RÉSUMÉ
BACKGROUND: First carpometacarpal (CMC) joint osteoarthritis (OA) is commonly encountered in clinical practice. The preferred surgical option when conservative therapy fails varies with the stage and nature of the disease. Denervation of the first CMC joint is a relatively new procedure for managing stable thumb CMC joint OA. Our objective was to review our experience and surgical technique with first CMC joint denervation surgery. METHODS: All patients who underwent first CMC joint denervation surgery from January 2015 through September 2017 were retrospectively identified. Before undergoing surgical CMC denervation, patients received a joint block at the first CMC joint with 0.25% bupivacaine. Only patients with a good response to injection were selected for surgical denervation. Patient demographics, preoperative and postoperative pain scores using a numeric rating scale, and grip strength using the Jamar Hydraulic Hand Dynamometer were analyzed. RESULTS: Of 10 patients (13 hands) with CMC joint OA, 8 patients (11 hands) met the inclusion criteria. Patients' average grip strength improved significantly after the procedure (from 38.4 ± 26.7 foot/lb to 50.2 ± 27.6 foot/lb; P = 0.007). The numeric rating scale pain score improved significantly from 7.8 ± 2.4 to 2.4 ± 1.8 (P < 0.001). Seven of 8 patients reported satisfaction with surgery. There were 2 complications. CONCLUSIONS: First CMC joint denervation provided good pain relief and improvement in grip strength in patients with thumb CMC joint OA. This minimally invasive technique proved to be a good option for providing optimal pain control and improvement in strength with minimal and mild complications.
Sujet(s)
Articulations carpométacarpiennes/chirurgie , Dénervation/méthodes , Arthrose/chirurgie , Sujet âgé , Anticoagulants/usage thérapeutique , Articulations carpométacarpiennes/innervation , Douleur chronique/prévention et contrôle , Femelle , Force de la main , Humains , Mâle , Adulte d'âge moyen , Douleur musculosquelettique/prévention et contrôle , Arthrose/physiopathologie , Mesure de la douleur , Douleur postopératoire/étiologie , Douleur postopératoire/physiopathologie , Études rétrospectives , Os trapézoïde/chirurgie , Résultat thérapeutiqueRÉSUMÉ
Bats are implicated as the natural reservoirs for several highly pathogenic viruses that can infect other animal species, including man. Here, we investigate the potential for two recently discovered bat rubulaviruses, Achimota virus 1 (AchPV1) and Achimota virus 2 (AchPV2), isolated from urine collected under urban bat (Eidolon helvum) roosts in Ghana, West Africa, to infect small laboratory animals. AchPV1 and AchPV2 are classified in the family Paramyxoviridae and cluster with other bat derived zoonotic rubulaviruses (i.e. Sosuga, Menangle and Tioman viruses). To assess the susceptibility of AchPV1 and AchPV2 in animals, infection studies were conducted in ferrets, guinea pigs and mice. Seroconversion, immunohistological evidence of infection, and viral shedding were identified in ferrets and guinea pigs, but not in mice. Infection was associated with respiratory disease in ferrets. Viral genome was detected in a range of tissues from ferrets and guinea pigs, however virus isolation was only achieved from ferret tissues. The results from this study indicate Achimota viruses (AchPVs) are able to cross the species barrier. Consequently, vigilance for infection with and disease caused by these viruses in people and domesticated animals is warranted in sub-Saharan Africa and the Arabian Peninsula where the reservoir hosts are present.
Sujet(s)
Chiroptera/virologie , Infections à Paramyxoviridae/médecine vétérinaire , Paramyxoviridae/physiologie , Animaux , Anticorps antiviraux/sang , Antigènes viraux/métabolisme , Bronches/anatomopathologie , Cellules épithéliales/anatomopathologie , Cellules épithéliales/virologie , Femelle , Furets/sang , Furets/virologie , Cochons d'Inde/sang , Cochons d'Inde/virologie , Mâle , Souris de lignée BALB C , Tests de neutralisation , Paramyxoviridae/isolement et purification , Infections à Paramyxoviridae/sang , Infections à Paramyxoviridae/virologie , ARN viral/isolement et purification , Facteurs temps , Virémie/sang , Virémie/virologie , Excrétion virale/physiologieRÉSUMÉ
AIM: Current therapies against avian influenza (H5N1) provide limited clinical benefit. FBF-001 is a highly purified equine polyclonal immunoglobulin fragment against H5N1. METHODS: Using a ferret model of severe acute H5N1 infection, we assessed FBF-001 when administered on the same day or 1 day after viral challenge, in comparison with oseltamivir therapy. RESULTS: Untreated animals died 2-3 days after challenge. FBF-001 prevented most severe illness and reduced nasal viral load, with best efficacy when administered on the day of viral challenge. Oseltamivir and FBF-001 had synergistic impact on survival. CONCLUSION: FBF-001 prevented severe consequences of lethal H5N1 challenge in ferrets by controlling viral replication, an effect synergistic to oseltamivir. FBF-001 has recently been granted EMA orphan drug status.
