Your search keyword '"Avian Leukosis Virus classification"' showing total 174 results

1. Specific and Sensitive Visual Proviral DNA Detection of Major Pathogenic Avian Leukosis Virus Subgroups Using CRISPR-Associated Nuclease Cas13a.

Author

Xu Q, Zhang Y, Sadigh Y, Tang N, Chai J, Cheng Z, Gao Y, Qin A, Shen Z, Yao Y, and Nair V

Subjects

Animals, Poultry Diseases virology, Poultry Diseases diagnosis, Chickens virology, Sensitivity and Specificity, CRISPR-Associated Proteins genetics, CRISPR-Associated Proteins metabolism, Avian Leukosis Virus genetics, Avian Leukosis Virus isolation & purification, Avian Leukosis Virus classification, Proviruses genetics, Proviruses isolation & purification, Avian Leukosis virology, Avian Leukosis diagnosis, CRISPR-Cas Systems, DNA, Viral genetics

Abstract

Avian leukosis viruses (ALVs) include a group of avian retroviruses primarily associated with neoplastic diseases in poultry, commonly referred to as avian leukosis. Belonging to different subgroups based on their envelope properties, ALV subgroups A, B, and J (ALV-A, ALV-B, and ALV-J) are the most widespread in poultry populations. Early identification and removal of virus-shedding birds from infected flocks are essential for the ALVs' eradication. Therefore, the development of rapid, accurate, simple-to-use, and cost effective on-site diagnostic methods for the detection of ALV subgroups is very important. Cas13a, an RNA-guided RNA endonuclease that cleaves target single-stranded RNA, also exhibits non-specific endonuclease activity on any bystander RNA in close proximity. The distinct trans-cleavage activity of Cas13 has been exploited in the molecular diagnosis of multiple pathogens including several viruses. Here, we describe the development and application of a highly sensitive Cas13a-based molecular test for the specific detection of proviral DNA of ALV-A, B, and J subgroups. Prokaryotically expressed LwaCas13a, purified through ion exchange and size-exclusion chromatography, was combined with recombinase polymerase amplification (RPA) and T7 transcription to establish the SHERLOCK (specific high-sensitivity enzymatic reporter unlocking) molecular detection system for the detection of proviral DNA of ALV-A/B/J subgroups. This novel method that needs less sample input with a short turnaround time is based on isothermal detection at 37 °C with a color-based lateral flow readout. The detection limit of the assay for ALV-A/B/J subgroups was 50 copies with no cross reactivity with ALV-C/D/E subgroups and other avian oncogenic viruses such as reticuloendotheliosis virus (REV) and Marek's disease virus (MDV). The development and evaluation of a highly sensitive and specific visual method of detection of ALV-A/B/J nucleic acids using CRISPR-Cas13a described here will help in ALV detection in eradication programs.

Published

2024

2. Recombination of variable and host range regions of glycoprotein gp85 in different avian leukosis virus subgroup K isolates.

Author

Li X, Wang Y, Li J, Yu Z, Wei Y, Chen S, He L, Ding K, and Chen J

Subjects

Animals, China, Avian Leukosis Virus genetics, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, Chickens virology, Phylogeny, Avian Leukosis virology, Viral Envelope Proteins genetics, Viral Envelope Proteins metabolism, Poultry Diseases virology, Host Specificity, Recombination, Genetic

Abstract

Given the high prevalence of avian leukosis virus subgroup K (ALV-K) in chickens in China, the positive rate of ALV-K in local chickens in Henan province was investigated, and the genetic region encoding the glycoprotein gp85 of isolates from positive chickens was analyzed. The positive rate of ALV-K in local chickens in Henan was found to be 87.2% (41/47). Phylogenetic analysis of gp85 sequences revealed six clusters that differed in their host range regions (hr1 and hr2) and variable regions (vr1, vr2, and vr3). Evidence of recombination of hr1, hr2, vr1, vr2, and vr3 was observed between the different clusters. The isolate HN23LS02 appears to have obtained its hr1 and hr2 regions from separate lineages via recombination but without having a significant affect on the replication capacity of the virus., (© 2024. The Author(s), under exclusive licence to Springer-Verlag GmbH Austria, part of Springer Nature.)

Published

2024

3. Anti-CD81 antibody blocks vertical transmission of avian leukosis virus subgroup J.

Author

Liao L, Wu Z, Chen W, Zhang H, Li A, Yan Y, Xie Z, Li H, Lin W, Ma J, Zhang X, and Xie Q

Subjects

Animals, Chickens, Infectious Disease Transmission, Vertical, Tetraspanin 28 immunology, Antibodies metabolism, Avian Leukosis prevention & control, Avian Leukosis transmission, Avian Leukosis virology, Avian Leukosis Virus classification, Poultry Diseases prevention & control, Poultry Diseases transmission, Poultry Diseases virology

Abstract

Control of ALV-J in breed of chicken is still a serious issue that need more attention to be paid. Vertical transmission of ALV-J often give rise to more adverse pathogenicity. However, the way to elimination of ALV-J underlying vertical transmission remains not-well understood. In addition, effective vaccines or drugs have not been developed to prevent and control the transmission of ALV-J so far. CD81, a member of the tetraspanins superfamily, plays important roles in regulating membrane proteins, facilitating cells adhesion or fusion, and also participates in viral infection. The purpose of this study was to investigate whether antibodies against certain tetraspanins affect infection of ALV-J. Here, we showed that anti-CD81 antibody could inhibit viral RNA and protein level. We also found that anti-CD81 antibody interacts with viral protein p27, p32 and gp37. Moreover, treatment with antibody to CD81 can effectively prevent the vertical transmission of ALV-J in animal model. Collectively, current study provides new avenues for the control of ALV-J transmission., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2022

4. Knock-Out of Retrovirus Receptor Gene Tva in the Chicken Confers Resistance to Avian Leukosis Virus Subgroups A and K and Affects Cobalamin (Vitamin B 12 )-Dependent Level of Methylmalonic Acid.

Author

Koslová A, Trefil P, Mucksová J, Krchlíková V, Plachý J, Krijt J, Reinišová M, Kučerová D, Geryk J, Kalina J, Šenigl F, Elleder D, Kožich V, and Hejnar J

Subjects

Animals, Avian Leukosis Virus classification, Avian Proteins genetics, Chick Embryo, Female, Frameshift Mutation, Gene Editing, Gene Knockout Techniques, Male, Methylmalonic Acid blood, Receptors, Virus genetics, Avian Leukosis Virus physiology, Avian Proteins physiology, Chickens virology, Receptors, Virus physiology, Vitamin B 12 metabolism

Abstract

The chicken Tva cell surface protein, a member of the low-density lipoprotein receptor family, has been identified as an entry receptor for avian leukosis virus of classic subgroup A and newly emerging subgroup K. Because both viruses represent an important concern for the poultry industry, we introduced a frame-shifting deletion into the chicken tva locus with the aim of knocking-out Tva expression and creating a virus-resistant chicken line. The tva knock-out was prepared by CRISPR/Cas9 gene editing in chicken primordial germ cells and orthotopic transplantation of edited cells into the testes of sterilized recipient roosters. The resulting tva -/- chickens tested fully resistant to avian leukosis virus subgroups A and K, both in in vitro and in vivo assays, in contrast to their susceptible tva +/+ and tva +/- siblings. We also found a specific disorder of the cobalamin/vitamin B 12 metabolism in the tva knock-out chickens, which is in accordance with the recently recognized physiological function of Tva as a receptor for cobalamin in complex with transcobalamin transporter. Last but not least, we bring a new example of the de novo resistance created by CRISPR/Cas9 editing of pathogen dependence genes in farm animals and, furthermore, a new example of gene editing in chicken.

Published

2021

5. Avian leukosis virus subgroup J infection alters viral composition in the chicken gut.

Author

Chen Y, Li HW, Cong F, and Lian YX

Subjects

Animals, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Avian Leukosis Virus isolation & purification, Chickens virology, Feces virology, Female, Male, Virome, Viruses classification, Viruses genetics, Viruses isolation & purification, Avian Leukosis virology, Avian Leukosis Virus physiology, Gastrointestinal Tract virology, Poultry Diseases virology

Abstract

Chicken is one of the economically important poultry species. Avian leucosis virus subgroup J (ALV-J) has emerged as a serious cause of mortality and suboptimal performance of domestic chickens. Changes in virome may contribute to pathogenesis. Thus, it is important to investigate the effects of ALV-J infection on the composition of the virome in chicken. In the study metagenomic sequencing was used to characterize the virome of feces collected from the AVL-J infected chickens and the controls. Our results indicated that the chicken gut virome contained a diverse range of viruses that can be found in mammal, reptile, fish, and frogs. Furthermore, at the order, family and genus levels, AVL-J infection significantly altered the chicken gut virome composition. The predominant order was Herpesvirales, accounting for more than 96% of the chicken gut virome. Furthermore, the relative abundance of Caudovirales in the controls was higher than that in the AVL-J-infected chickens. At the family level, the relative abundance of Herpesviridae, Myoviridae, Alloherpesviridae, and Genomoviridae was significantly altered in the AVL-J-infected chickens compared with that in the controls. Additionally, the relative abundance of 15 genera showed a significant difference between the AVL-J-infected chickens and controls. These results will increase our understanding of the viral diversity and changes in the virome of chicken gut, with implications in chicken health., (© The Author(s) 2021. Published by Oxford University Press on behalf of FEMS.)

Published

2021

6. Pathologic Characterization of Coinfection with Histomonas meleagridis , Marek's Disease Virus, and Subtype J Avian Leukosis Virus in Chickens.

Author

Li M, Xiong H, Wu H, Hu D, Lin Y, Huang X, Wang J, Qi K, and Liu H

Subjects

Animals, Avian Leukosis pathology, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, Communicable Diseases, Emerging complications, Communicable Diseases, Emerging pathology, Communicable Diseases, Emerging veterinary, Liver pathology, Liver virology, Mardivirus classification, Mardivirus isolation & purification, Marek Disease pathology, Phylogeny, Poultry Diseases pathology, Protozoan Infections pathology, Spleen pathology, Spleen virology, Trichomonadida classification, Trichomonadida isolation & purification, Avian Leukosis complications, Chickens, Marek Disease complications, Poultry Diseases virology, Protozoan Infections complications

Abstract

Histomonas meleagridis is a trichomonad protozoan parasite that can cause an important poultry disease known as histomoniasis; Marek's disease virus (MDV) and subtype J avian leukosis virus (ALV-J) usually cause avian oncogenic diseases. Although these diseases have been reported in a single pathogen infection, information about their coinfection is scarce. This study reports a naturally occurring case of coinfection with H. meleagridis , MDV, and ALV-J in a local chicken flock at the age of 150 days. Necropsy revealed necrosis and swelling in the liver and spleen. Histologic analysis showed large areas of mild to severe necrosis of hepatocytes, with numerous intralesional trophozoites of H. meleagridis by H&E and periodic acid-Schiff staining; H&E staining showed pleomorphic and neoplastic lymphoid tumor cells in the liver and myeloid cells with eosinophilic cytoplasmic granules in the spleen. Coexpression of MDV and ALV-J antigens was detected in the liver by fluorescence multiplex immunohistochemistry staining. The 18S rRNA gene of H. meleagridis , meq gene of MDV, and gp85 gene of ALV-J were identified in mixed liver and spleen tissues by PCR and sequencing, respectively.

