ABSTRACT
BACKGROUND Bovine tuberculosis (TB) is a zoonotic disease caused by Mycobacterium bovis, responsible for causing major losses in livestock. A cost effective alternative to control the disease could be herd vaccination. The bacillus Calmette-Guérin (BCG) vaccine has a limited efficacy against bovine TB, but can improved by over-expression of protective antigens. The M. bovis antigen 85B demonstrates ability to induce protective immune response against bovine TB in animal models. However, current systems for the construction of recombinant BCG expressing multiple copies of the gene result in strains of low genetic stability that rapidly lose the plasmid in vivo. Employing antibiotic resistance as selective markers, these systems also compromise vaccine safety. We previously reported the construction of a stable BCG expression system using auxotrophic complementation as a selectable marker. OBJECTIVES The fundamental aim of this study was to construct strains of M. bovis BCG Pasteur and the auxotrophic M. bovis BCG ΔleuD expressing Ag85B and determine their stability in vivo. METHODS Employing the auxotrophic system, we constructed rBCG strains that expressed M. bovis Ag85B and compared their stability with a conventional BCG strain in mice. Stability was measured in terms of bacterial growth on the selective medium and retention of antigen expression. FINDINGS The auxotrophic complementation system was highly stable after 18 weeks, even during in vivo growth, as the selective pressure and expression of antigen were maintained comparing to the conventional vector. MAIN CONCLUSION The Ag85B continuous expression within the host may generate a stronger and long-lasting immune response compared to conventional systems.
Subject(s)
Animals , Female , Mice , Plasmids/genetics , Plasmids/immunology , BCG Vaccine/genetics , BCG Vaccine/immunology , Genetic Vectors/immunology , Mycobacterium bovis/genetics , Mycobacterium bovis/immunology , Antigens, Bacterial/immunology , Antigens, Bacterial/metabolism , Escherichia coli/genetics , Genetic Vectors , Mice, Inbred BALB CABSTRACT
Background: It is believed that Human Papillomavirus (HPV) and Human Immunodeficiency Virus coinfection contributes to increase the risk for cervical intraepithelial injuries. Several factors may contribute to cervical cancer (CC) development, including genetic variants such as TP53 and MDM2 gene polymorphisms. Materials and methods: A hundred HIV-infected women were examined for HPV detection and its genotypes, as well as the frequencies of the SNPs Arg72Pro and SNP309 and their associations with CC risk factors. Nested Polymerase Chain Reaction (nPCR) was used for HPV detection and PCR-RFLP for TP53 and MDM2 SNP309 genotyping. Results: HPV DNA was detected in 68% of samples. A higher frequency of low-risk HPV genotypes (66.7%) was observed when compared to high-risk genotypes (33.3%). Nine different HPV genotypes were identified, with the highest prevalence of HPV-6, followed by HPV-16 and 31. p53 Arg72Arg and SNP309 TG genotype were the most prevalent. HPV genotyping was performed by sequencing. Conclusion: The data obtained suggest that HIV-infected women are more susceptible to be infected by low-risk HPV (LR-HPV) genotypes than by high-risk (HR-HPV), and Pro72Pro of TP53 gene and TG of MDM2 SNP309 genotypes apparently seem to be protective factors among HIV-infected women for HPV acquisition and HR-HPV infection, respectively, in a sample of Southern Brazilian woman. Future investigations in larger populations are necessary to better understand the potential roles of these SNPs and the behavior of non-oncogenic HPV genotypes in HIV-mediated immunosuppression cases. .
Subject(s)
Adolescent , Adult , Female , Humans , Middle Aged , DNA, Viral/genetics , HIV Infections/complications , Papillomaviridae/genetics , Papillomavirus Infections/virology , Brazil , Cross-Sectional Studies , Genotype , Polymerase Chain Reaction , Polymorphism, Restriction Fragment Length , Papillomavirus Infections/complications , Socioeconomic FactorsABSTRACT
Diagnosis of leptospirosis by PCR is hampered due to the presence of substances on biological fluids. Here, we report an immunomagnetic separation step prior to PCR which improved the detection of Leptospira spp. in blood and urine samples from dogs. It resulted in a significant improvement on sensitivity for diagnosis of canine leptospirosis.
