs contained Ehrlichia canis DNA in their blood, which were sequenced, representing the first report of E. canis infecting dogs in the Amazon region of Brazil. Further studies are needed to evaluate the presence of other agents of human and animal ehrlichioses in Brazil. [Copyright &y& Elsevier]

Published

2007

29. Evaluation of Trypanosoma cruzi parasitic load by real-time PCR and blood culture in long-term kidney transplant recipients.

Author

Jesus Guimarães Ferreira J, Antonio de Almeida E, Barbosa Marcon GE, Gonçalves Lima R, Barroso Pereira M, Ramos Gadelha F, Mazzali M, Martins LC, Silva Wanderley J, and Botelho Costa SC

Subjects

Adult, Aged, Brazil, Chagas Disease parasitology, DNA, Protozoan blood, Female, Humans, Kidney Transplantation adverse effects, Male, Real-Time Polymerase Chain Reaction, Retrospective Studies, Chagas Disease diagnosis, Parasite Load methods, Transplant Recipients, Trypanosoma cruzi isolation & purification

Abstract

Introduction: Acute Chagas disease involving reactivation can occur after organ transplant, and follow-up by direct parasitological or molecular methods is essential for monitoring the parasitic load in such patients. In contrast, there is a little data on the parasitic load in long-term organ recipients. In this study, we examined the parasitic load in long-term kidney transplant patients and assessed the possibility of late Chagas disease reactivation., Methodology: Blood cultures and real-time PCR were used to assess the parasitic load in four immunosuppressed patients who underwent kidney transplants (between 1996 and 2014) and were also treated for parasites., Results: There were no positive blood culture or real-time PCR results in Chagas disease patients who received kidney transplants. The real-time PCR presented detection limit of 0.1 parasite equivalent/mL. The time interval between the transplant and sample collection varied from one to 19 years., Conclusions: No parasites were detected in the evaluated patients. The use of benznidazole and immunosuppressive therapy may have contributed to control the T. cruzi infection. In transplanted patients with Chagas disease, the use of methods such real-time PCR and blood culture can monitor the parasitic load and prevent disease reactivation., Competing Interests: No Conflict of Interest is declared, (Copyright (c) 2021 Juliana Jesus Guimarães Ferreira, Eros Antonio de Almeida, Glaucia Elisete Barbosa Marcon, Rodrigo Goncalves Lima, Mariane Barroso Pereira, Fernanda Ramos Gadelha, Marilda Mazzali, Luiz Claudio Martins, Jamiro Silva Wanderley, Sandra Cecilia Botelho Costa.)

Published

2021

30. Evaluation of HBV-Like Circulation in Wild and Farm Animals from Brazil and Uruguay.

Author

Vieira YR, Portilho MM, Oliveira FF, Guterres A, Dos Santos DRL, Villar LM, Mirazo S, Arbiza J, Dimache LAG, Almeida FQ, Brandão ML, Cordeiro JLP, Rocha FL, Azevedo FC, Lemos FG, Campos JBV, Macedo GC, Herrera HM, Péres IAS, Zimmermann NP, Piovezan U, Pellegrin AO, de Paula VS, and Pinto MA

Subjects

Animals, Animals, Domestic blood, Animals, Wild blood, Biomarkers blood, Brazil epidemiology, Hepatitis B blood, Hepatitis B diagnosis, Hepatitis B epidemiology, Polymerase Chain Reaction, Uruguay epidemiology, Animals, Domestic virology, Animals, Wild virology, DNA, Viral blood, Hepatitis B veterinary, Hepatitis B Antibodies blood, Hepatitis B Antigens blood