Published

2021

7. Rapid detection of avian leukosis virus subgroup J by cross-priming amplification.

Author

Xiang Y, Li L, Liu P, Yan L, Jiang Z, Yu Y, Li Y, Chen X, and Cao W

Subjects

Animals, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Biotinylation, Cells, Cultured, Chickens virology, DNA Primers, Electrophoresis, Agar Gel, Fluorescein-5-isothiocyanate analysis, Gold, Metal Nanoparticles, Polymerase Chain Reaction methods, Poultry Diseases diagnosis, Poultry Diseases virology, RNA, Viral genetics, Reagent Strips, Real-Time Polymerase Chain Reaction, Sensitivity and Specificity, Temperature, Tumor Virus Infections diagnosis, Tumor Virus Infections veterinary, Tumor Virus Infections virology, Viremia diagnosis, Viremia veterinary, Viremia virology, Avian Leukosis Virus isolation & purification, Nucleic Acid Amplification Techniques methods

Abstract

Avian leukosis virus subgroup J (ALV-J) causes oncogenic disease in chickens in China, resulting in great harm to poultry production, and remains widespread in China. Herein, we employed a cross-priming amplification (CPA) approach and a nucleic acid detection device to establish a visual rapid detection method for ALV-J. The sensitivity of CPA, polymerase chain reaction (PCR) and real-time PCR (RT-PCR) was compared, and the three methods were used to detect ALV-J in the cell cultures which inoculated with clinical plasma. The result showed when the amplification reaction was carried out at 60 °C for just 60 min, the sensitivity of CPA was 10 times higher than conventional PCR, with high specificity, which was comparable with RT-PCR, based on detection of 123 cell cultures which inoculated with clinical plasma, the coincidence rate with real-time PCR was 97.3% (71/73). CPA detection of ALV-J does not require an expensive PCR instrument; a simple water bath or incubator is sufficient for complete DNA amplification, and the closed nucleic acid detection device avoids aerosol pollution, making judgment of results more intuitive and objective. The CPA assay would be a promising simple, rapid and sensitive method for identification of ALV-J.

Published

2021

8. Molecular characteristics of subgroup J avian leukosis virus isolated from yellow breeder chickens in Guangdong, China, during 2016-2019.

Author

Liu P, Li L, Jiang Z, Yu Y, Chen X, Xiang Y, Chen J, Li Y, and Cao W

Subjects

3' Untranslated Regions, Amino Acid Sequence, Animals, Avian Leukosis Virus chemistry, Avian Leukosis Virus classification, China, DNA, Viral genetics, Genes, Viral, Genetic Variation, Phylogeny, Poultry Diseases prevention & control, Poultry Diseases virology, Transcription Factors metabolism, Whole Genome Sequencing, Avian Leukosis Virus genetics, Chickens genetics, Chickens virology

Abstract

Since 2005, subgroup J avian leukosis virus (ALV-J) infection has been present in yellow chickens in Guangdong, China, causing severe economic losses to the local poultry industry. ALV-J is a rapidly evolving retrovirus. To investigate the molecular characteristics of ALV-J isolates from yellow breeder chickens in Guangdong, 17 virus strains were isolated from 6549 anticoagulants from clinically healthy birds between 2016 and 2019, and completely sequenced and phylogenetically analyzed. Phylogenetic analysis of the gp85 gene showed that all isolated viruses were divided into three different branches. Notably, 41.2% (7/17) of the isolates shared a novel G2598A nucleotide mutation in the pol gene and caused the stop codon to be advanced by 8 positions. Nearly 200 nucleotides were deleted from the redundant TM (rTM) region in all strains, but all retained an intact direct repeat (DR1). 82.4% (14/17) of isolates contained a complete E element. Additionally, 29.4% (5/17) of isolates detected an 11 bp deletion in U3 region, and the AIB REP1 transcription factor is missing. The study indicated that ALV-J infection had still been prevalent in the yellow breeder chicken farms in Guangdong, and the genetic background of the strains is diverse. This study provides the latest data on the molecular characteristics of ALV-J, which will help to reveal the evolution trend of ALV-J and develop relevant prevention and control measures., (Copyright © 2021 The Author(s). Published by Elsevier B.V. All rights reserved.)

Published

2021

9. Phylogenetic Analysis of ALV-J Associated with Immune Responses in Yellow Chicken Flocks in South China.

Author

Zhang Q, Mo G, Xie T, Zhang Z, Fu H, Wei P, and Zhang X

Subjects

Animals, Avian Leukosis Virus classification, China, Enzyme-Linked Immunosorbent Assay, Interleukin-10 metabolism, Interleukin-4 metabolism, Interleukin-6 metabolism, Phylogeny, Avian Leukosis Virus pathogenicity, Chickens immunology, Chickens virology

Abstract

The aim of this study was to better understand the sequence characteristics and immune responses in avian leukosis virus subgroup J (ALV-J) infected yellow chicken flocks in South China. We isolated four strains of ALV-J virus from these flocks, which were then identified by several methods, including subtype-specific polymerase chain reaction (PCR), enzyme-linked immunosorbent assay (ELISA), and immunofluorescence assay (IFA). All four viruses were sequenced for their complete genomes and named GD19GZ01, GD19GZ02, GD19GZ03, and GD19GZ04. In comparison with the reference sequence, the homology analysis showed that the gag and pol genes were relatively conserved, whereas env contained much variation. Both GD19GZ01 and GD19GZ02 almost entirely lacked the rTM region and E element, while the latter was retained in GD19GZ03 and GD19GZ04. Moreover, the virus replication levels in GD19GZ03 and GD19GZ04were much higher than those in GD19GZ01 and GD19GZ02. And three virus recombination events in GD19GZ01 and GD19GZ02 were revealed by the results of PDR5 and SimPlot software analysis. Additionally, we found that some interferon-stimulating genes ( CH25H , MX , PKR , OAS , and ZAP ) and inflammatory mediators ( IL-4 , IL-6 , IL-10 , IL-12 , 1L-18 , and TNF-α ) were significantly upregulated in the immune system organs of clinical chickens. Taken together, these findings clarify and reveal the sequence characteristics and trends in the variation of ALV-J infection in yellow chicken flocks of South China., Competing Interests: The authors declare no conflict of interest., (Copyright © 2021 Qihong Zhang et al.)

Published

2021

10. Regulatory effects of chicken TRIM25 on the replication of ALV-A and the MDA5-mediated type I interferon response.

Author

Zhou JR, Liu JH, Li HM, Zhao Y, Cheng Z, Hou YM, and Guo HJ

Subjects

Animals, Avian Leukosis Virus classification, Cell Line, Gene Expression Regulation immunology, Gene Knockdown Techniques, Interferon-Induced Helicase, IFIH1 genetics, Interferon-beta genetics, Interferon-beta metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Transcription Factors genetics, Tripartite Motif Proteins genetics, Ubiquitin-Protein Ligases genetics, Up-Regulation, Virus Replication, Avian Leukosis Virus physiology, Chickens, Interferon-Induced Helicase, IFIH1 metabolism, Transcription Factors metabolism, Tripartite Motif Proteins metabolism, Ubiquitin-Protein Ligases metabolism

Abstract

This study focuses on the immunoregulatory effects of chicken TRIM25 on the replication of subgroup A of avian leukosis virus (ALV-A) and the MDA5-mediated type I interferon response. The ALV-A-SDAU09C1 strain was inoculated into DF1 cells and 1-day-old SPF chickens, and the expression of TRIM25 was detected at different time points after inoculation. A recombinant overexpression plasmid containing the chicken TRIM25 gene (TRIM25-GFP) was constructed and transfected into DF1 cells to analyse the effects of the overexpression of chicken TRIM25 on the replication of ALV-A and the expression of MDA5, MAVS and IFN-β. A small interfering RNA targeting chicken TRIM25 (TRIM25-siRNA) was prepared and transfected into DF1 cells to assess the effects of the knockdown of chicken TRIM25 on the replication of ALV-A and the expression of MDA5, MAVS and IFN-β. The results showed that chicken TRIM25 was significantly upregulated at all time points both in ALV-A-infected cells and in ALV-A-infected chickens. Overexpression of chicken TRIM25 in DF1 cells dramatically decreased the antigenic titres of ALV-A in the cell supernatant and upregulated the relative expression of MDA5, MAVS and IFN-β induced by ALV-A or by poly(I:C); in contrast, knockdown of chicken TRIM25 significantly increased the antigenic titres of ALV-A and downregulated the relative expression of MDA5, MAVS and IFN-β. It can be concluded that chicken TRIM25 can inhibit the replication of ALV-A and upregulate the MDA5 receptor-mediated type I interferon response in chickens. This study can help improve the understanding of the antiviral activities of chicken TRIM25 and enrich the knowledge of antiviral responses in chickens.

Published

2020

11. Identification of a novel epitope specific for Gp85 protein of avian leukosis virus subgroup K.

Author

Chen X, Wang H, Fang X, Gao K, Fang C, Gu Y, Gao Y, Wang X, Huang H, Liang X, and Yang Y

Subjects

Animals, Antibodies, Monoclonal isolation & purification, Antibodies, Viral immunology, Avian Leukosis diagnosis, Avian Leukosis Virus classification, Chickens, China, Epitopes isolation & purification, Poultry Diseases immunology, Antibodies, Monoclonal immunology, Avian Leukosis immunology, Avian Leukosis Virus immunology, Epitopes genetics, Epitopes immunology, Membrane Glycoproteins immunology, Poultry Diseases virology

Abstract

During the past two decades, avian leukosis virus (ALV) caused tremendous economic losses to poultry industry in China. ALV-K as a newly found subgroup in recent years, which made the control and eradication of ALV more difficult as they were originated from the recombination of different subgroups. To date, specific rapid detection methods refer to ALV-K are still missing. Gp85 is the main structural protein of the virus, which mediates the invasion of host cells by the virus and determinates the classification of subgroups. In this study, we prepared a monoclonal antibody (Mab) named Km3 against Gp85 of ALV-K. Immunofluorescence assay showed that Km3 specifically recognized the strains of ALV-K rather than the strains of ALV-A or ALV-J. To explain the subgroups specificity of Km3, the epitope cognized by the Mab was identified by Western blotting using 15 overlapping fragments spanning the Gp85. Finally, the peptide 129 AFGPRSIDTLSDWSRPQ 145 was identified as the minimal linear epitope recognized by Km3. Alignment of Gp85 from different subgroups showed that the epitope was highly conserved among ALV-K strains, which was quite different from that of the strains from ALV -A, -B and -J. In conclusion, the Mab Km3 may serve as a useful reagent for ALV-K detection and diagnosis in the future., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2020

12. Screening of immune biomarkers in different breeds of chickens infected with J subgroup of avian leukemia virus by proteomic.

Author

Ye F, Wang Y, He Q, Wang Z, Ma E, Zhu S, Yu H, Yin H, Zhao X, Li D, Xu H, Li H, and Zhu Q

Subjects

Animals, Avian Leukosis diagnosis, Avian Leukosis Virus classification, Biomarkers analysis, Breeding, Chickens classification, Female, Poultry Diseases virology, Avian Leukosis immunology, Avian Leukosis Virus immunology, Chickens virology, Poultry Diseases immunology, Proteomics

Abstract

Avian leucosis (AL) is a disease characterized by tumors and is caused by the avian leukosis virus (ALV). Because of the high variability of viruses and complex pathogenic mechanisms, screening and breeding J subgroup of ALV (ALV-J) resistant avian breeds is one of the strategies for prevention and treatment of AL, thus screening of significant immune markers is needed to promote the development of disease-resistant breeds. In this study, data-independent acquisition (DIA) technology was used to detect the DEPs of three breeds of chicken according to different comparison to investigate the potential markers. Results showed special DEPs for spleen development of each breed were detected, such as PCNT, DDB2, and ZNF62. These DEPs were involved in intestinal immune network used in production of IgA signaling pathways and related to immune response which can be used as potential markers for spleen development in different breeds. The DEPs such as RAB44 and TPN involved in viral myocarditis, transcriptional misregulation in cancer, and tuberculosis can be used as potential markers of spleen immune response after ALV-J infection in chickens. Pair-wise analysis was performed for the three breeds after the infection of ALV-J. The proteins such as RFX1, TAF10, and VH1 were differently expressed between three breeds. These DEPs involved in antigen processing and expression, acute myelogenous leukemia, and viral carcinogenesis can be used as potential immune markers after ALV-J infection of different genetic backgrounds. The screening of potential markers at protein level provides a strong theoretical research basis for disease resistance breeding in poultry.

