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. 2017 Nov 2;2(21):e81836. doi: 10.1172/jci.insight.81836

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(A) Representative kymographs obtained by membrane ruffling and (B) quantification, as performed in Figure 1, from cultured podocytes treated with the JAK1/3 inhibitor tofacitinib (100 nM, bottom row), which significantly attenuated IL-4–induced membrane ruffling compared with negative control (DMSO). Each symbol represents the average relative cell membrane displacement over time at 5 regions of a single cell. Mean ± SD of 2 experiments, with 2–3 cells/experiment (total of 5 cells analyzed/group). (C) Coomassie blue–stained SDS-PAGE and (D) spot albumin/creatinine ratios of urine from IL-4–treated mice treated with JAK1/3 inhibition, which significantly reduced IL-4–induced proteinuria. Urine was collected 24 hours after plasmid administration. Symbols represent individual mice, and bars represent the mean. Mean ± SEM of 2 experiments, with total of 5 mice/group. *P < 0.008 by 2-tailed Mann-Whitney.