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pmrx-ip-gfp-lc3-rfp (Addgene inc)

Name: pmrx-ip-gfp-lc3-rfp
Brand: Addgene inc
Rating: 90 (1 reviews)

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Addgene inc pmrx-ip-gfp-lc3-rfp
Pmrx Ip Gfp Lc3 Rfp, supplied by Addgene inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/pmrx-ip-gfp-lc3-rfp/product/Addgene inc
Average 90 stars, based on 1 article reviews

pmrx-ip-gfp-lc3-rfp - by Bioz Stars, 2026-02

90/100 stars

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Flux and turnover assays for evaluating Abx-induced autophagic response in myeloma cells. (A) Change in <t>LC3-II</t> expression levels in myeloma cells by Abx treatment (flux assay). Western blots revealed time course increases in LC3-II expression in KMS21 and KMS34 cells after 100 μM Abx treatment. ∗ P < .05 vs 0 hour. (B) Change in p62/SQSTM1 expression in myeloma cells by Abx treatment. Time course changes in p62/SQSTM expression were evaluated by western blots in KMS21 and KMS34 cells after treatment with 100 μM Abx. ∗ P < .05 vs 0 hour. (C) Turnover assay of myeloma cells by Abx. KMS21 and KMS34 cells were exposed to 100 μM Abx for 24 hours and cotreated with 100 μM resveratrol (Res) for an additional 18 hours or 10 nM bafilomycin (Baf) A1 for an additional 2 hours. Changes in LC3-II expression were evaluated by western blot. (D) Reporter assay for evaluation of LC3-II turnover. pMRX-IP-GFP-LC3-RFP-LC3ΔG–transduced KMS34 cells were treated with 0, 200, or 400 μM Abx for 48 hours. Cells were cocultured with 100 μM Res or 50 nM Baf A1 for an additional 12 hours. The effect on autophagy was evaluated by fluorescence microscopy. GFP levels were semiquantified by flow cytometry using FlowJo software. Ax, ambroxol; ctrl, control.

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Flux and turnover assays for evaluating Abx-induced autophagic response in myeloma cells. (A) Change in LC3-II expression levels in myeloma cells by Abx treatment (flux assay). Western blots revealed time course increases in LC3-II expression in KMS21 and KMS34 cells after 100 μM Abx treatment. ∗ P < .05 vs 0 hour. (B) Change in p62/SQSTM1 expression in myeloma cells by Abx treatment. Time course changes in p62/SQSTM expression were evaluated by western blots in KMS21 and KMS34 cells after treatment with 100 μM Abx. ∗ P < .05 vs 0 hour. (C) Turnover assay of myeloma cells by Abx. KMS21 and KMS34 cells were exposed to 100 μM Abx for 24 hours and cotreated with 100 μM resveratrol (Res) for an additional 18 hours or 10 nM bafilomycin (Baf) A1 for an additional 2 hours. Changes in LC3-II expression were evaluated by western blot. (D) Reporter assay for evaluation of LC3-II turnover. pMRX-IP-GFP-LC3-RFP-LC3ΔG–transduced KMS34 cells were treated with 0, 200, or 400 μM Abx for 48 hours. Cells were cocultured with 100 μM Res or 50 nM Baf A1 for an additional 12 hours. The effect on autophagy was evaluated by fluorescence microscopy. GFP levels were semiquantified by flow cytometry using FlowJo software. Ax, ambroxol; ctrl, control.

