il 25 Search Results


il 25  (Miltenyi Biotec)
90
Miltenyi Biotec il 25
Il 25, supplied by Miltenyi Biotec, 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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mouse il 25  (Elabscience Biotechnology)
94
Elabscience Biotechnology mouse il 25
OTUD6A expression is upregulated in airway epithelial cells in asthma. A‐B) Immunohistochemical (IHC) staining and quantification of OTUD6A in human lung tissues from healthy controls ( n = 2) and asthmatic patients ( n = 2). Scale bars: 100 µm. C‐D) Western blot analysis of OTUD6A expression in lung tissue from HDM‐CAM (C) and HDM‐AAM (D) mice. E‐F) Representative images of IHC for OTUD6A on mouse lung sections of HDM‐CAM and corresponding quantitative analysis ( n = 5). Scale bars: 100 µm. G‐H) Representative images of IHC for OTUD6A on mouse lung sections of HDM‐AAM and corresponding quantitative analysis ( n = 5). Scale bars; 100 µm. I‐J) Immunofluorescence staining for OTUD6A in the mouse lung tissue of HDM‐AAM and corresponding quantitative analysis ( n = 5). Scale bars: 50 µm. K) Western blot analysis of OTUD6A protein levels in BEAS‐2B cells stimulated with HDM (100 µg/mL) at indicated time points ( n = 5). L‐M) BEAS‐2B cells transfected with OTUD6A or control vector for 24 h. L) Western blot analysis of ZO‐1 and Occludin. M) RT‐qPCR analysis <t>of</t> <t>IL‐25</t> , IL‐33 , and TSLP mRNA levels ( n = 5). N‐O) HBEpiC cells transfected with OTUD6A or control vector for 24 h. N) Western blot analysis of ZO‐1 and Occludin. O) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). P‐Q) HBEpiC cells transfected with siOTUD6A or control vector for 48 h and stimulated with HDM (100 µg/mL) for 6 h. P) Western blot analysis of OTUD6A, ZO‐1, and Occludin. Q) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). Data are presented as mean ± SEM. P values determined by two‐tailed unpaired t‐test or one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).
Mouse Il 25, supplied by Elabscience Biotechnology, 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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sources anti il 17a nbp1 42746 rabbit igg  (Novus Biologicals)
94
Novus Biologicals sources anti il 17a nbp1 42746 rabbit igg
OTUD6A expression is upregulated in airway epithelial cells in asthma. A‐B) Immunohistochemical (IHC) staining and quantification of OTUD6A in human lung tissues from healthy controls ( n = 2) and asthmatic patients ( n = 2). Scale bars: 100 µm. C‐D) Western blot analysis of OTUD6A expression in lung tissue from HDM‐CAM (C) and HDM‐AAM (D) mice. E‐F) Representative images of IHC for OTUD6A on mouse lung sections of HDM‐CAM and corresponding quantitative analysis ( n = 5). Scale bars: 100 µm. G‐H) Representative images of IHC for OTUD6A on mouse lung sections of HDM‐AAM and corresponding quantitative analysis ( n = 5). Scale bars; 100 µm. I‐J) Immunofluorescence staining for OTUD6A in the mouse lung tissue of HDM‐AAM and corresponding quantitative analysis ( n = 5). Scale bars: 50 µm. K) Western blot analysis of OTUD6A protein levels in BEAS‐2B cells stimulated with HDM (100 µg/mL) at indicated time points ( n = 5). L‐M) BEAS‐2B cells transfected with OTUD6A or control vector for 24 h. L) Western blot analysis of ZO‐1 and Occludin. M) RT‐qPCR analysis <t>of</t> <t>IL‐25</t> , IL‐33 , and TSLP mRNA levels ( n = 5). N‐O) HBEpiC cells transfected with OTUD6A or control vector for 24 h. N) Western blot analysis of ZO‐1 and Occludin. O) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). P‐Q) HBEpiC cells transfected with siOTUD6A or control vector for 48 h and stimulated with HDM (100 µg/mL) for 6 h. P) Western blot analysis of OTUD6A, ZO‐1, and Occludin. Q) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). Data are presented as mean ± SEM. P values determined by two‐tailed unpaired t‐test or one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).
Sources Anti Il 17a Nbp1 42746 Rabbit Igg, supplied by Novus Biologicals, 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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human il 25 protein levels  (Boster Bio)
94
Boster Bio human il 25 protein levels
Aberrant SCC and goblet cell hyperplasia phenotype in nasal mucosa from patients with HDM-AR (A). POU2F3, DCAMKL1 and MUC5AC mRNA levels in nasal swab specimens from normal control (NC) (n = 17) and HDM-AR (n = 17) donors. (B–C). POU2F3 and MUC5AC proteins were detected and analyzed in total nasal mucosal cells obtained by nasal swabs from NC (n = 17) and HDM-AR (n = 17) donors (scale bar = 50 μm). (D). Release <t>of</t> <t>IL-25</t> protein in nasal secretions from NC (n = 15) and HDM-AR (n = 15) donors. Data are presented as medians with interquartile ranges. The Mann-Whitney U test was used in (A – D)
Human Il 25 Protein Levels, supplied by Boster Bio, 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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anti il 25  (R&D Systems)
92
R&D Systems anti il 25
Aberrant SCC and goblet cell hyperplasia phenotype in nasal mucosa from patients with HDM-AR (A). POU2F3, DCAMKL1 and MUC5AC mRNA levels in nasal swab specimens from normal control (NC) (n = 17) and HDM-AR (n = 17) donors. (B–C). POU2F3 and MUC5AC proteins were detected and analyzed in total nasal mucosal cells obtained by nasal swabs from NC (n = 17) and HDM-AR (n = 17) donors (scale bar = 50 μm). (D). Release <t>of</t> <t>IL-25</t> protein in nasal secretions from NC (n = 15) and HDM-AR (n = 15) donors. Data are presented as medians with interquartile ranges. The Mann-Whitney U test was used in (A – D)
Anti Il 25, supplied by R&D Systems, 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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human il 25  (Elabscience Biotechnology)
94
Elabscience Biotechnology human il 25
Aberrant SCC and goblet cell hyperplasia phenotype in nasal mucosa from patients with HDM-AR (A). POU2F3, DCAMKL1 and MUC5AC mRNA levels in nasal swab specimens from normal control (NC) (n = 17) and HDM-AR (n = 17) donors. (B–C). POU2F3 and MUC5AC proteins were detected and analyzed in total nasal mucosal cells obtained by nasal swabs from NC (n = 17) and HDM-AR (n = 17) donors (scale bar = 50 μm). (D). Release <t>of</t> <t>IL-25</t> protein in nasal secretions from NC (n = 15) and HDM-AR (n = 15) donors. Data are presented as medians with interquartile ranges. The Mann-Whitney U test was used in (A – D)
Human Il 25, supplied by Elabscience Biotechnology, 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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be0394 dextran sulfate sodium salt  (Bio X Cell)
94
Bio X Cell be0394 dextran sulfate sodium salt
Aberrant SCC and goblet cell hyperplasia phenotype in nasal mucosa from patients with HDM-AR (A). POU2F3, DCAMKL1 and MUC5AC mRNA levels in nasal swab specimens from normal control (NC) (n = 17) and HDM-AR (n = 17) donors. (B–C). POU2F3 and MUC5AC proteins were detected and analyzed in total nasal mucosal cells obtained by nasal swabs from NC (n = 17) and HDM-AR (n = 17) donors (scale bar = 50 μm). (D). Release <t>of</t> <t>IL-25</t> protein in nasal secretions from NC (n = 15) and HDM-AR (n = 15) donors. Data are presented as medians with interquartile ranges. The Mann-Whitney U test was used in (A – D)
Be0394 Dextran Sulfate Sodium Salt, supplied by Bio X Cell, 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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mouse antihuman il 17e mab  (R&D Systems)
90
R&D Systems mouse antihuman il 17e mab
Figure 1. <t>IL-17E</t> promotes skin inflammation and favors the preferential recruitment of neutrophils in vivo. Balb/c mice were intradermally injected with recombinant mouse IL-17E or saline in the back for 2 consecutive days. Skin samples were harvested on day 3. (a) Representative hematoxylin and eosin staining of skin from mice treated with IL-17E or saline (n ¼ 8). Original magnification 10. Scale bar ¼ 50 mm. (b) Profiling of the cellular infiltrate in the skin of saline- (black bars) and IL-17Eeinjected (red bars) mice by flow cytometry. Cumulative data from three independent experiments (n ¼ 8) are presented as absolute counts per cm2. (c) Representative flow cytometry plots of the experiment shown in b. Full-thickness line gates depict cell populations modified by IL- 17E treatment. Pseudocolor scale indicates absolute counts, and numbers in the gates refer to frequency relative to CD45þ cells. (d) Immunofluorescence analysis of skin sections stained for DAPI (blue), Ki67 (green), and cytokeratin 10 (red). Original magnification 40. Scale bar ¼ 20 mm. One representative result is shown (n ¼ 5). White arrows depict Ki-67 positive cells (left panel). Quantitative analysis of Ki67þ cells in the basal layer (n ¼ 5, right panel). (e) Quantitative analysis of the epidermal thickness based on hematoxylin and eosin-stained sections (n ¼ 5). (f) Gene expression analysis was performed using NanoString (Seattle, WA) technology in the skin of mice injected with IL-17E or saline for 3 hours. Volcano plot (left panel) displays differentially expressed genes upon IL-17E treatment. The y-axis corresponds to the mean expression value of log10 P-value, and the x-axis displays the log2 fold change value. The red dots represent the differentially expressed transcripts (threshold > 2 fold change). Heatmap (right panel) of differentially expressed mRNAs in IL-17Eeinjected versus saline (control) group (n ¼ 5). Expression values are colored based on their z-score after normalization across treatments.
