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recombinant wnt9b  (R&D Systems)


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    R&D Systems recombinant wnt9b
    (a) Schematic diagram of the full length PC1 construct employed in these studies. The positions of the Flag tag, HA tag, GPS site and tethered agonist (TA) are indicated, as is the position of the lysine residues whose availability for biotinylation is assessed in 1e. (b) Immunofluorescence detection and quantification of surface PC1 NTF following 3 hrs treatment with <t>Wnt9b.</t> Flag staining (NTF) was performed under non-permeabilizing conditions. HA staining, following permeabilization, revealed total cell quantity of CTF and was used to normalize surface staining. Scale bar=5μM. Graph depicts ratio of Flag to HA staining, normalized to the mean of this value obtained after vehicle treatment. (c) PC1 and 2 expressing-HEK293 cells were treated with Wnt9b or subjected to an alkaline stripping protocol and surface biotinylation was performed. Proteins recovered by streptavidin pull-down were probed with anti-Flag. Cell lysates were probed with anti-HA antibodies. Surface NTF is detected by anti-Flag antibody, and total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Flag to HA signal, normalized to the mean of this value obtained after vehicle treatment. (d) Western blot detection of total PC1 NTF using anti-Flag antibody. Cells were treated with vehicle or Wnt9b overnight. Bar graphs represent Flag/HA signal ratio. (e) Western blot detection of biotinylated PC1 CTF in experiment where cell surface biotinylation was followed by HA pulldown and streptavidin blotting. Results show increased accessibility of the Lys residue in the PC1-CTF TM6-7 extracellular loop (extracellular loop 3) upon Wnt9b treatment or following alkaline stripping. Total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Streptavidin to HA signal, normalized to the mean of this value obtained after vehicle treatment. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed for all of the panels except for the time course depicted in 1b, for which a paired Student t-Test was employed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.
    Recombinant Wnt9b, supplied by R&D Systems, used in various techniques. Bioz Stars score: 93/100, based on 5 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/recombinant wnt9b/product/R&D Systems
    Average 93 stars, based on 5 article reviews
    recombinant wnt9b - by Bioz Stars, 2026-05
    93/100 stars

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    1) Product Images from "Polycystin-1 acts as an atypical adhesion GPCR that responds to novel Wnt signaling and mechanical stimuli"

    Article Title: Polycystin-1 acts as an atypical adhesion GPCR that responds to novel Wnt signaling and mechanical stimuli

    Journal: bioRxiv

    doi: 10.1101/2025.05.21.655326

    (a) Schematic diagram of the full length PC1 construct employed in these studies. The positions of the Flag tag, HA tag, GPS site and tethered agonist (TA) are indicated, as is the position of the lysine residues whose availability for biotinylation is assessed in 1e. (b) Immunofluorescence detection and quantification of surface PC1 NTF following 3 hrs treatment with Wnt9b. Flag staining (NTF) was performed under non-permeabilizing conditions. HA staining, following permeabilization, revealed total cell quantity of CTF and was used to normalize surface staining. Scale bar=5μM. Graph depicts ratio of Flag to HA staining, normalized to the mean of this value obtained after vehicle treatment. (c) PC1 and 2 expressing-HEK293 cells were treated with Wnt9b or subjected to an alkaline stripping protocol and surface biotinylation was performed. Proteins recovered by streptavidin pull-down were probed with anti-Flag. Cell lysates were probed with anti-HA antibodies. Surface NTF is detected by anti-Flag antibody, and total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Flag to HA signal, normalized to the mean of this value obtained after vehicle treatment. (d) Western blot detection of total PC1 NTF using anti-Flag antibody. Cells were treated with vehicle or Wnt9b overnight. Bar graphs represent Flag/HA signal ratio. (e) Western blot detection of biotinylated PC1 CTF in experiment where cell surface biotinylation was followed by HA pulldown and streptavidin blotting. Results show increased accessibility of the Lys residue in the PC1-CTF TM6-7 extracellular loop (extracellular loop 3) upon Wnt9b treatment or following alkaline stripping. Total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Streptavidin to HA signal, normalized to the mean of this value obtained after vehicle treatment. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed for all of the panels except for the time course depicted in 1b, for which a paired Student t-Test was employed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.
    Figure Legend Snippet: (a) Schematic diagram of the full length PC1 construct employed in these studies. The positions of the Flag tag, HA tag, GPS site and tethered agonist (TA) are indicated, as is the position of the lysine residues whose availability for biotinylation is assessed in 1e. (b) Immunofluorescence detection and quantification of surface PC1 NTF following 3 hrs treatment with Wnt9b. Flag staining (NTF) was performed under non-permeabilizing conditions. HA staining, following permeabilization, revealed total cell quantity of CTF and was used to normalize surface staining. Scale bar=5μM. Graph depicts ratio of Flag to HA staining, normalized to the mean of this value obtained after vehicle treatment. (c) PC1 and 2 expressing-HEK293 cells were treated with Wnt9b or subjected to an alkaline stripping protocol and surface biotinylation was performed. Proteins recovered by streptavidin pull-down were probed with anti-Flag. Cell lysates were probed with anti-HA antibodies. Surface NTF is detected by anti-Flag antibody, and total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Flag to HA signal, normalized to the mean of this value obtained after vehicle treatment. (d) Western blot detection of total PC1 NTF using anti-Flag antibody. Cells were treated with vehicle or Wnt9b overnight. Bar graphs represent Flag/HA signal ratio. (e) Western blot detection of biotinylated PC1 CTF in experiment where cell surface biotinylation was followed by HA pulldown and streptavidin blotting. Results show increased accessibility of the Lys residue in the PC1-CTF TM6-7 extracellular loop (extracellular loop 3) upon Wnt9b treatment or following alkaline stripping. Total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Streptavidin to HA signal, normalized to the mean of this value obtained after vehicle treatment. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed for all of the panels except for the time course depicted in 1b, for which a paired Student t-Test was employed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.

