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9. Antigenic and Genetic Evolution of Equine Influenza A (H3N8) Virus from 1968 to 2007

Author

Lewis, N. S., primary, Daly, J. M., additional, Russell, C. A., additional, Horton, D. L., additional, Skepner, E., additional, Bryant, N. A., additional, Burke, D. F., additional, Rash, A. S., additional, Wood, J. L. N., additional, Chambers, T. M., additional, Fouchier, R. A. M., additional, Mumford, J. A., additional, Elton, D. M., additional, and Smith, D. J., additional

Published
2011
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10. A new modified live equine influenza virus vaccine: phenotypic stability, restricted spread and efficacy against heterologous virus challenge

Author

CHAMBERS, T. M., primary, HOLLAND, R. E., additional, TUDOR, L. R., additional, TOWNSEND, H. G. G., additional, COOK, A., additional, BOGDAN, J., additional, LUNN, D. P., additional, HUSSEY, S., additional, WHITAKER-DOWLING, P., additional, YOUNGNER, J. S., additional, SEBRING, R. W., additional, PENNER, S. J., additional, and STIEGLER, G. L., additional

Published
2010
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18. Intracellular localization of the viral polymerase proteins in cells infected with influenza virus and cells expressing PB1 protein from cloned cDNA

Author

Akkina, R K, Chambers, T M, Londo, D R, and Nayak, D P

Abstract

The biosynthesis, nuclear transport, and formation of a complex among the influenza polymerase proteins were studied in influenza virus-infected MDBK cells by using monospecific antisera. To obtain these monospecific antisera, portions of cloned cDNAs encoding the individual polymerase proteins (PB1, PB2, or PA) of A/WSN/33 influenza virus were expressed as fusion proteins in Escherichia coli, and the purified fusion proteins were injected into rabbits. Studies using indirect immunofluorescence showed that early in the infectious cycle (4 h postinfection) of influenza virus, PB1 and PB2 are present mainly in the nucleus, whereas PA is predominantly present in the cytoplasm of the virus-infected cells. Later, at 6 to 8 h postinfection, all three polymerase proteins are apparent both in the cytoplasm as well as the nucleus. Radiolabeling and immunoprecipitation analyses showed that the three polymerase proteins remain physically associated as a complex in either the presence or the absence of ribonucleoproteins. In the cytoplasm, the majority of the polymerase proteins remain unassociated, whereas in the nucleus they are present as a complex of three polymerase proteins. To determine whether a polymerase protein is transported into the nucleus individually, PB1 was expressed from the cloned cDNA by using the simian virus 40 late promoter expression vector. PB1 alone, in the absence of the other polymerase proteins or the nucleoprotein, accumulates in the nucleus. This suggests that the formation of a complex with other viral protein(s) is not required for either nuclear transport or nuclear accumulation of PB1 protein and that the PB1 protein may contain an intrinsic signal(s) for nuclear transport.

Published
1987
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19. Expression of defective-interfering influenza virus-specific transcripts and polypeptides in infected cells

Author

Akkina, R K, Chambers, T M, and Nayak, D P

Abstract

We have previously shown that influenza virus defective-interfering particle (DI) RNAs can be transcribed into polyadenylated complementary RNAs in vitro (Chanda et al., J. Virol. 45:55-61, 1983). In this paper we report that influenza virus DI RNAs can be transcribed into mRNAs in infected cells as well. The DI-specific RNAs (both plus and minus strands) were found to be synthesized in molar excess compared with RNAs of standard virus segments. In addition, two DI preparations (DI3 and DI7) produced novel polypeptides not present in standard virus-infected cells. These novel polypeptides in DI-infected cells were of PB2 origin, as were the major DI RNA species in both DI preparations. Furthermore, these polypeptides were shown to arise from the translation of functional mRNAs transcribed from DI3 and DI7 RNAs and not from either the degradation of PB2 protein or the incomplete translation of PB2 mRNA. Using mixed-infection tests with different DI preparations, we found that the ability of DI to produce detectable novel polypeptides does not necessarily confer any replicative or interfering advantage over other DI which do not produce detectable DI-specific polypeptides. The possible role of DI-specific polypeptides in DI-mediated interference is discussed.

Published
1984
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20. Effect of human alpha A interferon on influenza virus replication in MDBK cells

Author

Ransohoff, R M, Maroney, P A, Nayak, D P, Chambers, T M, and Nilsen, T W

Abstract

To determine the molecular mechanism whereby interferon induces resistance to influenza virus, we began an investigation of influenza virus replication in MDBK cells treated with recombinant human alpha A interferon. Negative- and positive-strand virus-specific RNA accumulation was monitored by blot hybridization with cloned probes. Primary transcription (transcription of infecting viral negative strands by the virion-associated polymerase) was inhibited by interferon treatment of MDBK cells. At moderate levels of interferon treatment (10 U/ml), this inhibition was restricted to transcripts of polymerase genes, whereas at higher levels of interferon treatment (50 U/ml), accumulation of all primary transcripts was markedly inhibited. Secondary transcripts and viral negative strands did not accumulate to any significant extent in interferon-treated MDBK cells. These results suggest that interferon-induced mechanisms which inhibit influenza virus replication in MDBK cells act at the level of primary transcription.

Published
1985
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21. Defective interfering virus associated with A/Chicken/Pennsylvania/83 influenza virus

Author

Chambers, T M and Webster, R G

Abstract

The A/Chicken/Pennsylvania/1/83 influenza virus, isolated from a respiratory infection of chickens, is an avirulent H5N2 virus containing subgenomic RNAs (W.J. Bean, Y. Kawaoka, J.M. Wood, J.E. Pearson, and R.G. Webster, J. Virol. 54:151-160, 1985). We show here that defective interfering particles are present in this virus population. The virus had a low ratio of plaque-forming to hemagglutinating units and produced interference with standard virus multiplication in infectious center reduction assays. Subgenomic RNAs were identified as internally deleted polymerase RNAs. We have confirmed that this virus protects chickens from lethal H5N2 influenza virus infection. This protective effect appeared to be due to the inhibition of virulent virus multiplication. Additionally, subgenomic RNAs derived from polymerase RNAs were detected in 5 of 18 RNA preparations from animal influenza virus isolates. Therefore, defective interfering particles are sometimes produced in natural influenza virus infections, not just under laboratory conditions. These particles may be capable of suppressing the pathogenic effect of virulent virus infections in nature.

