Reduced cellular susceptibility to in vitro HIV infection is associated with CD4+ T cell quiescence.

BACKGROUND: HIV preferentially establishes productive infection in activated CD4+ T cells. Since proportions of activated CD4+ T cells vary between individuals, this study aimed to determine if individuals with a greater proportion of activated CD4+ T cells would be more susceptible to in vitro HIV infection. METHODOLOGY/PRINCIPAL
FINDINGS: Unstimulated peripheral blood mononuclear cells (PBMC) from various donors were inoculated with HIV(ML1956)in vitro. HIV replication was evaluated by HIV p24 ELISA of culture supernatants and intracellular staining for HIV p24, which was detected by flow cytometry. Baseline T cell phenotypes and infected cell phenotypes were also evaluated by flow cytometry. Ex vivo phenotyping at the time of blood draw showed that elevated T cell activation and reduced Tregs were associated with increased cellular susceptibility to in vitro infection. Furthermore, the infected CD4+ T cell population was enriched for activated cells. CONCLUSION/SIGNIFICANCE: These data suggest that CD4+ T cell quiescence provides an environment less conducive to the establishment of HIV infection by limiting the pool of activated target cells.

Introduction

Known risks factors for sexual transmission of HIV include high viral loads in the infected partner or concurrent sexually transmitted infections in the uninfected partner. The availability of HIV-susceptible target cells in the uninfected partner may similarly influence the probability of transmission [1]. HIV preferentially establishes productive infection in activated CD4+ T cells due its dependency on host substrates for viral entry and replication [2], [3], [4], [5], [6]. Since individuals vary in their levels of activated CD4+ T cells, we hypothesize that those who have greater numbers of activated target CD4+ T cells may have elevated susceptibility to in vitro HIV infection.

In HIV-infected individuals, T cell activation is considered to be a major driving force in disease progression [7], [8], [9], [10], [11], but the relationship between immune activation and HIV infection susceptibility is not well defined. This issue has recently been explored in observational studies of HIV-exposed seronegative (HESN) individuals who remain uninfected by HIV, despite multiple exposures to the virus. While no single factor accounts for resistance to infection in all cases of HESN, recent studies from the Pumwani cohort point to a role for T cell immune quiescence in protection [12], [13], [14]. T cell immune quiescence refers to a state of low baseline immune activation, which was characterized by reduced frequencies of activated CD69+ CD4+ and CD8+ T cells [12], low levels of gene transcription in CD4+ T cells [13] and whole blood [14] and reduced baseline production of cytokines by CD4+ T cells [13] in HESN. Regulatory T cells (Tregs), which are involved in suppressing immune activation, were shown to be elevated in HESN from the Pumwani cohort, and represent a potential driver of T cell immune quiescence [12]. Evidence for T cell immune quiescence has also been observed in other cohorts. Low frequencies of activated T cells have been identified in HESN men who have sex with men [15], uninfected partners of HIV-infected individuals [16], [17] and HESN CSW [18]. Reduced spontaneous lymphoproliferation has also been observed in HESN compared to healthy control groups [15], [19].

In the present study, we sought to characterize T cell phenotypes before and after in vitro HIV infection and examined the relationship between infection susceptibility and target cell activation. We show that elevated cellular susceptibility to infection is associated with high levels of T cell activation ex vivo and that HIV preferentially targets activated CD4+ T cells.

Results

PBMC from Select Individuals Demonstrate Relative Resistance to HIV Infection in vitro

Unstimulated PBMC from 21 HIV-uninfected study participants from the Pumwani cohort were infected with HIVML1956 at a MOI of 0.1 in six replicate wells. Virus levels were quantified in supernatants collected on day 9 post-inoculation.

The level of viral production varied between individuals. Fourteen of 21 individuals demonstrated productive infection in at least two replicate wells. Five individuals demonstrated productive infection in all six replicate wells and had higher average levels of virus production per well compared to the other participants. At the other end of the spectrum, seven individuals had no detectable p24 levels in any of the replicate wells (Figure 1).

