Your search keyword '"Luo, Ting Rong"' showing total 14 results

1. Activation of NF-[subκ]B in cells productively infected with HSV-1 depends on activated protein kinase R and plays no apparent role in blocking apoptosis.

Author

Taddeo, Brunella, Luo, Ting Rong, Weiran Zhang, and Roizman, Bernard

Subjects

*HERPES simplex virus, *PROTEIN kinases, *NF-kappa B, *APOPTOSIS, *DOUBLE-stranded RNA

Abstract

Microarray data reported elsewhere indicated that herpes simplex virus I induces the up-regulation of nuclear factor &key;B (NF-&key;B)regulated genes, including that of its inhibitor, I&key;Bα, consistent with the reports that wild-type virus induces the activation of NF-&key;B. In this report we show that activation of NF-&key;B in infected cells is linked to the activation of protein kinase R (PKR). Specifically: (i) PKR is activated in infected cells although the effects of the activated enzyme on protein synthesis are negated by the viral gene 1,134.5, which encodes a protein phosphatase la accessory factor that enables the dephosphorylation of the a subunit of eukaryotic translation initiation factor 2. NF-&key;B is activated in wild-type murine embryonic fibroblasts but not in related PKR-null cells. (ii) In cells infected with a replication-competent δγ134.5 mutant (R5104), but carrying a Us11 gene expressed early in infection, eukaryotic translation initiation factor 2α is not phosphorylated, and in in vitro assays, PKR bound to the Us11 protein is not phosphorylated on subsequent addition of double-stranded RNA. Here we report that this mutant does not activate PKR, has no effect on the accumulation of I&key;Bα, and does not cause the translocation of NF-&key;B in infected cells. (iii) One hypothesis advanced for the activation of NF-&key;B is that it blocks apoptosis induced by viral gene products. The replication-competent R5104 mutant does not induce the programmed cell's death. We conclude that in herpes simplex virus 1-infected cells, activation of NF-&key;B depends on activation of PKR and that NF-&key;B is not required to block apoptosis in productively infected cells. [ABSTRACT FROM AUTHOR]

Published

2003

2. Transcriptomic Analysis of mRNA Expression Profiles in the Microglia of Mouse Brains Infected with Rabies Viruses of Varying Virulence.

Author

Liu, Jundan, Li, Wangchang, Yu, Dongling, Jin, Rong, Hou, Hualin, Ling, Xiaoqing, Kiflu, Abraha Bahlbi, Wei, Xiankai, Yang, Xiaogan, Li, Xiaoning, He, Yongming, and Luo, Ting Rong

Subjects

*VIRUS virulence, *GENE expression, *RABIES virus, *JAK-STAT pathway, *DOG bites, *TRANSCRIPTOMES

Abstract

Rabies is a lethal encephalitis caused by the rabies virus (RABV) with a fatality rate near 100% after the onset of clinical symptoms in humans and animals. Microglia are resident immune cells in the central nervous system. Few studies have been conducted on the functional role of microglia in RABV infection. Here, we performed a transcriptomic analysis of mRNA expression profiles in the microglia of mouse brains intracerebrally infected with RABV. We successfully isolated single microglial cells from the mouse brains. The survival rate of dissociated microglial cells was 81.91%–96.7%, and the purity was 88.3%. Transcriptomic analysis revealed 22,079 differentially expressed mRNAs identified in the microglia of mouse brains infected with RABV strains (rRC-HL, GX074, and CVS-24) of varying virulence at 4 and 7 days post-infection (dpi) compared to the control group. The numbers of DEGs versus the control at 4 and 7 dpi in mice infected with rRC-HL, GX074, and CVS-24 were 3622 and 4590, 265 and 4901, and 4079 and 6337. The GO enrichment analysis showed that response to stress, response to external stimulus, regulation of response to stimulus, and immune system process were abundant during RABV infection. The KEGG analysis indicated that the Tlr, Tnf, RIG-I, NOD, NF-κB, MAPK, and Jak-STAT signaling pathways were involved in RABV infection at both 4 and 7 dpi. However, some phagocytosis and cell signal transduction processes, such as endocytosis, p53, phospholipase D, and oxidative phosphorylation signaling pathways, were only expressed at 7 dpi. The involvement of the Tnf and Tlr signaling pathways prompted us to construct a protein–protein interaction (PPI) network of these pathways. The PPI revealed 8 DEGs, including Mmp9, Jun, Pik3r1, and Mapk12. Notably, Il-1b interacted with Tnf and Il-6 with combined scores of 0.973 and 0.981, respectively. RABV causes significant changes in mRNA expression profiles in the microglia in mice. 22,079 differentially expressed mRNAs were identified in the microglia of mice infected with RABV strains of varying virulence at 4 and 7 dpi. The DEGs were evaluated using GO, KEGG, and PPI network analysis. Many immune pathways were up-regulated in RABV-infected groups. The findings will help elucidate the microglial molecular mechanisms of cellular metabolism dysregulated by RABV and may provide important information for investigating RABV pathogenesis and therapeutic methods. [ABSTRACT FROM AUTHOR]

