edar Search Results


goat anti edar  (R&D Systems)
94
R&D Systems goat anti edar
Goat Anti Edar, supplied by R&D Systems, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 94 stars, based on 1 article reviews
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gene exp edar mm00839685 m1  (Thermo Fisher)
85
Thermo Fisher gene exp edar mm00839685 m1
Gene Exp Edar Mm00839685 M1, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 85/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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edar  (Proteintech)
93
Proteintech edar
Vinburnine promotes <t>IR‐EDAR‐NFκB‐induced</t> apoptosis and pyroptosis. A) Reactome analysis of upregulated differential genes after 5µ m Vin / 2Gy IR treatment for 48h. B) Heatmap of differential gene expression in transcriptomics. C) qPCR of EDAR mRNA in NPC cells treated with 5µ m Vin / 2Gy IR for 48h ( n = 3). D) Protein expression of EDAR in the cell membrane/cytoplasm after being treated with 5µ m Vin / 2Gy IR for 48h. E) <t>Western</t> <t>blotting</t> detected the protein expression levels of the NFκB pathway (p65/p50) and pyroptosis index (GSDME/N‐GSDME/ Cleaved‐Caspase3) after 5µ m Vin / 2Gy IR treatment for 48h. Upon activation of the NFκB signaling pathway, its downstream signal, Caspase3, undergoes cleavage. This cleavage then cuts GSDME to form N‐GSDME, ultimately resulting in the pyroptosis of the cells. F) The binding of p65 to the EDAR promoter in the treated SUNE1 cells was detected by ChIP assay. G) The CB‐Dock2 website predicts the structural complex of vinburnine bound with the EDAR protein. Vinburnine is colored green; EDAR is colored grey and yellow. H) SPR technology proved that EDAR is the target of vinburnine. I) The Co‐IP experiment confirmed that after treatment with 5µ m Vin+2Gy IR, EDAR formed more protein complexes with EDARADD/TRAF6. Multiple samples were presented using mean ± standard deviation (SD). C) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. F) Statistical analysis with One‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.
Edar, supplied by Proteintech, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 93 stars, based on 1 article reviews
edar - by Bioz Stars, 2026-02
93/100 stars
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edar  (Santa Cruz Biotechnology)
91
Santa Cruz Biotechnology edar
Vinburnine promotes <t>IR‐EDAR‐NFκB‐induced</t> apoptosis and pyroptosis. A) Reactome analysis of upregulated differential genes after 5µ m Vin / 2Gy IR treatment for 48h. B) Heatmap of differential gene expression in transcriptomics. C) qPCR of EDAR mRNA in NPC cells treated with 5µ m Vin / 2Gy IR for 48h ( n = 3). D) Protein expression of EDAR in the cell membrane/cytoplasm after being treated with 5µ m Vin / 2Gy IR for 48h. E) <t>Western</t> <t>blotting</t> detected the protein expression levels of the NFκB pathway (p65/p50) and pyroptosis index (GSDME/N‐GSDME/ Cleaved‐Caspase3) after 5µ m Vin / 2Gy IR treatment for 48h. Upon activation of the NFκB signaling pathway, its downstream signal, Caspase3, undergoes cleavage. This cleavage then cuts GSDME to form N‐GSDME, ultimately resulting in the pyroptosis of the cells. F) The binding of p65 to the EDAR promoter in the treated SUNE1 cells was detected by ChIP assay. G) The CB‐Dock2 website predicts the structural complex of vinburnine bound with the EDAR protein. Vinburnine is colored green; EDAR is colored grey and yellow. H) SPR technology proved that EDAR is the target of vinburnine. I) The Co‐IP experiment confirmed that after treatment with 5µ m Vin+2Gy IR, EDAR formed more protein complexes with EDARADD/TRAF6. Multiple samples were presented using mean ± standard deviation (SD). C) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. F) Statistical analysis with One‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.
Edar, supplied by Santa Cruz Biotechnology, used in various techniques. Bioz Stars score: 91/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/edar/product/Santa Cruz Biotechnology
Average 91 stars, based on 1 article reviews
edar - by Bioz Stars, 2026-02
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rna probe  (Addgene inc)
92
Addgene inc rna probe
Vinburnine promotes <t>IR‐EDAR‐NFκB‐induced</t> apoptosis and pyroptosis. A) Reactome analysis of upregulated differential genes after 5µ m Vin / 2Gy IR treatment for 48h. B) Heatmap of differential gene expression in transcriptomics. C) qPCR of EDAR mRNA in NPC cells treated with 5µ m Vin / 2Gy IR for 48h ( n = 3). D) Protein expression of EDAR in the cell membrane/cytoplasm after being treated with 5µ m Vin / 2Gy IR for 48h. E) <t>Western</t> <t>blotting</t> detected the protein expression levels of the NFκB pathway (p65/p50) and pyroptosis index (GSDME/N‐GSDME/ Cleaved‐Caspase3) after 5µ m Vin / 2Gy IR treatment for 48h. Upon activation of the NFκB signaling pathway, its downstream signal, Caspase3, undergoes cleavage. This cleavage then cuts GSDME to form N‐GSDME, ultimately resulting in the pyroptosis of the cells. F) The binding of p65 to the EDAR promoter in the treated SUNE1 cells was detected by ChIP assay. G) The CB‐Dock2 website predicts the structural complex of vinburnine bound with the EDAR protein. Vinburnine is colored green; EDAR is colored grey and yellow. H) SPR technology proved that EDAR is the target of vinburnine. I) The Co‐IP experiment confirmed that after treatment with 5µ m Vin+2Gy IR, EDAR formed more protein complexes with EDARADD/TRAF6. Multiple samples were presented using mean ± standard deviation (SD). C) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. F) Statistical analysis with One‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.