Figure 1

Infection of unstimulated PBMC inoculated with HIVML1956.

Graph shows average level of HIV infection of replicate wells as determined by HIV p24 ELISA. Individual patients are represented by their study ID numbers. The number of replicate wells demonstrating productive infection (out of 6) is indicated below the patient study ID numbers.

Since study subjects were high-risk HIV-uninfected participants enrolled in the Pumwani commercial sex worker cohort, this study population included individuals who are HESN. In this cohort, we have defined an extreme phenotype of HESN, in which individuals are considered HESN if they remained HIV-uninfected for greater than 7 years of follow-up in the Pumwani cohort and were active in sex work during that time. Therefore, the proportion of individuals meeting these criteria for HESN was compared between those individuals with detectable viral replication and those with no detectable viral replication. No difference was detected in the proportion of HESN among individuals who did have detectable levels of viral replication (7/14) and those without detectable levels of viral replication (4/7) (p = 1.0). Age was also not significantly different between groups (p = 0.35).

High Levels of T Cell Activation and Reduced Tregs at Baseline are Associated with Elevated Susceptibility to HIV Infection in vitro

PBMC were phenotyped ex vivo (day 0) to address the roles of baseline T cell activation and Tregs in cellular susceptibility to infection. Baseline T cell phenotypes were compared between the 14 individuals who demonstrated viral replication and the seven individuals with no detectable viral replication (Table 1). Individuals with detectable levels of virus production had significantly higher baseline levels of CD4+ CD69+ T cells (p = 0.028). In addition, a trend was observed in which the presence of infection was associated with a modest reduction in Treg frequency (p = 0.093) (Figure 2).

Table 1

Effect of ex vivo T cell phenotype on susceptibility of unstimulated PBMC to infection with HIVML1956 virus at a MOI of 0.1.

T cell phenotype	No Detectable Virus (n = 7)	Virus Detected (n = 14)	p-valuea
Relative Expressionb
CD4+ CD69+	0.41 (0.24–1.00)	1.45 (0.48–2.31)	0.028
CD4+ CD38+	38.8 (23.8–49.6)	42.3 (34.9–46.2)	0.628
CD4+ HLA DR+	1.56 (0.80–2.32)	1.65 (1.24–2.48)	0.479
CD4+ CD38+/HLA DR+	0.75 (0.28–1.20)	0.73 (0.61–1.24)	0.737
CD4+ CCR5+	0.70 (0.46–1.56)	0.99 (0.63–1.35)	0.628
CD4+ CXCR4+	73.6 (35.2–86.1)	54.0 (40.8–84.0)	0.970
CD8+ CD69+	1.06 (0.53–1.88)	1.91 (0.67–4.59)	0.192
CD8+ CD38+	47.2 (41.1–48.2)	44.9 (43.3–46.8)	0.852
CD8+ HLA DR+	4.90 (2.92–8.60)	4.52 (3.56–5.28)	0.794
CD8+ CD38+/HLA DR+	2.81 (1.58–4.50)	2.44 (1.92–2.74)	0.682
Tregs (CD25+ FOXP3+)	1.07 (1.00–1.43)	0.94 (0.78–1.12)	0.093
Treg/CTLA-4+	23.2 (11.1–26.4)	22.0 (18.9–27.7)	0.682
Estimated number of cellsc
CD4+ CD69+	314.7 (156.5–432.5)	677.6 (311.4–1150)	0.093
CD4+ CD38+	19195 (15565–35354)	24400 (14117–29307)	0.970
CD4+ HLA DR+	804.6 (520.9–1212)	1020 (663.4–1335)	0.737
CD4+ CD38+/HLA DR+	476.1 (182.6–585.1)	476.1 (281.0–688.7)	0.794
CD4+ CCR5+	452.8 (206.1–1195)	482.4 (344.7–881.0)	0.970
CD4+ CXCR4+	47987 (15983–59581)	31633 (18104–51924)	0.576
CD8+ CD69+	210.9 (109.2–332.8)	379.3 (183.3–1013)	0.093
CD8+ CD38+	8514 (7642–12602)	10586 (7726–13124)	0.433
CD8+ HLA DR+	779.6 (499.8–2236)	1139 (798.6–1341)	0.852
CD8+ CD38+/HLA DR+	563.4 (286.6–1160)	615.7 (450.7–743.0)	0.970
Tregs (CD25+ FOXP3+)	740.4 (393.4–972.8)	537.6 (347.2–717.4)	0.109
Treg/CTLA-4+	171.8 (42.66–285.3)	107.0 (62.77–222.3)	0.433