Published

2023

3. Host Desmin Interacts with RABV Matrix Protein and Facilitates Virus Propagation.

Author

Zhang, Wen, Liu, Yuming, Li, Mengru, Zhu, Jian, Li, Xiaoning, Luo, Ting Rong, and Liang, Jingjing

Subjects

*CYTOPLASMIC filaments, *VIRAL proteins, *INTRACELLULAR tracking, *RABIES virus, *VIRUS diseases, *CYTOSKELETAL proteins

Abstract

Microfilaments and microtubules, two crucial structures of cytoskeletal networks, are usurped by various viruses for their entry, egress, and/or intracellular trafficking, including the Rabies virus (RABV). Intermediate filaments (IFs) are the third major component of cytoskeletal filaments; however, little is known about the role of IFs during the RABV infection. Here, we identified the IF protein desmin as a novel host interactor with the RABV matrix protein, and we show that this physical interaction has a functional impact on the virus lifecycle. We found that the overexpression of desmin facilitates the RABV infection by increasing the progeny virus yield, and the suppression of endogenous desmin inhibits virus replication. Furthermore, we used confocal microscopy to observe that the RABV-M co-localizes with desmin in IF bundles in the BHK-21 cells. Lastly, we found that mice challenged with RABV displayed an enhanced expression of desmin in the brains of infected animals. These findings reveal a desmin/RABV-M interaction that positively regulates the virus infection and suggests that the RABV may utilize cellular IFs as tracks for the intracellular transport of viral components and efficient budding. [ABSTRACT FROM AUTHOR]

Published

2023

4. Molecular epidemiology of rabies in Guangxi Province, south of China

Author

Liu, Qi, Xiong, Yi, Luo, Ting Rong, Wei, You-Chuan, Nan, Song-Jian, Liu, Fang, Pan, Yan, Feng, Li, Zhu, Wei, Liu, Ke, Guo, Jian-Gang, and Li, Hua-Ming

Subjects

*MEDICAL research, *RABIES, *VIRUS diseases, *EPIDEMIOLOGY

Abstract

Abstract: Background: Surveillance data for rabies in Guangxi Province in China showed that human rabies cases have gradually increased since 1996. Objective: To evaluate the epidemiology of rabies at the molecular level and provide suggestions for effective prevention of rabies in Guangxi. Study design: Since 2000, 1569 brains from suspected rabid animals were collected from different areas of Guangxi. Rabies virus was isolated from 42 samples. RT-PCR was used to amplify a 455 nucleotide segment of the 3′-terminal of the N gene. The sequencing data from that segment was used for phylogenetic analysis. Results: Nucleotide homology comparisons and phylogenetic tree analysis based on this sequence indicated that all the rabies virus isolates from Guangxi belonged to genotype 1 and could be divided into four groups. Groups I, II and IV included 23, 10 and 8 isolates, respectively. These had nucleotide homologies of 97.1–100%, 98.2–100% and 99.1–99.6%, respectively. Only the GXN119 strain belonged to group III. Group I had two group-specific mutations: T90N and E110D. Group II had one group-specific mutation of T42S. Conclusions: This study showed that rabies virus isolates from Guangxi have a close genetic relationship and topographical distribution. [Copyright &y& Elsevier]

Published

2007

5. Phosphorylation and dephosphorylation of threonine 188 in nucleoprotein is crucial for the replication of influenza A virus.

