Your search keyword '"Alvin W. Smith"' showing total 63 results

1. Identification of Human Junctional Adhesion Molecule 1 as a Functional Receptor for the Hom-1 Calicivirus on Human Cells

Author

Stanislav V. Sosnovtsev, Carlos Sandoval-Jaime, Gabriel I. Parra, Christine M. Tin, Ronald W. Jones, Jo Soden, Donna Barnes, Jim Freeth, Alvin W. Smith, and Kim Y. Green

Subjects

Microbiology, QR1-502

Abstract

ABSTRACT The Hom-1 vesivirus was reported in 1998 following the inadvertent transmission of the animal calicivirus San Miguel sea lion virus to a human host in a laboratory. We characterized the Hom-1 strain and investigated the mechanism by which human cells could be infected. An expression library of 3,559 human plasma membrane proteins was screened for reactivity with Hom-1 virus-like particles, and a single interacting protein, human junctional adhesion molecule 1 (hJAM1), was identified. Transient expression of hJAM1 conferred susceptibility to Hom-1 infection on nonpermissive Chinese hamster ovary (CHO) cells. Virus infection was markedly inhibited when CHO cells stably expressing hJAM were pretreated with anti-hJAM1 monoclonal antibodies. Cell lines of human origin were tested for growth of Hom-1, and efficient replication was observed in HepG2, HuH7, and SK-CO15 cells. The three cell lines (of hepatic or intestinal origin) were confirmed to express hJAM1 on their surface, and clustered regularly interspaced short palindromic repeats/Cas9-mediated knockout of the hJAM1 gene in each line abolished Hom-1 propagation. Taken together, our data indicate that entry of the Hom-1 vesivirus into these permissive human cell lines is mediated by the plasma membrane protein hJAM1 as a functional receptor. IMPORTANCE Vesiviruses, such as San Miguel sea lion virus and feline calicivirus, are typically associated with infection in animal hosts. Following the accidental infection of a laboratory worker with San Miguel sea lion virus, a related virus was isolated in cell culture and named Hom-1. In this study, we found that Hom-1 could be propagated in a number of human cell lines, making it the first calicivirus to replicate efficiently in cultured human cells. Screening of a library of human cell surface membrane proteins showed that the virus could utilize human junctional adhesion molecule 1 as a receptor to enter cells and initiate replication. The Hom-1 virus presents a new system for the study of calicivirus biology and species specificity.

Published

2017

2. Calicivirus Emergence from Ocean Reservoirs: Zoonotic and Interspecies Movements

Author

Alvin W. Smith, Douglas E. Skilling, Neil Cherry, Jay H. Mead, and David O. Matson

Subjects

United States, Medicine, Infectious and parasitic diseases, RC109-216

Abstract

Caliciviral infections in humans, among the most common causes of viral-induced vomiting and diarrhea, are caused by the Norwalk group of small round structured viruses, the Sapporo caliciviruses, and the hepatitis E agent. Human caliciviruses have been resistant to in vitro cultivation, and direct study of their origins and reservoirs outside infected humans or water and foods (such as shellfish contaminated with human sewage) has been difficult. Modes of transmission, other than direct fecal-oral routes, are not well understood. In contrast, animal viruses found in ocean reservoirs, which make up a second calicivirus group, can be cultivated in vitro. These viruses can emerge and infect terrestrial hosts, including humans. This article reviews the history of animal caliciviruses, their eventual recognition as zoonotic agents, and their potential usefulness as a predictive model for noncultivatable human and other animal caliciviruses (e.g., those seen in association with rabbit hemorrhagic disease).

Published

1998

3. Reply to Drs. Capucci, Lavazza, and Mead

Author

Alvin W. Smith, Neil J. Cherry, and David O. Matson

Subjects

United States, Medicine, Infectious and parasitic diseases, RC109-216

Published

1998

4. Elevated post-transfusion serum transaminase values associated with a highly significant trend for increasing prevalence of anti-Vesivirusantibody in Korean patients

Author

Heetae Lee, GwangPyo Ko, Eui Chong Kim, Alvin W. Smith, You-Hee Cho, and Jeong Soo Park

Subjects

Adult, Male, Hepatitis B virus, Blood transfusion, medicine.medical_treatment, Aspartate transaminase, Blood Donors, Hepacivirus, Antibodies, Viral, Serology, Immunoenzyme Techniques, Liver Function Tests, Virology, Republic of Korea, Confidence Intervals, Odds Ratio, Prevalence, medicine, Humans, Aspartate Aminotransferases, Antigens, Viral, Vesivirus, Aged, Caliciviridae Infections, Hepatitis, biology, medicine.diagnostic_test, business.industry, Transfusion Reaction, Alanine Transaminase, gamma-Glutamyltransferase, Middle Aged, Hepatitis B, medicine.disease, Hepatitis C, Logistic Models, Infectious Diseases, Liver, Alanine transaminase, Case-Control Studies, biology.protein, Elevated transaminases, Female, business, Liver function tests

Abstract

A highly significant increase in anti-Vesivirus (family Caliciviridae) antibody prevalence, along the axis from healthy blood donors; donors with elevated transaminase; patients with clinical hepatitis; and patients with post-transfusion/dialysis hepatitis, has been reported in human sera from the USA and Europe. Asian samples have now been tested retrospectively using serology and enzyme immunoassay (EIA) with a Vesivirus partial-capsid antigen expressed as a fusion protein. Anti-vesiviral antibodies were measured by optical densities (OD650) and compared in patients separated by age, gender and Groups A–F as follows: Control Group A, an Experimental Group B, which was divided further into Group C, patients with elevated enzymes (alanine transaminase (ALT), aspartate transaminase (AST), and γ-glutamyl transpeptidase (γ-GT); Group D, patients receiving transfused blood; Group E, patients with high enzyme levels after transfusion; and Group F, hepatitis B and C positive patients. Using multivariate logistic regression analyses, a significantly greater proportion of patients receiving transfusion(s), were positive for anti-Vesivirus antibody compared with non-transfused patients (P = 0.008; OR: 3.86, 95% CI: 1.43–10.43). Also, anti-Vesivirus antibody was significantly associated with elevated biochemical liver function tests: ALT ≥120 IU or AST ≥ 120 IU (P = 0.017; OR: 4.23, 95% CI: 1.30–13.80). In the blood transfusion group, anti-Vesivirus antibody was significantly correlated with high enzyme levels (ALT, P = 0.018; AST, P = 0.010; γ-GT, P = 0.020). These data provide serologic evidence of vesiviral transfusion–transmission-associated disease, which could include infection of any organ system where cytopathology resulted in high levels of either ALT or AST. J. Med. Virol. 84:1943–1952, 2012. © 2012 Wiley Periodicals, Inc.

Published

2012

5. Expression and self-assembly of virus-like particles from two genotypes of marine vesiviruses and development of an ELISA for the detection of antibodies

Author

Karin Bok, John D. Neill, Alvin W. Smith, Kimberlee B. Beckmen, Carlos H. Romero, Kathy A. Burek, Shasta D. McClenahan, Kim Y. Green, and Stanislav V. Sosnovtsev

Subjects

Serotype, Genotype, viruses, Enzyme-Linked Immunosorbent Assay, Antibodies, Viral, Microbiology, Article, Virus, Cell Line, Dogs, Antigen, Animals, Vesivirus, Caliciviridae Infections, Antiserum, Pacific Ocean, General Veterinary, biology, Virion, virus diseases, General Medicine, biology.organism_classification, Virology, Caliciviridae, Sea Lions, Capsid, biology.protein, Capsid Proteins, Antibody, Baculoviridae, Alaska

Abstract

Sequences encoding the major and minor capsid proteins (VP1 and VP2) from two marine vesivirus isolates (Steller sea lion viruses V810 and V1415) were engineered for expression of virus-like particles (VLPs) in the baculovirus system. The resulting VLPs were morphologically similar to native vesivirus virions. Purified VLPs were probed in immunoblots with pooled antisera specific for nine San Miguel sea lion virus (SMSV) types, and a predominant protein of approximately 60 kDa was detected. An enzyme linked immunosorbent assay (ELISA) for the detection of antibodies was developed in which the VLPs served as antigen. The VLPs were adsorbed to the wells of a microplate, and the specificity of the ELISA was established with hyperimmune sera raised against 24 serotypes of the genus Vesivirus . The ELISA was used to screen for the presence of vesivirus specific antibodies in the sera of free-ranging Steller sea lions. The ELISA results demonstrated that Steller sea lions that inhabit the Pacific Ocean waters of southeast Alaska are widely exposed to antigenically related marine vesiviruses, while no previous exposure could be demonstrated using VLP antigens in 17 Steller sea lions from the Aleutian Islands. The broad reactivity of these VLPs and their non-infectious nature will facilitate global sero-epidemiological studies aimed at determining the incidence and prevalence of marine vesiviruses in mammals that inhabit the Pacific and Atlantic oceans as well as susceptible terrestrial animals.

