Detection of Actinobacillus Pleuropneumoniae and Identification of Serotypes 1, 2, and 8 by Multiplex Polymerase Chain Reaction

Schuchert, Jennifer Ann

30 August 2002

Traditional immunological assays used to serotype Actinobacillus pleuropneumoniae have been problematic due to cross- reactivity between serotypes, particularly serotypes 6 and 8. To avoid these serological cross-reactions, a multiplex PCR assay was developed to detect A. pleuropneumoniae and identify serotypes 1, 2, and 8. Primers specific to the conserved capsular polysaccharide export region of A. pleuropneumoniae serotype 5 amplified a 880 bp fragment in all serotypes excluding serotype 4 or a 489 bp DNA fragment in all serotypes including serotype 4. Primers specific to the capsular polysaccharide biosynthesis regions of A. pleuropneumoniae serotypes 1, 2, and 8 amplified a 1.6 kb, a 1.7 kb, and 970 bp fragment in the respective serotype. This PCR assay detects A. pleuropneumoniae and identifies serotypes 1, 2, and 8. / Master of Science

Multiplex PCR

serotyping

Actinobacillus pleuropneumoniae

Desenvolvimento de uma vacina recombinante para circovirose suína e ensaios para diagnóstico molecular de PCV2 / Development of a recombinant vaccine for porcine circovirus associated disease and molecular assays to detect PCV2

Dezen, Diogenes

January 2011

O circovírus suíno tipo 2 (PCV2) é o principal agente da síndrome multissistêmica do definhamento do suíno (SMDS), uma doença mundialmente disseminada e que provoca perdas econômicas significativas para a suinocultura. Visando contribuir no diagnóstico da síndrome, o presente trabalho padronizou e comparou testes para a detecção do PCV2. Para isso, foram utilizadas as técnicas de amplificação por círculo rolante (ACR) e variações da PCR (convencional, tempo-real e competitiva). Utilizando a ACR foi possível obter a amplificação total de genomas do PCV2, os quais foram clonados, sequenciados e agrupados no genótipo PCV2b. Os genomas clonados foram isolados, recircularizados e transfectados em células PK-15. Este procedimento possibilitou a recuperação do vírus infeccioso em títulos de até 105,55 DICC50/mL. Portanto, a ACR foi uma ferramenta útil em estratégias de isolamento e sequenciamento do vírus. No entanto, a ACR foi menos sensível que a PCR para fins de detecção do PCV2. No segundo estudo, buscando métodos auxiliares no diagnóstico da SMDS, dois ensaios para a quantificação do PCV2 foram desenvolvidos. Estes ensaios foram baseados nas técnicas de PCR competitivo (cPCR) e de PCR em tempo real. Visando determinar qual seria o mais adequado para estimar a carga viral do PCV2, os dois métodos foram comparados. Ambos os ensaios foram capazes de detectar diferenças significativas entre o número de cópias de DNA de PCV2 encontradas em tecidos de animais saudáveis e acometidos pela SMDS (≥ 2,5 log10). No entanto, uma diferença média de 1,8 log10 na carga viral foi encontrada entre ensaios, onde as maiores cargas virais foram detectadas pela PCR em tempo real. Outro objetivo deste trabalho foi gerar vacinas baseadas na proteína do capsídeo (Cap) do PCV2. Assim, no terceiro estudo, três baculovírus recombinantes foram construídos de modo a expressar a proteína Cap. Em dois recombinantes, a seqüência de nucleotídeos do peptídeo sinal (PS) da glicoproteína I do herpesvírus bovino (BoHV-gI) foi inserida na extremidade 5’ do gene cap (ORF2). Além disso, um recombinante contendo a seqüência de nucleotídeos do PS foi construído sem o sinal de localização nuclear (NLS) de proteína Cap. Através do ensaio de imunoperoxidase em monocamada (IPMA), antígenos de PCV2 foram detectados em células Sf21 infectadas pelos três vírus recombinantes. Este resultado sugere que os recombinantes construídos são potenciais candidatos vacinais, uma vez que eles foram capazes de produzir antígenos de PCV2. / Porcine circovirus type 2 (PCV2) is the major agent of postweaning multisystemic wasting syndrome (PMWS), a worldwide spread disease that causes significant economic losses to the swine productive chain. Aiming to contribute in the diagnosis of the syndrome, this thesis compared and developed tests for PCV2 detection. For this, multiply-primed rolling-circle amplification (MPRCA) and PCR-based assays (conventional, real-time and competitive) were tested. The MPRCA allowed amplifying the full-length PCV2 genomes, which were cloned, sequenced and grouped on PCV2b genotype. The cloned genomes were isolated from the plasmids, recircularized and used for transfection in PK-15 cells. This procedure led to the production of infectious virus to titres up to 105.55 TCID50/mL. It was concluded that MPRCA is a useful tool to amplify PCV2 genomes in sight of sequencing and virus isolation strategies. However, it was less sensitive than PCR for diagnostic purposes. In the second study, searching for methods in support to PMWS diagnosis, two PCR assays were developed: a competitive PCR (cPCR) and a SYBR green real-time PCR. The quantitative PCR methods were compared to determine which would be more suitable to estimate the PCV2 DNA load. Both assays were able to detect significant differences between the numbers of PCV2 DNA copies found in tissues of PMWS-affected and non-PMWS-affected pigs (≥2.5 log10). However, a mean difference of 1.8 log10 on the viral load was found between assays, where the highest viral loads were detected by SYBR green real-time PCR. In the work outlined herein, another purpose was to generate vaccine candidates based on PCV2 capsid protein (Cap). Therefore, in the third study, three types of recombinant baculoviruses were constructed to express the Cap protein. In two recombinants, the nucleotide sequence from the signal peptide (SP) of bovine herpesvirus glycoprotein I (BoHV-gI) was inserted at the 5’ end of the cap gene (ORF2). Additionally, one recombinant containing the SP nucleotide sequence was constructed lacking the nuclear localization signal (NLS) of Cap protein. Through immunoperoxidase monolayer assay (IPMA), the PCV2 antigen was detected in Sf21 cells infected by the three recombinant viruses. This result suggests that the recombinants here constructed are potential vaccine candidates, once they were able to produce PCV2 antigens.