Mouse Antihuman Il 17e Mab, 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
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anti il 4  (Biogems International)
94
Biogems International anti il 4
Figure 1. <t>IL-17E</t> promotes skin inflammation and favors the preferential recruitment of neutrophils in vivo. Balb/c mice were intradermally injected with recombinant mouse IL-17E or saline in the back for 2 consecutive days. Skin samples were harvested on day 3. (a) Representative hematoxylin and eosin staining of skin from mice treated with IL-17E or saline (n ¼ 8). Original magnification 10. Scale bar ¼ 50 mm. (b) Profiling of the cellular infiltrate in the skin of saline- (black bars) and IL-17Eeinjected (red bars) mice by flow cytometry. Cumulative data from three independent experiments (n ¼ 8) are presented as absolute counts per cm2. (c) Representative flow cytometry plots of the experiment shown in b. Full-thickness line gates depict cell populations modified by IL- 17E treatment. Pseudocolor scale indicates absolute counts, and numbers in the gates refer to frequency relative to CD45þ cells. (d) Immunofluorescence analysis of skin sections stained for DAPI (blue), Ki67 (green), and cytokeratin 10 (red). Original magnification 40. Scale bar ¼ 20 mm. One representative result is shown (n ¼ 5). White arrows depict Ki-67 positive cells (left panel). Quantitative analysis of Ki67þ cells in the basal layer (n ¼ 5, right panel). (e) Quantitative analysis of the epidermal thickness based on hematoxylin and eosin-stained sections (n ¼ 5). (f) Gene expression analysis was performed using NanoString (Seattle, WA) technology in the skin of mice injected with IL-17E or saline for 3 hours. Volcano plot (left panel) displays differentially expressed genes upon IL-17E treatment. The y-axis corresponds to the mean expression value of log10 P-value, and the x-axis displays the log2 fold change value. The red dots represent the differentially expressed transcripts (threshold > 2 fold change). Heatmap (right panel) of differentially expressed mRNAs in IL-17Eeinjected versus saline (control) group (n ¼ 5). Expression values are colored based on their z-score after normalization across treatments.
Anti Il 4, supplied by Biogems International, 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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il 25 receptor gene  (Santa Cruz Biotechnology)
90
Santa Cruz Biotechnology il 25 receptor gene
Figure 1. <t>IL-17E</t> promotes skin inflammation and favors the preferential recruitment of neutrophils in vivo. Balb/c mice were intradermally injected with recombinant mouse IL-17E or saline in the back for 2 consecutive days. Skin samples were harvested on day 3. (a) Representative hematoxylin and eosin staining of skin from mice treated with IL-17E or saline (n ¼ 8). Original magnification 10. Scale bar ¼ 50 mm. (b) Profiling of the cellular infiltrate in the skin of saline- (black bars) and IL-17Eeinjected (red bars) mice by flow cytometry. Cumulative data from three independent experiments (n ¼ 8) are presented as absolute counts per cm2. (c) Representative flow cytometry plots of the experiment shown in b. Full-thickness line gates depict cell populations modified by IL- 17E treatment. Pseudocolor scale indicates absolute counts, and numbers in the gates refer to frequency relative to CD45þ cells. (d) Immunofluorescence analysis of skin sections stained for DAPI (blue), Ki67 (green), and cytokeratin 10 (red). Original magnification 40. Scale bar ¼ 20 mm. One representative result is shown (n ¼ 5). White arrows depict Ki-67 positive cells (left panel). Quantitative analysis of Ki67þ cells in the basal layer (n ¼ 5, right panel). (e) Quantitative analysis of the epidermal thickness based on hematoxylin and eosin-stained sections (n ¼ 5). (f) Gene expression analysis was performed using NanoString (Seattle, WA) technology in the skin of mice injected with IL-17E or saline for 3 hours. Volcano plot (left panel) displays differentially expressed genes upon IL-17E treatment. The y-axis corresponds to the mean expression value of log10 P-value, and the x-axis displays the log2 fold change value. The red dots represent the differentially expressed transcripts (threshold > 2 fold change). Heatmap (right panel) of differentially expressed mRNAs in IL-17Eeinjected versus saline (control) group (n ¼ 5). Expression values are colored based on their z-score after normalization across treatments.
Il 25 Receptor Gene, supplied by Santa Cruz Biotechnology, 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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anti mouse il 25 pab  (R&D Systems)
92
R&D Systems anti mouse il 25 pab
Figure 1. <t>IL-17E</t> promotes skin inflammation and favors the preferential recruitment of neutrophils in vivo. Balb/c mice were intradermally injected with recombinant mouse IL-17E or saline in the back for 2 consecutive days. Skin samples were harvested on day 3. (a) Representative hematoxylin and eosin staining of skin from mice treated with IL-17E or saline (n ¼ 8). Original magnification 10. Scale bar ¼ 50 mm. (b) Profiling of the cellular infiltrate in the skin of saline- (black bars) and IL-17Eeinjected (red bars) mice by flow cytometry. Cumulative data from three independent experiments (n ¼ 8) are presented as absolute counts per cm2. (c) Representative flow cytometry plots of the experiment shown in b. Full-thickness line gates depict cell populations modified by IL- 17E treatment. Pseudocolor scale indicates absolute counts, and numbers in the gates refer to frequency relative to CD45þ cells. (d) Immunofluorescence analysis of skin sections stained for DAPI (blue), Ki67 (green), and cytokeratin 10 (red). Original magnification 40. Scale bar ¼ 20 mm. One representative result is shown (n ¼ 5). White arrows depict Ki-67 positive cells (left panel). Quantitative analysis of Ki67þ cells in the basal layer (n ¼ 5, right panel). (e) Quantitative analysis of the epidermal thickness based on hematoxylin and eosin-stained sections (n ¼ 5). (f) Gene expression analysis was performed using NanoString (Seattle, WA) technology in the skin of mice injected with IL-17E or saline for 3 hours. Volcano plot (left panel) displays differentially expressed genes upon IL-17E treatment. The y-axis corresponds to the mean expression value of log10 P-value, and the x-axis displays the log2 fold change value. The red dots represent the differentially expressed transcripts (threshold > 2 fold change). Heatmap (right panel) of differentially expressed mRNAs in IL-17Eeinjected versus saline (control) group (n ¼ 5). Expression values are colored based on their z-score after normalization across treatments.
Anti Mouse Il 25 Pab, supplied by R&D Systems, 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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mouse antihuman il 25 antibody  (R&D Systems)
90
R&D Systems mouse antihuman il 25 antibody
Figure 1. <t>IL-17E</t> promotes skin inflammation and favors the preferential recruitment of neutrophils in vivo. Balb/c mice were intradermally injected with recombinant mouse IL-17E or saline in the back for 2 consecutive days. Skin samples were harvested on day 3. (a) Representative hematoxylin and eosin staining of skin from mice treated with IL-17E or saline (n ¼ 8). Original magnification 10. Scale bar ¼ 50 mm. (b) Profiling of the cellular infiltrate in the skin of saline- (black bars) and IL-17Eeinjected (red bars) mice by flow cytometry. Cumulative data from three independent experiments (n ¼ 8) are presented as absolute counts per cm2. (c) Representative flow cytometry plots of the experiment shown in b. Full-thickness line gates depict cell populations modified by IL- 17E treatment. Pseudocolor scale indicates absolute counts, and numbers in the gates refer to frequency relative to CD45þ cells. (d) Immunofluorescence analysis of skin sections stained for DAPI (blue), Ki67 (green), and cytokeratin 10 (red). Original magnification 40. Scale bar ¼ 20 mm. One representative result is shown (n ¼ 5). White arrows depict Ki-67 positive cells (left panel). Quantitative analysis of Ki67þ cells in the basal layer (n ¼ 5, right panel). (e) Quantitative analysis of the epidermal thickness based on hematoxylin and eosin-stained sections (n ¼ 5). (f) Gene expression analysis was performed using NanoString (Seattle, WA) technology in the skin of mice injected with IL-17E or saline for 3 hours. Volcano plot (left panel) displays differentially expressed genes upon IL-17E treatment. The y-axis corresponds to the mean expression value of log10 P-value, and the x-axis displays the log2 fold change value. The red dots represent the differentially expressed transcripts (threshold > 2 fold change). Heatmap (right panel) of differentially expressed mRNAs in IL-17Eeinjected versus saline (control) group (n ¼ 5). Expression values are colored based on their z-score after normalization across treatments.
Mouse Antihuman Il 25 Antibody, 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
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Image Search Results


