Your search keyword '"Xuming Ou"' showing total 14 results

1. Host miRNA and mRNA profiles during in DEF and duck after DHAV-1 infection

Author

Meng Wang, Zezheng Liu, Anchun Cheng, Mingshu Wang, Ying Wu, Qiao Yang, Bin Tian, Xuming Ou, Di Sun, Shaqiu Zhang, Dekang Zhu, Renyong Jia, Shun Chen, Mafeng Liu, Xin Xin Zhao, and Juan Huang

Subjects

DHAV-1, miRNA, mRNA, miR-155, SOCS1, Medicine, Science

Abstract

Abstract DHAV-1 is a highly infectious pathogen that can cause acute hepatitis in ducklings. MicroRNA (miRNA) plays an essential regulatory role in virus response. We characterized and compared miRNA and mRNA expression profiles in duck embryonic fibroblasts (DEF) and the liver of ducklings infected with DHAV-1. DHAV-1 infected DEF was divided into infection group (D group) and blank group (M group), and DHAV-1 infected duckling group was divided into infection group (H group) and blank group (N group). D vs. M have 130 differentially expressed (DE) miRNA (DEM) and 2204 differentially expressed (DE) mRNA (DEG), H vs. N have 72 DEM and 1976 DEG. By the intersection of D vs. M and H vs. N comparisons, 15 upregulated DEM, 5 downregulated DEM, 340 upregulated DEG and 50 downregulated DEG were found with both in vivo and in vitro DHAV-1 infection. In particular, we identified the same DE miRNA target genes and functional annotations of DE mRNA. We enriched with multiple gene ontology (GO) and the Kyoto Encyclopedia of Genes and Genomes (KEGG) pathways, which may have important roles in viral virulence, host immunity, and metabolism. We selected miR-155, which is co-upregulated, and found that miR-155 targets SOCS1 to inhibit DHVA-1 replication.

Published

2024

2. Duck enteritis virus UL7 is a late gene and the UL7-encoded protein co-localizes with pUL51

Author

Jie Huang, Mingshu Wang, Anchun Cheng, Bin Tian, Xuming Ou, Ying Wu, Qiao Yang, Di Sun, Shaqiu Zhang, Sai Mao, Xinxin Zhao, Juan Huang, Qun Gao, Dekang Zhu, Renyong Jia, Shun Chen, and Mafeng Liu

Subjects

duck enteritis virus, UL7 protein, UL51 protein, late gene, co-localization, Biology (General), QH301-705.5

Abstract

BackgroundDuck enteritis virus (DEV) belongs to Alphaherpesvirinae; little is known about the DEV UL7 gene and its encoded protein. This study examined the molecular characteristics of DEV pUL7 in vitro and determined whether DEV pUL7 co-localizes with pUL51.ResultsThe results showed that UL7 can be regarded as a late gene. Moreover, immunofluorescence assay revealed that pUL7 was located around the perinuclear cytoplasmic region and co-localized with pUL51 in the cytoplasm and nucleus after transfection into duck embryo fibroblast cells (DEFs).ConclusionIn conclusion, we identified the molecular characteristics of the DEV UL7 gene, which is a late gene, and the co-localization of its encoded protein with pUL51 in transfected DEFs, enriching our understanding of pUL7 and future research directions.

Published

2024

3. Regulation of alphaherpesvirus protein via post-translational phosphorylation

Author

Tong Zhou, Mingshu Wang, Anchun Cheng, Qiao Yang, Bin Tian, Ying Wu, Renyong Jia, Shun Chen, Mafeng Liu, Xin-Xin Zhao, Xuming Ou, Sai Mao, Di Sun, Shaqiu Zhang, Dekang Zhu, Juan Huang, Qun Gao, Yanling Yu, and Ling Zhang

Subjects

Alphaherpesvirus, viral proteins, protein kinases, phosphorylated proteins, phosphorylation modification, Veterinary medicine, SF600-1100

Abstract

Abstract An alphaherpesvirus carries dozens of viral proteins in the envelope, tegument and capsid structure, and each protein plays an indispensable role in virus adsorption, invasion, uncoating and release. After infecting the host, a virus eliminates unfavourable factors via multiple mechanisms to escape or suppress the attack of the host immune system. Post-translational modification of proteins, especially phosphorylation, regulates changes in protein conformation and biological activity through a series of complex mechanisms. Many viruses have evolved mechanisms to leverage host phosphorylation systems to regulate viral protein activity and establish a suitable cellular environment for efficient viral replication and virulence. In this paper, viral protein kinases and the regulation of viral protein function mediated via the phosphorylation of alphaherpesvirus proteins are described. In addition, this paper provides new ideas for further research into the role played by the post-translational modification of viral proteins in the virus life cycle, which will be helpful for understanding the mechanisms of viral infection of a host and may lead to new directions of antiviral treatment.