Published
1987
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22. In vitro transcription of defective interfering particles of influenza virus produces polyadenylic acid-containing complementary RNAs

Author

Chanda, P K, Chambers, T M, and Nayak, D P

Abstract

Influenza virus defective interfering (DI) RNAs, which originate from polymerase genes by simple internal deletion, can be transcribed in vitro. These DI RNA transcripts contain covalently linked polyadenylic acid, and their synthesis is dependent on ApG or capped RNAs as primers. Furthermore, like the standard viral RNA transcripts, they are complementary in nature and are slightly smaller in size compared with the corresponding DI RNAs. Hybridization of the specific DI RNA transcripts with the corresponding DI RNA segments and analysis of the duplex RNA by gel electrophoresis indicate that they are not incomplete polymerase gene transcripts, but rather the transcripts of the DI RNAs. Since influenza virus DI RNAs contain both the 5' and the 3' termini and transcribe polyadenylic acid-containing complementary RNAs in vitro the mechanism of interference may differ from that of the 5' DI RNAs of Sendai and vesicular stomatitis viruses.

Published
1983
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23. Interaction between anthelmintic treatment and vaccine responses in ponies naturally infected with cyathostomins.

Author

Nielsen MK, Rubinson EF, Chambers TM, Horohov DW, Wagner B, Betancourt A, Reedy SE, and Jacobsen S

Subjects
Animals, Cytokines analysis, Female, Horses, Immunoglobulin G blood, Male, Strongyle Infections, Equine immunology, Vaccination, Anthelmintics therapeutic use, Strongyle Infections, Equine drug therapy, Vaccines immunology
Abstract

Anthelmintics and vaccines are commonly given concurrently in routine equine management, but it is unknown to what extent an interaction between the two exists. Cyathostomins can modulate the local immune response by stimulating a type 2 helper T cell (Th2) response. In addition, anti-inflammatory effects of ivermectin have been found in rodent models. It is unknown whether these anti-inflammatory effects affect the acute phase response elicited by commonly used vaccines. This study evaluated how the acute phase inflammatory response, leukocyte expression of pro-inflammatory cytokines, and vaccine-specific titers induced by simultaneous injection of three vaccines (West Nile Virus, Equine Herpes Rhinopneumonitis, and Keyhole Limpet Hemocyanin) were modulated by concurrent administration of ivermectin or pyrantel pamoate in ponies naturally infected with cyathostomins. Mixed-breed yearling ponies were blocked by gender and fecal strongyle egg count, then randomly assigned to three treatment groups: ivermectin (n=8), pyrantel pamoate (n=8), and control (n=7). All ponies received vaccinations intramuscularly on days 0 and 29, and anthelmintics were administered on the same days. Whole blood, serum and plasma samples were collected one, three and 14 days after each vaccination. Samples were analyzed for concentrations of acute phase reactants (haptoglobin, serum amyloid A, fibrinogen and iron), mRNA expression levels of cytokines (interleukin (IL)-1β, IL-4, IL-10, tumor necrosis factor (TNF)-α and interferon (IFN)-γ) in leukocytes, and vaccine-specific antibody titers. A marked acute-phase response was noted following both vaccinations. In contrast, the pattern of change in cytokine expression was less pronounced and more variable. Statistical differences were observed between groups for haptoglobin, fibrinogen, IL-1β, IL-4, and IL-10, but differences were generally small and none of the vaccine titers were different between the groups. Taken together, the study found some signs of modulation of immunologic or inflammatory responses to the administered vaccines, when anthelmintics were administered concurrently, but these are unlikely to have practical implications for vaccination routines., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published
2015
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24. Characterization of the in situ immunological responses to vaccine adjuvants.

Author

Horohov DW, Dunham J, Liu C, Betancourt A, Stewart JC, Page AE, and Chambers TM

Subjects
Animals, Cytokines genetics, Female, Gene Expression, Horse Diseases immunology, Horse Diseases prevention & control, Influenza A virus immunology, Lymphocyte Activation, Male, Orthomyxoviridae Infections immunology, Orthomyxoviridae Infections prevention & control, Orthomyxoviridae Infections veterinary, RNA, Messenger genetics, RNA, Messenger metabolism, Th1 Cells immunology, Th2 Cells immunology, Vaccines, Inactivated administration & dosage, Adjuvants, Immunologic administration & dosage, Horses immunology, Influenza Vaccines administration & dosage
Abstract

Adjuvants are included with many inactivated and some modified live vaccines to enhance immune responses to specific antigens. While early vaccines relied exclusively upon aluminum salts, still the major adjuvant used in human vaccines, other adjuvant products are used in veterinary medicine. In addition to enhancing antigen presentation, adjuvants can also enhance the development of specific immune responses. Thus, alum adjuvants often preferentially stimulate humoral immune responses. By contrast, lipid-based adjuvants are often more effective at stimulating cell-mediated immune responses. Metastim(®) is a lipid-based adjuvant reported to elicit both humoral and cellular immune responses, though the mechanism responsible for this activity remains unclear. In this study, we compared the ability of equine influenza virus vaccines containing either saline or Metastim(®) or an aluminum phosphate adjuvant to stimulate antigen presenting cell function in vivo. Six ponies were intradermally inoculated with inactivated equine influenza (KY97) mixed with either adjuvant or saline. Multiple sites were injected so that biopsies could be collected at different times post injection. The 4mm punch biopsies were formalin-fixed, paraffin-embedded, and stained with hematoxylin and eosin (H&E). Total RNA was isolated from 2mm punch biopsies for the determination of gene expression by real-time PCR. H&E staining revealed a variety of cells recruited to the injection sites, including lymphocytes, neutrophils, eosinophils and macrophages. Real-time PCR analysis of the injection site confirmed this cellular infiltration and identified increased expression of activation markers. Both vaccines also stimulated gene expressions of pro-inflammatory cytokines. The vaccine containing Metastim(®) elicited significantly higher gene expression of interferon-γ, IL-12, CD4 and CD83 compared to alum (p<0.05). While the greater induction of IFNγ-related gene expression indicates that Metastim(®) can elicit Th-1 immune responses more effectively than the aluminum salt, there was also evidence of Th2 cytokine induction., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published
2015
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25. Immunosenescence of the equine immune system.

