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egfp pp1cb d63a mypt1  (Addgene inc)


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    Structured Review

    Addgene inc egfp pp1cb d63a mypt1
    (A) Depiction of relevant clusters of PCDH7 isoform-c interactome determined by GFP mediated affinity pulldown followed by LC-MS/MS. Red inset depicts a set of phosphatase subunits and phosphatase regulatory proteins, green inset highlighting components of myosin complexes, and blue inset showing members of ERM proteins. (B) Immunostaining of RPE1 cells expressing PCDH7-GFP (green), <t>MYPT1</t> (PPP1R12A) (red) and fluorescent phalloidin (blue). (C) Immunoblotting for GFP pulldown of <t>EGFP-PP1CB-MYPT1</t> fusion, EGFP-PP1CB*-MYPT1 <t>(D63A)</t> mutant and control construct with cotransfection of PCDH7c-V5 construct. Membranes were blotted using anti-V5, anti-MYPT1, anti-GFP and anti-tubulin antibodies. I (Input), FT(Flow Through), E (Elution) (D) Quantification of proximity ligation assay (PLA) showing fluorescence dots per cell for PCDH7- GFP (anti-GFP) and MYPT1 (anti-MYPT1) interaction (n=29) along with single primary antibody controls, MYPT1 (n=30) and GFP (n=30). ****p<0.0001.
    Egfp Pp1cb D63a Mypt1, supplied by Addgene inc, used in various techniques. Bioz Stars score: 94/100, based on 169 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/product/egfp+pp1cb+mypt1/bio_rxiv__2021__09__21__460794-205-15-11?v=Addgene+inc
    Average 94 stars, based on 169 article reviews
    egfp pp1cb d63a mypt1 - by Bioz Stars, 2026-07
    94/100 stars

    Images

    1) Product Images from "PCDH7 Promotes Cell Migration by Regulating Myosin Activity"

    Article Title: PCDH7 Promotes Cell Migration by Regulating Myosin Activity

    Journal: bioRxiv

    doi: 10.1101/2021.09.21.460794

    (A) Depiction of relevant clusters of PCDH7 isoform-c interactome determined by GFP mediated affinity pulldown followed by LC-MS/MS. Red inset depicts a set of phosphatase subunits and phosphatase regulatory proteins, green inset highlighting components of myosin complexes, and blue inset showing members of ERM proteins. (B) Immunostaining of RPE1 cells expressing PCDH7-GFP (green), MYPT1 (PPP1R12A) (red) and fluorescent phalloidin (blue). (C) Immunoblotting for GFP pulldown of EGFP-PP1CB-MYPT1 fusion, EGFP-PP1CB*-MYPT1 (D63A) mutant and control construct with cotransfection of PCDH7c-V5 construct. Membranes were blotted using anti-V5, anti-MYPT1, anti-GFP and anti-tubulin antibodies. I (Input), FT(Flow Through), E (Elution) (D) Quantification of proximity ligation assay (PLA) showing fluorescence dots per cell for PCDH7- GFP (anti-GFP) and MYPT1 (anti-MYPT1) interaction (n=29) along with single primary antibody controls, MYPT1 (n=30) and GFP (n=30). ****p<0.0001.
    Figure Legend Snippet: (A) Depiction of relevant clusters of PCDH7 isoform-c interactome determined by GFP mediated affinity pulldown followed by LC-MS/MS. Red inset depicts a set of phosphatase subunits and phosphatase regulatory proteins, green inset highlighting components of myosin complexes, and blue inset showing members of ERM proteins. (B) Immunostaining of RPE1 cells expressing PCDH7-GFP (green), MYPT1 (PPP1R12A) (red) and fluorescent phalloidin (blue). (C) Immunoblotting for GFP pulldown of EGFP-PP1CB-MYPT1 fusion, EGFP-PP1CB*-MYPT1 (D63A) mutant and control construct with cotransfection of PCDH7c-V5 construct. Membranes were blotted using anti-V5, anti-MYPT1, anti-GFP and anti-tubulin antibodies. I (Input), FT(Flow Through), E (Elution) (D) Quantification of proximity ligation assay (PLA) showing fluorescence dots per cell for PCDH7- GFP (anti-GFP) and MYPT1 (anti-MYPT1) interaction (n=29) along with single primary antibody controls, MYPT1 (n=30) and GFP (n=30). ****p<0.0001.

    Techniques Used: Liquid Chromatography with Mass Spectroscopy, Immunostaining, Expressing, Western Blot, Mutagenesis, Construct, Cotransfection, Proximity Ligation Assay, Fluorescence



    Similar Products

    94
    Addgene inc egfp pp1cb d63a mypt1
    (A) Depiction of relevant clusters of PCDH7 isoform-c interactome determined by GFP mediated affinity pulldown followed by LC-MS/MS. Red inset depicts a set of phosphatase subunits and phosphatase regulatory proteins, green inset highlighting components of myosin complexes, and blue inset showing members of ERM proteins. (B) Immunostaining of RPE1 cells expressing PCDH7-GFP (green), <t>MYPT1</t> (PPP1R12A) (red) and fluorescent phalloidin (blue). (C) Immunoblotting for GFP pulldown of <t>EGFP-PP1CB-MYPT1</t> fusion, EGFP-PP1CB*-MYPT1 <t>(D63A)</t> mutant and control construct with cotransfection of PCDH7c-V5 construct. Membranes were blotted using anti-V5, anti-MYPT1, anti-GFP and anti-tubulin antibodies. I (Input), FT(Flow Through), E (Elution) (D) Quantification of proximity ligation assay (PLA) showing fluorescence dots per cell for PCDH7- GFP (anti-GFP) and MYPT1 (anti-MYPT1) interaction (n=29) along with single primary antibody controls, MYPT1 (n=30) and GFP (n=30). ****p<0.0001.
    Egfp Pp1cb D63a Mypt1, supplied by Addgene inc, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/product/egfp+pp1cb+mypt1/bio_rxiv__2021__09__21__460794-205-15-11?v=Addgene+inc
    Average 94 stars, based on 1 article reviews
    egfp pp1cb d63a mypt1 - by Bioz Stars, 2026-07
    94/100 stars
      Buy from Supplier