Rna Probe, supplied by Addgene inc, used in various techniques. Bioz Stars score: 92/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 92 stars, based on 1 article reviews
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polyclonal anti edar antibodies  (R&D Systems)
90
R&D Systems polyclonal anti edar antibodies
Vinburnine promotes <t>IR‐EDAR‐NFκB‐induced</t> apoptosis and pyroptosis. A) Reactome analysis of upregulated differential genes after 5µ m Vin / 2Gy IR treatment for 48h. B) Heatmap of differential gene expression in transcriptomics. C) qPCR of EDAR mRNA in NPC cells treated with 5µ m Vin / 2Gy IR for 48h ( n = 3). D) Protein expression of EDAR in the cell membrane/cytoplasm after being treated with 5µ m Vin / 2Gy IR for 48h. E) <t>Western</t> <t>blotting</t> detected the protein expression levels of the NFκB pathway (p65/p50) and pyroptosis index (GSDME/N‐GSDME/ Cleaved‐Caspase3) after 5µ m Vin / 2Gy IR treatment for 48h. Upon activation of the NFκB signaling pathway, its downstream signal, Caspase3, undergoes cleavage. This cleavage then cuts GSDME to form N‐GSDME, ultimately resulting in the pyroptosis of the cells. F) The binding of p65 to the EDAR promoter in the treated SUNE1 cells was detected by ChIP assay. G) The CB‐Dock2 website predicts the structural complex of vinburnine bound with the EDAR protein. Vinburnine is colored green; EDAR is colored grey and yellow. H) SPR technology proved that EDAR is the target of vinburnine. I) The Co‐IP experiment confirmed that after treatment with 5µ m Vin+2Gy IR, EDAR formed more protein complexes with EDARADD/TRAF6. Multiple samples were presented using mean ± standard deviation (SD). C) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. F) Statistical analysis with One‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.
Polyclonal Anti Edar Antibodies, supplied by R&D Systems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/polyclonal anti edar antibodies/product/R&D Systems
Average 90 stars, based on 1 article reviews
polyclonal anti edar antibodies - by Bioz Stars, 2026-02
90/100 stars
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goat polyclonal edar  (R&D Systems)
93
R&D Systems goat polyclonal edar
Vinburnine promotes <t>IR‐EDAR‐NFκB‐induced</t> apoptosis and pyroptosis. A) Reactome analysis of upregulated differential genes after 5µ m Vin / 2Gy IR treatment for 48h. B) Heatmap of differential gene expression in transcriptomics. C) qPCR of EDAR mRNA in NPC cells treated with 5µ m Vin / 2Gy IR for 48h ( n = 3). D) Protein expression of EDAR in the cell membrane/cytoplasm after being treated with 5µ m Vin / 2Gy IR for 48h. E) <t>Western</t> <t>blotting</t> detected the protein expression levels of the NFκB pathway (p65/p50) and pyroptosis index (GSDME/N‐GSDME/ Cleaved‐Caspase3) after 5µ m Vin / 2Gy IR treatment for 48h. Upon activation of the NFκB signaling pathway, its downstream signal, Caspase3, undergoes cleavage. This cleavage then cuts GSDME to form N‐GSDME, ultimately resulting in the pyroptosis of the cells. F) The binding of p65 to the EDAR promoter in the treated SUNE1 cells was detected by ChIP assay. G) The CB‐Dock2 website predicts the structural complex of vinburnine bound with the EDAR protein. Vinburnine is colored green; EDAR is colored grey and yellow. H) SPR technology proved that EDAR is the target of vinburnine. I) The Co‐IP experiment confirmed that after treatment with 5µ m Vin+2Gy IR, EDAR formed more protein complexes with EDARADD/TRAF6. Multiple samples were presented using mean ± standard deviation (SD). C) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. F) Statistical analysis with One‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.
Goat Polyclonal Edar, supplied by R&D Systems, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/goat polyclonal edar/product/R&D Systems
Average 93 stars, based on 1 article reviews
goat polyclonal edar - by Bioz Stars, 2026-02
93/100 stars
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recombinant mouse edar protein  (R&D Systems)
86
R&D Systems recombinant mouse edar protein
