Evidence for rapid disappearance of initially expanded HIV-specific CD8<sup>+</sup>T cell clones during primary HIV infection

Pantaleo, Giuseppe; Soudeyns, Hugo; Demarest, James F.; Vaccarezza, Mauro; Graziosi, Cecilia; Paolucci, Stefania; Daucher, Marybeth; Cohen, Oren J.; Denis, François; Biddison, William E.; Sékaly, Rafick Pierre; Fauci, Anthony S.

doi:10.1073/pnas.94.18.9848

Cited by 186 publications

(123 citation statements)

References 53 publications

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“…For example, the production of T cells is reduced in untreated patients, as is the life span of the T cells (30,31), yet, with antiviral treatment, the generation of precursor cells increased again and exceeded the normal rate, while the t 1/2 of T cells remained strongly reduced (32,33). After treatment, there is an initial increase in the numbers of memory T cells, and only later do frequencies of T cells with a naive phenotype return to approximately the normal range, at which time CD8 cell numbers fall (34,35). Moreover, the frequency of recall Ag-specific memory T cells in the blood may change if they are redistributed between the extralymphoid compartments and the recirculating pool, as has been postulated; additionally, depletion/exhaustion and regeneration may contribute to the overall T cell repertoire in ways that are still debated (36,37).…”

Section: Discussionmentioning

confidence: 99%

“…Most of these studies came to the conclusion that T cell reactivity declines with the progression of HIV infection, but they left open the questions of how T cell function correlates with virus load and whether this loss of function is a result of decreased frequencies or decreased cytokine output, i.e., whether it is a function of T cell exhaustion, the dilution of these cells by virus-specific CD8 cells, or their suppressed state. Although many of these changes seem to be reversible after HAART therapy (34,35), the extent to which specific immune reactivity is restored remains unclear. All 22 patients that we studied were undergoing this therapy, so it was important for us to establish how the reactivity of individual T cells to recall Ags in these patients compares with that of healthy individuals.…”

Section: Discussionmentioning

confidence: 99%

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Direct Visualization of Cytokine-Producing Recall Antigen-Specific CD4 Memory T Cells in Healthy Individuals and HIV Patients

Helms

Boehm

Asaad

et al. 2000

The Journal of Immunology

122

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We have used computer-assisted cytokine ELISA spot analysis to measure the frequencies, the type of cytokine, and the amount of cytokine produced by individual recall Ag-specific CD4 memory cells in freshly isolated blood. We studied the memory cells specific for tetanus toxoid and purified protein derivative in 18 healthy individuals and in 22 HIV-infected patients on highly active antiretroviral therapy (HAART). In healthy individuals, the frequency, cytokine signature, and cytokine production per cell of these memory cells were stable over time. Although it is presently unclear whether the maintenance of the memory T cell pool depends upon Ag persistence, cross-reactive Ag stimulation, or cytokine-driven bystander stimulations and expansions, our data strongly argue for a stable memory cell pool in healthy individuals. In HIV patients, however, the frequency of these memory cells was a function of the viral load. The decreased numbers of functional memory cells in patients with high viral loads might provide one mechanism behind the immunodeficient state. Although the cytokine output per cell was unaffected in most patients (20 of 24), in some patients (4 of 24) it was >100-fold reduced, which might provide an additional mechanism to account for the reduced immunocompetence of these patients. The ability to visualize directly and quantify the cytokine produced by the low frequency memory cells in freshly isolated blood that have been physiologically stimulated by Ag should aid comprehensive studies of the Ag-specific memory cell pool in vivo, in health and disease.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Direct Visualization of Cytokine-Producing Recall Antigen-Specific CD4 Memory T Cells in Healthy Individuals and HIV Patients

Helms

Boehm

Asaad

et al. 2000

The Journal of Immunology

122

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“…During highly replicative chronic viral infections such as HIV-1, hepatitis B or hepatitis C virus infection in humans, or lymphocytic choriomeningitis virus (LCMV) in mice, virus-specific CD8 + T cells initially expand and acquire effector functions early after infection but then gradually lose these functions [1][2][3][4][5][6][7][8] in a hier-archical manner: first the ability to produce IL-2 and to proliferate, then TNF-α secretion and last IFN-γ production become impaired [9][10][11][12]. This T-cell dysfunction, also termed CD8 + T-cell exhaustion, is well studied after infection of mice with a high dose of LCMV clone 13 or LCMV-Docile [13].…”

Section: Introductionmentioning

confidence: 99%

Antigen amount dictates CD8⁺T‐cell exhaustion during chronic viral infection irrespective of the type of antigen presenting cell