OTUD6A expression is upregulated in airway epithelial cells in asthma. A‐B) Immunohistochemical (IHC) staining and quantification of OTUD6A in human lung tissues from healthy controls ( n = 2) and asthmatic patients ( n = 2). Scale bars: 100 µm. C‐D) Western blot analysis of OTUD6A expression in lung tissue from HDM‐CAM (C) and HDM‐AAM (D) mice. E‐F) Representative images of IHC for OTUD6A on mouse lung sections of HDM‐CAM and corresponding quantitative analysis ( n = 5). Scale bars: 100 µm. G‐H) Representative images of IHC for OTUD6A on mouse lung sections of HDM‐AAM and corresponding quantitative analysis ( n = 5). Scale bars; 100 µm. I‐J) Immunofluorescence staining for OTUD6A in the mouse lung tissue of HDM‐AAM and corresponding quantitative analysis ( n = 5). Scale bars: 50 µm. K) Western blot analysis of OTUD6A protein levels in BEAS‐2B cells stimulated with HDM (100 µg/mL) at indicated time points ( n = 5). L‐M) BEAS‐2B cells transfected with OTUD6A or control vector for 24 h. L) Western blot analysis of ZO‐1 and Occludin. M) RT‐qPCR analysis of IL‐25 , IL‐33 , and TSLP mRNA levels ( n = 5). N‐O) HBEpiC cells transfected with OTUD6A or control vector for 24 h. N) Western blot analysis of ZO‐1 and Occludin. O) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). P‐Q) HBEpiC cells transfected with siOTUD6A or control vector for 48 h and stimulated with HDM (100 µg/mL) for 6 h. P) Western blot analysis of OTUD6A, ZO‐1, and Occludin. Q) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). Data are presented as mean ± SEM. P values determined by two‐tailed unpaired t‐test or one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Journal: Advanced Science

Article Title: OTUD6A in Airway Epithelial Cells Exacerbates Allergic Asthma by Promoting Airway Inflammation and Airway Remodeling Through Deubiquitination of hResistin/mRELMα

doi: 10.1002/advs.202516355

Figure Lengend Snippet: OTUD6A expression is upregulated in airway epithelial cells in asthma. A‐B) Immunohistochemical (IHC) staining and quantification of OTUD6A in human lung tissues from healthy controls ( n = 2) and asthmatic patients ( n = 2). Scale bars: 100 µm. C‐D) Western blot analysis of OTUD6A expression in lung tissue from HDM‐CAM (C) and HDM‐AAM (D) mice. E‐F) Representative images of IHC for OTUD6A on mouse lung sections of HDM‐CAM and corresponding quantitative analysis ( n = 5). Scale bars: 100 µm. G‐H) Representative images of IHC for OTUD6A on mouse lung sections of HDM‐AAM and corresponding quantitative analysis ( n = 5). Scale bars; 100 µm. I‐J) Immunofluorescence staining for OTUD6A in the mouse lung tissue of HDM‐AAM and corresponding quantitative analysis ( n = 5). Scale bars: 50 µm. K) Western blot analysis of OTUD6A protein levels in BEAS‐2B cells stimulated with HDM (100 µg/mL) at indicated time points ( n = 5). L‐M) BEAS‐2B cells transfected with OTUD6A or control vector for 24 h. L) Western blot analysis of ZO‐1 and Occludin. M) RT‐qPCR analysis of IL‐25 , IL‐33 , and TSLP mRNA levels ( n = 5). N‐O) HBEpiC cells transfected with OTUD6A or control vector for 24 h. N) Western blot analysis of ZO‐1 and Occludin. O) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). P‐Q) HBEpiC cells transfected with siOTUD6A or control vector for 48 h and stimulated with HDM (100 µg/mL) for 6 h. P) Western blot analysis of OTUD6A, ZO‐1, and Occludin. Q) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). Data are presented as mean ± SEM. P values determined by two‐tailed unpaired t‐test or one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Article Snippet: Human IL‐25 (Cat# E‐EL‐H1648)/IL‐33 (E‐EL‐H2402)/TSLP (Cat# E‐EL‐H1598)/Resistin (Cat# E‐EL‐H1213) ELISA kits, and mouse IL‐25 (Cat# E‐EL‐M0187)/IL‐33 (Cat# E‐EL‐M2642)/TSLP (Cat# E‐EL‐M0642) ELISA kits were purchased from Elabscience (Wuhan, China).