Published

2020

13. Isolation and molecular characterization of the first subgroup J avian leukosis virus from chicken in Pakistan.

Author

Farooque M, Li X, Hussain A, Fayyaz A, Bao Y, Xing L, Yu M, Chang F, Wang S, Liu P, Chen Y, Pan Q, Qi X, Gao L, Li K, Liu C, Zhang Y, Cui H, Wang X, and Gao Y

Subjects

3' Untranslated Regions, Animals, Avian Leukosis pathology, Avian Leukosis Virus isolation & purification, Cell Line, Chickens virology, DNA, Viral, Molecular Epidemiology, Pakistan epidemiology, Phylogeny, Poultry Diseases virology, Sequence Analysis, DNA, Viral Envelope Proteins genetics, Whole Genome Sequencing, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus genetics

Abstract

Since subgroup J avian leukosis virus (ALV-J) was first isolated in the United Kingdom in 1988, it has seriously hindered the development of the poultry industry worldwide. Although cases of ALV-J infection have been reported as early as 2001 in Pakistan, there was no further research on the isolation and molecular characteristics of ALVs. In the present study, we first isolated two ALVs from suspicious clinical samples that were collected from a desi chicken farm in Pakistan. The results of multiplex PCR and indirect immunofluorescent antibody assays confirmed that the two isolates (PK19FA01 and PK19SA01) belonged to ALV-J. The complete genomes of the two isolates were amplified, sequenced, and systematically analyzed. We found that gp85 of PK19FA01 was more similar to that of the prototype strain HPRS103, whereas gp85 of PK19SA01 was more similar to that of American strains. The two isolates contained an intact E element of 147 residues and had a unique 135 bp deletion in the redundant transmembrane of the 3' untranslated region. The U3 region of the two isolates was highly homologous to that of American ALV-J strains. To our knowledge, this is the first report of the isolation, complete genome sequencing, and systematic molecular epidemiological investigation of ALV-J in Pakistan. Our findings could enrich epidemiological data and might contributed to more effective measures to prevent and control avian leukosis in Pakistan., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2020

14. Recombinant subgroup B avian leukosis virus combined with the subgroup J env gene significantly increases its pathogenicity.

Author

Li Q, Wang P, Li M, Lin L, Shi M, Li H, Deng Q, Teng H, Mo M, Wei T, and Wei P

Subjects

Animals, Avian Leukosis immunology, Avian Leukosis Virus classification, Cell Line, Chickens virology, Fibroblasts virology, Poultry Diseases immunology, Poultry Diseases virology, Recombination, Genetic, Viral Tropism, Viremia, Virulence, Avian Leukosis virology, Avian Leukosis Virus genetics, Avian Leukosis Virus pathogenicity, Genes, env, Virus Replication

Abstract

The differences among different sub-groups of the avian leukosis virus (ALV) genome are mainly concentrated in the env gene, which binds to cell-specific receptors and determines the characteristics of viral tropism and pathogenicity. In this study, two rescued viruses rGX15MM6-2 (ALV of subgroup J, ALV-J) and rGX14FF03 (ALV of subgroup B, ALV-B) and a recombinant virus rALV-B-Jenv (ALV-B's backbone with ALV-J's env) were generated and tested utilizing both in vitro and in vivo experiments. The results showed that the replication ability of the viruses released in DF-1 cell cultures was listed in order as rGX15MM6-2 > rALV-B-Jenv > rGX14FF03. rGX15MM6-2 caused the most serious suppression of body weight gain, exhibited a significant negative effect on the development of immune organs (P < 0.05) and lower antibody responses to vaccinations with the commercial oil-emulsion vaccines (OEVs) (P<0.05) in the challenged chickens. The viral detection showed that the positive rate in blood from the birds infected with rALV-B-Jenv were respectively higher than those from the birds infected with rGX14FF03 (P < 0.05). At 25 wpi, similar tumors were found in the abdominal cavity of the birds in rGX15MM6-2 and rALV-B-Jenv groups. The results demonstrated that the ALV-J env gene significantly increases the pathogenicity of the recombinant ALV-B. With the increasing incidence of co-infections of different subgroups of ALV in the field, the possibility of viral recombination is increasing and demands further study., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2020

15. Complete genome sequence of a novel recombinant avian leukosis virus isolated from a three-yellow chicken.

Author

Sun T, Wang X, Han W, Ma X, Yin W, Fang B, Lin X, and Li Y

Subjects

Animals, Avian Leukosis Virus isolation & purification, Chickens, China, Phylogeny, Reassortant Viruses classification, Reassortant Viruses isolation & purification, Viral Proteins genetics, Whole Genome Sequencing, Avian Leukosis virology, Avian Leukosis Virus classification, Genome, Viral, Poultry Diseases virology

Abstract

In this study, an avian leukosis virus (ALV) strain (GX-2020-01) was isolated from a three-yellow chicken, and its complete genome was 7570 bp long with the typical organization "5'LTR-gag-pol-env-3'LTR." Phylogenetic analysis and sequence comparison revealed that it belongs to the ALV-J subgroup. However, the LTR region of GX-2020-01 is highly similar to that of reference strains of ALV-K/E (96.61%-97.10%), demonstrating that this novel isolate is a natural recombinant. The replication efficiency of GX-2020-01 was significantly lower than the previously isolated ALV-J strain (NX0101), indicating that the recombination event might have resulted in slower virus replication, making it harder for it to be detected through routine testing.

Published

2020

16. Neuropathogenicity of newly isolated avian leukosis viruses from chickens with osteopetrosis and mesenchymal neoplasms.

Author

Nishiura H, Kubota I, Kondo Y, Kachi M, Hatai H, Sasaki J, Goryo M, and Ochiai K

Subjects

Animals, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Cerebellum abnormalities, Cerebellum virology, Chick Embryo, Developmental Disabilities virology, Encephalitis veterinary, Encephalitis virology, Female, Glioma virology, Myxosarcoma veterinary, Myxosarcoma virology, Nervous System Malformations veterinary, Nervous System Malformations virology, Osteopetrosis virology, Phylogeny, Recombination, Genetic, Rhabdomyosarcoma veterinary, Rhabdomyosarcoma virology, Specific Pathogen-Free Organisms, Avian Leukosis virology, Avian Leukosis Virus pathogenicity, Chickens virology, Glioma veterinary, Osteopetrosis veterinary, Poultry Diseases virology

Abstract

ABSTRACT The prototype fowl glioma-inducing virus (FGVp) causes fowl glioma and cerebellar hypoplasia in chickens. In this study, we investigated whether a strain of avian leukosis virus (ALV), associated with avian osteopetrosis and mesenchymal neoplasms, is able to induce fowl glioma. We encountered avian osteopetrosis and mesenchymal neoplasms, including myxosarcoma and rhabdomyosarcoma, in Japanese native chickens used for both egg-laying and meat production. These birds were also affected by non-suppurative encephalitis and glioma in their brains. Four ALV strains (GifN&#95;001, GifN&#95;002, GifN&#95;004, GifN&#95;005) were isolated, and a phylogenic analysis of env SU showed that these isolates were classified into different clusters from FGVp and the variants previously reported. Whereas the env SU shared a high identity (94.7%) with that of Rous sarcoma virus (strain Schmidt-Ruppin B) (RSV-SRB), the identity between env TM of GifN&#95;001 and that of FGVp was high (94.5%), indicating that GifN&#95;strains may emerge by recombination between FGVp and other exogenous ALVs. Specific-pathogen-free chickens inoculated in ovo with GifN&#95;001 revealed fowl glioma and cerebellar hypoplasia. These results suggest that the newly isolated strains have acquired neuropathogenicity to chickens.

Published

2020

17. Avian leukosis virus subgroup J induces B cell anergy mediated by Lyn inhibited BCR signal transduction.

Author

He S, Zheng G, Yang X, Dong J, Zhou D, Venugopal N, Yao Y, and Cheng Z

Subjects

Animals, Avian Leukosis immunology, Avian Leukosis virology, Avian Leukosis Virus classification, B-Lymphocytes virology, Chickens immunology, Chickens virology, Gene Expression Regulation, Phosphorylation, Poultry Diseases virology, Specific Pathogen-Free Organisms, Up-Regulation, Avian Leukosis Virus immunology, B-Lymphocytes immunology, Clonal Anergy, Signal Transduction immunology, src-Family Kinases genetics

Abstract

Immune tolerance induced by avian leukosis virus subgroup J (ALV-J) is a prerequisite for tumorigenesis. Although we had reported that B cell anergy induced by ALV-J was the main reason for immune tolerance, the molecular mechanism still remains unclear. Here, we found SU protein of ALV-J interacted with tyrosine kinase Lyn (a key protein in BCR signaling pathway) by confocal laser scanning microscopy and co-immunoprecipitation test, which suggested that Lyn might play an important role in B cell anergy induced by ALV-J. Correspondingly, the mRNA and protein level of Lyn was significantly up-regulated in B cells after ALV-J infection. Subsequently, the phosphorylated protein levels of Lyn at Tyr507 site were significantly up-regulated in ALV-J-infected B cells after BCR signal activation, but the phosphorylated protein level of Syk (a direct substrate of Lyn) at Tyr525/526 site, Ca 2+ flux, and NF-κB p65 protein level were significantly down-regulated. Interestingly, the phosphorylated protein level of Syk at Tyr525/526 site, Ca 2+ flux, and NF-κB p65 protein level were both significantly retrieved after the shLyn treatment in B cells infected by ALV-J. In summary, these results indicated that ALV-J activated the negative regulatory effect of phosphorylated Lyn protein at 507 site in BCR signal transduction pathway and then mediated B cell anergy, which will provide a new insight for revealing the pathogenesis of immune tolerance induced by ALV-J., Competing Interests: Declaration of Competing Interest The authors declare that they have no conflict of interest., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2020

18. Development and evaluation of a gp85 protein-based subgroup-specific indirect enzyme-linked immunosorbent assay for the detection of anti-subgroup J avian leukosis virus antibodies.

Author

Chang F, Xing L, Xing Z, Yu M, Bao Y, Wang S, Farooque M, Li X, Liu P, Pan Q, Qi X, Gao L, Li K, Liu C, Zhang Y, Cui H, Wang X, and Gao Y

Subjects

Animals, Avian Leukosis Virus classification, Cell Line, Chickens virology, Fluorescent Antibody Technique, Indirect, HEK293 Cells, Humans, Sensitivity and Specificity, Antibodies, Viral isolation & purification, Avian Leukosis Virus immunology, Enzyme Assays, Enzyme-Linked Immunosorbent Assay, Viral Envelope Proteins immunology

Abstract

Avian leukosis virus subgroup J (ALV-J) is an important pathogen for various neoplasms and causes significant economic losses in the poultry industry. Serological detection of specific antibodies against ALV-J infection is important for successful clinical diagnosis. Here, a 293F stable cell line was established to stably express gp85 protein. In this cell line, gp85 protein was expressed at approximately 30 mg/L. A subgroup-specific indirect enzyme-linked immunosorbent assay (iELISA) was developed using ALV-J gp85 protein as coated antigen to detect antibodies against ALV-J. The sensitivity of the iELISA (1:51200 diluted in serum) was 16 times more than that of indirect immunofluorescence assay (IFA; 1:3200 diluted in serum). Moreover, there was no crossreactivity with antibodies against other common avian viruses and other avian leukosis virus subgroups, such as subgroups A and B. The practicality of the iELISA was further evaluated by experimental infection and clinical samples. The results from experimental infection indicated that anti-ALV-J antibodies were readily detected by iELISA as early as 4 weeks after ALV-J infection, and positive antibodies were detected until 20 weeks, with an antibody-positive rate of 11.1% to 33.3%. Moreover, analysis of clinical samples showed that 9.49% of samples were positive for anti-ALV-J antibodies, and the concordance rate of iELISA and IFA was 99.24%. Overall, these results suggested that the subgroup-specific iELISA developed in this study had good sensitivity, specificity, and feasibility. This iELISA will be very useful for epidemiological surveillance, diagnosis, and eradication of ALV-J in poultry farms.

