RÉSUMÉ
African swine fever (ASF) and classical swine fever (CSF) are two highly infectious transboundary animal diseases (TADs) that are serious threats to the pig industry worldwide, including in China, the world's largest pork producer. In this study, a duplex real-time PCR assay was developed for the rapid detection and differentiation of African swine fever virus (ASFV) and classical swine fever virus (CSFV). The assay was performed on a portable, battery-powered PCR thermocycler with a low sample throughput (termed as 'T-COR4 assay'). The feasibility and reliability of the T-COR4 assay as a possible field method was investigated by testing clinical samples collected in China. When evaluated with reference materials or samples from experimental infections, the assay performed in a reliable manner, producing results comparable to those obtained from stationary PCR platforms. Of 59 clinical samples, 41 had results identical to a two-step CSFV real-time PCR assay. No ASFV was detected in these samples. The T-COR4 assay was technically easy to perform and produced results within 3 h, including sample preparation. In combination with a simple sample preparation method, the T-COR4 assay provides a new tool for the field diagnosis and differentiation of ASF and CSF, which could be of particular value in remote areas.
Sujet(s)
Virus de la peste porcine africaine/isolement et purification , Peste porcine africaine/diagnostic , Virus de la peste porcine classique/isolement et purification , Peste porcine classique/diagnostic , Réaction de polymérisation en chaine en temps réel/médecine vétérinaire , Peste porcine africaine/virologie , Virus de la peste porcine africaine/génétique , Animaux , Peste porcine classique/virologie , Virus de la peste porcine classique/génétique , Réaction de polymérisation en chaine en temps réel/méthodes , Reproductibilité des résultats , Sensibilité et spécificité , SuidaeRÉSUMÉ
Sustainable food production capable of feeding a growing human population is a significant global challenge, and is a priority encompassed within the United Nations Millennium Development Goal to 'eradicate extreme poverty and hunger'. Infectious diseases reduce the productivity of farm animals, and the globalised trade of animals and their products increases the threat of disease incursion. Accurate and rapid diagnostic tests are an essential component of contingency plans to detect, control and eradicate such diseases. Diagnosis involves a 'pipeline' that normally starts with clinical suspicion, followed by collecting samples, transporting specimens to a centralised laboratory setting (e.g. national/international Reference Laboratories), analysing these samples using a range of diagnostic tests and reporting the results. However, the transport of specimens from the field to the laboratory can be a lengthy process that can delay critical decision-making and severely affect the quality of the samples. This important limitation of centralised diagnostic testing has motivated the development of tools for the rapid, simple detection of livestock pathogens. Recent advances in the development of technologies for personalised human medicine have motivated the development of prototype diagnostic tests for a wide selection of diseases of livestock. However, many of these tests are not yet routinely used or commercially available. This paper critically reviews the most promising examples of such assays, and highlights the challenges that remain to transition these tests from applied research and development into routine use.
La production durable de denrées alimentaires pour nourrir une population humaine en constante augmentation constitue un vaste enjeu planétaire ainsi que l'une des priorités définies par les Nations Unies dans le cadre des Objectifs du Millénaire pour le développement visant à « éradiquer l'extrême pauvreté et la faim dans le monde ¼. D'une part, les maladies animales réduisent la productivité des animaux d'élevage ; d'autre part, la mondialisation des échanges d'animaux et de produits d'origine animale intensifie les risques d'incursion de maladies. L'utilisation de tests de diagnostic rapides et fiables est une composante essentielle des plans d'urgence visant à détecter, contrôler et éradiquer ces maladies. Une procédure de diagnostic est généralement constituée de plusieurs opérations, depuis la suspicion clinique, la collecte d'échantillons, leur transport vers un laboratoire central (par exemple un laboratoire de référence national/international), jusqu'à l'analyse de ces échantillons au moyen d'une série de tests diagnostiques et la notification des résultats. Néanmoins, le transport des échantillons depuis le terrain jusqu'au laboratoire est parfois un processus très long qui peut retarder la prise de décisions cruciales, voire compromettre gravement la qualité des échantillons. Cette limitation importante des procédures diagnostiques centralisées a incité à mettre au point des outils permettant une détection rapide et aisée des agents pathogènes affectant le bétail. Les progrès récents accomplis dans les technologies relevant de la médecine humaine personnalisée ont encouragé le développement de prototypes d'épreuves de diagnostic pour nombre de maladies du bétail. Toutefois, plusieurs de ces tests ne sont pas encore utilisés en routine ni disponibles commercialement. Les auteurs font le point sur les exemples les plus prometteurs de ces tests et soulignent les difficultés restant à résoudre pour que ces tests puissent évoluer d'une application en recherche et développement à une utilisation en routine.
