Early proliferation of CCR5+ CD38+++ antigen-specific CD4+ Th1 effector cells during primary HIV-1 infection

doi:10.1182/blood-2005-01-0206

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Blood, 1 September 2005, Vol. 106, No. 5, pp. 1660-1667.
Prepublished online as a Blood First Edition Paper on May 19, 2005; DOI 10.1182/blood-2005-01-0206.

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IMMUNOBIOLOGY
Early proliferation of CCR5⁺ CD38⁺⁺⁺ antigen-specific CD4⁺ Th1 effector cells during primary HIV-1 infection
John J. Zaunders, Mee Ling Munier, Daniel E. Kaufmann, Susanna Ip, Pat Grey, Don Smith, Tim Ramacciotti, Dick Quan, Robert Finlayson, John Kaldor, Eric S. Rosenberg, Bruce D. Walker, David A. Cooper, Anthony D. Kelleher, on behalf of the PHAEDRA Study Team
From the Centre for Immunology, St. Vincent's Hospital, Sydney, New South Wales, Australia; Partners AIDS Research Center, Massachusetts General Hospital, Boston, MA; National Centre in HIV Epidemiology and Clinical Research, University of New South Wales, Sydney, Australia; Holdsworth House General Practice, Sydney, New South Wales, Australia; and Taylor Square Private Clinic, Sydney, New South Wales, Australia.

   Abstract

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
Appendix
References

We investigated whether HIV-1 antigen-specific CD4⁺ T cellsexpressed the viral coreceptor CCR5 during primary HIV-1 infection(PHI). In the peripheral blood of subjects with very early PHI(< 22 days after onset of symptoms), there was a 10- to 20-foldincrease in the proportion of highly activated (CD38⁺⁺⁺) andproliferating (Ki-67⁺) CD4⁺ T cells that expressed CCR5⁺, andwere mostly T-cell intracellular antigen-1 (TIA-1)⁺ perforin⁺granzyme B⁺. Inthe same patient samples, CD4⁺ T cells producinginterferon (IFN)– ${gamma}$ in response to HIV group-specific antigen(Gag) peptides were readily detected (median, 0.58%) by intracellularcytokine assay—these cells were again predominantly CD38⁺⁺⁺,Ki-67⁺, and TIA-⁺⁺, as well as Bcl-2^low. On average, 20% ofthe Gag-specific CD4⁺ T cells also expressed interleukin-2 (IL-2)and were CD127 (IL-7R)⁺. Taken together, these results suggestthat Gag-specific T-helper 1 (Th1) effector cells express CCR5during the primary response and may include precursors of long-termself-renewing memory cells. However, in PHI subjects with laterpresentation, antigen-specific CD4⁺ T cells could not be readilydetected (median, 0.08%), coinciding with a 5-fold lower levelof the CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells. These results suggest thatthe antiviral response to HIV-1 infection includes highly activatedCCR5⁺CD4⁺ cytotoxic effector cells, which are susceptible toboth apoptosis and cytopathic infection with HIV-1, and rapidlydecline.