Author

Li, Yun, Sun, Lei, Zheng, Weinan, Madina·Mahesutihan, null, Li, Jing, Bi, Yuhai, Wang, Heran, Liu, Wenjun, and Luo, Ting Rong

Subjects

*INFLUENZA viruses, *PHOSPHORYLATION, *THREONINE, *NUCLEOPROTEINS, *VIRAL replication, *GENETIC transcription

Abstract

Nucleoprotein (NP) is a major component of the viral ribonucleoprotein (vRNP) complex that is responsible for viral replication, transcription and packaging of influenza A virus. Phosphorylation of NP plays an important role during viral infection. In the present study, we identified threonine 188 (T188) as a novel phosphorylated residue in the NP of influenza A virus by using mass spectrometry. T188 is located within nuclear export signal 2 (NES2) which is chromosome region maintenance 1 (CRM1)-independent. We observed that the phosphorylation and dephosphorylation of residue T188 regulated viral replication by controlling NES2-dependent NP nuclear export and the polymerase activity of the vRNP complex. Our findings provide further insights for understanding the replication of influenza A virus. [ABSTRACT FROM AUTHOR]

Published

2018

6. IRF1 up-regulates isg15 gene expression in dsRNA stimulation or CSFV infection by targeting nucleotides −487 to −325 in the 5′ flanking region.

Author

Li, Xiao-Quan, Li, Xiao Ning, Liang, Jing-Jing, Cai, Xin-Bin, Tao, Qian, Li, Yu-Xiao, Qin, Qing, Xu, Su-Ping, and Luo, Ting Rong

Subjects

*INTERFERON regulatory factors, *UBIQUITIN, *IMMUNE response, *GENE expression, *CLASSICAL swine fever

Abstract

Interferon (IFN)-stimulated gene 15 (ISG15) encodes a ubiquitin-like protein that is heavily involved in immune response elicitation. As an important member of interferon regulatory factor (IRF) family, IRF1 can activate the expression of multiple genes, including the human optineurin gene (Sudhakar et al., 2013). In this study, a sequence in the promoter region of the optineurin gene was compared to the 5′ flanking region of the porcine isg15 gene. Porcine IRF1 also possesses antiviral activity against several swine viruses (Li et al., 2015), but the mechanism is not well understood. Herein, we report that porcine IRF1 and ISG15 were up-regulated in porcine kidney (PK-15) cells following stimulation with double-stranded RNA (dsRNA) or classical swine fever virus (CSFV) infection. We also found that siRNA-mediated knockdown of IRF1 expression resulted in lower ISG15 expression in response to polyinosinic:polycytidylic acid [poly(I:C)] or CSFV infection. The overexpression of IRF1 resulted in ISG15 up-regulation. IRF1 was shown to translocate to the nucleus in response to dsRNA stimulation. To further identify the functional domain of the isg15 gene that promotes IRF1 transcriptional activity, firefly luciferase and ISG15 reporter systems were constructed. The results of the firefly luciferase and ISG15 reporter assay suggested that IRF1 mediates the up-regulation of ISG15. Nucleotides −487 to −325, located in the 5′ flanking region of the isg15 gene, constituted the promoter region of IRF1. ChIP assay indicated that IRF1 protein was able to interact with the DNA in the 5′fr of isg15 gene in cells. As an innate immune response protein with broad-spectrum antiviral activity, the up-regulation of ISG15 mediated by IRF1 in porcine cells is reported for the first time. These results warrant further investigation into the antiviral activity of porcine IRF1 against reported swine viruses. [ABSTRACT FROM AUTHOR]

Published

2018

7. A recombinant rabies virus expressing a phosphoprotein–eGFP fusion is rescued and applied to the rapid virus neutralization antibody assay.

