1. Immunology and Inflammation

T follicular helper 17 (Tfh17) cells are superior for immunological memory maintenance

  1. Xin Gao
  2. Kaiming Luo
  3. Diya Wang
  4. Yunbo Wei
  5. Yin Yao
  6. Jun Deng
  7. Yang Yang
  8. Qunxiong Zeng
  9. Xiaoru Dong
  10. Le Xiong
  11. Dongcheng Gong
  12. Lin Lin
  13. Kai Pohl
  14. Shaoling Liu
  15. Yu Liu
  16. Lu Liu
  17. Thi HO Nguyen
  18. Lilith F Allen
  19. Katherine Kedzierska
  20. Yanliang Jin
  21. Mei-Rong Du
  22. Wanping Chen
  23. Liangjing Lu
  24. Nan Shen
  25. Zheng Liu
  26. Ian A Cockburn  Is a corresponding author
  27. Wenjing Luo  Is a corresponding author
  28. Di Yu  Is a corresponding author
  1. Immunology and Infectious Disease Division, John Curtin School of Medical Research, The Australian National University, Australia
  2. China-Australia Centre for Personalised Immunology, Renji Hospital, School of Medicine, Shanghai Jiao Tong University, China
  3. Department of Occupational and Environmental Health and the Ministry of Education Key Lab of Hazard Assessment and Control in Special Operational Environment, School of Public Health, Fourth Military Medical University, China
  4. Laboratory of Immunology for Environment and Health, Shandong Analysis and Test Center, Qilu University of Technology, Shandong Academy of Sciences, China
  5. Department of Otolaryngology-Head and Neck Surgery, Tongji Hospital, Tongji Medical College, Huazhong University of Science and Technology, China
  6. Frazer Institute, Faculty of Medicine, University of Queensland, Australia
  7. Department of Rheumatology, Shanghai Institute of Rheumatology, Renji Hospital, School of Medicine, Shanghai Jiao Tong University, China
  8. Department of Laboratory Medicine, Ruijin Hospital, School of Medicine, Shanghai Jiao Tong University, China
  9. Shanghai Children's Medical Centre, Shanghai Jiao Tong University, China
  10. Obstetrics and Gynecology Hospital of Fudan University (Shanghai Red House Obstetrics and Gynecology Hospital), China
  11. Department of Microbiology and Immunology, Peter Doherty Institute for Infection and Immunity, University of Melbourne, Australia
  12. Ian Frazer Centre for Children’s Immunotherapy Research, Children’s Health Research Centre, Faculty of Medicine, University of Queensland, Australia
https://doi.org/10.7554/eLife.82217
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Cite this article
  1. Xin Gao
  2. Kaiming Luo
  3. Diya Wang
  4. Yunbo Wei
  5. Yin Yao
  6. Jun Deng
  7. Yang Yang
  8. Qunxiong Zeng
  9. Xiaoru Dong
  10. Le Xiong
  11. Dongcheng Gong
  12. Lin Lin
  13. Kai Pohl
  14. Shaoling Liu
  15. Yu Liu
  16. Lu Liu
  17. Thi HO Nguyen
  18. Lilith F Allen
  19. Katherine Kedzierska
  20. Yanliang Jin
  21. Mei-Rong Du
  22. Wanping Chen
  23. Liangjing Lu
  24. Nan Shen
  25. Zheng Liu
  26. Ian A Cockburn
  27. Wenjing Luo
  28. Di Yu
(2023)
T follicular helper 17 (Tfh17) cells are superior for immunological memory maintenance
eLife 12:e82217.
https://doi.org/10.7554/eLife.82217
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Peer review process

This article was accepted for publication as part of eLife's original publishing model.

