Affiliation:
1. Division of Immunology and Allergy, Department of Medicine, Centre Hospitalier Universitaire Vaudois, Lausanne, Switzerland
Abstract
ABSTRACT
To monitor antigen-specific CD4
+
T cells during a recall immune response to tetanus toxoid (TT), a sequential analysis including ex vivo phenotyping and cytokine flow cytometry, followed by cloning and T-cell-receptor (TCR) spectratyping of cytokine-positive CD4
+
T cells, was performed. Grossly, twice as many TT-specific CD4
+
T-cell clones, ex vivo derived from the CCR7
+/−
CD69
+
interleukin-2-positive (IL-2
+
) CD4
+
subsets, belonged to the central memory (T
CM
; CD62L
+
CD27
+
CCR7
+
) compared to the effector memory population (T
EM
; CD62L
−
CD27
−
CCR7
−
). After the boost, a predominant expansion of the T
CM
population was observed with more limited variations of the T
EM
population. TCR beta-chain-variable region (BV) spectratyping and sequencing confirmed a large concordance between most frequently expressed BV TCR-CDR3 from ex vivo-sorted CCR7
+/−
CD69
+
IL-2
+
CD4
+
subsets and BV usage of in vitro-derived TT-specific CD4
+
T-cell clones, further demonstrating the highly polyclonal but stable character of the specific recall response to TT. Taken together, ex vivo flow cytometry analysis focused on the CCR7
+/−
CD69
+
IL-2
+
CD4
+
subsets appears to target the bulk of antigen-specific T cells and to reach an analytical power sufficient to adequately delineate in field trials the profile of the antigen-specific response to vaccine.
Publisher
American Society for Microbiology
Subject
Microbiology (medical),Clinical Biochemistry,Immunology,Immunology and Allergy
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