(A) DEG effect size of AXL across PDAC patient cohorts (10, 15, 18, 28, 29). (B–D) Invasion assay of BL PANC1 cells transfected with AXL (siAXL) or control siRNA (siCtrl). (B) Representative DAPI staining of invaded cells. Scale bar: 50 μm. (C) Immunoblot for AXL and β-actin. (D) Quantification of B. Scatterplots show average counts and means ± SD. Statistical significance was determined by an unpaired Student’s t test. n = 6. (E and F) Immunoblot for AXL, ROBO3, p-STAT3, total STAT3, and β-actin, in BL PANC1 (E) and MiaPaCa2 (F) cells transfected with siAXL or siCtrl. (G and H) Immunoblot for AXL, p-STAT3, STAT3, and β-actin, in ROBO3^hi-classified GCDX57 (G) and GCDX5 (H) cells transfected with siAXL or siCtrl. (I) Immunoblot of co-immunoprecipitation of AXL for AXL and p-STAT3 in AXL pulldown, IgG control, and input. (C and E–I) Representative of n = 3 independent experiments; β-actin as loading control. (J–L) GSEA of RNA-Seq data for shRNA depletion of AXL (shAXL) and control shRNA (shCtrl) (ref. 38; GEO GSE128417) for selected MSigDB gene sets. NESs and FDR q values are indicated. (M) Transcript correlation analysis of compartment-specific transcriptional profiles of PDAC patients. Tumor resection material was FACS-sorted into epithelial (EPCAM⁺CD45^–; n = 29; “Epi”), immune (EPCAM^–CD45⁺; n = 27), and CAF-enriched (EPCAM^–CD45^–; n = 7; “CAF-enr”) and RNA-Seq performed. Spearman’s correlation (indicated by color) was calculated from epithelial AXL to epithelial WNT10A and immune and CAF-enriched IL-6. Significant correlations are indicated by their P values. (N and O) GSEA of RNA-Seq data for shAXL versus shCtrl (N; as in J–L) and for siROBO3 versus siCtrl (O; as in Figure 3, F–K) for stroma-related MSigDB gene sets. NESs are shown in bar graphs, and –log10 FDR q values are indicated as line graphs. str, stripped; GO, Gene Ontology.