Published

2020

19. Precise CRISPR/Cas9 editing of the NHE1 gene renders chickens resistant to the J subgroup of avian leukosis virus.

Author

Koslová A, Trefil P, Mucksová J, Reinišová M, Plachý J, Kalina J, Kučerová D, Geryk J, Krchlíková V, Lejčková B, and Hejnar J

Subjects

Animals, Animals, Genetically Modified genetics, Animals, Genetically Modified immunology, Animals, Genetically Modified virology, Avian Leukosis genetics, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus physiology, Avian Proteins immunology, CRISPR-Cas Systems, Chickens, Disease Resistance, Female, Gene Editing, Male, Poultry Diseases genetics, Poultry Diseases virology, Sodium-Hydrogen Exchanger 1 immunology, Avian Leukosis immunology, Avian Leukosis Virus genetics, Avian Proteins genetics, Poultry Diseases immunology, Sodium-Hydrogen Exchanger 1 genetics

Abstract

Avian leukosis virus subgroup J (ALV-J) is an important concern for the poultry industry. Replication of ALV-J depends on a functional cellular receptor, the chicken Na + /H + exchanger type 1 (chNHE1). Tryptophan residue number 38 of chNHE1 (W38) in the extracellular portion of this molecule is a critical amino acid for virus entry. We describe a CRISPR/Cas9-mediated deletion of W38 in chicken primordial germ cells and the successful production of the gene-edited birds. The resistance to ALV-J was examined both in vitro and in vivo, and the ΔW38 homozygous chickens tested ALV-J-resistant, in contrast to ΔW38 heterozygotes and wild-type birds, which were ALV-J-susceptible. Deletion of W38 did not manifest any visible side effect. Our data clearly demonstrate the antiviral resistance conferred by precise CRISPR/Cas9 gene editing in the chicken. Furthermore, our highly efficient CRISPR/Cas9 gene editing in primordial germ cells represents a substantial addition to genotechnology in the chicken, an important food source and research model., Competing Interests: Competing interest statement: A.K., P.T., J.M., M.R., J.P., J.K., D.K., and J.H. are inventors in a patent application related to this work (CZ patent application no. PV 2019-392). The other authors declare no competing interests.

Published

2020

20. Systematic Identification of Host Immune Key Factors Influencing Viral Infection in PBL of ALV-J Infected SPF Chicken.

Author

Dai M, Li S, Shi K, Liao J, Sun H, and Liao M

Subjects

Animals, Antibodies, Viral blood, Avian Leukosis virology, Avian Leukosis Virus classification, CD8-Positive T-Lymphocytes immunology, Chemokine CXCL1 immunology, Chickens immunology, Chickens virology, Immunity, Humoral, Leukocytes, Mononuclear immunology, Myxovirus Resistance Proteins genetics, Specific Pathogen-Free Organisms, Viremia immunology, Avian Leukosis immunology, Avian Leukosis Virus immunology, Host Microbial Interactions immunology, Interferons immunology, Leukocytes, Mononuclear virology

Abstract

Although research related to avian leukosis virus subgroup J (ALV-J) has lasted for more than a century, the systematic identification of host immune key factors against ALV-J infection has not been reported. In this study, we establish an infection model in which four-week-old SPF chickens are infected with ALV-J strain CHN06, after which the host immune response is detected. We found that the expression of two antiviral interferon-stimulated genes (ISGs) (Mx1 and IFIT5) were increased in ALV-J infected peripheral blood lymphocytes (PBL). A significant CD8 + T cell response induced by ALV-J appeared as early as seven days post-infection (DPI), and humoral immunity starting from 21 DPI differed greatly in the time scale of induction level. Meanwhile, the ALV-J viremia was significantly decreased before antibody production at 14 DPI, and eliminated at 21 DPI under a very low antibody level. The up-regulated CD8 + T cell in the thymus (14DPI) and PBL (7 DPI and 21 DPI) was detected, indicating that the thymus may provide the output of CD8 + T cell to PBL, which was related to virus clearance. Besides, up-regulated chemokine CXCLi1 at 7 DPI in PBL was observed, which may be related to the migration of the CD8 + T cell from the thymus to PBL. More importantly, the CD8 high+ T cell response of the CD8αβ phenotype may produce granzyme K, NK lysin, or IFN-γ for clearing viruses. These findings provide novel insights and direction for developing effective ALV-J vaccines., Competing Interests: The authors declare no conflict of interest. The funders had no role in the design of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript, or in the decision to publish the results.

Published

2020

21. Identification and characterization of a novel natural recombinant avian leucosis virus from Chinese indigenous chicken flock.

Author

Liang X, Gu Y, Chen X, Li T, Gao Y, Wang X, Fang C, Fang S, and Yang Y

Subjects

Animals, Avian Leukosis Virus isolation & purification, Chickens, China, Cluster Analysis, Phylogeny, Sequence Analysis, DNA, Sequence Homology, Amino Acid, Viral Proteins genetics, Whole Genome Sequencing, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Poultry Diseases virology, Recombination, Genetic

Abstract

Avian leukosis virus (ALV) caused tremendous economic losses to poultry industry all over the world, especially in China. One natural recombinant ALV strain, designated as HB2015032, was isolated from indigenous chickens with neoplastic diseases in Hubei, China. The complete proviral genome of HB2015032 is 7703 bp in length. Sequence analysis showed that the Env of HB2015032 exhibited 99.3% similarity with that of a ALV subgroup K (ALV-K) isolate JS11C1 at amino acid level. Phylogenetic analysis revealed that both gp85 and gp37 of HB2015032 were clustered in the same branch with JS11C1 and other ALV-K strains isolated from Chinese indigenous chickens in recent years. However, the pol gene, the 3' untranslated region (3' UTR), and the 3' long terminal repeat (3' LTR) of HB2015032 were more closely related to ALV-J prototype HPRS-103, and clustered in the same branch with ALV-J strains. Furthermore, the pol gene of HB2015032 contained a premature stop codon that resulted in a truncated Pol protein with 22 amino acid residues missing, which was a unique feature of the pol gene of ALV-J. 3'UTR of HB2015032 containing entire DR1, E element and U3. E element of HB2015032 contained one base deletion, which resulted in a c-Ets-1 binding site. In addition, U3 region of HB2015032 contains most of the transcription regulatory elements of ALV-J, including two CAAT boxes, Y boxes, CArG boxes, PRE boxes, NFAP-1 boxes, and one TATA box. These results suggest that isolate HB2015032 was a novel recombinant ALV-K containing the ALV-K env gene and the ALV-J backbone and exhibiting high pathogenicity.

Published

2019

22. Taishan Pinus Massoniana pollen polysaccharide inhibits the replication of acute tumorigenic ALV-J and its associated tumor growth.

Author

Wang Q, Miao Y, Xu Y, Meng X, Cui W, Wang Y, Zhu L, Sha Z, Wei K, and Zhu R

Subjects

Animals, Antiviral Agents chemistry, Antiviral Agents pharmacology, Avian Leukosis Virus classification, Avian Leukosis Virus physiology, Cell Line, Chickens, Polysaccharides chemistry, RNA, Messenger genetics, RNA, Messenger metabolism, Virus Replication drug effects, Avian Leukosis Virus drug effects, Pinus chemistry, Pollen chemistry, Polysaccharides pharmacology

Abstract

Avian leukosis virus subgroup J (ALV-J) has resulted in considerable economic losses in the poultry industry. In recent years, fibrosarcoma induced by ALV-J, which contains the v-fps oncogene, has gained momentum, and this has brought about new challenges to the poultry industry. To study the inhibitory effects of Taishan Pinus Massoniana pollen polysaccharide (TPPPS) on acute ALV-J infection and tumor development, antiviral and antitumor models of the Fu-J (SDAU1005) strain of ALV-J were established in vitro and in vivo. The results of in vitro experiments showed that TPPPS significantly inhibited viral replication in a dose-dependent manner during adsorption and pretreatment stages. The results of in vivo experiments have shown that TPPPS significantly reduced the viral load in the plasma and tumor tissues, as well as inhibited tumor growth. We further examined the difference in transcriptome expression by using RNA-Seq technology. A total of 560 differentially expressed genes were identified that included 329 up-regulated genes and 231 down-regulated genes. The up-regulated genes were mainly immune-related genes, whereas the down-regulated genes were mainly tumor-regulated genes. Gene Ontology (GO) term enrichment included immune system processes, positive regulation of immune system processes, regulation of immune system processes, leukocyte activation, cell activation, and protein binding. Kyoto Encyclopedia of Genes and Genomes (KEGG) pathway analysis revealed that the main immune and tumor-related pathways included T-cell receptor signaling pathway, cytokine-cytokine receptor interactions, natural killer cell-mediated cytotoxicity, PI3K-Akt signaling pathway, JAK-STAT signaling pathway, NF-κB signaling pathway, and Ras signaling pathway. In summary, our results preliminarily point to the antiviral and antitumor mechanism of TPPPS in vivo and in vitro., (Copyright © 2019. Published by Elsevier B.V.)

Published

2019

23. The Novel Avian Leukosis Virus Subgroup K Shares Its Cellular Receptor with Subgroup A.

Author

Přikryl D, Plachý J, Kučerová D, Koslová A, Reinišová M, Šenigl F, and Hejnar J

Subjects

Animals, Avian Leukosis metabolism, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus physiology, Cell Line, Chickens, Disease Susceptibility, Fibroblasts cytology, Fibroblasts metabolism, Fibroblasts virology, Mesocricetus, Species Specificity, Virus Internalization, Avian Leukosis genetics, Avian Leukosis Virus pathogenicity, Avian Proteins genetics, Avian Proteins metabolism, Receptors, Virus genetics, Receptors, Virus metabolism

Abstract

Avian leukosis virus subgroup K (ALV-K) is composed of newly emerging isolates, which, in sequence analyses, cluster separately from the well-characterized subgroups A, B, C, D, E, and J. However, it remains unclear whether ALV-K represents an independent ALV subgroup with regard to receptor usage, host range, and superinfection interference. In the present study, we examined the host range of the Chinese infectious isolate JS11C1, an ALV-K prototype, and we found substantial overlap of species that were either resistant or susceptible to ALV-A and JS11C1. Ectopic expression of the chicken tva gene in mammalian cells conferred susceptibility to JS11C1, while genetic ablation of the tva gene rendered chicken DF-1 cells resistant to infection by JS11C1. Thus, tva expression is both sufficient and necessary for JS11C1 entry. Receptor sharing was also manifested in superinfection interference, with preinfection of cells with ALV-A, but not ALV-B or ALV-J, blocking subsequent JS11C1 infection. Finally, direct binding of JS11C1 and Tva was demonstrated by preincubation of the virus with soluble Tva, which substantially decreased viral infectivity in susceptible chicken cells. Collectively, these findings indicate that JS11C1 represents a new and bona fide ALV subgroup that utilizes Tva for cell entry and binds to a site other than that for ALV-A. IMPORTANCE ALV consists of several subgroups that are particularly characterized by their receptor usage, which subsequently dictates the host range and tropism of the virus. A few newly emerging and highly pathogenic Chinese ALV strains have recently been suggested to be an independent subgroup, ALV-K, based solely on their genomic sequences. Here, we performed a series of experiments with the ALV-K strain JS11C1, which showed its dependence on the Tva cell surface receptor. Due to the sharing of this receptor with ALV-A, both subgroups were able to interfere with superinfection. Because ALV-K could become an important pathogen and a significant threat to the poultry industry in Asia, the identification of a specific receptor could help in the breeding of resistant chicken lines with receptor variants with decreased susceptibility to the virus., (Copyright © 2019 American Society for Microbiology.)

Published

2019

24. Co-infection of vvMDV with multiple subgroups of avian leukosis viruses in indigenous chicken flocks in China.

Author

Li T, Xie J, Liang G, Ren D, Sun S, Lv L, Xie Q, Shao H, Gao W, Qin A, and Ye J

Subjects

Animals, Avian Leukosis epidemiology, Avian Leukosis Virus genetics, China epidemiology, Marek Disease epidemiology, Phylogeny, Virulence, Avian Leukosis virology, Avian Leukosis Virus classification, Chickens, Coinfection, Marek Disease virology

Abstract

Background: In China, although the ALV eradication program and the MD vaccination strategy greatly reduce the disease burdens caused by the infection of ALV and MDV, the frequent emergence of novel ALV-K or vvMDV in the vaccinated chicken flock challenges the current control strategies for both diseases., Results: In Guangdong Province, an indigenous chicken flock was infected with neoplastic disease. Hematoxylin-eosin staining of the tissues showed the typical characteristics of MDV and classical ALV infection. The PCR and sequencing data demonstrated that the identified MDV was clustered into a very virulent MDV strain endemic in domestic chickens in China. Moreover, subgroups ALV-A and ALV-K were efficiently recovered from two samples. The full genome sequence revealed that the ALV-K isolate was phylogenetically close to the ALV TW3593 isolate from Taiwan Province., Conclusions: A co-infection of vvMDV with multiple ALV subgroups emerged in a chicken flock with neoplastic disease in Guangdong Province. The co-infection with different subgroups of ALV with vvMDV in one chicken flock poses the risk for the emergence of novel ALVs and heavily burdens the control strategy for MDV.