Abstract

The origin of the hepatitis B virus is a subject of wide deliberation among researchers. As a result, increasing academic interest has focused on the spread of the virus in different animal species. However, the sources of viral infection for many of these animals are unknown since transmission may occur from animal to animal, human to human, animal to human, and human to animal. The aim of this study was to evaluate hepadnavirus circulation in wild and farm animals (including animals raised under wild or free conditions) from different sites in Brazil and Uruguay using serological and molecular tools. A total of 487 domestic wild and farm animals were screened for hepatitis B virus (HBV) serological markers and tested via quantitative and qualitative polymerase chain reaction (PCR) to detect viral DNA. We report evidence of HBsAg (surface antigen of HBV) and total anti-HBc (HBV core antigen) markers as well as low-copy hepadnavirus DNA among domestic and wild animals. According to our results, which were confirmed by partial genome sequencing, as the proximity between humans and animals increases, the potential for pathogen dispersal also increases. A wider knowledge and understanding of reverse zoonoses should be sought for an effective One Health response.

Published

2019

31. Assessing the relationship between organic farming practices and microbiological characteristics of organic lettuce varieties (Lactuca sativa L.) grown in Sao Paulo, Brazil.

Author

Maffei DF, Moreira DA, Silva MBR, Faria DB, Saldaña E, Ishimura I, Landgraf M, and Franco BDGM

Subjects

Brazil, Escherichia coli genetics, Escherichia coli growth & development, Farms, Humans, Organic Agriculture standards, Salmonella genetics, Salmonella growth & development, Escherichia coli isolation & purification, Food Microbiology, Lactuca microbiology, Organic Agriculture statistics & numerical data, Salmonella isolation & purification

Abstract

Aims: This study aimed to gather information on farming practices employed in organic lettuce fields in Sao Paulo, Brazil and associate these practices with the microbiological characteristics of the products., Methods and Results: Practices were surveyed using a questionnaire applied in ten farms, where 200 heads of lettuce were collected and submitted to enumeration of total coliforms and generic Escherichia coli and tested for Salmonella spp. using culture and molecular (qPCR) methods. Based on the responses, the farms could be clustered in two groups: group 1, comprised by six farms, where chicken manure was used as fertilizer in most of them and the composting process was not performed on site; and group 2, comprised by four farms, where other types of fertilizer were used, and the composting process was performed on site. Generic E. coli was detected in 56 (28%) samples, with an average of 1·1 ± 0·7 log MPN per g. Salmonella DNA was detected in two (1%) samples by qPCR., Conclusions: The prevalence and bacterial loads of generic E. coli, and the occurrence of Salmonella, even at low populations undetectable by conventional culture methods, highlight the need for control measures during farming practices to reduce microbial contamination and risks of foodborne illnesses. These measures include the use of properly composted manure and appropriate washing procedures for leafy vegetables before consumption., Significance and Impact of the Study: The obtained data contribute to a better understanding of the farming practices of organically grown lettuces in Sao Paulo, Brazil., (© 2019 The Society for Applied Microbiology.)

Published

2019

32. Reverse transcriptase droplet digital PCR to identify the emerging vesicular virus Senecavirus A in biological samples.

Author

Pinheiro-de-Oliveira TF, Fonseca-Júnior AA, Camargos MF, Laguardia-Nascimento M, Giannattasio-Ferraz S, Cottorello ACP, de Oliveira AM, Góes-Neto A, and Barbosa-Stancioli EF

Subjects

Animals, Brazil epidemiology, Communicable Diseases, Emerging epidemiology, Communicable Diseases, Emerging virology, Enterovirus B, Human genetics, Enterovirus B, Human isolation & purification, Picornaviridae genetics, Picornaviridae Infections epidemiology, Picornaviridae Infections virology, RNA, Viral analysis, Sensitivity and Specificity, Swine, Swine Diseases virology, Swine Vesicular Disease epidemiology, Swine Vesicular Disease virology, Communicable Diseases, Emerging veterinary, Disease Outbreaks veterinary, Picornaviridae isolation & purification, Picornaviridae Infections veterinary, Reverse Transcriptase Polymerase Chain Reaction veterinary, Swine Diseases epidemiology