    94
    Addgene inc egfp pp1cb mypt1
    (A) Depiction of relevant clusters of PCDH7 isoform-c interactome determined by GFP mediated affinity pulldown followed by LC-MS/MS. Red inset depicts a set of phosphatase subunits and phosphatase regulatory proteins, green inset highlighting components of myosin complexes, and blue inset showing members of ERM proteins. (B) Immunostaining of RPE1 cells expressing PCDH7-GFP (green), <t>MYPT1</t> (PPP1R12A) (red) and fluorescent phalloidin (blue). (C) Immunoblotting for GFP pulldown of <t>EGFP-PP1CB-MYPT1</t> fusion, EGFP-PP1CB*-MYPT1 <t>(D63A)</t> mutant and control construct with cotransfection of PCDH7c-V5 construct. Membranes were blotted using anti-V5, anti-MYPT1, anti-GFP and anti-tubulin antibodies. I (Input), FT(Flow Through), E (Elution) (D) Quantification of proximity ligation assay (PLA) showing fluorescence dots per cell for PCDH7- GFP (anti-GFP) and MYPT1 (anti-MYPT1) interaction (n=29) along with single primary antibody controls, MYPT1 (n=30) and GFP (n=30). ****p<0.0001.
    Egfp Pp1cb Mypt1, supplied by Addgene inc, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/product/egfp+pp1cb+mypt1/bio_rxiv__2021__09__21__460794-205-12-11?v=Addgene+inc
    Average 94 stars, based on 1 article reviews
    egfp pp1cb mypt1 - by Bioz Stars, 2026-07
    94/100 stars
      Buy from Supplier

    Image Search Results


    (A) Depiction of relevant clusters of PCDH7 isoform-c interactome determined by GFP mediated affinity pulldown followed by LC-MS/MS. Red inset depicts a set of phosphatase subunits and phosphatase regulatory proteins, green inset highlighting components of myosin complexes, and blue inset showing members of ERM proteins. (B) Immunostaining of RPE1 cells expressing PCDH7-GFP (green), MYPT1 (PPP1R12A) (red) and fluorescent phalloidin (blue). (C) Immunoblotting for GFP pulldown of EGFP-PP1CB-MYPT1 fusion, EGFP-PP1CB*-MYPT1 (D63A) mutant and control construct with cotransfection of PCDH7c-V5 construct. Membranes were blotted using anti-V5, anti-MYPT1, anti-GFP and anti-tubulin antibodies. I (Input), FT(Flow Through), E (Elution) (D) Quantification of proximity ligation assay (PLA) showing fluorescence dots per cell for PCDH7- GFP (anti-GFP) and MYPT1 (anti-MYPT1) interaction (n=29) along with single primary antibody controls, MYPT1 (n=30) and GFP (n=30). ****p<0.0001.

    Journal: bioRxiv

    Article Title: PCDH7 Promotes Cell Migration by Regulating Myosin Activity

    doi: 10.1101/2021.09.21.460794

    Figure Lengend Snippet: (A) Depiction of relevant clusters of PCDH7 isoform-c interactome determined by GFP mediated affinity pulldown followed by LC-MS/MS. Red inset depicts a set of phosphatase subunits and phosphatase regulatory proteins, green inset highlighting components of myosin complexes, and blue inset showing members of ERM proteins. (B) Immunostaining of RPE1 cells expressing PCDH7-GFP (green), MYPT1 (PPP1R12A) (red) and fluorescent phalloidin (blue). (C) Immunoblotting for GFP pulldown of EGFP-PP1CB-MYPT1 fusion, EGFP-PP1CB*-MYPT1 (D63A) mutant and control construct with cotransfection of PCDH7c-V5 construct. Membranes were blotted using anti-V5, anti-MYPT1, anti-GFP and anti-tubulin antibodies. I (Input), FT(Flow Through), E (Elution) (D) Quantification of proximity ligation assay (PLA) showing fluorescence dots per cell for PCDH7- GFP (anti-GFP) and MYPT1 (anti-MYPT1) interaction (n=29) along with single primary antibody controls, MYPT1 (n=30) and GFP (n=30). ****p<0.0001.

    Article Snippet: For PCDH7- V5 constructs, PCDH7b and PCDH7c were cloned into PLEX_307 (Addgene#41392). eGFP- PP1CB-MYPT1 and eGFP-PP1CB(D63A)-MYPT1 were provided by Mathieu Bollen from KU, Leuven and generated as previously described ( ).

    Techniques: Liquid Chromatography with Mass Spectroscopy, Immunostaining, Expressing, Western Blot, Mutagenesis, Construct, Cotransfection, Proximity Ligation Assay, Fluorescence