Techniques: Expressing, Immunohistochemical staining, Immunohistochemistry, Western Blot, Immunofluorescence, Staining, Transfection, Control, Plasmid Preparation, Quantitative RT-PCR, Enzyme-linked Immunosorbent Assay, Two Tailed Test

OTUD6A knockout alleviates asthma in HDM‐induced acute asthma model. A) Schematic diagram depicting the procedure of HDM‐AAM. B) AHR assessed via acetylcholine challenge ( n = 5). C) Serum IgE levels measured by ELISA ( n = 5). D) Representative H&E and PAS staining of lung tissue. Scale bars: 100 µm. E) Quantification of bronchial epithelial thickness ( n = 5). F) BALF eosinophil counts determined by Wright‐Giemsa staining ( n = 5). G‐J) IL‐5 and IL‐13 levels in BALF (G, H) and lung homogenates (I, J) measured by ELISA ( n = 5). K‐N) RT‐qPCR analysis of Il5 , Il13 , Muc5ac , and Muc5b mRNA levels in lung tissue ( n = 5). O) ELISA analysis of IL‐25, IL‐33, and TSLP levels in BALF ( n = 5). P) Western blot and quantification of ZO‐1 and Occludin in lung tissues. Data are presented as mean ± SEM. P values determined by one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Journal: Advanced Science

Article Title: OTUD6A in Airway Epithelial Cells Exacerbates Allergic Asthma by Promoting Airway Inflammation and Airway Remodeling Through Deubiquitination of hResistin/mRELMα

doi: 10.1002/advs.202516355

Figure Lengend Snippet: OTUD6A knockout alleviates asthma in HDM‐induced acute asthma model. A) Schematic diagram depicting the procedure of HDM‐AAM. B) AHR assessed via acetylcholine challenge ( n = 5). C) Serum IgE levels measured by ELISA ( n = 5). D) Representative H&E and PAS staining of lung tissue. Scale bars: 100 µm. E) Quantification of bronchial epithelial thickness ( n = 5). F) BALF eosinophil counts determined by Wright‐Giemsa staining ( n = 5). G‐J) IL‐5 and IL‐13 levels in BALF (G, H) and lung homogenates (I, J) measured by ELISA ( n = 5). K‐N) RT‐qPCR analysis of Il5 , Il13 , Muc5ac , and Muc5b mRNA levels in lung tissue ( n = 5). O) ELISA analysis of IL‐25, IL‐33, and TSLP levels in BALF ( n = 5). P) Western blot and quantification of ZO‐1 and Occludin in lung tissues. Data are presented as mean ± SEM. P values determined by one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Article Snippet: Human IL‐25 (Cat# E‐EL‐H1648)/IL‐33 (E‐EL‐H2402)/TSLP (Cat# E‐EL‐H1598)/Resistin (Cat# E‐EL‐H1213) ELISA kits, and mouse IL‐25 (Cat# E‐EL‐M0187)/IL‐33 (Cat# E‐EL‐M2642)/TSLP (Cat# E‐EL‐M0642) ELISA kits were purchased from Elabscience (Wuhan, China).

Techniques: Knock-Out, Enzyme-linked Immunosorbent Assay, Staining, Quantitative RT-PCR, Western Blot

OTUD6A knockout mitigates asthma in HDM‐induced chronic asthma model. A) Schematic diagram depicting the procedure of HDM‐CAM. B‐D) Rn, Ers, and Rrs assessed via methacholine challenge ( n = 5). E) Representative H&E staining of lung tissue. Scale bars: 100 µm. F) Serum IgE levels measured by ELISA ( n = 5). G‐H) Total cell counts (G) and protein concentration (H) in BALF ( n = 5). I‐L) IL‐5 and IL‐13 levels in BALF (I, J) and lung homogenates (K, L) measured by ELISA ( n = 5). M‐R) RT‐qPCR analysis of Il5 , Il13 , Muc5ac , Tslp , Il25 , and Il33 mRNA level in lung tissues ( n = 5). S‐U) ELISA analysis of IL‐25, IL‐33, and TSLP levels in BALF ( n = 5). Data are presented as mean ± SEM. P values determined by one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Journal: Advanced Science

Article Title: OTUD6A in Airway Epithelial Cells Exacerbates Allergic Asthma by Promoting Airway Inflammation and Airway Remodeling Through Deubiquitination of hResistin/mRELMα

doi: 10.1002/advs.202516355

Figure Lengend Snippet: OTUD6A knockout mitigates asthma in HDM‐induced chronic asthma model. A) Schematic diagram depicting the procedure of HDM‐CAM. B‐D) Rn, Ers, and Rrs assessed via methacholine challenge ( n = 5). E) Representative H&E staining of lung tissue. Scale bars: 100 µm. F) Serum IgE levels measured by ELISA ( n = 5). G‐H) Total cell counts (G) and protein concentration (H) in BALF ( n = 5). I‐L) IL‐5 and IL‐13 levels in BALF (I, J) and lung homogenates (K, L) measured by ELISA ( n = 5). M‐R) RT‐qPCR analysis of Il5 , Il13 , Muc5ac , Tslp , Il25 , and Il33 mRNA level in lung tissues ( n = 5). S‐U) ELISA analysis of IL‐25, IL‐33, and TSLP levels in BALF ( n = 5). Data are presented as mean ± SEM. P values determined by one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Article Snippet: Human IL‐25 (Cat# E‐EL‐H1648)/IL‐33 (E‐EL‐H2402)/TSLP (Cat# E‐EL‐H1598)/Resistin (Cat# E‐EL‐H1213) ELISA kits, and mouse IL‐25 (Cat# E‐EL‐M0187)/IL‐33 (Cat# E‐EL‐M2642)/TSLP (Cat# E‐EL‐M0642) ELISA kits were purchased from Elabscience (Wuhan, China).

Techniques: Knock-Out, Staining, Enzyme-linked Immunosorbent Assay, Protein Concentration, Quantitative RT-PCR

hResistin/PI3K mediates OTUD6A‐induced EMT process and the expression of epithelial‐derived alarmins. A‐G) BEAS‐2B cells transfected with siResistin for 48 h and then transfected with Flag‐OTUD6A for 24 h. A) RT‐qPCR analysis of TSLP , IL‐25 , IL‐33 mRNA level in BEAS‐2B cells ( n = 5). B) ELISA analysis of TSLP, IL‐25, and IL‐33 levels in cell supernatant ( n = 5). C) RT‐qPCR analysis of TGFB1 , ACTA2 , COL1A1 mRNA level in BEAS‐2B cells ( n = 5). D‐E) Western blot analysis of OTUD6A, hResistin, EMT, and PI3K/AKT markers. F) Immunofluorescence staining of E‐cadherin and N‐cadherin. Scale bars: 50 µm. G) Cell wound healing assay. Scale bars: 50 µm. H‐K) BEAS‐2B cells were pretreated with LY294002 (30 µ m ) for 30 min and transfected with Flag‐OTUD6A for 24 h. H) Western blot analysis of hResistin and EMT markers. I‐K) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). Data are presented as mean ± SEM. P values determined by one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Journal: Advanced Science

Article Title: OTUD6A in Airway Epithelial Cells Exacerbates Allergic Asthma by Promoting Airway Inflammation and Airway Remodeling Through Deubiquitination of hResistin/mRELMα

doi: 10.1002/advs.202516355

Figure Lengend Snippet: hResistin/PI3K mediates OTUD6A‐induced EMT process and the expression of epithelial‐derived alarmins. A‐G) BEAS‐2B cells transfected with siResistin for 48 h and then transfected with Flag‐OTUD6A for 24 h. A) RT‐qPCR analysis of TSLP , IL‐25 , IL‐33 mRNA level in BEAS‐2B cells ( n = 5). B) ELISA analysis of TSLP, IL‐25, and IL‐33 levels in cell supernatant ( n = 5). C) RT‐qPCR analysis of TGFB1 , ACTA2 , COL1A1 mRNA level in BEAS‐2B cells ( n = 5). D‐E) Western blot analysis of OTUD6A, hResistin, EMT, and PI3K/AKT markers. F) Immunofluorescence staining of E‐cadherin and N‐cadherin. Scale bars: 50 µm. G) Cell wound healing assay. Scale bars: 50 µm. H‐K) BEAS‐2B cells were pretreated with LY294002 (30 µ m ) for 30 min and transfected with Flag‐OTUD6A for 24 h. H) Western blot analysis of hResistin and EMT markers. I‐K) ELISA analysis of IL‐33, IL‐25, and TSLP levels in cell supernatant ( n = 5). Data are presented as mean ± SEM. P values determined by one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Article Snippet: Human IL‐25 (Cat# E‐EL‐H1648)/IL‐33 (E‐EL‐H2402)/TSLP (Cat# E‐EL‐H1598)/Resistin (Cat# E‐EL‐H1213) ELISA kits, and mouse IL‐25 (Cat# E‐EL‐M0187)/IL‐33 (Cat# E‐EL‐M2642)/TSLP (Cat# E‐EL‐M0642) ELISA kits were purchased from Elabscience (Wuhan, China).