   Introduction

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
Appendix
References

Antigen-specific memory CD4⁺ T cells are not often found inuntreated chronic HIV-1 infection, using the standard in vitroproliferation assay.¹ It remains unknown whether the scarcityof proliferative HIV-specific CD4⁺ T cells is due to dysfunction,^2,3inappropriate apoptosis,⁴ or is a result of cytopathic infectionof these cells.⁵ This deficit of antigen-specific CD4⁺ T cellsmay represent a major impediment to immune control of HIV-1infection. In most, but not all, animal models of adaptive immuneresponses to viral infection, optimal clearance of virus dependson synergistic interactions between antigen-specific populationsof helper CD4⁺ T cells, antibody-producing B cells, and cytotoxicCD8⁺ T cells.^6,7 In particular, it is believed that effectiveCD8⁺ T-cell function in HIV-1 infection is reliant on CD4⁺ T-cellfunction.⁸
Previous studies of primary immune responses to viral infectionin mice have shown that antigen-specific T-helper 1 (Th1) CD4responses can be readily detected in the early stages of theinfection, but rapidly decline as antigen is cleared.^9,10 Similarly,human CD4⁺ T-cell immune responses to primary herpesvirus infectionsexhibit a peak response in the first few weeks,^11,12 with markedlyreduced responses at follow-up. These results suggest that antigen-specificCD4⁺ T cells should be generated at a relatively high levelduring primary HIV-1 infection.
Interferon (IFN)– ${gamma}$ producing antigen-specific CD4⁺ T cellshave been demonstrated in primary HIV-1 infection, despite highlevels of viremia.^13-17 Furthermore, proliferative responseswere maintained if antiretroviral therapy was instituted duringacute HIV-1 infection.^13,14,18 Further evidence for the presenceof antigen-specific CD4 T cells is the production of high-affinity,isotype-switched antibodies to HIV-1, which presumably requiresthe provision of help for B-cell responses by CXCR5⁺ CD4⁺ follicularhelper T cells.^19,20
Although CD4⁺ T cells that proliferate in vitro in responseto HIV-1 antigens are mostly absent in untreated chronicallyinfected subjects, an average of approximately 0.1% of peripheralblood CD4⁺ T cells capable of producing IFN- ${gamma}$ can be detectedin most HIV-infected individuals by enzyme-linked immunospot(ELISPOT) assay or by intracellular cytokine assay.^21,22 Itis an absence of those HIV-specific CD4⁺ T cells that synthesizeIL-2^23-27 that probably causes the proliferative defect in viremicpatients.^26,28 However, IL-2–producing CD4⁺ memory cellstypically belong to the CCR7⁺, CCR5^– central memory subset,²⁹and therefore are not directly susceptible to infection by CCR5-tropicHIV-1 strains in early infection. Furthermore, 2 recent studiesof HIV-specific IFN- ${gamma}$ –producing CD4⁺ T cells during primaryHIV-1 infection (PHI) has shown that the vast majority wereCCR7^– cells which did not produce IL-2.^16,30 In the latterstudy, IL-2–producing antigen-specific CD4⁺ T cells werereadily detected in control subjects with Epstein-Barr virus(EBV) or herpes simplex virus (HSV) infections.³⁰
A possible explanation may come from studies of murine models,which suggest that resting memory CD4⁺ T cells arise directlyfrom effector cells.^31,32 Theoretically, then, IL-2–producingHIV-specific memory cells may be derived from Th1 effector cells,which reportedly express CCR5.³³ We have previously found thatapproximately 50%, on average, of CD4⁺ T cells proliferatingin vivo during primary HIV-1 infection express CCR5.³⁴ If theproliferating CD4⁺ T cells included antigen-specific effectorcells, then it is likely that many of these activated effectorcells were CCR5⁺. Recently we confirmed the existence of CCR5⁺antigen-specific CD4⁺ T cells in a HIV⁺ long-term nonprogressorinfected with an attenuated strain of HIV-1.³⁵ These CCR5⁺ cellsproduced IL-2 and proliferated strongly in response to HIV-1p24. Furthermore, these cells were also cytotoxic T lymphocytes(CTLs), similar to cloned CD4⁺ T cells from patients treatedearly in acute HIV-1 infection³⁶ and consistent with our previousfinding that perforin⁺ CD4⁺ T cells were elevated in HIV-1 infection.³⁷A similar population of cytomegalovirus (CMV)–specificCCR5⁺ cytotoxic CD4⁺ T cells was also found in healthy adults,at surprisingly high frequencies.³⁵
We hypothesized that there would be CCR5⁺ antigen-specific CD4⁺T cells produced at the earliest stages of primary HIV-1 infection.We first examined the phenotype of activated, proliferatingeffector CD4⁺ T cells in PHI, and then used the flow cytometricintracellular cytokine assay to determine the cell surface phenotypeof antigen-specific CD4⁺ T cells, which subsequently allowedus to further define these cells in samples of fresh whole blood.

   Patients, materials, and methods

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
Appendix
References

Patients
A total of 33 patients, diagnosed with primary HIV-1 infection,³⁴and who then enrolled in the PHAEDRA observational cohort, wereincluded in this study. All patients were males whose risk groupwas sex with males. Symptoms associated with primary HIV-1 infectionwere recorded as previously described.³⁸
Patients were subdivided into 2 groups, early PHI (n = 19) andlate PHI (n = 14), based on serology at presentation and clinicalhistory of onset of symptoms (Table 1). A Western blot intensityscore (Ramacciotti T, Cunningham P, Grey P, et al, manuscriptin preparation) was calculated as the sum of each band, multipliedby its intensity on a scale of 1+ to 3+ (for example, a subjectwith no bands will have a score of 0, while a subject with 3bands of 1+ intensity and 1 band of 2+ intensity will have ascore of 5). Early PHI was defined as having a Western blotintensity score of 5 or less, and in our subject group, thiscorresponded to presentation within 22 days following onsetof symptoms. Late PHI was defined as an intensity score greaterthan 5, and all these subjects in our cohort had a score of12 or higher, and presented 28 days or more since onset of symptoms.Two subjects in the late PHI group did not record any symptomsof PHI, and therefore the midpoint between their last negativeand first positive HIV antibody tests was used as an estimateof infection date.

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Table 1.. Demographics of primary HIV-1 infection (PHI) patients