Vinburnine promotes <t>IR‐EDAR‐NFκB‐induced</t> apoptosis and pyroptosis. A) Reactome analysis of upregulated differential genes after 5µ m Vin / 2Gy IR treatment for 48h. B) Heatmap of differential gene expression in transcriptomics. C) qPCR of EDAR mRNA in NPC cells treated with 5µ m Vin / 2Gy IR for 48h ( n = 3). D) Protein expression of EDAR in the cell membrane/cytoplasm after being treated with 5µ m Vin / 2Gy IR for 48h. E) <t>Western</t> <t>blotting</t> detected the protein expression levels of the NFκB pathway (p65/p50) and pyroptosis index (GSDME/N‐GSDME/ Cleaved‐Caspase3) after 5µ m Vin / 2Gy IR treatment for 48h. Upon activation of the NFκB signaling pathway, its downstream signal, Caspase3, undergoes cleavage. This cleavage then cuts GSDME to form N‐GSDME, ultimately resulting in the pyroptosis of the cells. F) The binding of p65 to the EDAR promoter in the treated SUNE1 cells was detected by ChIP assay. G) The CB‐Dock2 website predicts the structural complex of vinburnine bound with the EDAR protein. Vinburnine is colored green; EDAR is colored grey and yellow. H) SPR technology proved that EDAR is the target of vinburnine. I) The Co‐IP experiment confirmed that after treatment with 5µ m Vin+2Gy IR, EDAR formed more protein complexes with EDARADD/TRAF6. Multiple samples were presented using mean ± standard deviation (SD). C) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. F) Statistical analysis with One‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.
Recombinant Mouse Edar Protein, supplied by R&D Systems, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 86 stars, based on 1 article reviews
recombinant mouse edar protein - by Bioz Stars, 2026-02
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gene exp edar hs00223468 m1  (Thermo Fisher)
93
Thermo Fisher gene exp edar hs00223468 m1
Effects of <t>EDAR</t> knockdown in skin cells. ( a ) Wound-healing efficiency after EDAR knockdown in keratinocytes (HaCaT). ( b ) Representative image from in vitro scratch wound-healing assay; scale bar = 146 μm. Yellow lines represent the wound boundary. ( c ) Expression of genes related to wound healing in EDAR knockdown cells. Error bars represent the standard error of the mean. * p < 0.05, ** p < 0.01; student t -test.
Gene Exp Edar Hs00223468 M1, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 93 stars, based on 1 article reviews
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anti edar  (R&D Systems)
91
R&D Systems anti edar
A hypothetical model of <t>Eda1/Edar-regulated</t> bone homeostasis. Based on our in vitro and in vivo results, a hypothetical model suggests that Eda1/Edar interactions <t>between</t> <t>EDA-presenting</t> osteoblasts and Edar-presenting osteoclasts may be a relevant communicational signal enabling concerted postnatal bone homeostasis ( A ) and that Eda1 induces Nfat and/or NF-κB transcriptional activation, leading to the expression of osteoclastic activity-associated genes, such as Ctsk , Mmp9 , Trap , and Tcirg1 ( B ). Inversely, Eda1 deficiency in mice may result in diminished osteoclastic activity, resulting in osteopetrosis-like changes and causing a disturbed intramembranous bone homeostasis during a postnatal period.
Anti Edar, supplied by R&D Systems, used in various techniques. Bioz Stars score: 91/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 91 stars, based on 1 article reviews
anti edar - by Bioz Stars, 2026-02
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edar genbank  (Nissen)
90
Nissen edar genbank
A hypothetical model of <t>Eda1/Edar-regulated</t> bone homeostasis. Based on our in vitro and in vivo results, a hypothetical model suggests that Eda1/Edar interactions <t>between</t> <t>EDA-presenting</t> osteoblasts and Edar-presenting osteoclasts may be a relevant communicational signal enabling concerted postnatal bone homeostasis ( A ) and that Eda1 induces Nfat and/or NF-κB transcriptional activation, leading to the expression of osteoclastic activity-associated genes, such as Ctsk , Mmp9 , Trap , and Tcirg1 ( B ). Inversely, Eda1 deficiency in mice may result in diminished osteoclastic activity, resulting in osteopetrosis-like changes and causing a disturbed intramembranous bone homeostasis during a postnatal period.
Edar Genbank, supplied by Nissen, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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edar genbank - by Bioz Stars, 2026-02
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zebrafish eda and edar mutants  (Rohner)
90
Rohner zebrafish eda and edar mutants
A hypothetical model of <t>Eda1/Edar-regulated</t> bone homeostasis. Based on our in vitro and in vivo results, a hypothetical model suggests that Eda1/Edar interactions <t>between</t> <t>EDA-presenting</t> osteoblasts and Edar-presenting osteoclasts may be a relevant communicational signal enabling concerted postnatal bone homeostasis ( A ) and that Eda1 induces Nfat and/or NF-κB transcriptional activation, leading to the expression of osteoclastic activity-associated genes, such as Ctsk , Mmp9 , Trap , and Tcirg1 ( B ). Inversely, Eda1 deficiency in mice may result in diminished osteoclastic activity, resulting in osteopetrosis-like changes and causing a disturbed intramembranous bone homeostasis during a postnatal period.
Zebrafish Eda And Edar Mutants, supplied by Rohner, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Image Search Results