Published

2022

4. The DHAV-1 protein VP1 interacts with PI3KC3 to induce autophagy through the PI3KC3 complex

Author

Juan Li, Mingshu Wang, Shan Zhou, Anchun Cheng, Xuming Ou, Di Sun, Ying Wu, Qiao Yang, Qun Gao, Juan Huang, Bin Tian, Sai Mao, Shaqiu Zhang, Xinxin Zhao, Renyong Jia, Mafeng Liu, Dekang Zhu, Shun Chen, Yunya Liu, Yanling Yu, Ling Zhang, and Leichang Pan

Subjects

Duck hepatitis A virus type 1, VP1, autophagy, PI3KC3, Beclin1, Veterinary medicine, SF600-1100

Abstract

Abstract Duck hepatitis A virus type 1 (DHAV-1) is one of the main pathogens responsible for death in ducklings. Autophagy is a catabolic process that maintains cellular homeostasis, and the PI3KC3 protein plays an important role in the initiation of autophagy. DHAV-1 infection induces autophagy in duck embryo fibroblasts (DEFs) but the molecular mechanism between it and autophagy has not been reported. First, we determined that DHAV-1 infection induces autophagy in DEFs and that autophagy induction is dependent on the integrity of viral proteins by infecting DEFs with UV-inactivated or heat-inactivated DHAV-1. Then, in experiments using the pharmacological autophagy inducer rapamycin and the autophagy inhibitor chloroquine, autophagy inhibition was shown to reduce intracellular and extracellular DHAV-1 genome copies and viral titres. These results suggest that autophagy activated by DHAV-1 infection in DEFs affects DHAV-1 proliferation and extracellular release. Next, we screened the autophagy-inducing effects of the DHAV-1 structural proteins VP0, VP3, and VP1 and found that all DHAV-1 structural proteins could induce autophagy in DEFs but not the full autophagic flux. Finally, we found that VP1 promotes protein expression of PI3KC3 and Beclin1 by western blot experiments and that VP1 interacts with PI3KC3 by co-immunoprecipitation experiments; moreover, 3-MA-induced knockdown of PI3KC3 inhibited VP1 protein-induced autophagy in DEFs. In conclusion, the DHAV-1 structural protein VP1 regulates the PI3KC3 complex by interacting with PI3KC3 to induce autophagy in DEFs.

Published

2022

5. BX795, a kinase inhibitor, inhibit duck plague virus infection via targeting US3 kinase

Author

Yanming Tian, Bin Tian, Mingshu Wang, Dongjie Cai, Anchun Cheng, Wei Zhang, Ying Wu, Qiao Yang, Xuming Ou, Di Sun, Shaqiu Zhang, Sai Mao, XinXin Zhao, Juan Huang, Qun Gao, Dekang Zhu, Renyong Jia, Shun Chen, and Mafeng Liu

Subjects

antiviral agent, BX795, duck plague virus, US3 kinase, Animal culture, SF1-1100

Abstract

ABSTRACT: Duck plague virus (DPV) is a typical DNA virus of waterfowl, it causes huge economic losses to the duck industry due to the higher mortality and lower egg production. The disease is one of the frequent epidemics and outbreaks on duck farms because present vaccines could not provide complete immunity and there are no specific antiviral drugs available. Therefore, the development of antiviral drugs is urgently needed. In this study, we evaluated the antiviral activity of BX795, a specific kinase inhibitor of 3-phosphoinositide-dependent kinase 1 (PDK1), protein kinase B (AKT) and Tank binding kinase 1 (TBK1), against DPV in different duck cells. Our study demonstrated that BX795 reveals prominent antiviral activity in a dose-dependent manner in different types of duck cells. Time-addition and antiviral duration analysis uncovered that BX795 inhibits viral infection therapeutically and its antiviral activity lasts longer than 96 h. Further studies have shown that BX795 prevents cell-to-cell spread of the DPV rather than affects other stage of viral life cycle. Mechanistically, BX795 can inhibit DPV US3 kinase activity, reduce the phosphorylation of US3 substrates, and prevent the interaction between US3 and UL47. Taking together, our study demonstrated BX795, which disrupts the viral kinase activity, is a candidate antiviral agent for DPV.

