The effect of PRMT5 knockdown by siRNA on the protein abundance of LILRB4. (a) Western blot analysis of PRMT5 and LILRB4 protein in MV-4-11 cells of the CON group, si-CN group, and si-PRMT5 group after corresponding treatment for 48 h. β-Actin was used as the internal control. Subsequent grayscale analysis revealed the expression levels of (b) PRMT5 protein and (b) LILRB4 protein in MV-4-11 cells of the si-PRMT5 group were lower than those of other two groups. (d) Western blot analysis of PRMT5 and LILRB4 proteins in THP-1 cells of the CON group, si-CN group, and si-PRMT5 group after corresponding treatment for 48 h. β-Actin was used as the internal control. Subsequent grayscale analysis revealed that the expression levels of (e) PRMT5 protein and (f) LILRB4 protein in THP-1 cells of the si-PRMT5 group were lower than those of other two groups. All the experiments were repeated for three times. Data are expressed by (; ).