Your search keyword '"Christopher D. Richardson"' showing total 5 results

1. The novel hemagglutinin-esterase genes of human torovirus and Breda virus

Author

Lynn Duckmanton, Raymond Tellier, Martin Petric, and Christopher D. Richardson

Subjects

Serotype, Cancer Research, Immunoelectron microscopy, Guinea Pigs, Immunoblotting, Molecular Sequence Data, Torovirus, Hemagglutinins, Viral, Dot blot, Article, Feces, Virology, Animals, Humans, Amino Acid Sequence, Cloning, Molecular, Microscopy, Immunoelectron, Human torovirus, Gene, Novel hemagglutinin-esterase genes, biology, Hemagglutinin esterase, Reverse Transcriptase Polymerase Chain Reaction, Immune Sera, Nucleic acid sequence, Amplicon, biology.organism_classification, Molecular biology, Infectious Diseases, Acetylesterase, Cattle, Breda virus, Sequence Alignment, Viral Fusion Proteins

Abstract

Human torovirus (HTV) and Breda virus (BRV), members of the genus torovirus in the family Coronaviridae, are established infectious agents of humans and cattle, respectively. The hemagglutinin-esterase (HE) gene of Breda virus serotype 2 (BRV-2) has been identified and the nucleotide sequence for BRV serotype 1 (BRV-1) genome which contains the open reading frames for the viral structural proteins has been reported revealing the presence of a 1.25 kb gene whose nucleotide sequence is identical to that of the BRV-2 HE gene. In this study, we amplified the 1.2kb HE gene from the HTV genome using long RT-PCR and sequenced the amplicon directly. At the nucleotide level, the HTV HE gene manifests 85% sequence identity to the HE genes of BRV-1 and BRV-2 and 89% identity with the X pseudogene sequence of BEV. The 1.25 kb amplicons which contained the HE genes of BRV-1 and HTV were cloned and expressed in a baculovirus system and the proteins purified by sodium dodecyl sulphate-polyacrylamide gel electrophoresis. Hyperimmune sera prepared in guinea pigs against these proteins were reactive with both bovine torovirus (BTV) and human torovirus (HTV) antigens. By immunoblot, they reacted specifically with a 65 kDa protein corresponding in size to the torovirus HE protein. Furthermore, the hyperimmune sera but not the preimmune sera reacted with a series of BTV-positive and HTV-positive fecal specimens by immunoblot and dot blot analysis. By immunoelectron microscopy (IEM) torovirus particles from BTV-positive specimens from calves with diarrhea and HTV-positive specimens from patients were aggregated by the hyperimmune sera. Human convalescent sera and gnotobiotic calf post-infection sera reacted by immunoblot with the expressed 65 kDa protein. The expressed HE protein of HTV has important diagnostic potential.

Published

1999

2. Sequence analysis of human coronavirus 229E mRNAs 4 and 5: evidence for polymorphism and homology with myelin basic protein

Author

Janet N. Stewart, Samir Mounir, Pierre J. Talbot, Patricia Jouvenne, and Christopher D. Richardson

Subjects

Cancer Research, Human coronavirus 229E, Sequence analysis, Coronaviridae, Transmissible gastroenteritis coronavirus, Molecular Sequence Data, Biology, medicine.disease_cause, Article, Cell Line, Open Reading Frames, Virology, Sequence Homology, Nucleic Acid, medicine, Coding region, Animals, Humans, Amino Acid Sequence, RNA, Messenger, Polymorphism, 229E, Gene, Lung, Coronavirus, Genetics, Base Composition, Polymorphism, Genetic, Base Sequence, Nucleic acid sequence, RNA, Myelin Basic Protein, mRNA 5, mRNA 4, biology.organism_classification, Embryo, Mammalian, Molecular biology, Infectious Diseases, RNA, Viral, Chromosome Deletion, Nucleotide sequence, Human