Published

2023

6. Multiple functions of heterogeneous nuclear ribonucleoproteins in the positive single-stranded RNA virus life cycle

Author

Jingming Wang, Di Sun, Mingshu Wang, Anchun Cheng, Yukun Zhu, Sai Mao, Xuming Ou, Xinxin Zhao, Juan Huang, Qun Gao, Shaqiu Zhang, Qiao Yang, Ying Wu, Dekang Zhu, Renyong Jia, Shun Chen, and Mafeng Liu

Subjects

host-pathogen interaction, positive single-stranded RNA virus, heterogeneous nuclear ribonucleoprotein, viral life cycle, immune response, Immunologic diseases. Allergy, RC581-607

Abstract

The heterogeneous nuclear ribonucleoproteins (hnRNPs) are a diverse family of RNA binding proteins that are implicated in RNA metabolism, such as alternative splicing, mRNA stabilization and translational regulation. According to their different cellular localization, hnRNPs display multiple functions. Most hnRNPs were predominantly located in the nucleus, but some of them could redistribute to the cytoplasm during virus infection. HnRNPs consist of different domains and motifs that enable these proteins to recognize predetermined nucleotide sequences. In the virus-host interactions, hnRNPs specifically bind to viral RNA or proteins. And some of the viral protein-hnRNP interactions require the viral RNA or other host factors as the intermediate. Through various mechanisms, hnRNPs could regulate viral translation, viral genome replication, the switch of translation to replication and virion release. This review highlights the common features and the distinguish roles of hnRNPs in the life cycle of positive single-stranded RNA viruses.

Published

2022

7. Evaluation of safety and immunogenicity of duck-plague virus gC/gE double gene deletion

Author

Peilin Ruan, Xin Feng, Anchun Cheng, Mingshu Wang, Wei Zhang, Ying Wu, Qiao Yang, Bin Tian, Xuming Ou, Di Sun, Shaqiu Zhang, Sai Mao, Dekang Zhu, Renyong Jia, Shun Chen, Mafeng Liu, Xin-Xin Zhao, Juan Huang, Qun Gao, Yanling Yu, Ling Zhang, and Leichang Pan

Subjects

duck plague, gC, gE, gene deletion, immunogenicity, vaccine, Immunologic diseases. Allergy, RC581-607

Abstract

Duck plague caused by duck plague virus (DPV) is a highly contagious disease that can cause serious morbidity and death in waterfowl such as ducks and geese, and bring huge economic losses to the duck industry. In this study, on the basis of the duck plague virus gC gene deletion strain CHv-ΔgC, based on the duck plague virus bacterial artificial chromosome (BAC) platform in our laboratory, the gE gene was knocked out using the traceless deletion technology to obtain gC/gE double gene deletion candidate vaccine strain CHv-ΔgC/gE. The double gene deletion strain (CHv-ΔgC/gE) constructed in this study has greatly weakened virulence, no pathogenicity to ducks, and stable genetic characteristics in vitro and in vivo. Ducks immunized with CHv-ΔgC/gE can produce neutralizing antibodies and ELISA antibody levels comparable to those of commercial duck plague attenuated vaccine immunization, and can resist 100 LD50 CHv challenge of ducks, with good immune protection effect. It has the potential to be further developed into duck plague gC/gE double gene deletion, marked attenuated vaccine.

Published

2022

8. Duck enteritis virus pUL47, as a late structural protein localized in the nucleus, mainly depends on residues 40 to 50 and 768 to 777 and inhibits IFN-β signalling by interacting with STAT1

Author

Tianqiong He, Mingshu Wang, Anchun Cheng, Qiao Yang, Renyong Jia, Ying Wu, Juan Huang, Shun Chen, Xin-Xin Zhao, Mafeng Liu, Dekang Zhu, Shaqiu Zhang, Xuming Ou, Sai Mao, Qun Gao, Di Sun, XinJian Wen, Bin Tian, Yunya Liu, Yanling Yu, Ling Zhang, Leichang Pan, and Xiaoyue Chen