El logro de una producción sostenible de alimentos en cantidad suficiente para abastecer a una población humana cada vez más numerosa es una difícil empresa que el mundo tiene ante sí, que además entronca con una de las prioridades plasmadas en los Objetivos de Desarrollo del Milenio de las Naciones Unidas: «erradicar la pobreza extrema y el hambre¼. Las enfermedades infecciosas merman la productividad de los animales de granja, al tiempo que el comercio mundializado de animales y sus derivados amplifica la amenaza de incursiones infecciosas. La existencia de pruebas de diagnóstico rápidas y exactas es un elemento básico de todo plan de emergencia encaminado a detectar, controlar y erradicar esas enfermedades. Las labores de diagnóstico entrañan un «circuito¼ que normalmente empieza con la sospecha clínica, sigue con la obtención de muestras, su transporte a un laboratorio central (como un laboratorio de referencia nacional o internacional) y su análisis mediante diversas pruebas de diagnóstico y culmina con la notificación de los resultados. Sin embargo, el transporte hasta un laboratorio de las muestras obtenidas sobre el terreno es a veces un proceso lento, que puede retrasar la adopción de decisiones cruciales y mermar sensiblemente la calidad de las muestras. Este importante inconveniente derivado de la realización centralizada de pruebas ha llevado a concebir herramientas que permitan detectar de forma rápida y sencilla patógenos presentes en el ganado. Los avances registrados últimamente en la obtención de tecnologías destinadas a la medicina humana personalizada han propiciado también la elaboración de prototipos de pruebas para diagnosticar numerosas enfermedades del ganado, aunque muchas de ellas todavía no se utilizan sistemáticamente ni están comercializadas. Los autores, tras examinar en clave crítica los más prometedores ejemplos de estos nuevos ensayos, señalan las dificultades que aún subsisten para que estas pruebas puedan pasar del ámbito de la investigación aplicada y el desarrollo al de su utilización sistemática.
Sujet(s)
Maladies de l'animal/diagnostic , Bétail , Dépistage de masse/médecine vétérinaire , Analyse sur le lieu d'intervention , Médecine vétérinaire/méthodes , Animaux , Dosage immunologique/médecine vétérinaire , Techniques d'amplification d'acides nucléiques/médecine vétérinaire , Facteurs tempsSujet(s)
Maladies de l'animal/microbiologie , Bactéries/génétique , Génomique/méthodes , Techniques d'amplification d'acides nucléiques/méthodes , Virus/génétique , Animaux , Animaux domestiques , Animaux sauvages , Infections bactériennes/épidémiologie , Infections bactériennes/microbiologie , Infections bactériennes/médecine vétérinaire , Surveillance de la population , Maladies virales/épidémiologie , Maladies virales/médecine vétérinaire , Maladies virales/virologieRÉSUMÉ
Next-generation sequencing (NGS), also referred to as deep, high-throughput or massively parallel sequencing, is a powerful new tool that can be used for the complex diagnosis and intensive monitoring of infectious disease in veterinary medicine. NGS technologies are also being increasingly used to study the aetiology, genomics, evolution and epidemiology of infectious disease, as well as host-pathogen interactions and other aspects of infection biology. This review briefly summarises recent progress and achievements in this field by first introducing a range of novel techniques and then presenting examples of NGS applications in veterinary infection biology. Various work steps and processes for sampling and sample preparation, sequence analysis and comparative genomics, and improving the accuracy of genomic prediction are discussed, as are bioinformatics requirements. Examples of sequencing-based applications and comparative genomics in veterinary medicine are then provided. This review is based on novel references selected from the literature and on experiences of the World Organisation for Animal Health (OIE) Collaborating Centre for the Biotechnology-based Diagnosis of Infectious Diseases in Veterinary Medicine, Uppsala, Sweden.
Le séquençage de nouvelle génération (également désigné « séquençage à très haut débit ¼ ou « séquençage massivement parallèle ¼) est un nouvel outil extrêmement puissant permettant de procéder à des diagnostics sophistiqués et d'assurer un contrôle vétérinaire intensif de maladies infectieuses complexes. Les technologies du séquençage de nouvelle génération sont également d'un grand secours pour étudier l'étiologie, la génomique, l'évolution et l'épidémiologie des maladies infectieuses ainsi que les interactions hôtesagents pathogènes et bien d'autres aspects de la biologie des maladies infectieuses. Pour présenter les progrès et les accomplissements les plus récents dans ce domaine, les auteurs décrivent d'abord une série de techniques innovantes puis quelques exemples d'applications du séquençage de nouvelle génération dans le champ de la biologie des maladies animales infectieuses. Ils exposent un certain nombre d'étapes et de processus opérationnels régissant la sélection et la préparation des échantillons, l'analyse séquentielle et les études de génomique comparative, ainsi que ceux qui permettent d'améliorer la justesse prédictive de la génomique ; les exigences particulières de la bio-informatique sont également évoquées. Cette analyse est complétée par quelques exemples d'applications de l'analyse séquentielle et de la génomique comparative en médecine vétérinaire. Cette synthèse est basée sur une sélection de références bibliographiques récentes ainsi que sur l'expérience acquise par le Centre collaborateur de l'Organisation mondiale de la santé animale (OIE) pour le diagnostic basé sur la biotechnologie des maladies infectieuses en médecine vétérinaire, situé à Uppsala (Suède).