p-values calculated using non-parametric Mann-Whitney U test. Parameters that demonstrated statistically significant (p<0.05) or trending (p<0.10) p-values are highlighted in bold text.

Relative expression of phenotypic markers is listed as median of percent positive (+) cells. Interquartile range is shown in parentheses.

Estimated number of cells was calculated from flow cytometry proportions based on seeding 105 cells per well. Interquartile range is shown in parentheses.

Figure 2

T cell phenotypes of unstimulated PBMC with differential susceptibility to in vitro infection with HIVML1956.

PBMC were immunophenotyped ex vivo to assess T cell activation and Tregs prior to inoculation with HIVML1956 in vitro. PBMC with no detectable infection (n = 7) were compared to those demonstrating productive infection (n = 14) at 9 days post-inoculation. (A) PBMC with undetectable levels of virus production by day 9 post-inoculation had lower frequencies of CD4+ CD69+ T cells. (B) PBMC with undetectable levels of virus production by day 9 post-inoculation had higher frequencies of Tregs (defined as CD25hi FOXP3+), but the difference was not statistically significant. P-values were calculated using the Mann-Whitney U test.

Since comparing proportions of activated cells between groups does not account for differences in the size of CD4+ or CD8+ T cell populations, the estimated number of cells of each phenotype were calculated based on the percentages observed by flow cytometry. These calculated T cell counts were compared between the 14 individuals who demonstrated viral replication and the seven individuals with no detectable viral replication (Table 1). Consistent with the differences in percentages of CD4+ CD69+ T cells between groups, a trend was observed in which individuals with detectable levels of virus production had higher baseline levels of total CD4+ CD69+ T cells (p = 0.093). Although the calculated number of Tregs was lower in individuals with detectable viral replication, this difference was not statistically significant. Also of note, the estimated count of CD8+ CD69+ T cells was higher in individuals demonstrating detectable viral replication, consistent with an activated T cell phenotype in these subjects.

Activated CD4+ T Cells are Enriched in the HIV p24+ Cell Population

When infection cultures were terminated, cells were harvested and stained for intracellular HIV p24 and markers of T cell activation and Tregs (Figure 3A). T cell phenotypes were compared between infected (HIV p24+) and uninfected (HIV p24-) CD4+ T cells from infection cultures (n = 12). A higher proportion of infected cells were CD69+ HLA DR+ (p = 0.005), CD69+ HLA DR- (p = 0.0005) or CD69- HLA DR+ (p = 0.0005) compared to uninfected cells (Figure 3B). In addition to CD69 and HLA DR, expression of CD25 and CD127 was evaluated on infected cells. A greater proportion of infected cells were CD25hi CD127lo compared to uninfected cells (p = 0.0005) (Figure 3B). This is consistent with a Treg phenotype, but these markers may also reflect the phenotype of activated conventional T cells.

Figure 3

Phenotypes of HIV-infected unstimulated CD4+ T cells.

(A) CD4+ T cells were evaluated for infection by intracellular staining for HIV p24. Cells were gated on singlets, lymphocytes and live cells before discriminating CD4+ T cells. Infected (p24+) and uninfected cells (p24-) were phenotyped for markers of Tregs (defined as CD25hi, CD127lo) and T cell activation (CD69, HLA DR). (B) Comparison of T cell phenotypes between infected and uninfected CD4+ T cells (n = 12). Higher frequencies of infected cells were activated (CD69+ HLA DR+, CD69+ HLA DR- or CD69- HLA DR+) or demonstrated a Treg phenotype (CD25hi CD127lo) compared to uninfected cells. P-values were calculated using the Wilcoxon signed-rank test for matched pairs.