Vinburnine promotes IR‐EDAR‐NFκB‐induced apoptosis and pyroptosis. A) Reactome analysis of upregulated differential genes after 5µ m Vin / 2Gy IR treatment for 48h. B) Heatmap of differential gene expression in transcriptomics. C) qPCR of EDAR mRNA in NPC cells treated with 5µ m Vin / 2Gy IR for 48h ( n = 3). D) Protein expression of EDAR in the cell membrane/cytoplasm after being treated with 5µ m Vin / 2Gy IR for 48h. E) Western blotting detected the protein expression levels of the NFκB pathway (p65/p50) and pyroptosis index (GSDME/N‐GSDME/ Cleaved‐Caspase3) after 5µ m Vin / 2Gy IR treatment for 48h. Upon activation of the NFκB signaling pathway, its downstream signal, Caspase3, undergoes cleavage. This cleavage then cuts GSDME to form N‐GSDME, ultimately resulting in the pyroptosis of the cells. F) The binding of p65 to the EDAR promoter in the treated SUNE1 cells was detected by ChIP assay. G) The CB‐Dock2 website predicts the structural complex of vinburnine bound with the EDAR protein. Vinburnine is colored green; EDAR is colored grey and yellow. H) SPR technology proved that EDAR is the target of vinburnine. I) The Co‐IP experiment confirmed that after treatment with 5µ m Vin+2Gy IR, EDAR formed more protein complexes with EDARADD/TRAF6. Multiple samples were presented using mean ± standard deviation (SD). C) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. F) Statistical analysis with One‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.