La secuenciación de próxima generación, también denominada secuenciación profunda, de alto rendimiento o masivamente paralela, es una nueva y poderosa herramienta para efectuar diagnósticos complejos y vigilar muy de cerca enfermedades infecciosas complejas en el ámbito de la medicina veterinaria. Estas técnicas también se utilizan cada vez más para estudiar la etiología, genómica, evolución y epidemiología de las enfermedades infecciosas, así como las interacciones entre patógeno y anfitrión y otros aspectos de la biología de las infecciones. Los autores resumen brevemente una serie de logros y adelantos obtenidos últimamente en este ámbito, presentando en primer lugar un conjunto de técnicas novedosas y ofreciendo después ejemplos de aplicaciones de la secuenciación de próxima generación a la biología de las infecciones veterinarias. También describen varios protocolos y procesos de trabajo para la obtención y preparación de muestras, el análisis de secuencias y las labores de genómica comparada, explican cómo mejorar la exactitud de la predicción genómica y examinan las herramientas bioinformáticas necesarias para ello. A continuación presentan ejemplos de aplicaciones basadas en técnicas de secuenciación y en la genómica comparada en medicina veterinaria. Este artículo está basado en referencias muy recientes, tomadas de publicaciones científicas, y en la experiencia del Centro Colaborador de la Organización Mundial de Sanidad Animal (OIE) para el Diagnóstico de las enfermedades infecciosas de la medicina veterinaria basado en la biotecnología, sito en Upsala (Suecia).
Sujet(s)
Maladies de l'animal/microbiologie , Génome , Génomique/méthodes , Techniques d'amplification d'acides nucléiques/méthodes , Animaux , Médecine vétérinaire/méthodesRÉSUMÉ
Newcastle disease virus (NDV), also known as virulent forms of avian paramyxovirus serotype 1 (AMPV-1), is the causative agent of Newcastle disease affecting many species of birds and causing heavy losses to the poultry industry worldwide. Early, rapid and sensitive detection of the viruses or the viral nucleic acids is very important for disease diagnosis and control. This study aimed to evaluate sample preparation under field conditions and the application of a real-time RT-PCR method in the portable T-COR4 platform for the rapid, on-site detection of NDV on a farm. In the laboratory setting, the portable real-time RT-PCR assay had a similar performance compared with that obtained with a larger, stationary Rotor Gene real-time thermocycler. In the field conditions, viral nucleic acids were manually extracted just outside of animal units with minimal equipment and real-time RT-PCR detection was performed with the portable thermocycler T-COR4 placed in a nearby room. The portable assay at the farm detected viral RNA in 15 samples and reached an agreement of 83% (39/47) when the same RNA preparations were tested in the Rotor Gene thermocycler under the laboratory setting. The results demonstrated the feasibility of performing field detection but also the need to improve and further simplify sample preparation procedures.
Sujet(s)
Maladie de Newcastle/diagnostic , Virus de la maladie de Newcastle/isolement et purification , Maladies de la volaille/diagnostic , Trousses de réactifs pour diagnostic/médecine vétérinaire , Réaction de polymérisation en chaine en temps réel/médecine vétérinaire , Animaux , Études de faisabilité , Maladie de Newcastle/virologie , Virus de la maladie de Newcastle/génétique , Techniques d'amplification d'acides nucléiques/médecine vétérinaire , Volaille , Maladies de la volaille/virologie , ARN viral/analyse , Trousses de réactifs pour diagnostic/normes , Réaction de polymérisation en chaine en temps réel/méthodes , RT-PCR/méthodes , RT-PCR/médecine vétérinaireRÉSUMÉ
Two European laboratories independently detected atypical bovine pestiviral nucleic acids in three commercial batches of foetal bovine serum (FBS) that was claimed by the producers to be of Australian origin. Additional batches of FBS were obtained directly from Australia to exclude possible contamination of the Australian FBS with that of South American origin during manufacturing/packaging in European countries. RT-PCR amplification of partial 5'untranslated region and the complete N(pro) gene yielded a specific band with expected size, which was confirmed by DNA sequencing. Bayesian analysis of sequence data demonstrated a closer phylogenetic relation of the newly detected atypical bovine pestiviruses to those of South American origin, which were related to the recognized bovine pestivirus species, bovine viral diarrhoea virus. Taken together, the results indicated the presence of atypical bovine pestiviruses in the Australian FBS, and most likely in Australian Continent.