Techniques: Expressing, Derivative Assay, Transfection, Quantitative RT-PCR, Enzyme-linked Immunosorbent Assay, Western Blot, Immunofluorescence, Staining, Wound Healing Assay

Lung‐specific OTUD6A knockdown attenuates HDM‐induced asthma. A) Schematic diagram depicting the procedure of HDM‐induced chronic asthma model. B) Western blot analysis of OTUD6A and mRELMα in lung tissues. C) AHR assessed via acetylcholine challenge ( n = 5). D) H&E staining of lung tissues. Scale bars: 100 µm. E) Serum IgE levels measured by ELISA ( n = 5). F‐G) Total cell counts (F) and protein concentration (G) in BALF ( n = 5). H‐I) IL‐5 (H) and IL‐13 (I) levels in BALF measured by ELISA ( n = 5). J‐L) RT‐qPCR analysis of Il4, Il5 , and Muc5ac mRNA levels in lung tissues ( n = 5). M) ELISA analysis of IL‐25, IL‐33, and TSLP levels in BALF (n = 5). N) Serum TGF‐β1 levels measured by ELISA ( n = 5). O) Masson's trichrome staining of lung sections. Scale bars: 100 µm. P) RT‐qPCR analysis of Tgfb1 , Acta2 , and Col1a1 mRNA levels in lung tissues ( n = 5). Q) Western blot analysis of Vimentin, TGFβ1, α‐SMA, and Fibronectin in the lung tissues. R) Western blot analysis of PI3K/AKT in the lung tissues. S) Western blot analysis of EMT markers in the lung tissues. Data are presented as mean ± SEM. P values determined by one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Journal: Advanced Science

Article Title: OTUD6A in Airway Epithelial Cells Exacerbates Allergic Asthma by Promoting Airway Inflammation and Airway Remodeling Through Deubiquitination of hResistin/mRELMα

doi: 10.1002/advs.202516355

Figure Lengend Snippet: Lung‐specific OTUD6A knockdown attenuates HDM‐induced asthma. A) Schematic diagram depicting the procedure of HDM‐induced chronic asthma model. B) Western blot analysis of OTUD6A and mRELMα in lung tissues. C) AHR assessed via acetylcholine challenge ( n = 5). D) H&E staining of lung tissues. Scale bars: 100 µm. E) Serum IgE levels measured by ELISA ( n = 5). F‐G) Total cell counts (F) and protein concentration (G) in BALF ( n = 5). H‐I) IL‐5 (H) and IL‐13 (I) levels in BALF measured by ELISA ( n = 5). J‐L) RT‐qPCR analysis of Il4, Il5 , and Muc5ac mRNA levels in lung tissues ( n = 5). M) ELISA analysis of IL‐25, IL‐33, and TSLP levels in BALF (n = 5). N) Serum TGF‐β1 levels measured by ELISA ( n = 5). O) Masson's trichrome staining of lung sections. Scale bars: 100 µm. P) RT‐qPCR analysis of Tgfb1 , Acta2 , and Col1a1 mRNA levels in lung tissues ( n = 5). Q) Western blot analysis of Vimentin, TGFβ1, α‐SMA, and Fibronectin in the lung tissues. R) Western blot analysis of PI3K/AKT in the lung tissues. S) Western blot analysis of EMT markers in the lung tissues. Data are presented as mean ± SEM. P values determined by one‐way ANOVA (* p < 0.05, ** p < 0.01, *** p < 0.001).

Article Snippet: Human IL‐25 (Cat# E‐EL‐H1648)/IL‐33 (E‐EL‐H2402)/TSLP (Cat# E‐EL‐H1598)/Resistin (Cat# E‐EL‐H1213) ELISA kits, and mouse IL‐25 (Cat# E‐EL‐M0187)/IL‐33 (Cat# E‐EL‐M2642)/TSLP (Cat# E‐EL‐M0642) ELISA kits were purchased from Elabscience (Wuhan, China).

Techniques: Knockdown, Western Blot, Staining, Enzyme-linked Immunosorbent Assay, Protein Concentration, Quantitative RT-PCR

Aberrant SCC and goblet cell hyperplasia phenotype in nasal mucosa from patients with HDM-AR (A). POU2F3, DCAMKL1 and MUC5AC mRNA levels in nasal swab specimens from normal control (NC) (n = 17) and HDM-AR (n = 17) donors. (B–C). POU2F3 and MUC5AC proteins were detected and analyzed in total nasal mucosal cells obtained by nasal swabs from NC (n = 17) and HDM-AR (n = 17) donors (scale bar = 50 μm). (D). Release of IL-25 protein in nasal secretions from NC (n = 15) and HDM-AR (n = 15) donors. Data are presented as medians with interquartile ranges. The Mann-Whitney U test was used in (A – D)

Journal: The World Allergy Organization Journal

Article Title: Solitary chemosensory cells amplify eosinophilic inflammation via PAR-2 activation in house dust mite-sensitized allergic rhinitis

doi: 10.1016/j.waojou.2026.101336

Figure Lengend Snippet: Aberrant SCC and goblet cell hyperplasia phenotype in nasal mucosa from patients with HDM-AR (A). POU2F3, DCAMKL1 and MUC5AC mRNA levels in nasal swab specimens from normal control (NC) (n = 17) and HDM-AR (n = 17) donors. (B–C). POU2F3 and MUC5AC proteins were detected and analyzed in total nasal mucosal cells obtained by nasal swabs from NC (n = 17) and HDM-AR (n = 17) donors (scale bar = 50 μm). (D). Release of IL-25 protein in nasal secretions from NC (n = 15) and HDM-AR (n = 15) donors. Data are presented as medians with interquartile ranges. The Mann-Whitney U test was used in (A – D)

Article Snippet: Human IL-25 protein levels in nasal secretions and supernatants for hNECs collected from the apical chambers of the ALI culture system were measured with an ELISA kit (BosterBio, Pleasanton, CA, USA) following the manufacturer's instructions.

