Your search keyword '"Xie, Zhixun"' showing total 41 results

1. A multiplex fluorescence-based loop-mediated isothermal amplification assay for identifying chicken parvovirus, chicken infectious anaemia virus, and fowl aviadenovirus serotype 4.

Author

Fan, Qing, Xie, Zhixun, Zhang, Yanfang, Xie, Zhiqin, Xie, Liji, Huang, Jiaoling, Zeng, Tingting, Wang, Sheng, Luo, Sisi, and Li, Meng

Subjects

*PARVOVIRUSES, *PARVOVIRUS B19, *POULTRY, *COMORBIDITY, *MIXED infections, *CHICKENS, *ANEMIA

Abstract

Chicken parvovirus (ChPV), chicken infectious anaemia virus (CIAV) and fowl adenovirus serotype 4 (FAdV-4) are avian viruses that have emerged in recent years and have endangered the global poultry industry, causing great economic loss. In this study, a multiplex fluorescence-based loop-mediated isothermal amplification (mLAMP) assay for detecting ChPV, CIAV and FAdV-4 was developed to simultaneously diagnose single and mixed infections in chickens. Three primer sets and composite probes were designed according to the conserved regions of the NS gene of ChPV, VP1 gene of CIAV and hexon gene of FAdV-4. Each composite probe was labelled with a different fluorophore, which was detached to release the fluorescence signal after amplification. The target viruses were distinguished based on the colour of the mLAMP products. The mLAMP assay was shown to be sensitive, with detection limits of 307 copies of recombinant plasmids containing the ChPV target genes, 749 copies of CIAV and 648 copies of FAdV-4. The assay exhibited good specificity and no cross-reactivity with other symptomatically related avian viruses. When used on field materials, the results of the mLAMP assay were in 100% agreement with those of the previously published PCR assay. The mLAMP assay is rapid, economical, sensitive and specific, and the results of amplification are directly observable by eye. Therefore, the mLAMP assay is a useful tool for the clinical detection of ChPV, CIAV and FAdV-4 and can be applied in rural areas. [ABSTRACT FROM AUTHOR]

Published

2023

2. Development of a visual multiplex fluorescent LAMP assay for the detection of foot-and-mouth disease, vesicular stomatitis and bluetongue viruses.

Author

Fan, Qing, Xie, Zhixun, Wei, You, Zhang, Yanfang, Xie, Zhiqin, Xie, Liji, Huang, Jiaoling, Zeng, Tingting, Wang, Sheng, Luo, Sisi, and Li, Meng

Subjects

*FLUORESCENT lamps, *VESICULAR stomatitis, *LOOP-mediated isothermal amplification, *BLUETONGUE virus, *FOOT & mouth disease, *BLUETONGUE, *PLANT viruses

Abstract

Loop-mediated isothermal amplification (LAMP) is a nucleic acid amplification technique that can be used to amplify target genes at a constant temperature, and it has several advantages, including convenience, specificity and sensitivity. However, due to the special interpretation methods of this technology for reaction results, all the previously reported LAMP detection methods have been restricted to identifying a single target, which limits the application of this technology. In this study, we modified conventional LAMP to include a quencher-fluorophore composite probe complementary to the F1c segment of the inner primer FIP; upon strand separation, a gain in the visible fluorescent signal was observed. The probes could be labeled with different fluorophores, showing different colors at the corresponding wavelengths. Therefore, this multiplex LAMP (mLAMP) assay can simultaneously detect 1–3 target sequences in a single LAMP reaction tube, and the results are more accurate and intuitive. In this study, we comprehensively demonstrated a single-reaction mLAMP assay for the robust detection of three cattle viruses without nonspecific amplification of other related pathogenic cattle viruses. The detection limit of this mLAMP assay was as low as 526–2477 copies/reaction for the recombinant plasmids. It is expected that this mLAMP assay can be widely used in clinical diagnosis. [ABSTRACT FROM AUTHOR]

Published

2022

3. Survey of low pathogenic avian influenza viruses in live poultry markets in Guangxi Province, Southern China, 2016–2019.

Author

Luo, Sisi, Xie, Zhixun, Li, Meng, Li, Dan, Xie, Liji, Huang, Jiaoling, Zhang, Minxiu, Zeng, Tingting, Wang, Sheng, Fan, Qing, Zhang, Yanfang, Xie, Zhiqin, Deng, Xianwen, and Liu, Jiabo

Subjects

*AVIAN influenza, *AVIAN influenza A virus, *COVID-19, *POULTRY, *MIXED infections, *VIRUS virulence, *DISEASE management

Abstract

Low pathogenic avian influenza viruses (LPAIVs) have been widespread in poultry and wild birds throughout the world for many decades. LPAIV infections are usually asymptomatic or cause subclinical symptoms. However, the genetic reassortment of LPAIVs may generate novel viruses with increased virulence and cross-species transmission, posing potential risks to public health. To evaluate the epidemic potential and infection landscape of LPAIVs in Guangxi Province, China, we collected and analyzed throat and cloacal swab samples from chickens, ducks and geese from the live poultry markets on a regular basis from 2016 to 2019. Among the 7,567 samples, 974 (12.87%) were LPAIVs-positive, with 890 single and 84 mixed infections. Higher yearly isolation rates were observed in 2017 and 2018. Additionally, geese had the highest isolation rate, followed by ducks and chickens. Seasonally, spring had the highest isolation rate. Subtype H3, H4, H6 and H9 viruses were detected over prolonged periods, while H1 and H11 viruses were detected transiently. The predominant subtypes in chickens, ducks and geese were H9, H3, and H6, respectively. The 84 mixed infection samples contained 22 combinations. Most mixed infections involved two subtypes, with H3 + H4 as the most common combination. Our study provides important epidemiological data regarding the isolation rates, distributions of prevalent subtypes and mixed infections of LPAIVs. These results will improve our knowledge and ability to control epidemics, guide disease management strategies and provide early awareness of newly emerged AIV reassortants with pandemic potential. [ABSTRACT FROM AUTHOR]

Published

2021

4. Study of the activation of the PI3K/Akt pathway by the motif of σ A and σ NS proteins of avian reovirus.

Author

Xie, Liji, Xie, Zhixun, Wang, Sheng, Deng, Xianwen, and Xie, Zhiqin

Subjects

*GENETIC engineering, *CELLULAR signal transduction, *WESTERN immunoblotting, *PROTEINS

Abstract

The present study was conducted to determine whether avian reovirus (ARV) activates the phosphatidylinositol 3-kinase-dependent Akt (PI3K/Akt) pathway according to the PXXP or YXXXM motifs of σA and σNS proteins. Gene splicing by overlap extension PCR was used to change the PXXP or YXXXM motifs of the σA and σNS genes. Plasmid constructs that contain mutant σA and σNS genes were generated and transfected into Vero cells, and the expression levels of the corresponding genes were quantified according to immunofluorescence and Western blot analyses. The Akt phosphorylation (P-Akt) profile of the transfected Vero cells was examined by flow cytometry and Western blot. The results showed that the σA and σNS genes were expressed in the Vero cells, and P-Akt expression in the σA mutant groups (amino acids 110–114 and 114–117) was markedly decreased. The results indicated that the σA protein of ARV activates the PI3K/Akt pathway via the PXXP motif. The results of this study reveal the mechanisms by which ARV manipulates the cellular signal transduction pathways, which may provide new ideas for novel drug targets. [ABSTRACT FROM AUTHOR]

Published

2020

5. Altered gene expression profiles of the MDA5 signaling pathway in peripheral blood lymphocytes of chickens infected with avian reovirus.

Author

Xie, Liji, Xie, Zhixun, Wang, Sheng, Huang, Jiaoling, Deng, Xianwen, Xie, Zhiqin, Luo, Sisi, Zeng, Tingting, Zhang, Yanfang, and Zhang, Minxiu

Subjects

*GENE expression profiling, *INFECTIOUS arthritis, *CHICKEN diseases, *POULTRY industry, *LYMPHOCYTES, *NECROTIC enteritis, *CHICKENS

Abstract

Avian reovirus (ARV) is a member of the genus Orthoreovirus in the family Reoviridae and causes a severe syndrome including viral arthritis that leads to considerable losses in the poultry industry. Innate immunity plays a significant role in host defense against ARV. Here, we explored the interaction between ARV and the host innate immune system by measuring mRNA expression levels of several genes associated with the MDA5 signaling pathway. The results showed that expression peaks for MDA5, MAVS, TRAF3, TRAF6, IRF7, IKKɛ, TBK1 and NF-κB occurred at 3 days postinfection (dpi). Moreover, type I IFN (IFN-α, IFN-β) and IL-12 expression levels peaked at 3 dpi, while type II IFN (IFN-γ), IL-6, IL-17 and IL-18 expression reached a maximum level at 1 dpi. IL-8 changed at 5 dpi, and IL-1β and TNF-α changed at 7 dpi. Interestingly, several key IFN-stimulated genes (ISGs), including IFITM1, IFITM2, IFITM5, Mx1 and OASL, were simultaneously upregulated and reached maximum values at 3 dpi. These data indicate that the MDA5 signaling pathway and innate immune cytokines were induced after ARV infection, which would contribute to the ARV-host interaction, especially at the early infection stage. [ABSTRACT FROM AUTHOR]

