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rho activator i  (Cytoskeleton Inc)


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    Structured Review

    Cytoskeleton Inc rho activator i
    Rho Activator I, supplied by Cytoskeleton Inc, used in various techniques. Bioz Stars score: 95/100, based on 69 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/rho activator i/product/Cytoskeleton Inc
    Average 95 stars, based on 69 article reviews
    rho activator i - by Bioz Stars, 2026-03
    95/100 stars

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    Dsg3 in response to inter- and intra-cellular force changes (A) Schematic diagram of Dsg3 tension sensor (TS) and tailless control sensor (TL). TSMod was inserted into the intracellular domain of Dsg3. (B) Immunostaining images of desmoplakin (DP) for HaCaT cells expressing Dsg3 TS or TL. Cells were immunostained for DP to check for the co-expression with sensors and nuclei were labeled with DAPI. Scale bar: 10 μm. (C) Immunogold image for HaCaT cells expressing the Dsg3 tension sensor. Positive signals were observed at desmosomes, suggesting that Dsg3 tension sensors incorporated into desmosomal cadherins. Scale bar: 500 nm. (D) Fluorescent images of donor (mTFP) and acceptor (Venus) and heatmap images of FRET ratio when Dsg3 TS/Dsg3 TL expressed HaCaT cells were exposed to EGTA for 30 min, 5 mM RhoA activator <t>(CN01)</t> for 30 min, ROCK inhibitor (Y27632) for 12h. Scale bar: 10 μm. (E and F) Quantitative analysis of FRET ratio at the cell-cell contact shown in D. (G) Heatmap images of FRET ratio in HaCaT cells treated with the following conditions: untreated control (No Abs), 2 μg/mL AK23 (AK23-2), 10 μg/mL AK23 (AK23-10), 2 μg/mL PVIgG (PVIgG-2) and 100 μg/mL PVIgG (PVIgG-100) at 0h, 4h, 8h, and 24h. Scale bar: 10 μm. (H) Quantitative analysis of corresponding FRET ratio. All values are mean ± SD ( n ≥ 30). ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.005, ns, p > 0.05. Three repeats for all conditions.
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    Dsg3 in response to inter- and intra-cellular force changes (A) Schematic diagram of Dsg3 tension sensor (TS) and tailless control sensor (TL). TSMod was inserted into the intracellular domain of Dsg3. (B) Immunostaining images of desmoplakin (DP) for HaCaT cells expressing Dsg3 TS or TL. Cells were immunostained for DP to check for the co-expression with sensors and nuclei were labeled with DAPI. Scale bar: 10 μm. (C) Immunogold image for HaCaT cells expressing the Dsg3 tension sensor. Positive signals were observed at desmosomes, suggesting that Dsg3 tension sensors incorporated into desmosomal cadherins. Scale bar: 500 nm. (D) Fluorescent images of donor (mTFP) and acceptor (Venus) and heatmap images of FRET ratio when Dsg3 TS/Dsg3 TL expressed HaCaT cells were exposed to EGTA for 30 min, 5 mM RhoA activator <t>(CN01)</t> for 30 min, ROCK inhibitor (Y27632) for 12h. Scale bar: 10 μm. (E and F) Quantitative analysis of FRET ratio at the cell-cell contact shown in D. (G) Heatmap images of FRET ratio in HaCaT cells treated with the following conditions: untreated control (No Abs), 2 μg/mL AK23 (AK23-2), 10 μg/mL AK23 (AK23-10), 2 μg/mL PVIgG (PVIgG-2) and 100 μg/mL PVIgG (PVIgG-100) at 0h, 4h, 8h, and 24h. Scale bar: 10 μm. (H) Quantitative analysis of corresponding FRET ratio. All values are mean ± SD ( n ≥ 30). ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.005, ns, p > 0.05. Three repeats for all conditions.
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    Dsg3 in response to inter- and intra-cellular force changes (A) Schematic diagram of Dsg3 tension sensor (TS) and tailless control sensor (TL). TSMod was inserted into the intracellular domain of Dsg3. (B) Immunostaining images of desmoplakin (DP) for HaCaT cells expressing Dsg3 TS or TL. Cells were immunostained for DP to check for the co-expression with sensors and nuclei were labeled with DAPI. Scale bar: 10 μm. (C) Immunogold image for HaCaT cells expressing the Dsg3 tension sensor. Positive signals were observed at desmosomes, suggesting that Dsg3 tension sensors incorporated into desmosomal cadherins. Scale bar: 500 nm. (D) Fluorescent images of donor (mTFP) and acceptor (Venus) and heatmap images of FRET ratio when Dsg3 TS/Dsg3 TL expressed HaCaT cells were exposed to EGTA for 30 min, 5 mM RhoA activator <t>(CN01)</t> for 30 min, ROCK inhibitor (Y27632) for 12h. Scale bar: 10 μm. (E and F) Quantitative analysis of FRET ratio at the cell-cell contact shown in D. (G) Heatmap images of FRET ratio in HaCaT cells treated with the following conditions: untreated control (No Abs), 2 μg/mL AK23 (AK23-2), 10 μg/mL AK23 (AK23-10), 2 μg/mL PVIgG (PVIgG-2) and 100 μg/mL PVIgG (PVIgG-100) at 0h, 4h, 8h, and 24h. Scale bar: 10 μm. (H) Quantitative analysis of corresponding FRET ratio. All values are mean ± SD ( n ≥ 30). ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.005, ns, p > 0.05. Three repeats for all conditions.
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    Image Search Results