Published

2019

25. Outbreak of myelocytomatosis caused by mutational avian leukosis virus subgroup J in China, 2018.

Author

Zhou D, Xue J, Zhang Y, Wang G, Feng Y, Hu L, Shang Y, and Cheng Z

Subjects

Animals, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, China epidemiology, Mutation, Phylogeny, Poultry Diseases virology, Avian Leukosis epidemiology, Avian Leukosis Virus physiology, Chickens, Disease Outbreaks veterinary, Poultry Diseases epidemiology

Abstract

Avian leukosis virus subgroup J (ALV-J) was isolated in meat-type breeder chickens for the first time in 1988 in the United Kingdom. Due to the application of an eradication program, there were fewer reports related to myelocytomatosis or ALV-J in China after 2013. However, there was another breakout almost simultaneously in six provinces of China in February 2018. On-site, 15- to 20-week-old broiler breeder chickens showed depression, paralysis and weight loss. Mortality for certain flocks reached 15%. Sick chickens showed numerous yellow-white neoplasms growing in the sternum, rib and lumbar vertebra and had hepatic and renal metastasis. Histopathological observation showed all neoplasms were myelocytomas, and there were massive myelocyte-like tumour cells in the liver, kidney and bone marrow. To explore the aetiology of this re-outbreak of myelocytomatosis in China, we collected tumour-bearing chickens and isolated six strains of ALV-J (GM0209-1 to -6). Phylogenetic analysis of gp85 and gp37 showed GM0209 strains were clearly distinct from the prototype strain of ADOL-7501, HPRS-103 and NX0101, and there was a mutation, R176G, in the conserved region between hr1 and hr2 regions of gp85, which was not found in other 44 ALV-J strains. The 3'UTR nucleotide sequences of GM0209 isolates showed there was a signature deletion of 11 nt that was also present in 3'UTR sequences of SCDY1 and NHH, two isolates that have a reported association with haemangioma, indicating this deletion could not determine the tumour type induced by ALV-J. Although the eradication program of ALV-J has been successfully applied in China, the outbreak of ALV-J still occurred, and the virus strain spread quickly. Thus, the biocharacteristics and pathogenesis of mutational ALV-J should be further studied., (© 2018 Blackwell Verlag GmbH.)

Published

2019

26. Avian leukosis virus subgroup - J as a contaminant in live commercially available poultry vaccines distributed in Nigeria.

Author

Shittu I, Adedeji AJ, Luka PD, Asala OO, Sati NM, Nwagbo IO, Chinyere CN, Arowolo OO, Adole JA, Emennaa P, Abdu PA, and Joannis TM

Subjects

Animals, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Gene Products, env classification, Gene Products, env genetics, Gene Products, env immunology, Nigeria, Phylogeny, Polymerase Chain Reaction methods, Poultry, Poultry Diseases virology, Vaccines, Attenuated immunology, Avian Leukosis immunology, Avian Leukosis Virus immunology, Drug Contamination, Poultry Diseases immunology, Viral Vaccines immunology

Abstract

Globally, vaccines are used to prevent and control the menace of infectious diseases in livestock with some reported to be inadvertently contaminated with extraneous agents (EAs). With the aim of screening and characterizing for some selected EAs, 44 live viral poultry vaccines were randomly selected based on availability. The vaccines comprised 14 manufacturers in 10 different countries including Nigeria were screened by Polymerase Chain Reaction. In 9% (4/44) of the vaccines, contamination with only avian leukosis virus (ALV) subgroup J (ALV-J) was recorded. Other exogenous ALV subgroups, chicken infectious anemia and infectious laryngotracheitis viruses were absent. The EAs was found in infectious bursal disease (n = 1), Fowlpox (n = 2) and Mareks disease (n = 1) vaccines. Phylogenetic analysis of the ALV-J env gene showed clustering with contemporary group I and II. The result underscores the importance of screening vaccines to avoid the introduction and spread of EAs that could pose a threat to poultry production., (Copyright © 2018 International Alliance for Biological Standardization. Published by Elsevier Ltd. All rights reserved.)

Published

2019

27. Identification of novel B-cell epitope in gp85 of subgroup J avian leukosis virus and its application in diagnosis of disease.

Author

Qian K, Tian X, Shao H, Ye J, Yao Y, Nair V, and Qin A

Subjects

Animals, Antibodies, Monoclonal immunology, Antibodies, Viral immunology, Avian Leukosis immunology, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Epitope Mapping, Epitopes, B-Lymphocyte chemistry, Poultry Diseases diagnosis, Poultry Diseases immunology, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics, Avian Leukosis Virus immunology, Chickens, Epitopes, B-Lymphocyte immunology, Poultry Diseases virology, Viral Envelope Proteins immunology

Abstract

Background: The gp85 is the main envelope protein of avian leukosis subgroup J (ALV-J) involved in virus neutralization. Here, we mapped the epitope in ALV-J gp85 by ELISA using synthetic peptides and developed epitope based diagnostic methods for ALV-J infection., Results: The results revealed that monoclonal antibody (mAb) JE9 recognized 83 WDPQEL 88 motif, which was highly conserved in gp85 among different ALV-J strains by homology analysis. Moreover, after evaluation with two hundred and forty sera samples obtained from different chicken farms, the epitope-based peptide ELISA had much higher sensitivity than commercial ELISA kit for antibody detection of ALV-J., Conclusions: A novel B-cell epitope recognized by the mAb JE9 was identified. The developed peptide-ELISA based on this novel B-cell epitope could be useful in laboratory viral diagnosis, routine surveillance in chicken farms, and also in understanding the pathogenesis of ALV-J.

Published

2018

28. Molecular characteristics of avian leukosis viruses isolated from indigenous chicken breeds in China.

Author

Su Q, Li Y, Li W, Cui S, Tian S, Cui Z, Zhao P, and Chang S

Subjects

Amino Acid Sequence, Animals, Avian Leukosis virology, Avian Leukosis Virus classification, China, Phylogeny, Poultry Diseases virology, Avian Leukosis epidemiology, Avian Leukosis Virus genetics, Chickens, Gene Products, pol genetics, Poultry Diseases epidemiology

Abstract

To assess the status of avian leukosis virus (ALV) infection in indigenous chicken breeds in China, 121 plasma samples collected from various indigenous chicken breeds were tested for the presence of ALV from 2015 to 2016. A total of 14 ALV strains were isolated and identified, including two ALV-A strains, one ALV-B strain, eight ALV-J strains, and three ALV-K strains. To study the genome structure, biological characteristics, and the evolutionary relationships of the ALV-K strains with other known subgroup strains from infected chickens, we determined the complete genome sequence of the three ALV-K strains and performed comparative analysis using the whole genome sequence or selected sequence elements. The replication rates of the three ALV-K strains were markedly lower than the rates of other ALVs, and they shared a common mutation in the pol gene, which had not been previously observed. In addition, nine putative recombinant events were detected in the genomes of the three newly isolated ALV-K strains, with high statistical support. This was the first report of an ALV-K reorganization event, which has contributed to its genetic evolution. In summary, we established a robust classification system for ALV, especially for ALV-K, and revealed additional genomic diversity for the ALV strains in indigenous chicken breeds. Therefore additional works are warranted to explore ALV genomics and epidemiology.

Published

2018

29. Avian leukosis virus subgroup J promotes cell proliferation and cell cycle progression through miR-221 by targeting CDKN1B.

Author

Ren C, Yu M, Zhang Y, Fan M, Chang F, Xing L, Liu Y, Wang Y, Qi X, Liu C, Zhang Y, Cui H, Li K, Gao L, Pan Q, Wang X, and Gao Y

Subjects

Animals, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Carcinogenesis genetics, Cell Cycle physiology, Cell Line, Chickens virology, Computational Biology, Down-Regulation, Fibroblasts physiology, Fibroblasts virology, Poultry Diseases virology, Avian Leukosis Virus physiology, Cell Cycle genetics, Cell Proliferation, Cyclin-Dependent Kinase Inhibitor p27 genetics, Host-Pathogen Interactions, MicroRNAs genetics

Abstract

Avian leukosis virus subgroup J (ALV-J), a highly oncogenic retrovirus, causes leukemia-like proliferative diseases in chickens. microRNAs post-transcriptionally suppress targets and are involved in the development of various tumors. We previously showed that miR-221 is upregulated in ALV-J-induced tumors. In this study, we analyzed the possible function of miR-221 in ALV-J tumorigenesis. The target validation system showed that CDKN1B is a target of miR-221 and is downregulated in ALV-J infection. As CDKN1B arrests the cell cycle and regulates its progression, we analyzed the proliferation of ALV-J-infected DF-1 cells. ALV-J-infection-induced DF1 cell derepression of G1/S transition and overproliferation required high miR-221 expression followed by CDKN1B downregulation. Cell cycle pathway analysis showed that ALV-J infection induced DF-1 cell overproliferation via the CDKN1B-CDK2/CDK6 pathway. Thus, miR-221 may play an important role in ALV-J-induced aggressive growth of DF-1 cells; these findings have expanded our insights into the mechanism underlying ALV-J infection and tumorigenesis., (Copyright © 2018 Elsevier Inc. All rights reserved.)

Published

2018

30. Co-infection of fowl adenovirus with different immunosuppressive viruses in a chicken flock.

Author

Meng F, Dong G, Zhang Y, Tian S, Cui Z, Chang S, and Zhao P

Subjects

Adenoviridae Infections epidemiology, Adenoviridae Infections virology, Animals, Avian Leukosis epidemiology, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, Chicken anemia virus classification, Chicken anemia virus isolation & purification, Circoviridae Infections epidemiology, Circoviridae Infections veterinary, Circoviridae Infections virology, Coinfection epidemiology, Coinfection virology, Female, Fowl adenovirus A classification, Phylogeny, Poultry Diseases virology, Reticuloendotheliosis virus classification, Reticuloendotheliosis virus isolation & purification, Retroviridae Infections epidemiology, Retroviridae Infections veterinary, Retroviridae Infections virology, Tumor Virus Infections epidemiology, Tumor Virus Infections veterinary, Tumor Virus Infections virology, Adenoviridae Infections veterinary, Chickens, Coinfection veterinary, Fowl adenovirus A isolation & purification, Poultry Diseases epidemiology

Abstract

In poultry, fowl adenovirus (FAdV) and immunosuppressive virus co-infection is likely to cause decreased egg production, inclusion body hepatitis, and pericardial effusion syndrome. In this study, fowl adenovirus infection was found in parental and descendent generations of chickens. We used quantitative polymerase chain reaction (PCR) and dot blot hybridization to detect the infection of reticuloendotheliosis (REV), avian leukosis virus (ALV), and chicken infectious anemia virus (CIAV) in 480 plasma samples. The test samples were 34.58% FADV-positive, 22.29% REV-positive, 7.5% CAV-positive, and 0.63% ALV-positive. Sequence analysis showed that FADV belonged to serotype 7, which can cause inclusion body hepatitis. The ALV strain was ALV-A, in which the homology of gp85 gene and SDAU09C1 was 97.3%. The positive rate was lower because of the purification of avian leukemia, whereas the phylogenetic tree analysis of REV showed that the highest homology was with IBD-C1605, which was derived from a vaccine isolate. Through pathogen detection in poultry we present, to our knowledge, the first discovery of fowl adenovirus type 7 infection in parental chickens and found that there was co-infection of FAdV and several immunosuppressive viruses, such as the purified ALV and CIAV. This indicates that multiple infection of different viruses is ever-present, and more attention should be given in the diagnosis process.

Published

2018

31. Phylogenetic Analysis and Pathogenicity Assessment of the Emerging Recombinant Subgroup K of Avian Leukosis Virus in South China.