Published

2019

6. Analysis of Chicken IFITM3 Gene Expression and Its Effect on Avian Reovirus Replication.

Author

Ren, Hongyu, Wang, Sheng, Xie, Zhixun, Wan, Lijun, Xie, Liji, Luo, Sisi, Li, Meng, Xie, Zhiqin, Fan, Qing, Zeng, Tingting, Zhang, Yanfang, Zhang, Minxiu, Huang, Jiaoling, and Wei, You

Subjects

*CHICKENS, *GENE expression, *CANARIES, *MALLARD, *LARGE intestine, *CHICKEN embryos, *INTERFERON receptors

Abstract

Interferon-inducible transmembrane protein 3 (IFITM3) is an antiviral factor that plays an important role in the host innate immune response against viruses. Previous studies have shown that IFITM3 is upregulated in various tissues and organs after avian reovirus (ARV) infection, which suggests that IFITM3 may be involved in the antiviral response after ARV infection. In this study, the chicken IFITM3 gene was cloned and analyzed bioinformatically. Then, the role of chicken IFITM3 in ARV infection was further explored. The results showed that the molecular weight of the chicken IFITM3 protein was approximately 13 kDa. This protein was found to be localized mainly in the cytoplasm, and its protein structure contained the CD225 domain. The homology analysis and phylogenetic tree analysis showed that the IFITM3 genes of different species exhibited great variation during genetic evolution, and chicken IFITM3 shared the highest homology with that of Anas platyrhynchos and displayed relatively low homology with those of birds such as Anser cygnoides and Serinus canaria. An analysis of the distribution of chicken IFITM3 in tissues and organs revealed that the IFITM3 gene was expressed at its highest level in the intestine and in large quantities in immune organs, such as the bursa of Fabricius, thymus and spleen. Further studies showed that the overexpression of IFITM3 in chicken embryo fibroblasts (DF-1) could inhibit the replication of ARV, whereas the inhibition of IFITM3 expression in DF-1 cells promoted ARV replication. In addition, chicken IFITM3 may exert negative feedback regulatory effects on the expression of TBK1, IFN-γ and IRF1 during ARV infection, and it is speculated that IFITM3 may participate in the innate immune response after ARV infection by negatively regulating the expression of TBK1, IFN-γ and IRF1. The results of this study further enrich the understanding of the role and function of chicken IFITM3 in ARV infection and provide a theoretical basis for an in-depth understanding of the antiviral mechanism of host resistance to ARV infection. [ABSTRACT FROM AUTHOR]

Published

2024

7. Development of duplex fluorescence-based loop-mediated isothermal amplification assay for detection of Mycoplasma bovis and bovine herpes virus 1.

Author

Fan, Qing, Xie, Zhixun, Xie, Zhiqin, Xie, Liji, Huang, Jiaoling, Zhang, Yanfan, Zeng, Tingting, Zhang, Minxiu, Wan, Sheng, Luo, Sisi, Liu, Jiabo, and Deng, Xianwen

Subjects

*MYCOPLASMA bovis, *BOVINE herpesvirus-1, *GENE amplification, *RESPIRATORY disease diagnosis, *FLUORESCENCE, *VIRUSES

Abstract

Highlights • A DLAMP method was developed for simultaneous detection of MB and BHV-1 and applied to clinical samples. • The DLAMP results were visualized by the colors of fluorescent-dye-conjugated DLAMP products. • The DLAMP assay shows high specificity and sensitivity. Abstract Mycoplasma bovis (MB) and bovine herpes virus 1 (BHV-1) are two important pathogens that cause bovine respiratory disease in the beef feedlot and dairy industries. The aim of this study was to develop and validate a duplex fluorescence-based loop-mediated isothermal amplification (DLAMP) assay for simultaneous detection of MB and BHV-1. Two sets of specific primers for each pathogen were designed to target the unique sequences of the MB uvrC gene and the BHV-1 gB gene. The inner primer for BHV-1 was synthesized with the fluorophore FAM at the 5′ end to detect the BHV-1 gB gene, and the inner primer for MB was synthesized with the fluorophore CY5 at the 5′ end to detect the MB uvrC gene. The DLAMP reaction conditions were optimized for rapid and specific detection of MB and BHV-1. The DLAMP assay developed here could specifically detect MB and BHV-1 without cross-reaction with other known non-target bovine pathogens. The sensitivity of this DLAMP assay was as low as 2 × 102 copies for recombinant plasmids containing the MB and BHV-1 target genes. In a detection test of 125 clinical samples, the positive rates for MB, BHV-1 and co-infection were 44.8%, 13.6% and 1.6%, respectively. Furthermore, the sensitivity and specificity of DLAMP were determined as 95%–96.6% and 100%, respectively, of those of field sample detection by the real-time polymerase chain reaction (PCR) assay recommended by the World Organisation for Animal Health. Overall, DLAMP provides a rapid, sensitive and specific assay for the identification of MB and BHV-1 in clinical specimens and for epidemiological surveillance. [ABSTRACT FROM AUTHOR]

Published

2018

8. Transcriptomic and Translatomic Analyses Reveal Insights into the Signaling Pathways of the Innate Immune Response in the Spleens of SPF Chickens Infected with Avian Reovirus.

Author

Wang, Sheng, Huang, Tengda, Xie, Zhixun, Wan, Lijun, Ren, Hongyu, Wu, Tian, Xie, Liji, Luo, Sisi, Li, Meng, Xie, Zhiqin, Fan, Qing, Huang, Jiaoling, Zeng, Tingting, Zhang, Yanfang, Zhang, Minxiu, and Wei, You

Subjects

*REOVIRUSES, *IMMUNE response, *CELLULAR signal transduction, *INFECTIOUS arthritis, *GENE expression, *SPLEEN

Abstract

Avian reovirus (ARV) infection is prevalent in farmed poultry and causes viral arthritis and severe immunosuppression. The spleen plays a very important part in protecting hosts against infectious pathogens. In this research, transcriptome and translatome sequencing technology were combined to investigate the mechanisms of transcriptional and translational regulation in the spleen after ARV infection. On a genome-wide scale, ARV infection can significantly reduce the translation efficiency (TE) of splenic genes. Differentially expressed translational efficiency genes (DTEGs) were identified, including 15 upregulated DTEGs and 396 downregulated DTEGs. These DTEGs were mainly enriched in immune regulation signaling pathways, which indicates that ARV infection reduces the innate immune response in the spleen. In addition, combined analyses revealed that the innate immune response involves the effects of transcriptional and translational regulation. Moreover, we discovered the key gene IL4I1, the most significantly upregulated gene at both the transcriptional and translational levels. Further studies in DF1 cells showed that overexpression of IL4I1 could inhibit the replication of ARV, while inhibiting the expression of endogenous IL4I1 with siRNA promoted the replication of ARV. Overexpression of IL4I1 significantly downregulated the mRNA expression of IFN-β, LGP2, TBK1 and NF-κB; however, the expression of these genes was significantly upregulated after inhibition of IL4I1, suggesting that IL4I1 may be a negative feedback effect of innate immune signaling pathways. In addition, there may be an interaction between IL4I1 and ARV σA protein, and we speculate that the IL4I1 protein plays a regulatory role by interacting with the σA protein. This study not only provides a new perspective on the regulatory mechanisms of the innate immune response after ARV infection but also enriches the knowledge of the host defense mechanisms against ARV invasion and the outcome of ARV evasion of the host's innate immune response. [ABSTRACT FROM AUTHOR]

Published

2023

9. Development of a GeXP-multiplex PCR assay for the simultaneous detection and differentiation of six cattle viruses.

Author

Fan, Qing, Xie, Zhixun, Xie, Zhiqin, Deng, Xianwen, Xie, Liji, Huang, Li, Luo, Sisi, Huang, Jiaoling, Zhang, Yanfang, Zeng, Tingting, Wang, Sheng, Liu, Jiabo, and Pang, Yaoshan

Subjects

*GENE expression, *MOLECULAR genetics, *NON-coding RNA, *EPIDEMIOLOGICAL research, *ELECTROPHORESIS