    Techniques Used: Construct, FLAG-tag, Immunofluorescence, Staining, Expressing, Stripping Membranes, Western Blot, Residue, Control

    (a) GSK3β co-immunoprecipitates with PC1 following NTF removal by exposure to high pH (strip) or Wnt9b. GSK3β associated with PC1 after 5 minutes of Wnt9b treatment. (b) GSK3β co-immunoprecipitates with PC1 from lysates prepared from Tg248 Pkd1 BAC-transgenic mouse kidneys. (c) Fluorescent biosensor assay of endogenous GSK3β kinase activity in HEK293 cells. PC1 and 2 inhibit GSK3β and this effect is enhanced by 3 hrs treatment with 13nM Wnt9b. Scale bar=100 μM. Graph depicts fluorescence intensity measured in each condition normalized to mean of that measured in cells that express GFP alone. (d) GSK3β kinase assay employing a peptide that electrophoretically migrates in agarose faster when phosphorylated. Lysates from PC1-expressing mouse kidney were compared to similar aged WT kidney lysates. Graph shows mean of the ratio of GSK3β-phosphorylated peptide (PP) to unphosphorylated peptide (P) under each condition. (e) Detection of S9 phosphorylated GSK3β in lysates from un-induced, pre-cystic and cystic kidneys. Blots were probed with anti pan-GSK3β, anti pS9-GSK3β and anti-actin antibodies. Graph depicts the mean of the ratio of the pS9-GSK3β signal to the pan GSK3β signal for each condition. (f) Fluorescent biosensor assay of endogenous GSK3β kinase activity in immortalized murine M113 cells. Untransfected cells were compared to cells expressing PC1 and PC2 as well as to PC1 and 2 expressing cells treated with Wnt9b for 3hrs Scale bar=100 μM. Graph depicts fluorescence intensity measured in each condition normalized to mean of that measured in cells that express GFP alone. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.
    Figure Legend Snippet: (a) GSK3β co-immunoprecipitates with PC1 following NTF removal by exposure to high pH (strip) or Wnt9b. GSK3β associated with PC1 after 5 minutes of Wnt9b treatment. (b) GSK3β co-immunoprecipitates with PC1 from lysates prepared from Tg248 Pkd1 BAC-transgenic mouse kidneys. (c) Fluorescent biosensor assay of endogenous GSK3β kinase activity in HEK293 cells. PC1 and 2 inhibit GSK3β and this effect is enhanced by 3 hrs treatment with 13nM Wnt9b. Scale bar=100 μM. Graph depicts fluorescence intensity measured in each condition normalized to mean of that measured in cells that express GFP alone. (d) GSK3β kinase assay employing a peptide that electrophoretically migrates in agarose faster when phosphorylated. Lysates from PC1-expressing mouse kidney were compared to similar aged WT kidney lysates. Graph shows mean of the ratio of GSK3β-phosphorylated peptide (PP) to unphosphorylated peptide (P) under each condition. (e) Detection of S9 phosphorylated GSK3β in lysates from un-induced, pre-cystic and cystic kidneys. Blots were probed with anti pan-GSK3β, anti pS9-GSK3β and anti-actin antibodies. Graph depicts the mean of the ratio of the pS9-GSK3β signal to the pan GSK3β signal for each condition. (f) Fluorescent biosensor assay of endogenous GSK3β kinase activity in immortalized murine M113 cells. Untransfected cells were compared to cells expressing PC1 and PC2 as well as to PC1 and 2 expressing cells treated with Wnt9b for 3hrs Scale bar=100 μM. Graph depicts fluorescence intensity measured in each condition normalized to mean of that measured in cells that express GFP alone. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.

    Techniques Used: Stripping Membranes, Transgenic Assay, Biosensor Assay, Activity Assay, Fluorescence, Kinase Assay, Expressing, Control

