Publikation

Integrin-Alpha IIb Identifies Murine Lymph Node Lymphatic Endothelial Cells Responsive to RANKL

Wissenschaftlicher Artikel/Review - 24.03.2016

Bereiche
PubMed
DOI

Zitation
Cordeiro O, Lanza F, Cupedo T, Ludewig B, Léon C, Yagita H, Rot A, Coles M, Eckly A, Li Z, Bénézech C, Romera-Hernandez M, Alloush F, Rauber S, Brouard N, Chypre M, Mueller C. Integrin-Alpha IIb Identifies Murine Lymph Node Lymphatic Endothelial Cells Responsive to RANKL. PloS one 2016; 11:e0151848.
Art
Wissenschaftlicher Artikel/Review (Englisch)
Zeitschrift
PloS one 2016; 11
Veröffentlichungsdatum
24.03.2016
eISSN (Online)
1932-6203
Seiten
e0151848
Kurzbeschreibung/Zielsetzung

Microenvironment and activation signals likely imprint heterogeneity in the lymphatic endothelial cell (LEC) population. Particularly LECs of secondary lymphoid organs are exposed to different cell types and immune stimuli. However, our understanding of the nature of LEC activation signals and their cell source within the secondary lymphoid organ in the steady state remains incomplete. Here we show that integrin alpha 2b (ITGA2b), known to be carried by platelets, megakaryocytes and hematopoietic progenitors, is expressed by a lymph node subset of LECs, residing in medullary, cortical and subcapsular sinuses. In the subcapsular sinus, the floor but not the ceiling layer expresses the integrin, being excluded from ACKR4+ LECs but overlapping with MAdCAM-1 expression. ITGA2b expression increases in response to immunization, raising the possibility that heterogeneous ITGA2b levels reflect variation in exposure to activation signals. We show that alterations of the level of receptor activator of NF-κB ligand (RANKL), by overexpression, neutralization or deletion from stromal marginal reticular cells, affected the proportion of ITGA2b+ LECs. Lymph node LECs but not peripheral LECs express RANK. In addition, we found that lymphotoxin-β receptor signaling likewise regulated the proportion of ITGA2b+ LECs. These findings demonstrate that stromal reticular cells activate LECs via RANKL and support the action of hematopoietic cell-derived lymphotoxin.