Journal: Advanced Science

Article Title: Vinburnine Sensitizes Radiotherapy Efficacy in Nasopharyngeal Carcinoma by Triggering Pyroptosis and Immune Responses via Activation of EDAR‐NFκB Pathway

doi: 10.1002/advs.202506139

Figure Lengend Snippet: Vinburnine promotes IR‐EDAR‐NFκB‐induced apoptosis and pyroptosis. A) Reactome analysis of upregulated differential genes after 5µ m Vin / 2Gy IR treatment for 48h. B) Heatmap of differential gene expression in transcriptomics. C) qPCR of EDAR mRNA in NPC cells treated with 5µ m Vin / 2Gy IR for 48h ( n = 3). D) Protein expression of EDAR in the cell membrane/cytoplasm after being treated with 5µ m Vin / 2Gy IR for 48h. E) Western blotting detected the protein expression levels of the NFκB pathway (p65/p50) and pyroptosis index (GSDME/N‐GSDME/ Cleaved‐Caspase3) after 5µ m Vin / 2Gy IR treatment for 48h. Upon activation of the NFκB signaling pathway, its downstream signal, Caspase3, undergoes cleavage. This cleavage then cuts GSDME to form N‐GSDME, ultimately resulting in the pyroptosis of the cells. F) The binding of p65 to the EDAR promoter in the treated SUNE1 cells was detected by ChIP assay. G) The CB‐Dock2 website predicts the structural complex of vinburnine bound with the EDAR protein. Vinburnine is colored green; EDAR is colored grey and yellow. H) SPR technology proved that EDAR is the target of vinburnine. I) The Co‐IP experiment confirmed that after treatment with 5µ m Vin+2Gy IR, EDAR formed more protein complexes with EDARADD/TRAF6. Multiple samples were presented using mean ± standard deviation (SD). C) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. F) Statistical analysis with One‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.

Article Snippet: Subsequently, western blotting confirmed that EDAR (Proteintech, China) formed protein complexes with EDARADD (Abclone, China) and TRAF6 (Immunoway, USA).

Techniques: Gene Expression, Expressing, Membrane, Western Blot, Activation Assay, Binding Assay, Co-Immunoprecipitation Assay, Standard Deviation

Knocking down EDAR suppresses the radiosensitization effect of vinburnine. A) The cytotoxic effect of 5uM Vin/2Gy IR on EDAR‐knockdown cells was assessed using the CCK‐8 assay ( n = 5). B) Following EDAR knockdown, cells were treated with 5uM Vin/2Gy IR. Colony formation was evaluated by crystal violet staining (left) and the number of colonies was quantified (right) ( n = 3). C–E) Flow cytometry detected the apoptosis/ROS levels/mitochondrial membrane potential of the Vin±IR‐treated cells after EDAR knockdown ( n = 3). F) After EDAR knockdown, western blotting detected the protein expression (p65/p50/GSDME/N‐GSDME/Cleaved‐Caspase3) in the treated group. Multiple samples were presented using mean ± standard deviation (SD). A–E) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.