Journal: Blood Neoplasia

Article Title: Ambroxol induces myeloma cell death by inhibiting autophagy

doi: 10.1016/j.bneo.2025.100100

Figure Lengend Snippet: Flux and turnover assays for evaluating Abx-induced autophagic response in myeloma cells. (A) Change in LC3-II expression levels in myeloma cells by Abx treatment (flux assay). Western blots revealed time course increases in LC3-II expression in KMS21 and KMS34 cells after 100 μM Abx treatment. ∗ P < .05 vs 0 hour. (B) Change in p62/SQSTM1 expression in myeloma cells by Abx treatment. Time course changes in p62/SQSTM expression were evaluated by western blots in KMS21 and KMS34 cells after treatment with 100 μM Abx. ∗ P < .05 vs 0 hour. (C) Turnover assay of myeloma cells by Abx. KMS21 and KMS34 cells were exposed to 100 μM Abx for 24 hours and cotreated with 100 μM resveratrol (Res) for an additional 18 hours or 10 nM bafilomycin (Baf) A1 for an additional 2 hours. Changes in LC3-II expression were evaluated by western blot. (D) Reporter assay for evaluation of LC3-II turnover. pMRX-IP-GFP-LC3-RFP-LC3ΔG–transduced KMS34 cells were treated with 0, 200, or 400 μM Abx for 48 hours. Cells were cocultured with 100 μM Res or 50 nM Baf A1 for an additional 12 hours. The effect on autophagy was evaluated by fluorescence microscopy. GFP levels were semiquantified by flow cytometry using FlowJo software. Ax, ambroxol; ctrl, control.

Article Snippet: For the fluorescent LC3 reporter assay, pMRX-IP-GFP-LC3-RFP-LC3ΔG (Addgene, Watertown, MA) was retrovirally transduced to KMS34 cells.

Techniques: Expressing, Flux Assay, Western Blot, Turnover Assay, Reporter Assay, Fluorescence, Microscopy, Flow Cytometry, Software, Control

$Flux assays and turnover assays of the effects of antimyeloma drugs used singly or in combination with Abx. (A) Change in LC3-II and p62/SQSTM1 expression levels in myeloma cells by existing antimyeloma drugs (flux assay). KMS34 cells were incubated with various concentrations of bortezomib (Btz), lenalidomide (Len), and panobinostat (Pan) for 72 hours, and the protein expressions were evaluated by western blots. ∗ P < .05 vs 0 nM. (B) Turnover assay using existing antimyeloma drugs. For Btz, KMS34 cells were incubated with 8 nM Btz for 3 hours, after which 1 nM Baf A1 or 100 μM Res was added. The cells were then incubated for an additional 3 and 12 hours, respectively. For Len, Len-sensitive MUM24 cells were cultured with 1 μM Len for 48 hours. Then, 1 nM Baf A1 or 100 μM Res was added to Len-pretreated MUM24 cells, and the cells were incubated for an additional 3 or 12 hours, respectively. For Pan, KMS34 cells were treated with 20 nM Pan for 48 hours. Then, 1 nM Baf A1 or 100 μM Res was added to Pan-pretreated KMS34 cells, and the cells were incubated for an additional 3 or 12 hours, respectively. LC3B-II and p62 levels were evaluated by western blots. ∗ P < .05. (C) Synergism of Abx with known antimyeloma drugs. KMS21, KMS34, and MUM24 cells were incubated with various concentrations of Abx plus Btz, Len, or Pan for 72 hours. Cell viability was evaluated by WST-1 assay. CIs were calculated by the Chou-Talalay method. Fa-CI plots are illustrated. (D) Growth inhibition by combination treatment of Abx plus Pan with or without Btz was evaluated by WST-1 assay. KMS21 and KMS34 cells were incubated with various concentrations of Abx in the presence of Pan and Btz for 72 hours. Abx0.5 (0.5 viability) compared with no drug treatment (1.0 viability) of the KMS21 and KMS34 cells are also found as Abx0.5. (E) MCL1 expression by Abx with antimyeloma drugs. KMS21 and KMS34 cells were treated with 200 μM Abx plus 8 nM Btz or 20 nM Pan for 24 hours. MCL1 expression was evaluated by western blot. ∗ P < .05; ∗∗ P < .01. (F) Western blot indicating caspase activation by combination treatment of Abx with Pan or Btz. KMS21 cells were treated with 200 μM Abx and 20 nM Pan or 8 nM Btz for 24 hours unless otherwise stated. (G) Expression levels of sirtuin 2, FOXK1, and ATG products and the level of UPR by combination treatment with 200 μM Abx and 20 nM Pan for 24 hours in KMS34 cells. RNA sequence analysis revealed that the Sirtuin 2 and FOXK1 gene expressions were upregulated by Abx treatment ( A-B). ctrl, control; Fa, fractional effect.$

