(A and B) The inhibitory phosphorylations of GSK3β (pT390 and pS9) were decreased in PD-L1–deficient cells. (A) Control, PD-L1–knockdown, and PD-L1–knockout MDA-MB-231 cells were analyzed by immunoblotting using indicated antibodies. (B) The intensity of pT390-GSK3β and pS9-GSK3β were measured and normalized against total GSK3β in each group. Results was then normalized against the control group. (C) Snail exhibited stronger association with β-Trcp in PD-L1–deficient MDA-MB-231 cells. Endogenous Snail was immunoprecipitated from parental or KO-1 MDA-MB-231 cells. β-Trcp associated with Snail was determined by immunoblotting. (D) PD-L1–deficient cells exhibited significantly less p38-MAPK activity. The activating phosphorylation of p38-MAPK (p-p38) was determined by immunoblotting. The relative activity of p38-MAPK was represented by the ratio of p-p38 to total p38. (E) Selective inhibition of p38-MAPK suppressed the PD-L1–induced expression of Snail. MDA-MB-231 cells stably expressing PD-L1 were established by lentivirus-mediated infection. These cells were pretreated with SB203580 (10 μM) for 2 hours before transfection with siNC or siPD-L1 for 48 hours with SB203580, then subjected to immunoblotting analysis using indicated antibodies. After normalizing against β-actin levels, the expression level of Snail in each group was quantified. (B and D) Results (n = 3 3 independent experiments) were plotted as mean ± SEM and statistically analyzed using unpaired 2-tailed Student’s t test with the P value adjusted by Bonferroni’s method. *, P < 0.05; **, P < 0.01; ***, P < 0.001. (E) Results (n = 3 independent experiments) were plotted as mean ± SEM and statistically analyzed using 1-way ANOVA with the P value adjusted by Tukey’s honestly significant differences (HSD) using R function “aov” and “TukeyHSD” from package “stats” in R version 3.6.3. **, P < 0.01; ***, P < 0.001.