Subject(s)
Animals , Dogs , Diagnostic Techniques and Procedures , Immunogenetics , In Vitro Techniques , Leptospira interrogans serovar canicola , Leptospirosis , Polymerase Chain Reaction/methods , Dogs , MethodsABSTRACT
The development of diagnostic tests which can readily differentiate between vaccinated and tuberculosis-infected individuals is crucial for the wider utilization of bacillus Calmette-Guérin (BCG) as vaccine in humans and animals. BCG_0092 is an antigen that elicits specific delayed type hypersensitivity reactions similar in size and morphological aspects to that elicited by purified protein derivative, in both animals and humans infected with the tubercle bacilli. We carried out bioinformatics analyses of the BCG_0092 and designed a diagnostic test by using the predicted MHC class I epitopes. In addition, we performed a knockout of this gene by homologous recombination in the BCG vaccine strain to allow differentiation of vaccinated from infected individuals. For that, the flanking sequences of the target gene (BCG_0092)were cloned into a suicide vector. Spontaneous double crossovers, which result in wild type revertants or knockouts were selected using SacB. BCG_0092 is present only in members of the Mycobacterium tuberculosis complex. Eight predicted MHC class I epitopes with potential for immunological diagnosis were defined, allowing the design of a specific diagnostic test. The strategy used to delete the (BCG_0092) gene from BCG was successful. The knockout genotype was confirmed by PCR and by Southern blot. The mutant BCG strain has the potential of inducing protection against tuberculosis without interfering with the diagnostic test based on the use of selected epitopes from BCG_0092.
Subject(s)
Humans , Adjuvants, Immunologic , Epitopes, T-Lymphocyte/immunology , Mycobacterium tuberculosis/immunology , Tuberculosis/diagnosis , Tuberculosis/immunology , BCG Vaccine/immunology , Computational Biology , Epitopes, T-Lymphocyte/analysis , Gene Knockout Techniques , Histocompatibility Antigens Class I/immunology , Hypersensitivity, Delayed/immunology , Mycobacterium bovis/genetics , Mycobacterium bovis/immunology , Mycobacterium tuberculosis/genetics , Tuberculosis Vaccines/immunology , Tuberculosis/prevention & controlABSTRACT
The objective of this study was to evaluate neuropeptide Y (NPY) and sea bream gonadotropin-release hormone (sbGnRH) gene expression in juvenile and adult males of Brazilian flounder. Hypothalamuses from fish were sampled for total RNA extraction. After cDNA synthesis, real-time PCR was used to measure gene expression. NPY showed approximately 2-fold increases in their mRNA levels while sbGnRH showed 3-fold increases in adult fish. These results suggest that these peptides could be involved on hypothalamic regulation of Brazilian flounder sexual maturation.
O objetivo deste estudo foi avaliar a expressão gênica do neuropeptídeo Y (NPY) e da variante sea bream do hormônio liberador de gonadotrofinas (sbGnRH) em linguados machos juvenis e adultos. O hipotálamo foi isolado para a extração de RNA total. Após a síntese de cDNA, a PCR em tempo real foi usada para avaliar a expressão gênica. Foi observado um aumento de aproximadamente duas vezes nos níveis de NPY e de aproximadamente três vezes nos níveis de sbGnRH nos peixes adultos. Esses resultados demonstram que estes peptídeos podem estar envolvidos na regulação, via hipotálamo, da maturação sexual no linguado.
