Your search keyword '"Jeremy D. Volkening"' showing total 4 results

1. Presence of Newcastle disease viruses of sub-genotypes Vc and VIn in backyard chickens and in apparently healthy wild birds from Mexico in 2017

Author

Claudio L. Afonso, Diana V. Cortés-Espinosa, Iryna V. Goraichuk, Salman Latif Butt, Helena Lage Ferreira, Tonya L. Taylor, Kiril M. Dimitrov, Angel E. Absalón, Jeremy D. Volkening, David L. Suarez, and J. L. Marín-Cruz

Subjects

animal structures, Genotype, viruses, Newcastle disease virus, Virulence, Animals, Wild, Genome, Viral, Newcastle disease, Virus, Birds, 03 medical and health sciences, Virology, Genetics, Animals, Columbidae, Mexico, Molecular Biology, Phylogeny, 030304 developmental biology, Whole genome sequencing, 0303 health sciences, Whole Genome Sequencing, biology, 030306 microbiology, Nucleic acid sequence, Outbreak, General Medicine, biology.organism_classification, Minion, SEQUENCIAMENTO GENÉTICO, Chickens

Abstract

Virulent Newcastle disease viruses (NDV) have been present in Mexico since 1946, and recently, multiple outbreaks have been reported in the country. Here, we characterized eleven NDV isolated from apparently healthy wild birds and backyard chickens in three different locations of Jalisco, Mexico in 2017. Total RNA from NDV was reverse-transcribed, and 1285 nucleotides, which includes 3/4 of the fusion gene, was amplified and sequenced using a long-read MinION sequencing method. The sequences were 99.99-100% identical to the corresponding region obtained using the Illumina MiSeq. Phylogenetic analysis using MinION sequences demonstrated that nine virulent NDV from wild birds belonged to sub-genotypes Vc and VIn, and two backyard chicken isolates were of sub-genotype Vc. The sub-genotype Vc viruses had nucleotide sequence identity that ranged from 97.7 to 98% to a virus of the same sub-genotype isolated from a chicken in Mexico in 2010. Three viruses from pigeons had 96.3-98.7% nucleotide identity to sub-genotype VIn pigeon viruses, commonly referred to as pigeon paramyxovirus, isolated in the USA during 2000-2016. This study demonstrates that viruses of sub-genotype Vc are still present in Mexico, and the detection of this sub-genotype in both chickens and wild birds suggests that transmission among these species may represent a biosecurity risk. This is the first detection and complete genome sequencing of genotype VI NDV from Mexico. In addition, the utilization of an optimized long-read sequencing method for rapid virulence and genotype identification using the Oxford nanopore MinION system is demonstrated.

Published

2019

2. Expression of chicken parvovirus VP2 in chicken embryo fibroblasts requires codon optimization for production of naked DNA and vectored meleagrid herpesvirus type 1 vaccines

Author

Fenglan Li, Jeremy D. Volkening, Robert Mullis, Laszlo Zsak, John Mercado, and Stephen J. Spatz

Subjects

animal structures, viruses, Genetic Vectors, Gene Expression, Enzyme-Linked Immunosorbent Assay, Chick Embryo, Biology, Antibodies, Viral, Fluorescence, DNA vaccination, Green fluorescent protein, Herpesvirus 1, Meleagrid, Parvovirus, Genes, Reporter, Virology, Vaccines, DNA, Genetics, Animals, Vector (molecular biology), Codon, Molecular Biology, Gene, virus diseases, Viral Vaccines, General Medicine, Transfection, Fibroblasts, Immunohistochemistry, Molecular biology, Internal ribosome entry site, Capsid, Naked DNA, embryonic structures, Capsid Proteins, Chickens

Abstract

Meleagrid herpesvirus type 1 (MeHV-1) is an ideal vector for the expression of antigens from pathogenic avian organisms in order to generate vaccines. Chicken parvovirus (ChPV) is a widespread infectious virus that causes serious disease in chickens. It is one of the etiological agents largely suspected in causing Runting Stunting Syndrome (RSS) in chickens. Initial attempts to express the wild-type gene encoding the capsid protein VP2 of ChPV by insertion into the thymidine kinase gene of MeHV-1 were unsuccessful. However, transient expression of a codon-optimized synthetic VP2 gene cloned into the bicistronic vector pIRES2-Ds-Red2, could be demonstrated by immunocytochemical staining of transfected chicken embryo fibroblasts (CEFs). Red fluorescence could also be detected in these transfected cells since the red fluorescent protein gene is downstream from the internal ribosome entry site (IRES). Strikingly, fluorescence could not be demonstrated in cells transiently transfected with the bicistronic vector containing the wild-type or non-codon-optimized VP2 gene. Immunocytochemical staining of these cells also failed to demonstrate expression of wild-type VP2, indicating that the lack of expression was at the RNA level and the VP2 protein was not toxic to CEFs. Chickens vaccinated with a DNA vaccine consisting of the bicistronic vector containing the codon-optimized VP2 elicited a humoral immune response as measured by a VP2-specific ELISA. This VP2 codon-optimized bicistronic cassette was rescued into the MeHV-1 genome generating a vectored vaccine against ChPV disease.