Abstract

Senecavirus A (SVA) belonging to the family Picornaviridae, genus Senecavirus was incidentally isolated in 2002 from the PER.C6 (transformed foetal retinoblast) cell line. However, currently, this virus is associated with vesicular disease in swine and it has been reported in countries such as the United States of America, Canada, China, Thailand and Colombia. In Brazil, the SVA was firstly reported in 2015 in outbreaks of vesicular disease in swine, clinically indistinguishable of Foot-and-mouth disease, a contagious viral disease that generates substantial economic losses. In the present work, it was standardized a diagnostic tool for SVA based on RNA reverse transcriptase droplet digital PCR (RT-ddPCR) using one-step and two-step approaches. Analytical sensitivity and specificity were done in parallel with real-time PCR, RT-qPCR (one-step and two-step) for comparison of sensitivity and specificity of both methods. In the standardization of RT-ddPCR, the double-quenched probe and the temperature gradient were crucial to reduce background and improve amplitude between positive and negative droplets. The limit of detection and analytical specificity of techniques of one-step techniques showed superior performance than two-step methods described here. Additionally, the results showed 94.2% concordance (p < 0.001) for RT-ddPCR and RT-qPCR using the one-step assay approach and biological samples from Brazilian outbreaks of Senecavirus A. However, ddRT-PCR had a better performance than RT-PCR when swine serum pools were tested. According to the results, the one-step RT-ddPCR and RT-qPCR is highlighted to be used as an auxiliary diagnostic tool for Senecavirus A and for viral RNA absolute quantification in biological samples (RT-ddPCR), being a useful tool for vesicular diseases control programs., (© 2019 Blackwell Verlag GmbH.)

Published

2019

33. Detection of bacterial contamination in platelet concentrates from Brazilian donors by molecular amplification of the ribosomal 16S gene.

Author

Viana JD, Ferreira SC, Matana SR, Rossi F, Patel P, Garson JA, Rocha V, Tedder R, Mendrone-Júnior A, and Levi JE

Subjects

Brazil, Humans, Bacteria genetics, Blood Donors, Blood Platelets microbiology, Genes, rRNA genetics, Nucleic Acid Amplification Techniques, RNA, Bacterial genetics, RNA, Ribosomal, 16S genetics

Abstract

Objective: The aim of our work was to establish a semi-automated high-throughput DNA amplification method for the universal screening of bacteria in platelet concentrates (PCs)., Background: Among cases of transfusion transmission of infectious agents, bacterial contamination ranks first in the number of events, morbidity and mortality. Transmission occurs mainly by transfused PCs. Automated culture is adopted by some blood banks for screening of bacterial contamination, but this procedure is expensive and has a relatively long turnaround time., Methods: PCs were spiked with suspensions of five different bacterial species in a final concentration of 1 and 10 colony-forming units (CFU) per millilitre. After incubation, the presence of bacteria was investigated by real-time polymerase chain reaction (PCR) and by the Enhanced Bacterial Detection System (eBDS, Pall) assay as a reference method. Real-time PCR amplification was performed with a set of universal primers and probes targeting the 16S rRNA gene. Co-amplification of human mitochondrial DNA served as an internal control., Results: Using the real-time PCR method, it was possible to detect the presence of all bacterial species tested with an initial concentration of 10 CFU mL -1 24 h after contamination, except for Staphylococcus hominis. The PCR assay also detected, at 24 h, the presence of Serratia marcescens and Enterobacter cloacae with an initial concentration of 1 CFU mL -1 ., Conclusions: The real-time PCR assay may be a reliable alternative to conventional culture methods in the screening of bacterial contamination of PCs, enabling bacterial detection even with a low initial concentration of microorganisms., (© 2018 British Blood Transfusion Society.)