Journal: Advanced Science

Article Title: Vinburnine Sensitizes Radiotherapy Efficacy in Nasopharyngeal Carcinoma by Triggering Pyroptosis and Immune Responses via Activation of EDAR‐NFκB Pathway

doi: 10.1002/advs.202506139

Figure Lengend Snippet: Knocking down EDAR suppresses the radiosensitization effect of vinburnine. A) The cytotoxic effect of 5uM Vin/2Gy IR on EDAR‐knockdown cells was assessed using the CCK‐8 assay ( n = 5). B) Following EDAR knockdown, cells were treated with 5uM Vin/2Gy IR. Colony formation was evaluated by crystal violet staining (left) and the number of colonies was quantified (right) ( n = 3). C–E) Flow cytometry detected the apoptosis/ROS levels/mitochondrial membrane potential of the Vin±IR‐treated cells after EDAR knockdown ( n = 3). F) After EDAR knockdown, western blotting detected the protein expression (p65/p50/GSDME/N‐GSDME/Cleaved‐Caspase3) in the treated group. Multiple samples were presented using mean ± standard deviation (SD). A–E) Statistical analysis with Two‐way ANOVA was used to analyze the statistical differences among multiple groups. * p < 0.05, ** p < 0.01, *** p < 0.001, **** p < 0.0001, ns for non‐significant.

Article Snippet: Subsequently, western blotting confirmed that EDAR (Proteintech, China) formed protein complexes with EDARADD (Abclone, China) and TRAF6 (Immunoway, USA).

Techniques: Knockdown, CCK-8 Assay, Staining, Flow Cytometry, Membrane, Western Blot, Expressing, Standard Deviation

Effects of EDAR knockdown in skin cells. ( a ) Wound-healing efficiency after EDAR knockdown in keratinocytes (HaCaT). ( b ) Representative image from in vitro scratch wound-healing assay; scale bar = 146 μm. Yellow lines represent the wound boundary. ( c ) Expression of genes related to wound healing in EDAR knockdown cells. Error bars represent the standard error of the mean. * p < 0.05, ** p < 0.01; student t -test.

Journal: Biomolecules

Article Title: Fine Wrinkle Improvement through Bioactive Materials That Modulate EDAR and BNC2 Gene Expression

doi: 10.3390/biom14030279

Figure Lengend Snippet: Effects of EDAR knockdown in skin cells. ( a ) Wound-healing efficiency after EDAR knockdown in keratinocytes (HaCaT). ( b ) Representative image from in vitro scratch wound-healing assay; scale bar = 146 μm. Yellow lines represent the wound boundary. ( c ) Expression of genes related to wound healing in EDAR knockdown cells. Error bars represent the standard error of the mean. * p < 0.05, ** p < 0.01; student t -test.

Article Snippet: The PCR reaction conditions were as follows: 30 cycles at 95 °C for 45 s, 60 °C for 1 min, and 72 °C for 45 s. qPCR was performed using the following commercial Taqman primers (Thermofisher): EDAR (Hs00223468_m1); BNC2 (Hs00417700_m1); MMP1 (Hs00899658_m1); COL4A1 (Hs00266237_m1); AQP3 (Hs01105469_g1); IVL (Hs00846307_s1); COL1A1 (Hs00164004_m1); HAS3 (Hs00193436_m1); LAMA3 (Hs00165042_m1); ITGA6 (Hs01041011_m1); FGF10 (Hs01045105_m1); FGF2 (Hs04187682_g1); TGFβ (Hs00998133_m1); CAT (Hs00937395_m1); GPX1 (Hs01028922_g1); and SOD1 (Hs00166575_m1).

Techniques: Knockdown, In Vitro, Wound Healing Assay, Expressing

The screening of EDAR and BNC2 expression-regulating materials. ( a ) The materials that increased the expression of EDAR . Relative expression of EDAR in keratinocytes (HaCaT) treated with various candidates. ( b ) The materials that decreased the expression of BNC2 . Relative expression of BNC2 in fibroblasts (Hs68) treated with various candidates. Error bars indicate the standard error of the mean. * p < 0.05, ** p < 0.01; student t -test.

Journal: Biomolecules

Article Title: Fine Wrinkle Improvement through Bioactive Materials That Modulate EDAR and BNC2 Gene Expression

doi: 10.3390/biom14030279

Figure Lengend Snippet: The screening of EDAR and BNC2 expression-regulating materials. ( a ) The materials that increased the expression of EDAR . Relative expression of EDAR in keratinocytes (HaCaT) treated with various candidates. ( b ) The materials that decreased the expression of BNC2 . Relative expression of BNC2 in fibroblasts (Hs68) treated with various candidates. Error bars indicate the standard error of the mean. * p < 0.05, ** p < 0.01; student t -test.