Circovirose suína

PCR

Vacina

Diagnostico molecular

PCV2

Vaccine

PMWS

MPRCA

Real-time PCR

Competitive PCR

Baculovirus

Aplicação de métodos moleculares no diagnóstico de endoftalmite bacteriana / Use of molecular methods to bacterial endophthalmitis diagnostic

Bispo, Paulo José Martins [UNIFESP]

29 April 2009

Made available in DSpace on 2015-07-22T20:49:25Z (GMT). No. of bitstreams: 0 Previous issue date: 2009-04-29. Added 1 bitstream(s) on 2015-08-11T03:26:21Z : No. of bitstreams: 1 Publico-178.pdf: 625763 bytes, checksum: bd311a8cd3f7ff010bc833233dd4c82b (MD5) / Objetivo: Desenvolvimento e aplicação de protocolos de Nested Multiplex PCR e PCR em Tempo Real para a detecção bacteriana e classificação de Gram em amostras de humor aquoso e vítreo coletadas de pacientes com suspeita clínica de endoftalmite. Métodos: Especificidade analítica foi estabelecida utilizando 31 microrganismos clinicamente importantes, 20 gram-positivos e 11 gram-negativos. Reação cruzada com DNA humano e DNA fúngico foi testada. Amostras controles de humor aquoso coletadas após facoemulsificação foram incluídas. Sensibilidade analítica para as metodologias de PCR foram determinadas utilizando diluição seriada 1:10 de DNA extraído de S. epidermidis e E. coli. As técnicas foram posteriormente aplicadas e testadas em amostras de humor aquoso e vítreo coletadas de pacientes com diagnóstico clínico de endoftalmite. Preparações comerciais de Taq DNA polimerase foram pré-tratadas com DNaseI. Resultados: Amplificação genérica do gene 16S rDNA foi positiva para todos os isolados bacterianos. Classificação de Gram pela técnica de Nested Multiplex PCR não foi possível apenas para isolados de Acinetobacter spp. Utilizando PCR Multiplex em Tempo Real, todos os isolados foram classificados por Gram, sendo que P. acnes exibiu um padrão misto de amplificação. Limite de detecção da metodologia de Nested Multiplex PCR foi de 1 fg/μl para S. epidermidis e E.coli. A sensibilidade de detecção para S. epidermidis e E. coli utilizando reação para detecção universal bacteriana por PCR em Tempo Real com SYBR Green foi de 100 fg/μl (E = 0,82 e 0,86; r2 = 0,99) e 1 pg/μl utilizando metodologia de PCR Multiplex em Tempo Real com Sondas TaqMan (E = 0,66 e 0,77; r2 = 0,99). A positividade da cultura para detecção bacteriana a partir de amostras de humor aquoso e vítreo foi de 47,6% e pelas metodologias de Nested Multiplex PCR e PCR em Tempo Real foi de 100% e 95,2% respectivamente. Entre as amostras negativas por cultura (n=10), a metodologia de Nested Multiplex PCR foi positiva para todas (100%) e PCR em Tempo Real em 90% dos casos (9/10). Entretanto, a proporção de falso-positivos pela metodologia de Nested Multiplex PCR (65,4%) foi superior aos valores obtidos por PCR em Tempo Real (7,7%). A classificação de gram foi obtida em 88,8% dos casos por Nested PCR e 100% por PCR em Tempo Real. A correlação entre a identificação clássica e classificação de Gram molecular foi 63,6% para ambas as técnicas. A identificação pelo sequenciamento dos produtos obtidos por Nested Multiplex PCR e PCR em Tempo Real apresentou correlação de 100% e 88,8%, respectivamente, quando comparada a