Author

Tang, Hai-Bo, Lu, Zhuan-Ling, Wei, Xian-Kai, Zhong, Yi-Zhi, Zhong, Tao-Zhen, Pan, Yan, Luo, Yang, Liao, Su-Huan, Minamoto, Nobuyuki, and Luo, Ting Rong

Subjects

*RECOMBINANT viruses, *GENE expression in viruses, *RABIES transmission, *RABIES vaccines, *PREVENTIVE medicine, *GREEN fluorescent protein

Abstract

Rabies remains a worldwide concern, and dogs are a major vector for rabies virus (RABV) transmission. Vaccination is used in China to control the spread of rabies in dogs, a practice which necessitates effective, efficient, and high-throughput methods to confirm vaccination. The current rapid fluorescent focus inhibition test (RFFIT) method to measure virus-neutralizing antibody titers in the serum involves multiple steps, and more efficient methods are needed to match the increasing demand for this type of monitoring. In this study, based on the parental rRC-HL strain, a recombinant RABV rRV-eGFP expressing enhanced green fluorescent protein (eGFP) fused with RABV P protein was generated by a reverse genetic technique. The rRV-eGFP grew stably and successfully expressed P–eGFP fusion in Neuro-2A (NA) host cells. Furthermore, the P protein was shown to co-localize with eGFP in rRV-eGFP-infected NA cells. Since eGFP is easily detected in infected cells under a fluorescence microscope, rRV-eGFP could be used to establish a more rapid virus-neutralizing antibody titers assay based on RFFIT, designated as the RFFIT-eGFP method. From 69 canine serum samples, the RFFIT-eGFP method was shown to be as specific and as sensitive as the RFFIT method, suggesting that it might represent a faster tool than conventional RFFIT for measuring RABV virus-neutralizing antibody titers in canine sera without sacrificing accuracy. [ABSTRACT FROM AUTHOR]

Published

2015

8. Re-emergence of Rabies in the Guangxi Province of Southern China.

Author

Tang, Hai-Bo, Pan, Yan, Wei, Xian-Kai, Lu, Zhuan-Ling, Lu, Wu, Yang, Jian, He, Xiao-Xia, Xie, Lin-Juan, Zeng, Lan, Zheng, Lie-Feng, Xiong, Yi, Minamoto, Nobuyuki, and Luo, Ting Rong

Subjects

*RABIES, *RABIES virus, *RHINOVIRUSES, *Q fever, *G proteins, *MONOCLONAL antibodies, *DOG bites, *ZOONOSES, *AMINO acids

Abstract

Background: Human rabies cases in the Guangxi province of China decreased from 839 in 1982 to 24 in 1995, but subsequently underwent a sharp increase, and has since maintained a high level. Methodology/Principal Findings: 3,040 brain samples from normal dogs and cats were collected from 14 districts of Guangxi and assessed by RT-PCR. The brain samples showed an average rabies virus (RV) positivity rate of 3.26%, but reached 4.71% for the period Apr 2002 to Dec 2003. A total of 30 isolates were obtained from normal dogs and 28 isolates from rabid animals by the mouse inoculation test (MIT). Six representative group I and II RV isolates showed an LD50 of 10−5.35/ml to 10−6.19/ml. The reactivity of monoclonal antibodies (MAbs) to group I and II RV isolates from the Guangxi major epidemic showed that eight anti-G MAbs showed strong reactivity with isolates of group I and II with titers of ≥10,000; however, the MAbs 9-6, 13-3 and 12-14 showed lower reactivity. Phylogenetic analysis based on the G gene demonstrated that the Guangxi RV isolates have similar topologies with strong bootstrap values and are closely bonded. Alignment of deduced amino acids revealed that the mature G protein has four substitutions A96S, L132F, N436S, and A447I specific to group I, and 13 substitutions T90M, Y168C, S204G, T249I, P253S, S289T, V332I, Q382H, V427I, L474P, R463K Q486H, and T487N specific to group II, coinciding with the phylogenetic analysis of the isolates. Conclusions: Re-emergence of human rabies has mainly occurred in rural areas of Guangxi since 1996. The human rabies incidence rate increased is related with RV positive rate of normal dogs. The Guangxi isolates tested showed a similar pathogenicity and antigenicity. The results of phylogenetic analysis coincide with that of alignment of deduced amino acids. Author Summary: Rabies is a worldwide zoonosis disease and is of considerable public health threat and hazard. The Guangxi province of southern China is a severe rabies epidemic region. Human rabies cases decreased from 839 in 1982 to 24 in 1995 in Guangxi as a result of a dog vaccination campaign. However, the number subsequently underwent a sharp increase, and has since maintained a high level. This study reports the systematic surveillance of rabies in Guangxi over the 30-year period from 1982 to 2012. The data revealed that a re-emergence of human rabies has occurred mainly in rural areas of Guangxi since 1996. Human rabies incidence rate increased follows increased instances of RV positive normal dogs. To further understand this re-emergence of rabies, the biological properties of the rabies virus (RV), including the RV-positive rate of normal dogs, pathogenicity, antigenicity and evolution, have been evaluated. The Guangxi isolates all showed similar pathogenicity and antigenicity. These isolates also exhibited similar topologies with strong bootstrap values in the two groups and were closely bonded. Thus these findings will be helpful to understanding the epidemiological situation for rabies in Guangxi. [ABSTRACT FROM AUTHOR]