Published

2018

34. Prevalence of Toxoplasma gondii DNA in Processed Pork Meat.

Author

Costa DF, Fowler F, Silveira C, Nóbrega MJ, Nobrega HAJ, Nascimento H, Rizzo LV, Commodaro AG, and Belfort R Jr

Subjects

Animals, Brazil, Food Contamination, Prevalence, Real-Time Polymerase Chain Reaction, Swine, Toxoplasma, DNA, Protozoan analysis, Food Microbiology, Meat Products parasitology, Toxoplasmosis, Animal etiology

Abstract

Toxoplasma gondii infection may be attributed to the ingestion of pork meat and contaminated water. In southern Brazil, the prevalence of blindness caused by T. gondii is the highest in the world. Our purpose is to determine the frequency of T. gondii DNA in commercial fresh sausage and cured salami samples from Rio Grande do Sul state, south of Brazil. A total of 118 samples (sausage and salami) from 8 different producers were collected and DNA was extracted. Real-time polymerase chain reaction (qPCR) technique was performed to detect T. gondii DNA using B1 marker. The frequency of T. gondii DNA among the total number of samples (sausage and salami) was 39% (46/118). Among these, a higher frequency of positivity was observed in the sausage samples (47.5%) when compared with the salami samples (17%). However, the mean parasite concentration was significantly higher in the salami samples. The prevalence of T. gondii DNA in fresh sausage and cured salami may indicate that infected pigs may be an important source of infections and a public health hazard to be considered.

Published

2018

35. Canine visceral leishmaniasis diagnosis: a comparative performance of serological and molecular tests in symptomatic and asymptomatic dogs.

Author

de Carvalho FLN, Riboldi EO, Bello GL, Ramos RR, Barcellos RB, Gehlen M, Halon ML, Romão PRT, Dallegrave E, and Rossetti MLR

Subjects

Animals, Asymptomatic Infections, Brazil, Chromatography, Affinity methods, Dog Diseases parasitology, Dogs, Enzyme-Linked Immunosorbent Assay methods, Leishmaniasis, Visceral parasitology, Real-Time Polymerase Chain Reaction methods, Chromatography, Affinity veterinary, Dog Diseases diagnosis, Enzyme-Linked Immunosorbent Assay veterinary, Leishmania infantum isolation & purification, Leishmaniasis, Visceral diagnosis, Real-Time Polymerase Chain Reaction veterinary

Abstract

Although serological assays have been widely used for the diagnosis of canine visceral leishmaniasis (CVL), they present different performances depending on the clinical profile of the dogs. This study evaluated the accuracy of serological tests, immunochromatographic (Dual Path Platform: DPP®) and enzyme-linked immunosorbent (ELISA EIE®), for CVL in relation to the detection of Leishmania DNA through real-time polymerase chain reaction (real-time PCR) in samples from symptomatic and asymptomatic dogs from a non-endemic area in the state of Rio Grande do Sul, Southern Brazil. Serum from 140 dogs (39 symptomatic and 101 asymptomatic) was tested by DPP and ELISA followed by real-time PCR. From a total of 140 samples evaluated, Leishmania DNA was detected by real-time PCR in 41.4% (58/140). Moreover, 67.2% of samples positive in real-time PCR were positive in both DPP and ELISA (39/58), showing moderate agreement between methods. In the symptomatic group, one sample non-reactive in both serological assays was positive in real-time PCR, whereas in the asymptomatic group, 17.8% non-reactive or undetermined samples in serological assays were positive in the molecular method. Leishmania DNA was not detected in 17.9% reactive samples by serological assays from the symptomatic group, and in 3.9% from asymptomatic dogs. Real-time PCR demonstrated greater homogeneity between symptomatic and asymptomatic groups compared with DPP and ELISA. The molecular method can help to establish the correct CVL diagnosis, particularly in asymptomatic dogs, avoiding undesirable euthanasia.