Published

2010

6. A capsid gene-based real-time reverse transcription polymerase chain reaction assay for the detection of marine vesiviruses in the Caliciviridae

Author

John D. Neill, Stanislav V. Sosnovtsev, Crystal R. Rhodes, Kim Y. Green, Shasta D. McClenahan, Alvin W. Smith, Carlos H. Romero, and Karin Bok

Subjects

Molecular Sequence Data, Sensitivity and Specificity, Article, Virus, Virology, biology.animal, Animals, Vesivirus, Mink, Gene, Caliciviridae Infections, DNA Primers, Feline calicivirus, Base Sequence, biology, Reverse Transcriptase Polymerase Chain Reaction, biology.organism_classification, Caliciviridae, Reverse transcription polymerase chain reaction, Capsid, RNA, Viral, Capsid Proteins, Water Microbiology, Sequence Alignment

Abstract

A real-time reverse transcription polymerase chain reaction (rtRT-PCR) assay was developed for the identification of marine vesiviruses. The primers were designed to target a 176-nucleotide fragment within a highly conserved region of the San Miguel sea lion viruses (SMSVs) capsid gene. The assay detected viral RNA from nine marine vesivirus serotypes described previously, including two serotypes (SMSV-8 and SMSV-12) not identified with presently available molecular assays, a highly-related bovine vesivirus strain (Bos-1), a mink vesivirus strain (MCV), and two novel genotypes isolated recently from Steller sea lions (SSL V810 and V1415). The real-time assay did not amplify sequences from the corresponding genomic regions of feline calicivirus (also in the genus Vesivirus) and representative members of the genus Norovirus. The rtRT-PCR assay described below may prove useful as a diagnostic tool for the detection of currently circulating, emerging and previously described marine vesiviruses in clinical samples, especially when large numbers are screened in surveillance studies of these restricted viruses.

Published

2009

7. Development of a real-time reverse transcription polymerase chain reaction assay for detection of marine caliciviruses (genus Vesivirus)

Author

Emily J. Cooper, Andrew Shaw, Scott M. Reid, Alvin W. Smith, Donald P. King, Nick J. Knowles, Geoffrey H. Hutchings, and Nigel P. Ferris

Subjects

Time Factors, Swine, viruses, Molecular Sequence Data, RNA-dependent RNA polymerase, Genome, Viral, Vesicular stomatitis Indiana virus, Sensitivity and Specificity, Virus, Cell Line, Microbiology, Vesicular Stomatitis, Swine Vesicular Disease, Sequence Homology, Nucleic Acid, Virology, Animals, Vesivirus, Serotyping, Swine vesicular disease, DNA Primers, Base Sequence, biology, Reverse Transcriptase Polymerase Chain Reaction, RNA-Dependent RNA Polymerase, biology.organism_classification, Caliciviridae, Sea Lions, Foot-and-Mouth Disease, RNA, Viral, Vesicular exanthema of swine virus, Cattle, Vesicular Exanthema of Swine, Nucleic Acid Amplification Techniques

Abstract

Marine caliciviruses form a distinct lineage within the genus Vesivirus (family Caliciviridae). This group includes vesicular exanthema of swine virus (VESV) and San Miguel sea lion virus (SMSV) and other related viruses which have been proposed to be marine in origin isolated from a variety of terrestrial and marine animals. Rapid and reliable detection of marine caliciviruses is important as these viruses appear to be widespread and can cause vesicular disease in a wide variety of susceptible hosts including pigs and experimentally infected cattle where clinical signs cannot be easily distinguished from foot-and-mouth disease (FMD), swine vesicular disease (SVD) and vesicular stomatitis (VS). A real-time RT-PCR assay targeting conserved nucleotide sequences in the RNA-dependent RNA polymerase (3D) region of the genome successfully detected cell culture-grown virus preparations of more than thirty marine calicivirus serotypes. Only the atypical SMSV serotypes 8 and 12 failed to be detected, which provided further indication of genetic divergence between these and the other calicivirus serotypes said to be marine in origin. The real-time RT-PCR assay also specifically amplified RNA from samples collected following experimental inoculation of pigs with VESV. No cross-reactivity was demonstrated when the assay was tested with RNA prepared from representative viruses of FMD, SVD and VS. The real-time RT-PCR assay described is a sensitive and specific tool for detection and differential diagnosis of these viruses from other vesicular-disease causing viruses.

Published

2007

8. Vesivirus viremia and seroprevalence in humans

Author

Alvin W. Smith, David O. Matson, Patrick L. Iversen, Karin Bok, David A. Stein, and Douglas E. Skilling

Subjects

Genes, Viral, Population, Molecular Sequence Data, Viremia, Blood Donors, Antibodies, Viral, Polymerase Chain Reaction, Article, Serology, Seroepidemiologic Studies, Virology, medicine, Seroprevalence, Humans, Vesivirus, human, Amino Acid Sequence, education, Caliciviridae Infections, Hepatitis, education.field_of_study, viremia, biology, seroprevalence, Base Sequence, calicivirus, Alanine Transaminase, DNA-Directed RNA Polymerases, biology.organism_classification, medicine.disease, Caliciviridae, United States, Infectious Diseases, Immunology, Capsid Proteins, Viral disease, Sequence Alignment, Research Article

Abstract

Pathogenic caliciviruses of the genus Vesivirus circulate in oceanic ecosystems and spread to and among terrestrial mammals. Isolation of Vesivirus from natural and laboratory infections in humans led to this investigation of Vesivirus seroprevalence and viremia. Sera from four groups were tested for antibodies to Vesivirus as follows: blood donors whose units were cleared for donation, blood donors whose units were not accepted for donation solely because of elevated blood liver alanine aminotransferase (ALT) concentrations, patients with clinical hepatitis of unknown but suspected infectious cause, and patients with clinical hepatitis of unknown cause but associated with blood transfusion or dialysis. Additionally, sera were tested for Vesivirus genome by three methods: dot‐blot and two reverse transcription‐polymerase chain reaction (RT‐PCR) methods. The calculated seroprevalence against Vesivirus virions within these groups (N = 765) was 12%, 21%, 29%, and 47%, respectively (P

Published

2006

9. Isolation and characterization of a new Vesivirus from rabbits

Author

David O. Matson, Alvin W. Smith, José M. Martín-Alonso, Angeles Machín, Nathan K. Keefer, Gloria del Barrio, Patrick L. Iversen, Lorenzo González-Molleda, Douglas E. Skilling, and Francisco Parra

Subjects

animal diseases, viruses, Molecular Sequence Data, Genome, Viral, Biology, Virus, Open Reading Frames, fluids and secretions, Virology, Consensus Sequence, biology.domesticated_animal, Animals, Vesivirus, Phylogeny, Genetics, Phylogenetic tree, Base Sequence, Nucleic acid sequence, Calicivirus, virus diseases, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, Caliciviridae, RNA genome, Open reading frame, Oligodeoxyribonucleotides, DNA, Viral, RNA, Viral, Rabbits, European rabbit

Abstract

This report describes the isolation, cDNA cloning, complete genome nucleotide sequence, and partial characterization of a new cultivable calicivirus isolated from juvenile feeder European rabbits (Oryctolagus cuniculus) showing symptoms of diarrhea. Absence of neutralization by type-specific neutralizing antibodies for 40 caliciviruses and phylogenetic sequence comparisons of the open reading frame 1-encoded polyprotein with those of other caliciviruses demonstrate that this new calicivirus is a putative novel member of the Vesivirus genus which is closely related to the marine calicivirus subgroup. According to its putative classification, this new virus has been named rabbit vesivirus.

Published

2005

10. New Calicivirus isolated from walrus

Author

Howard A. Fields, Lilia Ganova-Raeva, Alvin W. Smith, and Yury Khudyakov

Subjects

Cancer Research, viruses, Genome, Viral, Biology, Genome, Feces, Open Reading Frames, Virology, Animals, Vesivirus, Amino Acid Sequence, Cloning, Molecular, Phylogeny, Caliciviridae Infections, Polyproteins, Genomic organization, Genetics, Sequence Homology, Amino Acid, Reverse Transcriptase Polymerase Chain Reaction, Nucleic acid sequence, Calicivirus, Sequence Analysis, DNA, biology.organism_classification, Caliciviridae, Protein Structure, Tertiary, Infectious Diseases, Capsid, Suppression subtractive hybridization, RNA, Viral, Capsid Proteins, Walruses, Sequence Alignment

Abstract

The nucleotide sequence and genome organization of a new member of Caliciviridae was determined. Cell culture inoculated with fecal matter from walrus was used to recover fragments of a new virus by Suppression Subtractive Hybridization (SSH). The isolate was identified as a member of the Vesivirus genus of Caliciviridae and designated the name Walrus Calicivirus (WCV). Sets of PCR primers spanning the entire putative genome were designed using known sequences of other vesiviruses. The assembled genome was 8289 nucleotides (nt) long and shared no more than 87% identity with sequences of the other members of the genus Vesivirus. The largest open reading frame (ORF1) between positions 4-5646 encoded a polyprotein. ORF2, found at position 5652-7778, encoded a putative capsid protein. ORF3 overlapped ORF2 and encoded a small basic protein. Comparative analysis of multiple caliciviral capsid proteins was performed to propose a uniform capsid structural organization for this viral family.