identificação fenotípica. Conclusões: As metodologias de PCR apresentaram boa correlação quando comparadas com os resultados da cultura e a detecção passou de 47,6% por cultura para 100%, demonstrando serem testes viáveis e mais sensíveis para a caracterização laboratorial de endoftalmite. / Objective: Development and application of Nested Multiplex PCR and Real Time PCR assays for detection and Gram classification of bacteria using aqueous and vitreous humor collected from patients with suspected endophthalmitis. Methods: Analytical specificity was established using 31 clinically important pathogens, 20 gram-positive and 11 gram-negative. Specificity was also tested using human DNA and fungal DNA. Control samples of non-infected aqueous humor collected at the end of phacoemulsification surgery were included. Analytical sensitivity was determined using a 10-fold dilution of S. epidermidis and E. coli DNA. After, methodologies were tested in aqueous and vitreous humor collected from patients with clinical diagnosis of endophthalmitis. Comercial Taq polymersase preparations were DNA decontaminated using DNaseI pretreatment. Results: Universal amplification of 16S rDNA was achieved for all bacterial isolated. Nested Multiplex PCR failed only to determine the Gram status of Acinetobacter spp. Gram classification was achieved for every bacterial isolates using a Multiplex Gram-Specific TaqMan-based PCR, and only a P. acnes isolate showed a mixed signal. Limit of detection using Nested Multiplex PCR was 1 fg/μl for both S. epidermidis and E. coli. Sensitivity for detection of S. epidermidis and E. coli DNA using a SYBR Green 16S rDNA-based universal PCR was 100 fg/μl (E = 0.82 and 0.86; r2 = 0.99) and 1 pg/μl using a Multiplex Gram-Specific TaqMan-based PCR (E = 0.66 and 0.77; r2 = 0.99). Culture was positive in 47.6% of aqueous and vitreous humor analysis. Nested Multiplex PCR and Real Time PCR assays were positive in 100% and 95.2% of these cases, respectively. Among negative culture samples, Nested Multiplex PCR was positive for all (100%) and Real Time PCR assays in 90% of cases (9/10). Gram classification was completed for 88.8% and 100% samples using Nested Multiplex PCR and Real Time PCR methodologies, respectively. Correlation of 63.6% between microbiological and molecular Gram classification was observed using both molecular assays. 16S rDNA sequence-based identification using Nested Multiplex PCR and Real Time PCR products showed 100% and 88.8% correlation respectively when compared with phenotypic identification. Conclusions: Both PCR methodologies presented good correlation when compared with culture-proven results and bacterial detection was improved from 47.6%% to 100% showing to be feasible tests for laboratorial characterization of bacterial endophthalmitis. / TEDE / BV UNIFESP: Teses e dissertações

Endoftalmite bacteriana

Infecções intra-oculares

Multiplex PCR

Nested PCR

PCR em Tempo Real

Desenvolvimento de uma vacina recombinante para circovirose suína e ensaios para diagnóstico molecular de PCV2 / Development of a recombinant vaccine for porcine circovirus associated disease and molecular assays to detect PCV2

