RESEARCH
HIGHLIGHTS
HIGHLIGHT ADVISORS
CEZMI AKDIS
SWISS INSTITUTE OF ALLERGYAND ASTHMA RESEARCH,SWITZERLAND
BRUCE BEUTLER
SCRIPPS RESEARCH INSTITUTE,USA
PETER CRESSWELL
YALE UNIVERSITY, USA
JAMES DI SANTO
PASTEUR INSTITUTE, FRANCE
GARY KORETZKY
UNIVERSITY OFPENNSYLVANIA, USA
CHARLES MACKAY
GARVAN INSTITUTE OFMEDICAL RESEARCH,AUSTRALIA
CORNELIS J. M. MELIEF
LEIDEN UNIVERSITY MEDICALCENTRE, THE NETHERLANDS
MICHEL NUSSENZWEIG
THE ROCKEFELLER UNIVERSITY,USA
SARAH ROWLAND-JONES
CENTRE FOR TROPICALMEDICINE, OXFORD, UK
ALAN SHER
NATIONAL INSTITUTE OFALLERGY AND INFECTIOUSDISEASE, USA
ANDREAS STRASSER
THE WALTER AND ELIZA HALLINSTITUTE, AUSTRALIA
MEGAN SYKES
HARVARD MEDICAL SCHOOL,USA
ERIC VIVIER
CENTRE D’IMMUNOLOGIE DEMARSEILLE-LUMINY, FRANCE
MATTHIAS VON HERRATH
LA JOLLA INSTITUTE FORALLERGY AND IMMUNOLOGY,USA.
New research published in TheJournal of Immunology shows thatantigen-presenting cells such asdendritic cells (DCs) are not alwaysrequired to link innate immune sig-nals through Toll-like receptors(TLRs) to adaptive T-cell responses.This study showed that TLR expres-sion by T cells can lead to directeffects of pathogen-associated mole-cular patterns (PAMPs) on adaptiveimmunity.
Stimulation of TLRs on DCsresults in DC maturation andinduces the upregulation of MHCand co-stimulatory molecules andthe production of pro-inflammatorycytokines. The mature DCs in turnpresent antigen to, and stimulate,T cells. However, in this study, acti-vated mouse CD4+ T cells were alsoshown to express TLRs, indicatingthe possibility of a direct effect.Specifically, purified CD4+CD25–
T cells expressed mRNA encodingTLR3 and TLR9 but not TLR2 andTLR4. In the absence of suitablemonoclonal antibodies to detectTLR protein, the mRNA results wereconfirmed by stimulation with theTLR3 ligand poly(I:C) and the TLR9ligand CpG-containing DNA. Theseligands induced nuclear factor-κB(NF-κB) and mitogen-activated pro-tein kinase (MAPK) activation in theactivated T cells, in contrast to theTLR4 ligand lipopolysaccharide.
Having shown that T-cell TLR3and TLR9 are functional in terms ofsignalling, Laurence Turka and col-leagues looked at the downstream
effects. They showed that stimulationwith poly(I:C) or CpG-containingDNA increased the survival of a puri-fied population of activated CD4+
T cells in vitro. The increase in viablecell number occurred without anychange in proliferation. When acti-vated T cells were stimulated withpoly(I:C) or CpG DNA and thenadoptively transferred into congenichosts, survival was also increased in vivo compared with unstimulatedcells, as indicated by an increasedpercentage of transferred T cells inthe host spleen and an increased proliferative response to restimula-tion with the cognate antigen.Therefore, TLR signalling in T cellsmight improve memory responsesby promoting the survival of T cellsafter primary stimulation.
Using specific inhibitors, the T-cellsurvival response mediated by TLRswas shown to depend on NF-κB butnot MAPK activation. Consistent
with previous knowledge of TLR sig-nalling, CpG-DNA-mediated survivalthrough TLR9 depended on theadaptor molecule MyD88, whereaspoly(I:C)-mediated survival throughTLR3 did not. This indicates that bothMyD88-dependent and -independentpathways can activate NF-κB to medi-ate increased survival in T cells. Theend result of these two pathways wasupregulation of expression of theanti-apoptotic molecule BCL-X
L.
The authors speculate that theability of T cells to respond directlyto PAMPs, without using DCs as anintermediary, might be one way inwhich we have evolved to deal withpathogens that try to evade theimmune system by inhibiting DCfunction.
Kirsty Minton
References and linksORIGINAL RESEARCH PAPER Gelman, A. E.,Zhang, J., Choi, Y. & Turka, L. A. Toll-like receptorligands directly promote activated CD4+ T-cellsurvival. J. Immunol. 172, 6065–6073 (2004).
Cutting out the middle man
T- C E L L R E S P O N S E S
488 | JULY 2004 | VOLUME 4 www.nature.com/reviews/immunol
BLAHBLAHBLAHBLAHBLAH!!
BLAHBLAHBLAH!!
Recommended
