T cell receptor–induced phosphoinositide-3-kinase p110δ activity is required for T cell localization to antigenic tissue in mice
Sarah J. Jarmin, … , Klaus Okkenhaug, Federica M. Marelli-Berg
Sarah J. Jarmin, … , Klaus Okkenhaug, Federica M. Marelli-Berg
Published February 7, 2008
Citation Information: J Clin Invest. 2008;118(3):1154-1164. https://doi.org/10.1172/JCI33267.
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Research Article Immunology

T cell receptor–induced phosphoinositide-3-kinase p110δ activity is required for T cell localization to antigenic tissue in mice

Abstract

The establishment of T cell–mediated inflammation requires the migration of primed T lymphocytes from the blood stream and their retention in antigenic sites. While naive T lymphocyte recirculation in the lymph and blood is constitutively regulated and occurs in the absence of inflammation, the recruitment of primed T cells to nonlymphoid tissue and their retention at the site are enhanced by various inflammatory signals, including TCR engagement by antigen-displaying endothelium and resident antigen-presenting cells. In this study, we investigated whether signals downstream of TCR ligation mediated by the phosphoinositide-3-kinase (PI3K) subunit p110δ contributed to the regulation of these events. T lymphocytes from mice expressing catalytically inactive p110δ displayed normal constitutive trafficking and migratory responses to nonspecific stimuli. However, these cells lost susceptibility to TCR-induced migration and failed to localize efficiently to antigenic tissue. Importantly, we showed that antigen-induced T cell trafficking and subsequent inflammation was abrogated by selective pharmacological inhibition of PI3K p110δ activity. These observations suggest that pharmacological targeting of p110δ activity is a viable strategy for the therapy of T cell–mediated pathology.

Authors

Sarah J. Jarmin, Rachel David, Liang Ma, Jan-Guo Chai, Hamlata Dewchand, Aya Takesono, Anne J. Ridley, Klaus Okkenhaug, Federica M. Marelli-Berg

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Figure 5

PI3K p110δ is required for tissue infiltration by antigen-specific T cells.

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PI3K p110δ is required for tissue infiltration by antigen-specific T cel...
Female and male C57BL/6 mice were treated i.p. with 600 U IFN-γ. After 48 hours, 3 × 106 PKH26-labeled WT or p110δD910A HY-specific H2-Ab–restricted CD4+ T cells (107/mouse) were injected i.p. The presence of labeled T cells in the peritoneal membrane and lavage was analyzed after 24 hours by wide-field fluorescence microscopy (A and B) and flow cytometry (C and D), respectively. In addition, the presence of labeled cells in the spleen was quantified by wide-field fluorescence microscopy (E). Original magnification, ×10. Tissue infiltration was quantified by randomly selecting ten ×10-magnified fields and assessing the number of fluorescent cells in each field. The mean values ± SD observed in samples from at least 3 animals are summarized in B and E (infiltration of the peritoneal membrane and spleen, respectively) and D (cells retrieved in the peritoneal lavage). B and D: *P < 0.004 versus p110δD910A; E: *P < 0.02 versus p110δD910A.