Article Snippet: The PCR reaction conditions were as follows: 30 cycles at 95 °C for 45 s, 60 °C for 1 min, and 72 °C for 45 s. qPCR was performed using the following commercial Taqman primers (Thermofisher): EDAR (Hs00223468_m1); BNC2 (Hs00417700_m1); MMP1 (Hs00899658_m1); COL4A1 (Hs00266237_m1); AQP3 (Hs01105469_g1); IVL (Hs00846307_s1); COL1A1 (Hs00164004_m1); HAS3 (Hs00193436_m1); LAMA3 (Hs00165042_m1); ITGA6 (Hs01041011_m1); FGF10 (Hs01045105_m1); FGF2 (Hs04187682_g1); TGFβ (Hs00998133_m1); CAT (Hs00937395_m1); GPX1 (Hs01028922_g1); and SOD1 (Hs00166575_m1).

Techniques: Expressing

Analysis of the wound-healing effects of EDAR expression-regulating materials through in vitro experiments. ( a ) Wound-healing efficacy of EDAR expression-upregulating materials in HaCaT. ( b ) Representative image from the in vitro scratch wound-healing assay; scale bar = 122 μm. Yellow lines represent the wound boundary. ( c ) The enhancement of FGF10 expression by EDAR -upregulating materials. ( d ) The enhancement of FGF2 expression by EDAR -upregulating materials. ( e ) The enhancement of TGFβ1 expression by EDAR -upregulating materials. Error bars represent the standard error of the mean. * p < 0.05, ** p < 0.01; student t -test.

Journal: Biomolecules

Article Title: Fine Wrinkle Improvement through Bioactive Materials That Modulate EDAR and BNC2 Gene Expression

doi: 10.3390/biom14030279

Figure Lengend Snippet: Analysis of the wound-healing effects of EDAR expression-regulating materials through in vitro experiments. ( a ) Wound-healing efficacy of EDAR expression-upregulating materials in HaCaT. ( b ) Representative image from the in vitro scratch wound-healing assay; scale bar = 122 μm. Yellow lines represent the wound boundary. ( c ) The enhancement of FGF10 expression by EDAR -upregulating materials. ( d ) The enhancement of FGF2 expression by EDAR -upregulating materials. ( e ) The enhancement of TGFβ1 expression by EDAR -upregulating materials. Error bars represent the standard error of the mean. * p < 0.05, ** p < 0.01; student t -test.

Article Snippet: The PCR reaction conditions were as follows: 30 cycles at 95 °C for 45 s, 60 °C for 1 min, and 72 °C for 45 s. qPCR was performed using the following commercial Taqman primers (Thermofisher): EDAR (Hs00223468_m1); BNC2 (Hs00417700_m1); MMP1 (Hs00899658_m1); COL4A1 (Hs00266237_m1); AQP3 (Hs01105469_g1); IVL (Hs00846307_s1); COL1A1 (Hs00164004_m1); HAS3 (Hs00193436_m1); LAMA3 (Hs00165042_m1); ITGA6 (Hs01041011_m1); FGF10 (Hs01045105_m1); FGF2 (Hs04187682_g1); TGFβ (Hs00998133_m1); CAT (Hs00937395_m1); GPX1 (Hs01028922_g1); and SOD1 (Hs00166575_m1).

Techniques: Expressing, In Vitro, Wound Healing Assay

Dermal collagen enhancement and wrinkle improvement by the LG formula containing EDAR and BNC2 expression-regulating materials. ( a ) The enhancement of dermal collagen by the LG formula. ( b ) Representative images of 3D skin; scale bar = 275 μm. ( c ) The comparison of the wrinkle improvement rate between retinol- and LG formula-treated groups. The LG formula included lupeol, sucralfate, oryzanol, and phloretin. ( d ) Representative images captured using Antera 3D at 0 and 8 weeks of treatment. * p < 0.05; student t -test.