History

  1. Version of Record published
  2. Accepted Manuscript published
  3. Accepted
  4. Preprint posted
  5. Received

Decision letter

  1. Tomohiro Kurosaki
    Reviewing Editor; Osaka University, Japan
  2. Satyajit Rath
    Senior Editor; Indian Institute of Science Education and Research (IISER), India
  3. Masato Kubo
    Reviewer; RIKEN, Japan
  4. Joe Craft
    Reviewer; Yale University School of Medicine, United States

Our editorial process produces two outputs: (i) public reviews designed to be posted alongside the preprint for the benefit of readers; (ii) feedback on the manuscript for the authors, including requests for revisions, shown below. We also include an acceptance summary that explains what the editors found interesting or important about the work.

Decision letter after peer review:

Thank you for submitting your article "Type 17 Follicular Helper T (Tfh17) Cells are Superior for Memory Maintenance" for consideration by eLife. Your article has been reviewed by 3 peer reviewers, and the evaluation has been overseen by a Reviewing Editor and Satyajit Rath as the Senior Editor. The following individuals involved in review of your submission have agreed to reveal their identity: Masato Kubo (Reviewer #1); Joe Craft (Reviewer #2).

The reviewers have discussed their reviews with one another, and the Reviewing Editor has drafted this to help you prepare a revised submission.

Essential revisions:

1) As the reviewer 3 suggested, the Figure 7F should be removed or modified, and the text should be clarified so it is clear that all the human Tfh work should be clearly labelled as cTfh.

2) As all the reviewers request, authors should provide the functional data in regard to clarifying the advantage of Tfh17cm cells in humoral immunity. Do they have an advantage over becoming GC Tfh cells compared to Tfh1 and Tfh2 cm populations, and if so, do they have a different phenotype within the GC, or is part of their effect on pre-GC (CSR)?

Reviewer #1 (Recommendations for the authors):

This reviewer personally recommends that the author provide more evidence to indicate the functional relevance of Th17-derived Tfhcm instead of a phenotypical change of chemokine receptor expression.

Reviewer #3 (Recommendations for the authors):

The authors need to clearly describe how they define cTfh in the text (p7), as multiple other labs define cTfh in other ways, with the inclusion of markers (ICOS, CD38, PD-1) in addition to CXCR5, as is used here.

Any use of CXCR5+ cells from the blood must be referred to as cTfh, not Tfh, to clearly distinguish these cells from real Tfh cells found in secondary lymphoid organs.

What is the functional relevance of dividing CXCR5+ cells into TfhEM and TfhCM (figure 3)? I'm not sure that more subsets of cTfh cells are required to make the point about Tfh1/2/17 maintenance and recall.

Using CD45- as a surrogate for immunological age is a huge oversimplification and should not be used as it is incorrect. The authors either need to; remove these plots from the manuscript entirely, rename "immunological age" as what is actually is, %CD45RA- of CD4+ ensuring that they do not imply that this is a surrogate for immunological age, or use a previously validated method to estimate biological age e.g. an epigenetic clock. This reviewer prefers the first suggestion as it is not clear what this analysis adds, as the %CD45RA- cells does not perform better than age in years in the correlations supplied.

https://doi.org/10.7554/eLife.82217.sa1

Author response

Essential revisions:

1) As the reviewer 3 suggested, the Figure 7F should be removed or modified, and the text should be clarified so it is clear that all the human Tfh work should be clearly labelled as cTfh.

Thank you for your suggestions.

  • Figure 7F has been removed.

  • The names for all human Tfh populations in blood have been updated as cTfh (e.g., cTfh1/2/17) in the text and in the figures. We also added a table (Table 1) to summarize the definition of all different Tfh populations in our study as reference.

2) As all the reviewers request, authors should provide the functional data in regard to clarifying the advantage of Tfh17cm cells in humoral immunity. Do they have an advantage over becoming GC Tfh cells compared to Tfh1 and Tfh2 cm populations, and if so, do they have a different phenotype within the GC, or is part of their effect on pre-GC (CSR)?

Following the suggestion from the editor and reviewers, we have conducted several new experiments to investigate the advantage of Tfh17 cells as compared to Tfh1 or Tfh2 cells in humoral immunity. Three non-exclusive hypotheses have been tested.

