Go to The Journal of Clinical Investigation
  • About
  • Editors
  • Consulting Editors
  • For authors
  • Publication ethics
  • Publication alerts by email
  • Transfers
  • Advertising
  • Job board
  • Contact
  • Physician-Scientist Development
  • Current issue
  • Past issues
  • By specialty
    • COVID-19
    • Cardiology
    • Immunology
    • Metabolism
    • Nephrology
    • Oncology
    • Pulmonology
    • All ...
  • Videos
  • Collections
    • In-Press Preview
    • Resource and Technical Advances
    • Clinical Research and Public Health
    • Research Letters
    • Editorials
    • Perspectives
    • Physician-Scientist Development
    • Reviews
    • Top read articles

  • Current issue
  • Past issues
  • Specialties
  • In-Press Preview
  • Resource and Technical Advances
  • Clinical Research and Public Health
  • Research Letters
  • Editorials
  • Perspectives
  • Physician-Scientist Development
  • Reviews
  • Top read articles
  • About
  • Editors
  • Consulting Editors
  • For authors
  • Publication ethics
  • Publication alerts by email
  • Transfers
  • Advertising
  • Job board
  • Contact
Rare variable M. tuberculosis antigens induce predominant Th17 responses in human infection
Paul Ogongo, Liya Wassie, Anthony Tran, Devin Columbus, Julia Huffaker, Lisa Sharling, Gregory Ouma, Samuel Gurrion Ouma, Kidist Bobosha, Cecilia S. Lindestam Arlehamn, Neel R. Gandhi, Sara C. Auld, Jyothi Rengarajan, Cheryl L. Day, Artur Queiroz, Mariana Araújo-Pereira, Eduardo Fukutani, Bruno B. Andrade, John D. Altman, Henry M. Blumberg, Joel D. Ernst, the TBRU ASTRa Study Group
Paul Ogongo, Liya Wassie, Anthony Tran, Devin Columbus, Julia Huffaker, Lisa Sharling, Gregory Ouma, Samuel Gurrion Ouma, Kidist Bobosha, Cecilia S. Lindestam Arlehamn, Neel R. Gandhi, Sara C. Auld, Jyothi Rengarajan, Cheryl L. Day, Artur Queiroz, Mariana Araújo-Pereira, Eduardo Fukutani, Bruno B. Andrade, John D. Altman, Henry M. Blumberg, Joel D. Ernst, the TBRU ASTRa Study Group
View: Text | PDF
Clinical Research and Public Health Immunology Infectious disease Microbiology

Rare variable M. tuberculosis antigens induce predominant Th17 responses in human infection

  • Text
  • PDF
Abstract

CD4 T cells are essential for immunity to M tuberculosis (Mtb), and emerging evidence indicates that IL-17–producing Th17 cells contribute to immunity to Mtb. While identifying protective T cell effector functions is important for TB vaccine design, T cell antigen specificity is also likely to be important. To identify antigens that induce protective immunity, we reasoned that, as in other pathogens, effective immune recognition drives sequence diversity in individual Mtb antigens. We previously identified Mtb genes under evolutionary diversifying selection pressure whose products we term Rare Variable Mtb Antigens (RVMA). Here, in 2 distinct human cohorts with recent exposure to TB, we found that RVMA preferentially induce CD4 T cells that express RoRγt and produce IL-17, in contrast to “classical” Mtb antigens that induce T cells that produce IFN-γ. Together with emerging evidence showing human Th17 responses are associated with prevention of progression to TB disease, our results suggest that RVMA can be valuable antigens in vaccines for those already infected with Mtb to amplify existing antigen-specific Th17 responses to prevent TB disease.

Authors

Paul Ogongo, Liya Wassie, Anthony Tran, Devin Columbus, Julia Huffaker, Lisa Sharling, Gregory Ouma, Samuel Gurrion Ouma, Kidist Bobosha, Cecilia S. Lindestam Arlehamn, Neel R. Gandhi, Sara C. Auld, Jyothi Rengarajan, Cheryl L. Day, Artur Queiroz, Mariana Araújo-Pereira, Eduardo Fukutani, Bruno B. Andrade, John D. Altman, Henry M. Blumberg, Joel D. Ernst, the TBRU ASTRa Study Group

×

Figure 1

Distinct Mtb antigens elicit T cell responses with different functional properties (Cohort 1).

Options: View larger image (or click on image) Download as PowerPoint
Distinct Mtb antigens elicit T cell responses with different functional ...
(A) Whole blood samples from QFT+HIV– participants in Cohort 1 (KEMRI, Kisumu, Kenya) were stimulated with 60 individual Mtb antigens as overlapping peptides (1 μg/mL) for 7 days, and supernatants were harvested to quantitate IFN-γ by ELISA. The antigens are arranged left to right (antigens 1–60) according to their positions on the Mtb chromosome, and individual participant samples are arranged in rows. Data presented are results after subtraction of the average of 6 unstimulated wells as the background response. IFN-γ levels are color coded according to magnitude, with red for the lowest and green for the highest responses. Responses greater than the highest standard were assigned the value of the highest standard (1,000 pg/mL). Selected antigens are highlighted at the top of the heatmap, with arrows indicating 6 of the 7 RVMA. The identity of all of the antigens ordered in the same fashion is available in ref. 37. (B) Whole blood IFN-γ response magnitude of selected classical antigens (Tb10.4 [EsxH], PE13, PPE18, Ag85B, PPE46, Ag85A, CFP-10, ESAT-6, and EspI) compared with the 6 RVMA (Rv0010c, Rv0012, RimJ, LldD2, Rv2719c, and TB7.3); the red horizontal line represents the median response. Statistical significance was determined by the Mann-Whitney U test. (C) Representative flow cytometry plots comparing CD4 T cells producing IFN-γ or IL-17 in response to stimulation with one of the RVMA (Rv0012); background response for each cytokine is shown for comparison. (D and E) Cryopreserved peripheral blood mononuclear cells (PBMC) were stimulated with indicated antigens (2 mg/mL) for a total of 20 hours in the presence of Golgi Stop and Golgi Plug as well as costimulatory antibodies anti-CD28 and anti-CD49d; cytokine production by CD4+ T cells was determined by intracellular cytokine staining and flow cytometry. Data are values after subtraction of unstimulated cells, with values lower than the unstimulated control cells indicated below the dotted line (cut-off of positive response). The frequency of participants with a detectable response is shown at the top of each antigen plot. Each symbol is a distinct participant; the horizontal blue line indicates the median cytokine response. Results for RVMA are shown in D, and results for the classical antigens are shown in E.

Copyright © 2026 American Society for Clinical Investigation
ISSN 2379-3708

Sign up for email alerts