One subject, no. 9400101, was originally diagnosed with earlyPHI, but was concurrently diagnosed with primary CMV infection,exhibiting a new CMV immunoglobulin M (IgM)⁺ reactivity, togetherwith detectable CMV viral load, 1 week after PHI diagnosis.Therefore, this individual was excluded from the cohort analyses,and was considered separately. CMV serology was performed byroutine diagnostic assay (Vidas; BioMerieux, Marcy-l'Etoile,France).
Healthy HIV-negative university and hospital staff members wererecruited as controls for this study. The PHAEDRA study wasapproved by the local institutional ethics committee, and allsubjects gave informed consent.
Cell-surface phenotyping of peripheral blood CD4⁺ T cells
Staining of T lymphocyte subsets in fresh peripheral blood and6-color flow cytometric analysis on a dual-laser LSR II flowcytometer (Becton Dickinson, San Jose, CA), was performed aspreviously described.³⁵ Monoclonal antibodies used were CD3–peridininchlorophyll protein (PerCP)–Cy5.5, CD4-phycoerythrin (PE)–Cy7,CD8-allophycocyanin (APC)–Cy7, CD11a–fluorosceinisothiocyanate (FITC), CD27-FITC, CD28-PE, CD38-APC, CD38-PE,and CD38-FITC, human leukocyte antigen (HLA)–DR–FITC,CD57-FITC, CD62L-FITC, CD95-PE, CD154 (CD40L)–PE, andIL-2R ${alpha}$ (CD25)–PE and IL-2R ${alpha}$ -FITC (from Becton Dickinson);CXCR4-PE, CCR5-APC, CCR5-PE, and CCR5-FITC, CCR7-PE, CD45RA-APC,CD45RO-FITC, tumor necrosis factor receptor 2 (TNFR2) (CD120b)–PE,Ki-67–FITC, Bcl-2–PE and Bcl-2–FITC, IL-12R ${beta}$ 1–PE,perforin-FITC, and granzyme A–FITC (Pharmingen, San Diego,CA); TIA-1/GMP-17–PE, IL-2R ${beta}$ (CD122)–PE, and IL-7R(CD127)–PE (Beckman Coulter, Hialeah, FL); IL-18R–PE(R&D Systems, Minneapolis, MN); and granzyme B–APC(Caltag, Burlingame, CA).
For CCR5 analysis, whole blood was processed an average of 1.75hours after venepuncture, to minimize spontaneous loss of thismarker, as previously described.³⁵ Intracellular staining wasperformed using FACSlyse and FACSPermeabilizing Reagents (BectonDickinson) according to the manufacturer's directions, and analyzedas previously described.³⁴
Intracellular cytokine assay
A subset of 14 consecutive patients (7 early PHI and 7 latePHI) were studied for the presence of HIV group-specific antigen(Gag)–specific CD4⁺ T cells using a whole-blood intracellularcytokine (ICC) assay³⁵ using 6-color flow cytometry. OverlappingHIV-1 Gag 15-mer peptides, from the sequence of strain HXB2,were obtained from the NIH AIDS reference reagents program.Gag peptides were used as a pool of 122 peptides, at an individualconcentration of 2 µg/mL each. For analysis, 300 000 eventswere collected, T lymphocytes were first gated on CD3-PerCP-Cy5.5versus side scatter, then on CD4-PE-Cy7⁺/CD8-APC-Cy7^–cells, and finally IFN- ${gamma}$ –APC⁺ cells were analyzed for thevarious FITC and PE antibodies. This method has a validatedcut-off for positive results of 0.08% of CD4⁺ T cells, basedon background results plus 3 times the standard deviation, fromstudy of 16 HIV^– controls (Munier M, Ip S, Zaunders J,et al, manuscript in preparation).
Statistics
Lymphocyte phenotyping results were expressed as a percentageof CD4⁺ T lymphocytes. Results for each cohort were expressedas medians and interquartile ranges. The Mann-Whitney U testwas performed to compare early and late subgroups of primaryHIV-1 infection patients with each other and with the HIV^–controls, using Statview v5.0 for Macintosh (Abacus Concepts,Berkeley, CA). A 2-sided P value less than .05 was consideredstatistically significant. The relationship between differentphenotypes was determined by Spearman rank correlation (Statview).Graphs of longitudinal data were plotted with Lowess curve-fitting,with tension set to 66% (Statview).

   Results

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
Appendix
References

Changes in CD4⁺ T-cell subsets during early PHI
Several subsets of CD4⁺ T cells were present only as very minorsubsets in HIV^– controls, but were found to be prominentin patients with early PHI. In particular, CCR5⁺CD38⁺⁺⁺ CD4⁺T cells (Figure 1A) were highly elevated during early PHI, comparedwith late PHI and healthy adult controls (medians: 5.3% vs 1.0%vs 0.3% of CD4⁺ T cells, respectively; Figure 1E).
CCR5⁺TIA⁺Ki-67⁺ (Figure 1B) and perforin⁺granzyme B⁺ (Figure 1C)CD4⁺ T cells were also elevated during early PHI, comparedwith late PHI and healthy controls (3.6% vs 1.0% vs 0.2% and11.6% vs 5.% vs 1.6%, respectively; Figure 1E).
Similarly, there was an elevation in CD127 (IL-7R)^– CD57^–(Figure 1D) CD4⁺ T cells during early PHI, compared with latePHI and healthy controls (medians: 13.7% vs 6.9% vs 5.2%, respectively;Figure 1E). These CD127^– CD4⁺ T cells were also CD45RA^–(not shown).

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Figure 1.. Changes in cell-surface phenotypes of CD4⁺ T cells during primary HIV-1 infection. Flow cytometry histograms, gated on CD3⁺CD4⁺ T cells, show increases in (A) CCR5⁺CD38⁺⁺⁺; (B) CCR5⁺TIA-1⁺Ki-67⁺; (C) perforin⁺granzyme B⁺; and (D) CD127^– CD57^– T cells from representative early PHI patients and HIV^– controls. Subpopulations in quadrants are shown as percentages of CD3⁺CD4⁺ (A, C, D) or CD3⁺CD4⁺Ki-67⁺ (B) cells. Results from all patients and controls are summarized in panel E. Box plots show 10th, 25th, median, 75th, and 90th percentiles for each marker for each cohort.