1) To test whether Tfh17 cells can better survive than Tfh1/2 cells, we transferred either OT-II iTfh1, iTfh2 or iTfh17 cells into CD28KO mice and counted the numbers of transferred cells in the spleen after 1 day and 35 days (Figure 8A). While the numbers of transferred iTfh1/2/17 cells were comparable on day1, the numbers of transferred iTfh17 cells were significantly higher than iTfh1 cells on day35 (Figure 8B-C), suggesting that iTfh17 cells had superior survival capacity over iTfh1 but not iTfh2 cells.

2) To test whether Tfh17 cells may maintain better potential to differentiate into GC-Tfh cells after resting, we transferred either OT-II iTfh1, iTfh2 or iTfh17 cells into CD28KO mice together with NP-specific B1-8 cells, followed by an immediate NP-OVA immunization at day 1 or a delayed NP-OVA immunization to examine the formation of GC-Tfh cells (Figure 8D). In the immediate immunization, iTfh1/2/17 cells expanded and differentiated into GC-Tfh in comparable manners after immunization (Figure 8E-G). However, in the delayed immunization (day 35), iTfh17 cells showed higher expansion than iTfh1 but not iTfh2 cells (Figure 8E). Furthermore, iTfh17 cells differentiated into more GC-Tfh cells than both iTfh1 and iTfh2 cells (Figure 8F-G). These results suggest that iTfh17 cells maintained a better potential to generated GC-Tfh cells compared to Tfh1 or Tfh2 cells, in addition to a better survival than iTfh1 cells.

(3) To compare the B cell helper function between iTfh1/2/17-derived GC-Tfh cells, we sorted iTfh1/2/17-derived CXCR5hi PD-1hi GC-Tfh cells in the same experiment as in ‘(2)’ and measured the expressions of key functional genes in GC-Tfh cells including Pdcd1, Cxcr5, Icos, Cd40lg, Il21 and Bcl6. In the delayed immunization. Despite of better BGC and BASC responses in the iTfh17 group, we found no significant differences in these gene expression among iTfh1/2/17-derived GC-Tfh cells (Figure 8—figure supplement 1A-B). Such results suggest that iTfh1/2/17-derived GC-Tfh cells had comparable B helper function.

In summary, our results suggested that the superior immunological memory maintenance of iTfh17 cells was attributed to their better survival capacity and better maintenance of the potential to differentiate into GC-Tfh cells, rather than better B cell helper function on per cell basis than that of iTfh1 or iTfh2 cells.

Furthermore, we measured the expressions of IFNγ and Il4 in iTfh1/2/17 derived GC-Tfh cells and demonstrated iTfh1 and iTfh2-derived GC-Tfh cells showed featured of increased IFNγ and Il4 respectively, as their counterpart Th1 and Th2 cells (Figure 8—figure supplement 1C). In agreement with polarized cytokine profiles, we detected that iTfh1 cells promoted isotype switching to IgG2a/IgG3 while iTfh2 cells promoted isotype switching to IgG1/IgE (Figure 8—figure supplement 1D). These results suggest iTfh1/2 cells retained polarised cytokine profiles that promote specific class-switch recombination after antigen re-exposure.

We have added the new results and updated the manuscript accordingly (line 348-386).

Reviewer #1 (Recommendations for the authors):

This reviewer personally recommends that the author provide more evidence to indicate the functional relevance of Th17-derived Tfhcm instead of a phenotypical change of chemokine receptor expression.

This recommendation is related to this reviewer’s above comment on the relevance of CCR6 expression to Tfh17’s function. It should be noted that the expression of CCR6 was used as a marker to identify Tfh17 subsets and the difference of Tfh17 and Tfh1/2 is broad and beyond CCR6. We have now added more results to investigate the survival and differentiation potential of Tfh17 v.s. Tfh1/2 cells (new Figure 8). Please refer to the response (2) to Essential Revisions for details.