Sujet(s)
Diarrhée virale bovine-maladie des muqueuses/diagnostic , Maladies des bovins/diagnostic , Virus de la diarrhée virale bovine/isolement et purification , Sang foetal/virologie , ARN viral/génétique , Régions 5' non traduites/génétique , Animaux , Australie , Théorème de Bayes , Diarrhée virale bovine-maladie des muqueuses/génétique , Bovins , Maladies des bovins/génétique , Maladies des bovins/virologie , Virus de la diarrhée virale bovine/classification , Virus de la diarrhée virale bovine/génétique , Génome viral , Phylogenèse , ARN messager/génétique , ARN viral/sang , Réaction de polymérisation en chaine en temps réel , RT-PCRRÉSUMÉ
PURPOSE: In Germany, reliable data about the prevalence of urogenital Chlamydia trachomatis infections, causative genotypes, as well as corresponding clinical, demographic and behavioural information are sparse. We, therefore, performed a prospective prevalence study including 1,003 sexually active volunteers of a Southern German city. METHODS: Study participants completed a standardised questionnaire and provided first void urine samples for analysis. Our screening strategy included the performance of two nucleic acid amplification tests with different target genes, enabling the detection of the new Swedish variant of C. trachomatis (nvCT). Direct genotyping of positive specimens was performed by sequence analysis of the ompA gene. RESULTS AND CONCLUSION: The overall prevalence of C. trachomatis infection was 4.2 % in women and 4.6 % in men. A relatively high prevalence of 8.3 % was found in men older than 25 years. Never using condoms was an independent risk factor for infection. The most common symptom was discharge; however, 64.5 % of infected females and all of the infected men were asymptomatic, supporting the need for screening programmes. The most frequently encountered genotypes were E (46.5 %), F (20.9 %) and K (14.0 %). Since the nvCT was detected in one female student, this is one of the rare studies that reports on the molecular identification of nvCT apart from Sweden.
Sujet(s)
Infections à Chlamydia/épidémiologie , Chlamydia trachomatis/génétique , Génotype , Adolescent , Adulte , Infections à Chlamydia/diagnostic , Chlamydia trachomatis/classification , Femelle , Techniques de génotypage/méthodes , Allemagne/épidémiologie , Humains , Mâle , Prévalence , Comportement sexuel , Enquêtes et questionnaires , Jeune adulteRÉSUMÉ
African swine fever virus (ASFV) causes one of the most dreaded transboundary animal diseases (TADs) in Suidae. African swine fever (ASF) often causes high rates of morbidity and mortality, which can reach 100% in domestic swine. To date, serological diagnosis has the drawback of not being able to differentiate variants of this virus. Previous studies have identified the 22 genotypes based on sequence variation in the C-terminal region of the p72 gene, which has become the standard for categorizing ASFVs. This article describes a genotyping assay developed using a segment of PCR-amplified genomic DNA of approximately 450 bp, which encompasses the C-terminal end of the p72 gene. Complementary paired DNA probes of 15 or 17 bp in length, which are identical except for a single nucleotide polymorphism (SNP) in the central position, were designed to either individually or in combination differentiate between the 22 genotypes. The assay was developed using xMAP technology; probes were covalently linked to microspheres, hybridized to PCR product, labelled with a reporter and read in the Luminex 200 analyzer. Characterization of the sample was performed by comparing fluorescence of the paired SNP probes, that is, the probe with higher fluorescence in a complementary pair identified the SNP that a particular sample possessed. In the final assay, a total of 52 probes were employed, 24 SNP pairs and 4 for general detection. One or more samples from each of the 22 genotypes were tested. The assay was able to detect and distinguish all 22 genotypes. This novel assay provides a powerful novel tool for the simultaneous rapid diagnosis and genotypic differentiation of ASF.