Published

2013

3. Comparative full genome analysis of four infectious laryngotracheitis virus (Gallid herpesvirus-1) virulent isolates from the United States

Author

Egbert Mundt, Claudio L. Afonso, Gerald F. Kutish, Calvin L. Keeler, L. Zsak, Sylva M. Riblet, C. M. Boettger, Stephen J. Spatz, K. F. Clark, Maricarmen García, Jeremy D. Volkening, and Daniel L. Rock

Subjects

Gallid herpesvirus 1, Sequence analysis, Molecular Sequence Data, Mutation, Missense, Genome, Viral, Genome, Immediate early protein, DNA sequencing, Open Reading Frames, Viral Proteins, Herpesvirus 1, Gallid, Virology, Genetics, Animals, Point Mutation, ORFS, Molecular Biology, Poultry Diseases, Whole genome sequencing, biology, Genetic Variation, Herpesviridae Infections, Sequence Analysis, DNA, General Medicine, biology.organism_classification, United States, GenBank, DNA, Viral, Chickens

Abstract

Gallid herpesvirus-1 (GaHV-1), commonly named infectious laryngotracheitis (ILT) virus, causes the respiratory disease in chickens known as ILT. The molecular determinants associated with differences in pathogenicity of GaHV-1 strains are not completely understood, and a comparison of genomic sequences of isolates that belong to different genotypes could help identify genes involved in virulence. Dideoxy sequencing, 454 pyrosequencing and Illumina sequencing-by-synthesis were used to determine the nucleotide sequences of four genotypes of virulent strains from GaHV-1 groups I-VI. Three hundred and twenty-five open reading frames (ORFs) were compared with those of the recently sequenced genome of the Serva vaccine strain. Only four ORFs, ORF C, U(L)37, ICP4 and U(S)2 differed in amino acid (aa) lengths among the newly sequenced genomes. Genome sequence alignments were used to identify two regions (5' terminus and the unique short/repeat short junction) that contained deletions. Seventy-eight synonymous and 118 non-synonymous amino acid substitutions were identified with the examined ORFs. Exclusive to the genome of the Serva vaccine strain, seven non-synonymous mutations were identified in the predicted translation products of the genes encoding glycoproteins gB, gE, gL and gM and three non-structural proteins U(L)28 (DNA packaging protein), U(L)5 (helicase-primase) and the immediate early protein ICP4. Furthermore, our comparative sequence analysis of published and newly sequenced GaHV-1 isolates has provided evidence placing the cleavage/packaging site (a-like sequence) within the inverted repeats instead of its placement at the 3' end of the U(L) region as annotated in the GenBank's entries NC006623 and HQ630064.

Published

2011

4. Dynamic equilibrium of Marek's disease genomes during in vitro serial passage

Author

Jeremy D. Volkening, Isabel M. Gimeno, Stephen J. Spatz, Richard L. Witter, and Mohammad Heidari

Subjects

Virus Cultivation, Genotype, Population, Virulence, Chick Embryo, Genome, Viral, Biology, Virus Replication, Deep sequencing, Open Reading Frames, Serial passage, Virology, Genetic variation, Genetics, Marek Disease, Animals, Serial Passage, education, Promoter Regions, Genetic, Molecular Biology, Gene, Herpesvirus 2, Gallid, Sequence Deletion, Marek's disease, education.field_of_study, High-Throughput Nucleotide Sequencing, Nuclear Proteins, General Medicine, Oncogene Proteins, Viral, Sequence Analysis, DNA, Fibroblasts, biology.organism_classification, Phenotype, Mutagenesis, Insertional, DNA, Viral, Trans-Activators, Nucleic Acid Conformation

Abstract

Attenuation of Gallid herpesvirus-2 (GaHV-2), the causative agent of Marek’s disease, can occur through serial passage of a virulent field isolate in avian embryo fibroblasts. In order to gain a better understanding of the genes involved in attenuation and associate observed changes in phenotype with specific genetic variations, the genomic DNA sequence of a single GaHV-2 virulent strain (648A) was determined at defined passage intervals. Biological characterization of these “interval-isolates” in chickens previously indicated that the ability to induce transient paralysis was lost by passages 40 and the ability to induce persistent neurological disease was lost after passage 80, coincident with the loss of neoplastic lesion formation. Deep sequencing of the interval-isolates allowed for a detailed cataloguing of the mutations that exist within a single passage population and the frequency with which a given mutation occurs across passages. Gross genetic alterations were identified in both novel and well-characterized genes and cis-acting regions involved in replication and cleavage/packaging. Deletions in genes encoding the virulence factors vLipase, vIL8, and RLORF4, as well as a deletion in the promoter of ICP4, appeared between passages 61 and 101. Three mutations in the virus-encoded telomerase which predominated in late passages were also identified. Overall, the frequency of mutations fluctuated greatly during serial passage and few genetic changes were absolute. This indicates that serial passage of GaHV-2 results in the generation of a collection of genomes with limited sequence heterogeneity.

Published

2012