Effects of Mycobacterium tuberculosis EsxV/W Fusion Protein on the Phenotype of Mycolicibacterium smegmatis and Macrophage Function

Abstract

Abstract: Objective：To construct recombinant Mycolicibacterium smegmatis（MS） expressing Mycobacterium tuberculosis EsxV/W
fusion protein and analyze the phenotype of the recombinant MS and its effect on the macrophage function. Methods: The EsxV/W
fusion protein was obtained by prokaryotic expression, and polyclonal antibody was prepared by immunizing mice with purified EsxV/W
fusion protein. The recombinant strain MS-EsxV/W and the control strain MS-vec were constructed by electroporation, and the
expression of the fusion protein in MS was detected by using the generated polyclonal antibody. The colony morphology, biofilm
formation, and growth rate of the recombinant MS expressing EsxV/W fusion protein were analyzed. The survival ability of the
recombinant MS under different conditions, such as lysozyme, malachite green, low pH, SDS, H2O2 and NaNO2, was determined using
colony counting method to assess the impact of EsxV/W fusion protein on the phenotype of MS. The recombinant MS was used to infect
ANA-1 macrophages. The release of NO from ANA-1 cells was detected by Griess method. Enzyme-linked immunosorbent assay was
performed to measure the release of tumor necrosis factor-α （TNF-α） and interleukin-6 （IL-6） from ANA-1 cells, and the survival
ability of the recombinant MS in ANA-1 cells was determined using colony counting method. Results：The recombinant strain MSEsxV/
W expressing EsxV/W fusion protein, was successfully constructed. The expression of EsxV/W fusion protein had no significant
effect on the colony morphology, biofilm formation and growth rate of MS. The expression of EsxV/W fusion protein did not change the
tolerance of MS to lysozyme, malachite green or low pH, but decreased the tolerance to SDS and increased the tolerance to H2O2 and
NaNO2. After infecting ANA-1 cells for a certain period of time, the release of NO, TNF-α and IL-6 in ANA-1 cells infected by MSEsxV/
W was significantly increased compared with MS-vec, and the intracellular survival ability of MS-EsxV/W was higher than that
of MS-vec. Conclusion：The EsxV/W fusion protein can change the phenotype of MS and regulate the immune response of ANA-1
macrophages, which is conducive to the subsequent investigation of the function of esxV/W gene

Key words: Mycobacterium tuberculosis, Mycolicibacterium smegmatis, EsxV/W fusion protein, ANA-1 cells

CLC Number:

R392.12

Yu Haiyan, Li Yujie, Ren Qin, Yang Guoping. Effects of Mycobacterium tuberculosis EsxV/W Fusion Protein on the Phenotype of Mycolicibacterium smegmatis and Macrophage Function[J]. Journal of Dali University, 2024, 9(2): 32-38.

References

〔1〕 FINE P E M. Variation in Protection by BCG： Implications
of and for Heterologous Immunity〔J〕. Lancet，1995，346
（8986）：1339-1345.
〔2〕 CRAMPIN A C，GLYNN J R，FINE P E M. What Has
Karonga Taught Us? Tuberculosis Studied over Three De⁃
cades〔J〕. Int J Tuberc Lung Dis，2009，13（2）：153-164.
〔3〕 BEHR M A，WILSON M A，GILL W P，et al. Comparative
Genomics of BCG Vaccines by Whole Genome DNA Micro⁃
array〔J〕. Science，1999，284（5419）：1520-1523.
〔4〕 MUSTAFA A S. Vaccine Potential of Mycobacterium
tuberculosis-Specific Genomic Regions：In vitro Studies in
Humans〔J〕. Expert Rev Vaccines，2009，8（10）：1309-
1312.