Abstract

Foot-and-mouth disease virus (FMDV), Bluetongue virus (BTV), Vesicular stomatitis Virus (VSV), Bovine viral diarrheal (BVDV), Bovine rotavirus (BRV), and Bovine herpesvirus 1 (IBRV) are common cattle infectious viruses that cause a great economic loss every year in many parts of the world. A rapid and high-throughput GenomeLab Gene Expression Profiler (GeXP) analyzer-based multiplex PCR assay was developed for the simultaneous detection and differentiation of these six cattle viruses. Six pairs of chimeric primers consisting of both the gene-specific primer and a universal primer were designed and used for amplification. Then capillary electrophoresis was used to separate the fluorescent labeled PCR products according to the amplicons size. The specificity of GeXP-multiplex PCR assay was examined with samples of the single template and mixed template of six viruses. The sensitivity was evaluated using the GeXP-multiplex PCR assay on serial 10-fold dilutions of ssRNAs obtained via in vitro transcription. To further evaluate the reliability, 305 clinical samples were tested by the GeXP-multiplex PCR assay. The results showed that the corresponding virus specific fragments of genes were amplified. The detection limit of the GeXP-multiplex PCR assay was 100 copies/μL in a mixed sample of ssRNAs containing target genes of six different cattle viruses, whereas the detection limit for the Gexp-mono PCR assay for a single target gene was 10 copies/μL. In detection of viruses in 305 clinical samples, the results of GeXP were consistent with simplex real-time PCR. Analysis of positive samples by sequencing demonstrated that the GeXP-multiplex PCR assay had no false positive samples of nonspecific amplification. In conclusion, this GeXP-multiplex PCR assay is a high throughput, specific, sensitive, rapid and simple method for the detection and differentiation of six cattle viruses. It is an effective tool that can be applied for the rapid differential diagnosis of clinical samples and for epidemiological investigation. [ABSTRACT FROM AUTHOR]

Published

2017

10. Genetic and phylogenetic analysis of a novel parvovirus isolated from chickens in Guangxi, China.

Author

Feng, Bin, Xie, Zhixun, Deng, Xianwen, Xie, Liji, Xie, Zhiqin, Huang, Li, Fan, Qin, Luo, Sisi, Huang, Jiaoling, Zhang, Yanfang, Zeng, Tingting, Wang, Sheng, and Wang, Leyi

Subjects

*PARVOVIRUS diseases, *CHICKEN diseases, *NUCLEOTIDE sequencing, *VIRAL genomes, *INFECTIOUS disease transmission, *DIAGNOSIS

Abstract

A previously unidentified chicken parvovirus (ChPV) strain, associated with runting-stunting syndrome (RSS), is now endemic among chickens in China. To explore the genetic diversity of ChPV strains, we determined the first complete genome sequence of a novel ChPV isolate (GX-CH-PV-7) identified in chickens in Guang Xi, China, and showed moderate genome sequence similarity to reference strains. Analysis showed that the viral genome sequence is 86.4 %-93.9 % identical to those of other ChPVs. Genetic and phylogenetic analyses showed that this newly emergent GX-CH-PV-7 is closely related to Gallus gallus enteric parvovirus isolate ChPV 798 from the USA, indicating that they may share a common ancestor. The complete DNA sequence is 4612 bp long with an A+T content of 56.66 %. We determined the first complete genome sequence of a previously unidentified ChPV strain to elucidate its origin and evolutionary status. [ABSTRACT FROM AUTHOR]

Published

2016

11. Avian reovirus σA and σNS proteins activate the phosphatidylinositol 3-kinase-dependent Akt signalling pathway.

Author

Xie, Liji, Xie, Zhixun, Huang, Li, Fan, Qing, Luo, Sisi, Huang, Jiaoling, Deng, Xianwen, Xie, Zhiqin, Zeng, Tingting, Zhang, Yanfang, and Wang, Sheng

Subjects

*REOVIRUSES, *VIRAL proteins, *PHOSPHATIDYLINOSITOL 3-kinases, *PROTEIN kinase B, *VIRAL genes, *AMINO acid sequence

Abstract

The present study was conducted to identify avian reovirus (ARV) proteins that can activate the phosphatidylinositol 3-kinase (PI3K)-dependent Akt pathway. Based on ARV protein amino acid sequence analysis, σA, σNS, μA, μB and μNS were identified as putative proteins capable of mediating PI3K/Akt pathway activation. The recombinant plasmids σA-pcAGEN, σNS-pcAGEN, μA-pcAGEN, μB-pcAGEN and μNS-pcAGEN were constructed and used to transfect Vero cells, and the expression levels of the corresponding genes were quantified by immunofluorescence and Western blot analysis. Phosphorylated Akt (P-Akt) levels in the transfected cells were measured by flow cytometry and Western blot analysis. The results showed that the σA, σNS, μA, μB and μNS genes were expressed in Vero cells. σA-expressing and σNS-expressing cells had higher P-Akt levels than negative control cells, pcAGEN-expressing cells and cells designed to express other proteins (i.e., μA, μB and μNS). Pre-treatment with the PI3K inhibitor LY294002 inhibited Akt phosphorylation in σA- and σNS-expressing cells. These results indicate that the σA and σNS proteins can activate the PI3K/Akt pathway. [ABSTRACT FROM AUTHOR]

Published

2016

12. Silver nanoparticles coated graphene electrochemical sensor for the ultrasensitive analysis of avian influenza virus H7.

Author

Huang, Jiaoling, Xie, Zhixun, Xie, Zhiqin, Luo, Sisi, Xie, Liji, Huang, Li, Fan, Qing, Zhang, Yanfang, Wang, Sheng, and Zeng, Tingting

Subjects

*ELECTROCHEMICAL sensors, *SILVER nanoparticles, *GRAPHENE, *SURFACE coatings, *AVIAN influenza A virus, *MONOCLONAL antibodies

Abstract

A new, highly sensitive electrochemical immunosensor with a sandwich-type immunoassay format was designed to quantify avian influenza virus H7 (AIV H7) by using silver nanoparticle-graphene (AgNPs-G) as trace labels in clinical immunoassays. The device consists of a gold electrode coated with gold nanoparticle-graphene nanocomposites (AuNPs-G), the gold nanoparticle surface of which can be further modified with H7-monoclonal antibodies (MAbs). The immunoassay was performed with H7-polyclonal antibodies (PAbs) that were attached to the AgNPs-G surface (PAb-AgNPs-G). This method of using PAb-AgNPs-G as detection antibodies shows high signal amplification and exhibits a dynamic working range of 1.6 × 10 −3 ∼16 ng/mL, with a low detection limit of 1.6 pg/mL at a signal-to-noise ratio of 3σ. In summary, we showed that this novel immunosensor is highly specific and sensitive to AIV H7, and the established assay could potentially be applied to rapidly detect other pathogenic microorganisms. [ABSTRACT FROM AUTHOR]

Published

2016

13. Simultaneous detection of four different neuraminidase types of avian influenza A H5 viruses by multiplex reverse transcription PCR using a Ge XP analyser.

Author

Li, Meng, Xie, Zhixun, Xie, Zhiqin, Liu, Jiabo, Xie, Liji, Deng, Xianwen, Luo, Sisi, Fan, Qing, Huang, Li, Huang, Jiaoling, Zhang, Yanfang, Zeng, Tingting, and Feng, Jiaxun

Subjects

*NEURAMINIDASE, *REVERSE transcriptase polymerase chain reaction, *AVIAN influenza, *GERMANIUM, *NUCLEOTIDE sequence

Abstract

Objectives In order to develop a multiplex RT- PCR assay using the Ge XP analyser for the simultaneous detection of four different NA serotypes of H5-subtype AIVs, effective to control and reduce H5 subtype of avian influenza outbreak. Design Six pairs of primers were designed using conserved and specific sequences of the AIV subtypes H5, N1, N2, N6 and N8 in GenBank. Each gene-specific primer was fused at the 5′ end to a universal sequence to generate six pairs of chimeric primers, and one pair of universal primers was used for RT- PCR, and PCR product separation and detection were performed by capillary electrophoresis using the GenomeLab Ge XP genetic analysis system. Setting Single and mixed avian pathogen cDNA/ DNA templates were employed to evaluate the specificity of a multiplex assay with a Ge XP analyser. Corresponding specific DNA products were amplified for each gene, revealing amplification peaks for M, H5, N1, N2, N6 and N8 genes from four different NA subtypes of influenza A H5 virus. Sample A total of 180 cloacal swabs were collected from poultry at live bird markets. Main outcome measures The multiplex PCR assay demonstrated excellent specificity, with each pair of specific primers generating only products corresponding to the target genes and without cross-amplification with other NA-subtype influenza viruses or other avian pathogens. Using various premixed ss RNAs containing known AIV target genes, the detection limit for the multiplex assay was determined to be 102 copies/μl. The Ge XP assay was further evaluated using 180 clinical specimens and compared with RRT- PCR (real-time reverse transcriptase PCR) and virus isolation. Conclusions This Ge XP analyser-based multiplex assay for four different NA subtypes of H5 HPAI viruses is both highly specific and sensitive and can be used as a rapid and direct diagnostic assay for testing clinical samples. [ABSTRACT FROM AUTHOR]

Published

2016

14. Molecular characterization of emerging chicken and turkey parvovirus variants and novel strains in Guangxi, China.

Author

Zhang, Yanfang, Feng, Bin, Xie, Zhixun, Zhang, Minxiu, Fan, Qing, Deng, Xianwen, Xie, Zhiqin, Li, Meng, Zeng, Tingting, Xie, Liji, Luo, Sisi, Huang, Jiaoling, and Wang, Sheng

Subjects

*WHOLE genome sequencing, *CHICKENS, *AMINO acid sequence, *SEQUENCE alignment, *NUCLEOTIDE sequence

