L-selectin Dimerization Enhances Tether Formation to Properly Spaced Ligand

Oren Dwir,Douglas A Steeber,Ulrich S Schwarz,Raymond T Camphausen,Geoffrey S Kansas,Thomas F Tedder,Ronen Alon

doi:10.1074/jbc.m201999200

Oren Dwir, Douglas A Steeber + Show 5 more

Open Access

https://doi.org/10.1074/jbc.m201999200

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Abstract

Selectin counterreceptors are glycoprotein scaffolds bearing multiple carbohydrate ligands with exceptional ability to tether flowing cells under disruptive shear forces. Bond clusters may facilitate formation and stabilization of selectin tethers. L-selectin ligation has been shown to enhance L-selectin rolling on endothelial surfaces. We now report that monoclonal antibodies-induced L-selectin dimerization enhances L-selectin leukocyte tethering to purified physiological L-selectin ligands and glycopeptides. Microkinetic analysis of individual tethers suggests that leukocyte rolling is enhanced through the dimerization-induced increase in tether formation, rather than by tether stabilization. Notably, L-selectin dimerization failed to augment L-selectin-mediated adhesion below a threshold ligand density, suggesting that L-selectin dimerization enhanced adhesiveness only to properly clustered ligand. In contrast, an epidermal growth factor domain substitution of L-selectin enhanced tether formation to L-selectin ligands irrespective of ligand density, suggesting that this domain controls intrinsic ligand binding properties of L-selectin without inducing L-selectin dimerization. Strikingly, at low ligand densities, where L-selectin tethering was not responsive to dimerization, elevated shear stress restored sensitivity of tethering to selectin dimerization. This is the first indication that shear stress augments effective selectin ligand density at local contact sites by promoting L-selectin encounter of immobilized ligand.

Highlights

Selectins are specialized C-type lectins that mediate the reversible capture of circulating cell subsets to specific vessel walls and its subsequent rolling tethers in the direction of flow [1, 2]
We first characterized the effect of L-selectin dimerization on L-selectin adhesiveness to a purified PSGL-1 homodimer
Dissection of the augmenting effects of the dimerizing mAb revealed that both the ability of L-selectin-expressing cells to initiate tethers to high density PSGL-1 (110 sites/␮m2) and the conversion of these initial tethers into subsequent rolling were enhanced by L-selectin dimerization (Fig. 1, A and B)

Summary

EXPERIMENTAL PROCEDURES

The function-blocking anti-L-selectin mAb, DREG-200 [26], the anti L-selectin mAbs, LAM1–101 and LAM1–118 (both directed against the SCR domain of L-selectin) [27], and the anti-PSGL-1 mAb, PL-1 [28], were used as purified Ig. PSGL-1 was diluted to concentrations of 0.001– 0.2 ␮g/ml in coating medium (PBS supplemented with 20 mM bicarbonate, pH 8.5) and adsorbed onto a polystyrene plate for 15 h at 4 °C. Stock solutions of GlyCAM-1, fucoidin, or DREG-200 were diluted in coating medium and adsorbed onto the plates at 37 °C for 2 h. Neutralite avidin was diluted in PBS supplemented with 40 mM bicarbonate, pH 9.0, and immediately adsorbed onto a polystyrene plate for 15 h at 4 °C, washed five times with PBS, and blocked with PBS supplemented with 2% HSA for 2 h at 4 °C. The PSGL-1-derived peptides monobiotinylated in their CЈ termini, were each diluted in cell binding medium (see below) and adsorbed for 4 h on the avidin-coated plate

Laminar Flow Assays

Computerized Microkinetic Analysis

RESULTS

DISCUSSION