Detection of antigen‐specific T cells by cytokine flow cytometry: the use of whole blood may underestimate frequencies

Hoffmeister, Bodo; Bunde, Torsten; Rudawsky, Ina Maria; Volk, Hans‐Dieter; Kern, Florian

doi:10.1002/eji.200324223

Cited by 36 publications

(25 citation statements)

References 20 publications

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“…However, our results are similar to those of Dunn et al, who similarly stimulated whole blood with CMV peptide pool and lysate (2). It is possible that use of whole blood may underestimate the frequency of CMV specific T cells as recently reported by Hoffmeister et al (27), although others have not observed significant quantitative differences in CMV-responses using these two types of specimens (28). The frequencies of CD8 + T cell IFNγ responses may also be lower in the present study due to the stringency in the cutoffs used.…”

Section: Discussionsupporting

confidence: 92%

CMV Antigen-Specific CD4+ and CD8+ T Cell IFNγ Expression and Proliferation Responses in Healthy CMV-Seropositive Individuals

Sinclair¹,

Black²,

Epling³

et al. 2004

Viral Immunol

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CMV-specific CD4 + and CD8 + T cell IFNγ expression and proliferation were measured in healthy volunteers by flow cytometry after CMV lysate or CMV pp65 or IE peptide pool stimulation. Cutoff values were set to maximize specificity (i.e., no false positive CMV-seronegatives). Sensitivity (defined as a positive response in CMV-seropositives to at least one of the 3 antigen preparations used) was 100% for CMV-specific CD4 + and CD8 + T cell IFNγ expression and CD4 + T cell proliferation and 95.4% for CMV-specific CD8 + T cell proliferation. All 22 CMV-seropositive individuals had positive responses by at least three of these four measurements. These findings support the concept that a multiplicity of antigen-specific functional immune responses and persistence of robust virus-specific CD4 + T cells are important components of protective immunity in this chronic viral infection.

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Section: Discussionsupporting

confidence: 92%

CMV Antigen-Specific CD4+ and CD8+ T Cell IFNγ Expression and Proliferation Responses in Healthy CMV-Seropositive Individuals

Sinclair¹,

Black²,

Epling³

et al. 2004

Viral Immunol

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“…Undiluted whole blood consistently yielded higher T cell frequencies than purified PBMCs [42]. However, a more recent study [26] also using similar stimuli and the same T cell readout (intracellular IFN-g staining) reached the opposite conclusion: responses were consistently higher in PBMCs than in whole blood, occurred at lower concentrations of stimulant and were sometimes detected only on PBMCs [26]. In conclusion, further studies are needed to settle the question of the sensitivity of whole blood versus PBMC assays, and how red blood cell lysis affects T cell recovery and function.…”

Section: Use Of Whole Blood Versus Pbmcsmentioning

confidence: 90%

“…However, when whole blood assays were performed in parallel, lithium heparin yielded slightly higher CMV-specific responses [26]. Hence, we recommend using heparin as anticoagulant for T cell assays (level of evidence: C).…”

Section: Anti-coagulantsmentioning

confidence: 99%

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Isolation and preservation of peripheral blood mononuclear cells for analysis of islet antigen-reactive T cell responses: position statement of the T-Cell Workshop Committee of the Immunology of Diabetes Society

Mallone

Mannering

Brooks-Worrell

et al. 2010

Clinical and Experimental Immunology

215

190

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Summary Autoimmune T cell responses directed against insulin‐producing β cells are central to the pathogenesis of type 1 diabetes (T1D). Detection of such responses is therefore critical to provide novel biomarkers for T1D ‘immune staging’ and to understand the mechanisms underlying the disease. While different T cell assays are being developed for these purposes, it is important to optimize and standardize methods for processing human blood samples for these assays. To this end, we review data relevant to critical parameters in peripheral blood mononuclear cell (PBMC) isolation, (cryo)preservation, distribution and usage for detecting antigen‐specific T cell responses. Based on these data, we propose recommendations on processing blood samples for T cell assays and identify gaps in knowledge that need to be addressed. These recommendations may be relevant not only for the analysis of T cell responses in autoimmune disease, but also in cancer and infectious disease, particularly in the context of clinical trials.

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“…The surprisingly high concentration of IFN-␥ secreted into the extracellular medium in the subgroup of monoclonal TCRV␤13.1 ϩ /CD4 ϩ T-LGL patients in response to a single hCMV peptide complementary to the HLA-DRB1*0701 allele is particularly enlightening; this is particularly true if we consider that the observed response could represent only part of the response actually occurring in vivo because antigen presentation developed in vitro by PB cells could be considerably less efficient as it is limited to circulating cells (dendritic cells and B lymphocytes) that are considered to be precursors of professional antigen-presenting cells 44 and because of the potential interference of plasma proteins with both antigen uptake and HLA loading. 45 Immunologic T-cell responses against viruses and other antigens are typically associated with clonal selection of T cells with restricted antigen specificities. 46 This is particularly evident among CD8 ϩ cytotoxic/ effector T cells 46 ; in turn, CD4 ϩ T cells typically show a broader recognition of peptide epitopes probably the result of the existence of less stringent anchor positions in HLA class II vs HLA class I molecules.…”

Section: Discussionmentioning

confidence: 99%

Expanded cells in monoclonal TCR-αβ+/CD4+/NKa+/CD8−/+dim T-LGL lymphocytosis recognize hCMV antigens

Rodríguez-Caballero

García‐Montero

Bárcena

et al. 2008

Blood

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Detection of antigen‐specific T cells by cytokine flow cytometry: the use of whole blood may underestimate frequencies

Cited by 36 publications

References 20 publications

CMV Antigen-Specific CD4<SUP>+</SUP> and CD8<SUP>+</SUP> T Cell IFNγ Expression and Proliferation Responses in Healthy CMV-Seropositive Individuals

CMV Antigen-Specific CD4<SUP>+</SUP> and CD8<SUP>+</SUP> T Cell IFNγ Expression and Proliferation Responses in Healthy CMV-Seropositive Individuals

Isolation and preservation of peripheral blood mononuclear cells for analysis of islet antigen-reactive T cell responses: position statement of the T-Cell Workshop Committee of the Immunology of Diabetes Society

Expanded cells in monoclonal TCR-αβ+/CD4+/NKa+/CD8−/+dim T-LGL lymphocytosis recognize hCMV antigens

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