Published

2004

11. Inhibition of Vesivirus Infections in Mammalian Tissue Culture with Antisense Morpholino Oligomers

Author

Douglas E. Skilling, David A. Stein, Alvin W. Smith, and Patrick L. Iversen

Subjects

Morpholino, Swine, viruses, Blotting, Western, Virus Replication, Cell Line, Open Reading Frames, Chlorocebus aethiops, Genetics, Animals, Vesivirus, Pharmacology, biology, Oligonucleotide, RNA, Oligonucleotides, Antisense, biology.organism_classification, Virology, Molecular biology, Microscopy, Electron, Titer, Open reading frame, Microscopy, Fluorescence, Viral replication, Cell culture, Protein Biosynthesis

Abstract

Caliciviruses infect and cause disease in animals and humans. They are nonenveloped, positive-stranded RNA viruses with a genome of approximately 7.5 kb that encodes viral proteins in three open reading frames (ORF). Antisense oligomers targeting one of the three ORF of caliciviruses of the genus Vesivirus significantly inhibit viral replication in tissue culture. Porcine kidney and African green monkey kidney cells were infected with Vesivirus isolates SMSV-13 and PCV Pan-1. Phosphorodiamidate morpholino oligomers (PMO) with sequence complementary to the AUG translation start site regions of ORF1, ORF2, and ORF3 were evaluated for their effect on viral titer. Scrape-loading delivered PMO to 50%-70% of the cells of the two cell lines, as measured by fluorescence microscopy and flow cytometry. A PMO targeting ORF3 caused a significant increase in viral titer. A PMO targeting ORF2, a scrambled PMO control sequence, and an unrelated PMO antisense sequence did not alter viral titer. Various PMO sequences antisense to an upstream region of ORF1 were effective in reducing viral titer up to 80% in a dose-dependent and sequence-specific manner. The extent of viral titer reduction was proportional to the delivery of PMO to cells. These observations demonstrate that antisense PMO can disrupt caliciviral gene function in a nucleic acid sequence-specific manner and are potentially effective antiviral agents.

Published

2001

12. Development of a reverse transcription polymerase chain reaction procedure for the detection of marine caliciviruses with potential application for nucleotide sequencing

Author

Nigel P. Ferris, Scott M. Reid, Alvin W. Smith, David M Ansell, Nick J. Knowles, and Geoffrey H. Hutchings

Subjects

Dolphins, viruses, Biology, Sensitivity and Specificity, Virus, law.invention, Vesicular Stomatitis, law, Virology, Animals, Swine vesicular disease, Polymerase chain reaction, Genetics, Vesicular exanthema of swine virus, Gorilla gorilla, Reverse Transcriptase Polymerase Chain Reaction, Crotalus, Sequence Analysis, DNA, biology.organism_classification, Caliciviridae, Reverse transcription polymerase chain reaction, Cats, Cattle, Primer (molecular biology)

Abstract

A reverse transcription polymerase chain reaction (RT-PCR) procedure is described for the detection of marine caliciviruses including vesicular exanthema of swine virus (VESV), San Miguel sea lion virus (SMSV), bovine Tillamook virus (BCV Bos-1) and caliciviruses (CV) isolated from dolphin (Cetacean CV), gorilla (Primate CV) and rattlesnake (Reptile CV) using primers (1F and 1R) designed from the capsid-coding region of the viral genome. These primers were compared with those described by Neill, J.D. and Seal, B.S., 1995: Development of PCR primers for specific amplification of two distinct regions of the genomes of San Miguel sea lion and vesicular exanthema of swine viruses, Mol. Cell. Probes 9, 33-38 (Hel1/Hel2), which had been designed from the 2C-like region of the calicivirus genome. Both sets proved to be extremely useful diagnostic tools for all of the known marine calicivirus serotypes with the exception of three: SMSV-8 and -12 and mink CV suggesting that these three caliciviruses may belong to a different group. Neither of the two primer sets reacted with strains of the vesicular disease viruses of foot-and-mouth disease (FMD), swine vesicular disease (SVD) or vesicular stomatitis (VS) nor with two feline caliciviruses (FCV). The 1F/1R primer set has the advantage over the Hel1/Hel2 set in that it generates a larger PCR product for nucleotide sequence investigations and so provides greater opportunity for identifying molecular differences between the viruses.

Published

1999

13. ISOLATION OF REPTILIAN CALICIVIRUS CROTALUS TYPE 1 FROM FERAL PINNIPEDS

Author

Robin F. Brown, Tomas Berke, Douglas E. Skilling, Alvin W. Smith, David O. Matson, E. S. Berry, and Jeffrey E. Barlough

Subjects

Serotype, Mouth, Ecology, Zalophus californianus, Seals, Earless, Rectum, Calicivirus, Zoology, Animals, Wild, Snakes, Aquatic animal, Crotalus, Biology, Antibodies, Viral, biology.organism_classification, California, Callorhinus ursinus, Animals, Anura, Fur seal, Eumetopias jubatus, Caliciviridae, Ecology, Evolution, Behavior and Systematics, Caliciviridae Infections

Abstract

Ten virus isolates were obtained from three species of marine mammals sampled on San Miguel Island (California, USA) and 1,200 km north on Rogue Reef (Oregon, USA) during tagging operations in 1986-87. Seven of these 10 were derived from 30 sampled Steller sea lion (Eumetopias jubatus pups, while two of 10 were isolated from one of 19 sampled California sea lion (Zalophus californianus californianus pups, and the remaining isolate was derived from 30 sampled northern fur seal (Callorhinus ursinus) pups. All 10 isolates were identified as belonging to a single serotype, reptilian calicivirus Crotalus type 1 (RCV Cro-1), previously isolated from both healthy and diseased snakes and frogs in a California zoologic collection. The marine samples also showed that nine of 30 Steller sea lion pups, one of 19 California sea lion pups and zero of 30 fur seal pups were producing type specific neutralizing antibodies to RCV Cro-1. This represents the first reported instance of the isolation from marine sources of calicivirus originally isolated from a terrestrial species.

Published

1998

14. Phylogenetic analysis of the caliciviruses

Author

Tamas Berke, Alvin W. Smith, Brian Golding, David Cubitt, Xi Jiang, David O. Matson, and Marianne Wolfaardt

Subjects

Genetics, biology, Phylogenetic tree, viruses, Calicivirus, virus diseases, biology.organism_classification, medicine.disease_cause, Virology, Caliciviridae, Hypervariable region, fluids and secretions, Infectious Diseases, Hepatitis E virus, Phylogenetics, medicine, Vesicular exanthema of swine virus, Vesivirus

Abstract

A phylogenetic portrait of the genus Calicivirus in the family Caliciviridae was developed based upon published sequences and newly characterized calicivirus (CV) strains, including additional Sapporo-like HuCV strains in pediatric diarrhea stool specimens from South Africa, the United Kingdom, and the United States. Distance and parsimony methods were applied to nucleotide and amino acid sequences of human and animal calicivirus 3D RNA-dependent RNA polymerase (∼470nt) and capsid hypervariable regions (∼1,200nt) to generate phylogenetic trees. Pairwise amino acid identity in the 3D region among the Sapporo-like strains ranged from 61%; to 100%. Human and animal caliciviruses (HuCVs and AnCVs) separated into five genogroups: small round-structured viruses (SRSV), Sapporo-like, and hepatitis E virus (HEV)-like HuCVs and rabbit-, and vesicular exanthema of swine virus (VESV)-like AnCVs, each with a distinct genome organization. Each genogroup, including the Sapporo-like HuCVs, subdivided further into subgenogroups. The capsid region trees had higher levels of confidence than the 3D region trees and limited conclusions about genogroups could be drawn from the 3D region analyses. This analysis suggested that CVs include five potential virus subfamilies. J. Med. Virol. 52:419–424, 1997. © 1997 Wiley-Liss, Inc.

Published

1997

15. Genetic characterization of a reptilian calicivirus (Cro1)

Author

Carlos Sandoval-Jaime, Kim Y. Green, Stanislav V. Sosnovtsev, Gabriel I. Parra, and Alvin W. Smith

Subjects

Virus Cultivation, viruses, Molecular Sequence Data, Cro1, Genome, Viral, Biology, Genome, California, Virus, Disease Outbreaks, lcsh:Infectious and parasitic diseases, Complete genome, Sequence Homology, Nucleic Acid, Virology, Chlorocebus aethiops, Animals, Cluster Analysis, lcsh:RC109-216, Vesivirus, Vero Cells, Phylogeny, Caliciviridae Infections, Whole genome sequencing, Phylogenetic tree, Research, Crotalus, Calicivirus, Sequence Analysis, DNA, Vesivirus phylogeny, biology.organism_classification, Infectious Diseases, Capsid, Viral evolution, RNA, Viral, Reptile calicivirus, Animals, Zoo

Abstract

Background Vesiviruses in the family Caliciviridae infect a broad range of animal hosts including mammals, birds, fish, amphibians and reptiles. The vesivirus Cro1 strains were isolated from diseased snakes in the San Diego zoo in 1978 and reported as the first caliciviruses found in reptiles. The goal of this study was to characterize the Cro1 strain 780032I that was isolated in cell culture from a rock rattlesnake (Crotalus lepidus) in the original outbreak. Results We re-amplified the original virus stock in Vero cells, and determined its full-length genome sequence. The Cro1 genome is 8296 nucleotides (nt) in length and has a typical vesivirus organization, with three open reading frames (ORF), ORF1 (5643 nt), ORF2 (2121 nt), and ORF3 (348 nt) encoding a nonstructural polyprotein, the major capsid protein precursor, and a minor structural protein, respectively. Phylogenetic analysis of the full-length genome sequence revealed that the Cro1 virus clustered most closely with the VESV species of the genus Vesivirus, but was genetically distinct (82-83% identities with closest strains). Conclusions This is the first description of a full-length genome sequence from a reptile calicivirus (Cro1). The availability of the Cro1 genome sequence should facilitate investigation of the molecular mechanisms involved in Cro1 virus evolution and host range.