Discussion

HIV preferentially establishes productive infection in activated T cells. While it is established that immune activation is a major driving factor in HIV disease progression, its relevance in susceptibility to infection is not well understood. We hypothesized that cells from individuals with high levels of baseline immune activation would be more susceptible to in vitro HIV infection. As such, we assessed the infectability of unstimulated PBMC from 21 HIV-uninfected women and addressed the role of target cell activation on susceptibility to infection.

Of the 21 samples exposed to HIVML1956 at an MOI of 0.1, one third showed no evidence of HIV replication following 9 days of culture. However, lack of detectable viral replication does not imply absolute resistance to infection. The assay used in the present study does not rule out the presence of low levels of viral replication or latent infection.

Baseline T cell phenotypes were analyzed in unstimulated PBMC prior to inoculation with virus, demonstrating that individuals with detectable levels of HIV replication by day 9 post-infection had significantly higher levels of CD4+ CD69+ T cells and a trend toward lower levels of Tregs compared to those with no detectable viral replication by day 9 (Figure 2). This in vitro data supports our previous observation of low CD4+ CD69+ T cells and elevated Tregs in ex vivo PBMC from HESN women compared to susceptible controls [12].

There was no association between in vitro HIV susceptibility and expression of the chronic activation markers HLA DR or CD38 (Table 1). This suggests that increased cellular susceptibility to in vitro infection is largely a consequence of activation at the earliest stages of the cell cycle. Future studies should include additional markers of cell cycle entry such as Ki67 to confirm this observation.

High levels of T cell activation may promote HIV infection by increasing the availability of activated target cells. HIV can enter quiescent CD4+ T cells [20], [21], [22], [23], [24], but the processes of reverse transcription and integration are inefficient and often result in abortive infections [20], [21], [23]. CD69 is expressed early in the cell cycle, indicating that CD69- cells are quiescent, and do not effectively support HIV replication [25], [26]. As such, the association between lack of detectable viral replication on day 9 post-inoculation and reduced baseline frequencies of CD4+ CD69+ T cells supports the hypothesis that T cell immune quiescence can limit infection by reducing the pool of activated HIV target cells. Tregs suppress T cell activation and responses, so elevated levels of Tregs may protect against HIV infection by limiting activation of target CD4+ T cells. Additionally, Tregs can directly suppress HIV infection through a cAMP-dependent mechanism [27], [28]. HIV replication is negatively regulated by cAMP due to inhibition of HIV DNA nuclear import, integration and transcription [29], [30], and blockage of HIV LTR activation by NF-κB [31]. Further studies involving Treg depletion experiments will be needed to ascertain the role of Tregs in modulating susceptibility of unstimulated PBMC to HIV infection in vitro.

To characterize the activation status of cells that did support HIV replication, phenotypes of infected cells were analyzed by flow cytometry. Consistent with the preferential infection of activated CD4+ T cells by HIV, the infected (HIV p24+) CD4+ T cell population contained a significantly higher proportion of activated T cells than the uninfected (HIV p24-) CD4+ T cell population. Tregs were also significantly enriched within the HIV p24+ CD4+ T cell population. However, it should be noted that in the present study, Tregs were defined by expression of high levels of CD25 and low levels of CD127/IL-7Rα, and not by FOXP3, due to complications with co-staining of the intracellular markers p24 and FOXP3. Since activated cells upregulate CD25 and downregulate CD127, the Treg populations evaluated here may not be pure, and potentially represent some activated cells. As discussed above, Tregs suppress immune activation so they may play a beneficial role in preventing infection. However, Tregs can also be infected with HIV [32], [33], [34], suggesting that elevated Tregs may actually provide additional target cells for HIV infection.