Sujet(s)
Virus de la peste porcine africaine/génétique , Peste porcine africaine/diagnostic , ADN viral/génétique , Génome viral , Séquençage par oligonucléotides en batterie/méthodes , Polymorphisme de nucléotide simple , Peste porcine africaine/virologie , Virus de la peste porcine africaine/isolement et purification , Animaux , Marqueurs biologiques/analyse , Génotype , Réaction de polymérisation en chaine en temps réel , SuidaeRÉSUMÉ
Considering the 'One Health' principles, the links between animal and human health are very strong. Both domestic and wild animals are sources of infectious agents that cause diseases in humans. Poor animal health may also indirectly affect human health, through reduced access to food. A large number of infectious diseases of animals, the transboundary animal diseases, spread rapidly across borders. Robust and accurate diagnostic assays are needed to detect the infectious agents rapidly and to limit their spread. A large arsenal of novel assays has been developed during the last three decades, with a tremendous impact on the detection of infectious agents. The new diagnostic methods are mostly laboratory-based and expensive, requiring sophisticated equipment and special skills. However, rapid and cheap field-based assays have also been developed. Herein, the authors give several examples of the development of novel assays, with special focus on the 'One Health' principles.
Sujet(s)
Maladies de l'animal/épidémiologie , Maladies transmissibles/médecine vétérinaire , Maladies d'origine alimentaire/épidémiologie , Animaux , Maladies transmissibles/épidémiologie , Maladies transmissibles/microbiologie , Maladies transmissibles/virologie , Santé mondiale , Humains , Surveillance de la populationRÉSUMÉ
Sequencing methods have improved rapidly since the first versions of the Sanger techniques, facilitating the development of very powerful tools for detecting and identifying various pathogens, such as viruses, bacteria and other microbes. The ongoing development of high-throughput sequencing (HTS; also known as next-generation sequencing) technologies has resulted in a dramatic reduction in DNA sequencing costs, making the technology more accessible to the average laboratory. In this White Paper of the World Organisation for Animal Health (OIE) Collaborating Centre for the Biotechnology-based Diagnosis of Infectious Diseases in Veterinary Medicine (Uppsala, Sweden), several approaches and examples of HTS are summarised, and their diagnostic applicability is briefly discussed. Selected future aspects of HTS are outlined, including the need for bioinformatic resources, with a focus on improving the diagnosis and control of infectious diseases in veterinary medicine.
Sujet(s)
Maladies de l'animal/microbiologie , Maladies transmissibles/diagnostic , Séquençage nucléotidique à haut débit/médecine vétérinaire , Médecine vétérinaire/économie , Médecine vétérinaire/méthodes , Maladies de l'animal/diagnostic , Maladies de l'animal/économie , Animaux , Maladies transmissibles/économie , Union européenne , Banque de gènes , Séquençage nucléotidique à haut débit/économie , Techniques de diagnostic moléculaire/économie , Techniques de diagnostic moléculaire/méthodes , Techniques de diagnostic moléculaire/médecine vétérinaireRÉSUMÉ
In this study the design and development of two real-time PCR assays for the rapid, sensitive and specific detection of infectious laryngotracheitis virus (ILTV) DNA is described. A Primer-Probe Energy Transfer (PriProET) assay and 5' conjugated Minor Groove Binder (MGB) method are compared and contrasted. Both have been designed to target the thymidine kinase gene of the ILTV genome. Both PriProET and MGB assays are capable of detecting 20 copies of a DNA standard per reaction and are linear from 2×10(8) to 2×10(2)copies/µl. Neither PriProET, nor MGB reacted with heterologous herpesviruses, indicating a high specificity of the two methods as novel tools for virus detection and identification. This study demonstrates the suitability of PriProET and 5' conjugated MGB probes as real-time PCR chemistries for the diagnosis of respiratory diseases caused by ILTV.
Sujet(s)
Amorces ADN/composition chimique , Amorces ADN/génétique , ADN viral/isolement et purification , Infections à Herpesviridae/médecine vétérinaire , Herpèsvirus aviaire de type 1/isolement et purification , Réaction de polymérisation en chaîne/méthodes , Maladies de la volaille/diagnostic , Animaux , Séquence nucléotidique , ADN viral/génétique , Infections à Herpesviridae/diagnostic , Infections à Herpesviridae/virologie , Herpèsvirus aviaire de type 1/génétique , Données de séquences moléculaires , Volaille , Maladies de la volaille/virologie , Sensibilité et spécificitéRÉSUMÉ
African swine fever virus (ASFV) is a highly pathogenic DNA virus that is the causative agent of African swine fever (ASF), an infectious disease of domestic and wild pigs of all breeds and ages, causing a range of syndromes. Acute disease is characterized by high fever, haemorrhages in the reticuloendothelial system, and a high mortality rate. A powerful novel diagnostic assay based on the Linear-After-The-Exponential-PCR (LATE-PCR) principle was developed to detect ASFV. LATE-PCR is an advanced form of asymmetric PCR which results in direct amplification of large amount of single-stranded DNA. Fluorescent readings are acquired using endpoint analysis after PCR amplification. Amplification of the correct product is verified by melting curve analysis. The assay was designed to amplify the VP72 gene of ASFV genome. Nineteen ASFV DNA cell culture virus strains and three tissue samples (spleen, tonsil, and liver) from infected experimental pigs were tested. Virus was detected in all of the cell culture and tissue samples. None of five ASFV-related viruses tested produced a positive signal, demonstrating the high specificity of the assay. The sensitivity of the LATE-PCR assay was determined in two separate real-time monoplex reactions using samples of synthetic ASFV and synthetic control-DNA targets that were diluted serially from 109 to 1 initial copies per reaction. The detection limit was 1 and 10 copies/reaction, respectively. The sensitivity of the assay was also tested in a duplex end-point reactions comprised of a constant level of 150 copies of synthetic control-DNA and a clinical sample of spleen tissue diluted serially from 10⻹ to 10â»5. The detection limit was 10â»5 dilution which corresponds to approximately 1 copy/reaction. Since the assay is designed to be used in either laboratory settings or in a portable PCR machine (Bio-Seeq Portable Veterinary Diagnostics Laboratory; Smiths Detection, Watford UK), the LATE-PCR provides a robust and novel tool for the diagnosis of ASF both in the laboratory and in the field.