Published

2012

16. Virus-specific antiviral treatment for controlling severe and fatal outbreaks of feline calicivirus infection

Author

Steve E. Poet, Alvin W. Smith, Kimberli Longley, Sherry S. Weaver, Patrick L. Iversen, Peter D. O'Hanley, David O. Matson, Michael A. Stone, Douglas E. Skilling, and Janet R. Christensen

Subjects

Male, Dose, Morpholines, Disease, Cat Diseases, Antiviral Agents, Virus, Disease Outbreaks, Morpholinos, Medicine, Animals, Caliciviridae Infections, Hepatitis, General Veterinary, business.industry, Therapeutic effect, Calicivirus, Outbreak, General Medicine, medicine.disease, Virology, Immunology, Cats, Female, Viral disease, business, Calicivirus, Feline

Abstract

Objective—To test the life-sparing and therapeutic effect of a parenterally administered virus-specific antiviral phosphorodiamidate morpholino oligomer (PMO) for treating kittens during outbreaks of severe viral disease. Animals—112 kittens of various sex and age in 4 trials involving 3 outbreaks of naturally developing caliciviral disease. Procedures—Each trial provided an opportunity to investigate the disease. A calicivirus isolated from the liver of a cat that died with hemorrhage and hepatitis was sequenced, and a PMO that had sequence specificity complementary to a 5' region was synthesized. In vitro efficacy of the PMO was tested against the isolate, followed by 3 trials in outbreaks of severe caliciviral disease. The PMO was administered starting on day 1 of disease onset (0.7 to 5.0 mg/kg, SC, q 24 h) and continuing for up to 7 days. Survival time, clinical recovery, and caliciviral shedding were compared by use of various antiviral dosages. In a fourth trial involving nonfatal disease, a control treatment was administered for comparison. Results—In vitro blockage of caliciviral replication by the PMO was dose dependent. In trials 1 to 3 in which survival was the endpoint, 47 of 59 cats receiving PMO survived but only 3 of 31 survived without PMO treatment. Antiviral treatment reduced viral shedding and hastened clinical recovery, as measured by weight gains and clinical condition. Conclusions and Clinical Relevance—These data provided evidence that virus-specific PMOs were effective in treating kittens with severe Vesivirus disease and suggested a broader application for other viruses and species, including humans.

Published

2008

17. Prevalence of vesivirus in a laboratory-based set of serum samples obtained from dairy and beef cattle

Author

Alvin W. Smith, David O. Matson, Douglas E. Skilling, James F. Evermann, and Andreas Kurth

Subjects

Serotype, Male, Veterinary medicine, Cattle Diseases, Enzyme-Linked Immunosorbent Assay, Beef cattle, Antibodies, Viral, Animal science, Seroepidemiologic Studies, Seroprevalence, Medicine, Animals, Vesivirus, Caliciviridae Infections, biology, General Veterinary, business.industry, General Medicine, Serum samples, biology.organism_classification, United States, Logistic Models, Herd, biology.protein, Cattle, Female, Antibody, business

Abstract

Objective—To examine sera obtained from dairy and beef cattle to detect antibodies against vesivirus and compare seroprevalence among cattle within the sample population. Sample Population—Cattle sera from 8 western states and Maryland submitted to the Washington Animal Disease Diagnostic Laboratory during 1999 and 2000. Procedure—Sera were analyzed for vesivirus-specific antibodies by use of a recombinant vesivirus–San Miguel sea lion virus serotype 5–capsid peptide antigen in an indirect ELISA. Results—Overall, 693 sera were tested and 105 (15.2%) had positive results. Seropositive cattle were from 7 states (all cattle from Montana and Maryland 10 and 4, respectively were seronegative). Overall seroprevalence for antivesivirus antibody in herds ranged between 0% and 80% (median, 14%). Higher antibody prevalence was significantly associated with older age, dairy rather than beef cattle, and reasons for submission. Logistic regression of factors (abortion, respiratory tract disease, and all other reasons for sample submission) revealed that older age and other reasons were independently associated with higher seroprevalence. Higher seropositive optical density values for the ELISA were observed among older cattle and cattle that aborted, compared with values for cattle with respiratory tract disease or other reasons for submission. Conclusions and Clinical Relevance—This laboratory-based surveillance sample provided a point estimate of seroprevalence against vesivirus among cattle in 9 US states. This suggests that vesivirus infection is widespread with high prevalence in some herds. Risk factors associated with vesivirus seroprevalence in beef and dairy cattle should be confirmed in population-based studies.

Published

2006

18. Infectious disease and the decline of Steller sea lions (Eumetopias jubatus) in Alaska, USA: insights from serologic data

Author

Kathy A. Burek, Frances M. D. Gulland, Gay Sheffield, Kimberlee B. Beckmen, Enid Keyes, Terry R. Spraker, Alvin W. Smith, Douglas E. Skilling, James F. Evermann, Jeffery L. Stott, Jerry T. Saliki, and Andrew W. Trites

Subjects

Male, animal diseases, Population, Antibodies, Viral, Serology, Marine mammal, Seroepidemiologic Studies, Cause of Death, Animals, Sea lion, education, Ecology, Evolution, Behavior and Systematics, Population Density, education.field_of_study, Ecology, biology, Bacterial Infections, biology.organism_classification, Serum samples, Antibodies, Bacterial, Sea Lions, Animals, Newborn, Infectious disease (medical specialty), Virus Diseases, Female, Eumetopias jubatus, Leptospira interrogans, Alaska

Abstract

Serologic data were examined to determine whether infectious disease may have played a role in the decline of Steller sea lions (Eumetopias jubatus) in the Gulf of Alaska and Aleutian Islands, USA. Available published data, unpublished data, and recent collections (1997-2000) were compared and reviewed. Data were stratified by geography to compare the declining western Alaskan population in the Aleutian Islands through eastern Prince William Sound to the increasing population in southeastern Alaska. Prevalences of antibodies from the 1970s to the early 1990s were noted for Leptospira interrogans, Chlamydophila psittaci, Brucella spp., phocid herpesvirus-1, and calciviruses. Serum samples collected from 1997-2000 were tested for antibodies to these agents as well as to marine mammal morbilliviruses, canine parvovirus, and canine adenovirus-1 and -2. Conclusions could not be drawn about changes in antibody prevalence to these agents during the decline of Steller sea lions, however, because data were incomplete or not comparable as a result of inconsistencies in testing techniques. Despite these shortcomings, results provided no convincing evidence of significant exposure of Steller sea lions to morbilliviruses, Brucella spp., canine parvovirus, or L. interrogans. Steller sea lions have been exposed to phocid herpesviruses, caliciviruses, canine adenovirus, and C. psittaci or to cross-reactive organisms in regions of both increasing and decreasing sea lion abundance. Based on similar antibody prevalence estimates from the increasing and decreasing populations, these agents are unlikely to have been the primary cause of the population decline. They may have contributed to the decline or impeded population recovery, however, because of undetected mortality and morbidity or reductions of fecundity and body condition in animals under other stresses. Systematic monitoring for disease agents and their effects is needed to determine whether infectious disease currently plays a role in the decline and lack of recovery of Steller sea lions.

Published

2005

19. Ice as a reservoir for pathogenic human viruses: specifically, caliciviruses, influenza viruses, and enteroviruses

Author

Scott O. Rogers, Alvin W. Smith, John D. Castello, and Douglas E. Skilling

Subjects

Disease reservoir, Cold climate, Biology, Permafrost, World health, Microbiology, Disease Outbreaks, Humans, Seawater, Ecosystem, Disease Reservoirs, Enterovirus, Cryopreservation, geography, geography.geographical_feature_category, Ice, Glacier, Influenza a, General Medicine, Cold Climate, Orthomyxoviridae, Virus Diseases, Lake ice, Ice sheet, Water Microbiology, human activities, Caliciviridae

Abstract

Hundreds of isolates of viable bacteria and fungi have been recovered from ancient ice and permafrost. Evidence supports the hypothesis that viral pathogens also are preserved in ice repositories, such as glaciers, ice sheets, and lake ice. Proof may depend upon narrowing the search by applying specific criteria, which would target candidate viruses. Such criteria include viral pathogens likely to occur in great abundance, likely to be readily transported into ice, and then participate in ongoing disease cycles suggestive of their having been deposited in and subsequently released from ice. Caliciviruses, influenza A, and some enteroviruses appear to satisfy all three criteria. Environmental ice appears to be an important abiotic reservoir for pathogenic microbes. World health and eradication of specific pathogens could be affected by this huge reservoir.

