CD4⁺CD25^High Treg cells in HIV/HTLV Co-infected patients with neuropathy: high expression of Alpha4 integrin and lower expression of Foxp3 transcription factor

The results presented herein, phenotypically characterizing Tregs in HIV/HTLV co-infected patients, indicate an impairment of Treg cells in co-infected individuals presenting neurological symptoms. We first observed that the frequency of CD4 T cells with high expression of CD25 was eight-fold higher in HIV/HTLV Neur group than in the mono-infected group. Our data are in keeping with a previous report showing increased frequency of CD4⁺CD25⁺ cells in HIV/HTLV co-infected individuals compared to HIV mono-infected and controls [4]. This effect may be mediated by the Tax encoded by HTLV-1, since this protein is a strong activator of host genes that regulate cell growth, including the gene encoding IL-2 and the alpha chain of its receptor, CD25 [15].

Although we did not find a significant change in Treg counts between the control and the HIV Neur group, it has been described that HIV-1 infected patients receiving ART present higher frequencies of Treg cells, possibly associated with increase in thymic production and export of these lymphocytes [16]. Such divergent results may be due to differences among the cohorts, since in our study we enrolled individuals with neurological dysfunction and CD4 T cell counts less than 350 cells/μL. When analyzing data from the co-infected group, we observed significantly higher absolute and relative Treg cell counts. Our results corroborate previous evidence revealing that HTLV-1 infection leads to an increase in the frequency of Treg cells [17]. It is likely that these changes are due to the spontaneous lymphoproliferation mediated by the Tax protein encoded by HTLV-1. We cannot, however, rule out that the higher frequency of these cells in HIV/HTLV Neur group is merely the consequence of relocation or recruitment of Treg cells from other organs to the circulation. Irrespective of the underlying mechanism, this higher proportion of Treg cells in HIV/HTLV-1 co-infection could favor the modulation of antiviral response.

It has been described that the suppressive function of Treg is associated with the density of Foxp3 expression [18‐20]. On the other hand, the Foxp3 density differs between effector and regulatory cells [19, 20]. We observed a mild Foxp3 MFI decrease in HIV/HTLV Neur patients as compared to the control group. Yet, these levels did not differ from those observed for the CD4⁺CD25^low effector cells in the control and HIV Neur groups. It is thus possible that in the HIV/HTLV Neur group, cells with the Treg phenotype have impaired function. Reports of Tregs with lower levels of Foxp3 and defective function have been described in HTLV-1 mono-infected patients with HAM/TSP [11, 12]. It has also been shown that reduced levels of Foxp3 in HAM/TSP were correlated with high proviral load and high expression of the Tax-1 protein of HTLV-1 [11].

Under physiologic conditions, higher levels of Tregs will proportionally decrease the frequency of activated T cells. A study conducted in pregnant women found an inverse correlation between Tregs and activated CD4⁺HLA-DR⁺CD38⁺ cells in HIV uninfected but not in HIV infected women [21]. We also found an inverse correlation between the frequencies of activated CD4⁺HLA-DR⁺ cells and Tregs in the control group. Similar to a previous report [4], we found an elevated frequency of CD4⁺HLA-DR⁺ cells in HIV/HTLV Neur patients, which positively correlated with frequencies of Treg cells in the co-infected group, but not in mono-infected individuals. A study conducted in ART naïve HIV infected patients revealed a positive correlation between the frequency of Tregs and CD4⁺HLA-DR⁺CD38⁺ cells in fast progressors but not in slow progressors [9]. Taken together, our results suggest that in HIV infection the rate of CD4 T cell activation is not balanced by Tregs. This unbalance is more evident when the HTLV co-infection is present. Our findings corroborate the notion that the presence of HTLV may favor fast progression to AIDS [4].

Cells with the Treg phenotype expressing the α4 integrin chain (CD49d) of VLA-4 and LPAM-1 may function as pro-inflammatory effector cells that secrete IFN-γ or IL-17 [5]. The removal of such lymphocytes from the pool of regulatory T cells was described as being associated with the induction of a strong suppressive activity [5]. In our study, we found that HIV/HTLV Neur patients presented not only higher frequency of Treg cells bearing the CD4⁺CD25^HighFoxp3⁺CD49d⁺ phenotype, but also showed higher CD49d density. Although we have not evaluated the secretion of inflammatory cytokines by these cells, our data suggest that co-infection by HTLV-1 is associated with higher frequency of CD4⁺CD25^HighFoxp3⁺, broadly defined as potentially inflammatory Treg cells. However further experiments to assess the functionality of these CD4⁺CD25^HighFoxp3⁺ by expression of inflammatory cytokines as IFN-γ and IL-17 need to be conducted to better understand the role of these cells with Treg phenotype. From a standpoint of migratory capacity, the high density of α4 integrin suggests that these cells may migrate efficiently to inflamed CNS by interaction of VLA-4/VCAM and/or to the gut, the primary site of HIV replication, using a mechanism dependent of LPAM-1/MAdCAM interaction.

Infection with HTLV-1 per se, enhances expression of the integrin VLA-4 in lymphocytes [22, 23]. Thus, the higher CD49d levels indicate that these cells are preferentially infected with HTLV-1 [24]. CD4⁺CD25^HighFoxp3⁺ cells with potential to migrate to CNS may also be HIV reservoirs [25] and release HIV-1 neurotoxic proteins in the CNS. It has been demonstrated that the HIV-1 Nef protein released into the extracellular environment induces neuron death [25, 26]. Accordingly, it is plausible to conceive that co-infection may act as a co-factor for inducing CNS pathology mediated by either HTLV-1 or HIV-1.