Published

2014

9. Re-emergence of Rabies in the Guangxi Province of Southern China.

Author

Tang, Hai-Bo, Pan, Yan, Wei, Xian-Kai, Lu, Zhuan-Ling, Lu, Wu, Yang, Jian, He, Xiao-Xia, Xie, Lin-Juan, Zeng, Lan, Zheng, Lie-Feng, Xiong, Yi, Minamoto, Nobuyuki, and Luo, Ting Rong

Subjects

*RABIES in dogs, *RABIES virus, *CATS, *VACCINATION, *MONOCLONAL antibodies, *STATISTICAL bootstrapping, *PHYLOGENY

Abstract

Background: Human rabies cases in the Guangxi province of China decreased from 839 in 1982 to 24 in 1995, but subsequently underwent a sharp increase, and has since maintained a high level. Methodology/Principal Findings: 3,040 brain samples from normal dogs and cats were collected from 14 districts of Guangxi and assessed by RT-PCR. The brain samples showed an average rabies virus (RV) positivity rate of 3.26%, but reached 4.71% for the period Apr 2002 to Dec 2003. A total of 30 isolates were obtained from normal dogs and 28 isolates from rabid animals by the mouse inoculation test (MIT). Six representative group I and II RV isolates showed an LD50 of 10−5.35/ml to 10−6.19/ml. The reactivity of monoclonal antibodies (MAbs) to group I and II RV isolates from the Guangxi major epidemic showed that eight anti-G MAbs showed strong reactivity with isolates of group I and II with titers of ≥10,000; however, the MAbs 9-6, 13-3 and 12-14 showed lower reactivity. Phylogenetic analysis based on the G gene demonstrated that the Guangxi RV isolates have similar topologies with strong bootstrap values and are closely bonded. Alignment of deduced amino acids revealed that the mature G protein has four substitutions A96S, L132F, N436S, and A447I specific to group I, and 13 substitutions T90M, Y168C, S204G, T249I, P253S, S289T, V332I, Q382H, V427I, L474P, R463K Q486H, and T487N specific to group II, coinciding with the phylogenetic analysis of the isolates. Conclusions: Re-emergence of human rabies has mainly occurred in rural areas of Guangxi since 1996. The human rabies incidence rate increased is related with RV positive rate of normal dogs. The Guangxi isolates tested showed a similar pathogenicity and antigenicity. The results of phylogenetic analysis coincide with that of alignment of deduced amino acids. [ABSTRACT FROM AUTHOR]

Published

2014

10. Cloning and expression of Toll-like receptors 1 and 2 from a teleost fish, the orange-spotted grouper Epinephelus coioides

Author

Wei, You Chuan, Pan, Ting Shuang, Chang, Ming Xian, Huang, Bei, Xu, Zhen, Luo, Ting Rong, and Nie, P.