Author

Horohov DW, Adams AA, and Chambers TM

Subjects
Age Factors, Animals, Immunity, Cellular immunology, Influenza A virus immunology, Aging immunology, Horses immunology, Influenza Vaccines immunology, Vaccination veterinary
Abstract

It is widely recognized that advanced age is associated with alterations in immunological responses that likely contribute to increased morbidity and mortality in the elderly population. This decreased efficacy of the immune system with age is referred to as 'immunosenescence' and has been reported for a number of species. Similar age-related changes are seen in horses and are manifested as decreased responsiveness to vaccination in vivo and diminished proliferative responses to mitogens in vitro. The underlying mechanism responsible for these impaired immunological responses remains unknown. This paper reviews some of our recent findings on immunosenescence in horses. Recent results on the immune response of aged horses to vaccination with a novel recombinant influenza vaccine are also discussed., (Copyright 2009 Elsevier Ltd. All rights reserved.)

Published
2010
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26. A new modified live equine influenza virus vaccine: phenotypic stability, restricted spread and efficacy against heterologous virus challenge.

Author

Chambers TM, Holland RE, Tudor LR, Townsend HG, Cook A, Bogdan J, Lunn DP, Hussey S, Whitaker-Dowling P, Youngner JS, Sebring RW, Penner SJ, and Stiegler GL

Subjects
Administration, Intranasal, Animals, Female, Horse Diseases transmission, Horses, Influenza Vaccines administration & dosage, Influenza Vaccines immunology, Male, Nebulizers and Vaporizers veterinary, Orthomyxoviridae Infections prevention & control, Orthomyxoviridae Infections transmission, Phenotype, Safety, Serial Passage, Time Factors, Treatment Outcome, Vaccination veterinary, Vaccines, Attenuated administration & dosage, Vaccines, Attenuated immunology, Vaccines, Attenuated standards, Virus Shedding, Horse Diseases prevention & control, Influenza A virus immunology, Influenza Vaccines standards, Orthomyxoviridae Infections veterinary
Abstract

Flu Avert IN vaccine is a new, live attenuated virus vaccine for equine influenza. We tested this vaccine in vivo to ascertain 1) its safety and stability when subjected to serial horse to horse passage, 2) whether it spread spontaneously from horse to horse and 3) its ability to protect against heterologous equine influenza challenge viruses of epidemiological relevance. For the stability study, the vaccine was administered to 5 ponies. Nasal swabs were collected and pooled fluids administered directly to 4 successive groups of naïve ponies by intranasal inoculation. Viruses isolated from the last group retained the vaccine's full attenuation phenotype, with no reversion to the wild-type virus phenotype or production of clinical influenza disease. The vaccine virus spread spontaneously to only 1 of 13 nonvaccinated horses/ponies when these were comingled with 39 vaccinates in the same field. For the heterologous protection study, a challenge model system was utilised in which vaccinated or naïve control horses and ponies were exposed to the challenge virus by inhalation of virus-containing aerosols. Challenge viruses included influenza A/equine-2/Kentucky/98, a recent representative of the 'American' lineage of equine-2 influenza viruses; and A/equine-2/Saskatoon/90, representative of the 'Eurasian' lineage. Clinical signs among challenged animals were recorded daily using a standardised scoring protocol. With both challenge viruses, control animals reliably contracted clinical signs of influenza, whereas vaccinated animals were reliably protected from clinical disease. These results demonstrate that Flu Avert IN vaccine is safe and phenotypically stable, has low spontaneous transmissibility and is effective in protecting horses against challenge viruses representative of those in circulation worldwide.

Published
2001
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27. The involvement of a stress-activated pathway in equine influenza virus-mediated apoptosis.

Author

Lin C, Zimmer SG, Lu Z, Holland RE Jr, Dong Q, and Chambers TM

Subjects
Animals, Carbazoles pharmacology, Carvedilol, Cell Line, Cytopathogenic Effect, Viral, DNA Fragmentation, Dogs, Enzyme Activation, In Situ Nick-End Labeling, Mitogen-Activated Protein Kinase 8, Oligodeoxyribonucleotides, Antisense pharmacology, Oxidative Stress, Propanolamines pharmacology, Signal Transduction, Transforming Growth Factor beta biosynthesis, Virus Replication drug effects, Apoptosis, Influenza A virus, Mitogen-Activated Protein Kinases metabolism, Orthomyxoviridae Infections enzymology
Abstract

We have shown elsewhere that equine-2 influenza virus (EIV; subtype H3N8) induced pronounced cell death in infected cells through apoptosis as demonstrated by DNA fragmentation assay and a combined TUNEL and immunostaining scheme. In this study, we investigated the mechanism of EIV-mediated cytotoxicity on a permissive mammalian epithelial cell line, Madin-Darby canine kidney (MDCK) cells. EIV infection increased the cellular levels of oxidative stress and c-Jun/AP-1 protein (which is known to be affected by oxidative stress), as well as its DNA binding activity. Increased production of TGF-beta1, an inducer of c-Jun N-terminal kinase or stress-activated protein kinase (JNK/SAPK) activation, was also detected in EIV-infected MDCK cells. It has been reported that TGF-beta may initiate a signaling cascade leading to JNK/SAPK activation. Addition of c-Jun antisense oligodeoxynucleotide, antioxidant N-acetyl-cysteine (NAC), JNK/SAPK inhibitor carvedilol, or TGF-beta-neutralizing antibody effectively blocked c-Jun/AP-1 upregulation and TGF-beta1 production mediated by EIV infection. These treatments also attenuated EIV-induced cytopathogenic effects (CPE) and apoptosis. Our results suggest that a stress-activated pathway is involved in apoptosis mediated by EIV infection. It is likely that EIV infection turns on the JNK/SAPK cascade, which modulates the activity of apoptosis-promoting regulatory factor c-Jun/AP-1 and epithelial growth inhibitory cytokine TGF-beta., (Copyright 2001 Academic Press.)

Published
2001
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28. Derivation and characterization of a live attenuated equine influenza vaccine virus.