Journal: Blood Neoplasia

Article Title: Ambroxol induces myeloma cell death by inhibiting autophagy

doi: 10.1016/j.bneo.2025.100100

Figure Lengend Snippet: Flux assays and turnover assays of the effects of antimyeloma drugs used singly or in combination with Abx. (A) Change in LC3-II and p62/SQSTM1 expression levels in myeloma cells by existing antimyeloma drugs (flux assay). KMS34 cells were incubated with various concentrations of bortezomib (Btz), lenalidomide (Len), and panobinostat (Pan) for 72 hours, and the protein expressions were evaluated by western blots. ∗ P < .05 vs 0 nM. (B) Turnover assay using existing antimyeloma drugs. For Btz, KMS34 cells were incubated with 8 nM Btz for 3 hours, after which 1 nM Baf A1 or 100 μM Res was added. The cells were then incubated for an additional 3 and 12 hours, respectively. For Len, Len-sensitive MUM24 cells were cultured with 1 μM Len for 48 hours. Then, 1 nM Baf A1 or 100 μM Res was added to Len-pretreated MUM24 cells, and the cells were incubated for an additional 3 or 12 hours, respectively. For Pan, KMS34 cells were treated with 20 nM Pan for 48 hours. Then, 1 nM Baf A1 or 100 μM Res was added to Pan-pretreated KMS34 cells, and the cells were incubated for an additional 3 or 12 hours, respectively. LC3B-II and p62 levels were evaluated by western blots. ∗ P < .05. (C) Synergism of Abx with known antimyeloma drugs. KMS21, KMS34, and MUM24 cells were incubated with various concentrations of Abx plus Btz, Len, or Pan for 72 hours. Cell viability was evaluated by WST-1 assay. CIs were calculated by the Chou-Talalay method. Fa-CI plots are illustrated. (D) Growth inhibition by combination treatment of Abx plus Pan with or without Btz was evaluated by WST-1 assay. KMS21 and KMS34 cells were incubated with various concentrations of Abx in the presence of Pan and Btz for 72 hours. Abx0.5 (0.5 viability) compared with no drug treatment (1.0 viability) of the KMS21 and KMS34 cells are also found as Abx0.5. (E) MCL1 expression by Abx with antimyeloma drugs. KMS21 and KMS34 cells were treated with 200 μM Abx plus 8 nM Btz or 20 nM Pan for 24 hours. MCL1 expression was evaluated by western blot. ∗ P < .05; ∗∗ P < .01. (F) Western blot indicating caspase activation by combination treatment of Abx with Pan or Btz. KMS21 cells were treated with 200 μM Abx and 20 nM Pan or 8 nM Btz for 24 hours unless otherwise stated. (G) Expression levels of sirtuin 2, FOXK1, and ATG products and the level of UPR by combination treatment with 200 μM Abx and 20 nM Pan for 24 hours in KMS34 cells. RNA sequence analysis revealed that the Sirtuin 2 and FOXK1 gene expressions were upregulated by Abx treatment ( A-B). ctrl, control; Fa, fractional effect.

Article Snippet: For the fluorescent LC3 reporter assay, pMRX-IP-GFP-LC3-RFP-LC3ΔG (Addgene, Watertown, MA) was retrovirally transduced to KMS34 cells.

Techniques: Expressing, Flux Assay, Incubation, Western Blot, Turnover Assay, Cell Culture, WST-1 Assay, Inhibition, Activation Assay, Sequencing, Control