Human Immunodeficiency Virus (HIV) infection is characterized by immune dysfunction
that predisposes infected individuals to opportunistic infections such as Mycobacterium
Tuberculosis (MTB). The result of this is an exacerbation of HIV-TB related deaths
annually. Therefore there is an imperative need for HIV-TB focused research that aims to
identify immunological factors that are involved in the control of MTB and HIV in both
mono- and co-infected individuals. The CD161+ CD4+ T cell subset is linked to a distinct
phenotypic and functional profile. Importantly, these CD161+ T cells may act as an
important component of immunological defense and provide protection in infected tissues.
CD161+ CD4+ T cells have also been identified as the precursor population of Th17 cells
and it has been previously reported that reduction of CD161+ CD4+ T cells during HIV
infection may limit Th17 reconstitution (Prendergast et al., 2010). This may ultimately
contribute to impairment of mucosal immunity leading to the acquisition of opportunistic
infections such as MTB and disease progression in HIV infected individuals. Our study
aimed to comprehensively characterise the impact of HIV and MTB infection on the
CD161+ CD4+ T cell subset and to assess the frequency, phenotype and function of these
cells. The study also aimed to correlate the longitudinal variation in frequency, phenotype
and function with markers of HIV disease progression.
Methods
The frequency, phenotype and function of the CD161+ CD4+ T cell subset was measured
by flow cytometry. For the frequency and phenotypic assessment, whole blood was
collected from HIV negative and HIV/MTB mono and co-infected subjects (n = 17 per
patient group). Whole blood was surface stained with antibodies specific to CD3, CD4,
CD8, CD161 and chemokine receptors CD103, CCR6, CXCR4, CCR5 and CXCR6. The
percentage positive expression of CD161 on CD4+ T cells and chemokine receptor
expression was measured. The functional assessment of CD161+ CD4+ T cells involved
PBMC stimulation with antigenic stimulant, phorbol 12-myristate 13-acetate (PMA) and
ionomycin or ESAT-6/CFP-10, GAG, TB10.4 and Ag85a followed by intracellular
cytokine staining for IFN-γ, IL-17A, IL-22 and TNF-α. A subgroup of HIV negative
(frequency and phenotype, n = 10, function n = 7) and HIV mono-infected subjects
(frequency and phenotype, n = 10, function n = 7) were longitudinally followed to assess
variations in the frequency, phenotype and function of CD161+ CD4+ T cells over time.
Results
The CD161+ CD4+ T cell subset demonstrated high-level expression of chemokine
receptors CCR5, CCR6, CXCR4 and low-level expression of CD103 and CXCR6. The
subset also demonstrated the ability to produce cytokines IFN-γ, IL17A, IL-22 and TNF-α
in healthy subjects. Analysis of HIV infected samples revealed a significant reduction in
the frequency of the CD161+ CD4+ subset (median = 06.86%, p < 0.0001) compared to
that of healthy individuals (median = 14.75%). Correlation of the subset frequency to
markers of disease progression revealed a positive trend to CD4 count (r = 0.2590,
p = 0.0787) and a significant negative correlation to viral load (r = -0.3522, p = 0.0152).
Unlike with HIV infection, no significant changes in CD161+ CD4+ T cell frequency was
observed in individuals with LTBI (mono- or HIV co-infected) or active TB disease
compared to that of the healthy patient group. However, the exception to this was HIV
infected individuals with active TB disease (co-infected) (median = 03.80%, p < 0.0001).
Decreased CCR6 expression on CD161+ CD4+ T cells was observed in HIV monoinfected
(p = 0.0065) and HIV infected individuals with active TB disease (p = 0.007). No
functional changes were observed in both the HIV and MTB mono- and co-infected
cohorts following non-specific stimulation. An interesting positive trend in correlation
between IFN-γ production and CD4 count (r = 0.2727, p = 0.0733) was demonstrated with
a significant negative correlation between IFN-γ production and viral load observed
following non-specific antigenic stimulation (r = -0.3705, p = 0.0133). CD161+ CD4+ T
cells demonstrated antigen-specific T cell responses to peptides ESAT-6/CFP-10, TB10.4,
Ag85a and GAG in a small proportion of 69 study participants with variable ranges in
magnitude of the responses observed. The longitudinal assessment of CD161+ CD4+ T
cell frequency and phenotype demonstrated low-level proportion of CD4+ T cells
expressing CD161 and CCR6 expression longitudinally maintained in HIV mono-infected
compared to that of healthy individuals.
Conclusion
The phenotypic and functional profile of the CD161+ CD4+ T cell population indicates
that it may be an important component of immunological defense that may provide
mucosal defense and protection at epithelial sites and tissues e.g. expression of tissue
homing markers like CCR6 and the production of cytokines such as IL-17A and IL-22
(important in mucosal immunity). HIV infection is associated with a reduced frequency of
CD161+ CD4+ T cells. The correlation between CD161+ CD4+ T cell frequency and
markers of disease progression suggests that the observed low-level frequency in HIV
infected individuals may in part be a result of non-specific HIV-mediated depletion of
CD4+ T cells. However, lower levels of CD161+ CD4+ T cells in HIV infected individuals
could also be a result of naturally lower levels being present in individuals prior to
infection, thereby making these individuals more susceptible to HIV infection. The
significantly reduced levels of CCR6 expression on CD161+ CD4+ T cells in HIV monoinfected
individuals may also be an indication of cell subset migration to gut associated
lymphoid tissue (GALT, target site of HIV replication) during HIV infection. Given their
potential role in mediating signals that are essential for immune responses to microbes and
microbial products, migration of CCR6+ CD161+ CD4+ T cells to target sites of HIV
infection could serve as a protective measure in the fight against HIV infection. Although
there were no observable changes in the functional capacity of the CD161+ CD4+ T subset
in HIV infection, we believe that the reduction in frequency may contribute to HIV disease
progression and susceptibility to opportunistic infections such as MTB or active TB
disease. Unlike with HIV infection, infection with MTB appeared to have no significant
impact on CD161+ CD4+ T cells as there were no observable differences in frequency or
the functional capacity of the cell subset following PMA stimulation. However, MTB and
HIV antigen-specific responses were observed in a small proportion of the total 69 subjects
tested. This therefore indicates that a subset of CD161+ CD4+ T cells may act in an HIV
and MTB-specific manner. Additional MTB and HIV-specific responses may be present in
this CD161+ CD4+ population and may only be identified through stimulation with
additional antigenic targets.
Further investigation of CD161+ CD4+ T cells should be performed at the actual sites of
infection to investigate if CD161+ CD4+ T cells are concentrated at sites of disease. Also
it may be important to investigate the polyfunctionality of CD161+ CD4+ T cells to
understand the multifunctional capacity of the cell subset in providing immunological
defense to pathogens such as HIV and MTB. / Thesis (M.Med.)-University of KwaZulu-Natal, Durban, 2012.
Identifer | oai:union.ndltd.org:netd.ac.za/oai:union.ndltd.org:ukzn/oai:http://researchspace.ukzn.ac.za:10413/9642 |
Date | January 2012 |
Creators | Govender, Pamla. |
Contributors | Kasprowicz, Victoria. |
Source Sets | South African National ETD Portal |
Language | en_ZA |
Detected Language | English |
Type | Thesis |
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