ABSTRACT
The silver catfi sh (Rhamdia quelen) is an endemic American fi sh species. The sperm of each species has its own peculiarities and biological characteristics, which infl uence the success of mass DNA transfer methods. Our objective in this study was to evaluate different sperm-mediated gene transfer (SMGT) methods to obtain transgenic silver catfi sh. Different treatments for the incorporation of a foreign pEGFP plasmid group were used: (1) dehydrated/ rehydrated (DR), (2) dehydrated/rehydrated/electroporated (DRE), (3) electroporated (E), (4) incubated with seminal plasma (INC); and (5) incubated in the absence of seminal plasma (INCSP). Sperm motility, time of activity duration (TAD), fertilization rate (FR), hatching rate (HR) and sperm morphology were also evaluated. The polymerase chain reaction (PCR) positivity rates for the presence of the transgene were: DRE 60%; DR 40%; E 25%; INC 5% and INCSP 25%. The rates of embryo EGFP expression were: DRE 63%; DR 44%; E 34%; INC 8% and INCSP 38%. The fertilization rate in the control and DRE treatments groups were higher than in the DR group, but the E, INC and INCSP treatment groups had the lowest rate. The hatching rates of the DRE, DR and control groups were higher than in the INCSP, INC and E treatment groups (P>0.05). There were no differences among the DRE and DR, E and DR, E and INCSP groups in expression and PCR positivity rates of enhanced green fl uorescent protein (EGFP) in embryos. Scanning electron microscopy also did not show any change in sperm morphology among treatment groups. To the best of our knowledge, this is the fi rst report on transgene transmission of exogenous DNA into silver catfi sh larvae through SMGT technology.
ABSTRACT
With the aim of isolating Leptospira spp., blood serum, kidney, liver and genital tract of 137 female swine (40 sows and 97 gilts) and also urine samples from 22 sows were collected in a slaughterhouse in the State of São Paulo, from April 2003 to August 2004. Four isolates were obtained from animals that presented microagglutination test (MAT) titers > 100 for the serovar Pomona and one was obtained from an animal negative by MAT in which Leptospira was isolated from the liver and reproductive tract. The presence of leptospiral DNA was investigated by PCR, and positive results were found in kidneys of 11 females, liver of two, genital tract of two and urine of one of them. Nephrosis, interstitial multifocal nephritis, moderate to severe changing, hyalines cylinders and hemorrhagic focuses, hepatic and uterine horns congestion were histological lesions observed in higher frequency in animals positive for leptospira. The silver impregnation (Warthin Starry) confirmed the presence of spirochetes in renal tubules of four females with positive leptospira cultures from kidneys. The serogroup of the five isolates was identified as Pomona by cross agglutination with reference polyclonal antibodies. Molecular characterization of the isolates was carried out by variable-number tandem-repeats analysis. All the isolates revealed a pattern distinct from the L. interrogans Pomona type strain, but identical to a previously identified pattern from strains isolated in Argentina belonging to serovar Pomona.
Amostras de soro sanguíneo, rim, fígado e trato genital de 137 fêmeas suínas (40 matrizes e 97 marrãs) e de urina de 22 matrizes foram colhidas em abatedouro no Estado de São Paulo, no período de abril de 2003 a agosto de 2004 tendo como objetivo o isolamento de Leptospira spp. Quatro estirpes foram isoladas de animais que apresentaram títulos, no teste de soroaglutinação microscópica (SAM) > 100, para o sorovar Pomona e de um animal, não reagente na SAM, em que houve isolamento de leptospiras do fígado e aparelho reprodutor. A presença do DNA de leptospira foi investigada pela técnica da PCR e foram observados resultados positivos nos rins de 11 fêmeas, no fígado de duas, no aparelho reprodutor de duas e na urina de uma delas. Nefrose, nefrite intersticial multifocal variando de moderada a severa, cilindros hialinos e focos hemorrágicos, congestão hepática e de cornos uterinos foram lesões histológicas evidenciadas com freqüência mais alta em animais positivos para leptospira. A impregnação argêntica (Warthin Starry) confirmou a presença de espiroquetas nos túbulos renais das quatro fêmeas onde houve cultura positiva para leptospiras dos rins. O sorogrupo dos cinco isolados foi identificado como Pomona pela técnica de aglutinação cruzada com anticorpos policlonais de referência. A caracterização molecular dos isolados foi realizada pela análise do número variável de repetições em tandem (VNTR). Os mesmos revelaram um padrão distinto da estirpe padrão de L. interrogans sorovar Pomona, porém idêntico a um padrão previamente identificado em estirpes isoladas na Argentina, pertencentes ao sorovar Pomona.