    (a) PC1 ΔNTF co-immunoprecipitates with GSK3β to the same extent as Wnt9b-stimulated full length PC1. Less GSK3β co-immunoprecipitates with PC1 ΔNTF+ΔTA , which lacks a tethered agonist. The graph depicts the ratio of GSK3β signal to the HA signal, normalized to the value of this ratio for the HEK 1+2 condition. (b) GSK3β biosensor shows that PC1 ΔNTF inhibits GSK3β to the same extent as a maximal concentration (10 μM) of GSK3β inhibitor SB-216763. PC1 ΔNTF+ΔTA does not inhibit GSK3β. The graph depicts the ratio of GFP fluorescence in each condition, normalized to the mean of this value obtained with cells that express GFP alone. (c) Confocal Z-stack imaging of PC1 ΔNTF and PC1 ΔNTF+ΔTA detected with anti-HA antibody added to the media bathing unfixed and non-permeabilized cells shows that both proteins expressed in the absence of PC2 reach the surfaces of HEK293 cells. (d) PC1 ΔNTF+ΔTA , lacking the Stachel sequence, does not inhibit the GSK3β in the fluorescence biosensor assay. The ability of PC1 ΔNTF+ΔTA to inhibit GSK3β can be partially restored by addition of soluble Stachel peptide (300 μM). Scrambled Stachel sequence (scrm) did not produce this effect. Versions of the PC1 ΔNTF protein that carry successive groups of alanine substitutions in the sequences of their tethered agonists (PC1 ΔNTF -Ala1-4) do not inhibit GSK3β. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panel 3d the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.
    Figure Legend Snippet: (a) PC1 ΔNTF co-immunoprecipitates with GSK3β to the same extent as Wnt9b-stimulated full length PC1. Less GSK3β co-immunoprecipitates with PC1 ΔNTF+ΔTA , which lacks a tethered agonist. The graph depicts the ratio of GSK3β signal to the HA signal, normalized to the value of this ratio for the HEK 1+2 condition. (b) GSK3β biosensor shows that PC1 ΔNTF inhibits GSK3β to the same extent as a maximal concentration (10 μM) of GSK3β inhibitor SB-216763. PC1 ΔNTF+ΔTA does not inhibit GSK3β. The graph depicts the ratio of GFP fluorescence in each condition, normalized to the mean of this value obtained with cells that express GFP alone. (c) Confocal Z-stack imaging of PC1 ΔNTF and PC1 ΔNTF+ΔTA detected with anti-HA antibody added to the media bathing unfixed and non-permeabilized cells shows that both proteins expressed in the absence of PC2 reach the surfaces of HEK293 cells. (d) PC1 ΔNTF+ΔTA , lacking the Stachel sequence, does not inhibit the GSK3β in the fluorescence biosensor assay. The ability of PC1 ΔNTF+ΔTA to inhibit GSK3β can be partially restored by addition of soluble Stachel peptide (300 μM). Scrambled Stachel sequence (scrm) did not produce this effect. Versions of the PC1 ΔNTF protein that carry successive groups of alanine substitutions in the sequences of their tethered agonists (PC1 ΔNTF -Ala1-4) do not inhibit GSK3β. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panel 3d the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.

    Techniques Used: Concentration Assay, Fluorescence, Imaging, Sequencing, Biosensor Assay, Control

    (a) GSK3β activity measured +/− Gα13 or RhoA or control (Ctrl) siRNAs, or ROCK inhibitor Y27632. Suppressing Gα13, RhoA or ROCK dampened GSK3β inhibition by Wnt9b-stimulated PC1 or PC1ΔNTF. 10 μM SB-216763 (SB) treatment demonstrates fluorescence detected with maximal GSK3β inhibition. Graph depicts means of ratios of GFP signals normalized to mean of value obtained with cells transfected with GFP and Ctrl RNAi. (b) GTP-bound RhoA abundance was assessed by rotekin RhoA-GTP binding domain bead pull-down, followed by western blotting for RhoA. Wnt9b stimulation of PC1, or PC1ΔNTF expression, increased GTP-bound RhoA. Graph depicts means of ratios of RhoA-GTP signal, normalized to mean of value obtained with empty vector (EV) transfection. The quantity of RhoA-GTP is also substantially higher in lysates prepared from the kidneys of Tg248 Pkd1 BAC-transgenic mice as compared to that present in lysates of wild type mouse kidneys. (c) and (d) Detection of in vitro (c) and in vivo (d) quantity of Gα13 present in anti-HA precipitates of PC1 was assessed by western blotting. Wnt9b treatment modestly but significantly increased quantity of PC1-associated Gα13 PC1 (c). Graphs in c and d depict means of ratios of signal detected in Wnt9b-treated condition, normalized to mean of value obtained with vehicle-treated cells. Graph depicts the intensity of the Gα13 signal in each condition normalized to the corresponding HA signal. (e) Biosensor assay to detect importance of G-protein binding site of PC1 for regulation of GSK3β. PC1 or PC1 ΔNTF lacking its G-protein binding site, or PC1 carrying a mutation within the G-protein binding site sequence (ΔL4132), does not inhibit GSK3β. Similarly, soluble Stachel peptide does not induce GSK3β inhibition in cells expressing PC1 ΔNTF+ΔTA+ΔL4132 . Graph depicts ratio of GFP fluorescence, normalized to mean of value obtained with cells expressing GFP alone. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values ≤ 0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panels 4a and 4f the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.
    Figure Legend Snippet: (a) GSK3β activity measured +/− Gα13 or RhoA or control (Ctrl) siRNAs, or ROCK inhibitor Y27632. Suppressing Gα13, RhoA or ROCK dampened GSK3β inhibition by Wnt9b-stimulated PC1 or PC1ΔNTF. 10 μM SB-216763 (SB) treatment demonstrates fluorescence detected with maximal GSK3β inhibition. Graph depicts means of ratios of GFP signals normalized to mean of value obtained with cells transfected with GFP and Ctrl RNAi. (b) GTP-bound RhoA abundance was assessed by rotekin RhoA-GTP binding domain bead pull-down, followed by western blotting for RhoA. Wnt9b stimulation of PC1, or PC1ΔNTF expression, increased GTP-bound RhoA. Graph depicts means of ratios of RhoA-GTP signal, normalized to mean of value obtained with empty vector (EV) transfection. The quantity of RhoA-GTP is also substantially higher in lysates prepared from the kidneys of Tg248 Pkd1 BAC-transgenic mice as compared to that present in lysates of wild type mouse kidneys. (c) and (d) Detection of in vitro (c) and in vivo (d) quantity of Gα13 present in anti-HA precipitates of PC1 was assessed by western blotting. Wnt9b treatment modestly but significantly increased quantity of PC1-associated Gα13 PC1 (c). Graphs in c and d depict means of ratios of signal detected in Wnt9b-treated condition, normalized to mean of value obtained with vehicle-treated cells. Graph depicts the intensity of the Gα13 signal in each condition normalized to the corresponding HA signal. (e) Biosensor assay to detect importance of G-protein binding site of PC1 for regulation of GSK3β. PC1 or PC1 ΔNTF lacking its G-protein binding site, or PC1 carrying a mutation within the G-protein binding site sequence (ΔL4132), does not inhibit GSK3β. Similarly, soluble Stachel peptide does not induce GSK3β inhibition in cells expressing PC1 ΔNTF+ΔTA+ΔL4132 . Graph depicts ratio of GFP fluorescence, normalized to mean of value obtained with cells expressing GFP alone. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values ≤ 0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panels 4a and 4f the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.

