Literature DB >> 25322675

CD11c(+)  CD103(+) cells of Mycobacterium tuberculosis-infected C57BL/6 but not of BALB/c mice induce a high frequency of interferon-γ- or interleukin-17-producing CD4(+) cells.

Cássia A Sérgio1, Thais B Bertolini, Ana Flávia Gembre, Rafael Q Prado, Vânia L D Bonato.   

Abstract

The magnitude of the cellular adaptive immune response is critical for the control of Mycobacterium tuberculosis infection in the chronic phase. In addition, the genetic background is equally important for resistance or susceptibility to tuberculosis. In this study, we addressed whether lung populations of dendritic cells, obtained from genetically different hosts, would play a role in the magnitude and function of CD4(+) populations generated after M. tuberculosis infection. Thirty days post-infection, C57BL/6 mice, which generate a stronger interferon-γ (IFN-γ)-mediated immune response than BALB/c mice, exhibited a higher number and frequency of lung CD11c(+)  CD11b(-)  CD103(+) cells compared with BALB/c mice, which exhibited a high frequency of lung CD11c(+)  CD11b(+)  CD103(-) cells. CD11c(+)  CD11b(-)  CD103(+) cells, purified from lungs of infected C57BL/6 mice, but not from infected BALB/c mice, induced a higher frequency of IFN-γ-producing or interleukin-17 (IL-17)-producing CD4(+) cells. Moreover, CD4(+) cells also arrive at the lung of C57BL/6 mice faster than in BALB/c mice. This pattern of immune response seems to be associated with higher gene expression for CCL4, CCL19, CCL20 and CCR5 in the lungs of infected C57BL/6 mice compared with infected BALB/c mice. The results described here show that the magnitude of IFN-γ-producing or IL-17-producing CD4(+) cells is dependent on CD11c(+)  CD11b(-)  CD103(+) cells, and this pattern of immune response is directly associated with the host genetic background. Therefore, differences in the genetic background contribute to the identification of immunological biomarkers that can be used to design human assays to predict progression of M. tuberculosis infection.
© 2014 John Wiley & Sons Ltd.

Entities:  

Keywords:  T helper type 1 cells; T helper type 17 cells; dendritic cells; genetic background; tuberculosis

Mesh:

Substances:

Year:  2015        PMID: 25322675      PMCID: PMC4368164          DOI: 10.1111/imm.12411

Source DB:  PubMed          Journal:  Immunology        ISSN: 0019-2805            Impact factor:   7.397


  47 in total

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5.  Direct comparison of low-dose and Cornell-like models of chronic and reactivation tuberculosis in genetically susceptible I/St and resistant B6 mice.

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Journal:  Tuberculosis (Edinb)       Date:  2004-12-31       Impact factor: 3.131

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Authors:  I Kramnik; W F Dietrich; P Demant; B R Bloom
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Authors:  M Gonzalez-Juarrero; O C Turner; J Turner; P Marietta; J V Brooks; I M Orme
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Authors:  R Ribeiro-Rodrigues; T Resende Co; R Rojas; Z Toossi; R Dietze; W H Boom; E Maciel; C S Hirsch
Journal:  Clin Exp Immunol       Date:  2006-04       Impact factor: 4.330

10.  Progression of chronic pulmonary tuberculosis in mice aerogenically infected with virulent Mycobacterium tuberculosis.

Authors:  E R Rhoades; A A Frank; I M Orme
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  11 in total

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3.  Genetic background affects the expansion of macrophage subsets in the lungs of Mycobacterium tuberculosis-infected hosts.

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Journal:  Immunology       Date:  2016-05       Impact factor: 7.397

4.  Neonatal Fc Receptor Regulation of Lung Immunoglobulin and CD103+ Dendritic Cells Confers Transient Susceptibility to Tuberculosis.

Authors:  Alexis Vogelzang; Laura Lozza; Stephen T Reece; Carolina Perdomo; Ulrike Zedler; Karin Hahnke; Dagmar Oberbeck-Mueller; Anca Dorhoi; Stefan H E Kaufmann
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5.  Targeting dendritic cells to accelerate T-cell activation overcomes a bottleneck in tuberculosis vaccine efficacy.

Authors:  Kristin L Griffiths; Mushtaq Ahmed; Shibali Das; Radha Gopal; William Horne; Terry D Connell; Kelly D Moynihan; Jay K Kolls; Darrell J Irvine; Maxim N Artyomov; Javier Rangel-Moreno; Shabaana A Khader
Journal:  Nat Commun       Date:  2016-12-22       Impact factor: 14.919

6.  M2 macrophages or IL-33 treatment attenuate ongoing Mycobacterium tuberculosis infection.

Authors:  A R Piñeros; L W Campos; D M Fonseca; T B Bertolini; A F Gembre; R Q Prado; J C Alves-Filho; S G Ramos; M Russo; V L D Bonato
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9.  PPE38 Protein of Mycobacterium tuberculosis Inhibits Macrophage MHC Class I Expression and Dampens CD8+ T Cell Responses.

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10.  CCR4-dependent reduction in the number and suppressor function of CD4+Foxp3+ cells augments IFN-γ-mediated pulmonary inflammation and aggravates tuberculosis pathogenesis.

Authors:  Thais B Bertolini; Annie R Piñeros; Rafael Q Prado; Ana Flávia Gembre; Leandra N Z Ramalho; José Carlos Alves-Filho; Vânia L D Bonato
Journal:  Cell Death Dis       Date:  2018-12-21       Impact factor: 8.469

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