Sujet(s)
Virus de la peste porcine africaine/physiologie , Peste porcine africaine/diagnostic , Élevage/méthodes , Réaction de polymérisation en chaîne , Virus de la peste porcine africaine/génétique , Animaux , ADN simple brin , ADN viral , Sensibilité et spécificité , Suidae , Protéines virales/génétiqueRÉSUMÉ
Hepatitis E infections in humans are usually acquired in endemic countries in Asia or Africa. In Sweden 17 cases infected in Europe, between 1993 and 2009, were identified. All had clinical hepatitis E with unknown source of infection. Hepatitis E virus (HEV) was identified in faecal samples from 63 piglets in 12 pig farms in Sweden. HEV was also identified in blood from 13 out of 159 investigated Swedish wild boars from nine counties. Partial HEV genomes from humans, pigs and wild boars were sequenced and compared by phylogeny. The results showed close relatedness between HEV strains from piglets from the same farm and from wild boars from the same county. HEV strains from humans showed relatedness with strains from pigs and wild boars from the same county. This study showed that HEV strains form geographical clusters in the phylogenetic tree. The methods used in this study may thus be used for tracing the origin of an infecting strain. Furthermore, this study indicated that there are endemic sources of human HEV infections in Sweden.
Sujet(s)
Virus de l'hépatite E/classification , Virus de l'hépatite E/génétique , Hépatite E/épidémiologie , Hépatite E/médecine vétérinaire , Maladies des porcs/épidémiologie , Maladies des porcs/virologie , Sujet âgé , Animaux , Sang/virologie , Analyse de regroupements , Fèces/virologie , Femelle , Génotype , Hépatite E/virologie , Virus de l'hépatite E/isolement et purification , Humains , Mâle , Adulte d'âge moyen , Épidémiologie moléculaire , Typage moléculaire , Phylogenèse , ARN viral/génétique , ARN viral/isolement et purification , Analyse de séquence d'ADN , Sus scrofa , Suède/épidémiologie , SuidaeRÉSUMÉ
A real-time RT-PCR assay based on the primer-probe energy transfer (PriProET) was developed to detect all 24 serotypes of bluetongue virus (BTV). BTV causes serious disease, primarily in sheep, but in other ruminants as well. A distinguishing characteristic of the assay is its tolerance toward mutations in the probe region. Furthermore, melting curve analysis following immediately PCR confirms specific probe hybridization and can reveal mutations in the probe region by showing a difference in the melting point. The assay sensitivity was in the range of 10-100 target copies and the specificity tests showed no positive results for heterologous pathogens. The assay was tested on clinical samples from BTV 8 outbreaks in Sweden and Denmark in 2008. The lowest detection limit for that serotype, determined with PCR standards, was 57 genome copies. The assay sensitivity for some other serotypes that circulate currently in Europe was also determined. BTV 2, 4, 9 and 16 were tested on available cell culture samples and the detection limits were 109, 12, 13 and 24 copies, respectively. This assay provides an important tool for early and rapid detection of a wide range of BTV strains, including emerging strains.