Published

2018

36. Development and validation of a duplex real-time PCR assay for the diagnosis of equine piroplasmosis.

Author

Lobanov VA, Peckle M, Massard CL, Brad Scandrett W, and Gajadhar AA

Subjects

Animals, Babesia isolation & purification, Babesiosis epidemiology, Babesiosis parasitology, Brazil epidemiology, Canada epidemiology, Enzyme-Linked Immunosorbent Assay veterinary, Horse Diseases parasitology, Horses, Japan epidemiology, Protozoan Infections, Animal diagnosis, Protozoan Infections, Animal epidemiology, RNA, Ribosomal, 18S genetics, Real-Time Polymerase Chain Reaction methods, Reproducibility of Results, Risk Factors, Seroepidemiologic Studies, Theileria isolation & purification, Ticks, Babesia genetics, Babesiosis diagnosis, Horse Diseases diagnosis, Real-Time Polymerase Chain Reaction veterinary, Theileria genetics

Abstract

Background: Equine piroplasmosis (EP) is an economically significant infection of horses and other equine species caused by the tick-borne protozoa Theileria equi and Babesia caballi. The long-term carrier state in infected animals makes importation of such subclinical cases a major risk factor for the introduction of EP into non-enzootic areas. Regulatory testing for EP relies on screening of equines by serological methods. The definitive diagnosis of EP infection in individual animals will benefit from the availability of sensitive direct detection methods, for example, when used as confirmatory assays for non-negative serological test results. The objectives of this study were to develop a real-time quantitative polymerase chain reaction (qPCR) assay for simultaneous detection of both agents of EP, perform comprehensive evaluation of its performance and assess the assay's utility for regulatory testing., Results: We developed a duplex qPCR targeting the ema-1 gene of T. equi and the 18S rRNA gene of B. caballi and demonstrated that the assay has high analytical sensitivities for both piroplasm species. Validation of the duplex qPCR on samples from 362 competitive enzyme-linked immunosorbent assay (cELISA)-negative horses from Canada and the United States yielded no false-positive reactions. The assay's performance was further evaluated using samples collected from 430 horses of unknown EP status from a highly endemic area in Brazil. This set of samples was also tested by a single-target 18S rRNA qPCR for T. equi developed at the OIE reference laboratory for EP in Japan, and a previously published single-target 18S rRNA qPCR for B. caballi whose oligonucleotides we adopted for use in the duplex qPCR. Matching serum samples were tested for antibodies to these parasites using cELISA. By the duplex qPCR, T. equi-specific 18S rRNA qPCR and cELISA, infections with T. equi were detected in 87.9% (95% confidence interval, CI: 84.5-90.7%), 90.5% (95% CI: 87.3-92.3%) and 87.4% (95% CI: 84.0-90.2%) of the horses, respectively. The B. caballi prevalence estimates were 9.3% (95% CI: 6.9-12.4%) by the duplex qPCR and 7.9% (95% CI: 5.7-10.9%) by the respective single-target qPCR assay. These values were markedly lower compared to the seroprevalence of 58.6% (95% CI: 53.9-63.2%) obtained by B. caballi-specific cELISA. The relative diagnostic sensitivity of the duplex qPCR for T. equi was 95.5%, as 359 of the 376 horses with exposure to T. equi confirmed by cELISA had parasitemia levels above the detection limit of the molecular assay. In contrast, only 39 (15.5%) of the 252 horses with detectable B. caballi-specific antibodies were positive for this piroplasm species by the duplex qPCR., Conclusions: The duplex qPCR described here performed comparably to the existing single-target qPCR assays for T. equi and B. caballi and will be more cost-effective in terms of results turnaround time and reagent costs when both pathogens are being targeted for disease control and epidemiological investigations. These validation data also support the reliability of the ema-1 gene-specific oligonucleotides developed in this study for confirmatory testing of non-negative serological test results for T. equi by qPCR. However, the B. caballi-specific qPCR cannot be similarly recommended as a confirmatory assay for routine regulatory testing due to the low level of agreement with serological test results demonstrated in this study. Further studies are needed to determine the transmission risk posed by PCR-negative equines with detectable antibodies to B. caballi.