Author

Zhao Z, Rao M, Liao M, and Cao W

Subjects

Animals, Avian Leukosis pathology, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, Chickens, China, Genome, Viral, Sequence Homology, Terminal Repeat Sequences, Viral Proteins genetics, Whole Genome Sequencing, Avian Leukosis virology, Avian Leukosis Virus genetics, Avian Leukosis Virus pathogenicity, Genetic Variation, Phylogeny, Recombination, Genetic

Abstract

In recent years, cases of avian leukosis virus (ALV) infection have become more frequent in China. We isolated 6 ALV strains from yellow feather broiler breeders in south China from 2014 to 2016. Their full genomes were sequenced, compared, and analyzed with other reference strains of ALV. The complete genomic nucleotide sequences of GD150509, GD160403, GD160607, GDFX0601, and GDFX0602 were 7482 bp in length, whereas GDFX0603 was 7480 bp. They shared 99.7% to 99.8% identity with each other. Homology analysis showed that the gag , pol , long terminal repeats (LTRs), and the transmembrane region (gp37) of the env genes of the 6 viruses were well conserved to endogenous counterpart sequences (>97.8%). However, the gp85 genes displayed high variability with any known chicken ALV strains. Growth kinetics of DF-1 cells infected with the isolated ALV showed viral titers that were lower than those infected with the GD13 (ALV-A), CD08 (ALV-B), and CHN06 (ALV-J) on day 7 post-infection. The infected Specific-pathogen-free (SPF) chickens could produce continuous viremia, atrophy of immune organs, growth retardation and no tumors were observed. These subgroup ALVs are unique and may be common in south China. The results suggested that updating the control and eradication program of exogenous ALV for yellow feather broiler breeders in south China needs to be considered because of the emergence of the new subgroup viruses., Competing Interests: The authors declare no conflict of interest.

Published

2018

32. Characterization of subgroup J avian Leukosis virus isolated from Chinese indigenous chickens.

Author

Meng F, Li Q, Zhang Y, Zhang Z, Tian S, Cui Z, Chang S, and Zhao P

Subjects

Amino Acid Sequence, Animals, Avian Leukosis pathology, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, China, Mutation, Phylogeny, Poultry Diseases pathology, Terminal Repeat Sequences, Viral Envelope Proteins genetics, Avian Leukosis virology, Avian Leukosis Virus genetics, Chickens virology, Poultry Diseases virology

Abstract

Background: In spite of the purification of the laying hens and broilers of avian leukosis virus (ALV) has made remarkable achievements, the infection of ALV was still serious in Chinese indigenous chickens., Methods: In order to assess the epidemic state of avian leukosis virus in indigenous chickens in China, 10 novel strains of ALV subgroup J (ALV-J), named JS16JH01 to JS16JH10, were isolated and identified by virus isolation and immunofluorescence antibody assays from a Chinese local breed farm with a sporadic incidence of tumors. To understand their virological characteristics further, the proviral genome of ENV-LTR was sequenced and compared with the reference strains., Results: The homology of the gp85 gene between the ten ALV-J strains and NX0101 was in the range from 89.7-94.8% at the nuclear acid level. In addition, their gp85 genes were quite varied, with identities of 92-98% with themselves at the nuclear acid level. There were several snp and indel sites in the amino acid sequence of gp85 genes after comparison with other reference strains of ALV. Interestingly, a novel insertion in the gp85 region was found in two strains, JS16JH01 and JS16JH07, compared with NX0101 and HPRS-103., Discussion: At present, owing to the large-scale purification of ALV in China, laying hens and broiler chickens with ALV infection are rarely detected, but ALVs are still frequently detected in the local chickens, which suggests that more efforts should be applied to the purification of ALV from indigenous chickens.

Published

2018

33. Diversity and evolution analysis of glycoprotein GP85 from avian leukosis virus subgroup J isolates from chickens of different genetic backgrounds during 1989-2016: Coexistence of five extremely different clusters.

Author

Wang P, Lin L, Li H, Yang Y, Huang T, and Wei P

Subjects

Animals, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, Chickens, China, Avian Leukosis virology, Avian Leukosis Virus genetics, Evolution, Molecular, Genetic Variation, Poultry Diseases virology, Viral Envelope Proteins genetics

Abstract

ALV-J has caused the most serious losses to the poultry industry in China. The gp85-coding sequence of ALV-J is known to be prone to mutation, but any association between the gp85 gene and breed of chicken remains unclear. A comprehensive and systematic study of the evolutionary process of ALV-J in China is needed. In this study, we compared and analyzed gp85 gene sequences from 198 ALV-J isolates, originating from China, USA, UK and France during 1989-2016. These were sorted into five clusters. Cluster 1, 2, 3, 4 and 5 included isolates from chicken types of different genetic backgrounds, e.g. white-feather broiler, Guangxi indigenous chicken breeds, Yellow chickens and layer chickens respectively. A correlation comparison of amino acid sequence similarities in the gp85 protein among the five clusters showed significant differences (P < 0.01) with the exception being when the third and fifth cluster were compared (P > 0.05). Results of entropy analysis of the gp85 sequences revealed that cluster 3 had the largest variation and cluster 1 had the least variation. The N-glycosylation sites in the majority of isolates numbered 14, 16, 17, 16 and 16, respectively, with regards to clusters 1-5. In addition, 5 isolates from cluster 3 had one more glycosylation site than the other isolates from cluster 3. Our study provides evidence that there were five extremely different ALV-J clusters during 1989-2016 and that the gp85 genes isolated from indigenous chicken breed isolates had the largest variation.

Published

2018

34. Novel avian leukosis viruses from domestic chicken breeds in mainland China.

Author

Shao H, Wang L, Sang J, Li T, Liu Y, Wan Z, Qian K, Qin A, and Ye J

Subjects

Animals, Animals, Domestic virology, Avian Leukosis Virus genetics, Avian Leukosis Virus isolation & purification, Chickens virology, China, Phylogeny, Avian Leukosis virology, Avian Leukosis Virus classification, Poultry Diseases virology, Terminal Repeat Sequences, Viral Envelope Proteins genetics

Abstract

Two novel avian leukosis viruses (ALVs) were isolated from 1380 whole blood samples taken from domestic chicken breeds in China. The two ALVs were uniquely different from the env (Envelope) genes of ALV A-J and carried an LTR (long terminal repeat) cluster from ALV-E. Large scale sequence analysis further showed that these ALVs (with different env and LTRs) were recently endemic in domestic chicken breeds in both China and Japan. The emergence of these novel ALVs is challenging the current ALV eradication program, and as such novel ALVs should be monitored in a timely and careful manner to stop their transmission and further recombination in the future.

Published

2017

35. Growth retardation induced by avian leukosis virus subgroup J associated with down-regulated Wnt/β-catenin pathway.

Author

Feng W, Zhou D, Meng W, Li G, Zhuang P, Pan Z, Wang G, and Cheng Z

Subjects

Animals, Avian Leukosis complications, Avian Leukosis genetics, Avian Leukosis Virus classification, Cell Line, Cell Proliferation, Cluster Analysis, Gene Expression Profiling, Gene Expression Regulation, MicroRNAs genetics, Transcription Factors metabolism, beta Catenin genetics, beta Catenin metabolism, Avian Leukosis metabolism, Avian Leukosis virology, Avian Leukosis Virus physiology, Chickens, Phenotype, Wnt Signaling Pathway

Abstract

Avian leukosis virus subgroup J (ALV-J), an oncogenic retrovirus, induces growth retardation and neoplasia in chickens, leading to enormous economic losses in poultry industry. Increasing evidences showed several signal pathways involved in ALV-J infection. However, what signaling pathway involved in growth retardation is largely unknown. To explore the possible signaling pathway, we tested the cell proliferation and associated miRNAs in ALV-J infected CEF cells by CCK-8 and Hiseq, respectively. The results showed that cell proliferation was significantly inhibited by ALV-J and three associated miRNAs were identified to target Wnt/β-catenin pathway. To verify the Wnt/β-catenin pathway involved in cell growth retardation, we analyzed the key molecules of Wnt pathway in ALV-J infected CEF cells. Our data demonstrated that protein expression of β-catenin was decreased significantly post ALV-J infection compared with the normal (P < 0.05). The impact of this down-regulation caused low expression of known target genes (Axin2, CyclinD1, Tcf4 and Lef1). Further, to obtain in vivo evidence, we set up an ALV-J infection model. Post 7 weeks infection, ALV-J infected chickens showed significant growth retardation. Subsequent tests showed that the expression of β-catenin, Tcf1, Tcf4, Lef1, Axin2 and CyclinD1 were down-regulated in muscles of growth retardation chickens. Taken together, all data demonstrated that chicken growth retardation caused by ALV-J associated with down-regulated Wnt/β-catenin signaling pathway., (Copyright © 2017 Elsevier Ltd. All rights reserved.)

Published

2017

36. Identification of New World Quails Susceptible to Infection with Avian Leukosis Virus Subgroup J.

Author

Plachý J, Reinišová M, Kučerová D, Šenigl F, Stepanets V, Hron T, Trejbalová K, Elleder D, and Hejnar J

Subjects

Amino Acid Sequence, Amino Acids, Animals, Avian Leukosis metabolism, Avian Leukosis Virus classification, Cells, Cultured, Disease Resistance genetics, Evolution, Molecular, Gene Expression, Genetic Loci, Host Specificity, Host-Pathogen Interactions, Phylogeny, Polymorphism, Genetic, Protein Interaction Domains and Motifs, Sodium-Hydrogen Exchangers chemistry, Sodium-Hydrogen Exchangers genetics, Sodium-Hydrogen Exchangers metabolism, Virus Replication, Avian Leukosis genetics, Avian Leukosis virology, Avian Leukosis Virus physiology, Disease Susceptibility, Quail

Abstract

The J subgroup of avian leukosis virus (ALV-J) infects domestic chickens, jungle fowl, and turkeys. This virus enters the host cell through a receptor encoded by the tvj locus and identified as Na + /H + exchanger 1. The resistance to avian leukosis virus subgroup J in a great majority of galliform species has been explained by deletions or substitutions of the critical tryptophan 38 in the first extracellular loop of Na + /H + exchanger 1. Because there are concerns of transspecies virus transmission, we studied natural polymorphisms and susceptibility/resistance in wild galliforms and found the presence of tryptophan 38 in four species of New World quails. The embryo fibroblasts of New World quails are susceptible to infection with avian leukosis virus subgroup J, and the cloned Na + /H + exchanger 1 confers susceptibility on the otherwise resistant host. New World quails are also susceptible to new avian leukosis virus subgroup J variants but resistant to subgroups A and B and weakly susceptible to subgroups C and D of avian sarcoma/leukosis virus due to obvious defects of the respective receptors. Our results suggest that the avian leukosis virus subgroup J could be transmitted to New World quails and establish a natural reservoir of circulating virus with a potential for further evolution., Importance: Since its spread in broiler chickens in China and Southeast Asia in 2000, ALV-J remains a major enzootic challenge for the poultry industry. Although the virus diversifies rapidly in the poultry, its spillover and circulation in wild bird species has been prevented by the resistance of most species to ALV-J. It is, nevertheless, important to understand the evolution of the virus and its potential host range in wild birds. Because resistance to avian retroviruses is due particularly to receptor incompatibility, we studied Na + /H + exchanger 1, the receptor for ALV-J. In New World quails, we found a receptor compatible with virus entry, and we confirmed the susceptibilities of four New World quail species in vitro We propose that a prospective molecular epidemiology study be conducted to identify species with the potential to become reservoirs for ALV-J., (Copyright © 2017 American Society for Microbiology.)

Published

2017

37. Molecular epidemiology of J-subgroup avian leukosis virus isolated from meat-type chickens in southern China between 2013 and 2014.

Author

Lin W, Li X, Dai Z, Zhang X, Chang S, Zhao P, Zhang H, Chen F, and Xie Q

Subjects

Animals, Avian Leukosis Virus genetics, Chickens, China epidemiology, Molecular Epidemiology, Phylogeny, Point Mutation, Sequence Analysis, DNA, Avian Leukosis epidemiology, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, Genotype, Poultry Diseases epidemiology, Poultry Diseases virology

Abstract

Members of avian leukosis virus subgroup J (ALV-J) cause various diseases associated with tumor formation and decreased fertility, resulting in major economic losses in the poultry industry worldwide. To assess the status of ALV-J infection in meat-type chickens in southern China, the molecular epidemiology of ALV-J strains was investigated. A total of 265 clinical samples collected from southern China from 2013 to 2014 were investigated in this study for the presence of ALV-J, which resulted in 12 virus isolates. Phylogenetic analysis showed that 91.7 % (11/12) of the ALV-J isolates have possessed high homology to Chinese layer isolates and belong to one subgroup. One of the ALV isolates (designated GD1411-1) was relatively closely related to the ALV-J broiler isolates, indicating that the GD1411-1 isolate might be a transition strain. Several unique nucleotide substitutions in gp85 and the U3 region were detected in all 12 ALV-J isolates. This study provides some interesting information on the molecular characterization of ALV-J isolates. These findings will be beneficial for understanding of the pathogenic mechanism of ALV-J infection.