Author

Youngner JS, Whitaker-Dowling P, Chambers TM, Rushlow KE, and Sebring R

Subjects
Animals, Antibodies, Viral blood, Cells, Cultured, Chick Embryo, Cold Temperature, Dogs, Electrophoresis, Polyacrylamide Gel veterinary, Hemagglutination Inhibition Tests, Horses, Orthomyxoviridae Infections immunology, Orthomyxoviridae Infections virology, Random Allocation, Vaccination veterinary, Vaccines, Attenuated immunology, Vaccines, Attenuated standards, Viral Plaque Assay veterinary, Viral Proteins analysis, Horse Diseases immunology, Horse Diseases virology, Influenza A virus immunology, Influenza Vaccines immunology, Orthomyxoviridae Infections veterinary
Abstract

Objective: To develop and characterize a cold-adapted live attenuated equine-2 influenza virus effective as an intranasal vaccine., Animals: 8 ponies approximately 18 months of age., Procedures: A wild-type equine-2 virus, A/Equine/Kentucky/1/91 (H3N8), was serially passaged in embryonated chicken eggs at temperatures gradually reduced in a stepwise manner from 34 C to 30 C to 28 C to 26 C. At different passages, infected allantoic fluids were tested for the ability of progeny virus to replicate in Madin-Darby canine kidney (MDCK) cells at 34 C and 39.5 C. Virus clones that replicated at 26 C in eggs and at 34 C in MDCK cells, but not at 39.5 C in MDCK cells, were tested for stability of the cold-adapted, temperature-sensitive (ts), and protein synthesis phenotypes. A stable clone, P821, was evaluated for safety, ability to replicate, and immunogenicity after intranasal administration in ponies., Results: Randomly selected clones from the 49th passage were all ts with plaquing efficiencies of < 10(-6) (ratio of 39.5 C:34 C) and retained this phenotype after 5 serial passages at 34 C in either embryonated eggs or MDCK cells. The clone selected as the vaccine candidate (P821) had the desired degree of attenuation. Administered intranasally to seronegative ponies, the virus caused no adverse reactions or overt signs of clinical disease, replicated in the upper portion of the respiratory tract, and induced a strong serum antibody response., Conclusion and Clinical Relevance: A candidate live attenuated influenza vaccine virus was derived by cold-adaptation of a wild-type equine-2 influenza virus, A/Equine/Kentucky/1/91, in embryonated eggs.

Published
2001
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29. Safety, efficacy, and immunogenicity of a modified-live equine influenza virus vaccine in ponies after induction of exercise-induced immunosuppression.

Author

Lunn DP, Hussey S, Sebing R, Rushlow KE, Radecki SV, Whitaker-Dowling P, Youngner JS, Chambers TM, Holland RE Jr, and Horohov DW

Subjects
Administration, Intranasal, Animals, Antibodies, Viral biosynthesis, Hemagglutination Inhibition Tests veterinary, Horse Diseases prevention & control, Horses, Immunoglobulin A biosynthesis, Immunoglobulin G biosynthesis, Immunosuppression Therapy veterinary, Influenza Vaccines immunology, Lymphocyte Activation immunology, Nebulizers and Vaporizers veterinary, Orthomyxoviridae Infections immunology, Orthomyxoviridae Infections prevention & control, Prospective Studies, Safety, Time Factors, Treatment Outcome, Vaccination veterinary, Vaccines, Attenuated immunology, Vaccines, Attenuated standards, Virus Shedding, Horse Diseases immunology, Immune Tolerance immunology, Influenza A virus immunology, Influenza Vaccines standards, Orthomyxoviridae Infections veterinary, Physical Exertion physiology
Abstract

Objective: To determine safety, efficacy, and immunogenicity of an intranasal cold-adapted modified-live equine influenza virus vaccine administered to ponies following induction of exercise-induced immunosuppression., Design: Prospective study., Animals: Fifteen 9- to 15-month old ponies that had not had influenza., Procedure: Five ponies were vaccinated after 5 days of strenuous exercise on a high-speed treadmill, 5 were vaccinated without undergoing exercise, and 5 were not vaccinated or exercised and served as controls. Three months later, all ponies were challenged by nebulization of homologous equine influenza virus. Clinical and hematologic responses and viral shedding were monitored, and serum and nasal secretions were collected for determination of influenza-virus-specific antibody isotype responses., Results: Exercise caused immunosuppression, as indicated by depression of lymphocyte proliferation in response to pokeweed mitogen. Vaccination did not result in adverse clinical effects, and none of the vaccinated ponies developed clinical signs of infection following challenge exposure. In contrast, challenge exposure caused marked clinical signs of respiratory tract disease in 4 control ponies. Vaccinated and control ponies shed virus after challenge exposure. Antibody responses to vaccination were restricted to serum IgGa and IgGb responses in both vaccination groups. After challenge exposure, ponies in all groups generated serum IgGa and IgGb and nasal IgA responses. Patterns of serum hemagglutination inhibition titers were similar to patterns of IgGa and IgGb responses., Conclusions and Clinical Relevance: Results suggested that administration of this MLV vaccine to ponies with exercise-induced immunosuppression was safe and that administration of a single dose to ponies provided clinical protection 3 months later.

Published
2001
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30. Sialic acid species as a determinant of the host range of influenza A viruses.

Author

Suzuki Y, Ito T, Suzuki T, Holland RE Jr, Chambers TM, Kiso M, Ishida H, and Kawaoka Y

Subjects
Animals, Humans, Species Specificity, Virus Replication, Influenza A virus physiology, Influenza, Human metabolism, Influenza, Human virology, N-Acetylneuraminic Acid metabolism
Abstract

The distribution of sialic acid (SA) species varies among animal species, but the biological role of this variation is largely unknown. Influenza viruses differ in their ability to recognize SA-galactose (Gal) linkages, depending on the animal hosts from which they are isolated. For example, human viruses preferentially recognize SA linked to Gal by the alpha2,6(SAalpha2,6Gal) linkage, while equine viruses favor SAalpha2,3Gal. However, whether a difference in relative abundance of specific SA species (N-acetylneuraminic acid [NeuAc] and N-glycolylneuraminic acid [NeuGc]) among different animals affects the replicative potential of influenza viruses is uncertain. We therefore examined the requirement for the hemagglutinin (HA) for support of viral replication in horses, using viruses whose HAs differ in receptor specificity. A virus with an HA recognizing NeuAcalpha2,6Gal but not NeuAcalpha2,3Gal or NeuGcalpha2,3Gal failed to replicate in horses, while one with an HA recognizing the NeuGcalpha2,3Gal moiety replicated in horses. Furthermore, biochemical and immunohistochemical analyses and a lectin-binding assay demonstrated the abundance of the NeuGcalpha2,3Gal moiety in epithelial cells of horse trachea, indicating that recognition of this moiety is critical for viral replication in horses. Thus, these results provide evidence of a biological effect of different SA species in different animals.

