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Deletion of DP148R, DP71L, and DP96R Attenuates African Swine Fever Virus, and the Mutant Strain Confers Complete Protection against Homologous Challenges in Pigs.

Abstract
The African swine fever virus (ASFV) has caused a devastating pandemic in domestic and wild swine, causing economic losses to the global swine industry. Recombinant live attenuated vaccines are an attractive option for ASFV treatment. However, safe and effective vaccines against ASFV are still scarce, and more high-quality experimental vaccine strains need to be developed. In this study, we revealed that deletion of the ASFV genes DP148R, DP71L, and DP96R from the highly virulent isolate ASFV CN/GS/2018 (ASFV-GS) substantially attenuated virulence in swine. Pigs infected with 104 50% hemadsorbing doses of the virus with these gene deletions remained healthy during the 19-day observation period. No ASFV infection was detected in contact pigs under the experimental conditions. Importantly, the inoculated pigs were protected against homologous challenges. Additionally, RNA sequence analysis showed that deletion of these viral genes induced significant upregulation of the host histone H3.1 gene (H3.1) and downregulation of the ASFV MGF110-7L gene. Knocking down the expression of H3.1 resulted in high levels of ASFV replication in primary porcine macrophages in vitro. These findings indicate that the deletion mutant virus ASFV-GS-Δ18R/NL/UK is a novel potential live attenuated vaccine candidate and one of the few experimental vaccine strains reported to induce full protection against the highly virulent ASFV-GS virus strain. IMPORTANCE Ongoing outbreaks of African swine fever (ASF) have considerably damaged the pig industry in affected countries. Thus, a safe and effective vaccine is important to control African swine fever spread. Here, an ASFV strain with three gene deletions was developed by knocking out the viral genes DP148R (MGF360-18R), NL (DP71L), and UK (DP96R). The results showed that the recombinant virus was completely attenuated in pigs and provided strong protection against parental virus challenge. Additionally, no viral genomes were detected in the sera of pigs housed with animals infected with the deletion mutant. Furthermore, transcriptome sequencing (RNA-seq) analysis revealed significant upregulation of histone H3.1 in virus-infected macrophage cultures and downregulation of the ASFV MGF110-7L gene after viral DP148R, UK, and NL deletion. Our study provides a valuable live attenuated vaccine candidate and potential gene targets for developing strategies for anti-ASFV treatment.
AuthorsXiaolan Qi, Tao Feng, Zhao Ma, Linlin Zheng, Huanan Liu, Zhengwang Shi, Chaochao Shen, Pan Li, Panxue Wu, Yi Ru, Dan Li, Zixiang Zhu, Hong Tian, Sen Wu, Haixue Zheng
JournalJournal of virology (J Virol) Vol. 97 Issue 4 Pg. e0024723 (04 27 2023) ISSN: 1098-5514 [Electronic] United States
PMID37017515 (Publication Type: Journal Article, Research Support, Non-U.S. Gov't)
Chemical References
  • Histones
  • Vaccines, Attenuated
  • Viral Vaccines
  • Virulence Factors
  • DP71L protein, African swine fever virus
  • DP148R protein African swine fever virus
  • DP96R protein, African swine fever virus
Topics
  • Animals
  • African Swine Fever (immunology, virology)
  • African Swine Fever Virus (genetics, immunology, pathogenicity)
  • Cells, Cultured
  • Gene Deletion
  • Genes, Viral (genetics)
  • Histones (genetics)
  • Swine
  • Vaccines, Attenuated (immunology)
  • Viral Vaccines (immunology)
  • Virulence Factors (genetics)

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