Sujet(s)
Virus de la langue bleue/classification , Virus de la langue bleue/génétique , Fièvre catarrhale du mouton/diagnostic , Amorces ADN/génétique , Sondes oligonucléotidiques/génétique , RT-PCR/méthodes , Animaux , Fièvre catarrhale du mouton/virologie , Virus de la langue bleue/isolement et purification , Amorces ADN/composition chimique , Danemark/épidémiologie , Épidémies de maladies , Transfert d'énergie , Génotype , Mutation , Sondes oligonucléotidiques/composition chimique , Sensibilité et spécificité , Ovis , Suède/épidémiologie , Température de transitionRÉSUMÉ
In 2004, an atypical pestivirus named D32/00_'HoBi', isolated from foetal calf serum (FCS) originating from Brazil, was described (Schirrmeier et al., 2004). A few years later, a closely related virus (Th/04_KhonKaen) was detected in serum from a calf in Thailand, indicating that this group of atypical pestiviruses already is spread in cattle populations in various regions of the world. At the Friedrich-Loeffler-Institute, Insel Riems, Germany, FCS batches are regularly tested for pestivirus contamination, in general with positive PCR results, and in some cases the contaminants have been typed as 'HoBi'-like. At the National Veterinary Institute (SVA) in Uppsala, Sweden, a recent event with contaminated FCS ruined much of the ongoing cell culture work. From the FCS and the contaminated cells we were able to amplify and sequence nucleic acid from three different pestivirus strains, including BVDV-1, -2 and 'HoBi'-like; this in a commercial FCS that had been tested free from pestivirus by the manufacturer. In this short communication we review the current status of atypical 'HoBi'-like pestiviruses, describe recent findings and discuss the implications thereof.
Sujet(s)
Variation génétique , Pestivirus/génétique , Animaux , Techniques de culture cellulaire , Milieux de culture , Pestivirus/classification , Pestivirus/isolement et purification , PhylogenèseRÉSUMÉ
Avian influenza has become a serious concern from both veterinary and public health points of view. National and international organisations, veterinary health authorities, research institutions, diagnostic laboratories and field services make enormous efforts worldwide to detect, combat and prevent this important disease. Accordingly, the standard diagnostic protocols are being supported by a wide variety of molecular detection techniques, including improved polymerase chain reaction assays, microarray-based detection and characterisation methods, very rapid sequencing, simple pen-side tests and other on-site approaches. These recently developed 'closer to the field' methods allow rapid detection of influenza viruses and the identification of pathogenicity variants. However, in order to harmonise the diagnosis worldwide, attention has to be paid to the validation and standardisation of these technologies, to avoid erroneous interpretation of assay results, and, consequently, inappropriate epidemiological measures. This review gives an overview of the current and potential future developments related to avian influenza diagnostics.
Sujet(s)
Virus de la grippe A/isolement et purification , Grippe chez les oiseaux/diagnostic , Animaux , Oiseaux , Diagnostic différentiel , Virus de la grippe A/génétique , Virus de la grippe A/pathogénicité , Nanotechnologie , Maladie de Newcastle/diagnostic , Séquençage par oligonucléotides en batterie/méthodes , Séquençage par oligonucléotides en batterie/médecine vétérinaire , Systèmes automatisés lit malade , Réaction de polymérisation en chaîne/méthodes , Réaction de polymérisation en chaîne/médecine vétérinaire , RT-PCR/tendances , RT-PCR/médecine vétérinaireRÉSUMÉ
A real-time reverse-transcription PCR was developed to detect and pathotype Newcastle disease viruses (NDV) in clinical samples. Degenerate oligonucleotide primers and TaqMan probes with nonfluorescent minor groove binder (MGB) quencher amplified and hybridized to a region in the fusion protein (F) gene that corresponds to the cleavage site of the F0 precursor, which is a key determinant of NDV pathogenicity. The application of degenerate primers and TaqMan MGB probes provided high specificity to the assay, as was shown by the successful and rapid pathotype determination of 39 NDV strains representing all the known genotypes (I to VIII) and pathotypes (lentogens/mesogens/velogens). The PCR assays specific for lentogenic and velogenic/mesogenic strains had high analytical sensitivity, detecting approximately 10 and 20 copies of the target molecule per reaction, respectively. The detection limit was also determined in terms of 50% egg infective dose (EID(50)) by using dilution series of virus stock solutions to be approximately 10(1.0) and 10(-1.3) EID(50)/ml for lentogens and velogens/mesogens, respectively. Organ, swab, and stool specimens from experimentally infected animals were tested to prove the clinical suitability of the method. The results of this study suggest that the described real-time PCR assay has the potential to be used for the rapid detection/pathotyping of NDV isolates and qualitative/quantitative measurement of the virus load.