Abstract

Human coronaviruses (HCV) are important pathogens responsible for respiratory, gastrointestinal and possibly neurological disorders. To better understand the molecular biology of the prototype HCV-229E strain, the nucleotide sequence of the 5'-unique regions of mRNAs 4 and 5 were determined from cloned cDNAs. Sequence analysis of the cDNAs synthesized from mRNA 4 revealed a major difference with previously published results. However, polymerase chain reaction amplification of this region showed that the sequenced cDNAs were produced from minor RNA species, an indication of possible genetic polymorphism in this region of the viral genome. The mutated messenger RNA 4 contains two ORFs: (1) ORF4a consisting of 132 nucleotides which potentially encodes a 44-amino acid polypeptide of 4653 Da; this coding sequence is preceded by a consensus transcriptional initiation sequence, CUAAACU, similar to the ones found upstream of the N and M genes; (2) ORF4b of 249 nucleotides potentially encoding an 83-amino acid basic and leucine-rich polypeptide of 9550 Da. On the other hand, mRNA 5 contains one single ORF of 231 nucleotides which could encode a 77-amino acid basic and leucine-rich polypeptide of 9046 Da. This putative protein presents a significant degree of amino acid homology (33%) with its counterpart found in transmissible gastroenteritis coronavirus (TGEV). The proteins in the two different viruses exhibit similar molecular weights and are extremely hydrophobic. Interestingly, a sequence homology of five amino acids was found between the protein encoded by ORF4b of HCV-229E and an immunologically important region of human myelin basic protein.

Published

1992

3. Notice of retraction to 'The novel hemagglutinin-esterase genes of human torovirus and Breda virus'

Author

Christopher D. Richardson, Lynn Duckmanton, Martin Petric, and Raymond Tellier

Subjects

Cancer Research, Infectious Diseases, Hemagglutinin esterase, Human torovirus, Virology, Biology, Gene, Virus, Breda Virus

Published

2001

4. Influenza virus M2 protein is an integral membrane protein expressed on the infected-cell surface

Author

Robert A. Lamb, Suzanne Zebedee, and Christopher D. Richardson

Subjects

Cancer Research, Vesicle-associated membrane protein 8, Hemagglutinin (influenza), Fluorescent Antibody Technique, Neuraminidase, Biology, medicine.disease_cause, General Biochemistry, Genetics and Molecular Biology, Virus, Cell Line, Viral Matrix Proteins, Viral Envelope Proteins, Virology, Infected cell, Influenza A virus, medicine, Cytotoxic T cell, Animals, Trypsin, Amino Acid Sequence, Amino Acids, Integral membrane protein, Immunosorbent Techniques, Immune Sera, Cell Membrane, Molecular biology, Hemagglutinins, Infectious Diseases, Membrane protein, M2 proton channel, biology.protein

Abstract

The influenza A virus M 2 protein is expressed abundantly at the cell surface, and in addition to the hemagglutinin (HA) and neuraminidase (NA), is a third virus-specific membrane protein. M 2 has an internal hydrophobic membrane anchorage domain and associates with the same cellular membrane fractions as HA and NA. Trypsin treatment of infected cells and immunoprecipitation with site-specific antisera indicate that a minimum of 18 NH 2 -terminal amino acids of M 2 are exposed at the cell surface. Ten NH 2 -terminal residues are conserved in all strains of influenza A virus for which sequences are available. Antibodies can recognize M 2 on the cell surface and therefore it may be an infected-cell surface antigen. We discuss properties of M 2 that match it to the elusive major target molecule on influenza A virus-infected cells for crossreactive cytotoxic T cells.

Published

1985

5. Functional expression of the hemagglutinin and fusion proteins of measles virus in a baculovirus expression system

Author

Philip Marshall, Dalius J. Briedis, Christopher D. Richardson, Manon Lalumière, Ghalib Alkhatib, and Jorge Vialard

Subjects

Measles virus, Cancer Research, Infectious Diseases, biology, Functional expression, Virology, Baculovirus expression, Hemagglutinin, biology.organism_classification, Fusion protein

Published

1988