The phenotype and survival of antigen-stimulated transgenic CD4 T cells in vivo: the influence of persisting antigen

doi:10.1093/intimm/dxh392

International Immunology Advance Access published online on February 15, 2006
International Immunology, doi:10.1093/intimm/dxh392

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© The Japanese Society for Immunology. 2006. All rights reserved. For permissions, please e-mail: journals.permissions@oxfordjournals.org
Received July 13, 2005
Accepted January 2, 2006

Article

The phenotype and survival of antigen-stimulated transgenic CD4 T cells in vivo: the influence of persisting antigen

C.-P. Yang ¹, S. M. Sparshott ¹, D. Duffy ¹, P. Garside ², and E. B. Bell ¹ ^*

¹ Division of Immunology, Life Sciences Faculty, University of Manchester, UK
² Division of Immunology, Infection and Immunity, University of Glasgow, UK

^* To whom correspondence should be addressed.
E. B. Bell, E-mail: eric.bell{at}manchester.ac.uk

Abstract

Naive and primed/memory CD4 T cells are distinguished by changesin the expression of activation/adhesion molecules that correspondwith an altered function. Adoptively transferred TCR transgenic(tg) CD4 T cells specific for ovalbumin peptide (OVA-pep) wereanalysed for changing phenotype and the speed of change in vivofollowing antigen challenge with alum-precipitated (ap) OVA-pep,a conjugate that stimulated a T_h2-type cytokine response. Thechange of CD45RB in relation to number of divisions showed thatthe transition from CD45RB^hi (naive) to CD45RB^low (primed/memory)was incremental; with each cell cycle the number of CD45RB^himolecules on the cell surface was diluted by approximately halfand replaced by the low-weight isoform. Similarly, the changeto CD44^hi expression increased gradually during four roundsof proliferation. The loss of CD62L expression occurred earlyand was independent of cell division. CD69 was up-regulatedquickly within 1-2 cycles, but down-regulated after about sevendivisions. The expression of CD49d was not altered during theearly rounds of division, although it was up-regulated on 30-60%of tg T cells dividing repeatedly ( $≥$ 8 cycles). When analysedon day 3 following stimulation, CD25 was no longer up-regulated.The intra-peritoneal injection of ap-OVA-pep stimulated tg Tcells in the spleen and mesenteric lymph node one day in advanceof those in more distant peripheral lymph nodes. Evidence indicatedthat residual antigen persisted for at least 4 weeks and wasable to stimulate naive tg T cells. However, residual antigenhad no net effect on extending or reducing survival of the transferredpopulation.

Keywords: CD45R; CD4 T cells; DO11.10; T cell memory.

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