g actin cytoskeleton polymerization Search Results


rala g lisa activation assay  (Cytoskeleton Inc)
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Cytoskeleton Inc rala g lisa activation assay
Rala G Lisa Activation Assay, supplied by Cytoskeleton Inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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biotinylated g-actin  (Cytoskeleton Inc)
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Cytoskeleton Inc biotinylated g-actin
Biotinylated G Actin, supplied by Cytoskeleton Inc, 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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p21 rac1 activated kinase 1 pak1  (Cytoskeleton Inc)
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Cytoskeleton Inc p21 rac1 activated kinase 1 pak1
P21 Rac1 Activated Kinase 1 Pak1, supplied by Cytoskeleton Inc, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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vivo assay kit  (Cytoskeleton Inc)
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Vivo Assay Kit, supplied by Cytoskeleton Inc, used in various techniques. Bioz Stars score: 97/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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cdc42 activation kit  (Cytoskeleton Inc)
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Cytoskeleton Inc cdc42 activation kit
Par6 and ECT2 activate <t>Cdc42</t> and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.
Cdc42 Activation Kit, supplied by Cytoskeleton Inc, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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monomeric actin g actin  (Cytoskeleton Inc)
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Cytoskeleton Inc monomeric actin g actin
Par6 and ECT2 activate <t>Cdc42</t> and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.
Monomeric Actin G Actin, supplied by Cytoskeleton Inc, 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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cba 110 rhoa rac1 cdc42 g lisa activation kit cytoskeleton inc  (Cytoskeleton Inc)
94
Cytoskeleton Inc cba 110 rhoa rac1 cdc42 g lisa activation kit cytoskeleton inc
Par6 and ECT2 activate <t>Cdc42</t> and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.
Cba 110 Rhoa Rac1 Cdc42 G Lisa Activation Kit Cytoskeleton Inc, supplied by Cytoskeleton Inc, 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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spy555 actin probe  (Cytoskeleton Inc)
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Cytoskeleton Inc spy555 actin probe
Par6 and ECT2 activate <t>Cdc42</t> and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.
Spy555 Actin Probe, supplied by Cytoskeleton Inc, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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rabbit anti rhoa antibody  (Cytoskeleton Inc)
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Cytoskeleton Inc rabbit anti rhoa antibody
Par6 and ECT2 activate <t>Cdc42</t> and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.
Rabbit Anti Rhoa Antibody, supplied by Cytoskeleton Inc, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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unlabeled g actin  (Cytoskeleton Inc)
96
Cytoskeleton Inc unlabeled g actin
Par6 and ECT2 activate <t>Cdc42</t> and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.
Unlabeled G Actin, supplied by Cytoskeleton Inc, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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actin stain 555 phalloidin  (Cytoskeleton Inc)
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Cytoskeleton Inc actin stain 555 phalloidin
Par6 and ECT2 activate <t>Cdc42</t> and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.
Actin Stain 555 Phalloidin, supplied by Cytoskeleton Inc, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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mouse anti rhoa  (Cytoskeleton Inc)
94
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Par6 and ECT2 activate <t>Cdc42</t> and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.
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Image Search Results


Par6 and ECT2 activate Cdc42 and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.

Journal:

Article Title: Nucleotide Exchange Factor ECT2 Interacts with the Polarity Protein Complex Par6/Par3/Protein Kinase C? (PKC?) and Regulates PKC? Activity

doi: 10.1128/MCB.24.15.6665-6675.2004

Figure Lengend Snippet: Par6 and ECT2 activate Cdc42 and PKCζ. (A) (Left panel) HeLa cells transfected with Myc-ECT2-ΔN5 together with Flag-Par6C vector or vector alone were lysed, and GTP-bound Cdc42 was pulled down with GST-PBD beads. The Western blot was carried out with anti-Cdc42 antibody. (Right panel) Similar experiments were performed in MDCK cells except that Flag-ECT2-ΔN5 was used. Accumulation of GTP-bound Rac1 was also estimated (lower panel). Similar results were obtained in three independent experiments. (B) Silencing of ECT2 reduces GTP-bound Cdc42. HeLa cells were treated with ECT2 siRNA or control luciferase siRNA (co) for 5 h and then transfected with Flag-Par6C. Cells were lysed 20 h after transfection, and GTP-bound Cdc42 was pulled down with GST-PBD-Sepharose beads. Western blots were carried out with anti-Cdc42, anti-ECT2, or anti-Flag antibody. These results were reproduced in three independent experiments. (C) ECT2 stimulates PKCζ activity. Cos7 cells transfected with the HA-tagged PKCζ expression vector in combination with the ECT2 and Flag-Par6C vectors or vector alone were lysed, and HA-PKCζ was immunoprecipitated with anti-HA antibody. PKCζ activity was estimated by in vitro kinase assays with myelin basic protein as the substrate, followed by autoradiography (upper panel). The level of HA-PKCζ was detected by immunoblotting with anti-HA antibody (lower panel). X-ray-films were scanned, and signals were quantitated with NIH Image software. Data are representative of three independent experiments.

Article Snippet: GTP-bound Cdc42 was estimated by the Cdc42 activation kit (Cytoskeleton Inc.).

Techniques: Transfection, Plasmid Preparation, Western Blot, Luciferase, Activity Assay, Expressing, Immunoprecipitation, In Vitro, Autoradiography, Software