The roles of integrins in function of human neutrophils after their migration through endothelium into interstitial matrix.

We investigated the changes in neutrophil phenotype and function after transendothelial migration, and the roles played by integrin receptors in their behaviour. Neutrophils were tracked microscopically as they migrated through endothelial cells into collagen gels, and were retrieved at desired times. When endothelial cells were treated with increasing doses of tumour necrosis factor-α, neutrophils not only migrated in greater number, but also to a greater depth in the gel. Apoptosis was barely detectable in neutrophils retrieved after 24h, and many remained viable and motile at 48h. Neutrophils retrieved after 1h had increased oxidative capacity and at 24h had similar capacity as freshly-isolated neutrophils. However, by then they had impaired ability to phagocytose bacteria. Compared to fresh neutrophils, total mRNA was halved by 24h, but while ß2-integrin expression decreased, ß1- and ß3-integrin increased along with ICAM-1. Studies of integrin blockade indicated that while ß2-integrins were needed to cross the endothelial barrier, no integrins were required for migration within the gel. ß2-integrins also contributed to phagocytosis, but their binding was not required for prolonged survival. These results demonstrate a model for integrated analysis of neutrophil migration and function, and describe development of effector functions and the roles of integrins in human neutrophils for the first time.

Delay of migrating leukocytes by the basement membrane deposited by endothelial cells in long-term culture.

We investigated the migration of human leukocytes through endothelial cells (EC), and particularly their underlying basement membrane (BM). EC were cultured for 20days on 3µm-pore filters or collagen gels to form a distinct BM, and then treated with tumour necrosis factor-α, interleukin-1ß or interferon-γ. Neutrophil migration through the cytokine-treated EC and BM was delayed for 20-day compared to 4-day cultures. The BM alone obstructed chemotaxis of neutrophils, and if fresh EC were briefly cultured on stripped BM, there was again a hold-up in migration. In studies with lymphocytes and monocytes, we could detect little hold-up of migration for 20-day versus 4-day cultures, in either the filter- or gel-based models. Direct microscopic observations showed that BM also held-up neutrophil migration under conditions of flow. Treatment of upper and/or lower compartments of filters with antibodies against integrins, showed that neutrophil migration through the endothelial monolayer was dependent on ß(2)-integrins, but not ß1- or ß(3)-integrins. Migration from the subendothelial compartment was supported by ß1- and ß(2)-integrins for all cultures, but blockade of ß(3)-integrin only inhibited migration effectively for 20-day cultures. Flow cytometry indicated that there was no net increase in expression of ß1- or ß3-integrins during neutrophil migration, and that their specific subendothelial function was likely dependent on turnover of integrins during migration. These studies show that BM is a distinct barrier to migration of human neutrophils, and that ß(3)-integrins are particularly important in crossing this barrier. The lesser effect of BM on lymphocytes and monocytes supports the concept that crossing the BM is a separate, leukocyte-specific, regulated step in migration.

Responses of endothelial cells from different vessels to inflammatory cytokines and shear stress: evidence for the pliability of endothelial phenotype.

BACKGROUND/AIMS: Local haemodynamic and stromal microenvironments may determine the phenotype of endothelial cells (EC) and regulate their inflammatory responses. METHODS: We compared neutrophil recruitment by EC from human umbilical veins (HUVEC) or arteries (HUAEC) or from human coronary arteries (HCAEC) after 'static' culture or exposure to shear stress (2 Pa for 24 h) and treatment with tumour necrosis factor-alpha (TNF-alpha) or interleukin-1beta (IL-1beta). RESULTS: Static cultures of each type of EC recruited flowing neutrophils efficiently after treatment with TNF-alpha or IL-1beta; differences in culture media caused minor variations. After shear conditioning, the response of HUVEC to TNF-alpha (but not IL-1beta) was much reduced, while the responses of HUAEC and HCAEC to both cytokines were reduced. However, swapping the culture media suggested that the differences in the shear response arose largely from medium constituents, particularly basic fibroblast growth factor. When gene expression profiles for HUVEC were examined immediately after isolation, after 5 days in static culture and after re-exposure to shear, variations in gene expression were only partially attributable to the effects of changes in shear stress. CONCLUSIONS: The behaviour of cultured EC may depend as much on the physico-chemical culture conditions as on their origins. The EC phenotype appears to be highly pliable, with environmental factors, such as shear stress and growth factors, modifying responses in an inter-linked manner.