Your search keyword '"Liu, Hai-can"' showing total 7 results

1. Immunogenicity of Whole Mycobacterium intracellulare Proteins and Fingding on the Cross-Reactive Proteins between M. intracellulare and M. tuberculosis.

Author

XIAO, Shi Qi, XU, Da, DUAN, Hong Yang, FAN, Xue Ting, LI, Gui Lian, ZHANG, Wen, LI, Ma Chao, HAN, Na, LI, Xin Yao, LI, Na, ZHAO, Li lan, ZHAO, Xiu Qin, WAN, Kang Lin, LIU, Hai Can, and FENG, Wen Hai

Subjects

TUBERCULOSIS, BLOOD proteins, MYCOBACTERIUM, TUBERCULOSIS vaccines, PROTEINS, IMMUNOGLOBULIN M

Abstract

To evaluate the immunogenicity of Mycobacterium intracellulare proteins and determine the cross-reactive proteins between M. intracellulare and M. tuberculosis. Protein extracts from M. intracellulare were used to immunize BALB/c mice. The antigens were evaluated using cellular and humoral immunoassays. The common genes between M. intracellular and M. tuberculosis were identified using genome-wide comparative analysis, and cross-reactive proteins were screened using immunoproteome microarrays. Immunization with M. intracellulare proteins induced significantly higher levels of the cytokines interferon-γ (IFN-γ), interleukin-2 (IL-2), interleukin-12 (IL-12), interleukin-6 (IL-6) and immunoglobulins IgG, IgG1, IgM, and IgG2a in mouse serum. Bone marrow-derived macrophages isolated from mice immunized with M. intracellulare antigens displayed significantly lower bacillary loads than those isolated from mice immunized with adjuvants. Whole-genome sequence analysis revealed 396 common genes between M. intracellulare and M. tuberculosis. Microchip hybridization with M. tuberculosis proteins revealed the presence of 478 proteins in the serum of mice immunized with M. intracellulare protein extracts. Sixty common antigens were found using both microchip and genomic comparative analyses. This is the advanced study to investigate the immunogenicity of M. intracellulare proteins and the cross-reactive proteins between M. intracellulare and M. tuberculosis. The results revealed the presence of a number of cross-reactive proteins between M. intracellulare and M. tuberculosis. Therefore, this study provides a new way of identifying immunogenic proteins for use in tuberculosis vaccines against both M. intracellulare and M. tuberculosis in future. [ABSTRACT FROM AUTHOR]

Published

2021

2. Immunological Evaluation of a Novel Mycobacterium tuberculosis Antigen Rv0674.

Author

XIAO, Tong Yang, LIU, Hai Can, LI, Xiao Qin, HUANG, Ming Xiang, LI, Gui Lian, LI, Na, YAN, Yu Han, LUO, Qiao, WANG, Xue Zhi, LI, Ma Chao, and WAN, Kang Lin

Subjects

MYCOBACTERIUM tuberculosis, ANTIGENS, CELLULAR immunity, IMMUNOGLOBULIN G, HUMORAL immunity, INTERLEUKIN-6

Abstract

This study aimed to characterize the diagnostic and vaccine potential of a novel Mycobacterium tuberculosis antigen Rv0674. To evaluate the diagnostic potential and antigenicity of Rv0674, IgG was evaluated using ELISA and interferon (IFN)-γ was done by using ELISpot assay among TB patients and healthy donors. For immunogenicity evaluation, BALB/c mice were immunized with Rv0674. Cytokine production was determined by cytokine release assay using an ELISA kit, and the antibodies were tested using ELISA. The results of serum Elisa tests showed that Rv0674 specific immunoglobulin G (IgG) response was higher in TB patients than negative controls. And Rv0674 had good performance in serological test with sensitivity and specificity of 77.1% and 81.1%, respectively. While it shows poor sensitivity and specificity of 26.23% and 79.69% for IFN-γ tests. In BALB/c mice, Rv0674 adjuvant by DDA/Poly I:C could also induce a high level of IFN-γ, interleukin-2 and interleukin-6 as well as a high IgG titer in both high- and low-dose groups indicating that Rv0674 is essential in humoral and cellular immunity. Moreover, the cytokine profile and IgG isotype characterized Rv0674 as a Th1/Th2-mixed-type protective immunity with the predominance of Th1 cytokines. Rv0674 may be a good potential candidate for the development of TB serological diagnosis and a new TB vaccine. [ABSTRACT FROM AUTHOR]

Published

2019

3. Preliminary Study on Drug Susceptibility Profile and Resistance Mechanisms to Macrolides of Clinical Isolates of Non-tuberculous Mycobacteria from China.