Dezen, Diogenes

January 2011

O circovírus suíno tipo 2 (PCV2) é o principal agente da síndrome multissistêmica do definhamento do suíno (SMDS), uma doença mundialmente disseminada e que provoca perdas econômicas significativas para a suinocultura. Visando contribuir no diagnóstico da síndrome, o presente trabalho padronizou e comparou testes para a detecção do PCV2. Para isso, foram utilizadas as técnicas de amplificação por círculo rolante (ACR) e variações da PCR (convencional, tempo-real e competitiva). Utilizando a ACR foi possível obter a amplificação total de genomas do PCV2, os quais foram clonados, sequenciados e agrupados no genótipo PCV2b. Os genomas clonados foram isolados, recircularizados e transfectados em células PK-15. Este procedimento possibilitou a recuperação do vírus infeccioso em títulos de até 105,55 DICC50/mL. Portanto, a ACR foi uma ferramenta útil em estratégias de isolamento e sequenciamento do vírus. No entanto, a ACR foi menos sensível que a PCR para fins de detecção do PCV2. No segundo estudo, buscando métodos auxiliares no diagnóstico da SMDS, dois ensaios para a quantificação do PCV2 foram desenvolvidos. Estes ensaios foram baseados nas técnicas de PCR competitivo (cPCR) e de PCR em tempo real. Visando determinar qual seria o mais adequado para estimar a carga viral do PCV2, os dois métodos foram comparados. Ambos os ensaios foram capazes de detectar diferenças significativas entre o número de cópias de DNA de PCV2 encontradas em tecidos de animais saudáveis e acometidos pela SMDS (≥ 2,5 log10). No entanto, uma diferença média de 1,8 log10 na carga viral foi encontrada entre ensaios, onde as maiores cargas virais foram detectadas pela PCR em tempo real. Outro objetivo deste trabalho foi gerar vacinas baseadas na proteína do capsídeo (Cap) do PCV2. Assim, no terceiro estudo, três baculovírus recombinantes foram construídos de modo a expressar a proteína Cap. Em dois recombinantes, a seqüência de nucleotídeos do peptídeo sinal (PS) da glicoproteína I do herpesvírus bovino (BoHV-gI) foi inserida na extremidade 5’ do gene cap (ORF2). Além disso, um recombinante contendo a seqüência de nucleotídeos do PS foi construído sem o sinal de localização nuclear (NLS) de proteína Cap. Através do ensaio de imunoperoxidase em monocamada (IPMA), antígenos de PCV2 foram detectados em células Sf21 infectadas pelos três vírus recombinantes. Este resultado sugere que os recombinantes construídos são potenciais candidatos vacinais, uma vez que eles foram capazes de produzir antígenos de PCV2. / Porcine circovirus type 2 (PCV2) is the major agent of postweaning multisystemic wasting syndrome (PMWS), a worldwide spread disease that causes significant economic losses to the swine productive chain. Aiming to contribute in the diagnosis of the syndrome, this thesis compared and developed tests for PCV2 detection. For this, multiply-primed rolling-circle amplification (MPRCA) and PCR-based assays (conventional, real-time and competitive) were tested. The MPRCA allowed amplifying the full-length PCV2 genomes, which were cloned, sequenced and grouped on PCV2b genotype. The cloned genomes were isolated from the plasmids, recircularized and used for transfection in PK-15 cells. This procedure led to the production of infectious virus to titres up to 105.55 TCID50/mL. It was concluded that MPRCA is a useful tool to amplify PCV2 genomes in sight of sequencing and virus isolation strategies. However, it was less sensitive than PCR for diagnostic purposes. In the second study, searching for methods in support to PMWS diagnosis, two PCR assays were developed: a competitive PCR (cPCR) and a SYBR green real-time PCR. The quantitative PCR methods were compared to determine which would be more suitable to estimate the PCV2 DNA load. Both assays were able to detect significant differences between the numbers of PCV2 DNA copies found in tissues of PMWS-affected and non-PMWS-affected pigs (≥2.5 log10). However, a mean difference of 1.8 log10 on the viral load was found between assays, where the highest viral loads were detected by SYBR green real-time PCR. In the work outlined herein, another purpose was to generate vaccine candidates based on PCV2 capsid protein (Cap). Therefore, in the third study, three types of recombinant baculoviruses were constructed to express the Cap protein. In two recombinants, the nucleotide sequence from the signal peptide (SP) of bovine herpesvirus glycoprotein I (BoHV-gI) was inserted at the 5’ end of the cap gene (ORF2). Additionally, one recombinant containing the SP nucleotide sequence was constructed lacking the nuclear localization signal (NLS) of Cap protein. Through immunoperoxidase monolayer assay (IPMA), the PCV2 antigen was detected in Sf21 cells infected by the three recombinant viruses. This result suggests that the recombinants here constructed are potential vaccine candidates, once they were able to produce PCV2 antigens.