Published

2018

37. A new quantitative PCR method for the detection of Anaplasma platys in dogs based on the citrate synthase gene.

Author

da Silva CB, Pires MS, Vilela JA, Peckle M, da Costa RL, Vitari GL, Santos LA, Santos HA, and Massard CL

Subjects

Anaplasma genetics, Anaplasma metabolism, Anaplasmosis microbiology, Animals, Brazil, Citrate (si)-Synthase genetics, Citrate (si)-Synthase metabolism, DNA Primers, Dog Diseases microbiology, Dogs, Predictive Value of Tests, Real-Time Polymerase Chain Reaction veterinary, Anaplasma isolation & purification, Anaplasmosis diagnosis, Dog Diseases diagnosis

Abstract

Anaplasma platys is an obligate intracellular bacterium that primarily affects dogs, but it can also infect humans. Our study aimed to standardize a quantitative real-time (q)PCR method using the citrate synthase gene (gltA) as a specific target for A. platys detection in naturally infected dogs. Primers (gltA84F and gltA84R) and probe (PLATYSp) were designed to amplify an 84-bp fragment based on the gltA gene sequences of A. platys available in GenBank. A total of 186 dog blood samples originating from the Brazilian state of Rio de Janeiro were tested by qPCR. Additionally, the same samples were tested by cytology and a nested (n)PCR that targeted the 16S ribosomal DNA to determine the performance of our qPCR method compared to these existing techniques. Among the samples tested with qPCR, 17.2% were considered positive, significantly more than detected by nPCR (14.0%). Under optical microscopy, inclusions were observed in platelets of 25.3% of the samples, and among these samples, only 33.9% were identified as positive for A. platys using qPCR. The qPCR technique proved to be more specific than cytology and to have superior sensitivity to nPCR for detecting A. platys in dogs. The development of this new qPCR method contributes to the advancement of research involving A. platys Furthermore, it can be used to quantify the presence of this bacterium to evaluate the treatment of infected animals, or even as a more sensitive and specific tool for situations indicating possible clinical disease but with negative cytology., (© 2016 The Author(s).)

Published

2016

38. Detection of Leishmania infantum in 4 different dog samples by real-time PCR and ITS-1 nested PCR.

Author

Carvalho Ferreira AL, Carregal VM, de Almeida Ferreira S, Leite RS, and de Andrade AS

Subjects

Animals, Brazil, Conjunctiva parasitology, Dog Diseases parasitology, Dogs, Leishmania infantum genetics, Leishmaniasis, Visceral diagnosis, Leishmaniasis, Visceral parasitology, Specimen Handling methods, Dog Diseases diagnosis, Leishmania infantum isolation & purification, Leishmaniasis, Visceral veterinary, Polymerase Chain Reaction methods, Real-Time Polymerase Chain Reaction methods

Abstract

The canine visceral leishmaniasis (CVL) diagnosis is an important step of visceral leishmaniasis control program in Brazil, which involves the elimination of infected dogs, the main animal reservoir host of the disease. The aim of the present study was to evaluate a sensitive real-time PCR method for Leishmania infantum detection in 4 different clinical samples of dogs, including the noninvasive conjunctival swab (CS) sample. The results of real-time PCR were compared with those obtained using internal transcribed spacer 1 nested PCR. Animals were divided into 2 groups based on the absence or presence of CVL clinical sings. The CS associated with real-time PCR, using primers addressed to kinetoplast DNA minicircles, was able to detect L. infantum infection in 96.7% of dogs without clinical signs and in 100% of the symptomatic animals, demonstrating the importance of these procedures for diagnosing CVL., (Copyright © 2014 Elsevier Inc. All rights reserved.)

Published

2014

39. A Multiplex real-time PCR for detection of Mycoplasma gallisepticum and Mycoplasma synoviae in clinical samples from Brazilian commercial poultry flocks.