Abstract

Avian parvoviruses cause several enteric poultry diseases that have been increasingly diagnosed in Guangxi, China, since 2014. In this study, the whole-genome sequences of 32 strains of chicken parvovirus (ChPV) and 3 strains of turkey parvovirus (TuPV) were obtained by traditional PCR techniques. Phylogenetic analyses of 3 genes and full genome sequences were carried out, and 35 of the Guangxi ChPV/TuPV field strains were genetically different from 17 classic ChPV/TuPV reference strains. The nucleotide sequence alignment between ChPVs/TuPVs from Guangxi and other countries revealed 85.2–99.9% similarity, and the amino acid sequences showed 87.8–100% identity. The phylogenetic tree of these sequences could be divided into 6 distinct ChPV/TuPV groups. More importantly, 3 novel ChPV/TuPV groups were identified for the first time. Recombination analysis with RDP 5.0 revealed 15 recombinants in 35 ChPV/TuPV isolates. These recombination events were further confirmed by Simplot 3.5.1 analysis. Phylogenetic analysis based on full genomes showed that Guangxi ChPV/TuPV strains did not cluster according to their geographic origin, and the identified Guangxi ChPV/TuPV strains differed from the reference strains. Overall, whole-genome characterizations of emerging Guangxi ChPV and TuPV field strains will provide more detailed insights into ChPV/TuPV mutations and recombination and their relationships with molecular epidemiological features. [ABSTRACT FROM AUTHOR]

Published

2023

15. Simultaneous detection of eight swine reproductive and respiratory pathogens using a novel GeXP analyser-based multiplex PCR assay.

Author

Zhang, Minxiu, Xie, Zhixun, Xie, Liji, Deng, Xianwen, Xie, Zhiqin, Luo, Sisi, Liu, Jiabo, Pang, Yaoshan, and Khan, Mazhar I.

Subjects

*PORCINE reproductive & respiratory syndrome, *POLYMERASE chain reaction, *VIRUS identification, *GENE expression profiling, *CLASSICAL swine fever virus, *RNA viruses, *DIAGNOSIS

Abstract

A new high-throughput GenomeLab Gene Expression Profiler (GeXP) analyser-based multiplex PCR assay was developed for the detection of eight reproductive and respiratory pathogens in swine. The reproductive and respiratory pathogens include North American porcine reproductive and respiratory syndrome virus (PRRSV-NA), classical swine fever virus (CSFV), porcine circovirus 2 (PCV-2), swine influenza virus (SIV) (including H1 and H3 subtypes), porcine parvovirus (PPV), pseudorabies virus (PRV) and Japanese encephalitis virus (JEV). Nine pairs of specific chimeric primers were designed and used to initiate PCRs, and one pair of universal primers was used for subsequent PCR cycles. The specificity of the GeXP assay was examined using positive controls for each virus. The sensitivity was evaluated using serial ten-fold dilutions of in vitro-transcribed RNA from all of the RNA viruses and plasmids from DNA viruses. The GeXP assay was further evaluated using 114 clinical specimens and was compared with real-time PCR/single RT-PCR methods. The specificity of the GeXP assay for each pathogen was examined using single cDNA/DNA template. Specific amplification peaks of the reproductive and respiratory pathogens were observed on the GeXP analyser. The minimum copies per reaction detected for each virus by the GeXP assay were as follows: 1000 copies/μl for PRV; 100 copies/μl for CSFV, JEV, PCV-2 and PPV; and 10 copies/μl for SIV-H1, SIV-H3 and PRRSV-NA. Analysis of 114 clinical samples using the GeXP assay demonstrated that the GeXP assay had comparable detection to real-time PCR/single RT-PCR. This study demonstrated that the GeXP assay is a new method with high sensitivity and specificity for the identification of these swine reproductive and respiratory pathogens. The GeXP assay may be adopted for molecular epidemiological surveys of these reproductive and respiratory pathogens in swine populations. [ABSTRACT FROM AUTHOR]

Published

2015

16. Molecular characterization of emerging chicken and turkey parvovirus variants and novel strains in Guangxi, China.

Author

Zhang, Yanfang, Feng, Bin, Xie, Zhixun, Zhang, Minxiu, Fan, Qing, Deng, Xianwen, Xie, Zhiqin, Li, Meng, Zeng, Tingting, Xie, Liji, Luo, Sisi, Huang, Jiaoling, and Wang, Sheng

Subjects

*WHOLE genome sequencing, *CHICKENS, *AMINO acid sequence, *SEQUENCE alignment, *NUCLEOTIDE sequence

Abstract

Avian parvoviruses cause several enteric poultry diseases that have been increasingly diagnosed in Guangxi, China, since 2014. In this study, the whole-genome sequences of 32 strains of chicken parvovirus (ChPV) and 3 strains of turkey parvovirus (TuPV) were obtained by traditional PCR techniques. Phylogenetic analyses of 3 genes and full genome sequences were carried out, and 35 of the Guangxi ChPV/TuPV field strains were genetically different from 17 classic ChPV/TuPV reference strains. The nucleotide sequence alignment between ChPVs/TuPVs from Guangxi and other countries revealed 85.2–99.9% similarity, and the amino acid sequences showed 87.8–100% identity. The phylogenetic tree of these sequences could be divided into 6 distinct ChPV/TuPV groups. More importantly, 3 novel ChPV/TuPV groups were identified for the first time. Recombination analysis with RDP 5.0 revealed 15 recombinants in 35 ChPV/TuPV isolates. These recombination events were further confirmed by Simplot 3.5.1 analysis. Phylogenetic analysis based on full genomes showed that Guangxi ChPV/TuPV strains did not cluster according to their geographic origin, and the identified Guangxi ChPV/TuPV strains differed from the reference strains. Overall, whole-genome characterizations of emerging Guangxi ChPV and TuPV field strains will provide more detailed insights into ChPV/TuPV mutations and recombination and their relationships with molecular epidemiological features. [ABSTRACT FROM AUTHOR]

Published

2023

17. A polymerase chain reaction assay for detection of virulent and attenuated strains of duck plague virus.

Author

Xie, Liji, Xie, Zhixun, Huang, Li, Wang, Sheng, Huang, Jiaoling, Zhang, Yanfang, Zeng, Tingting, and Luo, Sisi

Subjects

*DUCK plague virus, *POLYMERASE chain reaction, *VIRAL vaccines, *VIRUS isolation, *PARAMYXOVIRUSES

Abstract

Sequence analysis of duck plague virus (DPV) revealed that there was a 528 bp (B fragment) deletion within the UL2 gene of DPV attenuated vaccine strain in comparison with field virulent strains. The finding of gene deletion provides a potential differentiation test between DPV virulent strain and attenuated strain based on their UL2 gene sizes. Thus we developed a polymerase chain reaction (PCR) assay targeting to the DPV UL2 gene for simultaneous detection of DPV virulent strain and attenuated strain, 827 bp for virulent strain and 299 bp for attenuated strain. This newly developed PCR for DPV was highly sensitive and specific. It detected as low as 100fg of DNA on both DPV virulent and attenuated strains, no same size bands were amplified from other duck viruses including duck paramyxovirus, duck tembusu virus, duck circovirus, Muscovy duck parvovirus, duck hepatitis virus type I, avian influenza virus and gosling plague virus. Therefore, this PCR assay can be used for the rapid, sensitive and specific detection of DPV virulent and attenuated strains affecting ducks. [ABSTRACT FROM AUTHOR]

Published

2017

18. Ultrasensitive Electrochemical Immunoassay for Avian Influenza Subtype H5 Using Nanocomposite.

Author

Xie, Zhixun, Huang, Jiaoling, Luo, Sisi, Xie, Zhiqin, Xie, Liji, Liu, Jiabo, Pang, Yaoshan, Deng, Xianwen, and Fan, Qing

Subjects

*ELECTROCHEMISTRY, *IMMUNOASSAY, *AVIAN influenza epidemiology, *NANOCOMPOSITE materials, *GRAPHENE oxide, *VETERINARY medicine

Abstract

We report a novel electrochemical immunosensor that can sensitively detect avian influenza virus H5 subtype (AIV H5) captured by graphene oxide-H5-polychonal antibodies-bovine serum albumin (GO-PAb-BSA) nanocomposite. The graphene oxide (GO) carried H5-polychonal antibody (PAb) were used as signal amplification materials. Upon signal amplification, the immunosensor showed a 256-fold increase in detection sensitivity compared to the immunosensor without GO-PAb-BSA. We designed a PAb labeling GO strategy and signal amplification procedure that allow ultrasensitive and selective detection of AIV H5. The established method responded to 2−15 HA unit/50 µL H5, with a linear calibration range from 2−15 to 2−8 HA unit/50 µL. In summary, we demonstrated that the immunosenser has a high specificity and sensitivity for AIV H5, and the established assay could be potentially applied in the rapid detection of other pathogenic microorganisms. [ABSTRACT FROM AUTHOR]

Published

2014

19. Detection of antibodies specific to the non-structural proteins of fowl adenoviruses in infected chickens but not in vaccinated chickens.