Circovirose suína

PCR

Vacina

Diagnostico molecular

PCV2

Vaccine

PMWS

MPRCA

Real-time PCR

Competitive PCR

Baculovirus

Desenvolvimento de uma vacina recombinante para circovirose suína e ensaios para diagnóstico molecular de PCV2 / Development of a recombinant vaccine for porcine circovirus associated disease and molecular assays to detect PCV2

Dezen, Diogenes

January 2011

O circovírus suíno tipo 2 (PCV2) é o principal agente da síndrome multissistêmica do definhamento do suíno (SMDS), uma doença mundialmente disseminada e que provoca perdas econômicas significativas para a suinocultura. Visando contribuir no diagnóstico da síndrome, o presente trabalho padronizou e comparou testes para a detecção do PCV2. Para isso, foram utilizadas as técnicas de amplificação por círculo rolante (ACR) e variações da PCR (convencional, tempo-real e competitiva). Utilizando a ACR foi possível obter a amplificação total de genomas do PCV2, os quais foram clonados, sequenciados e agrupados no genótipo PCV2b. Os genomas clonados foram isolados, recircularizados e transfectados em células PK-15. Este procedimento possibilitou a recuperação do vírus infeccioso em títulos de até 105,55 DICC50/mL. Portanto, a ACR foi uma ferramenta útil em estratégias de isolamento e sequenciamento do vírus. No entanto, a ACR foi menos sensível que a PCR para fins de detecção do PCV2. No segundo estudo, buscando métodos auxiliares no diagnóstico da SMDS, dois ensaios para a quantificação do PCV2 foram desenvolvidos. Estes ensaios foram baseados nas técnicas de PCR competitivo (cPCR) e de PCR em tempo real. Visando determinar qual seria o mais adequado para estimar a carga viral do PCV2, os dois métodos foram comparados. Ambos os ensaios foram capazes de detectar diferenças significativas entre o número de cópias de DNA de PCV2 encontradas em tecidos de animais saudáveis e acometidos pela SMDS (≥ 2,5 log10). No entanto, uma diferença média de 1,8 log10 na carga viral foi encontrada entre ensaios, onde as maiores cargas virais foram detectadas pela PCR em tempo real. Outro objetivo deste trabalho foi gerar vacinas baseadas na proteína do capsídeo (Cap) do PCV2. Assim, no terceiro estudo, três baculovírus recombinantes foram construídos de modo a expressar a proteína Cap. Em dois recombinantes, a seqüência de nucleotídeos do peptídeo sinal (PS) da glicoproteína I do herpesvírus bovino (BoHV-gI) foi inserida na extremidade 5’ do gene cap (ORF2). Além disso, um recombinante contendo a seqüência de nucleotídeos do PS foi construído sem o sinal de localização nuclear (NLS) de proteína Cap. Através do ensaio de imunoperoxidase em monocamada (IPMA), antígenos de PCV2 foram detectados em células Sf21 infectadas pelos três vírus recombinantes. Este resultado sugere que os recombinantes construídos são potenciais candidatos vacinais, uma vez que eles foram capazes de produzir antígenos de PCV2. / Porcine circovirus type 2 (PCV2) is the major agent of postweaning multisystemic wasting syndrome (PMWS), a worldwide spread disease that causes significant economic losses to the swine productive chain. Aiming to contribute in the diagnosis of the syndrome, this thesis compared and developed tests for PCV2 detection. For this, multiply-primed rolling-circle amplification (MPRCA) and PCR-based assays (conventional, real-time and competitive) were tested. The MPRCA allowed amplifying the full-length PCV2 genomes, which were cloned, sequenced and grouped on PCV2b genotype. The cloned genomes were isolated from the plasmids, recircularized and used for transfection in PK-15 cells. This procedure led to the production of infectious virus to titres up to 105.55 TCID50/mL. It was concluded that MPRCA is a useful tool to amplify PCV2 genomes in sight of sequencing and virus isolation strategies. However, it was less sensitive than PCR for diagnostic purposes. In the second study, searching for methods in support to PMWS diagnosis, two PCR assays were developed: a competitive PCR (cPCR) and a SYBR green real-time PCR. The quantitative PCR methods were compared to determine which would be more suitable to estimate the PCV2 DNA load. Both assays were able to detect significant differences between the numbers of PCV2 DNA copies found in tissues of PMWS-affected and non-PMWS-affected pigs (≥2.5 log10). However, a mean difference of 1.8 log10 on the viral load was found between assays, where the highest viral loads were detected by SYBR green real-time PCR. In the work outlined herein, another purpose was to generate vaccine candidates based on PCV2 capsid protein (Cap). Therefore, in the third study, three types of recombinant baculoviruses were constructed to express the Cap protein. In two recombinants, the nucleotide sequence from the signal peptide (SP) of bovine herpesvirus glycoprotein I (BoHV-gI) was inserted at the 5’ end of the cap gene (ORF2). Additionally, one recombinant containing the SP nucleotide sequence was constructed lacking the nuclear localization signal (NLS) of Cap protein. Through immunoperoxidase monolayer assay (IPMA), the PCV2 antigen was detected in Sf21 cells infected by the three recombinant viruses. This result suggests that the recombinants here constructed are potential vaccine candidates, once they were able to produce PCV2 antigens.