2012

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Chronic viral infections lead to CD8 + T-cell exhaustion, characterized by impaired cytokine secretion and loss of proliferative capacity. While viral load and T-cell dysfunction correlate, it is currently unclear whether the quality of a cell type presenting antigen determines the degree of T-cell exhaustion or if the overall amount of antigen recognized by T cells promotes exhaustion. We found that chronic lymphocytic choriomeningitis virus infection led to decreased CD8 + T-cell exhaustion in DC-MHC class I (MHCI) mice, in which CD8 IntroductionDuring highly replicative chronic viral infections such as HIV-1, hepatitis B or hepatitis C virus infection in humans, or lymphocytic choriomeningitis virus (LCMV) in mice, virus-specific CD8 + T cells initially expand and acquire effector functions early after infection but then gradually lose these functions [1][2][3][4][5][6][7][8] in a hierCorrespondence: Prof. Annette Oxenius e-mail: oxenius@micro.biol.ethz.ch archical manner: first the ability to produce IL-2 and to proliferate, then TNF-α secretion and last IFN-γ production become impaired [9][10][11][12]. This T-cell dysfunction, also termed CD8 + T-cell exhaustion, is well studied after infection of mice with a high dose of LCMV clone 13 or LCMV-Docile [13]. Infection of mice with a low dose of the same virus strains results in an acute resolved infection [13].Besides a role for immunoregulatory cytokines such as 15], , a role for inhibitory receptor expression (reviewed in [18]) and perhaps regulatory T cells [19] C 2012 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim www.eji-journal.eu Eur. J. Immunol. 2012. 42: 2290-2304 HIGHLIGHTS 2291as well as the availability of T-cell help [10,20] and , the overall duration and amount of antigen exposure seems to be a critical parameter driving CD8 + T-cell exhaustion. Recent work has highlighted a negative correlation between viral load and CTL function in chronically infected humans and mice [24][25][26][27]. Even though these studies indicate that high overall antigen levels correlate with T-cell exhaustion, it was never directly shown whether alterations of antigen levels can substantially influence T-cell function independently of the cell type presenting the antigen in vivo. Furthermore, as T-cell exhaustion and viral persistence mutually depend on each other and since alterations in one of the parameters affects the other one, it is often difficult to assign causal relationships, particularly in humans.Here, we made use of Tg(CD11c-β2m) × Tg(K14-β2m) × β2m −/− (DC-MHCI, where DC is defined as dendritic cell; MHCI is defined as MHC class I) mice to assess the role of antigen presenting cells versus antigen load in induction of CD8 + T-cell exhaustion upon chronic LCMV infection. DC-MHCI mice are β2m −/− mice that transgenically express β2m in DCs, keratinocytes, and thymic cortical epithelial cells, ensuring positive selection of CD8 + T cells in the thymus [28]. Thus, DC-MHCI mice can mount normal endogenous CD8 + T-cell responses, but peripheral CD8 + T cells can o...

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“…PBMC were cryopreserved in RPMI 1640 media with 10% FBS and 7.5% DMSO at Ϫ140°C. Standard 51 Cr release assays were performed as previously described (27 51 Cr labeled, washed, and plated at 1 ϫ 10 4 cells per well into 96-well round-bottom tissue culture plates. Fresh or cryopreserved PBMC were used as effectors.…”

Section: Cytotoxic T Cell Assaysmentioning

confidence: 99%

Maintenance of Large Numbers of Virus-Specific CD8+ T Cells in HIV-Infected Progressors and Long-Term Nonprogressors

Gea-Banacloche

Migueles

Martino

et al. 2000

The Journal of Immunology

247

192

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The virus-specific CD8+ T cell responses of 21 HIV-infected patients were studied including a unique cohort of long-term nonprogressors with low levels of plasma viral RNA and strong proliferative responses to HIV Ags. HIV-specific CD8+ T cell responses were studied by a combination of standard cytotoxic T cell (CTL) assays, MHC tetramers, and TCR repertoire analysis. The frequencies of CD8+ T cells specific to the majority of HIV gene products were measured by flow cytometric detection of intracellular IFN-γ in response to HIV-vaccinia recombinant-infected autologous B cells. Very high frequencies (0.8–18.0%) of circulating CD8+ T cells were found to be HIV specific. High frequencies of HIV-specific CD8+ T cells were not limited to long-tern nonprogressors with restriction of plasma virus. No correlation was found between the frequency of HIV-specific CD8+ T cells and levels of plasma viremia. In each case, the vast majority of cells (up to 17.2%) responded to gag-pol. Repertoire analysis showed these large numbers of Ag-specific cells were scattered throughout the repertoire and in the majority of cases not contained within large monoclonal expansions. These data demonstrate that high numbers of HIV-specific CD8+ T cells exist even in patients with high-level viremia and progressive disease. Further, they suggest that other qualitative parameters of the CD8+ T cell response may differentiate some patients with very low levels of plasma virus and nonprogressive disease.

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Evidence for rapid disappearance of initially expanded HIV-specific CD8⁺T cell clones during primary HIV infection

Cited by 186 publications

References 53 publications

Direct Visualization of Cytokine-Producing Recall Antigen-Specific CD4 Memory T Cells in Healthy Individuals and HIV Patients

Direct Visualization of Cytokine-Producing Recall Antigen-Specific CD4 Memory T Cells in Healthy Individuals and HIV Patients

Antigen amount dictates CD8⁺T‐cell exhaustion during chronic viral infection irrespective of the type of antigen presenting cell

Maintenance of Large Numbers of Virus-Specific CD8+ T Cells in HIV-Infected Progressors and Long-Term Nonprogressors

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Evidence for rapid disappearance of initially expanded HIV-specific CD8+T cell clones during primary HIV infection

Cited by 186 publications

References 53 publications

Direct Visualization of Cytokine-Producing Recall Antigen-Specific CD4 Memory T Cells in Healthy Individuals and HIV Patients

Direct Visualization of Cytokine-Producing Recall Antigen-Specific CD4 Memory T Cells in Healthy Individuals and HIV Patients

Antigen amount dictates CD8+T‐cell exhaustion during chronic viral infection irrespective of the type of antigen presenting cell

Maintenance of Large Numbers of Virus-Specific CD8+ T Cells in HIV-Infected Progressors and Long-Term Nonprogressors

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Evidence for rapid disappearance of initially expanded HIV-specific CD8⁺T cell clones during primary HIV infection

Antigen amount dictates CD8⁺T‐cell exhaustion during chronic viral infection irrespective of the type of antigen presenting cell