〔5〕 MUSTAFA A S. Immunological Characterization of Proteins

Expressed by Genes Located in Mycobacterium tuberculosis-
Specific Genomic Regions Encoding the ESAT6-Like Pro⁃
teins〔J〕. Vaccines，2021，9（1）：27.
〔6〕 SAFAR H A，EL-HASHIM A Z，AMOUDY H，et al. Myco⁃
bacterium tuberculosis-Specific Antigen Rv3619c Effec⁃
tively Alleviates Allergic Asthma in Mice〔J〕. Front Phar⁃
macol，2020，11：532199.
〔7〕 OSMAN M M，SHANAHAN J K，CHU F，et al. The C Ter⁃
minus of the Mycobacterium ESX-1 Secretion System Sub⁃
strate ESAT-6 Is Required for Phagosomal Membrane Dam⁃
age and Virulence〔J〕. Proc Natl Acad Sci USA，2022，119
（11）：e2122161119.
〔8〕 JUNG B G，WANG X S，YI N，et al. Early Secreted
Antigenic Target of 6-kDa of Mycobacterium tuberculosis
Stimulates IL-6 Production by Macrophages through Acti⁃
vation of STAT3〔J〕. Sci Rep，2017，7：40984.
〔9〕 JANG A R，CHOI J H，SHIN S J，et al. Mycobacterium
tuberculosis ESAT6 Induces IFN- β Gene Expression in
Macrophages via TLRS-Mediated Signaling〔J〕. Cytokine，
2018，104：104-109.
〔10〕 T J A S，J R，RAJAN A，et al. Features of the Biochemis⁃
try of Mycobacterium smegmatis，as a Possible Model for
Mycobacterium tuberculosis〔J〕. J Infect Public Health，
2020，13（9）： 1255-1264.
〔11〕 MARMIESSE M，BRODIN P，BUCHRIESER C，et al.
Macro-Array and Bioinformatic Analyses Reveal Myco⁃
bacterial ‘Core’ Genes，Variation in the ESAT-6 Gene
Family and New Phylogenetic Markers for the Mycobacte⁃
rium tuberculosis Complex〔J〕. Microbiology （Reading），
2004，150（Pt2）：483-496.
〔12〕 ZHANG M M，ZHAO J W，SUN Z Q，et al. Identification
of RD5-Encoded Mycobacterium tuberculosis Proteins as
B-Cell Antigens Used for Serodiagnosis of Tuberculo⁃
sis〔J〕. Clin Dev Immunol，2012，2012：738043.
〔13〕 MOHANTY S，DAL MOLIN M，GANGULI G，et al. Myco⁃
bacterium tuberculosis EsxO （Rv2346c） Promotes Bacil⁃
lary Survival by Inducing Oxidative Stress Mediated
Genomic Instability in Macrophages〔J〕. Tuberculosis，
2016，96：44-57.
〔14〕 SAFAR H A，MUSTAFA A S，AMOUDY H A，et al. The
Effect of Adjuvants and Delivery Systems on Th1，Th2，
Th17 and Treg Cytokine Responses in Mice Immunized
with Mycobacterium tuberculosis-Specific Proteins〔J〕.
PLoS One，2020，15（2）：e0228381.

[1]	Zhang Jinglan, Chen Ran. Validation Study of Xpert MTB/RIF in Diagnosis of Pulmonary Tuberculosis and Detection of Rifampicin Resistance [J]. Journal of Dali University, 2021, 6(10): 63-.
[2]	Li Ping, Li Congzhe, Wu Lixian. Effects of Mycobacterium tuberculosis with Different Virulence on the Apoptosis Rate of Mouse Dendritic Cells [J]. Journal of Dali University, 2020, 5(10): 35-39.
[3]	HAO Xian-Bin, NIE Heng, WANG Xu-Dong, TUN Li-Xian. Study on the Application of PFGE in Mtb Genotyping of HIV/Mtb Co-infection [J]. , 2019, 4(4): 26-30.
[4]	NIE Heng, GAO Zhi-Fang, WU Li-Xian. The Study of Auto-inducing Fermentation of Mycobacterium tuberculosis Protein MTB8.1 [J]. J4, 2014, 13(8): 18-22.
[5]	DONG Yi, WU Li-Xian. A Study of Genotyping in Mycobacterium tuberculosis Strains in Dali by VNTR Technique [J]. J4, 2014, 13(8): 23-25.
[6]	DENG Yi-Hao, HE Hong-Yun, WANG Yong. Research Progress of ESX-1 Secretion System of Mycobacterium tuberculosis [J]. J4, 2012, 11(12): 20-23.