Circovirose suína

PCR

Vacina

Diagnostico molecular

PCV2

Vaccine

PMWS

MPRCA

Real-time PCR

Competitive PCR

Baculovirus

Kvantifikace nukleových kyselin pomocí TaqMan sond - možnosti a limity s ohledem na způsob odběru, stáří a kvalitu vzorku lidských tkání / TaqMan-based nucleic acid quantification - abilities and limits with regards to type of collection, age and quality of human specimen

Herzogová, Eva

January 2014

Real-time PCR method is a type of PCR which allows continual monitoring of DNA amplification during every cycle of its process. It is mostly used for gene expression analysis. Based on the results of previous experiments, we decided to test out the effect of anticoagulants EDTA, heparin, sodium citrate and CPDA on the expression of selected genes of the immunological spectrum and further, to test how the time period between drawing the blood and processing of blood sample influences mRNA levels of selected genes that are determined by changes in gene expression and/or mRNA degradation. To quantify mRNA of the studied genes, we isolated total RNA from the peripheral blood leucocytes and transcribed it into cDNA by using the reverse transcription PCR. This cDNA served as a template for the real-time PCR. To examine the changes of the expression caused by the effect of each particular anticoagulants, peripheral blood derived from 10 volunteers was used (each donor's blood was taken into 3 vacuum tubes with EDTA, heparin and sodium citrate anticoagulant agents). Next to that, we obtained 10 buffy coat samples in transfusion blood bags with CPDA anticoagulant agent. Compared to blood cells influenced by one of the three anticoagulant agents present in vacuum tubes, cells from transfusion bags affected...

Detecção e caracterização de vírus em morcegos do Rio Grande do Sul, Brasil

Dupont, Priscilla Medeiros

January 2016

Algumas espécies de morcegos têm sido reconhecidas como reservatórios naturais de várias famílias virais, desempenhando um importante papel na trasmissão e manutenção desses micro organismos. Devido à descaracterização e fragmentação de habitats naturais, esses mamíferos buscam alternativas de abrigo e alimento, e assim, ficam cada vez mais expostos aos meios antrópicos e em contato com humanos e animais domésticos. Com exceção do vírus rábico, existem poucos trabalhos realizados na detecção de vírus em morcegos no Brasil. Em virtude disso, o presente estudo objetivou a detecção de vírus (circovírus, astrovírus, coronavírus e lyssavírus relacionados ao vírus da raiva) em amostras de órgãos de morcegos do estado do Rio Grande do Sul. Os ácidos nucléicos foram extraídos das amostras de órgãos de morcegos e submetidos à detecão por PCR e RT-PCR. Após a detecção, os fragmentos obtidos foram sequenciados para realizar análise filogenética dos vírus encontrados. Ao total foram analisadas 108 amostras de diferentes espécies e localidades, das quais dez foram positivas para circovírus, seis para coronavírus e 25 para astrovírus, este último sendo o primeiro registro do vírus em morcegos para o Brasil. Todas as amostras foram negativas para lyssavírus relacionados ao vírus da raiva. Análises filogenéticas revelaram que as sequências de circovírus agruparam em ambos os gêneros Circovirus e Cyclovirus, coronavírus no gênero Alphacoronavirus em dois clados diferentes e astrovírus no gênero Mamastrovirus junto com outros astrovírus de morcegos, o qual formam um clado separado dos outros mamíferos. Os resultados demonstram uma diversidade genética entre os vírus encontrados em diferentes espécies de morcegos, que possuem dietas alimentares e habitats distintos. / Some bat species have been recognized as natural reservoirs of several viral families, playing an important role in the transmission and maintaining of these micoorganism. Due to mischaracterization and fragmentation of natural habitats, these mammals seek shelter alternatives and food, and thus are increasingly exposed to anthropism, which make the contact with humans and domestic animals closer. With the exception of the rabies virus, there are few studies on the detection of viruses in bats in Brazil. Therefore, the present study aimed the detection of viruses (circovirus, astrovirus, coronavirus and rabies-related virus) in bats organs samples from Rio Grande do Sul state. Nucleic acids were extracted from bat organs samples and submitted to detection by PCR and RT-PCR. After detection, the obtained fragments were sequenced to perform phylogenetic analysis of the viruses found. From a total of 108 samples analyzed of different species and locations, ten were positive for circoviruses, six for coronaviruse and 25 for astrovirus, which was the first report of this virus in bats in Brazil. All samples were negative for rabies-related virus. Phylogenetic analyzes revealed that the sequences of circoviruses grouped in both Circovirus and Cyclovirus genus, coronaviruses in Alphacoronavirus genus in two different clades and astroviruses in Mamastrovirus genus along with other bats astrovirus, which form a separate clade from other mammals. Results demonstrate a genetic diversity among viruses found in different species of bats, which have different diets and habitats.

