To the editor:
We read with interest the article by Bignami et al that examined the miRNA profile of CD4+ T lymphocytes from patients infected with HIV-1 (long-term non-progressors or treatment naive) versus subjects multiply exposed but uninfected (MEU).1 One of the main findings was the differential expression of only a single miRNA, miR-155, between LTNP and naive HIV-1 infected patients whereas there were many more differentially expressed miRNAs noted between HIV-1 infected patients and MEU. It was suggested that the up-regulation of miR-155 in naive HIV-1 infected patients may contribute to pathogenesis.
miR-155 has previously been noted to play a role in the development of T regulatory cells (Tregs) in murine models.2 We separated out naive Tregs (nveTregs), effector/memory Tregs (eff/memTregs), and conventional naive CD4+ T cells (nveCD4+) from healthy donors based on the differential expression of CD62L, CD45RO, CD25 and CD127 and measured miR-155 levels in these subsets. Tregs were separated using established protocols3 and were: nveTregs (CD25+CD127lowCD62L+CD45RO−, eff/memTregs (CD25+CD127lowCD62L+/−CD45RO+) and nveCD4+ (CD25− CD127highCD62L+CD45RO−). We found miR-155 was strongly expressed in eff/memTregs compared with lower expression levels in both nveTregs and nve CD4+ subsets (Figure 1). Further, we found that levels of eff/memTregs are significantly increased in HIV-1 infected individuals with progressive infection (n = 12) versus those who are LTNPs (n = 9; P = .009 and data not shown), confirming previously reported observations.4 The higher level of activated Tregs with presumably increased miR-155 levels may explain why these levels were different between the 2 HIV-1 infected groups. It was noted in the article that Tregs from naive patients had higher circulating levels of HLA-DR (used as a marker of Treg activation) and we hypothesize that if miR-155 levels were examined in Treg subsets from LTNP versus naive that there would be a difference in miR-155 levels between activated Tregs and both non-activated Tregs and conventional CD4+ subsets and it may be the cell numbers within these sub-populations that explains why levels were noted to be higher in the naive population. Recently, the miRNA profiles from several lymphocyte subsets have been shown to reveal distinct miRNA signatures,5 which further adds to the argument that differences in T cell subsets in HIV-1 infection may be a cause of why there are differences in miRNA levels between various HIV-1 infected populations.
miR-155 expression in Treg subsets. Naive Tregs, effector/memory Tregs and naive conventional CD4+ T cell subsets were FACS sorted based on the phenotype indicated in the text. miR-155 expression was normalized to RNU44 (small-nucleolar RNA) and represented as fold change compared with naive CD4+ T cells. The statistical analysis used was non-parametric 1-way ANOVA Mann Whitney U test (Prism 4.0, GraphicPad).
miR-155 expression in Treg subsets. Naive Tregs, effector/memory Tregs and naive conventional CD4+ T cell subsets were FACS sorted based on the phenotype indicated in the text. miR-155 expression was normalized to RNU44 (small-nucleolar RNA) and represented as fold change compared with naive CD4+ T cells. The statistical analysis used was non-parametric 1-way ANOVA Mann Whitney U test (Prism 4.0, GraphicPad).
In addition, checking additional time points for each patient would be a reasonable next step to establish if the miRNA profile from CD4+ T lymphocytes is stable and can be used to distinguish HIV-1 infected, MEU and healthy donors. As a first step, we agree that examining miRNA levels extracted from total CD4+ T cells is a logical and practical place to start but as we start to understand the nuances of miRNA expression levels in T cell subsets, the future would suggest that more information will be gained by studying miRNA signatures within individual T cell subsets.
Authorship
N.S. and S.S. contributed equally to this letter.
Acknowledgments: This study was funded from the following sources: the Australian Government Department of Health and Ageing; the National Health and Medical Research (NHMRC) via a Program grant (510448), a PhD Scholarship (S.S.) and a Practitioner Fellowship (A.D.K.). The views expressed in this publication do not necessarily represent the position of the Australian Government.
Contribution: S.S., N.S., and A.D.K. wrote the letter; and C.P. and N.S. performed the experiments and analyzed the data.
Conflict-of-interest disclosure: The authors declare no competing financial interests.
Correspondence: Nabila Seddiki, The Vaccine Research Institute (VRI), Paris-Est Créteil University (UPEC), U955 Eq16, 8 rue du General Sarrail, Creteil 94 010, France; e-mail: nabila.seddiki@inserm.fr.
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