Published

2004

20. Antisense treatment of caliciviridae: an emerging disease agent of animals and humans

Author

Alvin W, Smith, David O, Matson, David A, Stein, Douglas E, Skilling, Andrew D, Kroeker, Tamas, Berke, and Patrick L, Iversen

Subjects

Species Specificity, Animals, Humans, Oligonucleotides, Antisense, Caliciviridae, Communicable Diseases, Emerging, Caliciviridae Infections

Abstract

The Earth's oceans are the primary reservoir for an emerging family of RNA viruses, the Caliciviridae, which can cause a spectrum of diseases in marine animals, wildlife, farm animals, pets and humans. Certain members of this family have unusually broad host ranges, and some are zoonotic (transmissible from animals to humans). The RNA virus replicative processes lack effective genetic repair mechanisms, and, therefore, virtually every calicivirus replicate is a mutant. Hence, traditional therapeutics dependent on specific nucleic acid sequences or protein epitopes lack the required diversity of sequence or conformational specificity that would be required to reliably detect, prevent or treat infections from these mutant clusters (quasi-species) of RNA viruses, including the Caliciviridae. Antisense technology using phosphorodiamidate morpholino oligomers shows promise in overcoming these current diagnostic and therapeutic problems inherent with newly emerging viral diseases.

Published

2002

21. Detection of vesicular exanthema of swine-like calicivirus in tissues from a naturally infected spontaneously aborted bovine fetus

Author

David O. Matson, Douglas E. Skilling, Alvin W. Smith, Tamas Berke, Andrew D. Kroeker, Patrick L. Iversen, and David A. Stein

Subjects

Pathology, medicine.medical_specialty, Cattle Diseases, Sequence Homology, Biology, Diagnosis, Differential, Fetus, medicine, Animals, Lung, Phylogeny, Caliciviridae Infections, Vesicular exanthema of swine virus, General Veterinary, Reverse Transcriptase Polymerase Chain Reaction, Calicivirus, Abortion, Veterinary, Virology, Fetal Diseases, Microscopy, Electron, RNA, Viral, Cattle, Female, Vesicular Exanthema of Swine, Caliciviridae

Published

2002

22. Virus Cycles in Aquatic Mammals, Poikilotherms, and Invertebrates

Author

Alvin W. Smith

Subjects

Poikilotherm, Host (biology), Ecology, viruses, Ecosystem, RNA virus, Water quality, Substrate (biology), Biology, biology.organism_classification, Virus, Invertebrate

Abstract

This chapter discusses virus cycles in aquatic mammals, poikilotherms, and invertebrates. It reviews the survival mechanisms and movements of ocean caliciviruses through diverse ecosystems and hosts. Members of the family Caliciviridae are naked single-stranded positive-sense RNA icosahedral viruses having one major capsid polypeptide and distinctive cuplike surface depressions. Caliciviruses have been shown to impact animal health while also receiving a high biological security classification as a foreign animal disease virus. These agents move through the environment in water and food, so that concerns for water quality and the public health aspects of food safety arise. The caliciviruses of ocean origin provide a classic model of RNA virus quasi-species movements played out across the global reaches of oceans, land masses, and the air. Viruses can be transported across the land and through the air, but they replicate only in water substrate. Their release from host tissues into bodies of water frequently provides them with a highly effective means of transport and survival outside the host cell.

Published

2000

23. Contributors

Author

Noreen J. Adcock, Jeremy A. Bruenn, Charles H. Calisher, Anju Chatterji, V. Gregory Chinchar, Victor R. DeFilippis, Claude M. Fauquet, Frank J. Fenner, Christon J. Hurst, Christina A. Kellogg, H.D. Alan Lindquist, Judith H. Myers, Debi P. Nayak, Robert A. Owens, John H. Paul, Michael L. Perdue, Lorne D. Rothman, Bruce S. Seal, Alvin W. Smith, Curtis A. Suttle, Glenn C. Telling, and Luis P. Villarreal

Published

2000

24. Complete nucleotide sequence and genomic organization of a primate calicivirus, Pan-1

Author

David O. Matson, Alvin W. Smith, Xi Jiang, J. E. Rinehart-Kim, and W.-M. Zhong

Subjects

Genetics, Untranslated region, Primates, DNA, Complementary, Base Sequence, viruses, Molecular Sequence Data, Nucleic acid sequence, Calicivirus, RNA, General Medicine, Genome, Viral, biochemical phenomena, metabolism, and nutrition, Biology, biology.organism_classification, Virology, Genome, Caliciviridae, Cats, Animals, Sequence Analysis, Genomic organization, Sequence (medicine)

Abstract

The primate calicivirus, Pan-1, was originally isolated from several primate species. It displayed typical calicivirus morphology by electron micro-scopy. We determined the genomic sequence of Pan-1 by cDNA cloning and direct RNA sequencing. Pan-1 shares a similar genomic organization and a high degree of sequence identity with feline caliciviruses. The Pan-1 genome contains 8 304 nucleotides, plus a poly-A tail, and is longer than any other calicivirus strains with a completely known sequence. The extra sequences of Pan-1 include a unique 424-nucleotide sequence at the 5′ end of ORF1, additional amino acids at the N-terminus of the capsid, and a longer 3′ UTR.

Published

1999

25. Genomic mapping of a calicivirus VPg

Author

Alvin W. Smith, Diane Dunham, Xi Jiang, Tamas Berke, and David O. Matson

Subjects

Primates, Picornavirus, Genes, Viral, RNase P, viruses, Molecular Sequence Data, Sequence alignment, Genome, Viral, Cell Line, Virology, Animals, Amino Acid Sequence, Gene, Peptide sequence, Phylogeny, Subgenomic mRNA, Genetics, biology, Sequence Homology, Amino Acid, Virulence, Viral Core Proteins, Calicivirus, RNA, Chromosome Mapping, General Medicine, biology.organism_classification, RNA, Viral, Caliciviridae

Abstract

We identified a primate calicivirus (Pan-1) VPg in Pan-1-infected cells. The Pan-1 VPg was associated with both genomic and subgenomic RNAs. RNase digestion of Pan-1 RNA yielded a residual protein of 16 kDa. The N-terminal sequence of Pan-1 VPg was determined by direct amino acid sequencing and mapped to a region of the genome equivalent to picornavirus VPgs. Alignment of this protein sequence with similar regions of other calicivirus genomes allowed identification of conserved amino acid motifs and potential boundaries of the calicivirus VPg genes. Proteinase K treatment abolished the infectivity of Pan-1 RNA, suggesting that Pan-1 VPg is required for RNA infectivity.

Published

1999

26. In vitro isolation and characterization of a calicivirus causing a vesicular disease of the hands and feet

Author

J. E. Barlough, S. E. Poet, J. Mead, T. Berke, David O. Matson, Douglas E. Skilling, Alvin W. Smith, and E. S. Berry

Subjects

Microbiology (medical), Serotype, Adult, Male, Seals, Earless, Population, Molecular Sequence Data, Human pathogen, Virus, Animals, Humans, Vesivirus, Amino Acid Sequence, education, Caliciviridae Infections, education.field_of_study, biology, Base Sequence, Foot, Calicivirus, biology.organism_classification, Hand, Virology, Caliciviridae, Infectious Diseases, Callorhinus ursinus, DNA, Viral

Abstract

We report that a calicivirus of oceanic origin, San Miguel sea lion virus serotype 5 (SMSV-5), is a human pathogen. This biotype was isolated originally from blisters on the flippers of northern fur seals (Callorhinus ursinus) and replicates readily in primate and human cell lines. It infects a phylogenetically diverse array of hosts (poikilotherms to primates) and induces type-specific neutralizing antibodies in exposed humans. Group antibody against a pooled antigen of SMSV-5 and two other serotypes was also observed in 18% of 300 blood donors from a population in the northwestern United States. The human calicivirus isolate designated SMSV-5 Homosapien-1 (SMSV-5 Hom-1) was recovered from a laboratory worker with systemic illness, including vesicular lesions on all four extremities. We believe this newly described human disease represents a paradigmatic shift in calicivirus disease recognition.

Published

1998

27. Detection of a non-cultivatable calicivirus from the white tern (Gygis alba rothschildi)

Author

William G. Gilmartin, Steven E. Poet, Alvin W. Smith, Jennifer L. Megyesi, and Douglas E. Skilling

Subjects

Gygis alba, viruses, Virus, Hawaii, Cell Line, Birds, Nest, Chlorocebus aethiops, Animals, Hatchling, Vero Cells, Ecology, Evolution, Behavior and Systematics, Caliciviridae Infections, Ecology, biology, Bird Diseases, Hybridization probe, Calicivirus, virus diseases, Nucleic Acid Hybridization, biology.organism_classification, Virology, Microscopy, Electron, DNA, Viral, RNA, Viral, African Green Monkey, Tern, Caliciviridae

Abstract

In April 1992, on Tern Island, French Frigate Shoals, Hawaii (USA), researchers observed a hand-reared white tern hatchling (Gygis alba rothschildi) develop vesicular lesions on the webbing between its toes, 6 days after falling out of its nest. Vesicular fluid collected from the foot lesions contained virus-like particles having typical calicivirus morphology. Calicivirus RNA was detected in the vesicular fluid by dot hybridization with a group-specific calicivirus copy DNA probe. Attempts to cultivate the virus in African green monkey kidney cells and porcine kidney cells were unsuccessful. This is the first report of a calicivirus infection associated with vesicular disease in a wild avian species.