Virologia veterinaria

Morcegos : Rio Grande do Sul

Circovirus

Chiroptera

PCR

Virus da raiva

Chiroptera

PCR

RT-PCR

Circoviruses

Astroviruses

Coronaviruses

Development of Real-Time PCR Based Methods for Detection of Viruses and Virus Antibodies

Elfaitouri, Amal

January 2006

Quantitative real-time PCR (QPCR) technology has been very useful for diagnosis of viral diseases. QPCR has recently reached a level of sensitivity, simplicity, and reproducibility which allows a large number of samples to be screened rapidly, make it a suitable tool for the clinical virology diagnostics. In this thesis, broadly targeted and degenerated quantitative QPCR assays were used. A somewhat novel single-tube real-time reverse transcription-polymerase chain reaction (QRT-PCR), with takes advantage of ability of rTth DNA polymerase to reverse transcribe RNA in the presence of Mn2+ at elevated temperatures and includes protection against amplimer contamination by using thermolabile UNG, was developed. A new technique for diagnostic of recent viral infection by detection of viral immunoglobulin M (IgM) was also developed. In the first paper, a sensitive single-tube QRT-PCR for detection of enteroviral RNA in patients with aseptic meningitis was presented. In the second paper, a single-serum-dilution real-time PCR-based PIA (PCR-enhanced immunoassay), called quantitative PIA (QPIA), to detect enterovirus IgM for diagnosis of EV infection in patients with aseptic meningitis, was also developed. In the third paper, a broadly targeted, simple, single tube degenerated quantitative QPCR technique for detection of JCV, BKV and SV40 DNA was developed. A conserved region of the VP2 gene of JCV, BKV and SV40 was targeted. A false positive result due to contamination with commonly used SV40 T-antigen plasmids was therefore avoided. In manuscript four, the QPIA assay provide a rational strategy for detection of EV IgM, allows the use of viral antigens isolate from newly diagnosed Type 1 diabetes patients (T1D-EV-QPIA) to measured IgM against diabetogenic viruses in serum from newly diagnosed T1D children, siblings, and healthy children. To conclude, novel broadly targeted real-time PCR methods for diagnosis of entero- and polyoma viral infections were developed.

Microbiology

Real-time PCR

broadly targeted PCR

degenerated PCR

rTth DNA polymerase

thermolabile UNG

QPIA

IgM

Mikrobiologi

Screening For Genetically Modified Tomatoes &amp / Tomato Seeds And Identification Of Cry1ac And Sam-k Specific Modifications Using Gene And Construct Specific Pcr