Subjects

DEV, UL47, NLS, localization, IFN-β, STAT1, Veterinary medicine, SF600-1100

Abstract

Abstract Duck enteritis virus (DEV) is a member of the Alphaherpesvirinae subfamily. The characteristics of some DEV genes have been reported. However, information regarding the DEV UL47 gene is limited. In this study, we identified the DEV UL47 gene encoding a late structural protein located in the nucleus of infected cells. We further found that two domains of DEV pUL47, amino acids (aa) 40 to 50 and 768 to 777, could function as nuclear localization sequence (NLS) to guide the nuclear localization of pUL47 and nuclear translocation of heterologous proteins, including enhanced green fluorescent protein (EGFP) and beta-galactosidase (β-Gal). Moreover, pUL47 significantly inhibited polyriboinosinic:polyribocytidylic acid [poly(I:C)]-induced interferon beta (IFN-β) production and downregulated interferon-stimulated gene (ISG) expression, such as Mx and oligoadenylate synthetase-like (OASL), by interacting with signal transducer and activator of transcription-1 (STAT1).

Published

2020

9. Host shutoff activity of VHS and SOX-like proteins: role in viral survival and immune evasion

Author

Tianqiong He, Mingshu Wang, Anchun Cheng, Qiao Yang, Ying Wu, Renyong Jia, Mafeng Liu, Dekang Zhu, Shun Chen, Shaqiu Zhang, Xin-Xin Zhao, Juan Huang, Di Sun, Sai Mao, Xuming Ou, Yin Wang, Zhiwen Xu, Zhengli Chen, Lin Zhu, Qihui Luo, Yunya Liu, Yanling Yu, Ling Zhang, Bin Tian, Leichang Pan, Mujeeb Ur Rehman, and Xiaoyue Chen

Subjects

Herpesvirus, Host shutoff, VHS, ICP27, SOX, mRNA, Infectious and parasitic diseases, RC109-216

Abstract

Abstract Background Host shutoff refers to the widespread downregulation of host gene expression and has emerged as a key process that facilitates the reallocation of cellular resources for viral replication and evasion of host antiviral immune responses. Main body The Herpesviridae family uses a number of proteins that are responsible for host shutoff by directly targeting messenger RNA (mRNA), including virion host shutoff (VHS) protein and the immediate-early regulatory protein ICP27 of herpes simplex virus types 1 (HSV-1) and the SOX (shutoff and exonuclease) protein and its homologs in Gammaherpesvirinae subfamilies, although these proteins are not homologous. In this review, we highlight evidence that host shutoff is promoted by the VHS, ICP27 and SOX-like proteins and that they also contribute to immune evasion. Conclusions Further studies regarding the host shutoff proteins will not only contribute to provide new insights into the viral replication, expression and host immune evasion process, but also provide new molecular targets for the development of antiviral drugs and therapies.

Published

2020

10. Alphaherpesvirus Major Tegument Protein VP22: Its Precise Function in the Viral Life Cycle

Author

Liping Wu, Anchun Cheng, Mingshu Wang, Renyong Jia, Qiao Yang, Ying Wu, Dekang Zhu, Xinxin Zhao, Shun Chen, Mafeng Liu, Shaqiu Zhang, Xuming Ou, Sai Mao, Qun Gao, Di Sun, Xinjian Wen, Yunya Liu, Yanling Yu, Ling Zhang, Bin Tian, Leichang Pan, and Xiaoyue Chen

Subjects

alphaherpesvirus, tegument protein VP22, secondary envelopment, viral replication, immune evasion, Microbiology, QR1-502

Abstract

Alphaherpesviruses are zoonotic pathogens that can cause a variety of diseases in humans and animals and severely damage health. Alphaherpesvirus infection is a slow and orderly process that can lie dormant for the lifetime of the host but may be reactivated when the immune system is compromised. All alphaherpesviruses feature a protein layer called the tegument that lies between the capsid and the envelope. Virus protein (VP) 22 is one of the most highly expressed tegument proteins; there are more than 2,000 copies of this protein in each viral particle. VP22 can interact with viral proteins, cellular proteins, and chromatin, and these interactions play important roles. This review summarizes the latest literature and discusses the roles of VP22 in viral gene transcription, protein synthesis, virion assembly, and viral cell-to-cell spread with the purpose of enhancing understanding of the life cycle of herpesviruses and other pathogens in host cells. The molecular interaction information herein provides important reference data.