Published

2016

38. Isolation, identification and evolution analysis of a novel subgroup of avian leukosis virus isolated from a local Chinese yellow broiler in South China.

Author

Li X, Lin W, Chang S, Zhao P, Zhang X, Liu Y, Chen W, Li B, Shu D, Zhang H, Chen F, and Xie Q

Subjects

Animals, Avian Leukosis Virus classification, Avian Leukosis Virus physiology, China, Cluster Analysis, DNA, Viral genetics, Genome, Viral, Phylogeny, Sequence Analysis, DNA, Sequence Homology, Virus Replication, Avian Leukosis Virus genetics, Avian Leukosis Virus isolation & purification, Chickens virology, Evolution, Molecular, Genetic Variation, Proviruses genetics, Proviruses isolation & purification

Abstract

Avian leukosis virus (ALV) causes high mortality associated with tumor formation and decreased fertility, and results in major economic losses in the poultry industry worldwide. Recently, a putative novel ALV subgroup virus named ALV-K was observed in Chinese local chickens. In this study, a novel ALV strain named GD14LZ was isolated from a Chinese local yellow broiler in 2014. The proviral genome was sequenced and phylogenetically analyzed. The replication ability and pathogenicity of this virus were also evaluated. The complete proviral genome sequence of GD14LZ was 7482 nt in length, with a genetic organization typical of replication-competent type C retroviruses lacking viral oncogenes. Sequence analysis showed that the gag, pol and gp37 genes of GD14LZ have high sequence similarity to those of other ALV strains (A-E subgroups), especially to those of ALV-E. The gp85 gene of the GD14LZ isolate showed a low sequence similarity to those other ALV strains (A-E subgroups) but showed high similarity to strains previously described as ALV-K. Phylogenetic analysis of gp85 also suggested that the GD14LZ isolate was related to ALV-K strains. Further study showed that this isolate replicated more slowly and was less pathogenic than other ALV strains. These results indicate that the GD14LZ isolate belongs to the novel subgroup ALV-K and probably arose by recombination of ALV-K with endogenous viruses with low replication and pathogenicity. This virus might have existed in local Chinese chickens for a long time.

Published

2016

39. Synergy of subgroup J avian leukosis virus and Eimeria tenella to increase pathogenesis in specific-pathogen-free chickens.

Author

Cui N, Wang Q, Shi W, Han L, Wang J, Ma X, Li H, Wang F, Su S, and Zhao X

Subjects

Animals, Animals, Newborn, Avian Leukosis etiology, Avian Leukosis Virus classification, Chickens parasitology, Chickens virology, Coccidiosis etiology, Coccidiosis veterinary, Coinfection etiology, Coinfection veterinary, Cytokines genetics, Immunity, Cellular genetics, RNA, Messenger genetics, RNA, Messenger metabolism, Specific Pathogen-Free Organisms, Virulence, Avian Leukosis Virus immunology, Avian Leukosis Virus pathogenicity, Chickens immunology, Eimeria tenella immunology, Eimeria tenella pathogenicity

Abstract

To investigate the effects of co-infections of subgroup J avian leukosis virus (ALV-J) and Eimeria tenella on the pathogenesis in specific-pathogen-free (SPF) white leghorn chickens, groups of chickens were infected with ALV-J strain NX0101 at one day of age or with E. tenella at 14 days of age or both. The control group was left uninfected and was mock-inoculated with phosphate buffer saline (PBS). Mortality rates, body weights, cecal lesions, and viremia of infected chickens in each group were evaluated. Immune status was evaluated by measuring several parameters: immune organ weight/body weight index, specific humoral responses to inactivated NDV vaccine and to inoculated E. tenella, proportions of blood CD3+CD4+ and CD3+CD8α+ lymphocytes and transcriptional levels of cytokines in blood and cecal tonsils. The results show that co-infections of ALV-J and E. tenella induced a higher mortality rate and a lower body weight in SPF chickens compared to single-pathogen infection. In co-infected chickens, ALV-J accelerated the disease symptoms induced by E. tenella, and the E. tenella extended the ALV-J viremia. Thymus atrophy, decrease in the humoral response levels to pathogens and the NDV vaccine, modifications in the blood lymphocyte sub-populations and transcriptional cytokine disorders were found in co-infected chickens compared to chickens infected with one pathogen alone and to controls. We underline a synergy between ALV-J and E. tenella that results in increasing pathogenesis in SPF chickens., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

40. Analysis of Quasispecies of Avain Leukosis Virus Subgroup J Using Sanger and High-throughput Sequencing.

Author

Meng F, Dong X, Hu T, Liu Y, Zhao Y, Lv Y, Chang S, Zhao P, and Cui Z

Subjects

Amino Acid Sequence, Animals, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Chickens, Genetic Variation, High-Throughput Nucleotide Sequencing instrumentation, Molecular Sequence Data, Mutation, Phylogeny, Avian Leukosis virology, Avian Leukosis Virus isolation & purification, High-Throughput Nucleotide Sequencing methods, Poultry Diseases virology

Abstract

Background: Avian leukosis viruses subgroup J (ALV-J) exists as a complex mixture of different, but closely related genomes named quasispecies subjected to continuous change according to the Principles of Darwinian evolution., Method: The present study seeks to compare conventional Sanger sequencing with deep sequencing using MiSeq platform to study quasispecies dynamics of ALV-J., Results: The accuracy and reproducibility of MiSeq sequencing was determined better than Sanger sequencing by running each experiment in duplicate. According to the mutational rate of single position and the ability to distinguish dominant quasispecies with two sequencing methods, conventional Sanger sequencing technique displayed high randomness due to few sequencing samples, while deep sequencing could reflect the composition of the quasispecies more accurately. In the mean time, the research of quasispecies via Sanger sequencing was simulated and analyzed with the aid of re-sampling strategy with replacement for 1000 times repeat from high-throughput sequencing data, which indicated that the higher antibody titer, the higher sequence entropy, the harder analyzing with the conventional Sanger sequencing, resulted in lower ratios of dominant variants., Conclusions: In sum, deep sequencing is better suited for detecting rare variants comprehensively. The simulation of Sanger sequencing that we propose here will also help to standardize quasispecies researching under different selection pressure based on next-generation sequencing data.

Published

2016

41. Identification of avian leukosis virus subgroup J-associated acutely transforming viruses carrying the v-src oncogene in layer chickens.

Author

Wang Y, Li J, Li Y, Fang L, Sun X, Chang S, Zhao P, and Cui Z

Subjects

Animals, Avian Leukosis diagnosis, Base Sequence, DNA, Viral, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Chickens, Genes, src, Genome, Viral

Abstract

To elucidate the molecular basis for the rapid oncogenicity of an acutely transforming avian leukosis virus (ALV), isolated from fibrosarcomas in Hy-Line Brown commercial layer chickens infected with ALV subgroup J (ALV-J), the complete genomic structure of the provirus was determined. In addition to ALV-J replication-complete virus SDAU1102, five proviral DNA genomes, named SJ-1, SJ-2, SJ-3, SJ-4 and SJ-5, carrying different lengths of the v-src oncogene were amplified from original tumours and chicken embryo fibroblasts (CEFs) infected with viral stocks. The genomic sequences of the SJ-1-SJ-5 provirus were closely related to that of SDAU1102 but were defective. The results of Western blot analysis and immunohistochemical staining also showed overexpression of the p60v-src protein in infected CEFs and tumour tissue. To the best of our knowledge, this is the first report of the isolation and identification of acutely transforming viruses carrying the v-src oncogene with ALV-J as the helper virus. It also offers insight into the generation of acutely transforming ALVs carrying the v-src oncogene.

Published

2016

42. [Cross-species Transmission of Avian Leukosis Virus Subgroup J].

Author

Shen Y, He M, Zhang J, Zhao M, Wang G, and Cheng Z

Subjects

Amino Acid Sequence, Animals, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Chickens, Ducks virology, Galliformes virology, Host Specificity, Molecular Sequence Data, Quail virology, Sequence Alignment, Turkeys virology, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics, Viral Envelope Proteins metabolism, Avian Leukosis transmission, Avian Leukosis virology, Avian Leukosis Virus physiology, Poultry Diseases transmission, Poultry Diseases virology

Abstract

Avian leukosis virus subgroup J (ALV-J) is an avian retrovirus that can induce myelocytomas. A high-frequency mutation in gene envelope endows ALV-J with the potential for cross-species transmission. We wished to ascertain if the ALV-J can spread across species under selection pressure in susceptible and resistant hosts. First, we inoculated (in turn) two susceptible host birds (specific pathogen-free (SPF) chickens and turkeys). Then, we inoculated three resistant hosts (pheasants, quails and ducks) to detect the viral shedding, pathologic changes, and genetic evolution of different isolates. We found that pheasants and quails were infected under the selective pressure that accumulates stepwise in different hosts, and that ducks were not infected. Infection rates for SPF chickens and turkeys were 100% (16/16), whereas those for pheasants and quails were 37.5% (6/16) and 11.1% (3/27). Infected hosts showed immune tolerance, and inflammation and tissue damage could be seen in the liver, spleen, kidneys and cardiovascular system. Non-synonymous mutation and synonymous ratio (NS/S) analyses revealed the NS/S in hypervariable region (hr) 2 of pheasants and quails was 2.5. That finding suggested that mutation of isolates in pheasants and quails was induced by selective pressure from the resistant host, and that the hr2 region is a critical domain in cross-species transmission of ALV-J. Sequencing showed that ALV-J isolates from turkeys, pheasants and quails had moved away from the original virus, and were closer to the ALV-J prototype strain HPRS-103. However, the HPRS-103 strain cannot infect pheasants and quails, so further studies are needed.

Published

2016

43. Rapid detection of the common avian leukosis virus subgroups by real-time loop-mediated isothermal amplification.

Author

Peng H, Qin L, Bi Y, Wang P, Zou G, Li J, Yang Y, Zhong X, and Wei P

Subjects

Animals, Chickens, China, DNA Primers genetics, Sensitivity and Specificity, Temperature, Time Factors, Veterinary Medicine methods, Avian Leukosis diagnosis, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Molecular Diagnostic Techniques methods, Nucleic Acid Amplification Techniques methods

Abstract

Background: Subgroups A, B, E and J are the major subgroups of avian leukosis virus (ALV) infecting chickens. ALV infection has become endemic in China and has a significant negative effect on the poultry industry. Consequently, there is an urgent need for a specific, sensitive and rapid method for diagnosis and eradication of ALV. Therefore, we developed a simple and rapid real-time loop-mediated isothermal amplification (LAMP) reaction for the timely detection of the common ALV subgroups, whereby the amplification can be obtained in 35 min under isothermal conditions at 63 °C, ability to specific, sensitive and rapid detect all the common ALV subgroups., Methods: A set of four specific primers was designed to target the sequences of the pol gene of ALV, and the loop-mediated isothermal amplification (LAMP) assay were developed and compared with PCR and virus isolation methods., Results: The results from specificity of the LAMP assay showed that only target ALVs DNA was amplified. The LAMP assay demonstrated a sensitivity of 20 copies/reaction of ALV DNA, which was 10 times higher than the conventional PCR measurement. To further evaluate the reliability of the method, the assay was evaluated with ALV DNA from a panel of 81 clinical samples suspected of ALV infection. The results verify that the LAMP method was more sensitive than the conventional PCR and virus isolation method., Conclusion: In conclusion, the developed LAMP assay was a simple, inexpensive, sensitive method for the rapid detection of the most common subgroups of ALV, and it provided a useful and practical tool in the eradication program for ALV in the poultry industry.