Sujet(s)
Amorces ADN/génétique , Maladie de Newcastle/virologie , Virus de la maladie de Newcastle/classification , Virus de la maladie de Newcastle/génétique , RT-PCR/méthodes , Structures anatomiques de l'animal/virologie , Animaux , Poulets , Fèces/virologie , Données de séquences moléculaires , ARN viral/génétique , Sensibilité et spécificité , Analyse de séquence d'ADN , Protéines de fusion viraleRÉSUMÉ
Highly conserved nucleotide stretches flanking the cleavage site of the haemagglutinin (HA) gene of influenza type A viruses were utilised for generating PCR amplicons from a broad range of avian influenza viruses (AIV) in a one-step real-time SYBR Green RT-PCR assay. The nucleotide sequencing of the amplified PCR products simultaneously reveals both the HA subtype and the pathotype of the AIV isolates, as we demonstrated in case of H5 subtype viruses. The specificity of the assay was confirmed by investigating 66 strains of AIV and nine heterologous pathogens, including influenza B, C and various avian pathogenic viruses. This assay enables a general HA subtype identification and pathotype determination of AIV isolates providing a useful alternative tool for avian influenza diagnosis.
Sujet(s)
Oiseaux/virologie , Glycoprotéine hémagglutinine du virus influenza/génétique , Virus de la grippe A/génétique , Grippe chez les oiseaux/diagnostic , Animaux , Virus de la grippe A/classification , Virus de la grippe A/isolement et purification , Grippe chez les oiseaux/virologie , ARN viral/génétique , RT-PCR/méthodes , Sensibilité et spécificité , Analyse de séquence d'ADNRÉSUMÉ
Nine viral diseases included in the World Organization for Animal Health list of notifiable diseases (former list A) were chosen for their contagiousness and high capacity of spreading to improve their diagnosis using new and emerging technologies. All the selected diseases--foot-and-mouth disease, swine vesicular disease, vesicular stomatitis, classical swine fever, African swine fever, bluetongue, African horse sickness, Newcastle disease and highly pathogenic avian influenza--are considered as transboundary diseases, which detection causes the prohibition of livestock exportation, and, thus, it leads to high economical losses. The applied diagnostic techniques can fall into two categories: (i) nucleic-acid detection, including padlock probes, real-time PCR with TaqMan, minor groove binding probes and fluorescence energy transfer reaction probes, isothermal amplification like the Cleavase/Invader assay or the loop-mediated amplification technology and the development of rapid kits for 'mobile' PCR and (ii) antigen-antibody detection systems like simplified and more sensitive ELISA tests. Besides, internal controls have been improved for nucleic acid-detecting methods by using an RNA plant virus--Cowpea Mosaic Virus--to ensure the stability of the RNA used as a positive control in diagnostic real-time RT-PCR assays. The development of these diagnosis techniques has required the joint efforts of a European consortium in which nine diagnostic laboratories and an SME who have collaborated since 2004 within the European Union-funded Lab-on-site project. The results obtained are shown in this paper.
Sujet(s)
Techniques de laboratoire clinique/médecine vétérinaire , Maladies transmissibles/médecine vétérinaire , Notification des maladies , Maladies virales/médecine vétérinaire , Animaux , Techniques de laboratoire clinique/normes , Maladies transmissibles/diagnostic , Test ELISA/méthodes , Test ELISA/normes , Test ELISA/médecine vétérinaire , Réaction de polymérisation en chaîne/méthodes , Réaction de polymérisation en chaîne/normes , Réaction de polymérisation en chaîne/médecine vétérinaire , Sensibilité et spécificité , Maladies virales/diagnosticRÉSUMÉ
The highly contagious transboundary animal diseases (TADs), e.g., foot-and-mouth disease (FMD), classical swine fever (CSF), African swine fever (ASF) and highly pathogenic avian influenza (HPAI) are regularly occurring and re-occurring on various continents, causing severe losses. This epidemiological situation indicates the urgent need for the development of powerful, robust and high capacity new diagnostic methods in order to detect and identify the causative agents very rapidly. This report is on the experiences of an OIE Collaborating Centre and those of the MULTIPLEX-PCR and the LAB-ON-SITE EU project consortia with the deveopment of novel methods for the improved molecular diagnosis of a range of viral diseases. Thermal amplification based real-time PCR methods (e.g.,TaqMan, Molecular Beacons, Primer-Probe Energy Transfer, and Light Upon eXtension (LUX) fluorogenic primers), and amplification without thermocycling have been elaborated for the improved diagnosis of TADs, such as FMD, swine vesicular disease, vesicular stomatitis, CSF, ASF, HPAI and Newcastle disease (ND). The simultaneous detection of various pathogens in a disease complex is facilitated by the development of multiplex PCR packages. By introducing nucleic acid extraction and pipetting robotics, together with the multi-channel real-time PCR machines, the molecular diagnostic procedures have become rapid, robust and automated. Quality control is strengthened by special precautions to avoid false positive and false negative results. By following the steps of OIE standardisation and validation, the diagnostic PCR assays have become nationally and nternationally standardised and harmonised. The development of additional methods, like padlock probes and microarrays, is further improving the arsenal of nucleic acid based novel molec ular diagnostic tests for TADs.