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Wnt3a attenuates acute lung injury by reducing P2X7 receptor-mediated lung cell death

This study investigates the protective role of Wnt3a in acute lung injury by reducing P2X7 receptor-mediated cell death in the lung. The expression of P2X receptors in lung cells, the effect of P2X7 receptor activation on lung cell death, and the inhibitory effect of Wnt3a on P2X7 receptor activity were assessed. The results suggest that Wnt3a may be a potential therapeutic target for the treatment of acute lung injury.

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Wnt3a attenuates acute lung injury by reducing P2X7 receptor-mediated lung cell death

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  1. Wnt3a attenuates acute lung injury by reducing P2X7 receptor–mediated lung type I cell death Yujie Guo, Amarjit Mishra, Tingting Weng, Narendranath Reddy Chintagari, Yang Wang, Chunling Zhao, Chaoqun Huang, and Lin Liu Online Data Supplement

  2. b P2X3R P2X1R P2X2R P2X4R P2X5R P2X6R P2X7R a E10 200 bp 100 bp HEK293-P2x7R HEK293 RLE-6TN MLE15 PRE-TII R3/1 A549 H441 RLF-6 E10 Lung P2X7R GAPDH E10 β-actin Supplementary Figure S1: Expression of P2X receptors in the lung cells. (a) Protein expression of P2X7R in different lung cell lines (20 µg total protein) was analyzed by Western blot using β-actin as an internal control. (b) mRNA expression of P2XRs in E10 cells and normal mouse lung tissues was determined by PCR using GAPDH as an loading control.

  3. a b * * * ** * * BzATP ̶ + + ̶ oATP ̶ ̶ + + Supplementary Figure S2: Activation of P2X7R causes E10 cell death. (a) E10 cells were incubated with different concentrations of BzATP for 12 hours. Cell number was counted. (b) E10 cells were treated with 400 µM BzATP in the absence or presence of 500 µM oATP for 12 hours, and the released LDH were measured. Data shown are means ± s.e.m. of three independent experiments. Statistical significance was determined by one-way ANOVA analysis with posthoc Tukey’s test. *P<0.001 v.s. control without any treatment or 0 time, **P<0.001 v.s. 400 µM BzATP.

  4. a c b * * # # Supplementary Figure S3: BzATP does not cause cell death in the absence of P2X7R. (a) E10 cells were transduced with adenovirus-based shRNA vectors [virus control (si-control), si-P2X7R (1) and si-P2X7R (2)] for 4 days and then treated with 400 µM BzATP for 12 hours. Released LDH were measured. A549 cells (b) and H441 cells (c) were incubated with different concentrations of BzATP for 12 hours. Cell viability was measured. Data shown are means ± s.e.m. of three independent experiments. *P<0.001 v.s. control, #P<0.005 v.s. si-control.

  5. Supplementary Figure S4:  P2X7R inhibits Wnt/β-catenin signaling. The relative mRNA expression of Wnt/β-catenin downstream genes in E10 cells treated with 400 µM BzATP for various times were determined using Real-time PCR. Data were normalized to 18S rRNA and expressed as a percent of 0 time. Data shown are means ± s.e.m. of three independent experiments.

  6. BzATP Con_CM BzATP Wnt3a_CM Control Control YO-PRO 100 μm Supplementary Figure S5: Effect of Wnt3a on P2X7R activity. E10 cells were treated with 400 µM BzATP for 15 min and incubated with YO-PRO dye for 10 min. The fluorescence was observed using a Nikon TE-2000 inverted microscope.

  7. BzATP Control LiCl (mM) 0 10 25 50 Supplementary Figure S6: Effect of LiCl on BzATP-induced cell death. E10 cells were treated with 10, 25, and 50 mM LiCl in the presence or absence of 400 µM BzATP for 8 hours, and then immuo-stained with anti-β-catenin antibodies . Scale bar: 50 µm. β-Catenin

  8. BzATP Supplementary Figure S7: Wnt3a reduces BAL proteins in BzATP-treated rat. The rats were intratracheally instilled with BzATP with control (Con) or Wnt3a conditioned medium for 24 hours. BAL protein concentration was measured. Values represent means ± s.e.m. Statistical significance was determined by one-way ANOVA analysis with posthoc Tukey’s test. *P<0.01 v.s. PBS alone group and **P<0.01 v.s. BzATP + Con_CM group (n=8/group). * * **

  9. Supplementary Figure S8: Original scans of western blots

  10. Supplementary Table S1. PCR primer sequences foe mouse genes

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