Author

Fraga AP, de Vargas T, Ikuta N, Fonseca AS, Celmer ÁJ, Marques EK, and Lunge VR

Subjects

Animals, Bacteriological Techniques methods, Brazil, Multiplex Polymerase Chain Reaction methods, Mycoplasma Infections diagnosis, Mycoplasma Infections microbiology, Mycoplasma gallisepticum genetics, Mycoplasma synoviae genetics, Poultry, Poultry Diseases microbiology, Sensitivity and Specificity, Molecular Diagnostic Techniques methods, Mycoplasma Infections veterinary, Mycoplasma gallisepticum isolation & purification, Mycoplasma synoviae isolation & purification, Poultry Diseases diagnosis, Real-Time Polymerase Chain Reaction methods, Veterinary Medicine methods

Abstract

Mycoplasma gallisepticum (MS) and Mycoplasma synoviae (MS) are important avian pathogens and cause economic losses to the poultry industry. Molecular biology techniques are currently used for a rapid detection of these pathogens and the adoption of control measures of the diseases. The aim of this study was to develop and validate a technique for simultaneous detection of MG and MS by multiplex real time polymerase chain reaction (PCR). The complete assay (Multiplex MGMS) was designed with primers and probes specific for each pathogen and developed to be carried out in a single tube reaction. Vaccines, MG and MS isolates and DNA from other Mycoplasma species were used for the development and validation of the method. Further, 78 pooled clinical samples from different poultry flocks in Brazil were obtained and used to determine the sensitivity and specificity of the technique in comparison to 2 real time PCR assays specific for MG (MG PCR) and MS (MS PCR). The results demonstrated an agreement of 100% (23 positive and 44 negative samples) between Multiplex MGMS and MG PCR in the analysis of 67 samples from MG positive and negative poultry flocks, and an agreement of 96.9% between Multiplex MGMS and MS PCR in the analysis of 64 samples from MS positive and negative poultry flocks. Considering the single amplification tests as the gold standard, the Multiplex MGMS showed 100% of specificity and sensitivity in the MG analysis and 94.7% sensitivity and 100% specificity in the MS analysis. This new assay could be used for rapid analysis of MG and MS in the poultry industry laboratories.

Published

2013

40. Evaluation of laboratory tests for dengue diagnosis in clinical specimens from consecutive patients with suspected dengue in Belo Horizonte, Brazil.

Author

Ferraz FO, Bomfim MR, Totola AH, Ávila TV, Cisalpino D, Pessanha JE, da Glória de Souza D, Teixeira Júnior AL, Nogueira ML, Bruna-Romero O, and Teixeira MM

Subjects

Adult, Antibodies, Viral blood, Antigens, Viral blood, Brazil, Enzyme-Linked Immunosorbent Assay methods, Female, Humans, Immunoglobulin M blood, Male, Middle Aged, Molecular Sequence Data, RNA, Viral genetics, Sensitivity and Specificity, Sequence Analysis, DNA, Chromatography, Affinity methods, Clinical Laboratory Techniques methods, Dengue diagnosis, Real-Time Polymerase Chain Reaction methods

Abstract

Background: Dengue is a widely spread arboviral disease in tropical and subtropical regions of the world. Dengue fever presents clinical characteristics similar to other febrile illness. Thus laboratory diagnosis is important for adequate management of the disease., Objectives: The present study was designed to evaluate the diagnostic performance of real-time PCR and serological methods for dengue in a real epidemic context., Study Design: Clinical data and blood samples were collected from consecutive patients with suspected dengue who attended a primary health care unit in Belo Horizonte, Brazil. Serologic methods and real-time PCR were performed in serum samples to confirm dengue diagnosis., Results: Among the 181 consecutive patients enrolled in this study with suspected dengue, 146 were considered positive by serological criteria (positive NS1 ELISA and/or anti-dengue IgM ELISA) and 138 were positive by real-time PCR. Clinical criteria were not sufficient for distinguishing between dengue and non-dengue febrile illness. The PCR reaction was pre-optimized using samples from patients with known viral infection. It had similar sensitivity compared to NS1 ELISA (88% and 89%, respectively). We also evaluated three commercial lateral flow immunochromatographic tests for NS1 detection (BIOEASY, BIORAD and PANBIO). All three tests showed high sensitivity (94%, 91% and 81%, respectively) for dengue diagnosis., Conclusion: According to our results it can be suggested that lateral flow tests for NS1 detection are the most feasible methods for early diagnosis of dengue., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013