Published
2000
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31. Comparison of the phenotypes of Streptococcus zooepidemicus isolated from tonsils of healthy horses and specimens obtained from foals and donkeys with pneumonia.

Author

Anzai T, Walker JA, Blair MB, Chambers TM, and Timoney JF

Subjects
Animals, DNA Primers, Genes, Bacterial, Phagocytosis, Phenotype, Pneumonia, Bacterial microbiology, Polymerase Chain Reaction, Reference Values, Streptococcal Infections microbiology, Streptococcus equi classification, Streptococcus equi isolation & purification, Equidae microbiology, Horse Diseases microbiology, Horses microbiology, Palatine Tonsil microbiology, Pneumonia, Bacterial veterinary, Streptococcal Infections veterinary, Streptococcus equi genetics
Abstract

Objective: To determine whether streptococcal pneumonia is caused by strains of Streptococcus zooepidemicus similar to those obtained from the tonsils of healthy horses., Sample Population: 5 tonsils from healthy horses, 8 tracheal washes and 6 lung specimens from foals with pneumonia, and 5 nasopharyngeal swab specimens from donkeys with acute bronchopneumonia., Procedure: Variable M-like protectively immunogenic SzP proteins of 5 isolates of S. zooepidemicus from each tonsil and clinical specimen were compared, using immunoblots. The SzP gene of 13 isolates representative of various SzP immunoblot phenotypes from 1 healthy horse and 9 horses and donkeys with pneumonia were sequenced and compared. Cell-associated hyaluronic acid concentration and resistance to phagocytosis of some isolates were measured., Results: Tonsils of each healthy horse were colonized by several SzP phenotypes similar to those of foals or donkeys with pneumonia. In contrast, multiple isolates from animals with pneumonia had the same SzP phenotype, indicating infection by a single strain or clone. Analysis of the SzP sequence confirmed that differences in immunoblot phenotype were associated with sequence differences and that several SzP genotypes were in healthy horses and animals with pneumonia. Isolates with high concentrations of cell-associated hyaluronic acid were more resistant to phagocytosis., Conclusions and Clinical Relevance: An SzP-specific immunoblot is a useful, sensitive measure of diversity among strains of S. zooepidemicus. Single strains with SzP phenotypes similar to those found in tonsils of healthy horses cause pneumonia. Because of the diversity of SzP phenotype and genotype among isolates from animals with pneumonia, SzP phenotype is not an important determinant of invasiveness or epizootic capabilities.

Published
2000
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32. Pharmacokinetics and therapeutic efficacy of rimantadine in horses experimentally infected with influenza virus A2.

Author

Rees WA, Harkins JD, Lu M, Holland RE Jr, Lehner AF, Tobin T, and Chambers TM

Subjects
Administration, Oral, Animals, Antibodies, Viral blood, Antiviral Agents administration & dosage, Antiviral Agents blood, Antiviral Agents standards, Area Under Curve, Biological Availability, Chick Embryo, Female, Gas Chromatography-Mass Spectrometry veterinary, Hemagglutination Inhibition Tests veterinary, Horse Diseases virology, Horses, Injections, Intravenous veterinary, Microbial Sensitivity Tests, Nasal Mucosa virology, Orthomyxoviridae Infections drug therapy, Rimantadine administration & dosage, Rimantadine blood, Rimantadine standards, Antiviral Agents pharmacokinetics, Horse Diseases drug therapy, Orthomyxoviridae drug effects, Orthomyxoviridae Infections veterinary, Rimantadine pharmacokinetics
Abstract

Objective: To determine pharmacokinetics of single and multiple doses of rimantadine hydrochloride in horses and to evaluate prophylactic efficacy of rimantadine in influenza virus-infected horses., Animals: 5 clinically normal horses and 8 horses seronegative to influenza A., Procedure: Horses were given rimantadine (7 mg/kg of body weight, i.v., once; 15 mg/kg, p.o., once; 30 mg/kg, p.o., once; and 30 mg/kg, p.o., q 12 h for 4 days) to determine disposition kinetics. Efficacy in induced infections was determined in horses seronegative to influenza virus A2. Rimantadine was administered (30 mg/kg, p.o., q 12 h for 7 days) beginning 12 hours before challenge-exposure to the virus., Results: Estimated mean peak plasma concentration of rimantadine after i.v. administration was 2.0 micrograms/ml, volume of distribution (mean +/- SD) at steady-state (Vdss) was 7.1 +/- 1.7 L/kg, plasma clearance after i.v. administration was 51 +/- 7 ml/min/kg, and beta-phase half-life was 2.0 +/- 0.4 hours. Oral administration of 15 mg of rimantadine/kg yielded peak plasma concentrations of < 50 ng/ml after 3 hours; a single oral administration of 30 mg/kg yielded mean peak plasma concentrations of 500 ng/ml with mean bioavailability (F) of 25%, beta-phase half-life of 2.2 +/- 0.3 hours, and clearance of 340 +/- 255 ml/min/kg. Multiple doses of rimantadine provided steady-state concentrations in plasma with peak and trough concentrations (mean +/- SEM) of 811 +/- 97 and 161 +/- 12 ng/ml, respectively. Rimantadine used prophylactically for induced influenza virus A2 infection was associated with significant decreases in rectal temperature and lung sounds., Conclusions and Clinical Relevance: Oral administration of rimantadine to horses can safely ameliorate clinical signs of influenza virus infection.