Author

LI, Fu, LI, Gui Lian, PANG, Hui, LIU, Hai Can, XIAO, Tong Yang, LI, Shuang Jun, LUO, Qiao, JIANG, Yi, WANG, Rui Bai, and WAN, Kang Lin

Subjects

DISEASE susceptibility, MACROLIDE antibiotics, CLINICAL trials, TUBERCULOSIS prevention, PUBLIC health

Abstract

Objective Macrolide susceptibility and drug resistance mechanisms of clinical non-tuberculous mycobacteria (NTM) isolates were preliminarily investigated for more accurate diagnosis and treatment of the infection in China. Methods Four macrolides, including clarithromycin (CLAR), azithromycin (AZM), roxithromycin (ROX), and erythromycin (ERY), were used to test the drug susceptibility of 310 clinical NTM isolates from six provinces of China with the broth microdilution method. Two resistance mechanisms, 23S rRNA and erm , were analyzed with nucleotide sequence analysis. Results Varied effectiveness of macrolides and species-specific resistance patterns were observed. Most Mycobacterium abscessus subsp. massiliense were susceptible and all M. fortuitum were highly resistant to macrolides. All the drugs, except for erythromycin, exhibited excellent activities against slow-growing mycobacteria, and drug resistance rates were below 22.2%. Only four highly resistant strains harbored 2,058/2,059 substitutions on rrl and none of other mutations were related to macrolide resistance. G2191A and T2221C on rrl were specific for the M. abscessus complex (MABC). Seven sites, G2140A, G2210C, C2217G, T2238C, T2322C, T2404C, and A2406G, were specifically carried by M. avium and M. intracellulare . Three sites, A2192G, T2358G, and A2636G, were observed only in M. fortuitum and one site G2152A was specific for M. gordonae . The genes erm (39) and erm (41) were detected in M. fortuitum and M. abscessus and inducible resistance was observed in relevant sequevar. Conclusion The susceptibility profile of macrolides against NTM was demonstrated. The well-known macrolide resistance mechanisms, 23S rRNA and erm , failed to account for all resistant NTM isolates, and further studies are warranted to investigate macrolide resistance mechanisms in various NTM species. [ABSTRACT FROM AUTHOR]

Published

2018

4. First Report in China on the Identification and Drug Sensitivity of Mycobacterium elephantis Isolated from the Milk of a Cow with Mastitis.

Author

JI, Ling Yun, XU, Dong Lei, YIN, Shu Peng, LIU, Hai Can, LI, Gui Lian, JIANG, Yi, WEI, Jian Hao, ZENG, Hao, LOU, Yong Liang, LYU, Jian Xin, and WAN, Kang Lin

Subjects

BOVINE mastitis, MYCOBACTERIUM, MILK quality, COW diseases, POLYMERASE chain reaction, RIBOSOMAL RNA

Abstract

Objective In this study, milk from a cow with mastitis was analyzed to determine the presence of mycobacterial infection. Milk quality and security problems pertaining to the safe consumption of dairy products were also discussed in this study. Methods Milk was preprocessed with 4% NaOH. Then, mycobacteria were isolated from the milk sample on L-J medium. The isolate was identified using multiple loci Polymerase Chain Reaction (PCR) and multi-locus sequence analysis with 16S rRNA , sodA , hsp65 , and ITS genes. The drug sensitivity of the isolate to 27 antibiotics was tested through alamar blue assay. Results Smooth, moist, pale yellow colonies appeared on the L-J medium within a week after inoculation. Based on the results of multiple loci PCR analysis, the isolate was preliminarily identified as non-tuberculous mycobacteria. The 16S rRNA , SodA , hsp65 , and ITS gene sequences of the isolate exhibited 99%, 99%, 99%, and 100% similarities, respectively, with those of the published reference strains of Mycobacterium elephantis (M. elephantis) . The drug sensitivity results showed that the strain is resistant to isoniazid, p-aminosalicylic acid, and trimesulf but is sensitive to ofloxacin, rifampicin, amikacin, capreomycin, moxifloxacin, kanamycin, levofloxacin, cycloserine, ethambutol, streptomycin, tobramycin, rifabutin, ciprofloxacin, linezolid, cefoxitin, clarithromycin, and minocycline. Conclusion To the best of our knowledge, this study is initially to report the isolation of M. elephantis from the milk of a cow with mastitis in China. [ABSTRACT FROM AUTHOR]

Published

2017

5. Molecular Characteristics and Drug Susceptibility of Mycobacterium tuberculosis Isolates from Patients Co-infected with Human Immunodeficiency Virus in Beijing, China.