Published

1996

28. Partial characterization of the genome of nine animal caliciviruses

Author

E. Poet, Xi Jiang, M. B. Dinulos, Brian Golding, Xianmin Dai, David O. Matson, Weiming Zhong, Alvin W. Smith, and Tamas Berke

Subjects

DNA, Complementary, Genes, Viral, Seals, Earless, Molecular Sequence Data, Sequence alignment, Genome, Viral, Biology, Genome, Polymerase Chain Reaction, fluids and secretions, Capsid, Phylogenetics, Virology, Complementary DNA, Sequence Homology, Nucleic Acid, Chlorocebus aethiops, Animals, Humans, Amino Acid Sequence, Cloning, Molecular, Gene, Vero Cells, Cells, Cultured, Phylogeny, Caliciviridae Infections, Genetics, Phylogenetic tree, Base Sequence, Sequence Homology, Amino Acid, Nucleic acid sequence, General Medicine, DNA-Directed RNA Polymerases, Sequence Analysis, DNA, biology.organism_classification, Caliciviridae, RNA, RNA, Viral, Capsid Proteins, Sequence Alignment

Abstract

Caliciviruses (CVs) include at least 42 distinct serotypes. Seventeen CV serotypes have been isolated from marine sources and are called San Miguel sea lion caliciviruses (SMSVs). CVs also have been isolated from reptiles, primates, and other terrestrial animals. Nucleotide sequences from portions of genome of prototype strains for six SMSV serotypes, the reptile CV, Cro-1, the cetacean CV, Tur-1, and the primate CV, Pan-1, are presented. cDNA products of the polymerase (all strains characterized) and capsid (SMSV-17) regions were produced by reverse transcription-polymerase chain reaction using Pan-1 primers. Comparisons of nucleotide and amino acid identity among these and published CV sequences indicated that the nine characterized CVs fall into a phylogenetic group that includes SMSV-1 and SMSV-4 and that is more closely related to other characterized animal CVs than to most human CVs. The phylogenetic analysis also indicated that distinct genera exist among the Caliciviridae. SMSV-17 and SMSV-4 are predicted to be closer to each other than other caliciviruses of known serotype; 574 (82%) of the 704 amino acids in the SMSV-17 and SMSV-4 capsid genes were identical.

Published

1996

29. Reply to Drs. Capucci, Lavazza, and Mead

Author

David O. Matson, Alvin W. Smith, and NJ Cherry

Subjects

lcsh:R, lcsh:Medicine, Library science, lcsh:RC109-216, Research article, Sociology, United States, Research Article, lcsh:Infectious and parasitic diseases

Published

1998

30. Serologic evidence of vesivirus-specific antibodies associated with abortion in horses

Author

Douglas E. Skilling, Andreas Kurth, and Alvin W. Smith

Subjects

Male, Indirect elisa, endocrine system, Veterinary medicine, animal diseases, Population, Abortion, Antibodies, Viral, Serology, Pregnancy, Animals, Medicine, Vesivirus, Horses, education, reproductive and urinary physiology, Caliciviridae Infections, education.field_of_study, biology, General Veterinary, urogenital system, business.industry, General Medicine, Abortion, Veterinary, biology.organism_classification, Peptide antigen, Specific antibody, biology.protein, Female, Horse Diseases, sense organs, Antibody, business

Abstract

Objective—To test horses for serologic evidence of an association between vesiviral antibodies and abortion. Sample Population—Sera from 141 horses. Procedures—2 experiments were conducted. Experiment 1 comprised sera obtained in 2001 and 2002 from 3 groups of horses (58 mares from farms with a history of abortion problems, 25 mares between 3 and 13 years of age with unknown reproductive histories that were sold at auction [breeding-age control mares], and 29 mixed-age males and yearling females sold at auction [negative control population]). Experiment 2 comprised sera from 3 groups of pregnant mares (10 pregnant mares fed Eastern tent caterpillars [ETCs], 9 pregnant mares fed ETC frass only, and 10 pregnant control mares). Sera were analyzed for antibodies against vesivirus by use of a validated recombinant vesivirusspecific peptide antigen in an indirect ELISA. Results—For experiment 1, 37 of 58 (63.8%) mares from farms with abortion problems were seropositive for vesivirus antibodies, whereas 10 of 25 (40%) breeding-age control mares were seropositive. All 29 mixed-age males and yearling females were seronegative for vesivirus antibodies. For experiment 2, 17 of 29 mares aborted (some from each group). Seropositive status for vesivirus antibodies increased from 47.1% (8/17) to 88.2% (15/17) for the pregnant mares that aborted during the experiment. Conclusion and Clinical Relevance—Significant association was detected between seropositive status for vesivirus and abortion in mares; consequently, vesivirus appears to be a pathogenic virus associated with abortion in mares. These data support adding vesivirus antibody testing into diagnostic screening to determine the cause for abortion in mares.

Published

2006

31. Release of RHD Virus in Australia

Author

Alvin W. Smith

Subjects

Multidisciplinary

Published

1996

32. FIRST ISOLATION OF A CALICIVIRUS FROM THE STELLER SEA LION (EUMETOPIAS JUBATUS)

Author

Douglas E. Skilling, Robin F. Brown, Jeffrey E. Barlough, E. S. Berry, and Alvin W. Smith

Subjects

Serotype, Ecology, biology, viruses, Rectum, Calicivirus, Oropharynx, biology.organism_classification, Isolation (microbiology), Caniformia, Sea Lions, Oregon, Marine mammal, Animals, Newborn, Animals, Sample collection, Sea lion, Eumetopias jubatus, Caliciviridae, San Miguel sea lion virus, Ecology, Evolution, Behavior and Systematics

Abstract

A calicivirus was isolated from the rectum of a Steller sea lion (Eumetopias jubatus) pup on Rogue Reef, off the southern Oregon coast. Based on the results of neutralization tests I with specific typing antisera, the isolate was identified as San Miguel sea lion virus serotype 6 (SMSV-6). Blood obtained from nine of 37 pups (24%) during virus sample collection procedures had specific neutralizing antibodies to SMSV-6. The isolation of SMSV-6 from a Steller sea lion represents, to our knowledge, the first isolation of any virus from this widely distributed marine mammal species, and serves to reconfirm the host-nonspecificity of yet another calicivirus of marine origin.

Published

1987

33. A new calicivirus isolated from a marine mammal

Author

Douglas E. Skilling, Alvin W. Smith, T. G. Akers, H. L. Bray, and A. B. Latham

Subjects

Serotype, Picornaviridae Infections, biology, Seals, Earless, animal diseases, Calicivirus, Introduced species, Aquatic animal, General Medicine, Antibodies, Viral, biology.organism_classification, Virology, Caliciviridae, Caniformia, Serology, Marine mammal, Elephant seal, Animals, Antigens, Viral

Abstract

A new serotype of calicivirus, designated as San Miguel sea lion virus type 6 (SMSV-6), was isolated from vesicular lesions on the flipper of a California sea lion pup. Serologic studies show that SMSV-6 neutralizing antibodies (SN) occur frequently among California sea lions and occasionally among northern fur seals. Feral swine, 1- to 6-week elephant seal pups and grey whales tested negative for SMSV-6 antibody.

Published

1979

34. ANTIBODIES TO MARINE CALICIVIRUSES IN THE STELLER SEA LION (EUMETOPIAS JUBATUS SCHREBER)

Author

Alvin W. Smith, Robert L. DeLong, E. S. Berry, Robin F. Brown, Jeffrey E. Barlough, and Enid A. Goodwin

Subjects

Serotype, Ecology, biology, Calicivirus, Zoology, Antibodies, Viral, biology.organism_classification, Caniformia, Sea Lions, Fetus, biology.protein, Animals, Antibody, Sea lion, Eumetopias jubatus, Caliciviridae, San Miguel sea lion virus, Ecology, Evolution, Behavior and Systematics, Zalophus

Abstract

Sera from 145 Steller sea lions (76 adults, three subadults, 37 pups, and 29 fetuses) were tested for neutralizing antibodies to nine marine calicivirus serotypes. Antibodies were found to San Miguel sea lion virus (SMSV) types 1, 5, 6, 7, 8, 10 and 13, and to Tillamook (bovine) calicivirus, but no antibodies were found to the walrus calicivirus. Titers (microtiter neutralization assay) ranged from 1:20 to 1:320, with many positive reactions at the higher dilutions (greater than or equal to 1:80). Antibodies to SMSV's 5 and 10 were most common among animals sampled in Alaskan waters, while antibodies to SMSV-6 were most common among pups from the southern Oregon coast. These data provide evidence that Steller sea lions, like their California sea lion (Zalophus c. californianus Lesson) counterparts, have experienced widespread exposure to multiple serotypes of marine caliciviruses.

Published

1987

35. Biophysical Comparisons of Calicivirus Serotypes Isolated from Pinnipeds

Author

M. E. Soergel, Alvin W. Smith, and Frederick L. Schaffer

Subjects

Serotype, viruses, Calicivirus, Picornaviridae, Biology, Virology, California, Caniformia, Cell Line, Infectious Diseases, Centrifugation, Density Gradient, Animals, Serotyping, San Miguel sea lion virus

Abstract

Biophysical properties of three new San Miquel sea lion virus isolates from pinnipeds were examined and compared with those of previously characterized serotypes. The caliciviruses showed an identical sedimentation rate of 183S in 5-20% sucrose. Buoyant densities in CsCl were in the range of 1.35-1.39 g/ml, with differences among the serotypes.