    Dsg3 in response to inter- and intra-cellular force changes (A) Schematic diagram of Dsg3 tension sensor (TS) and tailless control sensor (TL). TSMod was inserted into the intracellular domain of Dsg3. (B) Immunostaining images of desmoplakin (DP) for HaCaT cells expressing Dsg3 TS or TL. Cells were immunostained for DP to check for the co-expression with sensors and nuclei were labeled with DAPI. Scale bar: 10 μm. (C) Immunogold image for HaCaT cells expressing the Dsg3 tension sensor. Positive signals were observed at desmosomes, suggesting that Dsg3 tension sensors incorporated into desmosomal cadherins. Scale bar: 500 nm. (D) Fluorescent images of donor (mTFP) and acceptor (Venus) and heatmap images of FRET ratio when Dsg3 TS/Dsg3 TL expressed HaCaT cells were exposed to EGTA for 30 min, 5 mM RhoA activator (CN01) for 30 min, ROCK inhibitor (Y27632) for 12h. Scale bar: 10 μm. (E and F) Quantitative analysis of FRET ratio at the cell-cell contact shown in D. (G) Heatmap images of FRET ratio in HaCaT cells treated with the following conditions: untreated control (No Abs), 2 μg/mL AK23 (AK23-2), 10 μg/mL AK23 (AK23-10), 2 μg/mL PVIgG (PVIgG-2) and 100 μg/mL PVIgG (PVIgG-100) at 0h, 4h, 8h, and 24h. Scale bar: 10 μm. (H) Quantitative analysis of corresponding FRET ratio. All values are mean ± SD ( n ≥ 30). ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.005, ns, p > 0.05. Three repeats for all conditions.

    Journal: iScience

    Article Title: Desmosomal cadherin tension loss in pemphigus vulgaris mediated by the inhibition of active RhoA at cell-cell adhesions

    doi: 10.1016/j.isci.2025.113081

    Figure Lengend Snippet: Dsg3 in response to inter- and intra-cellular force changes (A) Schematic diagram of Dsg3 tension sensor (TS) and tailless control sensor (TL). TSMod was inserted into the intracellular domain of Dsg3. (B) Immunostaining images of desmoplakin (DP) for HaCaT cells expressing Dsg3 TS or TL. Cells were immunostained for DP to check for the co-expression with sensors and nuclei were labeled with DAPI. Scale bar: 10 μm. (C) Immunogold image for HaCaT cells expressing the Dsg3 tension sensor. Positive signals were observed at desmosomes, suggesting that Dsg3 tension sensors incorporated into desmosomal cadherins. Scale bar: 500 nm. (D) Fluorescent images of donor (mTFP) and acceptor (Venus) and heatmap images of FRET ratio when Dsg3 TS/Dsg3 TL expressed HaCaT cells were exposed to EGTA for 30 min, 5 mM RhoA activator (CN01) for 30 min, ROCK inhibitor (Y27632) for 12h. Scale bar: 10 μm. (E and F) Quantitative analysis of FRET ratio at the cell-cell contact shown in D. (G) Heatmap images of FRET ratio in HaCaT cells treated with the following conditions: untreated control (No Abs), 2 μg/mL AK23 (AK23-2), 10 μg/mL AK23 (AK23-10), 2 μg/mL PVIgG (PVIgG-2) and 100 μg/mL PVIgG (PVIgG-100) at 0h, 4h, 8h, and 24h. Scale bar: 10 μm. (H) Quantitative analysis of corresponding FRET ratio. All values are mean ± SD ( n ≥ 30). ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.005, ns, p > 0.05. Three repeats for all conditions.

    Article Snippet: Rho activator I (CN01) (Cytoskeleton) was used at a concentration of 1 unit/mL.