All the subset changes in early PHI were statistically significantwhen compared with healthy adult controls (P < .001), andalso when compared with late PHI (P < .01). Differences betweenlate PHI patients and HIV^– controls were also statisticallysignificant (P < .01; except for CD127(IL-7R)^– CD57^–CD4⁺ T cells, P = .05).
Intracellular cytokine assay of HIV-1 Gag-specific CD4⁺ T cells during PHI
In 6 out of 7 subjects studied during early PHI, Gag-specificCD4⁺ T cells were detected by IFN- ${gamma}$ production in the ICC assay,ranging from 0.3% to 1.6% of CD4⁺ T cells. Furthermore, HIV-1Gag-specific IFN- ${gamma}$ ⁺ CD4⁺ T cells were consistently CD38⁺⁺⁺ andBcl-2^dim (Figure 2A), mostly Ki-67⁺ and TIA-1/GMP-17⁺ (Figure 2B),CD40L⁺ (Figure 2C) and CD57^– (Figure 2D). A small,but consistent, proportion of IFN- ${gamma}$ ⁺ Gag-specific CD4⁺ T cellsalso produced IL-2 (Figure 2C) and expressed cell-surface CD127(Figure 2D).
Gag-specific IFN- ${gamma}$ ⁺ CD4⁺ T cells were found in only 1 patientwith late PHI and were too low to obtain reliable phenotypedata (not shown).
In contrast, CMV-specific IFN- ${gamma}$ ⁺ CD4⁺ T cells in 5 of the sameearly PHI individuals who were also CMV IgG seropositive, atthe same time points, were predominantly CD38^low and Bcl-2^high(Figure 3A), Ki-67^– (Figure 3B), and CD57⁺ (Figure 3C).CMV-specific CD4⁺ T cells were similar to Gag-specific CD4⁺T cells in their expression of TIA-1/GMP-17 (Figure 3B), CD127(Figure 3C), CD40L, and IL-2 (not shown). The phenotyping resultsfor HIV-specific and CMV-specific CD4⁺ T cells from all earlyPHI subjects studied are summarized in Figure 3D and E, respectively.
Of interest, patient no. 90400101, undergoing concurrent primaryHIV-1 and CMV infections, had 4.0% CMV-specific CD4⁺ T cellswhich were phenotypically very similar to his HIV-specific CD4⁺T cells, being CD38⁺⁺⁺ and Bcl-2^dim, CD57^–, Ki-67⁺, TIA-1/GMP-17⁺,and CD40L⁺ (data not shown).
In subjects with late PHI and in HIV^– adults (who wereCMV seropositive), CMV-specific IFN- ${gamma}$ ⁺ CD4⁺ T cells were alsoCD38^low and Bcl-2^high, Ki-67^– and CD57⁺, TIA-1/GMP-17⁺,and CD40L⁺ (summarized in Figure 3E). However, in HIV^–adult controls, there was an increased proportion of CMV-specificIFN- ${gamma}$ ⁺ CD4⁺ T cells which produced IL-2 and were CD127⁺ and CD57^–compared with both early (P < .01) and late PHI subjects(P < .02; Figure 3E). It is important to note that the lowexpression of CD38 and Ki-67 by CMV-specific CD4⁺ T cells suggeststhat their expression is not acutely up-regulated by the 6 hoursexposure to antigen in vitro.
Close relationship of circulating CCR5⁺, CD38⁺⁺⁺, and Gag-specific CD4⁺ T cells
When we compared the CD38⁺⁺⁺ phenotype of Gag-specific CD4⁺T cells, obtained from the ICC assays (Figure 2A), with thecoexpression of CCR5 on CD38⁺⁺⁺ CD4⁺ T cells in whole bloodsamples from the same patients at the same time points (Figure 1A),the results infer that antigen-specific CD4⁺ T cells wereCCR5⁺ immediately ex vivo. Direct examination of CCR5 expressionin the ICC assay was precluded by down-regulation of CCR5 bothspontaneously and in response to antigen.³⁵
Overall, Gag-specific CD4⁺ T cells detected by IFN- ${gamma}$ production,in subjects studied during early PHI, represented a median of0.58% of CD4⁺ T cells, whereas subjects with late PHI had asignificantly lower median, 0.08% (P < .01; Figure 4A), veryclose to the detection limit of the ICC. Again, this is consistentwith the relative levels of CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells in these2 subject subgroups (Figure 1E).
Moreover, we observed a very close correlation between the proportionof CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells and the proportion of IFN- ${gamma}$ ⁺ Gag-specificCD4⁺ T cells (rho = 0.76; P = .004; Figure 4B). The resultsshow, however, that the proportion of Gag-specific CD4⁺ T cellsconsistently represented only one-tenth of the proportion ofCCR5⁺CD38⁺⁺⁺ CD4⁺ T cells (Figure 4B).