Published

1975

36. METASTATIC ADENOCARCINOMA IN TWO CALIFORNIA SEA LIONS, Zalophus c. californianus

Author

G. V. More John, R. J. Brown, R. L. DeLONG, and Alvin W. Smith

Subjects

Male, Lung Neoplasms, Ecology, Zalophus californianus, biology, Liver Neoplasms, Metastatic adenocarcinoma, Zoology, Anatomy, Adenocarcinoma, biology.organism_classification, Kidney Neoplasms, Caniformia, Sea Lions, Animals, Female, Sea lion, Ecology, Evolution, Behavior and Systematics, Zalophus

Abstract

Two California sea lions (Zalophus californianus californianus) came to necropsy with morphologically identical metastatic tumors. These were of glandular epithelial origin and were widespread throughout the visceral organs. Both animals were found beached and dead within two months and were only 220 km apart.

Published

1980

37. PREVALENCE AND DISTRIBUTION OF SERUM NEUTRALIZING ANTIBODIES TO TILLAMOOK (BOVINE) CALICIVIRUS IN SELECTED POPULATIONS OF MARINE MAMMALS

Author

Alvin W. Smith, Jeffrey E. Barlough, E. S. Berry, and Douglas E. Skilling

Subjects

Male, Seals, Earless, Dolphins, Zoology, Cetacea, Antibodies, Viral, Animals, Ecology, Evolution, Behavior and Systematics, Ecology, biology, Whales, Calicivirus, Aquatic animal, biology.organism_classification, Caliciviridae, Caniformia, Callorhinus ursinus, biology.protein, Female, Walruses, Antibody, Eumetopias jubatus, Zalophus

Abstract

Neutralizing antibodies to Tillamook calicivirus (TCV) were found in sera collected from California sea lions (Zalophus c. californianus Lesson) in 1983 and 1984 and in sera collected from Steller sea lions (Eumetopias jubatus Schreber) in 1976 and 1985. The combined prevalence of antibodies for these two species was 10/228 = 4.38%. Titers ranged from 1:20 (five animals), to 1:40 (four animals), to 1:80 (one animal) by standard microtiter neutralization assay. The seropositive pinnipeds were dispersed widely along the margins of the eastern Pacific rim, from the Bering Sea to the Santa Barbara Channel. Antibodies to TCV were not found in sera collected from northern fur seals (Callorhinus ursinus L.), Pacific walruses (Odobenus rosmarus divergens Illiger), seals of the family Phocidae, or several cetacean species. Tillamook calicivirus was isolated originally in 1981 from dairy calves in Oregon; the finding of neutralizing antibodies in two widely distributed species of sea lions suggests the possibility of a marine origin for this agent.

Published

1987

38. Calicivirus (SMSV-5) infection in experimentally inoculated Opaleye fish(Girella nigricans)

Author

D. E. Skilling, Catharine M. Prato, Alvin W. Smith, and H. L. Bray

Subjects

Girella nigricans, animal diseases, Spleen, Biology, Cell Line, Microbiology, Fish Diseases, Virology, Chlorocebus aethiops, medicine, Animals, Seawater, San Miguel sea lion virus, Picornaviridae Infections, Inoculation, Fishes, Calicivirus, virus diseases, General Medicine, medicine.anatomical_structure, Salt water, Vero cell, Water Microbiology, Caliciviridae

Abstract

At 15 degrees C, San Miguel sea lion virus infected fish (Girella nigricans), producing 10(7).6 TCID50 per gram of spleen, replicated in Vero cells (10(8) TCID50/gm) and retained viability after 14 days exposure to salt water (10(5) TCID50/ml dropped to 10(2).

Published

1981

39. Size and efficiency

Author

Alvin W. Smith, James R. Montgomery, Lawrence W. Broomall, Beatrice T. Mahan, and Gerald W. McLaughlin

Subjects

Economic growth, Higher education, Cost effectiveness, business.industry, media_common.quotation_subject, School size, Education, Economies of scale, Microeconomics, Critical mass (sociodynamics), Order (exchange), ComputingMilieux_COMPUTERSANDEDUCATION, Institution, Economics, business, Large size, media_common

Abstract

It has been long assumed that it takes some optimum size in order to obtain a sufficient critical mass to have an economy of scale operation, but there has been little substantive study of the topic. This paper looks at the relationship between enrollment and costs at colleges and universities. The question under study is whether large size provides economy of scale for operating. The question, unfortunately, is masked by the complexity of an institution. The manner in which complexity, size, costs, and enrollment interrelate is the substance of this paper. The findings suggest that curricula and complexity have an exceedingly important bearing on per-student costs.

Published

1980

40. Ultrastructure of newly recognized caliciviruses of the dog and mink

Author

James F. Evermann, Douglas E. Skilling, Alvin W. Smith, and A. J. McKeirnan

Subjects

Glossitis, animal diseases, viruses, Infectious Disease, Hemorrhagic Pneumonia, Dogs, Virology, biology.animal, medicine, Animals, Electron Microscopy, Dog Diseases, Mink, Picornaviridae Infections, Hemorrhagic pneumonia, biology, Brief Report, Calicivirus, Pneumonia, General Medicine, medicine.disease, Microscopy, Electron, Ultrastructure, Caliciviridae

Abstract

Summary Two recently recognized viruses obtained from a dog with glossitis and from mink with hemorrhagic pneumonia were characterized by electron microscopy. The results of the negative-stained preparations indicated that the viruses were structurally compatible with the calicivirus group.

Published

1983

41. A simple, rapid method for preparation of virus isolates from cell culture for electron microscopy

Author

E. S. Berry, Douglas E. Skilling, Alvin W. Smith, and JE Barlough

Subjects

centrifugation, Chromatography, electron microscopy, viruses, Buoyant density, Cell Biology, Biology, Molecular biology, cells, cultured, Virus, Article, Pathology and Forensic Medicine, law.invention, Virus type, law, Cell culture, Centrifugation, Ultracentrifuge, Anatomy, Electron microscope, virus isolates

Abstract

Summary A simple procedure for the rapid preparation of virus isolates from cell culture for negative-contrast electron microscopy was devised. Using only conventional centrifugation steps (i.e. without ultracentrifugation), the procedure produced consistent, fine-quality preparations of a variety of virus types differing in size/shape and buoyant density.

Published

1986

42. Inhibition of norovirus replication by morpholino oligomers targeting the 5′-end of the genome

Author

David O. Matson, Patrick L. Iversen, Lorenzo González-Molleda, Alvin W. Smith, Victoria J. Cavanaugh, Carmelann Zintz, Karin Bok, Kyeong-Ok Chang, Kim Y. Green, and Ann E. Campbell

Subjects

Morpholino, Morpholines, viruses, ved/biology.organism_classification_rank.species, Biology, medicine.disease_cause, Virus Replication, Genome, Antiviral Agents, Article, Cell Line, Mice, fluids and secretions, Virology, medicine, Coding region, Animals, Humans, Antisense, Antiviral, ved/biology, Norovirus, RNA, virus diseases, biology.organism_classification, PMO, digestive system diseases, Viral replication, Protein Biosynthesis, RNA, Viral, Norwalk virus, Murine norovirus

Abstract

Noroviruses are an important cause of non-bacterial epidemic gastroenteritis, but no specific antiviral therapies are available. We investigated the inhibitory effect of phosphorodiamidiate morpholino oligomers (PMOs) targeted against norovirus sequences. A panel of peptide-conjugated PMOs (PPMOs) specific for the murine norovirus (MNV) genome was developed, and two PPMO compounds directed against the first AUG of the ORF1 coding sequence near the 5′-end of the genome proved effective in inhibiting MNV replication in cells. A consensus PPMO (designated Noro 1.1), designed to target the corresponding region of several diverse human norovirus genotypes, decreased the efficiency of protein translation in a cell-free luciferase reporter assay and inhibited Norwalk virus protein expression in replicon-bearing cells. Our data suggest that PPMOs directed against the relatively conserved 5′-end of the norovirus genome may show broad antiviral activity against this genetically diverse group of viruses.

43. Calicivirus Isolation and Persistence in a Pygmy Chimpanzee ( Pan paniscus )

Author

Douglas E. Skilling, Thomas L. Lester, Kurt Benirschke, Alvin W. Smith, and Philip K. Ensley

Subjects

Serotype, Lip lesion, Swine, animal diseases, viruses, Zoology, Antigen-Antibody Complex, Persistence (computer science), fluids and secretions, biology.animal, Animals, Humans, Primate, Antigens, Viral, Picornaviridae Infections, Multidisciplinary, biology, Calicivirus, Circulating antibodies, virus diseases, Hominidae, biochemical phenomena, metabolism, and nutrition, Isolation (microbiology), Virology, Pan paniscus, Microscopy, Electron, Cats, Cattle, Caliciviridae

Abstract

What may be the first calicivirus isolate from any primate species, including man, was recovered from a herpesvirus-like lip lesion on a pygmy chimpanzee and then, 6 months later, from the throat of the same animal. The infected individual and its cage mates had circulating antibodies that were type-specific for this calicivirus. The agent was antigenically different from 30 other calicivirus serotypes and is tentatively designated primate calicivirus Pan paniscus type 1 (PCV-Pan 1).