    Techniques Used: Activity Assay, Control, Inhibition, Fluorescence, Transfection, Binding Assay, Western Blot, Expressing, Plasmid Preparation, Transgenic Assay, In Vitro, In Vivo, Biosensor Assay, Protein Binding, Mutagenesis, Sequencing

    (a) Immunofluorescent localization of the full length PC1 (green) in the primary cilia of LLCPK1+2 cells treated with wnt9b, or with a combination of Wnt9b and barbadin. Cilia are detected by immunostaining for Arl13b (orange) (b) Immunofluorescent localization of PC1 ΔNTF and PC1 ΔNTFΔTA in the primary cilia of LLCPK cells. Barbadin treatment results in localization of PC1 ΔNTF to cilia, while treatment with soluble TA peptide causes loss of PC1 ΔNTF+ΔTA from the cilia. (c) Immunofluorescence detection of the full length PC1 in the primary cilia of cells treated with mechanical stimulation, with medium from cells preconditioned by mechanical stimulation or with ATP added to the medium. Barbadin and Apyrase treatment blocked the effects of mechanical stimulation and ATP on PC1 ciliary localization. Data are shown as mean ±SEM, n≥3 for all experiments. Scale bar = 5μ. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.
    Figure Legend Snippet: (a) Immunofluorescent localization of the full length PC1 (green) in the primary cilia of LLCPK1+2 cells treated with wnt9b, or with a combination of Wnt9b and barbadin. Cilia are detected by immunostaining for Arl13b (orange) (b) Immunofluorescent localization of PC1 ΔNTF and PC1 ΔNTFΔTA in the primary cilia of LLCPK cells. Barbadin treatment results in localization of PC1 ΔNTF to cilia, while treatment with soluble TA peptide causes loss of PC1 ΔNTF+ΔTA from the cilia. (c) Immunofluorescence detection of the full length PC1 in the primary cilia of cells treated with mechanical stimulation, with medium from cells preconditioned by mechanical stimulation or with ATP added to the medium. Barbadin and Apyrase treatment blocked the effects of mechanical stimulation and ATP on PC1 ciliary localization. Data are shown as mean ±SEM, n≥3 for all experiments. Scale bar = 5μ. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.

    Techniques Used: Immunostaining, Immunofluorescence, Control

    (a) Immunofluorescent detection of the localizations of PC1S3164A and PC1S3164D to the primary cilia in LLCPK cells. ATP treatment did not alter the ciliary distribution of PC1S3164A, whereas the ciliary exclusion of PC1 S3163D was reversed by Barbadin treatment. PKA inhibitor H89A treatment prevented the departure of PC1 from primary cilia that is induced by either ATP or Wnt9b treatment. (b) Biosensor assay was used to assess the importance of PC1 PKA phosphorylation site S3164 for PC1 activation-dependent inhibition of GSK3β kinase in HEK293 cells. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panel 3d the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.
    Figure Legend Snippet: (a) Immunofluorescent detection of the localizations of PC1S3164A and PC1S3164D to the primary cilia in LLCPK cells. ATP treatment did not alter the ciliary distribution of PC1S3164A, whereas the ciliary exclusion of PC1 S3163D was reversed by Barbadin treatment. PKA inhibitor H89A treatment prevented the departure of PC1 from primary cilia that is induced by either ATP or Wnt9b treatment. (b) Biosensor assay was used to assess the importance of PC1 PKA phosphorylation site S3164 for PC1 activation-dependent inhibition of GSK3β kinase in HEK293 cells. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panel 3d the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.

    Techniques Used: Biosensor Assay, Phospho-proteomics, Activation Assay, Inhibition, Control