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Figure 2.. Intracellular cytokine responses to HIV-1 Gag peptide pool. Flow cytometry histograms, gated on CD3⁺CD4⁺CD8^– T cells, show the phenotype of IFN- ${gamma}$ ⁺ cells: (A) Bcl-2 and CD38; (B) Ki-67 and TIA-1; (C) IL-2 and CD154 (CD40L); and (D) CD127 (IL-7R) and CD57. Subpopulations in quadrants are shown as percentages of CD3⁺CD4⁺CD8^– cells. Histograms are representative of 6 different subjects, all showing similar results.

Patient no. 90400101, who was undergoing both primary HIV-1and CMV infection, had 55% of CD4⁺ T cells with a CCR5⁺CD38⁺⁺⁺phenotype, and had 1.1% HIV-specific and 4.0% CMV-specific CD4⁺T cells. Therefore, in this individual, the combined proportionsof HIV- and CMV-specific CD4⁺ T cells were also close to one-tenthof the CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells. The much larger primary CD4⁺T cell response to CMV, compared with the response to HIV-1Gag, has previously been reported in 4 similarly coinfectedpatients.¹⁶
In this cross-sectional study of PHI patients at presentation,the level of CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells peaked within the first22 days following onset of symptoms, and appeared to declinerapidly after that time (Figure 4C). A similar peak was alsoobserved when plotted against Western blot (WB) intensity score(not shown). The level of CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells was highlyvariable and not all early PHI subjects exhibited a large populationof CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells. Nearly all of the early PHI patientsin the current study commenced treatment, so it has not beenpossible so far to conclusively define the natural history ofthe CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells in individual patients.
The level of CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells appeared to have a complexrelationship with viral load, but there was an association betweenthe 2 variables (rho = 0.63; P = .003; Figure 4D).

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Figure 3.. Intracellular cytokine responses to CMV lysate and comparison with responses to HIV-1 Gag peptide pool. Flow cytometry histograms, gated on CD3⁺CD4⁺CD8^– T cells, show the phenotype of IFN- ${gamma}$ ⁺ cells: (A) Bcl-2 and CD38; (B) Ki-67 and TIA-1; and (C) CD127 (IL-7R) and CD57. Subpopulations in quadrants are shown as percentages of CD3⁺CD4⁺CD8^– cells. Histograms shown are representative of results from 6 different subjects, all showing similar results. Results from all patients and controls are summarized in panels D-E. Bars represent means ± SE for each group of patients.

Further phenotyping of CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells in fresh whole blood
We investigated the expression of trafficking markers, adhesionmolecules, costimulatory molecules, and cytokine receptors onthe CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells in samples of fresh whole blood,from 4 subjects with early PHI. Representative results are shownin Figure 5.
The CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells exhibited relative up-regulationof the chemokine receptor CXCR3 and the cytokine receptor IL-12R ${beta}$ 1(Figure 5A), consistent with the phenotype of IFN- ${gamma}$ and IL-2producing Th1 CD4⁺ T cells.³³
The CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells slightly up-regulated CD122 (Figure 5B)and CD132 (not shown) but not CD25 (not shown), representingIL-2R ${beta}$ -, ${gamma}$ -, and ${alpha}$ -chains, respectively. Expression of TNFR2 (CD120b)was also increased (Figure 5B).
The cell-surface expression of IL-7R (CD127) was mostly down-regulated,although one-third of cells retained this receptor (Figure 5C).Also, there was a consistently observed minority of CCR5⁺CD38⁺⁺⁺that coexpressed CCR7 (Figure 5C), but these cells had completelydown-regulated CD45RA (not shown). These cells also maintainedexpression of CD62L (not shown) and had increased expressionof CD49d, integrin ${beta}$ 7, and LFA-1 (not shown), relative to otherCD4⁺ T cells.
The CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells also maintained expression ofthe costimulation molecules, CD28 and CD27 (not shown).

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Figure 4.. Relationship of Gag-specific CD4⁺ T cells to time since infection, subset changes, and viral load. (A) Comparison of levels of Gag-specific CD4⁺ T cells in early (;N=7) versus late (;N=7) PHI subjects. Box plots show 10th, 25th, median, 75th, and 90th percentiles for each cohort. (B) Plot of CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells in all PHI patients versus time since onset of symptoms. The regression line is a Lowess curve. (C) Correlation of Gag-specific CD4⁺ T cells with proportion of CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells in all PHI patients. Dotted horizontal line indicates zero on the y-axis. (D) Plot of CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells in all PHI patients versus plasma HIV-1 RNA viral load. The linear regression curve is shown.