To summarize, increased cellular susceptibility to in vitro HIV infection was associated with elevated activated CD4+ T cells and a trend toward reduced Tregs ex vivo. Furthermore, viral production was preferentially established in activated CD4+ T cells. These data are supported by findings in non-human primate models of SIV transmission, in which acute SIV infection is established in resting cells, but viral propagation and dissemination are fuelled by activated target cells present at sites of viral replication [2], [3], [35], [36]. Interestingly, use of the anti-inflammatory compound glycerol monolaurate blunted the inflammatory response and prevented infiltration of activated target cells, and resulted in protection from SIV infection [37].

There are several limitations to this study. First, the study subjects are high-risk HIV-uninfected women from the Pumwani cohort, and a proportion of these individuals are HESN. Lack of virus production was not restricted to HESN, and individuals with detectable levels of productive infection did not differ from those with no detectable productive infection in the proportion of participants who were HESN. However, it is likely that some of these subjects have additional mechanisms of resistance to infection. Future studies should include a low-risk HIV-uninfected control group and evaluate the effect of HESN status on susceptibility to in vitro infection. Second, the limited sensitivity of the HIV p24 ELISA and delayed kinetics of unstimulated infections required prolonged maintenance of cells in culture. Cultures with undetectable infection may have been latently infected or had low levels of viral replication. In addition, changes in the phenotype of the population of cells can be expected to occur over time. As such, future studies should employ more sensitive infection readouts and earlier time points.

The data presented here, along with observational studies in HESN [12], [13], [14], [15], [16], [17], [18], [19] and animal models [2], [3], [35], [36], [37], demonstrate that T cell immune quiescence is associated with resistance to HIV infection. The T cell immune quiescence model suggests that mechanisms of reducing inflammation and target cell activation should be considered during future HIV vaccine and microbicide development.

Materials and Methods

Study Subjects and Ethics Statement

The Research Ethics Boards at the University of Manitoba and Kenyatta National Hospital approved the study protocols. Study subjects were high-risk HIV-uninfected women enrolled in the Pumwani Commercial Sex Worker Cohort based in Nairobi, Kenya. Subjects were considered HESN if they remained HIV-uninfected for greater than 7 years of follow-up in the Pumwani cohort and were active in sex work during that time. Written informed consent was obtained from all study participants.

Virus Strain

The HIV-1 strain that was used for the in vitro infections was HIVML1956, a primary isolate from a HIV-infected participant of the Pumwani cohort. HIVML1956 was originally derived by primary co-culture with PHA-stimulated PBMC [38]. Briefly, PBMC from HIV-uninfected donors were stimulated with PHA for 3 days then co-cultured with PHA-stimulated PBMC from the HIV-infected patient. Co-cultures were maintained in RPMI containing 10% FCS, 1% Penicillin/Streptomycin/Fungizone and 100 IU IL-2, and were supplemented periodically with fresh PHA-stimulated feeder cells. Virus production was monitored in culture supernatant by HIV p24 ELISA. The supernatant was harvested at peak p24 production, and the virus was collected and stored at −135°C for future studies.

Full-length HIV proviral sequencing performed on the HIVML1956 isolate revealed that it is a recombinant of clades A2, C and D, consistent with a high proportion of circulating recombinant viruses in the cohort [39].

Infection of PBMC in vitro

Unstimulated PBMC (105 cells/well in 96 well microplates) from HIV-uninfected women (n = 21) were inoculated with HIVML1956 at a multiplicity of infection (MOI) of 0.1 in six replicate wells. Cells were incubated with virus for 4 hours in a total volume of 200 µl/well. The cells were then washed twice by centrifugation at 1200rpm for 5 minutes, and 150 µl of media was removed from the wells and replaced with fresh media after each wash. Cultures were maintained in RPMI containing 10% FCS, 1% Penicillin/Streptomycin/Fungizone and 10 IU IL-2. On day 3 post-inoculation, 100 µl of supernatant was removed from each well and replaced with 100 µl of fresh media. On days 9 and 16 post-inoculation of unstimulated cells, 100 µl of supernatant was harvested from each well and treated with 10 µl of 10% Triton-X-100 then frozen at −80°C for later HIV p24 determinations. Infection cultures were then terminated and cells were harvested for evaluation of infected cell phenotypes by flow cytometry.