Uckun, Esra

01 September 2007

This study was carried out to analyze tomato samples and tomato seeds, purchased from different food markets of Turkey randomly, for the presence of genetic modification by using PCR method as it allows more specific detection. The DNAs of collected samples were isolated according to CTAB DNA extraction protocol and also with extraction kits. Screening tests of tomatoes were done by targeting 35S promoter, NOS terminator and NptII kanamycin resistance gene with eight different primer sets. Real time PCR is used to confirm 35S and NOS positives results obtained from conventional PCR. In this study, it was observed that 14 out of 35 seed samples, and 14 out of 40 fresh tomato samples which were screened had at least one transgenic element of 35S promoter, NOS terminator and NPTII kanamycin resistance gene indicating the possible presence of genetic modifications. After screening, gene specific studies were carried out for PG, sam-k indicating F type ripening delayed tomato and the 35 1 N lines respectively and cry1Ac genes inserted in 5345-1 insect resistant tomato line. PG and sam-k specific primers were not amplified in any of the samples investigated whereas 18 out of 75 samples were cry1Ac positive and 1 out of 75 samples was sam-k positive. Positives were confirmed by sequence analysis. Additionally, construct specific primers specific to 5345-1 and 35 1 N lines were designed. PCR amplicons indicate the existence of the construct sequence. In order to verify the results, PCR products were sent to sequence analysis

QH Genetics 426-470

Detecção e caracterização de vírus em morcegos do Rio Grande do Sul, Brasil

Dupont, Priscilla Medeiros

January 2016

Algumas espécies de morcegos têm sido reconhecidas como reservatórios naturais de várias famílias virais, desempenhando um importante papel na trasmissão e manutenção desses micro organismos. Devido à descaracterização e fragmentação de habitats naturais, esses mamíferos buscam alternativas de abrigo e alimento, e assim, ficam cada vez mais expostos aos meios antrópicos e em contato com humanos e animais domésticos. Com exceção do vírus rábico, existem poucos trabalhos realizados na detecção de vírus em morcegos no Brasil. Em virtude disso, o presente estudo objetivou a detecção de vírus (circovírus, astrovírus, coronavírus e lyssavírus relacionados ao vírus da raiva) em amostras de órgãos de morcegos do estado do Rio Grande do Sul. Os ácidos nucléicos foram extraídos das amostras de órgãos de morcegos e submetidos à detecão por PCR e RT-PCR. Após a detecção, os fragmentos obtidos foram sequenciados para realizar análise filogenética dos vírus encontrados. Ao total foram analisadas 108 amostras de diferentes espécies e localidades, das quais dez foram positivas para circovírus, seis para coronavírus e 25 para astrovírus, este último sendo o primeiro registro do vírus em morcegos para o Brasil. Todas as amostras foram negativas para lyssavírus relacionados ao vírus da raiva. Análises filogenéticas revelaram que as sequências de circovírus agruparam em ambos os gêneros Circovirus e Cyclovirus, coronavírus no gênero Alphacoronavirus em dois clados diferentes e astrovírus no gênero Mamastrovirus junto com outros astrovírus de morcegos, o qual formam um clado separado dos outros mamíferos. Os resultados demonstram uma diversidade genética entre os vírus encontrados em diferentes espécies de morcegos, que possuem dietas alimentares e habitats distintos. / Some bat species have been recognized as natural reservoirs of several viral families, playing an important role in the transmission and maintaining of these micoorganism. Due to mischaracterization and fragmentation of natural habitats, these mammals seek shelter alternatives and food, and thus are increasingly exposed to anthropism, which make the contact with humans and domestic animals closer. With the exception of the rabies virus, there are few studies on the detection of viruses in bats in Brazil. Therefore, the present study aimed the detection of viruses (circovirus, astrovirus, coronavirus and rabies-related virus) in bats organs samples from Rio Grande do Sul state. Nucleic acids were extracted from bat organs samples and submitted to detection by PCR and RT-PCR. After detection, the obtained fragments were sequenced to perform phylogenetic analysis of the viruses found. From a total of 108 samples analyzed of different species and locations, ten were positive for circoviruses, six for coronaviruse and 25 for astrovirus, which was the first report of this virus in bats in Brazil. All samples were negative for rabies-related virus. Phylogenetic analyzes revealed that the sequences of circoviruses grouped in both Circovirus and Cyclovirus genus, coronaviruses in Alphacoronavirus genus in two different clades and astroviruses in Mamastrovirus genus along with other bats astrovirus, which form a separate clade from other mammals. Results demonstrate a genetic diversity among viruses found in different species of bats, which have different diets and habitats.

Virologia veterinaria

Morcegos : Rio Grande do Sul

Circovirus

Chiroptera

PCR

Virus da raiva

Chiroptera

PCR

RT-PCR

Circoviruses

Astroviruses

Coronaviruses