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    (a) Schematic diagram of the full length PC1 construct employed in these studies. The positions of the Flag tag, HA tag, GPS site and tethered agonist (TA) are indicated, as is the position of the lysine residues whose availability for biotinylation is assessed in 1e. (b) Immunofluorescence detection and quantification of surface PC1 NTF following 3 hrs treatment with <t>Wnt9b.</t> Flag staining (NTF) was performed under non-permeabilizing conditions. HA staining, following permeabilization, revealed total cell quantity of CTF and was used to normalize surface staining. Scale bar=5μM. Graph depicts ratio of Flag to HA staining, normalized to the mean of this value obtained after vehicle treatment. (c) PC1 and 2 expressing-HEK293 cells were treated with Wnt9b or subjected to an alkaline stripping protocol and surface biotinylation was performed. Proteins recovered by streptavidin pull-down were probed with anti-Flag. Cell lysates were probed with anti-HA antibodies. Surface NTF is detected by anti-Flag antibody, and total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Flag to HA signal, normalized to the mean of this value obtained after vehicle treatment. (d) Western blot detection of total PC1 NTF using anti-Flag antibody. Cells were treated with vehicle or Wnt9b overnight. Bar graphs represent Flag/HA signal ratio. (e) Western blot detection of biotinylated PC1 CTF in experiment where cell surface biotinylation was followed by HA pulldown and streptavidin blotting. Results show increased accessibility of the Lys residue in the PC1-CTF TM6-7 extracellular loop (extracellular loop 3) upon Wnt9b treatment or following alkaline stripping. Total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Streptavidin to HA signal, normalized to the mean of this value obtained after vehicle treatment. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed for all of the panels except for the time course depicted in 1b, for which a paired Student t-Test was employed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.
    Klf2α Wnt9b Signalling Pathway, supplied by Fukui Bank Ltd, 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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    (a) Schematic diagram of the full length PC1 construct employed in these studies. The positions of the Flag tag, HA tag, GPS site and tethered agonist (TA) are indicated, as is the position of the lysine residues whose availability for biotinylation is assessed in 1e. (b) Immunofluorescence detection and quantification of surface PC1 NTF following 3 hrs treatment with Wnt9b. Flag staining (NTF) was performed under non-permeabilizing conditions. HA staining, following permeabilization, revealed total cell quantity of CTF and was used to normalize surface staining. Scale bar=5μM. Graph depicts ratio of Flag to HA staining, normalized to the mean of this value obtained after vehicle treatment. (c) PC1 and 2 expressing-HEK293 cells were treated with Wnt9b or subjected to an alkaline stripping protocol and surface biotinylation was performed. Proteins recovered by streptavidin pull-down were probed with anti-Flag. Cell lysates were probed with anti-HA antibodies. Surface NTF is detected by anti-Flag antibody, and total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Flag to HA signal, normalized to the mean of this value obtained after vehicle treatment. (d) Western blot detection of total PC1 NTF using anti-Flag antibody. Cells were treated with vehicle or Wnt9b overnight. Bar graphs represent Flag/HA signal ratio. (e) Western blot detection of biotinylated PC1 CTF in experiment where cell surface biotinylation was followed by HA pulldown and streptavidin blotting. Results show increased accessibility of the Lys residue in the PC1-CTF TM6-7 extracellular loop (extracellular loop 3) upon Wnt9b treatment or following alkaline stripping. Total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Streptavidin to HA signal, normalized to the mean of this value obtained after vehicle treatment. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed for all of the panels except for the time course depicted in 1b, for which a paired Student t-Test was employed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.

    Journal: bioRxiv

    Article Title: Polycystin-1 acts as an atypical adhesion GPCR that responds to novel Wnt signaling and mechanical stimuli

    doi: 10.1101/2025.05.21.655326

    Figure Lengend Snippet: (a) Schematic diagram of the full length PC1 construct employed in these studies. The positions of the Flag tag, HA tag, GPS site and tethered agonist (TA) are indicated, as is the position of the lysine residues whose availability for biotinylation is assessed in 1e. (b) Immunofluorescence detection and quantification of surface PC1 NTF following 3 hrs treatment with Wnt9b. Flag staining (NTF) was performed under non-permeabilizing conditions. HA staining, following permeabilization, revealed total cell quantity of CTF and was used to normalize surface staining. Scale bar=5μM. Graph depicts ratio of Flag to HA staining, normalized to the mean of this value obtained after vehicle treatment. (c) PC1 and 2 expressing-HEK293 cells were treated with Wnt9b or subjected to an alkaline stripping protocol and surface biotinylation was performed. Proteins recovered by streptavidin pull-down were probed with anti-Flag. Cell lysates were probed with anti-HA antibodies. Surface NTF is detected by anti-Flag antibody, and total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Flag to HA signal, normalized to the mean of this value obtained after vehicle treatment. (d) Western blot detection of total PC1 NTF using anti-Flag antibody. Cells were treated with vehicle or Wnt9b overnight. Bar graphs represent Flag/HA signal ratio. (e) Western blot detection of biotinylated PC1 CTF in experiment where cell surface biotinylation was followed by HA pulldown and streptavidin blotting. Results show increased accessibility of the Lys residue in the PC1-CTF TM6-7 extracellular loop (extracellular loop 3) upon Wnt9b treatment or following alkaline stripping. Total cell-associated PC1 is represented by the HA signal. The graph depicts ratio of Streptavidin to HA signal, normalized to the mean of this value obtained after vehicle treatment. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed for all of the panels except for the time course depicted in 1b, for which a paired Student t-Test was employed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.

    Article Snippet: Recombinant Wnt9b (0.5ng/μL) (R&D Systems, 3669) was applied for 3 hrs or overnight.

    Techniques: Construct, FLAG-tag, Immunofluorescence, Staining, Expressing, Stripping Membranes, Western Blot, Residue, Control