HIV-1 Quantification in Supernatants

HIV p24 was measured in supernatants from infection cultures using a sandwich enzyme-linked immunosorbent assay (ELISA). ELISA plates were coated with anti-HIV p24 monoclonal IgG1 purified from supernatants of HIV-1 p24 hybridoma cells (183-H12-5C, NIH AIDS Research and Reference Reagent Program, Division of AIDS, NIAID, NIH). Frozen supernatants from infection cultures were thawed and 75 µl was transferred to ELISA plates. Detection of HIV p24 in supernatants was done using rabbit polyclonal anti-p24 detection antibody (Advanced Biotechnologies), followed by a biotin anti-rabbit goat IgG secondary antibody (Sigma). Streptavidin horseradish peroxidase (Invitrogen) and tetramethyl benzidine substrate solution (Invitrogen) were used detect binding of the secondary antibody. When plates were developed, 3% HCl was added to each well to stop the reaction. Optical density of wells was read at OD450nm on a SpectraMax Plus spectrophotometer (Molecular Devices). Data were acquired and analyzed using SoftMax Pro software, version 3.1.2 (Molecular Devices). The ELISA detected HIV p24 concentrations ranging from 280 to 0.273 ng/ml.

Flow Cytometry

PBMC were immunophenotyped to assess ex vivo T cell phenotypes at baseline (i.e. prior to infection). To assess T cell activation and HIV coreceptor expression, cells were stained with anti-CD69-FITC, anti-CD38-PECy5, anti-HLADR-APCCy7, anti-CCR5-PE, anti-CXCR4-PECy7, anti-CD4-AlexaFluor700, anti-CD3-Pacific Blue (all BD Biosciences), anti-CD8-PETR (Invitrogen) and Live/Dead Aqua dye (Invitrogen). To evaluate Tregs, cells were stained with anti-CD25-PE, anti-CTLA4-PECy5, anti-CD4-AlexaFluor700, anti-CD3-Pacific Blue (all BD Biosciences), anti-FOXP3-APC (clone PCH101, eBioscience) and Live/Dead Aqua dye (Invitrogen). FOXP3 staining was performed using the FOXP3 Staining Buffer Set (eBioscience). Tregs were defined as CD4+ T cells co-expressing high levels of CD25 and FOXP3. The total number of CD4+ or CD8+ T cells per well was calculated from flow cytometry percentages (i.e. CD4+ or CD8+ T cells as percent of total events) based on seeding 105 cells per well. Estimated number of cells of each phenotype was further calculated using percentages obtained by flow cytometry.

Cells collected from infection cultures were stained with anti-HLADR-PECy5, anti-CD69-APC, anti-CD127-PE, anti-CD25-APCCy7, anti-CD4-AlexaFluor700 (all BD Biosciences), anti-CD3-PETR (Invitrogen), anti-p24-FITC (KC57, Beckman Coulter) and Live/Dead Aqua dye (Invitrogen) to evaluate phenotypes of infected cells. Due to complications of co-staining HIV p24 and FOXP3, Tregs were defined by high expression of CD25 and low expression of CD127 for the analysis of infected cell phenotypes.

Stained samples were acquired on a LSRII flow cytometer (BD Biosciences). Samples were suspended in 250 µl of fixation buffer (BD Biosciences) prior to acquisition. When acquiring data, 50,000–100,000 lymphocyte events were acquired for each sample. Analysis of flow cytometry data was performed using FlowJo software, version 9.3.1 (Tree Star Inc., Ashland, OR).

Statistical Analysis

Comparison of HESN status between groups of individuals was performed using Fisher’s Exact Test. Comparisons of baseline phenotypes between groups of individuals were performed using non-parametric Mann-Whitney U tests. Comparisons of T cell phenotypes between infected and uninfected cells were performed using the Wilcoxon signed-rank test for matched pairs. Differences were considered to be statistically significant at p<0.05. All statistical analyses were performed using GraphPad Prism for Mac OS X, version 5.0a (GraphPad software, La Jolla, CA).