Author

Xie, Zhixun, Luo, Sisi, Fan, Qing, Xie, Liji, Liu, Jiabo, Xie, Zhiqin, Pang, Yaoshan, Deng, Xianwen, and Wang, Xiuqing

Subjects

*IMMUNOGLOBULINS, *ADENOVIRUSES, *CHICKEN diseases, *ENZYME-linked immunosorbent assay, *DIFFERENTIAL diagnosis, *VACCINATION

Abstract

Antibodies specific to the non-structural proteins of viruses are detected in virus-infected animals and show promise as a reliable diagnostic marker for virus infections. We examined the potential use of two non-structural proteins of fowl adenovirus (FAdV)-based, 100K and 33K, enzyme-linked immunosorbent assays (ELISAs) in the diagnosis of FAdVs. We cloned and expressed the 100K and 33K non-structural protein genes of the FAdVs in the pGEX-4T-1 plasmid vector. Purified 100K and 33K proteins alone or in combination were used as antigens in ELISAs. Antibodies specific to the 100K and 33K non-structural proteins were detected in chickens experimentally infected with FAdVs, but not in chickens vaccinated with inactivated FAdVs. In contrast, the agar gel precipitation (AGP) test detected FAdV-specific antibodies in 70.3% of the vaccinated chickens, suggesting that the non-structural protein-based ELISA could be used in the differential diagnosis of infected and vaccinated chickens. To further validate the 100K and 33K-based ELISA (100K-33K-ELISA) method, we compared its sensitivity and specificity with that of a whole virus-based ELISA and an AGP test in detecting FAdV-specific antibodies in 350 field samples. The results showed that the 100K-33K-ELISA exhibited a higher sensitivity than the AGP test and a comparable sensitivity and specificity to the whole virus ELISA. Overall, the 100K-33K-ELISA method is sensitive, specific and can be used to distinguish an acute FAdV infection from an inactivated virus-based vaccination response. [ABSTRACT FROM PUBLISHER]

Published

2013

20. A duplex quantitative real-time PCR assay for the detection of Haplosporidium and Perkinsus species in shellfish.

Author

Xie, Zhixun, Xie, Liji, Fan, Qing, Pang, Yaoshan, Deng, Xianwen, Xie, Zhi, Liu, Jiabo, and Khan, Mazhar

Subjects

*POLYMERASE chain reaction, *SHELLFISH, *PERKINSUS, *OLIGONUCLEOTIDES, *TOXOPLASMA gondii, *ESCHERICHIA coli

Abstract

A duplex quantitative real-time polymerase chain reaction (dq-PCR) assay was optimized to simultaneously detect Haplosporidium spp. and Perkinsus spp. of shellfish in one reaction. Two sets of specific oligonucleotide primers for Haplosporidium spp. and Perkinsus spp., along with two hydrolysis probes specific for each parasite group, were used in the assay. The dq-PCR results were detected and analyzed using the Light Cycler 2.0 software system. The dq-PCR identified and differentiated the two protozoan parasite groups. The sensitivity of the dq-PCR assay was 200 template copies for both Haplosporidium spp. and Perkinsus spp. No DNA product was amplified when known DNA from Marteilia refringens, Toxoplasma gondii, Bonamia ostreae, Escherichia coli, Cymndinium spp., Mykrocytos mackini, Vibrio parahaemolyticus, and shellfish tissue were used as templates. A total of 840 oyster samples from commercial cultivated shellfish farms from two coastal areas in China were randomly collected and tested by dq-PCR. The detection rate of Haplosporidium spp. was 8.6 % in the Qindao, Shandong coastal area, whereas Perkinsus spp. was 8.3 % coastal oysters cultivated from shellfish farms of Beihai, Guangxi. The dqPCR results suggested that Haplosporidium spp. was prevalent in oysters from Qindao, Shandong, while Perkinsus spp. was prevalent in oysters from the coastal areas of Beihai, Guangxi. This dq-PCR could be used as a diagnostic tool to detect Haplosporidium spp. and Perkinsus spp. in cultivated shellfish. [ABSTRACT FROM AUTHOR]

Published

2013

21. A reverse transcription loop-mediated isothermal amplification method for rapid detection of bovine viral diarrhea virus

Author

Fan, Qing, Xie, Zhixun, Xie, Liji, Liu, Jiabo, Pang, Yaoshan, Deng, Xianwen, Xie, Zhiqin, Peng, Yi, and Wang, Xiuqing

Subjects

*BOVINE viral diarrhea virus, *GENE amplification, *DETECTION of microorganisms, *RNA, *CROSS reactions (Immunology), *MICROBIOLOGICAL assay

Abstract

Abstract: A reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed and optimized to detect bovine viral diarrhea viral (BVDV) RNA. The RT-LAMP assay is highly sensitive and able to detect 4.67×100 copies of BVDV RNA. Additionally, the RT-LAMP method is capable of detecting both genotypes of BVDV. No cross-reaction with other bovine viruses was observed. The ability of RT-LAMP to detect BVDV RNA from bovine fecal swabs was also evaluated. Of the 88 fecal swabs, 38 were found to be positive by RT-LAMP assay, whereas 39 were positive by real-time RT-PCR. Taken together, the BVDV specific RT-LAMP method is highly specific and sensitive and can be used as a rapid and direct diagnostic assay for testing clinical samples. [Copyright &y& Elsevier]

Published

2012

22. Phylogeny and Pathogenicity of Subtype XIIb NDVs from Francolins in Southwestern China and Effective Protection by an Inactivated Vaccine.

Author

Zeng, Tingting, Xie, Liji, Xie, Zhixun, Huang, Jiaoling, Xie, Zhiqin, Huang, Qinghong, Luo, Sisi, Wang, Sheng, Li, Meng, Hua, Jun, Zhang, Yanfang, and Zhang, Minxiu

Subjects

*AMINO acid sequence, *NEWCASTLE disease virus, *PHYLOGENY, *VACCINES, *POULTRY products

Abstract

Most genotype XII newcastle disease viruses (NDVs) were isolated from poultry, chickens, or geese, with the exception of one subtype, XIIa NDV, which was isolated from a peacock. Here, two subtype XIIb NDVs, francolin/China/GX01/2017 and francolin/China/GX02/2017 (GX01 and GX02 hereafter), were isolated from francolins, which are resident birds in southern China. GX01 and GX02 were characterized as velogenic NDVs. Based on the weaker pathogenicity of these viruses in chickens, the amino acid sequences of seven proteins from genotype XII NDVs were compared, which revealed 17, 40, 15, 7, 32, 25, and 31 variations in the NP, P, M, F, HN, L, and V proteins, respectively, some of which could be responsible for this decreased pathogenicity. Epidemiological and phylogenetic analyses suggest that subtype XIIb NDVs have multiple transmission chains, and that resident birds may be involved in this process as intermediate hosts in which viruses keep evolving. Because of the increased pathogenicity of subtype XIIb NDVs, the protective efficacy of GX01 as an inactivated vaccine was evaluated and compared with that of two commercial inactivated vaccines in chickens. The results showed that the subtype XIIb NDVs could be candidate genotype-matched vaccine strains against genotype XII NDVs. [ABSTRACT FROM AUTHOR]

Published

2023

23. Development of a reverse transcription loop-mediated isothermal amplification assay for visual detection of avian reovirus.

Author

Xie, Zhixun, Peng, Yi, Luo, Sisi, Wang, Ying, Liu, Jiabo, Pang, Yaoshan, Deng, Xianwen, Xie, Zhiqin, Xie, Liji, Fan, Qing, Teng, Liqiong, and Wang, Xiuqing

Subjects

*REVERSE transcriptase polymerase chain reaction, *INFLUENZA A virus, *GENE amplification, *REOVIRUSES, *CROSS reactions (Immunology), *PATHOGENIC microorganisms, *VIRUSES

Abstract

Avian reovirus (ARV) is an important pathogen of poultry and causes significant economic losses to the poultry industry. To develop a rapid and sensitive method for the surveillance of ARV, a reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was established using a set of six primers specific to the S1 gene segment of ARV. The established assay was performed at 62oC for 60 min in a thermal block, and the result was visualized directly under daylight or ultraviolet light. The detection limit of the RT-LAMP assay was 10 fg total RNA, which was 100-fold higher than that of reverse transcriptase polymerase chain reactions. The specificity of the assay was supported by the lack of cross-reaction with other avian pathogens. Furthermore, viral RNAs of field isolates were successfully detected by the assay. Overall, the newly established RT-LAMP assay is simple, rapid, sensitive, specific, and can visually detect ARV without the use of any specialized equipment. [ABSTRACT FROM PUBLISHER]

Published

2012

24. Recombinant protein-based ELISA for detection and differentiation of antibodies against avian reovirus in vaccinated and non-vaccinated chickens

Author

Xie, Zhixun, Qin, Chunxiang, Xie, Liji, Liu, Jiabo, Pang, Yaoshan, Deng, Xianwen, Xie, Zhiqin, and Khan, Mazhar I.