Techniques: Control, MANN-WHITNEY

Derp induces SCC expansion and IL-25 overproduction in cultured hNECs. (A). POU2F3, DCAMKL1 and MUC5AC mRNA levels were detected in Derp and NT group of hNECs. (B–C). POU2F3 and MUC5AC proteins were detected and compared in hNECs from the Derp group and NT group by immunofluorescence staining (scale bar = 50 μm). (D – E). POU2F3, DCAMKL1 and IL-25 proteins were detected and compared in hNECs from the Derp and NT group by Western blot analysis. (F). Release of IL-25 protein in hNEC supernatants from the Derp and NT group. The experiments were performed in hNECs from 3 different donors. Data are presented as mean ± SD. The paired Student t-test was performed in (A) , (E) and (F) ; the unpaired Student t-test was used for comparison analysis in (C)

Journal: The World Allergy Organization Journal

Article Title: Solitary chemosensory cells amplify eosinophilic inflammation via PAR-2 activation in house dust mite-sensitized allergic rhinitis

doi: 10.1016/j.waojou.2026.101336

Figure Lengend Snippet: Derp induces SCC expansion and IL-25 overproduction in cultured hNECs. (A). POU2F3, DCAMKL1 and MUC5AC mRNA levels were detected in Derp and NT group of hNECs. (B–C). POU2F3 and MUC5AC proteins were detected and compared in hNECs from the Derp group and NT group by immunofluorescence staining (scale bar = 50 μm). (D – E). POU2F3, DCAMKL1 and IL-25 proteins were detected and compared in hNECs from the Derp and NT group by Western blot analysis. (F). Release of IL-25 protein in hNEC supernatants from the Derp and NT group. The experiments were performed in hNECs from 3 different donors. Data are presented as mean ± SD. The paired Student t-test was performed in (A) , (E) and (F) ; the unpaired Student t-test was used for comparison analysis in (C)

Article Snippet: Human IL-25 protein levels in nasal secretions and supernatants for hNECs collected from the apical chambers of the ALI culture system were measured with an ELISA kit (BosterBio, Pleasanton, CA, USA) following the manufacturer's instructions.

Techniques: Cell Culture, Immunofluorescence, Staining, Western Blot, Comparison

IL-25 triggers mucin production in hNECs and promoted the expression of IL-25 receptors in eosinophils in hNMCs. (A – B). MUC5AC protein was detected and anaylzed in human recombinant IL-25 protein -treated hNECs (n = 3) versus NT group (n = 3) by immunofluorescence staining (scale bar = 50 μm). (C). Proportion of CD45 + CD16 − Siglec-8 + IL-17RA + IL-17RB + eosinophils in human IL-25-treated hNMCs (n = 5) or NT group (n = 5) measured by flow cytometry. Data are presented as mean ± SD. The unpaired Student t-test was performed in (B) . The paired Student t-test was used in (C) . ns, not significant

Journal: The World Allergy Organization Journal

Article Title: Solitary chemosensory cells amplify eosinophilic inflammation via PAR-2 activation in house dust mite-sensitized allergic rhinitis

doi: 10.1016/j.waojou.2026.101336

Figure Lengend Snippet: IL-25 triggers mucin production in hNECs and promoted the expression of IL-25 receptors in eosinophils in hNMCs. (A – B). MUC5AC protein was detected and anaylzed in human recombinant IL-25 protein -treated hNECs (n = 3) versus NT group (n = 3) by immunofluorescence staining (scale bar = 50 μm). (C). Proportion of CD45 + CD16 − Siglec-8 + IL-17RA + IL-17RB + eosinophils in human IL-25-treated hNMCs (n = 5) or NT group (n = 5) measured by flow cytometry. Data are presented as mean ± SD. The unpaired Student t-test was performed in (B) . The paired Student t-test was used in (C) . ns, not significant

Article Snippet: Human IL-25 protein levels in nasal secretions and supernatants for hNECs collected from the apical chambers of the ALI culture system were measured with an ELISA kit (BosterBio, Pleasanton, CA, USA) following the manufacturer's instructions.

Techniques: Expressing, Recombinant, Immunofluorescence, Staining, Flow Cytometry

Derp promotes SCC expansion and mucin overproduction in hNECs in a PAR-2-dependent way. (A). PAR-2 mRNA level in Derp-treated and nontreated (NT) hNECs. (B). PAR-2 protein was analyzed in hNECs from Derp group versus NT group by Western-blot analysis. (C). POU2F3, DCAMKL1 and MUC5AC mRNA levels in NT, Derp-treated and Derp + AZ3451 (AZ)-treated hNECs. (D). POU2F3 and MUC5AC proteins detected and compared in hNECs from NT, Derp and Derp + AZ groups by immunofluorescence staining (scale bar = 50 μm). (E – F). POU2F3, DCAMKL1 and IL-25 proteins were detected and compared in hNECs from NT, Derp and Derp + AZ groups by Western-blot analysis. (G). Release of IL-25 protein in hNEC supernatants from NT, Derp and Derp + AZ groups. The experiments were performed in hNECs from 3 different donors. Data are presented as mean ± SD. The paired Student t-test was performed in (A) , (B) , (C) , (F) and (G) ; the unpaired Student t-test was used in (D) . ns, not significant

Journal: The World Allergy Organization Journal

Article Title: Solitary chemosensory cells amplify eosinophilic inflammation via PAR-2 activation in house dust mite-sensitized allergic rhinitis

doi: 10.1016/j.waojou.2026.101336

Figure Lengend Snippet: Derp promotes SCC expansion and mucin overproduction in hNECs in a PAR-2-dependent way. (A). PAR-2 mRNA level in Derp-treated and nontreated (NT) hNECs. (B). PAR-2 protein was analyzed in hNECs from Derp group versus NT group by Western-blot analysis. (C). POU2F3, DCAMKL1 and MUC5AC mRNA levels in NT, Derp-treated and Derp + AZ3451 (AZ)-treated hNECs. (D). POU2F3 and MUC5AC proteins detected and compared in hNECs from NT, Derp and Derp + AZ groups by immunofluorescence staining (scale bar = 50 μm). (E – F). POU2F3, DCAMKL1 and IL-25 proteins were detected and compared in hNECs from NT, Derp and Derp + AZ groups by Western-blot analysis. (G). Release of IL-25 protein in hNEC supernatants from NT, Derp and Derp + AZ groups. The experiments were performed in hNECs from 3 different donors. Data are presented as mean ± SD. The paired Student t-test was performed in (A) , (B) , (C) , (F) and (G) ; the unpaired Student t-test was used in (D) . ns, not significant

Article Snippet: Human IL-25 protein levels in nasal secretions and supernatants for hNECs collected from the apical chambers of the ALI culture system were measured with an ELISA kit (BosterBio, Pleasanton, CA, USA) following the manufacturer's instructions.

Techniques: Western Blot, Immunofluorescence, Staining

HDM stimulated the secretion of IL-25 and promoted the expression of IL-25 receptors in eosinophils in hNMCs. (A). Release of IL-25 protein was detected by ELISA assay in hNMC supernatants from NT (n = 5), Derp (n = 5) and Derp + AZ (n = 5) groups. (B). Proportion of CD45 + CD16 − Siglec-8 + IL-17RA + IL-17RB + eosinophils in hNMCs from NT (n = 5), Derp (n = 5) and Derp + AZ (n = 5) groups by flow cytometry. Data are presented as mean ± SD. The paired Student t-test was used in (A) and (B) . ns, not significant

Journal: The World Allergy Organization Journal

Article Title: Solitary chemosensory cells amplify eosinophilic inflammation via PAR-2 activation in house dust mite-sensitized allergic rhinitis

doi: 10.1016/j.waojou.2026.101336

Figure Lengend Snippet: HDM stimulated the secretion of IL-25 and promoted the expression of IL-25 receptors in eosinophils in hNMCs. (A). Release of IL-25 protein was detected by ELISA assay in hNMC supernatants from NT (n = 5), Derp (n = 5) and Derp + AZ (n = 5) groups. (B). Proportion of CD45 + CD16 − Siglec-8 + IL-17RA + IL-17RB + eosinophils in hNMCs from NT (n = 5), Derp (n = 5) and Derp + AZ (n = 5) groups by flow cytometry. Data are presented as mean ± SD. The paired Student t-test was used in (A) and (B) . ns, not significant

Article Snippet: Human IL-25 protein levels in nasal secretions and supernatants for hNECs collected from the apical chambers of the ALI culture system were measured with an ELISA kit (BosterBio, Pleasanton, CA, USA) following the manufacturer's instructions.