Sujet(s)
Anticorps antiviraux/usage thérapeutique , Antiviraux/usage thérapeutique , Immunisation passive/méthodes , Fragments Fab d'immunoglobuline/usage thérapeutique , Sous-type H5N1 du virus de la grippe A/physiologie , Infections à Orthomyxoviridae/thérapie , Oséltamivir/usage thérapeutique , Animaux , Modèles animaux de maladie humaine , Synergie des médicaments , Association de médicaments , Furets , Equus caballus , Médicament orphelin , Infections à Orthomyxoviridae/immunologie , Charge viraleRÉSUMÉ
Person-to-person transmission is a key feature of human Nipah virus outbreaks in Bangladesh. In contrast, in an outbreak of Nipah virus in Malaysia, people acquired infections from pigs. It is not known whether this important epidemiological difference is driven primarily by differences between NiV Bangladesh (NiV-BD) and Malaysia (NiV-MY) at a virus level, or by environmental or host factors. In a time course study, ferrets were oronasally exposed to equivalent doses of NiV-BD or NiV-MY. More rapid onset of productive infection and higher levels of virus replication in respiratory tract tissues were seen for NiV-BD compared to NiV-MY, corroborating our previous report of increased oral shedding of NiV-BD in ferrets and suggesting a contributory mechanism for increased NiV-BD transmission between people compared to NiV-MY. However, we recognize that transmission occurs within a social and environmental framework that may have an important and differentiating role in NiV transmission rates. With this in mind, ferret-to-ferret transmission of NiV-BD and NiV-MY was assessed under differing viral exposure conditions. Transmission was not identified for either virus when naïve ferrets were cohoused with experimentally-infected animals. In contrast, all naïve ferrets developed acute infection following assisted and direct exposure to oronasal fluid from animals that were shedding either NiV-BD or NiV-MY. Our findings for ferrets indicate that, although NiV-BD may be shed at higher levels than NiV-MY, transmission risk may be equivalently low under exposure conditions provided by cohabitation alone. In contrast, active transfer of infected bodily fluids consistently results in transmission, regardless of the virus strain. These observations suggest that the risk of NiV transmission is underpinned by social and environmental factors, and will have practical implications for managing transmission risk during outbreaks of human disease.
Sujet(s)
Infections à hénipavirus/transmission , Virus Nipah/physiologie , Animaux , Antigènes viraux/isolement et purification , Bangladesh , Chlorocebus aethiops , Modèles animaux de maladie humaine , Furets , Infections à hénipavirus/virologie , Humains , Poumon/anatomopathologie , Poumon/virologie , Malaisie , Virus Nipah/classification , ARN viral/analyse , ARN viral/sang , Répartition aléatoire , Infections de l'appareil respiratoire/virologie , Cellules Vero , Charge virale , Réplication virale , Excrétion viraleRÉSUMÉ
West Nile virus (WNV; family Flaviviridae; genus Flavivirus) group members are an important cause of viral meningoencephalitis in some areas of the world. They exhibit marked variation in pathogenicity, with some viral lineages (such as those from North America) causing high prevalence of severe neurological disease, whilst others (such as Australian Kunjin virus) rarely cause disease. The aim of this study was to characterize WNV disease in a mouse model and to elucidate the pathogenetic features that distinguish disease variation. Tenfold dilutions of five WNV strains (New York 1999, MRM16 and three horse isolates of WNV-Kunjin: Boort and two isolates from the 2011 Australian outbreak) were inoculated into mice by the intraperitoneal route. All isolates induced meningoencephalitis in different proportions of infected mice. WNVNY99 was the most pathogenic, the three horse isolates were of intermediate pathogenicity and WNVKUNV-MRM16 was the least, causing mostly asymptomatic disease with seroconversion. Infectivity, but not pathogenicity, was related to challenge dose. Using cluster analysis of the recorded clinical signs, histopathological lesions and antigen distribution scores, the cases could be classified into groups corresponding to disease severity. Metrics that were important in determining pathotype included neurological signs (paralysis and seizures), meningoencephalitis, brain antigen scores and replication in extra-neural tissues. Whereas all mice infected with WNVNY99 had extra-neural antigen, those infected with the WNV-Kunjin viruses only occasionally had antigen outside the nervous system. We conclude that the mouse model could be a useful tool for the assessment of pathotype for WNVs.