Subject(s)
Animals , In Vitro Techniques , Leptospira interrogans/isolation & purification , Serologic Tests , Swine , Diagnostic Techniques and Procedures , Methods , Polymerase Chain Reaction , MethodsABSTRACT
A leptospirose constitui um problema sanitário de importância mundial. Esta doença caracteriza-se por apresentar sintomas muito parecidos com os de outras doenças como a dengue e a gripe e, clinicamente é difícil de distingui-las. Técnicas de diagnóstico da leptospirose atualmente disponíveis apresentam baixa sensibilidade e ou especificidade. Por isso, tem havido um grande esforço no sentido de desenvolver testes rápidos e eficientes, baseados em técnicas de biologia molecular. Este trabalho objetivou a avaliação e otimização do Nested-PCR, para o diagnóstico de leptospirose. Para isso foi desenhado um par de primers que amplifica uma região de 264 pb do gene LipL32. A sensibilidade e especificidade do teste foram avaliadas utilizando 7 sorovares saprófitas e 35 sorovares patogênicos. Este PCR mostrou-se específico para leptospiras patogênicas, porém a sensibilidade não foi muito alta. Com o objetivo de melhorar a sensibilidade do teste , foi desenhado outro par de primers que amplifica uma região de 183 pb do gene LipL32, interna a de 264 pb para a realização do Nested-PCR. Nesta reação foi utilizado como DNA molde o produto da primeira amplificação. O Nested-PCR mostrou-se mais sensível que o PCR normal, pois foi capaz de detectar um baixo número de células bacterianas.
ABSTRACT
Leptospirosis is a worldwide sanitary problem. Its clinical signs resemble that of other diseases like Dengue and Flu, and it is difficult to distinguish between them. Currently available diagnostic methods shown low sensitivity and specificity. Efforts have been made to develop simpler, faster and more efficient diagnostic methods. The aim of this work was to evaluate and optimize a Nested-PCR method for diagnosis of leptospirosis. Primers were designed to amplify a 264 bp region within the LipL32 gene. The sensitivity and specificity of the assay was evaluated using seven saprophytic serovars and 35 pathogenic serovars. This technique showed to be very specific for pathogenic serovars, however it lacked sensitivity. In order to enhance the sensitivity, another primer pair was designed which amplify a 183 bp region within the 264 bp region in lipL32 gene, and used in a Nested-PCR assay. This approach was much more sensitive than traditional PCR.
A leptospirose constitui um problema sanitário de importância mundial. Esta doença caracteriza-se por apresentar sintomas muito parecidos com os de outras doenças como a dengue e a gripe e, clinicamente é difícil de distingui-las. Técnicas de diagnóstico da leptospirose atualmente disponíveis apresentam baixa sensibilidade e ou especificidade. Por isso, tem havido um grande esforço no sentido de desenvolver testes rápidos e eficientes, baseados em técnicas de biologia molecular. Este trabalho objetivou a avaliação e otimização do Nested-PCR, para o diagnóstico de leptospirose. Para isso foi desenhado um par de primers que amplifica uma região de 264 pb do gene LipL32. A sensibilidade e especificidade do teste foram avaliadas utilizando 7 sorovares saprófitas e 35 sorovares patogênicos. Este PCR mostrou-se específico para leptospiras patogênicas, porém a sensibilidade não foi muito alta. Com o objetivo de melhorar a sensibilidade do teste , foi desenhado outro par de primers que amplifica uma região de 183 pb do gene LipL32, interna a de 264 pb para a realização do Nested-PCR. Nesta reação foi utilizado como DNA molde o produto da primeira amplificação. O Nested-PCR mostrou-se mais sensível que o PCR normal, pois foi capaz de detectar um baixo número de células bacterianas.