    (a) GSK3β co-immunoprecipitates with PC1 following NTF removal by exposure to high pH (strip) or Wnt9b. GSK3β associated with PC1 after 5 minutes of Wnt9b treatment. (b) GSK3β co-immunoprecipitates with PC1 from lysates prepared from Tg248 Pkd1 BAC-transgenic mouse kidneys. (c) Fluorescent biosensor assay of endogenous GSK3β kinase activity in HEK293 cells. PC1 and 2 inhibit GSK3β and this effect is enhanced by 3 hrs treatment with 13nM Wnt9b. Scale bar=100 μM. Graph depicts fluorescence intensity measured in each condition normalized to mean of that measured in cells that express GFP alone. (d) GSK3β kinase assay employing a peptide that electrophoretically migrates in agarose faster when phosphorylated. Lysates from PC1-expressing mouse kidney were compared to similar aged WT kidney lysates. Graph shows mean of the ratio of GSK3β-phosphorylated peptide (PP) to unphosphorylated peptide (P) under each condition. (e) Detection of S9 phosphorylated GSK3β in lysates from un-induced, pre-cystic and cystic kidneys. Blots were probed with anti pan-GSK3β, anti pS9-GSK3β and anti-actin antibodies. Graph depicts the mean of the ratio of the pS9-GSK3β signal to the pan GSK3β signal for each condition. (f) Fluorescent biosensor assay of endogenous GSK3β kinase activity in immortalized murine M113 cells. Untransfected cells were compared to cells expressing PC1 and PC2 as well as to PC1 and 2 expressing cells treated with Wnt9b for 3hrs Scale bar=100 μM. Graph depicts fluorescence intensity measured in each condition normalized to mean of that measured in cells that express GFP alone. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.

    Journal: bioRxiv

    Article Title: Polycystin-1 acts as an atypical adhesion GPCR that responds to novel Wnt signaling and mechanical stimuli

    doi: 10.1101/2025.05.21.655326

    Figure Lengend Snippet: (a) GSK3β co-immunoprecipitates with PC1 following NTF removal by exposure to high pH (strip) or Wnt9b. GSK3β associated with PC1 after 5 minutes of Wnt9b treatment. (b) GSK3β co-immunoprecipitates with PC1 from lysates prepared from Tg248 Pkd1 BAC-transgenic mouse kidneys. (c) Fluorescent biosensor assay of endogenous GSK3β kinase activity in HEK293 cells. PC1 and 2 inhibit GSK3β and this effect is enhanced by 3 hrs treatment with 13nM Wnt9b. Scale bar=100 μM. Graph depicts fluorescence intensity measured in each condition normalized to mean of that measured in cells that express GFP alone. (d) GSK3β kinase assay employing a peptide that electrophoretically migrates in agarose faster when phosphorylated. Lysates from PC1-expressing mouse kidney were compared to similar aged WT kidney lysates. Graph shows mean of the ratio of GSK3β-phosphorylated peptide (PP) to unphosphorylated peptide (P) under each condition. (e) Detection of S9 phosphorylated GSK3β in lysates from un-induced, pre-cystic and cystic kidneys. Blots were probed with anti pan-GSK3β, anti pS9-GSK3β and anti-actin antibodies. Graph depicts the mean of the ratio of the pS9-GSK3β signal to the pan GSK3β signal for each condition. (f) Fluorescent biosensor assay of endogenous GSK3β kinase activity in immortalized murine M113 cells. Untransfected cells were compared to cells expressing PC1 and PC2 as well as to PC1 and 2 expressing cells treated with Wnt9b for 3hrs Scale bar=100 μM. Graph depicts fluorescence intensity measured in each condition normalized to mean of that measured in cells that express GFP alone. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant. *=P<0.05; **=P<0.01; ***=P<0.001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.

    Article Snippet: Recombinant Wnt9b (0.5ng/μL) (R&D Systems, 3669) was applied for 3 hrs or overnight.

    Techniques: Stripping Membranes, Transgenic Assay, Biosensor Assay, Activity Assay, Fluorescence, Kinase Assay, Expressing, Control

    (a) PC1 ΔNTF co-immunoprecipitates with GSK3β to the same extent as Wnt9b-stimulated full length PC1. Less GSK3β co-immunoprecipitates with PC1 ΔNTF+ΔTA , which lacks a tethered agonist. The graph depicts the ratio of GSK3β signal to the HA signal, normalized to the value of this ratio for the HEK 1+2 condition. (b) GSK3β biosensor shows that PC1 ΔNTF inhibits GSK3β to the same extent as a maximal concentration (10 μM) of GSK3β inhibitor SB-216763. PC1 ΔNTF+ΔTA does not inhibit GSK3β. The graph depicts the ratio of GFP fluorescence in each condition, normalized to the mean of this value obtained with cells that express GFP alone. (c) Confocal Z-stack imaging of PC1 ΔNTF and PC1 ΔNTF+ΔTA detected with anti-HA antibody added to the media bathing unfixed and non-permeabilized cells shows that both proteins expressed in the absence of PC2 reach the surfaces of HEK293 cells. (d) PC1 ΔNTF+ΔTA , lacking the Stachel sequence, does not inhibit the GSK3β in the fluorescence biosensor assay. The ability of PC1 ΔNTF+ΔTA to inhibit GSK3β can be partially restored by addition of soluble Stachel peptide (300 μM). Scrambled Stachel sequence (scrm) did not produce this effect. Versions of the PC1 ΔNTF protein that carry successive groups of alanine substitutions in the sequences of their tethered agonists (PC1 ΔNTF -Ala1-4) do not inhibit GSK3β. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panel 3d the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.

