Fig. 4

Dab2 Mediates Fluid-Phase and Receptor-Dependent Endocytosis in LREs

(A) Experimental scheme to mosaically inhibit Dab2 function. A dominant-negative (DN), QUAS:DN-Dab2:p2A-EGFP, construct was injected into Tg(cldn15la:QF2^pd1142) embryos to co-express DN-Dab2 and soluble eGFP to mark expressing cells in IECs and LREs. Larvae mosaically expressing DN-Dab2 were then gavaged with fDex or mCherry and imaged 5 h post-gavage.

(B and C) Live confocal images of fDex or mCherry uptake in 6 dpf Tg(cldn15la:QF2 ^pd1142) LREs mosaically expressing DN-Dab2. LREs expressing DN-Dab2 (marked with dotted line) showed reduced fDex (n = 6) (B) and mCherry (n = 3) (C) uptake relative to WT neighboring LREs. Scale bar, 20 μm.

(D) Live confocal images of 6 dpf dab2^pd1162 +/+, +/−, −⁄− LREs imaged 5 h after gavage with LY and mCherry. Scale bar, 50 μm.

(E) Internalization profiles of LY (left) and mCherry (right) from 6 dpf dab2 ^pd1162 +/+ (n = 5), +/− (n = 8), −⁄− (n = 6) larvae. dab2 mutants showed impaired internalization of both protein (mCherry) and fluid-phase (LY) cargos (arrows). Data are means ± S.E.M. Images in (C) are digitally stitched. See also Figures S5 and S6.