Techniques: Expressing, Enzyme-linked Immunosorbent Assay, Flow Cytometry

Figure 1. IL-17E promotes skin inflammation and favors the preferential recruitment of neutrophils in vivo. Balb/c mice were intradermally injected with recombinant mouse IL-17E or saline in the back for 2 consecutive days. Skin samples were harvested on day 3. (a) Representative hematoxylin and eosin staining of skin from mice treated with IL-17E or saline (n ¼ 8). Original magnification 10. Scale bar ¼ 50 mm. (b) Profiling of the cellular infiltrate in the skin of saline- (black bars) and IL-17Eeinjected (red bars) mice by flow cytometry. Cumulative data from three independent experiments (n ¼ 8) are presented as absolute counts per cm2. (c) Representative flow cytometry plots of the experiment shown in b. Full-thickness line gates depict cell populations modified by IL- 17E treatment. Pseudocolor scale indicates absolute counts, and numbers in the gates refer to frequency relative to CD45þ cells. (d) Immunofluorescence analysis of skin sections stained for DAPI (blue), Ki67 (green), and cytokeratin 10 (red). Original magnification 40. Scale bar ¼ 20 mm. One representative result is shown (n ¼ 5). White arrows depict Ki-67 positive cells (left panel). Quantitative analysis of Ki67þ cells in the basal layer (n ¼ 5, right panel). (e) Quantitative analysis of the epidermal thickness based on hematoxylin and eosin-stained sections (n ¼ 5). (f) Gene expression analysis was performed using NanoString (Seattle, WA) technology in the skin of mice injected with IL-17E or saline for 3 hours. Volcano plot (left panel) displays differentially expressed genes upon IL-17E treatment. The y-axis corresponds to the mean expression value of log10 P-value, and the x-axis displays the log2 fold change value. The red dots represent the differentially expressed transcripts (threshold > 2 fold change). Heatmap (right panel) of differentially expressed mRNAs in IL-17Eeinjected versus saline (control) group (n ¼ 5). Expression values are colored based on their z-score after normalization across treatments.

Journal: The Journal of investigative dermatology

Article Title: IL-17E (IL-25) Enhances Innate Immune Responses during Skin Inflammation.

doi: 10.1016/j.jid.2019.01.021

Figure Lengend Snippet: Figure 1. IL-17E promotes skin inflammation and favors the preferential recruitment of neutrophils in vivo. Balb/c mice were intradermally injected with recombinant mouse IL-17E or saline in the back for 2 consecutive days. Skin samples were harvested on day 3. (a) Representative hematoxylin and eosin staining of skin from mice treated with IL-17E or saline (n ¼ 8). Original magnification 10. Scale bar ¼ 50 mm. (b) Profiling of the cellular infiltrate in the skin of saline- (black bars) and IL-17Eeinjected (red bars) mice by flow cytometry. Cumulative data from three independent experiments (n ¼ 8) are presented as absolute counts per cm2. (c) Representative flow cytometry plots of the experiment shown in b. Full-thickness line gates depict cell populations modified by IL- 17E treatment. Pseudocolor scale indicates absolute counts, and numbers in the gates refer to frequency relative to CD45þ cells. (d) Immunofluorescence analysis of skin sections stained for DAPI (blue), Ki67 (green), and cytokeratin 10 (red). Original magnification 40. Scale bar ¼ 20 mm. One representative result is shown (n ¼ 5). White arrows depict Ki-67 positive cells (left panel). Quantitative analysis of Ki67þ cells in the basal layer (n ¼ 5, right panel). (e) Quantitative analysis of the epidermal thickness based on hematoxylin and eosin-stained sections (n ¼ 5). (f) Gene expression analysis was performed using NanoString (Seattle, WA) technology in the skin of mice injected with IL-17E or saline for 3 hours. Volcano plot (left panel) displays differentially expressed genes upon IL-17E treatment. The y-axis corresponds to the mean expression value of log10 P-value, and the x-axis displays the log2 fold change value. The red dots represent the differentially expressed transcripts (threshold > 2 fold change). Heatmap (right panel) of differentially expressed mRNAs in IL-17Eeinjected versus saline (control) group (n ¼ 5). Expression values are colored based on their z-score after normalization across treatments.

Article Snippet: Mouse antihuman IL-17E mAb (clone 182293) and polyclonal goat anti-human myeloperoxidase antibody were from R&D Systems, rabbit anti-human cytokeratin 10 was from BioSB (Santa Barbara, CA), and rat anti-mouse Ki67 mAb (clone 16A8) and rat anti-mouse Ly6G (clone 1A8) were from Biolegend.

Techniques: In Vivo, Injection, Recombinant, Saline, Staining, Cytometry, Gene Expression, Expressing, Control

Figure 3. IL-17E neutralization through blocking antibodies ameliorates imiquimod-induced skin inflammation. Wild-type balb/c mice were treated with imiquimod for 3 consecutive days on the shaved back skin and one ear. Next, 100 mg of neutralizing IL-17E antibody or isotype control were injected intraperitoneally1 day before the first application and 1 hour before every application. Skin and ear tissue samples were harvested on day 4. (a) Daily body weight variation and percentage of increase in ear swelling expressed as mean standard error of the mean (n ¼ 5). (b) Representative hematoxylin and eosin staining of the back skin and quantitative analysis of the epidermal thickness of imiquimod-treated mice injected with anti-IL-17E (n ¼ 11) or isotype control

Journal: The Journal of investigative dermatology

Article Title: IL-17E (IL-25) Enhances Innate Immune Responses during Skin Inflammation.

doi: 10.1016/j.jid.2019.01.021

Figure Lengend Snippet: Figure 3. IL-17E neutralization through blocking antibodies ameliorates imiquimod-induced skin inflammation. Wild-type balb/c mice were treated with imiquimod for 3 consecutive days on the shaved back skin and one ear. Next, 100 mg of neutralizing IL-17E antibody or isotype control were injected intraperitoneally1 day before the first application and 1 hour before every application. Skin and ear tissue samples were harvested on day 4. (a) Daily body weight variation and percentage of increase in ear swelling expressed as mean standard error of the mean (n ¼ 5). (b) Representative hematoxylin and eosin staining of the back skin and quantitative analysis of the epidermal thickness of imiquimod-treated mice injected with anti-IL-17E (n ¼ 11) or isotype control

Article Snippet: Mouse antihuman IL-17E mAb (clone 182293) and polyclonal goat anti-human myeloperoxidase antibody were from R&D Systems, rabbit anti-human cytokeratin 10 was from BioSB (Santa Barbara, CA), and rat anti-mouse Ki67 mAb (clone 16A8) and rat anti-mouse Ly6G (clone 1A8) were from Biolegend.

Techniques: Neutralization, Blocking Assay, Control, Injection, Staining

Figure 4. IL-17E neutralization affects innate immune cell infiltration during imiquimod-induced skin inflammation. Experimental condition, as in Figure 4. (a) Visualized t-SNE map of cells isolated from the skin of mice treated with imiquimod. Clusters (cell populations) were identified by manual gating. One representative result of each group is shown (n ¼ 10 for isotype control group; n ¼ 11 for a-IL-17E-treated group). (b) Based on clusters identified in a, median intensities for each marker were calculated and plotted as a heatmap. (c, d) Histogram showing the mean fluorescence intensity of the indicated markers in each cell cluster (c) belonging to the NK population (clusters 1e3) or (d) belonging to the neutrophil population (clusters 10 to 13) in the anti-IL-17E treated group. max, maximum; NK, natural killer; t-SNE, t-distributed stochastic neighbor embedding.