Published
1999

33. Rapid protocol for sequencing RNA virus using delta Taq version 2.0 DNA polymerase.

Author

Lai AC and Chambers TM

Subjects
Base Sequence, Hemagglutinins genetics, Influenza A virus genetics, Molecular Sequence Data, Polymerase Chain Reaction, Ribonucleases antagonists & inhibitors, Taq Polymerase, DNA-Directed DNA Polymerase, Orthomyxoviridae genetics, RNA, Viral chemistry, Sequence Analysis, RNA methods
Published
1995

34. Genetic and antigenic analysis of the influenza virus responsible for the 1992 Hong Kong equine influenza epizootic.

Author

Lai AC, Lin YP, Powell DG, Shortridge KF, Webster RG, Daly J, and Chambers TM

Subjects
Amino Acid Sequence, Animals, Genotype, Hemagglutinin Glycoproteins, Influenza Virus, Hemagglutinins, Viral chemistry, Hemagglutinins, Viral genetics, Hong Kong epidemiology, Horse Diseases virology, Horses, Humans, Influenza A virus immunology, Influenza, Human virology, Molecular Sequence Data, Time Factors, Antigens, Viral analysis, Disease Outbreaks, Horse Diseases epidemiology, Influenza A virus genetics, Influenza, Human veterinary
Abstract

An outbreak of influenza occurred among thoroughbred racehorses in Hong Kong in November-December 1992, with morbidity of 37%. All horses involved had been vaccinated against equine-1 and equine-2 influenza viruses but not against the virus responsible for the 1989 equine influenza outbreak in northern China (influenza A/equine/Jilin/89, subtype H3N8). Therefore the source and nature of the virus causing the Hong Kong outbreak was investigated. Virus isolated from a horse infected during the outbreak was used for genetic analysis. All the viral gene segments were similar to those of equine-2 (H3N8) influenza viruses and unrelated to those of equine/Jilin/89 virus. The nucleotide sequence of the viral hemagglutinin gene showed high homology (99.4%) to that of influenza A/equine/Suffolk/89 (H3N8) virus which has circulated extensively in Europe. However, these viruses differed in their antigenic reactivity to a panel of monoclonal antibodies. Preliminary epizootiological information plus the concordance of amino acid sequence between hemagglutinins of the Hong Kong isolate and a contemporaneous equine-2 influenza virus isolate from the United Kingdom indicated that the probable source of the Hong Kong outbreak was horses recently imported from England or Ireland.

Published
1994
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35. Rapid diagnosis of equine influenza by the Directigen FLU-A enzyme immunoassay.

Author

Chambers TM, Shortridge KF, Li PH, Powell DG, and Watkins KL

Subjects
Animals, Antigens, Viral analysis, Horse Diseases virology, Horses, Immunoenzyme Techniques veterinary, Influenza A virus immunology, Nasal Lavage Fluid microbiology, Orthomyxoviridae Infections diagnosis, Orthomyxoviridae Infections virology, Sensitivity and Specificity, Time Factors, Virology methods, Horse Diseases diagnosis, Influenza A virus isolation & purification, Orthomyxoviridae Infections veterinary
Abstract

The Directigen FLU-A enzyme immunoassay was tested for its ability to detect equine-2 influenza viruses in nasopharyngeal fluids from horses and ponies. A total of 125 swabs from experimental infections and from different sources of natural infection in the USA and Hong Kong were examined. The assay results were compared with the results of standard virus culture in embryonated chicken eggs or Madin-Darby canine kidney cells, and with the serology of the horses sampled. In comparison with virus culture the enzyme immunoassay exhibited 83 per cent sensitivity, 78 per cent specificity, 70 per cent positive predictive value and 88 per cent negative predictive value. The test appeared to be more sensitive than haemagglutination for the detection of low levels of virus in embryonated egg cultures. It also detected equine-1 influenza virus in culture. The test is rapid (15 minutes), simple, and should be a convenient method for the rapid diagnosis and screening of horses for equine influenza infection.

Published
1994
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36. Diagnosis of equine influenza by the polymerase chain reaction.

Author

Donofrio JC, Coonrod JD, and Chambers TM

Subjects
Animals, Base Sequence, Body Temperature, Chick Embryo, DNA Primers, Hemagglutination Tests methods, Horses, Influenza A virus genetics, Molecular Sequence Data, Oligonucleotide Probes, Orthomyxoviridae Infections diagnosis, RNA, Viral isolation & purification, Horse Diseases, Influenza A virus isolation & purification, Orthomyxoviridae Infections veterinary, Polymerase Chain Reaction methods
Abstract

Influenza A is a common respiratory infection of horses, and rapid diagnosis is important for its detection and control. Sensitive detection of influenza currently requires viral culture and is not always feasible. The polymerase chain reaction (PCR) was used to detect DNA produced by reverse transcription of equine influenza in stored nasal secretions, vaccines, and allantoic fluids. Primers directed at a target of 212 bp on conserved segment 7 (matrix gene) of human influenza A/Bangkok/1/79(H3N2) produced amplification products of appropriate size with influenza A/Equine/Prague/1/56 (H7N7), A/Equine/Miami/63 (H3N8), A/Equine/Kentucky/79 (H3N8), and A/Equine/Kentucky/2/91 (H3N8) in infected frozen allantoic fluids and in frozen extracts of nasal swabs of 2 horses with naturally acquired influenza. The products bound a 32P-labeled hybridization probe to an inner region of the target. Control samples, including nasal secretions from a horse infected with herpesvirus, were negative. In a prospective study, 2 ponies inhaled aerosols of influenza A/Equine/Kentucky/2/91 (H3N8), and thereafter supernatants of nasal swabs in transport medium were obtained daily for 10 days for culture and PCR. Amplification products were evaluated by size and binding of a 32P-labeled probe and also by dot-blotting and binding of a biotin-labeled probe. Culture detected influenza more consistently than did PCR in the first 2 days of infection, but PCR detected virus more often later in infection. Gels were the most sensitive, but radiometric and biotin-labeled probes gave specific results and were consistently positive from days 3-6. PCR is suitable for detection of equine influenza in clinical samples.

Published
1994
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37. Cross-reactivity of existing equine influenza vaccines with a new strain of equine influenza virus from China.