Subjects

*RECOMBINANT proteins, *ENZYME-linked immunosorbent assay, *REOVIRUSES, *VIRAL antibodies, *GENE expression, *PLASMID genetics, *CHICKEN diseases, *VACCINATION

Abstract

Abstract: Two nonstructural genes, σNS and P17, of avian reovirus (ARV) were cloned into the expression plasmid vector PGEX4T-1. Expressed proteins for σNS and P17 of avian reovirus were purified and used as antigens. Three indirect σNS enzyme-linked immunosorbent assays (ELISAs), σNS-ELISA, P17-ELISA and σNS-P17-ELISA were optimized and used as specific tests. Serum samples from reovirus-infected and vaccinated SPF chickens were tested with the three ELISAs and an agar gel precipitin (AGP) method. ELISAs specific for σNS, P17 and σNS-P17 were able to detect specific antibodies for avian reovirus in 88.9%, 61.1%, and 88.9% in infected samples, respectively, whereas the AGP detected 55.6% of the infected samples. The detection rates of ELISA specific antibodies for σNS, P17 and σNS-P17 on sera of vaccinated chickens were 6.7%, 0% and 6.7%. However, in comparison the AGP method detected 60.6% of antibodies in serum samples from vaccinated chickens. The results showed that the use of ELISAs specific for the nonstructural proteins might be able to distinguish between reovirus vaccinated and infected chickens. Further studies are in progress to validate these recombinant protein-based ELISAs under field conditions. [Copyright &y& Elsevier]

Published

2010

25. Complete sequence determination and analysis of the Guangxi Phasianus colchicus (Galliformes: Phasianidae) mitochondrial genome.

Author

Zhang, Yanfang, Xie, Zhixun, Xie, Zhiqin, Deng, Xianwen, Xie, Liji, Fan, Qing, Luo, Sisi, Liu, Jiabo, Huang, Li, Huang, Jiaoling, Zeng, Tingting, and Wang, Sheng

Subjects

*PHASIANIDAE, *MITOCHONDRIAL DNA, *BIRDS, *BIRD phylogeny, *NUCLEOTIDE sequencing, *TRANSFER RNA

Abstract

The complete mitochondrial genome sequence of the GuangxiPhasianus colchicuswas measured by PCR-based methods and analyzed in detail. Our research findings reveal that the entire mitochondrial genome ofP. colchicusis a circular molecule of length 16,687 bp (GenBank accession number: KT364526). The contents of A, T, C, and G in the mitochondrial genome were found to be 30.64%, 25.29%, 30.81% and 13.26%, respectively. The complete mitochondrial genome of theP. colchicusis a typical structure, including 13 protein-coding genes, 2 rRNA genes, 22 tRNA genes, and 1 control region (D-loop region). This complete mitochondrial genome sequence provides essential information in understanding phylogenetic relationships among Galliformes mitochondrial genomes. [ABSTRACT FROM AUTHOR]

Published

2016

26. Molecular characterization of the Cenxi classical three-buff chicken ( Gallus gallus domesticus ) based on mitochondrial DNA.

Author

Xie, Zhixun, Zhang, Yanfang, Deng, Xianwen, Xie, Zhiqin, Liu, Jiabo, Huang, Li, Huang, Jiaoling, Zeng, Tingting, and Wang, Sheng

Subjects

*ANIMAL genetics, *CHICKENS, *MITOCHONDRIAL DNA, *MOLECULAR genetics, *BIRD phylogeny, *BIRDS, *GENOMES

Abstract

The complete mitochondrial genome sequence of the Cenxi classical three-buff chicken was measured by PCR-based methods and analyzed in detail. Our research findings reveal that the entire mitochondrial genome of the Cenxi classical three-buff chicken is a circular molecule consisting of 16,786 bp (GenBank accession number: KM433666). The contents of A, T, C, and G in the mitochondrial genome were found to be 30.27%, 23.75%, 32.49% and 13.49%, respectively. The complete mitochondrial genome of the Cenxi classical three-buff chicken contains a typical structure, including 13 protein-coding genes, 2 rRNA genes, 22 tRNA genes and 1 control region (D-loop region). This complete mitochondrial genome sequence provides essential information in understanding phylogenetic relationships amongGallus gallus domesticusmitochondrial genomes. [ABSTRACT FROM AUTHOR]

Published

2016

27. Mitochondrial genome of the Luchuan pig ( Sus scrofa ).

Author

Zhang, Yanfang, Xie, Zhixun, Deng, Xianwen, Xie, Zhiqin, Liu, Jiabo, Xie, Liji, Luo, Sisi, Huang, Li, Huang, Jiaoling, Zeng, Tingting, and Wang, Sheng

Subjects

*WILD boar, *SWINE genetics, *MITOCHONDRIAL DNA, *POLYMERASE chain reaction, *MAMMAL genomes, *MAMMALS

Abstract

The complete mitochondrial genome sequence of the Luchuan pig was measured by PCR-based methods, primer-walking sequencing, and fragment cloning. The entire mitochondrial genome of the Luchuan pig was identified as a circular molecule consisting of 16,730 bp (GenBank accession number: KP126954). The contents of A, T, C, and G in the mitochondrial genome were found to be 34.65%, 25.80%, 26.19%, and 13.36%, respectively. The complete mitochondrial genome of the Luchuan pig contains a typical structure, including 13 protein-coding genes, two rRNA genes, 22 tRNA genes, and one control region (D-loop region). This complete mitochondrial genome sequence provides essential information in understanding phylogenetic relationships amongSus scrofadomestic mitochondrial genomes. [ABSTRACT FROM AUTHOR]

Published

2016

28. A multiplex RT-PCR for detection of type A influenza virus and differentiation of avian H5, H7, and H9 hemagglutinin subtypes

Author

Xie, Zhixun, Pang, Yao-shan, Liu, Jiabo, Deng, Xianwen, Tang, Xiaofei, Sun, Jianhua, and Khan, Mazhar I.

Subjects

*POLYMERASE chain reaction, *INFLUENZA viruses, *AVIAN influenza, *HEMAGGLUTININ

Abstract

Abstract: A multiplex reverse transcriptase-polymerase chain reaction (mRT-PCR) was developed and optimized for the detection of type A influenza virus; the assay simultaneously differentiates avian H5, H7 and H9 hemagglutinin subtypes. Four sets of specific oligonucleotide primers were used in this test for type A influenza virus, H5, H7 and H9 heamagglutinin subtypes. The mRT-PCR DNA products were visualized by gel electrophoresis and consisted of fragments of 860bp for H5, 634bp for H7, 488bp for H9 hemagglutinin subtypes, and 244bp for type A influenza virus. The common set primers for type A influenza virus were able to amplify a 244bp DNA band for any of the other subtypes of AIV. The mRT-PCR assay developed in this study was found to be sensitive and specific. Detection limit for PCR-amplified DNA products was 100pg for the subtypes H5, H7, and H9 and 10pg for type A influenza virus in all subtypes. No specific amplification bands of the same sizes (860, 634 and 488bp) could be amplified for RNA of other influenza hemagglutinin subtypes, nor specific amplification bands of type A influenza (244bp) for other viral or bacterial pathogens. [Copyright &y& Elsevier]

Published

2006

29. Electrochemical immunosensor with Cu(I)/Cu(II)-chitosan-graphene nanocomposite-based signal amplification for the detection of newcastle disease virus.

Author

Huang, Jiaoling, Xie, Zhixun, Huang, Yihong, Xie, Liji, Luo, Sisi, Fan, Qing, Zeng, Tingting, Zhang, Yanfang, Wang, Sheng, Zhang, Minxiu, Xie, Zhiqin, and Deng, Xianwen

Subjects

*CHITOSAN, *GRAPHENE, *NANOCOMPOSITE materials, *NEWCASTLE disease, *IMMUNE response

Abstract

An electrochemical immunoassay for the ultrasensitive detection of Newcastle disease virus (NDV) was developed using graphene and chitosan-conjugated Cu(I)/Cu(II) (Cu(I)/Cu(II)-Chi-Gra) for signal amplification. Graphene (Gra) was used for both the conjugation of an anti-Newcastle disease virus monoclonal antibody (MAb/NDV) and the immobilization of anti-Newcastle disease virus polyclonal antibodies (PAb/NDV). Cu(I)/Cu(II) was selected as an electroactive probe, immobilized on a chitosan-graphene (Chi-Gra) hybrid material, and detected by differential pulse voltammetry (DPV) after a sandwich-type immune response. Because Gra had a large surface area, many antibodies were loaded onto the electrochemical immunosensor to effectively increase the electrical signal. Additionally, the introduction of Gra significantly increased the loading amount of electroactive probes (Cu(I)/Cu(II)), and the electrical signal was further amplified. Cu(I)/Cu(II) and Cu(I)/Cu(II)-Chi-Gra were compared in detail to characterize the signal amplification ability of this platform. The results showed that this immunosensor exhibited excellent analytical performance in the detection of NDV in the concentration range of 100.13 to 105.13 EID50/0.1 mL, and it had a detection limit of 100.68 EID50/0.1 mL, which was calculated based on a signal-to-noise (S/N) ratio of 3. The resulting immunosensor also exhibited high sensitivity, good reproducibility and acceptable stability. [ABSTRACT FROM AUTHOR]