Journal: The Journal of investigative dermatology

Article Title: IL-17E (IL-25) Enhances Innate Immune Responses during Skin Inflammation.

doi: 10.1016/j.jid.2019.01.021

Figure Lengend Snippet: Figure 4. IL-17E neutralization affects innate immune cell infiltration during imiquimod-induced skin inflammation. Experimental condition, as in Figure 4. (a) Visualized t-SNE map of cells isolated from the skin of mice treated with imiquimod. Clusters (cell populations) were identified by manual gating. One representative result of each group is shown (n ¼ 10 for isotype control group; n ¼ 11 for a-IL-17E-treated group). (b) Based on clusters identified in a, median intensities for each marker were calculated and plotted as a heatmap. (c, d) Histogram showing the mean fluorescence intensity of the indicated markers in each cell cluster (c) belonging to the NK population (clusters 1e3) or (d) belonging to the neutrophil population (clusters 10 to 13) in the anti-IL-17E treated group. max, maximum; NK, natural killer; t-SNE, t-distributed stochastic neighbor embedding.

Article Snippet: Mouse antihuman IL-17E mAb (clone 182293) and polyclonal goat anti-human myeloperoxidase antibody were from R&D Systems, rabbit anti-human cytokeratin 10 was from BioSB (Santa Barbara, CA), and rat anti-mouse Ki67 mAb (clone 16A8) and rat anti-mouse Ly6G (clone 1A8) were from Biolegend.

Techniques: Neutralization, Isolation, Control, Marker

Figure 5. IL-17E promotes the recruitment of human neutrophils via activation of macrophages in a p38-dependent mechanism. (a) mRNA level of human IL-8 (left panel) and murine Cxcl1 and Cxcl2 (right panel) in IL-17Eetreated M2 macrophages from humans and mice, respectively. (b) IL-8 levels as assessed by ELISA in supernatants of primary keratinocytes (n ¼ 4) cultured in the presence of IL-17E or TNF (right panel). (c) mRNA levels assessed by quantitative PCR in M2 polarized macrophages pretreated for 30 minutes with a p38 MAPK (SB202190) or NF-kB inhibitor (JSH 23) and then stimulated with IL-17E for a further 6 hours. mRNA levels relative to the untreated condition are shown as mean standard error of the mean (n 5). (d) Immunoblotting analysis of M2 polarized macrophages stimulated with 100 ng/ml of IL-17E for the indicated time points (n ¼ 5, one representative result is shown). (e) Neutrophil migration induced by IL-8 (50 ng/ml) or IL-17E (100 ng/ml) in a classic Transwell assay (Nunc, Roskilde, Denmark) (left panel). M2 macrophages were left unstimulated (unstim.) or treated with IL-17E in the presence or not of SB202190 for 24 hours. Supernatants were retrieved and used to assess neutrophil migration. IL-8 neutralizing antibodies were added to the conditioned media of macrophages stimulated with IL-17E 30 minutes before assessing chemotaxis. Data from one representative experiment are expressed as relative to control media and presented as the mean standard error of the mean (n ¼ 3). (f) IL-8 protein levels assessed by ELISA in supernatants of M2 polarized macrophages. The protein levels relative to untreated condition are shown as mean standard error of the mean (n 5). Significant differences were assessed by Wilcoxon signed rank test. *P ¼ 0.01 to 0.05. Ctrl, control; min, minute; p-, phosphorylated.

Journal: The Journal of investigative dermatology

Article Title: IL-17E (IL-25) Enhances Innate Immune Responses during Skin Inflammation.

doi: 10.1016/j.jid.2019.01.021

Figure Lengend Snippet: Figure 5. IL-17E promotes the recruitment of human neutrophils via activation of macrophages in a p38-dependent mechanism. (a) mRNA level of human IL-8 (left panel) and murine Cxcl1 and Cxcl2 (right panel) in IL-17Eetreated M2 macrophages from humans and mice, respectively. (b) IL-8 levels as assessed by ELISA in supernatants of primary keratinocytes (n ¼ 4) cultured in the presence of IL-17E or TNF (right panel). (c) mRNA levels assessed by quantitative PCR in M2 polarized macrophages pretreated for 30 minutes with a p38 MAPK (SB202190) or NF-kB inhibitor (JSH 23) and then stimulated with IL-17E for a further 6 hours. mRNA levels relative to the untreated condition are shown as mean standard error of the mean (n 5). (d) Immunoblotting analysis of M2 polarized macrophages stimulated with 100 ng/ml of IL-17E for the indicated time points (n ¼ 5, one representative result is shown). (e) Neutrophil migration induced by IL-8 (50 ng/ml) or IL-17E (100 ng/ml) in a classic Transwell assay (Nunc, Roskilde, Denmark) (left panel). M2 macrophages were left unstimulated (unstim.) or treated with IL-17E in the presence or not of SB202190 for 24 hours. Supernatants were retrieved and used to assess neutrophil migration. IL-8 neutralizing antibodies were added to the conditioned media of macrophages stimulated with IL-17E 30 minutes before assessing chemotaxis. Data from one representative experiment are expressed as relative to control media and presented as the mean standard error of the mean (n ¼ 3). (f) IL-8 protein levels assessed by ELISA in supernatants of M2 polarized macrophages. The protein levels relative to untreated condition are shown as mean standard error of the mean (n 5). Significant differences were assessed by Wilcoxon signed rank test. *P ¼ 0.01 to 0.05. Ctrl, control; min, minute; p-, phosphorylated.

Article Snippet: Mouse antihuman IL-17E mAb (clone 182293) and polyclonal goat anti-human myeloperoxidase antibody were from R&D Systems, rabbit anti-human cytokeratin 10 was from BioSB (Santa Barbara, CA), and rat anti-mouse Ki67 mAb (clone 16A8) and rat anti-mouse Ly6G (clone 1A8) were from Biolegend.

Techniques: Activation Assay, Enzyme-linked Immunosorbent Assay, Cell Culture, Real-time Polymerase Chain Reaction, Western Blot, Migration, Transwell Assay, Chemotaxis Assay, Control

Figure 6. An increase in IL-17ED cells may indicate a neutrophil infiltration in human skin inflammatory conditions. Expression of myeloperoxidase (green) in combination with IL-17E (red) and DAPI (blue) assessed by immunofluorescence in the skin of healthy volunteers (n ¼ 4) and patients with acute generalized exanthematous pustulosis (n ¼ 3) and pyoderma gangrenosum (n ¼ 4). Original magnification 20. Scale bar ¼ 50 mm. (b) Quantification of dermal IL-17Eþ and MPOþ cells in the samples, as in a. (c) Quantification of the expression of IL-17E in the epidermis of the samples shown in a. AGEP, acute generalized exanthematous pustulosis; MPO, myeloperoxidase; PG, pyoderma gangrenosum.

Journal: The Journal of investigative dermatology

Article Title: IL-17E (IL-25) Enhances Innate Immune Responses during Skin Inflammation.

doi: 10.1016/j.jid.2019.01.021

Figure Lengend Snippet: Figure 6. An increase in IL-17ED cells may indicate a neutrophil infiltration in human skin inflammatory conditions. Expression of myeloperoxidase (green) in combination with IL-17E (red) and DAPI (blue) assessed by immunofluorescence in the skin of healthy volunteers (n ¼ 4) and patients with acute generalized exanthematous pustulosis (n ¼ 3) and pyoderma gangrenosum (n ¼ 4). Original magnification 20. Scale bar ¼ 50 mm. (b) Quantification of dermal IL-17Eþ and MPOþ cells in the samples, as in a. (c) Quantification of the expression of IL-17E in the epidermis of the samples shown in a. AGEP, acute generalized exanthematous pustulosis; MPO, myeloperoxidase; PG, pyoderma gangrenosum.

Article Snippet: Mouse antihuman IL-17E mAb (clone 182293) and polyclonal goat anti-human myeloperoxidase antibody were from R&D Systems, rabbit anti-human cytokeratin 10 was from BioSB (Santa Barbara, CA), and rat anti-mouse Ki67 mAb (clone 16A8) and rat anti-mouse Ly6G (clone 1A8) were from Biolegend.

Techniques: Expressing