Journal: Biomolecules

Article Title: Fine Wrinkle Improvement through Bioactive Materials That Modulate EDAR and BNC2 Gene Expression

doi: 10.3390/biom14030279

Figure Lengend Snippet: Dermal collagen enhancement and wrinkle improvement by the LG formula containing EDAR and BNC2 expression-regulating materials. ( a ) The enhancement of dermal collagen by the LG formula. ( b ) Representative images of 3D skin; scale bar = 275 μm. ( c ) The comparison of the wrinkle improvement rate between retinol- and LG formula-treated groups. The LG formula included lupeol, sucralfate, oryzanol, and phloretin. ( d ) Representative images captured using Antera 3D at 0 and 8 weeks of treatment. * p < 0.05; student t -test.

Article Snippet: The PCR reaction conditions were as follows: 30 cycles at 95 °C for 45 s, 60 °C for 1 min, and 72 °C for 45 s. qPCR was performed using the following commercial Taqman primers (Thermofisher): EDAR (Hs00223468_m1); BNC2 (Hs00417700_m1); MMP1 (Hs00899658_m1); COL4A1 (Hs00266237_m1); AQP3 (Hs01105469_g1); IVL (Hs00846307_s1); COL1A1 (Hs00164004_m1); HAS3 (Hs00193436_m1); LAMA3 (Hs00165042_m1); ITGA6 (Hs01041011_m1); FGF10 (Hs01045105_m1); FGF2 (Hs04187682_g1); TGFβ (Hs00998133_m1); CAT (Hs00937395_m1); GPX1 (Hs01028922_g1); and SOD1 (Hs00166575_m1).

Techniques: Expressing, Comparison

A hypothetical model of Eda1/Edar-regulated bone homeostasis. Based on our in vitro and in vivo results, a hypothetical model suggests that Eda1/Edar interactions between EDA-presenting osteoblasts and Edar-presenting osteoclasts may be a relevant communicational signal enabling concerted postnatal bone homeostasis ( A ) and that Eda1 induces Nfat and/or NF-κB transcriptional activation, leading to the expression of osteoclastic activity-associated genes, such as Ctsk , Mmp9 , Trap , and Tcirg1 ( B ). Inversely, Eda1 deficiency in mice may result in diminished osteoclastic activity, resulting in osteopetrosis-like changes and causing a disturbed intramembranous bone homeostasis during a postnatal period.

Journal: International Journal of Molecular Sciences

Article Title: Ectodysplasin A1 Deficiency Leads to Osteopetrosis-like Changes in Bones of the Skull Associated with Diminished Osteoclastic Activity

doi: 10.3390/ijms232012189

Figure Lengend Snippet: A hypothetical model of Eda1/Edar-regulated bone homeostasis. Based on our in vitro and in vivo results, a hypothetical model suggests that Eda1/Edar interactions between EDA-presenting osteoblasts and Edar-presenting osteoclasts may be a relevant communicational signal enabling concerted postnatal bone homeostasis ( A ) and that Eda1 induces Nfat and/or NF-κB transcriptional activation, leading to the expression of osteoclastic activity-associated genes, such as Ctsk , Mmp9 , Trap , and Tcirg1 ( B ). Inversely, Eda1 deficiency in mice may result in diminished osteoclastic activity, resulting in osteopetrosis-like changes and causing a disturbed intramembranous bone homeostasis during a postnatal period.

Article Snippet: After blocking in 5% nonfat dry milk/TBST containing 0.1% Tween for 2 h, membranes were incubated overnight at 4 °C with rabbit anti-Tcirg1 (Thermo Fisher Scientifics), anti-Mmp9 (Sigma-Aldrich), anti-Trap (Abcam), anti-phospho-p65 (Cell signaling), anti-Eda (Invitrogen), mouse anti-Nfatc1 (Sigma-Aldrich), anti-cathepsin K (Abcam), anti-Edar (R&D Systems, Minneapolis, MA, USA), and anti-GAPDH (Thermo Fisher Scientifics) antibodies, diluted in 2% BSA/TBST buffer.

Techniques: In Vitro, In Vivo, Activation Assay, Expressing, Activity Assay