Published

2020

30. Avian Orthoreoviruses: A Systematic Review of Their Distribution, Dissemination Patterns, and Genotypic Clustering.

Author

Rafique, Saba, Rashid, Farooq, Wei, You, Zeng, Tingting, Xie, Liji, and Xie, Zhixun

Subjects

*VIRAL tropism, *PROTEOLYTIC enzymes, *MALABSORPTION syndromes, *SYMPTOMS, *VACCINE effectiveness, *POULTRY farms

Abstract

Avian orthoreviruses have become a global challenge to the poultry industry, causing significant economic impacts on commercial poultry. Avian reoviruses (ARVs) are resistant to heat, proteolytic enzymes, a wide range of pH values, and disinfectants, so keeping chicken farms free of ARV infections is difficult. This review focuses on the global prevalence of ARVs and associated clinical signs and symptoms. The most common signs and symptoms include tenosynovitis/arthritis, malabsorption syndrome, runting–stunting syndrome, and respiratory diseases. Moreover, this review also focused on the characterization of ARVs in genotypic clusters (I–VI) and their relation to tissue tropism or viral distribution. The prevailing strains of ARV in Africa belong to all genotypic clusters (GCs) except for GC VI, whereas all GCs are present in Asia and the Americas. In addition, all ARV strains are associated with or belong to GC I-VI in Europe. Moreover, in Oceania, only GC V and VI are prevalent. This review also showed that, regardless of the genotypic cluster, tenosynovitis/arthritis was the predominant clinical manifestation, indicating its universal occurrence across all clusters. Globally, most avian reovirus infections can be prevented by vaccination against four major strains: S1133, 1733, 2408, and 2177. Nevertheless, these vaccines may not a provide sufficient defense against field isolates. Due to the increase in the number of ARV variants, classical vaccine approaches are being developed depending on the degree of antigenic similarity between the vaccine and field strains, which determines how successful the vaccination will be. Moreover, there is a need to look more closely at the antigenic and pathogenic properties of reported ARV strains. The information acquired will aid in the selection of more effective vaccine strains in combination with biosecurity and farm management methods to prevent ARV infections. [ABSTRACT FROM AUTHOR]

Published

2024

31. Analysis of the Rongshui Xiang duck (Anseriformes, Anatidae, Anas) mitochondrial DNA.

Author

Zhang, Yanfang, Xie, Zhixun, Xie, Liji, Deng, Xianwen, Xie, Zhiqin, Huang, Li, Huang, Jiaoling, and Zeng, Tingting

Subjects

*MITOCHONDRIAL DNA, *ANSERIFORMES, *ANATIDAE, *BIRDS, *GENETICS, *RIBOSOMAL RNA, *TRANSFER RNA

Abstract

The complete mitochondrial genome sequence of the Rongshui Xiang duck was measured by PCR-based methods. Our research findings reveal that the entire mitochondrial genome of the Rongshui Xiang duck is a circular molecule consisting of 16,605 bp (GenBank accession number: KJ833587). The contents of A, T, C, and G in the mitochondrial genome were found to be 29.20%, 22.20%, 32.82% and 15.79%, respectively, similar to the majority of avian species. The complete mitochondrial genome of the Rongshui Xiang duck contains 13 protein-coding genes, 2 rRNA genes, 22 tRNA genes, and 1 control region. The characteristics of the mitochondrial genome were analyzed in detail. Our complete mitochondrial genome sequence should provide essential information for understanding phylogenetic relationships among duck mitochondrial genomes. [ABSTRACT FROM PUBLISHER]

Published

2016

32. Sequence and gene organization of the Xilin small partridge duck ( Anseriformes, Anatidae, Anas ) mitochondrial DNA.

Author

Xie, Zhixun, Zhang, Yanfang, Xie, Liji, Deng, Xianwen, Xie, Zhiqin, Huang, Li, Huang, Jiaoling, and Zeng, Tingting

Subjects

*NUCLEOTIDE sequencing, *GENETICS, *BIRDS, *MITOCHONDRIAL DNA, *DUCKS, *ANSERIFORMES, *ANATIDAE, *BIRD phylogeny

Abstract

The complete mitochondrial genome sequence of the Xilin small partridge duck was measured by PCR-based methods. Our research findings revealed that the entire mitochondrial genome of the Xilin small partridge duck was 16,604 bp (GenBank accession number: KJ833586). The contents of A, T, C, and G in the mitochondrial genome were 29.20%, 22.19%, 32.82% and 15.79%, respectively, which were similar to the majority of most avian species. The complete mitochondrial genome of the Xilin small partridge duck contains 13 protein-coding genes, 2 rRNA genes, 22 tRNA genes, and 1 control region. Components of the Xilin small partridge duck’s mitochondrial genome were similar to those of otherAnatidaein gene arrangement and composition. The complete mitochondrial genome of the Xilin small partridge duck should provide essential information for understanding phylogenetic relationships of duck mitochondrial genome. [ABSTRACT FROM PUBLISHER]

Published

2016

33. Genetic characterization of the Longsheng duck ( Anas platyrhynchos ) based on the mitochondrial DNA.

Author

Zhang, Yanfang, Xie, Zhixun, Xie, Liji, Tan, Wei, Liu, Jiabo, Deng, Xianwen, Xie, Zhiqin, and Luo, Sisi

Subjects

*MALLARD, *MITOCHONDRIAL RNA, *MITOCHONDRIAL DNA, *BASE pairs, *DEOXYRIBOSE

Abstract

The complete mitochondrial genome sequence of the Longsheng duck was measured by PCR-based methods. Our research findings revealed that the entire mitochondrial genome of the Longsheng duck was 16,603 bp (GenBank accession number: KJ739616). The contents of A, T, C, and G in the mitochondrial genome were 29.22%, 22.21%, 32.79% and 15.77%, respectively, which were similar to the majority of most avian species. The complete mitochondrial genome of the Longsheng duck contains 13 protein-coding genes, 2 rRNA genes, 22 tRNA genes, and one control region. Components of the Longsheng duck’s mitochondrial genome were similar to those of otherAnas platyrhynchosin gene arrangement and composition. The complete mitochondrial genome of the Longsheng duck should provide essential information for understanding phylogenetic relationships of duck mitochondrial genome. [ABSTRACT FROM AUTHOR]

Published

2016

34. The complete mitochondrial genome of the Jingxi duck ( Anas platyrhynchos ).

Author

Xie, Zhixun, Zhang, Yanfang, Xie, Liji, Liu, Jiabo, Deng, Xianwen, Xie, Zhiqin, Fan, Qing, and Luo, Sisi

Subjects

*MALLARD, *GENOMES, *ANATIDAE, *PHYLOGENY, *GERMPLASM

Abstract

The entire mitochondrial genome of Jingxi duck from China was 16,603 bp in length, and has been analyzed for gene locations, length, start codons and stop codons. With the base composition of 29.20% for A, 22.19% for T, 32.82% for C, 15.79% for G, so the percentage of A and T (51.39%) was slightly higher than those of G and C. The Jingxi duck mitochondrial genome contained two ribosomal RNA genes, 13 protein-coding genes, 22 transfer RNA genes and one non-coding control region (D-loop region). The arrangement of these genes was the same as most birds. The complete mitochondrial genome sequence of the Jingxi duck will be useful for phylogenetics, and provide an important data set for further study on the germplasm resources. [ABSTRACT FROM AUTHOR]

Published

2016

35. Novel structures and mechanical properties of Zr2N: Ab initio description under high pressures.

Author

Wen, Minru, Xie, Xing, Xie, Zhixun, Dong, Huafeng, Zhang, Xin, Wu, Fugen, and Wang, Chong-Yu

Subjects

*THERMAL barrier coatings, *VICKERS hardness, *YOUNG'S modulus, *BRITTLE materials, *DENSITY functional theory, *ELASTIC modulus, *NITRIDES, *ELASTIC constants

Abstract

With the formation of structural vacancies, zirconium nitrides (key materials for cutting coatings, super wear-resistance, and thermal barrier coatings) display a variety of compositions and phases featuring both cation and nitrogen enrichment. This study presents a systematic exploration of the stable crystal structures of zirconium heminitride combining the evolutionary algorithm method and ab initio density functional theory calculations at pressures of 0 GPa, 30 GPa, 60 GPa, 90 GPa, 120 GPa, 150 GPa, and 200 GPa. In addition to the previously proposed phases P42/mnm-, Pnnm-, and Cmcm-Zr2N, five new high-pressure Zr2N phases of P4/nmm, I4/mcm, P21/m, , and C2/m are discovered. An enthalpy study of these candidate configurations reveals various structural phase transformations of Zr2N under pressure. By calculating the elastic constants and phonon dispersion, the mechanical and dynamical stabilities of all predicted structures are examined at ambient and high pressures. To understand the structure–property relationships, the mechanical properties of all Zr2N compounds are investigated, including the elastic moduli, Vickers hardness, and directional dependence of Young's modulus. The Cmcm-Zr2N phase is found to belong to the brittle materials and has the highest Vickers hardness (12.9 GPa) among all candidate phases, while the I4/mcm-Zr2N phase is the most ductile and has the lowest Vickers hardness (2.1 GPa). Furthermore, the electronic mechanism underlying the diverse mechanical behaviors of Zr2N structures is discussed by analyzing the partial density of states. [ABSTRACT FROM AUTHOR]

Published

2021

36. Production and identification of monoclonal antibodies and development of a sandwich ELISA for detection of the H3-subtype avian influenza virus antigen.

