The LTα1β2 then signals via LTβR to drive mesenchymal stromal cells to differentiate into lymphoid tissue organizer cells (LTos),[9] accompanied by the up-regulation of chemokine (e.g. CXCL13, CCL19 and CCL21) and adhesion molecule (e.g. vascular cell adhesion molecule-1, intercellular adhesion molecule-1, mucosal addressin cell adhesion molecule-1)[12] expression in the LN anlagen. Chemokines, as well as the up-regulated expression of RANKL high throughput screening assay and interleukin-7 (IL-7) by LTos,[9, 10] induce the recruitment and survival of further cells to the expanding LN anlagen.[13] The arrival of more LTα1β2-expressing cells, which includes few LTis[14] but after birth is dominated by lymphocytes

(both T and B cells),[15, 16] creates a positive feedback loop Selleckchem LY294002 (Fig. 1), further increasing signalling through the LTβR and

the subsequent expression of LTo-derived factors. Using conditional ablation of the Ltbr gene exclusively in VE-Cadherin+ endothelial stromal cells, Onder et al.[17] recently revealed that the development of multiple peripheral LNs required LT signalling specifically into this LTβR+ stromal compartment. Interestingly, not all LNs required endothelial sensitivity to LTα1β2, as the mesenteric LNs of the intestine were fully intact in these mice, hinting at a requirement for distinct LTβR+ stromal cell populations in the development of anatomically disparate peripheral LNs in vivo. Other homeostatic SLOs develop in a fundamentally similar way to the LN with only minor differences between tissues. For instance in the Peyer’s patches of the small intestine, although ligands of the receptor tyrosine kinase RET acting on a distinct population of CD45+ IL-7Rα− CD11c+ cells contributes to stromal activation in the developing anlagen,[18] LTis and LTα1β2 are still important in this developmental process,[4] although it is not clear if LTα1β2 expression is induced by RANK as in early LN development. However,

the earliest steps in homeostatic intestinal SLO development are still under intense investigation.[19] Lymphoid tissue organizers differentiate into the various non-haematopoietic stromal subtypes present in the adult SLO via LTβR signalling,[20] HSP90 although the ontogeny and lineage relationships of the various stromal cell subsets within the LN is still under investigation.[21, 22] Mesenchyme-derived stromal cells can be divided into several subsets including follicular dendritic cells (FDCs), marginal reticular cells and populations of fibroblastic reticular cells (FRCs). Lymph node stromal endothelial cells can be divided into blood endothelial cells and lymphatic endothelial cells,[23] and all SLOs contain high endothelial venules composed of endothelial cells with distinct morphology and phenotype. Four CD45− stromal subsets can therefore be identified by a dual CD31 (PECAM-1) and Podoplanin (gp38) stain.[23] Identification of further subsets can be achieved using a range of different surface markers (Table 1).