Construction and manipulation of a full-length infectious bacterial artificial chromosome clone of equine herpesvirus type 3 (EHV-3)
| Autor: | Armando Damiani, Mariela Rita Scrochi, M. Barrandeguy, Maksat Akhmedzhanov, A. Vissani, Nikolaus Osterrieder |
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| Rok vydání: | 2016 |
| Předmět: |
0301 basic medicine
Cancer Research Chromosomes Artificial Bacterial CIENCIAS MÉDICAS Y DE LA SALUD Otras Ciencias Biológicas Genetic Vectors DNA Recombinant Mutagenesis (molecular biology technique) Gene Expression Genome Viral Viral Plaque Assay Biology Recombinant virus EHV-3 Transfection Virus Replication Virus law.invention EQUID HERPESVIRUS 3 Biotecnología de la Salud Ciencias Biológicas 03 medical and health sciences Open Reading Frames law Virology Gene Order ECE Cloning Molecular Gene Cells Cultured BAC Genetics Bacterial artificial chromosome GE 030104 developmental biology Infectious Diseases Mutagenesis Recombinant DNA Equine herpesvirus Homologous recombination Genetic Engineering Herpesvirus 3 Equid CIENCIAS NATURALES Y EXACTAS Otras Biotecnologías de la Salud |
| Zdroj: | Virus research. 228 |
| ISSN: | 1872-7492 |
| Popis: | Equine herpesvirus type 3 (EHV-3) is the causal agent of equine coital exanthema, a disease characterized by pox-like lesions on the penis of stallions and the vulva of mares. Although the complete genomic sequence of EHV-3 has been recently made available, its genomic content remains poorly characterized and the molecular mechanisms of disease development not yet elucidated. In an attempt to facilitate genetic manipulation of EHV-3, we describe here the construction of a full-length infectious bacterial artificial chromosome (BAC) clone of EHV-3. Mini-F vector sequences were inserted into the intergenic region between ORF19 and ORF20 (UL41 and UL40, respectively) of EHV-3 strain C175 by homologous recombination in equine dermal cells (NBL-6). DNA of the resulting recombinant virus was electroporated into E. coli and a full-length EHV-3 BAC clone was recovered. Virus reconstituted after transfection of the EHV-3 BAC into NBL-6 cells showed growth properties in vitro that were indistinguishable from those of the parental virus. To assess the feasibility of mutagenesis of the cloned EHV-3 genome, recombinant viruses targeting the glycoprotein E (gE) gene were generated using Red recombination in E. coli and in vitro growth properties of the recombinant viruses were evaluated. We first repaired the gE (ORF74) coding region, since the parental virus used for BAC cloning specifies a truncated version of the gene, and then created gE-tagged and gE-null versions of the virus. Our results demonstrated that: (i) EHV-3 can be efficiently cloned as a BAC allowing easy manipulation of its genome; (ii) gE is dispensable for EHV-3 growth in vitro and is expressed as a product of approximately 110-kDa in infected cells; (iii) viruses having a deletion compromising gE expression or with a truncation of the cytoplasmic and transmembrane domains are significantly compromised with regard cell-to-cell spread. The cloning of EHV-3 as a BAC simplifies future studies to identify the role of its coding genes in viral pathogenesis and host immune responses. Fil: Akhmedzhanov, Maksat. Freie University Berlin; Alemania Fil: Scrochi, Mariela Rita. Universidad Nacional de La Plata. Facultad de Ciencias Veterinarias. Departamento de Microbiología. Cátedra de Virología; Argentina Fil: Barrandeguy, María Edith. Instituto Nacional de Tecnología Agropecuaria. Centro de Investigación en Ciencias Veterinarias y Agronómicas. Instituto de Virología; Argentina Fil: Vissani, Aldana. Instituto Nacional de Tecnología Agropecuaria. Centro de Investigación en Ciencias Veterinarias y Agronómicas. Instituto de Virología; Argentina Fil: Osterrieder, Nikolaus. Freie University Berlin; Alemania Fil: Damiani, Armando Mario. Freie University Berlin; Alemania. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina |
| Databáze: | OpenAIRE |
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