Author

Luo, Sisi, Deng, Xianwen, Xie, Zhixun, Huang, Jiaoling, Zhang, Minxiu, Li, Meng, Xie, Liji, Li, Dan, Fan, Qing, Wang, Sheng, Zeng, Tingting, Zhang, Yanfang, and Xie, Zhiqin

Subjects

*ENZYME-linked immunosorbent assay, *AVIAN influenza A virus, *MONOCLONAL antibodies, *WESTERN immunoblotting, *CELL fusion, *ANTIGENS, *INFLUENZA A virus

Abstract

The H3 subtype of avian influenza virus (AIV) is widespread in avian species and is frequently isolated in surveillance projects; thus, we have developed a more effective diagnostic approach of a monoclonal antibody (mAb)-based sandwich ELISA for the H3 AIV detection. First, we have produced the essential reagent of mAb against AIV H3 strains with the development of an mAb-Mouse immunization with a purified H3-subtype AIV strain and cell fusion to generate hybridoma cells. These cells were screened with hemagglutination inhibition (HI) tests, and optimal cells were subcloned. We chose a hybridoma cell line that steadily secreted a specific H3-subtype AIV mAb, designated 9F12, that belongs to the IgG1 subclass and has a K-type light chain. 9F12 was shown to bind specifically to the H3-subtype AIV antigen by both immunofluorescence assay and Western blot analysis. Finally, a 9F12-based sandwich ELISA was successfully developed and used to specifically test for this antigen. The sandwich ELISA conditions were optimized, and the specificity and sensitivity were validated. The results for clinical sample detection were consistent with viral isolation. Consequently, the 9F12-based sandwich ELISA is a specific, sensitive, robust, rapid and versatile diagnostic tool for H3-subtype AIV and provides a promising strategy for effective influenza virus prevention and control. [ABSTRACT FROM AUTHOR]

Published

2020

37. Correction: Development of a GeXP-multiplex PCR assay for the simultaneous detection and differentiation of six cattle viruses.

Author

Fan, Qing, Xie, Zhixun, Xie, Zhiqin, Deng, Xianwen, Xie, Liji, Huang, Li, Luo, Sisi, Huang, Jiaoling, Zhang, Yanfang, Zeng, Tingting, Wang, Sheng, Liu, Jiabo, and Pang, Yaoshan

Subjects

*CELL differentiation, *POLYMERASE chain reaction, *BIOLOGICAL assay

Published

2017

38. An attempt to develop a detection method specific for virulent duck plague virus strains based on the UL2 gene B fragment.

Author

Xie, Liji, Huang, Li, Xie, Zhixun, Wang, Sheng, Huang, Jiaoling, Zhang, Yanfang, and Zhong, Chuande

Subjects

*PLAGUE, *DUCKS, *MICROBIAL virulence, *POLYMERASE chain reaction, *FLUORESCENCE, *DISEASES

Abstract

A comparison of the unique long region 2 (UL2) gene sequences between 10 virulent and 11 attenuated duck plague virus (DPV) strains (including all DPV UL2 gene sequences registered in GenBank) showed that the UL2 genes in the attenuated DPV strains had a 528 bp deletion in the B fragment. Primers were designed based on the B fragment sequence of the UL2 gene in an attempt to establish a fluorescence quantitative polymerase chain reaction (PCR) and a conventional PCR detection method that could specifically detect virulent DPV strains (i.e. positive detection for virulent DPV strains and negative detection for attenuated DPV strains). Additionally, PCR products were cloned for sequence analysis. These two methods detected five attenuated DPV strains in addition to the virulent DPV strains. Sequence analysis of the PCR products showed that the amplified products were the B fragments of the UL2 gene. These results indicated that detection methods specific for virulent DPV strains could not be established using primers designed based on the UL2 gene B fragment. [ABSTRACT FROM AUTHOR]

Published

2017

39. Gallus NME/NM23 nucleoside diphosphate kinase 2 interacts with viral σA and affects the replication of avian reovirus.

Author

Xie, Liji, Wang, Sheng, Xie, Zhixun, Wang, Xiaohu, Wan, Lijun, Deng, Xianwen, Xie, Zhiqin, Luo, Sisi, Zeng, Tingting, Zhang, Minxiu, Fan, Qing, Huang, Jiaoling, Zhang, Yanfang, and Li, Meng

Subjects

*SMALL interfering RNA, *CYTOSKELETAL proteins, *CHICKEN embryos, *CHICKENS

Abstract

• Four host proteins interacting with ARV σA protein were screened by a yeast two-hybrid system. • NME2 was further validated as a σA-binding protein through co-immunoprecipitation. • The key interaction domain was identified at aa 121–416 in NME2 and at aa 71–139 in σA, respectively. • Overexpression of NME2 substantially inhibited ARV replication. Our present study aimed to identify host cell proteins that may interact with avian reovirus (ARV) σA protein and their potential effect on ARV replication. The ARV structural protein σA has been demonstrated to suppress interferon production and confirmed to activate the PI3K/Akt pathway. However, host cell factors interacting with σA to affect ARV replication remain unknown. In current study, a cDNA library of chicken embryo fibroblasts (CEFs) was constructed, and host cell proteins interacting with σA were screened by a yeast two-hybrid system. We identified four candidate cellular proteins that interact with ARV σA protein. Among them, Gallus NME/NM23 nucleoside diphosphate kinase 2 (NME2) was further validated as a σA-binding protein through co-immunoprecipitation. The key interaction domain was identified at amino acids (aa) 121–416 in NME2 and at aa 71–139 in σA, respectively. We demonstrated that overexpression of NME2 substantially inhibited ARV replication. In addition silencing NME2 by small interfering RNAs (siRNAs) resulted in marked enhancement of ARV replication. Our work has demonstrated that NME2 is a σA-binding protein that may affect ARV replication in CEF cells. [ABSTRACT FROM AUTHOR]

Published

2021

40. Role of phosphatidylinositol 3-kinase (PI3K) and Akt1 kinase in porcine reproductive and respiratory syndrome virus (PRRSV) replication.

Author

Wang, Xiuqing, Zhang, Hanmo, Abel, Alex, Young, Alan, Xie, Liji, and Xie, Zhixun

Subjects

*PHOSPHATIDYLINOSITOL 3-kinases, *PROTEIN kinase B, *PORCINE reproductive & respiratory syndrome, *VIRAL replication, *GENETIC transcription, *VIROLOGY, *VIRUSES

Abstract

We have previously reported that inhibition of phosphatidylinositol 3-kinase (PI3K) reduces porcine reproductive and respiratory syndrome (PRRSV) replication. Here, we further investigate the mechanism by which PI3K inhibition affects virus replication and the role of Akt1 kinase in virus replication. We found that PI3K inhibition reduced viral gene transcription by approximately 1.5-fold. Accordingly, viral protein synthesis was significantly reduced by PI3K inhibition. Interestingly, cells overexpressing the dominant negative mutant Akt1 exhibited a significant reduction in viral gene transcription compared to cells overexpressing the constitutively active Akt1. Viral protein synthesis was also enhanced in cells overexpressing the constitutively active Akt1. Overall, our data show that both PI3K and Akt1 play a role in viral gene expression, leading to an increase in virus replication. [ABSTRACT FROM AUTHOR]

Published

2014

41. Identification of a protein disulfide isomerase of Neospora caninum in excretory–secretory products and its IgA binding and enzymatic activities

Author

Liao, Min, Ma, Liqing, Bannai, Hiroshi, Lee, Eung-goo, Xie, Zhixun, Tang, Xiaofei, Zhang, Houshuang, Xuan, Xuenan, and Fujisaki, Kozo

Subjects

*MOLECULAR weights, *SURFACE chemistry, *DRUG therapy, *PHYSICAL & theoretical chemistry

Abstract

Abstract: A protein disulfide isomerase of Neospora caninum (NcPDI) with a molecular weight of 50kDa was identified in tachyzoite lysate and excretory–secretory (ES) products. The IgA antibody in 58.0% of the individual cattle tear samples recognized the NcPDI, which suggests that the PDI-specific antibody may be involved in defense against parasites. In addition, PDI-specific inhibitors and NcPDI antiserum showed inhibitory effects on the growth of N. caninum tachyzoites. Furthermore, the purified recombinant NcPDI demonstrated biological activities in vitro by catalysis and refolding of reduced RNase A and assisted in the recovery of native lysozyme. These findings indicate that NcPDI possesses PDI-specific enzymatic activity and could be a putative target for chemotherapy for neosporosis. [Copyright &y& Elsevier]

Published

2006