Subjects

*GENE expression, *CLONING, *OSTEICHTHYES, *EPINEPHELUS, *MARICULTURE, *NUCLEOTIDE sequence, *GENETIC code

Abstract

Abstract: The two Toll-like receptors, TLR1 and TLR2 were cloned from orange-spotted grouper, Epinephelus coioides, an important teleost fish in mariculture of Asia. The cDNA sequences of TLR1 and TLR2 are 3195 and 3439bp long, with an open reading frame (ORF) of 2406 and 2466bp, encoding 801 and 821 amino acids, respectively. The TLR family motifs, i.e. leucine-rich repeat (LRR) domains and Toll/interleukin (IL)-1 receptor (TIR) domains are conserved in the TLR1 and TLR2, with nine and ten leucine-rich repeat (LRR) domains, and with one TIR domain, respectively. The TLR1 and TLR2 had a constitutive expression in examined organs/tissues of naïve orange-spotted grouper, and an increased expression of TLR1 and TLR2 at mRNA level was observed in immune organs such as in spleen of LPS and Poly(I:C) stimulated fish. An increased expression of TLR1 and TLR2 was also recorded in immune organs of the fish injected with the bacterial pathogen, Vibrio alginolyticus. Similarly, a significant rise in the expression of MyD88, an adaptor molecule which forms signalling complex with intracellular TIR domain, thus leading to the production of pro-inflammatory cytokines, such as IL-1β, was also observed in the LPS- and Poly(I:C)-stimulated, and V. alginolyticus-infected fish, indicating the possible role of TLR1 and TLR2 in the MyD88 signalling pathway. However, the mechanism involved in the increased expression of TLR1 and TLR2 following LPS and Poly(I:C) stimulation is at present unknown in fish, and further research should be carried out to identify ligands of fish TLR1 and TLR2 in order to understand the function of these receptors. [Copyright &y& Elsevier]

Published

2011

11. Global transcriptional profiles in peripheral blood mononuclear cell during classical swine fever virus infection

Author

Li, Jun, Yu, Yan-Juan, Feng, Li, Cai, Xin-Bin, Tang, Hai-Bo, Sun, Shi-Kai, Zhang, Hong-Yun, Liang, Jing-Jing, and Luo, Ting Rong

Subjects

*CLASSICAL swine fever, *BLOOD cells, *GENETIC transformation, *GENETIC transcription, *LYMPHOCYTES, *MONOCYTES, *RNA, *IMMUNE response, *CELL cycle, *DNA microarrays

Abstract

Abstract: Classical swine fever virus (CSFV) is an etiologic agent that causes a highly contagious disease in pigs. Laying a foundation to solve problems in its pathogenic mechanism, microarray analysis was performed to detect the gene transcriptional profiles in peripheral blood mononuclear cells (PBMC) following infection with a Chinese highly virulent CSFV strain Shimen. Three susceptible pigs were inoculated intramuscularly with a lethal dose (1.0×106 TCID50) of CSFV. Pigs showed classical CSF signs, depletion of lymphocytes and monocytes consistent with CSFV infection, and the CSFV genome was also confirmed in the PBMC. The PBMC were isolated at 1, 3, 6 and 9 days post-inoculation (dpi). Total RNA were extracted and subjected to microarray analysis. Data showed that expression of 847 genes wherein 467 genes were known function and the remaining 380 genes were unknown function, and 541 up- and 306 down-regulation, altered after infection. There were 54, 181, 438 and 354 up- and 61, 120, 218 and 145 down-regulated genes presented on 1, 3, 6 and 9dpi, respectively. These genes were involved in immune response (14.5%), apoptosis (3.3%), signal transduction (7.6%), transcription (4.4%), metabolism (11%), transport (3.9%), development (6.8%) and cell cycle (3.7%). Results demonstrated its usefulness in exploring the pathogenic mechanisms of CSFV. [Copyright &y& Elsevier]

Published

2010

12. Vaccination demonstration zone successfully controls rabies in Guangxi Province, China.

Author

Wei, Xian-Kai, Xiong, Yi, Li, Xiao-Ning, Zheng, Min, Pan, Yan, He, Xiao-Xia, Liang, Jing-Jing, Liu, Cheng, Zhong, Yi-Zhi, Zou, Lian-Bin, Zheng, Lie-Feng, Guo, Jian-Gang, Li, Chang-Ting, Huang, Sheng-Bin, Gan, Jia-Zhong, Meng, Zhen-Mu, Yang, Jian, Tang, Hai-Bo, Liu, Qi, and Luo, Ting Rong