Author

Chambers TM

Subjects
Animals, Antibodies, Viral blood, China, Cross Reactions, Hemagglutination Inhibition Tests, Horses, Immune Sera immunology, Neutralization Tests, Orthomyxoviridae Infections prevention & control, Horse Diseases prevention & control, Influenza A virus immunology, Orthomyxoviridae Infections veterinary, Vaccination veterinary, Viral Vaccines immunology
Abstract

A novel strain of equine influenza virus, influenza A/equine/Jilin (China)/1/89, has emerged which is genetically distinct from all earlier strains of equine influenza. It is therefore possible that the vaccines against equine influenza may be unable to protect horses against disease caused by this virus strain. In vitro serological assays established that there were low levels of immunological cross-reactivity between the new virus, the current vaccine strains and the strains of equine-2 influenza virus now in circulation.

Published
1992
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38. Protection of chickens from lethal influenza virus infection by influenza A/chicken/Pennsylvania/1/83 virus: characterization of the protective effect.

Author

Chambers TM and Webster RG

Subjects
Animals, Chickens, Disease Outbreaks, Influenza A virus growth & development, Orthomyxoviridae Infections epidemiology, Propiolactone pharmacology, United States epidemiology, Virulence, Virus Activation, Influenza A virus pathogenicity, Orthomyxoviridae Infections prevention & control, Viral Vaccines therapeutic use
Abstract

The influenza A/chicken/Pennsylvania/1/83 (H5N2) virus is the first known example of an influenza virus isolated from a natural infection which contained primarily defective interfering particles (T. M. Chambers and R. G. Webster, J. Virol. 61, 1517-1523, 1987). In chickens, coinoculation of this virus together with the closely related but highly virulent influenza A/chicken/Pennsylvania/1370/83 virus results in reduced mortality compared to virulent virus infection alone (Bean et al., J. Virol. 54, 151-160, 1985). The biological basis of this protective effect has not been established. Protective activity required greater than or equal to 100-fold excess input of protecting virus over virulent virus, functioned effectively during the first generations of virulent virus multiplication, and also functioned against an antigenically heterologous (H7N7) virulent influenza virus. Protection was correlated with the complete inhibition of virulent virus spread to the brain of infected chickens. Plaque-purified chicken/Pennsylvania/1/83 virus depleted of defective interfering particles, and beta-propiolactone-inactivated virus, had no protective effect. These characteristics are consistent with the hypothesis that protection was the result of defective interfering particle-mediated interference with virulent virus multiplication within the respiratory tract of the chicken.

Published
1991
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39. Molecular characterization of a new hemagglutinin, subtype H14, of influenza A virus.

Author

Kawaoka Y, Yamnikova S, Chambers TM, Lvov DK, and Webster RG

Subjects
Amino Acid Sequence, Animals, Antigens, Viral analysis, Base Sequence, Chickens microbiology, Ducks microbiology, Ferrets microbiology, Hemagglutinins, Viral genetics, Influenza A virus genetics, Molecular Sequence Data, Phylogeny, RNA, Messenger genetics, Sequence Homology, Nucleic Acid, Virus Replication, Hemagglutinins, Viral immunology, Influenza A virus immunology
Abstract

Two influenza A viruses whose hemagglutinin (HA) did not react with any of the reference antisera for the 13 recognized HA subtypes were isolated from mallard ducks in the USSR. Antigenic analysis by hemagglutination inhibition and double immunodiffusion tests showed that the HAs of these viruses are similar to each other but distinct from the HAs of other influenza A viruses. Nucleotide sequence analysis showed that these HA genes differ from each other by only 21 nucleotides. However, they differ from all other HA subtypes at the amino acid level by at least 31% in HAI. Thus, we propose that the HAs of these viruses [A/Mallard/Gurjev/263/82 (H14N5) and A/Mallard/Gurjev/244/82 (H14N6) belong to a previously unrecognized subtype, and are designated H14. Unlike any other HAs of influenza viruses, the H14 HAs contained lysine at the cleavage site between HA1 and HA2 instead of arginine. Experimental infection of domestic poultry and ferrets with A/Mallard/Gurjev/263/82 (H14N5) showed that the virus is avirulent for these animals. Based on comparative sequence analysis of different HA genes, it is suggested that differences of 30% or more at the amino acid level in HA1 constitute separate subtypes. Phylogenetic analysis of representatives of each HA subtype showed that H14 is one of the most recently diverged lineages while H8 and H12 branched off early during the evolution of the HA subtypes. These latter two subtypes (H8 and H12) have been isolated very infrequently in recent years, suggesting that these old subtypes may be disappearing from the influenza reservoirs in nature.

Published
1990
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40. Conditional expression of foreign genes by temperature-sensitive mutants of vaccinia virus.

Author

Chambers TM, Essani K, and Webster RG

Subjects
DNA, Viral biosynthesis, Kinetics, Phenotype, Promoter Regions, Genetic, Temperature, DNA, Recombinant genetics, Gene Expression Regulation, Genetic Vectors, Mutation, Vaccinia virus genetics
Abstract

To assess the utility of two temperature-sensitive (ts) mutant vaccinia viruses as vectors for the conditional in vitro expression of recombinant foreign genes, we have studied the kinetics of expression of foreign genes incorporated into these viruses. At nonpermissive temperature, 40 degrees C, these viruses were defective either in DNA synthesis or in virus assembly. Foreign gene expression was affected by the nature of the ts lesion and by the nature of the vaccinia promoter positioned upstream from the foreign gene. With both vector viruses, a foreign gene controlled by the p7.5 early-late promoter was expressed at both 33 degrees and 40 degrees C. With the DNA synthesis-defective vector virus, foreign gene expression controlled by the p11 DNA synthesis-dependent late promoter was inhibited at 40 degrees C, but could be turned on by shift to 33 degrees C. This ts expression system provides an alternative to use of drugs that inhibit DNA synthesis as a means for experimental manipulation of gene expression. Both vector viruses can be used with existing vaccinia virus expression technology.

Published
1990
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41. Is the gene pool of influenza viruses in shorebirds and gulls different from that in wild ducks?