Author

LIU, Jie, WANG, Hui Zhu, LIAN, Lu Lu, YU, Yan Hua, ZHAO, Xiu Qin, GUO, Cai Ping, LIU, Hai Can, LIU, Shu Mei, ZHAO, Hui, ZENG, Zhao Ying, ZHAO, Xiu Ying, and WAN, Kang Lin

Subjects

MYCOBACTERIUM tuberculosis, MOLECULAR biology, MICROBIAL sensitivity tests, HIV-positive persons

Published

2015

6. A new Multilocus Sequence Analysis Scheme for Mycobacterium tuberculosis.

Author

LU, Bing, DONG, Hai Yan, ZHAO, Xiu Qin, LIU, Zhi Guang, LIU, Hai Can, ZHANG, Yuan Yuan, JIANG, Yi, and WAN, Kang Lin

Subjects

MYCOBACTERIUM tuberculosis, SEQUENCE analysis, SINGLE nucleotide polymorphisms, PHYLOGENY, GENOMES, EPIDEMIOLOGY, RESTRICTION fragment length polymorphisms, GENETICS

Abstract

Abstract: Objective: Tuberculosis remains one of the most serious infectious diseases in the world. In this study, a scheme of Mycobacterium tuberculosis (M. tuberculosis) multilocus sequence analysis (MLSA) was established for the phylogenetic and epidemiology analysis. Methods: To establish the scheme of M. tuberculosis MLSA, the genome of H37Rv, CCDC5079 and CCDC5180 were compared, and some variable genes were chosen to be the MLSA typing scheme. 44 M. tuberculosis clinical isolates were typed by MLSA, IS6110-RFLP, and soligotyping, to evaluate the MLSA methods. Results: After comparison of the genome, seven high discrimination gene loci (recX, rpsL, rmlC, rpmG1, mprA, gcvH, ideR) were chosen to be the MLSA typing scheme finally. 11 variable SNP sites of those seven genes were found among the 44 M. tuberculosis isolate strains and 11 sequence types (STs) were identified. Based on the Hunter-Gaston Index (HGI), MLSA typing was not as good for discrimination at the strain level as IS6110-RFLP, but the HGI was much better than that of spoligotyping. In addition, the MEGA analysis result of MLSA data was similar to spoligotyping/PGG lineage, showing a strong phylogenetic signal in the modern strains of M. tuberculosis. The MLSA data analysis by eBURST revealed that 4 sequence types (ST) came into a main cluster, showing the major clonal complexes in those 44 strains. Conclusion: MLSA genotyping not only can be used for molecular typing, but also is an ideal method for the phylogenetic analysis for M. tuberculosis. [Copyright &y& Elsevier]

Published

2012

7. Evaluation of Four Candidate VNTR Loci for Genotyping 225 Chinese Clinical Mycobacterium Tuberculosis Complex Strains.

Author

JIANG, Yi, LIU, Hai Can, ZHENG, Hua Jun, TANG, Biao, DOU, Xiang Feng, ZHAO, Xiu Qin, ZHU, Yong Qiang, LU, Bing, WANG, Sheng Yue, DONG, Hai Yan, ZHAO, Guo Ping, ZHANG, Yuan Yuan, KAN, Biao, and WAN, Kang Lin

Subjects

LOCUS (Genetics), MYCOBACTERIUM tuberculosis, CHINESE people, NUCLEOTIDE sequence, LUNG diseases, COMMUNICABLE diseases, DISEASES

Abstract

Abstract: Objective: To evaluate four candidate variable number tandem repeat (VNTR) loci for genotyping Mycobacterium tuberculosis complex strains. Methods: Genomic sequences for two M. tuberculosis strains (CCDC5079 and CCDC5180) were generated, and using published sequence data, four candidate VNTR loci were identified. The VNTRs were used to genotype 225 Chinese clinical M. tuberculosis complex strains. The discriminatory power of the VNTRs was evaluated using BioNumerics 5.0 software. Results: The Hunter-Gaston Index (HGI) for BJ1, BJ2, BJ3, and BJ4 loci was 0.634, 0.917, 0.697, and 0.910, respectively. Combining all four loci gave an HGI value of 0.995, thus confirming that the genotyping had good discriminatory power. The HGI values for BJ1, BJ2, BJ3, and BJ4, obtained from Beijing family strain genotyping, were 0.447, 0.878, 0.315, and 0.850, respectively. Combining all four loci produced an HGI value of 0.988 for genotyping the Beijing family strains. We observed unique patterns for M. bovis and M. africanum strains from the four loci. Conclusion: We have shown that the four VNTR loci can be successfully used for genotyping M. tuberculosis complex strains. Notably, these new loci may provide additional information about Chinese M. tuberculosis isolates than that currently afforded by established VNTR loci typing. [Copyright &y& Elsevier]

Published

2012