Published

1983

44. CALICIVIRUS ANTIBODIES IN WILD FOX POPULATIONS

Author

Alvin W. Smith, T. G. Akers, and Catherine M. Prato

Subjects

Ecology, animal diseases, Calicivirus, virus diseases, Transmission cycle, Biology, Virology, parasitic diseases, biology.protein, population characteristics, Antibody, Neutralizing antibody, San Miguel sea lion virus, geographic locations, Ecology, Evolution, Behavior and Systematics

Abstract

Three populations of wild foxes were sampled for serum neutralizing antibody to calicivirus (San Miguel sea lion virus) types 1-5. Neutralizing activity was detected in serum from gray foxes resident on Santa Cruz Island, California, but not in Arctic foxes from Alaska. The results indicate that foxes may be naturally infected with caliciviruses, but their role in the transmission cycle is unknown.

Published

1977

45. San Miguel Sea Lion Virus Isolation, Preliminary Characterization and Relationship to Vesicular Exanthema of Swine Virus

Author

Alvin W. Smith, Neylan A. Vedros, Stewart H. Madin, and Thomas G. Akers

Subjects

Hot Temperature, Virus Cultivation, Isolation (health care), Swine, animal diseases, Picornaviridae, Cytopathogenic Effect, Viral, Neutralization Tests, Pregnancy, Animals, Vesivirus, San Miguel sea lion virus, Disease Reservoirs, Multidisciplinary, biology, Animal disease, Outbreak, Abortion, Veterinary, Hydrogen-Ion Concentration, biology.organism_classification, Virology, Caniformia, Microscopy, Electron, RNA, Viral, Vesicular exanthema of swine virus, Female, Vesicular Exanthema of Swine, Foot-and-mouth disease virus

Abstract

BETWEEN 1932 and 1954 there were repeated outbreaks of vesicular exanthema of swine (VES) in Californian swine herds, but since 1956 no cases have occurred in the United States and this has been attributed to a federal law which prohibited the feeding of raw garbage to swine1. The continuing importance of vesicular diseases of swine, however, is suggested by reports from Italy2, Hong Kong3, Austria, Poland and Britain (personal communication from A. H. Dariri, Plum Island Animal Disease Laboratory, 1973) of a vesicular syndrome in swine that could not be ascribed to foot and mouth disease virus (FMDV).

Published

1973

46. Prevalence and distribution of four serotypes of SMSV serum neutralizing antibodies in wild animal populations

Author

H. L. Bray, T. G. Akers, Catherine M. Prato, and Alvin W. Smith

Subjects

Serotype, Male, Swine, Animals, Wild, Biology, Antibodies, Viral, Marine species, Marine bacteriophage, Neutralization Tests, Seroepidemiologic Studies, Animals, Serotyping, San Miguel sea lion virus, Ecology, Evolution, Behavior and Systematics, Caliciviridae Infections, Disease Reservoirs, Vesicular exanthema of swine virus, Sheep, Ecology, Goats, Fishes, Whales, Virology, Caniformia, Geographic distribution, biology.protein, Female, Antibody

Abstract

Serum neutralizing antibodies to four serotypes of San Miguel Sea Lion Virus (SMSV) were demonstrated in a variety of marine and terrestrial species. These results show a wide geographic distribution of SMS viruses in the marine environment and indicate that certain terrestrial mammals have been infected with these so-called marine viruses. Evidence is presented supporting the theory that unidentified submammalian marine species are a reservoir for SMSV.

Published

1976

47. Premature parturition in the California sea lion

Author

David B. Peakall, Robert W. Risebrough, William G. Gilmartin, Murray D. Dailey, Brock W De Lappe, John C. Sweeney, Alvin W. Smith, Lynn A. Griner, and Robert L. DeLong

Subjects

Male, Dichlorodiphenyl Dichloroethylene, Physiology, Picornaviridae, Trematode Infections, Biology, Virus, Fetus, Obstetric Labor, Premature, Pregnancy, Blubber, Animals, Leptospirosis, Sea lion, Nematode Infections, San Miguel sea lion virus, Ecology, Evolution, Behavior and Systematics, Premature parturition, Leptospira, Ecology, Age Factors, Abortion, Veterinary, biology.organism_classification, Polychlorinated Biphenyls, Caniformia, Leptospira pomona, Parasitology, Adipose Tissue, Liver, Virus Diseases, Immunology, Vesicular exanthema of swine virus, Nephritis, Interstitial, Female

Abstract

Twenty percent of the California sea lion pups born on San Miguel Island die due to premature parturition. Specimens collected from premature-partus animals resulted in recovery of a virus, San Miguel Sea Lion Virus, indistinguishable from Vesicular Exanthema of Swine Virus, and Leptospira pomona from some of the premature cows and pups. The age range of 10 females delivering healthy pups in June was 10-14 years. With one exception, the ages in 10 aborting females was 6-8 years. The p,p'-DDE levels of the premature parturient cows' blubber and liver were 7.6 and 4.8 times greater, respectively, than corresponding tissue concentrations in the full-term animals. Polychlorinated biphenyls residues were 4.4 and 3.8 times greater in aborting animals' blubber and liver than in the same tissues of full-term sea lions. Premature-partus females had tissue imbalances of mercury, selenium, cadmium and bromine. Pathology, parasitology, serum enzyme and hormone results are also presented. These data suggest an interrelationship of disease agents and environmental contaminants as the cause of premature parturition.

Published

1976

48. Serology and virology of the bowhead whale (Balaena mysticetus L.)

Author

Jeffrey E. Barlough, Kurt Benirschke, Douglas E. Skilling, Alvin W. Smith, and Thomas F. Albert

Subjects

Serotype, Virus Cultivation, Swine, viruses, Antibodies, Viral, Newcastle disease, Virus, Serology, Animals, Balaena, Ecology, Evolution, Behavior and Systematics, Ecology, biology, Bowhead whale, Whales, biology.organism_classification, Orthomyxoviridae, Virology, Antibodies, Bacterial, Paramyxoviridae, biology.protein, Vesicular Exanthema of Swine, Cetacea, Antibody, Leptospira interrogans, Caliciviridae

Abstract

Sera from four bowhead whales (Balaena mysticetus L.) were examined for the presence of specific antibodies, and tissue and swab samples from six and four animals respectively were processed for isolation of viruses and for initiation of bowhead whale cell cultures. All sera were negative for antibodies to nine serovars of Leptospira interrogans and to 21 orthomyxovirus subtypes and a paramyxovirus (Newcastle disease virus). All sera were positive, however, for neutralizing antibodies to one or more calicivirus serotypes. Two untyped adenoviruses were isolated from colon samples of two different whales, but neutralizing antibodies to the agents could not be demonstrated in any sera. Three primary bowhead whale cell cultures were derived from kidney (two cultures) and testis (one culture), from three individual whales.

Published

1987

49. Renal fibrosarcoma in the northern fur seal

Author

Alvin W. Smith, Mark C. Keyes, and Richard J. Brown

Subjects

Kidney, Pathology, medicine.medical_specialty, integumentary system, Ecology, biology, Fibrosarcoma, Fur Seals, Renal Fibrosarcoma, Anatomy, Histopathological examination, medicine.disease, biology.organism_classification, Kidney Neoplasms, Caniformia, medicine.anatomical_structure, Callorhinus ursinus, medicine, Animals, Female, Fur seal, Ecology, Evolution, Behavior and Systematics

Abstract

A 2-week-old northern fur seal female pup (Callorhinus ursinus) found dead in the Pribilof Islands had an irregular mass at the anterior pole of the right kidney. Histopathological examination revealed a fibrosarcoma.

Published

1975

50. Characterization of a new calicivirus isolated from feces of a dog

Author

Frederick L. Schaffer, J. W. Black, Douglas E. Skilling, W. D. Cubitt, M. E. Soergel, and Alvin W. Smith

Subjects

Diarrhea, viruses, Dolphins, Cross Reactions, Antibodies, Viral, Virus, Cell Line, Feces, Dogs, Cytopathogenic Effect, Viral, Virology, Animals, Dog Diseases, Serotyping, Genome size, Antigens, Viral, Antiserum, Picornaviridae Infections, biology, Calicivirus, RNA, General Medicine, biology.organism_classification, Caliciviridae, Cell culture, RNA, Viral

Abstract

Canine calicivirus (CaCV), isolated from feces of a dog with diarrhea, was readily propagated in cultures of canine cells and in a dolphin cell line. Serologic evidence indicated many dogs in at least one geographic area had been infected with CaCV, but its role as an etiologic agent of disease was not established. In cell culture most CaCV virions were strongly cell-associated making purification difficult. CaCV was established as a member of the Caliciviridae by morphology and physicochemical properties of virions (density, sedimentation rate, single major polypeptide, RNA genome size), although some of the properties differed slightly from those of previously described caliciviruses; evidence was also obtained for caliciviral RNA species in infected cells. Based on tests with antisera to numerous caliciviruses and presumed caliciviruses, CaCV appeared to be not closely related to any previously described virus except the stunting syndrome agent of chickens.

Published

1985