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IL-10–producing T cells suppress immune responses in anergic tuberculosis patients
Vassiliki A. Boussiotis, … , Jean-Marc Reynes, Anne E. Goldfeld
Vassiliki A. Boussiotis, … , Jean-Marc Reynes, Anne E. Goldfeld
Published May 1, 2000
Citation Information: J Clin Invest. 2000;105(9):1317-1325. https://doi.org/10.1172/JCI9918.
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Article

IL-10–producing T cells suppress immune responses in anergic tuberculosis patients

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Abstract

The lethality of Mycobacterium tuberculosis remains the highest among infectious organisms and is linked to inadequate immune response of the host. Containment and cure of tuberculosis requires an effective cell-mediated immune response, and the absence, during active tuberculosis infection, of delayed-type hypersensitivity (DTH) responses to mycobacterial antigens, defined as anergy, is associated with poor clinical outcome. To investigate the biochemical events associated with this anergy, we screened 206 patients with pulmonary tuberculosis and identified anergic patients by their lack of dermal reactivity to tuberculin purified protein derivative (PPD). In vitro stimulation of T cells with PPD induced production of IL-10, IFN-γ, and proliferation in PPD+ patients, whereas cells from anergic patients produced IL-10 but not IFN-γ and failed to proliferate in response to this treatment. Moreover, in anergic patients IL-10–producing T cells were constitutively present, and T-cell receptor–mediated (TCR-mediated) stimulation resulted in defective phosphorylation of TCRζ and defective activation of ZAP-70 and MAPK. These results show that T-cell anergy can be induced by antigen in vivo in the intact human host and provide new insights into mechanisms by which M. tuberculosis escapes immune surveillance.

Authors

Vassiliki A. Boussiotis, Eunice Y. Tsai, Edmond J. Yunis, Sok Thim, Julio C. Delgado, Christopher C. Dascher, Alla Berezovskaya, Dominique Rousset, Jean-Marc Reynes, Anne E. Goldfeld

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Figure 2

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Culture supernatants after PPD stimulation and CD4+ T cells from anergic...
Culture supernatants after PPD stimulation and CD4+ T cells from anergic TB patients inhibit allogeneic MLR. CD4+ T cells and APC from HLA-disparate healthy individuals were used as responders and stimulators, respectively. Incubation was continued for 7 days with either media alone or in the presence of the indicated concentrations of culture supernatants (Cs) collected at 36 hours after PPD stimulation of CD4+ T cells from PPD+ TB patients, anergic (PPD–) TB patients, and control healthy individuals, or with CD4+ T cells (Tc) from the same individuals. Response was examined by 3H-thymidine incorporation. Results from experiments with one representative patient among three tested in each group are shown.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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