   Discussion

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
Appendix
References

The current study of the phenotype of HIV-specific CD4⁺ T cells,in fresh whole-blood samples obtained during primary HIV-1 infection,demonstrated that these cells were highly activated CD38⁺⁺⁺cells. Parallel analysis of the same blood samples showed thatthe CD38⁺⁺⁺ CD4⁺ T cells coexpressed the HIV-1 coreceptor, CCR5.Together, these results establish that circulating HIV-1 antigen-specificCD4⁺ T cells were CCR5⁺ during primary HIV-1 infection. Expressionof CCR5 on these highly activated antigen-specific CD4⁺ T cellssuggests that they are likely to be particularly susceptibleto HIV-1 infection, and possibly lost as a result of eitherdirect cytopathic effect by HIV-1, or lysis by CD8⁺ CTLs.
Consistent with this possibility, our cross-sectional studyof patients at presentation found that there was an apparentrapid decline in antigen-specific CD4 T cells over time, asdefined both functionally (by ICC assay) and phenotypically(CCR5⁺CD38⁺⁺⁺). In order to establish whether loss of antigen-specificCD4⁺ T cells is due to HIV-1 infection, it will be importantto confirm the kinetics in more detailed longitudinal studiesof individual subjects. It will also be necessary to performcell sorting of CD38⁺⁺⁺ CD4⁺ T cells during early primary infectionand determine whether they preferentially contain HIV-1 DNA.Previous studies of CD4⁺ T cell subsets containing HIV-1 DNAhave shown relatively increased infection of antigen-specificCD4⁺ T cells⁵ but the cell surface expression of CCR5 in thatanalysis was not examined.
In the present study, HIV-1 Gag-specific CD4⁺ T cells were alsopredominantly Ki-67⁺, indicating proliferative expansion. Ithas been shown during acute simian immunodeficiency virus (SIV)infection that Ki-67⁺ CD4⁺ T cells in lymphoid tissue increasedramatically about 10 days following inoculation, and are themain producers of SIV during acute infection,³⁹ although againin that study, expression of CCR5 was not reported. Our resultswould suggest that proliferation of antigen-specific CD4⁺ Tcells contributes to an increase in target cells in lymphoidtissue. However, cell-cell transmission of SIV to adjacent Ki-67^–cells in lymphoid tissue was also observed during acute infection,³⁹suggesting that highly productively infected Ki-67⁺ CD4⁺ T cellsmay act as a focus of spreading infection.

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Figure 5.. Cell-surface expression of chemokine and cytokine receptors on CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells. (A) Expression of IL-12R ${beta}$ 1 and CXCR3 on CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells (top row) versus expression on all other CD4⁺ T cells (bottom row). (B) Expression of IL-2R ${beta}$ (CD122) and TNFR2 (CD120b) on CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells (top row) versus expression on all other CD4⁺ T cells (bottom row). (C) Expression of CCR7 and IL-7R (CD127) on CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells (top row) versus expression on all other CD4⁺ T cells (bottom row). Subpopulations in regions are shown as percentages of CCR5⁺CD38⁺⁺CD4⁺ cells (top row) or of CD4⁺ cells (bottom row). Histograms shown are representative of results from at least 3 different subjects, all showing similar results.