We agree with this reviewer that the function of CCR6 was not examined in our study. In addition to mediate the cell migration into the inflammatory sites, CCR6 also influences the position of lymphocytes in lymphoid organs (CCR6-dependent positioning of memory B cells is essential for their ability to mount a recall response to antigen, Journal of Immunology 2015; Early CCR6 expression on B cells modulates germinal centre kinetics and efficient antibody responses, Immunology and Cell Biology 2017). The role of CCR6 expression by Tfh17 cells in regulating the supremacy in immunological memory maintenance can be investigated in future study.

Reviewer #3 (Recommendations for the authors):

The authors need to clearly describe how they define cTfh in the text (p7), as multiple other labs define cTfh in other ways, with the inclusion of markers (ICOS, CD38, PD-1) in addition to CXCR5, as is used here.

In this study, cTfh cells were defined as CD4+ CD45RA- CXCR5+ cells (line 70) and are align with the field’s mainstream view. ICOS, CD38, PD-1 are expressed by a subpopulation of cTfh cells (CCR7loPD-1+ICOS+CD38+ cTFH cells are associated with active TFH differentiation – Yu D et al. Targeting TFH cells in human diseases and vaccination: rationale and practice, Nature Immunology 2022).

Any use of CXCR5+ cells from the blood must be referred to as cTfh, not Tfh, to clearly distinguish these cells from real Tfh cells found in secondary lymphoid organs.

Thank you for this suggestion and this has now been corrected throughout the text.

What is the functional relevance of dividing CXCR5+ cells into TfhEM and TfhCM (figure 3)? I'm not sure that more subsets of cTfh cells are required to make the point about Tfh1/2/17 maintenance and recall.

Many studies have reported the existence of CCR7+ and CCR7- cTfh cells that assemble conventional TCM and TEM T cell populations respectively. In our initial study, we experimentally demonstrated that early generated cTfh cells were largely all CCR7- cTfhEM cells and the phenotype was converted to CCR7+ cTfhCM cells (Figure 1F, He J et al. Circulating precursor CCR7loPD-1hi CXCR5+ CD4+ T cells indicate Tfh cell activity and promote antibody responses upon antigen reexposure, Immunity 2013). Therefore, due to the different kinetics of cTfhEM and cTfhCM generation, the preferential enrichment of cTfh1 in cTfhEM cells and the preferential enrichment of cTfh17 in cTfhCM suggest the difference of cTfh1/2/17 subsets in generation or maintenance. This was an important observation that motivated us to conduct the following investigation.

Using CD45- as a surrogate for immunological age is a huge oversimplification and should not be used as it is incorrect. The authors either need to; remove these plots from the manuscript entirely, rename "immunological age" as what is actually is, %CD45RA- of CD4+ ensuring that they do not imply that this is a surrogate for immunological age, or use a previously validated method to estimate biological age e.g. an epigenetic clock. This reviewer prefers the first suggestion as it is not clear what this analysis adds, as the %CD45RA- cells does not perform better than age in years in the correlations supplied.

This comment has been addressed by the response Essential revisions #1.

https://doi.org/10.7554/eLife.82217.sa2

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  1. Xin Gao
  2. Kaiming Luo
  3. Diya Wang
  4. Yunbo Wei
  5. Yin Yao
  6. Jun Deng
  7. Yang Yang
  8. Qunxiong Zeng
  9. Xiaoru Dong
  10. Le Xiong
  11. Dongcheng Gong
  12. Lin Lin
  13. Kai Pohl
  14. Shaoling Liu
  15. Yu Liu
  16. Lu Liu
  17. Thi HO Nguyen
  18. Lilith F Allen
  19. Katherine Kedzierska
  20. Yanliang Jin
  21. Mei-Rong Du
  22. Wanping Chen
  23. Liangjing Lu
  24. Nan Shen
  25. Zheng Liu
  26. Ian A Cockburn
  27. Wenjing Luo
  28. Di Yu
(2023)
T follicular helper 17 (Tfh17) cells are superior for immunological memory maintenance
eLife 12:e82217.
https://doi.org/10.7554/eLife.82217

Share this article

https://doi.org/10.7554/eLife.82217