Sujet(s)
Fièvre à virus West Nile/virologie , Virus du Nil occidental/pathogénicité , Animaux , Antigènes viraux/métabolisme , Système nerveux central/virologie , Modèles animaux de maladie humaine , Femelle , Maladies des chevaux/anatomopathologie , Maladies des chevaux/virologie , Equus caballus/virologie , Humains , Mâle , Souris , Spécificité d'organe , Spécificité d'espèce , Protéines virales non structurales/immunologie , Protéines virales non structurales/métabolisme , Virulence , Réplication virale , Fièvre à virus West Nile/anatomopathologie , Fièvre à virus West Nile/médecine vétérinaire , Virus du Nil occidental/immunologie , Virus du Nil occidental/physiologieRÉSUMÉ
In recent years, the emergence of several highly pathogenic zoonotic diseases in humans has led to a renewed emphasis on the interconnectedness of human, animal, and environmental health, otherwise known as One Health. For example, Hendra virus (HeV), a zoonotic paramyxovirus, was discovered in 1994, and since then, infections have occurred in 7 humans, each of whom had a strong epidemiologic link to similarly affected horses. As a consequence of these outbreaks, eradication of bat populations was discussed, despite their crucial environmental roles in pollination and reduction of the insect population. We describe the development and evaluation of a vaccine for horses with the potential for breaking the chain of HeV transmission from bats to horses to humans, thereby protecting horse, human, and environmental health. The HeV vaccine for horses is a key example of a One Health approach to the control of human disease.
Sujet(s)
Santé environnementale , Virus Hendra/immunologie , Infections à hénipavirus/prévention et contrôle , Maladies des chevaux/prévention et contrôle , Vaccins antiviraux/immunologie , Zoonoses/prévention et contrôle , Animaux , Anticorps antiviraux/sang , Anticorps antiviraux/immunologie , Femelle , Furets , Cochons d'Inde , Virus Hendra/génétique , Maladies des chevaux/anatomopathologie , Maladies des chevaux/virologie , Equus caballus , Humains , Immunisation , Tests de neutralisation , Zoonoses/anatomopathologie , Zoonoses/virologieRÉSUMÉ
BACKGROUND: Hendra virus (HeV) is an Australian bat-borne zoonotic paramyxovirus that repeatedly spills-over to horses causing fatal disease. Human cases have all been associated with close contact with infected horses. METHODS: A full-length antigenome clone of HeV was assembled, a reporter gene (GFP or luciferase) inserted between the P and M genes and transfected to 293T cells to generate infectious reporter gene-encoding recombinant viruses. These viruses were then assessed in vitro for expression of the reporter genes. The GFP expressing recombinant HeV was used to challenge ferrets to assess the virulence and tissue distribution by monitoring GFP expression in infected cells. RESULTS: Three recombinant HeV constructs were successfully cloned and rescued; a wild-type virus, a GFP-expressing virus and a firefly luciferase-expressing virus. In vitro characterisation demonstrated expression of the reporter genes, with levels proportional to the initial inoculum levels. Challenge of ferrets with the GFP virus demonstrated maintenance of the fatal phenotype with disease progressing to death consistent with that observed previously with the parental wild-type isolate of HeV. GFP expression could be observed in infected tissues collected from animals at euthanasia. CONCLUSIONS: Here, we report on the first successful rescue of recombinant HeV, including wild-type virus and viruses expressing two different reporter genes encoded as an additional gene cassette inserted between the P and M genes. We further demonstrate that the GFP virus retained the ability to cause fatal disease in a well-characterized ferret model of henipavirus infection despite the genome being an extra 1290 nucleotides in length.