    Journal: bioRxiv

    Article Title: Polycystin-1 acts as an atypical adhesion GPCR that responds to novel Wnt signaling and mechanical stimuli

    doi: 10.1101/2025.05.21.655326

    Figure Lengend Snippet: (a) PC1 ΔNTF co-immunoprecipitates with GSK3β to the same extent as Wnt9b-stimulated full length PC1. Less GSK3β co-immunoprecipitates with PC1 ΔNTF+ΔTA , which lacks a tethered agonist. The graph depicts the ratio of GSK3β signal to the HA signal, normalized to the value of this ratio for the HEK 1+2 condition. (b) GSK3β biosensor shows that PC1 ΔNTF inhibits GSK3β to the same extent as a maximal concentration (10 μM) of GSK3β inhibitor SB-216763. PC1 ΔNTF+ΔTA does not inhibit GSK3β. The graph depicts the ratio of GFP fluorescence in each condition, normalized to the mean of this value obtained with cells that express GFP alone. (c) Confocal Z-stack imaging of PC1 ΔNTF and PC1 ΔNTF+ΔTA detected with anti-HA antibody added to the media bathing unfixed and non-permeabilized cells shows that both proteins expressed in the absence of PC2 reach the surfaces of HEK293 cells. (d) PC1 ΔNTF+ΔTA , lacking the Stachel sequence, does not inhibit the GSK3β in the fluorescence biosensor assay. The ability of PC1 ΔNTF+ΔTA to inhibit GSK3β can be partially restored by addition of soluble Stachel peptide (300 μM). Scrambled Stachel sequence (scrm) did not produce this effect. Versions of the PC1 ΔNTF protein that carry successive groups of alanine substitutions in the sequences of their tethered agonists (PC1 ΔNTF -Ala1-4) do not inhibit GSK3β. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panel 3d the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.

    Article Snippet: Recombinant Wnt9b (0.5ng/μL) (R&D Systems, 3669) was applied for 3 hrs or overnight.

    Techniques: Concentration Assay, Fluorescence, Imaging, Sequencing, Biosensor Assay, Control

    (a) GSK3β activity measured +/− Gα13 or RhoA or control (Ctrl) siRNAs, or ROCK inhibitor Y27632. Suppressing Gα13, RhoA or ROCK dampened GSK3β inhibition by Wnt9b-stimulated PC1 or PC1ΔNTF. 10 μM SB-216763 (SB) treatment demonstrates fluorescence detected with maximal GSK3β inhibition. Graph depicts means of ratios of GFP signals normalized to mean of value obtained with cells transfected with GFP and Ctrl RNAi. (b) GTP-bound RhoA abundance was assessed by rotekin RhoA-GTP binding domain bead pull-down, followed by western blotting for RhoA. Wnt9b stimulation of PC1, or PC1ΔNTF expression, increased GTP-bound RhoA. Graph depicts means of ratios of RhoA-GTP signal, normalized to mean of value obtained with empty vector (EV) transfection. The quantity of RhoA-GTP is also substantially higher in lysates prepared from the kidneys of Tg248 Pkd1 BAC-transgenic mice as compared to that present in lysates of wild type mouse kidneys. (c) and (d) Detection of in vitro (c) and in vivo (d) quantity of Gα13 present in anti-HA precipitates of PC1 was assessed by western blotting. Wnt9b treatment modestly but significantly increased quantity of PC1-associated Gα13 PC1 (c). Graphs in c and d depict means of ratios of signal detected in Wnt9b-treated condition, normalized to mean of value obtained with vehicle-treated cells. Graph depicts the intensity of the Gα13 signal in each condition normalized to the corresponding HA signal. (e) Biosensor assay to detect importance of G-protein binding site of PC1 for regulation of GSK3β. PC1 or PC1 ΔNTF lacking its G-protein binding site, or PC1 carrying a mutation within the G-protein binding site sequence (ΔL4132), does not inhibit GSK3β. Similarly, soluble Stachel peptide does not induce GSK3β inhibition in cells expressing PC1 ΔNTF+ΔTA+ΔL4132 . Graph depicts ratio of GFP fluorescence, normalized to mean of value obtained with cells expressing GFP alone. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values ≤ 0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panels 4a and 4f the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.

    Journal: bioRxiv

    Article Title: Polycystin-1 acts as an atypical adhesion GPCR that responds to novel Wnt signaling and mechanical stimuli

    doi: 10.1101/2025.05.21.655326

    Figure Lengend Snippet: (a) GSK3β activity measured +/− Gα13 or RhoA or control (Ctrl) siRNAs, or ROCK inhibitor Y27632. Suppressing Gα13, RhoA or ROCK dampened GSK3β inhibition by Wnt9b-stimulated PC1 or PC1ΔNTF. 10 μM SB-216763 (SB) treatment demonstrates fluorescence detected with maximal GSK3β inhibition. Graph depicts means of ratios of GFP signals normalized to mean of value obtained with cells transfected with GFP and Ctrl RNAi. (b) GTP-bound RhoA abundance was assessed by rotekin RhoA-GTP binding domain bead pull-down, followed by western blotting for RhoA. Wnt9b stimulation of PC1, or PC1ΔNTF expression, increased GTP-bound RhoA. Graph depicts means of ratios of RhoA-GTP signal, normalized to mean of value obtained with empty vector (EV) transfection. The quantity of RhoA-GTP is also substantially higher in lysates prepared from the kidneys of Tg248 Pkd1 BAC-transgenic mice as compared to that present in lysates of wild type mouse kidneys. (c) and (d) Detection of in vitro (c) and in vivo (d) quantity of Gα13 present in anti-HA precipitates of PC1 was assessed by western blotting. Wnt9b treatment modestly but significantly increased quantity of PC1-associated Gα13 PC1 (c). Graphs in c and d depict means of ratios of signal detected in Wnt9b-treated condition, normalized to mean of value obtained with vehicle-treated cells. Graph depicts the intensity of the Gα13 signal in each condition normalized to the corresponding HA signal. (e) Biosensor assay to detect importance of G-protein binding site of PC1 for regulation of GSK3β. PC1 or PC1 ΔNTF lacking its G-protein binding site, or PC1 carrying a mutation within the G-protein binding site sequence (ΔL4132), does not inhibit GSK3β. Similarly, soluble Stachel peptide does not induce GSK3β inhibition in cells expressing PC1 ΔNTF+ΔTA+ΔL4132 . Graph depicts ratio of GFP fluorescence, normalized to mean of value obtained with cells expressing GFP alone. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values ≤ 0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panels 4a and 4f the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.