Author

Kawaoka Y, Chambers TM, Sladen WL, and Webster RG

Subjects
Animals, Animals, Wild microbiology, Influenza A virus classification, Influenza A virus isolation & purification, Influenza in Birds transmission, Species Specificity, Birds microbiology, Ducks microbiology, Genes, Viral, Influenza A virus genetics, Influenza in Birds microbiology
Abstract

Evidence is presented for a second major gene pool of influenza A viruses in nature. Shorebirds and gulls harbor influenza viruses when sampled in the spring and fall. Approximately half of the viruses isolated have the potential to infect ducks but the remainder do not. The hemagglutinin subtypes that are prevalent in wild ducks were rare or absent in shorebirds and gulls.

Published
1988
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42. Protection of chickens from lethal influenza infection by vaccinia-expressed hemagglutinin.

Author

Chambers TM, Kawaoka Y, and Webster RG

Subjects
Animals, Antibodies, Viral biosynthesis, B-Lymphocytes immunology, Chickens, Orthomyxoviridae Infections prevention & control, Vaccination, Vaccinia virus, Hemagglutinins, Viral immunology, Influenza A virus immunology, Orthomyxoviridae Infections veterinary, Poultry Diseases prevention & control, Vaccines immunology, Vaccines, Synthetic immunology
Abstract

To study the immune response of the chicken to specific influenza proteins, we have constructed a recombinant vaccinia virus containing the hemagglutinin gene of influenza A/Turkey/Ireland/1378/83 (H5N8). In mammalian cell culture the hemagglutinin expressed by this recombinant virus was full-length, cleaved into HA1 and HA2 in the absence of trypsin, and transported to the cell surface, confirming that other virus products are not required for cleavage activation. Chickens inoculated through the wing web with the live recombinant virus produced extremely low levels of hemagglutination-inhibiting or infectivity-neutralizing antibody. However, they were protected from lethal H5 influenza virus challenge. Protection extended to the antigenically distinct virulent H5 viruses, Chicken/Pennsylvania/1370/83 and Chicken/Scotland/59. Chemically bursectomized vaccinated chickens were not protected, whereas normal chickens with very low antibody levels (less than 10) obtained by passive transfer were protected in a dose-dependent fashion. This indicates that despite the low antibody titers induced by vaccination, protection was mediated by antibody.

Published
1988

43. Effect of ozonation on the mutagenicity of carcinogens in aqueous solution.

Author

Burleson GR and Chambers TM

Subjects
Alkylating Agents toxicity, Amines toxicity, Hydrazines toxicity, Nitroso Compounds toxicity, Water Pollutants, Chemical toxicity, Carcinogens, Mutagens toxicity, Ozone pharmacology
Abstract

Ozone is a very strong oxidizing agent that may be used in water purification. The effect of ozonation on the mutagenicity of mutagens and/or carcinogens of diverse chemical structures was evaluated as measured by the Salmonella/microsome assay. The effect of ozonation of 36 mutagens and/or carcinogens has been evaluated and the results of 15 reported here. The mutagenicity of polycyclic aromatic hydrocarbons and aromatic amines was inactivated by ozone treatment, while alkylating agents, nitro aromatics, and nitroso compounds were not affected. Ozonation of hydrazines produced mutagenic intermediates that may be susceptible to base-catalyzed hydrolysis. Therefore, depending on the chemical present, ozonation may be useful in the treatment of waters containing organic carcinogens, including drinking water, waste-water effluents, and other aqueous waste materials containing carcinogens.

Published
1982
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44. Antigenic and molecular characterization of subtype H13 hemagglutinin of influenza virus.

Author

Chambers TM, Yamnikova S, Kawaoka Y, Lvov DK, and Webster RG

Subjects
Amino Acid Sequence, Base Sequence, Genes, Viral, Hemagglutinins, Viral classification, Hemagglutinins, Viral genetics, Influenza A virus classification, Influenza A virus genetics, Molecular Sequence Data, RNA, Viral genetics, Hemagglutinins, Viral immunology, Influenza A virus immunology
Abstract

Influenza A viruses with subtype H13 hemagglutinin display an unusual host range. Although common in shorebirds, they are very rare or absent in wild ducks; additionally, H13 viruses have been isolated from a whale. To study the molecular basis for this host range, we have determined the complete nucleotide sequences of the hemagglutinin genes of three H13 influenza viruses from different species or geographical areas: A/gull/Maryland/77, A/gull/Astrachan (USSR)/84, and A/pilot whale/Maine/84. Based on the deduced amino acid sequences, H13 hemagglutinin shares the basic structure of other type A hemagglutinin subtypes such as H3, but has clearly diverged from other completely sequenced subtypes. Unique features of H13 hemagglutinin include the occurrence, near the receptor binding pocket, of residues Arg/Lys-227 and Trp-229 (H3 numbering); the significance of these are unknown. The sequence of the HA1-HA2 cleavage site resembles those of avirulent avian influenza viruses. The whale H13 hemagglutinin is similar to those from gulls, supporting the hypothesis that influenza viruses from avian sources can enter marine mammal populations but are probably not permanently maintained there. Antigenic analysis using a panel of monoclonal antibodies suggests that, like other subtypes, H13 viruses are heterogeneous, with different antigenic variants predominating in the eastern versus the western hemispheres.

Published
1989
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45. pH-sensitive mutagenic activity in ozone-treated 1,2-dimethylhydrazine in the Salmonella/microsome assay.

Author

Chambers TM and Burleson GR

Subjects
1,2-Dimethylhydrazine, Animals, Hydrogen-Ion Concentration, Mutagenicity Tests, Oxygen pharmacology, Rats, Carcinogens pharmacology, Dimethylhydrazines pharmacology, Methylhydrazines pharmacology, Mutagens pharmacology, Ozone pharmacology, Salmonella typhimurium drug effects
Abstract

Treatment with ozone inactivates the mutagenicity of many carcinogens in aqueous solution. The colon carcinogen, 1,2-dimethylhydrazine (DMH) has been reported an exception; ozone treatment converts dimethylhydrazine from a non-mutagen into a mutagen. In the Salmonella/microsome assay, the mutagenicity of ozone-treated dimethylhydrazine was dependent on pH. The ozonation product was a strong mutagen in acidic solution but was not mutagenic in basic solution. The mutagenicity of the acidic ozonation product was inactivated by raising the pH of the solution. Unlike untreated dimethylhydrazine, its ozonation product in basic solution was not converted to a mutagen in this ozone-low pH system.

Published
1982
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