An important question is whether all the observed CCR5⁺ CD38⁺⁺⁺CD4⁺ T cells were HIV specific. Our findings agree with earlierdescriptions of CD38⁺, Ki-67⁺ CMV- and EBV-specific CD4⁺ T cellsduring primary infection with these respective viruses.^11,12In the present study, 1 early PHI patient concurrently underwentprimary CMV infection and had high levels of both CMV- and HIV-specificCD4⁺ T cells that were similarly CCR5⁺CD38⁺⁺⁺ and Ki-67⁺. Conversely,in the other PHI patients (without evidence of primary CMV infection),our results showed that "bystander" CMV-specific effector memoryCD4⁺ T cells, at the same time points, were neither activated,nor proliferating. It should be noted, however, that a largefraction of these resting CMV-specific memory CD4⁺ T cells wereCD57⁺ and did not produce IL-2, suggesting that they were terminallydifferentiated effector cells, which previous in vitro studieswould predict were unlikely to proliferate.⁴⁰
There are several possible reasons why the level of HIV-specificCD4⁺ T cells measured in our assay may not match the level ofCD38⁺⁺⁺ CD4⁺ T cells in the blood samples, even if these cellswere largely antigen specific. We have not completely investigatedthe extent of CD4⁺ T-cell responses to all HIV-1 proteins. Moststudies do suggest that CD4⁺ T-cell responses to HIV-1 Gag arehighly immunodominant,¹ particularly in patients during acuteinfection¹⁶ as well as patients treated during acute infectionwho underwent treatment interruption.^41,42 However, glycoprotein(gp) 160–specific CD4⁺ T-cell responses were also commonlyfound in very early PHI in 1 report.⁴¹ Additional responsesmight also be detected to variant autologous sequences,⁴³ toframe-shifted peptides,⁴⁴ or to peptides from recombinant variants,⁴⁵but these were not tested in the present study. Moreover, theremay be a sublineage of antigen-specific Th1 effector cells whichdo not express IFN- ${gamma}$ , and may be precursors of memory cells.⁴⁶It has also been reported that major histocompatibility complex(MHC) class I tetramer⁺ HIV antigen-specific CD8⁺ T cells donot uniformly produce IFN- ${gamma}$ in response to their cognate antigenduring periods of high viremia following treatment interruptions.⁴⁷
Increased activation of CD4⁺ T cells is prominent in PHI⁴⁸ andthis activation is dramatically reduced following initiationof antiretroviral therapy.^34,49 Increased expression of CD38on T cells, particularly on CD8⁺ T cells, is highly correlatedwith disease progression during chronic HIV-1 infection.⁵⁰ ElevatedCD38 expression has also been reported on HIV-specific CD8⁺T cells during acute HIV-1, although at the same time it wasobserved that CMV- and EBV-specific CD8⁺ T cells similarly expressedrelatively high levels of CD38.^51,52 Therefore the questionof whether elevated activation is limited to HIV-specific Tcells remains unclear, but overall the present results indicatethat CD38 up-regulation on CD4⁺ T cells, early in infection,is related to antigen-specific activation. It will also be importantto determine whether CCR5 expression is coupled to elevatedCD38 expression throughout HIV-1 infection.
However, HIV-1 infection of CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells is probablynot the main reason why these cells decline in the circulationas the primary infection resolves. Studies in murine modelshave shown that CD4⁺ T cell responses to viral infection showa peak response in the range of 0.5% to 10% of CD4⁺ T cells,followed by a decrease of 10- to 20-fold.^9,10
Also, a similar peak and rapid decline in CMV-specific CD4⁺T cells has been observed in primary CMV infection.¹¹ Possibleexplanations for such a normal decline in viral antigen-specificCD4⁺ T cells include apoptosis and trafficking. Firstly, wehave now directly shown that the antigen-specific CD38⁺⁺⁺ CD4⁺T cells also contained decreased levels of Bcl-2. We had previouslyshown that CCR5⁺ and CD38⁺ T cells during acute HIV-1 infectioncontained low levels of Bcl-2 and spontaneously underwent apoptosisin vitro,⁵³ but these cells could be rescued from apoptosisby incubation with IL-15 or IL-2, which increased intracellularlevels of Bcl-2.⁵³ Th1 effector cells are particularly susceptibleto apoptosis,⁵⁴ and interestingly, the products of these cells,including IL-2, IFN- ${gamma}$ , and perforin, have all been shown to beinvolved in feedback regulation of T-cell responses in vivo.^55-58Comparison of primary HIV-1 infection with acute EBV infection,where we have also shown an elevation of CD38⁺⁺ CD4⁺ T cells,as well as proliferating CCR5⁺ CD4⁺ T cells with low Bcl-2 andincreased spontaneous apoptosis,^34,53 may allow study of a normalcontraction of these CD4⁺ effector cells.
Another possible reason for the observed decline of CCR5⁺CD38⁺⁺⁺CD4+ T cells may be trafficking out of the circulation to sitesof inflammation, consistent with the cell-surface phenotypeof CXCR3⁺ and CCR5⁺,⁵⁹ as well as high expression of LFA-1 andCD62L.⁶⁰ Antiviral CD8⁺ effector T cells proliferate in lymphnodes and the spleen, exit into the circulation, and then approximatelyhalf of these cells traffic to organs such as the bone marrow,lung, liver, and gut (reviewed in Masopust and Lefrancois⁶¹).In particular, it is believed that CCR5⁺ CD4⁺ T cells in gut-associatedlymphoid tissue represent a main target of HIV-1 in acute infection.^62,63We found that the majority of CCR5⁺ CD38⁺⁺⁺ CD4⁺ T cells expressedthe gut-homing marker, integrin ${alpha}$ 4 ${beta}$ 7. Interestingly, a previousstudy showed that there was a selective loss of the integrin ${alpha}$ 4 ${beta}$ 7⁺ subset of CCR5⁺ CD4⁺ T cells from the circulation duringacute HIV-1 infection.⁶⁴
However, the apparent decline in antigen-specific T cells mayalternatively simply reflect anergy of these cells, resultingin an inability to detect them by functional assays in vitro.Exhaustion of antigen-specific CD4⁺ T cells has been observedin persistent viral infections in mice.⁶⁵ Similarly, exposureto persistent antigen in vivo led to a dramatic reduction incytokine production by recently proliferated CD4⁺ T cells ina mouse model of anergy.⁶⁶ It is important to note that a histologicfeature of acute HIV-1infection is the accumulation of largenumbers of virions retained by the follicular dendritic cellnetwork within lymphoid tissue.⁶⁷ Constant exposure to HIV-1antigens, therefore, may prevent the transition to resting memorycells, or induce exhaustion. One study has already demonstratedthat CD4⁺ T cells specific for HIV-1 envelope, which had beenpresent at a detectable level during primary HIV-1 infection,only persisted at a greatly reduced, functionally undetectablelevel following resolution of the acute phase of infection⁴¹and required prolonged incubation in vitro in IL-2 containingmedium for detection.
Finally, it is possible that the antigen-specific CD4⁺ T cellsswitch to production of alternative cytokines not measured inthe current study, such as IL-10, rather than IFN- ${gamma}$ .⁶⁸ A morecomprehensive analysis of cytokines and effector molecules producedby the Gag-specific CD4⁺ T cells in PHI is now feasible andwarranted. Similarly, development of CD25⁺ suppressor cells⁶⁹may occur after resolution of the primary infection, blockingin vitro responsiveness and studies of the effect of depletionof such CD25+ CD4+ T cells may be informative.
Approximately half of the activated, proliferating CD4⁺ T cellsalso expressed markers of cytotoxic T lymphocytes, includingTIA-1/GMP-17/NKG-7, as well as granzyme B and perforin. Theresults of the current study are in agreement with previousfindings that immune responses to HIV-1 and CMV include CD4⁺T cells with a CTL phenotype and function.^35-37,70 These consistentfindings suggest that the normal role of CD4⁺ T cells is notjust to help B cells and CD8⁺ T cells, but also indicates adirect antiviral effect. It had been reported that MHC classII⁺ cells in vivo can present endogenously produced viral antigenicpeptides to CD4⁺ T cells⁷¹ and a recent paper has now shownthat CD4⁺ CTLs specifically clear viral peptide-loaded targetcells in vivo.⁷²
Most CCR5⁺CD38⁺⁺⁺ CD4⁺ T cells exhibited an up-regulation ofthe IL-2R ${beta}$ chain, but not the IL-2R ${alpha}$ chain, consistent with arole for IL-15 in survival of these cells.⁷³ We also found anup-regulation of the IL-12R ${beta}$ 1 chain on these cells, at leastduring the acute phase. Previous studies have shown that incubationwith IL-15^74,75 or IL-12⁷⁶ increased antigen-specific responsesin vitro. The presence of these receptors is consistent withthe ability of IL-15 to induce CCR5 expression on resting Tcells⁷⁷ and IL-12 to regulate CCR5 expression following T-cellactivation.⁷⁸ We also found an up-regulation of the TNFR2 onthe CCR5⁺ CD38⁺⁺⁺ CD4⁺ T cells, which may contribute to apoptosisin combination with low Bcl-2,⁷⁹ but may also be involved inenhancement of HIV-1 replication.⁸⁰
Studies of effector CD4⁺ cells in murine models suggest thatas viral antigen is cleared, a subset of effector cells willconvert to resting memory cells.^31,32 In particular, those antigen-specificCD4⁺ T cells which retain expression of the IL-7R are precursorsof memory cells.⁸¹ In our earlier study,³⁵ IL-7R^– CD38⁺⁺T cells from subjects during primary HIV-1 infection underwentspontaneous apoptosis in vitro, but we did not study whetherthere was a subset of activated T cells which retained IL-7Rand could be induced to become resting memory cells by incubationin vitro with IL-7, as suggested in the murine studies.⁸¹
We had also previously studied the T-cell receptor variablebeta chain (TCRVB) repertoire of Ki-67⁺, CD38⁺⁺, and CCR5⁺ CD4⁺T cells and found that it was surprisingly broad.⁵³ Taken togetherwith the current results, it is likely that many clones areinvolved in the initial antigen-specific response to HIV. Patientstreated during acute infection have the broadest responses toHIV proteins,⁴² which also suggests a broad base of responsesduring acute infection.
Our results showing expression of CCR5 on activated CD4⁺ T cellsmay help to explain the effects of immunosuppressive treatmentwith hydroxyurea⁸² and cyclosporine A⁸³ in acute HIV-1 infection.The presence of CCR5 on antigen-specific CD4⁺ T cells predictsthat blockade of this receptor will be particularly beneficial,not only during acute infection, but possibly also during therapeuticimmunization or treatment interruptions. It will also be importantto confirm that expression of IL-7R is an early marker of long-termself-renewing memory cells, and may represent a useful guideto vaccine efficacy.