    Article Snippet: Recombinant Wnt9b (0.5ng/μL) (R&D Systems, 3669) was applied for 3 hrs or overnight.

    Techniques: Activity Assay, Control, Inhibition, Fluorescence, Transfection, Binding Assay, Western Blot, Expressing, Plasmid Preparation, Transgenic Assay, In Vitro, In Vivo, Biosensor Assay, Protein Binding, Mutagenesis, Sequencing

    (a) Immunofluorescent localization of the full length PC1 (green) in the primary cilia of LLCPK1+2 cells treated with wnt9b, or with a combination of Wnt9b and barbadin. Cilia are detected by immunostaining for Arl13b (orange) (b) Immunofluorescent localization of PC1 ΔNTF and PC1 ΔNTFΔTA in the primary cilia of LLCPK cells. Barbadin treatment results in localization of PC1 ΔNTF to cilia, while treatment with soluble TA peptide causes loss of PC1 ΔNTF+ΔTA from the cilia. (c) Immunofluorescence detection of the full length PC1 in the primary cilia of cells treated with mechanical stimulation, with medium from cells preconditioned by mechanical stimulation or with ATP added to the medium. Barbadin and Apyrase treatment blocked the effects of mechanical stimulation and ATP on PC1 ciliary localization. Data are shown as mean ±SEM, n≥3 for all experiments. Scale bar = 5μ. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.

    Journal: bioRxiv

    Article Title: Polycystin-1 acts as an atypical adhesion GPCR that responds to novel Wnt signaling and mechanical stimuli

    doi: 10.1101/2025.05.21.655326

    Figure Lengend Snippet: (a) Immunofluorescent localization of the full length PC1 (green) in the primary cilia of LLCPK1+2 cells treated with wnt9b, or with a combination of Wnt9b and barbadin. Cilia are detected by immunostaining for Arl13b (orange) (b) Immunofluorescent localization of PC1 ΔNTF and PC1 ΔNTFΔTA in the primary cilia of LLCPK cells. Barbadin treatment results in localization of PC1 ΔNTF to cilia, while treatment with soluble TA peptide causes loss of PC1 ΔNTF+ΔTA from the cilia. (c) Immunofluorescence detection of the full length PC1 in the primary cilia of cells treated with mechanical stimulation, with medium from cells preconditioned by mechanical stimulation or with ATP added to the medium. Barbadin and Apyrase treatment blocked the effects of mechanical stimulation and ATP on PC1 ciliary localization. Data are shown as mean ±SEM, n≥3 for all experiments. Scale bar = 5μ. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated.

    Article Snippet: Recombinant Wnt9b (0.5ng/μL) (R&D Systems, 3669) was applied for 3 hrs or overnight.

    Techniques: Immunostaining, Immunofluorescence, Control

    (a) Immunofluorescent detection of the localizations of PC1S3164A and PC1S3164D to the primary cilia in LLCPK cells. ATP treatment did not alter the ciliary distribution of PC1S3164A, whereas the ciliary exclusion of PC1 S3163D was reversed by Barbadin treatment. PKA inhibitor H89A treatment prevented the departure of PC1 from primary cilia that is induced by either ATP or Wnt9b treatment. (b) Biosensor assay was used to assess the importance of PC1 PKA phosphorylation site S3164 for PC1 activation-dependent inhibition of GSK3β kinase in HEK293 cells. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panel 3d the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.

    Journal: bioRxiv

    Article Title: Polycystin-1 acts as an atypical adhesion GPCR that responds to novel Wnt signaling and mechanical stimuli

    doi: 10.1101/2025.05.21.655326

    Figure Lengend Snippet: (a) Immunofluorescent detection of the localizations of PC1S3164A and PC1S3164D to the primary cilia in LLCPK cells. ATP treatment did not alter the ciliary distribution of PC1S3164A, whereas the ciliary exclusion of PC1 S3163D was reversed by Barbadin treatment. PKA inhibitor H89A treatment prevented the departure of PC1 from primary cilia that is induced by either ATP or Wnt9b treatment. (b) Biosensor assay was used to assess the importance of PC1 PKA phosphorylation site S3164 for PC1 activation-dependent inhibition of GSK3β kinase in HEK293 cells. Data are shown as mean ±SEM, n≥3 for all experiments. To assess statistical significance unpaired Student t-Test analysis was performed. P values <0.05 were considered significant *=P<0.05; **=P<0.01; ***=P<0.001.; ****=P<0.0001 Differences between mean values obtained for experimental conditions versus control conditions that produce minimal and/or maximal signals were evaluated. In panel 3d the values obtained for each condition were compared to those obtained in the GFP alone condition (indicated by the symbols above each bar) and pairwise comparisons of the values obtained in a subset of conditions related by a single experimental manipulation are indicated by the brackets above the bars.

    Article Snippet: Recombinant Wnt9b (0.5ng/μL) (R&D Systems, 3669) was applied for 3 hrs or overnight.

    Techniques: Biosensor Assay, Phospho-proteomics, Activation Assay, Inhibition, Control