    Techniques: Control, Immunostaining, Expressing, Labeling

    PV Ab-induced tension loss at Dsg3 inhibits RhoA (A and B) Heatmap images and quantitative analysis of RhoA FRET ratio show the activities of active RhoA in response to 2 μg/mL AK23 and 10 μM Y27632 at 4h and 24h. All values are mean ± SD ( n ≥ 30). (C) Western blot results for active RhoA and total RhoA under treatment of AK23, Y27632 and AK23+CN01 compared with controls (No Abs) for 4h and 24h. (D) Quantified western blot data for the ratio of active RhoA/total RhoA under AK23 and Y27632 treatment for 4h and 24 h, compared with controls. All values are mean ± SD ( n ≥ 3). (E–H) RhoA FRET ratio in HaCaT cells exposed to 2 μg/mL of AK23, PX4-4, PX4-3, anti-TPO, AtS13, and PVIgG at 30 min, 4h, 8h, and 24h. All values are mean ± SD ( n ≥ 30). (I) Summary of the significance of RhoA FRET ratio change over 24h for the Abs tested (blue = no change, white = significant decrease). ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.005, ns, p > 0.05. Scale bar: 10 μm. Three repeats for all conditions.

    Journal: iScience

    Article Title: Desmosomal cadherin tension loss in pemphigus vulgaris mediated by the inhibition of active RhoA at cell-cell adhesions

    doi: 10.1016/j.isci.2025.113081

    Figure Lengend Snippet: PV Ab-induced tension loss at Dsg3 inhibits RhoA (A and B) Heatmap images and quantitative analysis of RhoA FRET ratio show the activities of active RhoA in response to 2 μg/mL AK23 and 10 μM Y27632 at 4h and 24h. All values are mean ± SD ( n ≥ 30). (C) Western blot results for active RhoA and total RhoA under treatment of AK23, Y27632 and AK23+CN01 compared with controls (No Abs) for 4h and 24h. (D) Quantified western blot data for the ratio of active RhoA/total RhoA under AK23 and Y27632 treatment for 4h and 24 h, compared with controls. All values are mean ± SD ( n ≥ 3). (E–H) RhoA FRET ratio in HaCaT cells exposed to 2 μg/mL of AK23, PX4-4, PX4-3, anti-TPO, AtS13, and PVIgG at 30 min, 4h, 8h, and 24h. All values are mean ± SD ( n ≥ 30). (I) Summary of the significance of RhoA FRET ratio change over 24h for the Abs tested (blue = no change, white = significant decrease). ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.005, ns, p > 0.05. Scale bar: 10 μm. Three repeats for all conditions.

    Article Snippet: Rho activator I (CN01) (Cytoskeleton) was used at a concentration of 1 unit/mL.

    Techniques: Western Blot

    Activation of RhoA restores the tension loss at cell adhesion induced by PV Abs HaCaT cells were with both 2 μg/mL of AK23 and 1 unit/mL CN01 at 4h and 24h, with CN01 being added in the final 30 min of the treatment. (A) CN01 increases the RhoA FRET ratio at both 4h and 24h. All values are mean ± SD ( n ≥ 30). (B) Quantified western blot data showing the ratio of active RhoA/total RhoA with AK23+CN01 treatment compared with controls (No Abs) for 4h and 24h. This quantifies the controls and AK23+CN01 western blot results shown in C. All values are mean ± SD ( n ≥ 3). (C) CN01 reduces the Dsg3 FRET ratio. All values are mean ± SD ( n ≥ 30). (D–F) Traction stress and junctional traction stress are increased in HaCaT cells treated with CN01. All values are mean ± SD ( n ≥ 30). ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.005, ns, p > 0.05. Scale bar: 15 μm. Three repeats for all conditions.

    Journal: iScience

    Article Title: Desmosomal cadherin tension loss in pemphigus vulgaris mediated by the inhibition of active RhoA at cell-cell adhesions

    doi: 10.1016/j.isci.2025.113081

    Figure Lengend Snippet: Activation of RhoA restores the tension loss at cell adhesion induced by PV Abs HaCaT cells were with both 2 μg/mL of AK23 and 1 unit/mL CN01 at 4h and 24h, with CN01 being added in the final 30 min of the treatment. (A) CN01 increases the RhoA FRET ratio at both 4h and 24h. All values are mean ± SD ( n ≥ 30). (B) Quantified western blot data showing the ratio of active RhoA/total RhoA with AK23+CN01 treatment compared with controls (No Abs) for 4h and 24h. This quantifies the controls and AK23+CN01 western blot results shown in C. All values are mean ± SD ( n ≥ 3). (C) CN01 reduces the Dsg3 FRET ratio. All values are mean ± SD ( n ≥ 30). (D–F) Traction stress and junctional traction stress are increased in HaCaT cells treated with CN01. All values are mean ± SD ( n ≥ 30). ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.005, ns, p > 0.05. Scale bar: 15 μm. Three repeats for all conditions.

    Article Snippet: Rho activator I (CN01) (Cytoskeleton) was used at a concentration of 1 unit/mL.

    Techniques: Activation Assay, Western Blot