Published

2015

44. MicroRNA-23b Promotes Avian Leukosis Virus Subgroup J (ALV-J) Replication by Targeting IRF1.

Author

Li Z, Chen B, Feng M, Ouyang H, Zheng M, Ye Q, Nie Q, and Zhang X

Subjects

3' Untranslated Regions, Animals, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, Gene Expression Profiling, Gene Expression Regulation, Gene Regulatory Networks, High-Throughput Nucleotide Sequencing, RNA, Messenger genetics, Reproducibility of Results, Transcriptome, Avian Leukosis genetics, Avian Leukosis virology, Avian Leukosis Virus physiology, Chickens, Interferon Regulatory Factor-1 genetics, MicroRNAs genetics, RNA Interference, Virus Replication

Abstract

Avian leukosis virus subgroup J (ALV-J) can cause several different leukemia-like proliferative diseases in the hemopoietic system of chickens. Here, we investigated the transcriptome profiles and miRNA expression profiles of ALV-J-infected and uninfected chicken spleens to identify the genes and miRNAs related to ALV-J invasion. In total, 252 genes and 167 miRNAs were differentially expressed in ALV-J-infected spleens compared to control uninfected spleens. miR-23b expression was up-regulated in ALV-J-infected spleens compared with the control spleens, and transcriptome analysis revealed that the expression of interferon regulatory factor 1 (IRF1) was down-regulated in ALV-J-infected spleens compared to uninfected spleens. A dual-luciferase reporter assay showed that IRF1 was a direct target of miR-23b. miR-23b overexpression significantly (P = 0.0022) decreased IRF1 mRNA levels and repressed IRF1-3'-UTR reporter activity. In vitro experiments revealed that miR-23b overexpression strengthened ALV-J replication, whereas miR-23b loss of function inhibited ALV-J replication. IRF1 overexpression inhibited ALV-J replication, and IRF1 knockdown enhanced ALV-J replication. Moreover, IRF1 overexpression significantly (P = 0.0014) increased IFN-β expression. In conclusion, these results suggested that miR-23b may play an important role in ALV-J replication by targeting IRF1.

Published

2015

45. Development and application of SYBR Green I real-time PCR assay for the separate detection of subgroup J Avian leukosis virus and multiplex detection of avian leukosis virus subgroups A and B.

Author

Dai M, Feng M, Liu D, Cao W, and Liao M

Subjects

Animals, Avian Leukosis diagnosis, Avian Leukosis Virus genetics, Benzothiazoles, Chickens, Diamines, Genes, Viral, Organic Chemicals, Quinolines, Reference Standards, Reproducibility of Results, Sensitivity and Specificity, Viral Load, Avian Leukosis virology, Avian Leukosis Virus classification, Multiplex Polymerase Chain Reaction methods, Real-Time Polymerase Chain Reaction methods

Abstract

Background: Subgroup A, B, and J ALVs are the most prevalent avian leukosis virus (ALV). Our study attempted to develop two SYBR Green I-based real-time PCR (RT-PCR) assays for specific detection of ALV subgroup J (ALV-J) and multiplex detection of ALV subgroups A and B (ALV-A/B), respectively., Results: The two assays showed high specificity for ALV-J and ALV-A/B and the sensitivity of the two assays was at least 100 times higher than that of the routine PCR assay. The minimum virus detection limit of virus culture, routine PCR and real-time PCR for detection of ALV-A strain was 10(3) TCID50 units, 10(2) TCID50 units and fewer than 10 TCID50 units, respectively. In addition, the coefficients of variation for intra- and inter-assay were both less than 5%. Forty clinical plasma samples were evaluated by real-time PCR, routine PCR, and virus culture with positive rates of 80% (32/40), 72.5% (29/40) and 62.5% (25/40), respectively. When the assay for detection of ALV-J was used to quantify the viral load of various organ tissues in chicken inoculated by ALV-J strains CHN06 and NX0101, the results exhibited that ALV-J genes could be detected in all organ tissues examined and the highest copies of ALV-J were mainly in heart and kidney samples at 30 weeks post-infection. Except in lung, the virus copies of CHN06 group were higher than that of NX0101 group in various organ tissues., Conclusions: The SYBR Green I-based real-time RT-PCR assay provides a powerful tool for the detection of ALV and study of virus replication and infection.

Published

2015

46. Genomic sequence analysis and biological characteristics of a rescued clone of avian leukosis virus strain JS11C1, isolated from indigenous chickens.

Author

Cui N, Su S, Chen Z, Zhao X, and Cui Z

Subjects

Animals, Avian Leukosis virology, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, Base Sequence, China, Cloning, Molecular, DNA, Viral genetics, Evolution, Molecular, Genome, Viral, Molecular Sequence Data, Phylogeny, Poultry Diseases virology, Sequence Homology, Nucleic Acid, Avian Leukosis Virus genetics, Chickens virology

Abstract

The strain JS11C1, a member of a putative new subgroup of avian leukosis virus (ALV) that is different from all six known subgroups from chickens based on Gp85 amino acid sequence comparison, was isolated from Chinese native chicken breeds in 2012. In order to further study the genome structure, biological characteristics, and the evolutionary relationship of the virus with others of known subgroups from infected chickens, we determined the complete genome sequence, constructed an infectious clone of ALV strain JS11C1, and performed comparative analysis using the whole genome sequence or elements with that of other ALVs available in GenBank. The results showed that the full-length sequence of the JS11C1 DNA provirus genome was 7707 bp, which is consistent with a genetic organization typical of a replication-competent type C retrovirus lacking viral oncogenes. The rescued infectious clone of JS11C1 showed similar growth rate and biological characteristics to its original virus. All the comparison analyses based on whole genomes support the opinion that the new isolates are relatively distantly related to any known subgroups of ALVs and might be classified as a new subgroup., (© 2014 The Authors.)

Published

2014

47. First finding of subgroup-E avian leukosis virus from wild ducks in China.

Author

Hao R, Han C, Liu L, and Zeng X

Subjects

Amino Acid Sequence, Animals, Avian Leukosis Virus classification, Avian Leukosis Virus genetics, Base Sequence, China epidemiology, Cloning, Molecular, Cluster Analysis, DNA Primers genetics, Molecular Sequence Data, Phylogeny, Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Sequence Homology, Species Specificity, Avian Leukosis epidemiology, Avian Leukosis virology, Avian Leukosis Virus isolation & purification, Ducks virology

Abstract

To analyze the status of avian leukosis virus subgroup E (ALV-E) in wild ducks in China, we collected 276 wild ducks, including 12 species, from four provinces of China. The PCR detection for ALV-E identified four samples as positive samples and the detection rate was 1.45%. The env sequences of ALV-E were cloned and sequenced. In gp85, genes of the four ALV-E strains showed a high homology (98.1-99.5%) with ev-1, ev-3, and SD0501 and more than 90% homology with other subgroup-A and subgroup-B avian leukosis viruses. However, they showed a slightly lower identity with subgroup-J (NX0101 and HPRS103), from 47.5 to 48.1%. Simultaneously, a further comparison with ALV-E representative isolates indicated that the amino acid substitutions of the four wild duck strains were distributed throughout the gp85. In total, these results suggested that the subgroup-E avian leukosis virus has been found in wild ducks in China., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published

2014

48. NHE1 gene associated with avian leukosis virus subgroup J infection in chicken.

Author

Chen B, Pan W, Zhang L, Liu J, Ouyang H, Nie Q, and Zhang X

Subjects

Alleles, Animals, Avian Leukosis Virus genetics, Avian Leukosis Virus immunology, Chickens, Female, Gene Expression, Genetic Predisposition to Disease, Genotype, Polymorphism, Single Nucleotide, Avian Leukosis genetics, Avian Leukosis Virus classification, Sodium-Hydrogen Exchangers genetics

Abstract

As a kind of binding protein, the type 1 Na(+)/H(+) exchanger (NHE1) is a receptor for the highly pathogenic Avian leukosis viruses-J subgroup (ALV-J) in chicken. In order to investigate the potential effect of chicken NHE1 gene on leukosis, we compared its expression between ALV-J-affected and -unaffected chicken, screened variations across the whole gene, and then performed association analysis with ALV-J affected/unaffected trait in three un-related chicken populations. We found that the NHE1 gene expressed in four immune tissues including spleen, bursa fabricius, liver, and thymus, and its expression was significantly up-regulated in liver and thymus of ALV-J-affected chickens (with leukosis phenotype) compared to -unaffected ones (ALV-J-negative controls). Thirty-six single nucleotide polymorphisms (SNP) were identified in a 6,105 bp region of the chicken NHE1 gene, giving rise to every 170 bp per SNP. Two SNP of g.4405A>G and g.5886C>G were genotyped with PCR-RFLP method. Results showed that g.4405A>G was significantly associated (P < 0.05) with ALV-J infection in all of the three chicken populations, including White Recessive Rock (WRR), Dwarf Yellow (DY) and Shiki Yellow (SY), while g.5886C>G was significantly associated (P < 0.05) with ALV-J infection in SY. These results indicated that the NHE1 gene was related to ALV-J infection in chicken.

Published

2014

49. Molecular characteristics of the complete genome of a J-subgroup avian leukosis virus strain isolated from Eurasian teal in China.

Author

Zeng X, Gao Y, Li D, Hao R, Liu W, Han C, Gao H, Qi X, Wang Y, Liu L, and Wang X

Subjects

Animals, Avian Leukosis Virus genetics, China, Cluster Analysis, DNA, Viral chemistry, Genotype, Molecular Sequence Data, Phylogeny, Proviruses classification, Proviruses genetics, Proviruses isolation & purification, Sequence Homology, Anseriformes virology, Avian Leukosis Virus classification, Avian Leukosis Virus isolation & purification, DNA, Viral genetics, Genome, Viral, Sequence Analysis, DNA

Abstract

The J-subgroup avian leukosis virus (ALV-J) strain WB11098J was isolated from a wild Eurasian teal, and its proviral genomic sequences were determined. The complete proviral sequence of WB11098J was 7868 nt long. WB11098J was 95.3.9 % identical to the prototype strain HPRS-103, 94.2 % identical to the American strain ADOL-7501, 94.5-94.7 % identical to Chinese broiler isolates, 94.8-97.5 % identical to layer chicken isolates, and 94.4-95.0 % identical to Chinese local chicken isolates at the nucleotide level. Phylogenetic analysis showed that the WB11098J isolate shared the greatest homology with the layer strain SD09DP03 and was included in the same cluster. Interestingly, two 19-bp insertions in the U3 regions of the 5'LTR and 5'UTR that were most likely derived from other retroviruses were found in the WB11098J isolate. These insertions separately introduced one E2BP-binding site in the U3 region of the 5'LTR and a RNA polymerase II transcription factor IIB and core promoter motif of ten elements in the 5'UTR. A 5-bp deletion was identified in the U3 region of the 5'LTR. No nucleotides were deleted in the rTM or DR-1 regions in the 3'UTR. A 1-bp deletion was detected in the E element and introduced a specific and distinct binding site for c-Ets-1. Our study is the first to report the molecular characteristics of the complete genome of an ALV-J that was isolated from a wild bird and will provide necessary information for further understanding of the evolution of ALV-J.

Published

2014

50. Synergetic effects of subgroup J avian leukosis virus and reticuloendotheliosis virus co-infection on growth retardation and immunosuppression in SPF chickens.

Author

Dong X, Ju S, Zhao P, Li Y, Meng F, Sun P, and Cui Z

Subjects

Animals, Avian Leukosis Virus isolation & purification, Bursa of Fabricius pathology, Bursa of Fabricius virology, Newcastle disease virus, Retroviridae Infections virology, Specific Pathogen-Free Organisms, Thymus Gland pathology, Thymus Gland virology, Tumor Virus Infections virology, Avian Leukosis Virus classification, Chickens, Coinfection, Poultry Diseases virology, Reticuloendotheliosis virus isolation & purification, Retroviridae Infections veterinary, Tumor Virus Infections veterinary

Abstract

To further understand the effect of co-infection of subgroup J avian leukosis virus (ALV-J) and reticuloendotheliosis virus (REV) in specific-pathogen-free (SPF) white leghorn chickens, the experiment was made to study the pathogenicity, the weight of body and immune organs, response to newcastle disease virus (NDV) and avian influenza virus subtype H9 (AIV-H9) vaccination. Chickens were randomly divided into four groups, which includes injection groups (REV, ALV-J, REV plus ALV-J), and negative control group. The pathogenesis experiments indicated that chickens co-infected with REV and ALV-J had significantly higher mortality rate than those of the chickens infected with REV or ALV-J alone (P<0.05). Chickens inoculated with REV and ALV-J had significantly lower weights than chickens in all other groups (P<0.05). There were no significant differences between the two single infection groups and co-infection group (P>0.05) on bursa and thymus over body wt ratios, however, chickens co-infected with REV and ALV-J had significantly lower titers than REV-infected chickens and ALV-J-infected chickens on HI antibody titers to ND and AIV-H9 after vaccination (P<0.05). These findings suggested that the co-infection of REV and ALV-J caused more serious growth retardation and immunosuppression in SPF chickens., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published

2014