Published

2020

11. Duck enteritis virus pUL47, as a late structural protein localized in the nucleus, mainly depends on residues 40 to 50 and 768 to 777 and inhibits IFN-β signalling by interacting with STAT1

Author

Xiaoyue Chen, Shun Chen, Shaqiu Zhang, Mingshu Wang, Renyong Jia, Xinxin Zhao, Leichang Pan, Yunya Liu, Yanling Yu, Dekang Zhu, Ling Zhang, Anchun Cheng, Qun Gao, Ying Wu, Bin Tian, Di Sun, Qiao Yang, Mafeng Liu, Sai Mao, Xinjian Wen, Tianqiong He, Juan Huang, and Xuming Ou

Subjects

0301 basic medicine, animal structures, [SDV]Life Sciences [q-bio], 030106 microbiology, Heterologous, NLS, localization, Green fluorescent protein, 03 medical and health sciences, STAT1, Alphaherpesvirinae, Marek Disease, Animals, UL47, Gene, Poultry Diseases, IFN-β, chemistry.chemical_classification, Cell Nucleus, Viral Structural Proteins, lcsh:Veterinary medicine, General Veterinary, biology, Activator (genetics), DEV, Interferon-beta, biology.organism_classification, Molecular biology, 3. Good health, Amino acid, Mardivirus, 030104 developmental biology, Ducks, STAT1 Transcription Factor, chemistry, embryonic structures, biology.protein, lcsh:SF600-1100, Nuclear localization sequence, Signal Transduction, Research Article

Abstract

Duck enteritis virus (DEV) is a member of the Alphaherpesvirinae subfamily. The characteristics of some DEV genes have been reported. However, information regarding the DEV UL47 gene is limited. In this study, we identified the DEV UL47 gene encoding a late structural protein located in the nucleus of infected cells. We further found that two domains of DEV pUL47, amino acids (aa) 40 to 50 and 768 to 777, could function as nuclear localization sequence (NLS) to guide the nuclear localization of pUL47 and nuclear translocation of heterologous proteins, including enhanced green fluorescent protein (EGFP) and beta-galactosidase (β-Gal). Moreover, pUL47 significantly inhibited polyriboinosinic:polyribocytidylic acid [poly(I:C)]-induced interferon beta (IFN-β) production and downregulated interferon-stimulated gene (ISG) expression, such as Mx and oligoadenylate synthetase-like (OASL), by interacting with signal transducer and activator of transcription-1 (STAT1).

Published

2020

12. Host shutoff activity of VHS and SOX-like proteins: role in viral survival and immune evasion

Author

Lin Zhu, Xuming Ou, Bin Tian, Di Sun, Yanling Yu, Leichang Pan, Anchun Cheng, Dekang Zhu, Renyong Jia, Zhiwen Xu, Yunya Liu, Xiaoyue Chen, Zhengli Chen, Qihui Luo, Ling Zhang, Qiao Yang, Mafeng Liu, Xinxin Zhao, Ying Wu, Shaqiu Zhang, Sai Mao, Shun Chen, Tianqiong He, Juan Huang, Yin Wang, Mingshu Wang, and Mujeeb Ur Rehman

Subjects

ICP27, 0301 basic medicine, mRNA, viruses, 030106 microbiology, Gene Expression, Host shutoff, Herpesvirus 1, Human, Review, Virus Replication, medicine.disease_cause, Herpesviridae, lcsh:Infectious and parasitic diseases, Cell Line, Immediate-Early Proteins, Viral Proteins, 03 medical and health sciences, Ribonucleases, Immune system, Downregulation and upregulation, Virology, Chlorocebus aethiops, medicine, Animals, Gammaherpesvirinae, lcsh:RC109-216, VHS, Vero Cells, Regulation of gene expression, Messenger RNA, Host Microbial Interactions, biology, Immune evasion, Virion, Herpesvirus, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, 030104 developmental biology, Infectious Diseases, Herpes simplex virus, Viral replication, SOX

Abstract

Background Host shutoff refers to the widespread downregulation of host gene expression and has emerged as a key process that facilitates the reallocation of cellular resources for viral replication and evasion of host antiviral immune responses. Main body The Herpesviridae family uses a number of proteins that are responsible for host shutoff by directly targeting messenger RNA (mRNA), including virion host shutoff (VHS) protein and the immediate-early regulatory protein ICP27 of herpes simplex virus types 1 (HSV-1) and the SOX (shutoff and exonuclease) protein and its homologs in Gammaherpesvirinae subfamilies, although these proteins are not homologous. In this review, we highlight evidence that host shutoff is promoted by the VHS, ICP27 and SOX-like proteins and that they also contribute to immune evasion. Conclusions Further studies regarding the host shutoff proteins will not only contribute to provide new insights into the viral replication, expression and host immune evasion process, but also provide new molecular targets for the development of antiviral drugs and therapies.