   Appendix

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
Appendix
References

Members of the PHAEDRA Study Team are P. Grey, J. Kaldor, D.A. Cooper, T. Ramacciotti, K. Petoumenos, D. Smith, M. Bloch,N. Medland, R. Finlayson, A. McFarlane, N. J. Roth, C. Workman,A. Carr, A. D. Kelleher, J. Zaunders, and P. Cunningham.

   Acknowledgements

The authors would like to thank the patients and their physiciansfor their participation, Kate McGhie, Ciara McGinley, and PalaneeAmmaranond for help with specimen organization and logistics,and the NIH Reference Reagents Program for provision of HIV-1overlapping Gag peptides.

   Footnotes

Submitted January 18, 2005; accepted April 22, 2005.
Prepublished online as Blood First Edition Paper, May 19, 2005;DOI 10.1182/blood-2005-01-0206.

Supported by the Commonwealth Department of Health and Ageingthrough the Australian National Council on AIDS, Hepatitis Cand Related Diseases (The National Centre in HIV Epidemiologyand Clinical Research). This project was funded by an AIEDRPgrant through the National Institutes of Health Division ofAIDS, and a program grant from the Australian National Healthand Medical Research Council.

A complete list of members of the Primary HIV and Early DiseaseResearch: Australian Cohort (PHAEDRA) Study Team appears inthe "Appendix."

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

Reprints: John Zaunders, Centre for Immunology, St Vincent's Hospital, Victoria St, Darlinghurst, NSW 2010 Australia; e-mail: j.zaunders{at}cfi.unsw.edu.au.

   References

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
Appendix
References

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