Subjects

*RABIES vaccines, *DOG vaccination, *RABIES in dogs, *SEROCONVERSION

Abstract

Background: Guangxi is the province most seriously affected by rabies virus (RABV) in China. Those most affected by RABV each year are people in rural areas, where dogs are the main cause of human infection with the virus.Methods: In this study, we established a rabies vaccination demonstration program that included eradication, core, and peripheral areas. This program was implemented for 9 years and comprised three stages: 12 counties in the first stage (2008-2010), 21 counties in the second stage (2011-2013), and then extending to all counties of Guangxi Province in the third stage (2014-2016). The program included a dog vaccination campaign, surveillance of clinically healthy dogs who may be potential RABV carriers, monitoring anti-RABV antibody titers in vaccinated dogs, and compiling and reporting statistics of human rabies cases.Results: The target effectiveness was achieved in the eradication, core, and peripheral areas in all three stages. The vaccination demonstration program successfully promoted RABV vaccination of domestic dogs throughout Guangxi Province by drawing upon the experience gained at key points. Compared with a vaccination coverage rate of 39.42-46.85% in Guangxi Province overall during 2003-2007, this rate gradually increased to 48.98-52.67% in 2008-2010, 60.24-69.67% in 2011-2013, and 70.09-71.53% in 2014-2016, thereby meeting World Health Organization requirements. The total cases of human rabies in the province decreased from 602 in 2004 to 41 cases in 2017.Conclusions: The present pilot vaccination program obviously increased the rabies vaccination and seroconversion rates, and effectively reduced the spread of rabies from dogs to humans as well as the number of human rabies cases, thus successfully controlling rabies in Guangxi. [ABSTRACT FROM AUTHOR]

Published

2018

13. Evolutionary analysis of rabies virus isolates from Guangxi Province of southern China.

Author

Wei, Xian-Kai, He, Xiao-Xia, Pan, Yan, Liu, Cheng, Tang, Hai-Bo, Zhong, Yi-Zhi, Li, Xiao-Ning, Liang, Jing-Jing, and Luo, Ting Rong

Subjects

*RABIES virus, *RABIES in dogs, *DISEASE vectors, *GENETICS, *VETERINARY medicine

Abstract

Background: Rabies is a severe epidemic in Guangxi province, China, with hundreds of deaths occurring each year. In the past six decades, rabies has emerged three times in Guangxi, and the province has reported the largest number of rabies cases in China. The domestic dog is the principal vector for rabies, and 95% of human cases are associated with transmission from dogs. Results: To understand the genetic relationship between street rabies virus (RABV) from Guangxi, genetic diversity analysis was performed using RABV isolates collected between 1999 and 2012. The N gene of 42 RABV isolates, and the P and M genes, as well as fragments of the 3′ terminus (L1–680) and the polymerase activity module of the L gene (Lpam) of 36 RABV isolates were sequenced. In addition, whole genome sequencing was performed for 5 RABV isolates. There was evidence of topological discrepancy in the phylogenetic trees based on different genes of the RABV isolates. Amino acid variation of the deduced N protein exhibited different patterns to those obtained from the P and M proteins reported here, and the previously reported G protein (Tang H. et al., PLoS Negl Trop Dis, 8(10): e3114, 2014), and L1–680 and Lpam. These RABV isolates were divided into three main branches against fixed strains. Conclusion: RABV is prevalent in Guangxi province and strains collected over the last two decades belong mainly to three groups (I, II, III). These RABV isolates reveal genetic diversity. Individual RABV genes from Guangxi exhibit different evolutionary characteristics. The results will have benefits for continuing comprehensive rabies surveillance, prevention and control in China. [ABSTRACT FROM AUTHOR]

Published

2018

14. Viperin inhibits rabies virus replication via reduced cholesterol and sphingomyelin and is regulated upstream by TLR4.

Author

Tang, Hai-Bo, Lu, Zhuan-Ling, Wei, Xian-Kai, Zhong, Tao-Zhen, Zhong, Yi-Zhi, Ouyang, Ling-Xuan, Luo, Yang, Xing, Xing-Wei, Liao, Fang, Peng, Ke-Ke, Deng, Chao-Qian, Minamoto, Nobuyuki, and Luo, Ting Rong

Published

2016