Published

2020

13. DPV UL41 gene encoding protein induces host shutoff activity and affects viral replication

Author

Ying Wu, Shun Chen, Mingshu Wang, Renyong Jia, Shaqiu Zhang, Qun Gao, Di Sun, Tianqiong He, Juan Huang, Anchun Cheng, Xuming Ou, Qiao Yang, Dekang Zhu, Mafeng Liu, Sai Mao, Bin Tian, and Xinxin Zhao

Subjects

Gene Expression Regulation, Viral, viruses, Alphaherpesvirinae, Biology, Virus Replication, medicine.disease_cause, Microbiology, Gene Expression Regulation, Enzymologic, Virus, Viral Proteins, 03 medical and health sciences, chemistry.chemical_compound, Ribonucleases, RNA polymerase, medicine, Protein biosynthesis, Animals, Gene, Cells, Cultured, Virus Release, 030304 developmental biology, 0303 health sciences, Messenger RNA, General Veterinary, Bird Diseases, 030306 microbiology, RNA, Herpesviridae Infections, General Medicine, Fibroblasts, Virology, Ducks, Herpes simplex virus, Viral replication, chemistry, Gene Deletion

Abstract

The virion host shutoff (VHS) protein, encoded by the UL41 gene of herpes simplex virus (HSV), specifically degrades mRNA and induces host shutoff. VHS and its homologs are highly conserved in the Alphaherpesvirinae subfamily. However, the role of the duck plague virus (DPV) UL41 gene is unclear. In this study, we found that the DPV UL41 gene-encoded protein (pUL41) degrades RNA polymerase (pol) II-transcribed translatable RNA and induces protein synthesis shutoff. DPV pUL41 was dispensable for viral replication, but the UL41-deleted mutant virus exhibited a significant viral growth defect and plaque size reduction in Duck embryo fibroblast (DEF) cells. Furthermore, DPV pUL41 regulated viral mRNA accumulation to affect viral DNA replication, release and cell-to-cell spread.

Published

2021

14. Outbreak of Avian Tuberculosis in Commercial Domestic Pekin Ducks (Anas platyrhynchos domestica)

Author

Shun Chen, Jiang-Bo Wang, Renyong Jia, Xiaoyue Chen, Anchun Cheng, Kunfeng Sun, Mingshu Wang, Qiao Yang, Ying Wu, Hong-Xi Chen, Xuming Ou, Xiao-Heng Song, Wang-Shu Zhou, Mafeng Liu, and Dekang Zhu

Subjects

0301 basic medicine, Anas, China, animal structures, 040301 veterinary sciences, animal diseases, Pekin duck, biology.animal_breed, Caseous necrosis, Disease Outbreaks, 0403 veterinary science, 03 medical and health sciences, Food Animals, RNA, Ribosomal, 16S, medicine, Animals, Pathogen, Poultry Diseases, General Immunology and Microbiology, biology, Tuberculosis, Avian, Outbreak, Sequence Analysis, DNA, 04 agricultural and veterinary sciences, biology.organism_classification, medicine.disease, Virology, Ducks, 030104 developmental biology, DNA Transposable Elements, Animal Science and Zoology, Flock, Mycobacterium avium, Mycobacterium, Avian tuberculosis

Abstract

SUMMARY Avian tuberculosis is a contagious disease affecting various domestic and wild bird species, and is caused by Mycobacterium avium. It is reported extremely rarely in commercial poultry flocks and has not been reported in commercial domestic ducks to date, with domestic ducks reported to be moderately resistant to M. avium infection. Here, we report the outbreak of avian tuberculosis in commercial Pekin duck (Anas platyrhynchos domestica) flocks. Postmortem and histopathologic findings included nodules presenting in the visceral organs of ducks, and granulomas with central caseous necrosis surrounded by infiltrating lymphocytes. The M. avium pathogen was isolated and further identified by Ziehl-Neelsen staining and PCR based on insert sequence IS901 and the 16S rRNA gene. We highlight that avian tuberculosis not only has economic significance for the duck industry, but also presents a potential zoonotic hazard to humans.

Published

2016