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live cell staining kit  (Beyotime)


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    Structured Review

    Beyotime live cell staining kit
    Characteristics of DMP nanoparticles and the proliferation-inhibiting effect of the DMP-mBim complex in vitro. ( A ) Size distribution and zeta potential of DMP nanoparticles. ( B ) Transmission electron microscopy (TEM) photomicrographs of DMP stained with phosphotungstic acid solution (scale bar: 50 nm). ( C ) <t>Cell</t> viability MTT assay of DMP and PEI25K in 293T cells. ( D ) Hemolysis test of DMP nanoparticles, Triton X-100 was used as positive control, and normal saline was used as negative control (***P<0.001, ****P<0.0001). ( E ) Critical micelle concentration evaluation of DMP using pyrene as the fluorescent dye. ( F ) Murine Bim mRNA (mBim) obtained by the in vitro transcription method was detected by electrophoresis. ( G ) Gel-retardation assay of mRNA and DMP at different weight ratios. ( H ) RNase protection electrophoresis assay of the DMP-mRNA complex. ( I ) Transfection efficiency of DMP-EGFP in SCC-VII cells (scale bar: 100 μm). ( J ) Bim levels in SCC-VII cells after DMP-mBim complex transfection (***P<0.001). ( K ) MTT assay of SCC-VII cells after DMP-mBim transfection and representative images. The cell viability and inhibition rate were also calculated (scale bar: 100 μm, ****P<0.0001). ( L ) Proliferation-inhibition ability of the DMP-mBim complex on SCC-VII cells evaluated by clonogenic assay (****P<0.0001). ( M ) Apoptosis-inducing ability of DMP-mBim complex in SCC-VII cells using Annexin V/PI <t>staining</t> by flow cytometry (****P<0.0001). ( N ) <t>Live/dead</t> staining evaluation of SCC-VII cells treated with the DMP-mBim complex (scale bar: 100 μm, ****P<0.0001).
    Live Cell Staining Kit, supplied by Beyotime, used in various techniques. Bioz Stars score: 99/100, based on 40 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/product/live+cell+staining+kit/pmc13025768-145-21-25?v=Beyotime
    Average 99 stars, based on 40 article reviews
    live cell staining kit - by Bioz Stars, 2026-07
    99/100 stars

    Images

    1) Product Images from "Sequential Release of mRNA Complex and T Cells by a Double-Layered Implantable Scaffold for Combination Therapy of Head and Neck Squamous Cell Carcinoma"

    Article Title: Sequential Release of mRNA Complex and T Cells by a Double-Layered Implantable Scaffold for Combination Therapy of Head and Neck Squamous Cell Carcinoma

    Journal: International Journal of Nanomedicine

    doi: 10.2147/IJN.S582078

    Characteristics of DMP nanoparticles and the proliferation-inhibiting effect of the DMP-mBim complex in vitro. ( A ) Size distribution and zeta potential of DMP nanoparticles. ( B ) Transmission electron microscopy (TEM) photomicrographs of DMP stained with phosphotungstic acid solution (scale bar: 50 nm). ( C ) Cell viability MTT assay of DMP and PEI25K in 293T cells. ( D ) Hemolysis test of DMP nanoparticles, Triton X-100 was used as positive control, and normal saline was used as negative control (***P<0.001, ****P<0.0001). ( E ) Critical micelle concentration evaluation of DMP using pyrene as the fluorescent dye. ( F ) Murine Bim mRNA (mBim) obtained by the in vitro transcription method was detected by electrophoresis. ( G ) Gel-retardation assay of mRNA and DMP at different weight ratios. ( H ) RNase protection electrophoresis assay of the DMP-mRNA complex. ( I ) Transfection efficiency of DMP-EGFP in SCC-VII cells (scale bar: 100 μm). ( J ) Bim levels in SCC-VII cells after DMP-mBim complex transfection (***P<0.001). ( K ) MTT assay of SCC-VII cells after DMP-mBim transfection and representative images. The cell viability and inhibition rate were also calculated (scale bar: 100 μm, ****P<0.0001). ( L ) Proliferation-inhibition ability of the DMP-mBim complex on SCC-VII cells evaluated by clonogenic assay (****P<0.0001). ( M ) Apoptosis-inducing ability of DMP-mBim complex in SCC-VII cells using Annexin V/PI staining by flow cytometry (****P<0.0001). ( N ) Live/dead staining evaluation of SCC-VII cells treated with the DMP-mBim complex (scale bar: 100 μm, ****P<0.0001).
    Figure Legend Snippet: Characteristics of DMP nanoparticles and the proliferation-inhibiting effect of the DMP-mBim complex in vitro. ( A ) Size distribution and zeta potential of DMP nanoparticles. ( B ) Transmission electron microscopy (TEM) photomicrographs of DMP stained with phosphotungstic acid solution (scale bar: 50 nm). ( C ) Cell viability MTT assay of DMP and PEI25K in 293T cells. ( D ) Hemolysis test of DMP nanoparticles, Triton X-100 was used as positive control, and normal saline was used as negative control (***P<0.001, ****P<0.0001). ( E ) Critical micelle concentration evaluation of DMP using pyrene as the fluorescent dye. ( F ) Murine Bim mRNA (mBim) obtained by the in vitro transcription method was detected by electrophoresis. ( G ) Gel-retardation assay of mRNA and DMP at different weight ratios. ( H ) RNase protection electrophoresis assay of the DMP-mRNA complex. ( I ) Transfection efficiency of DMP-EGFP in SCC-VII cells (scale bar: 100 μm). ( J ) Bim levels in SCC-VII cells after DMP-mBim complex transfection (***P<0.001). ( K ) MTT assay of SCC-VII cells after DMP-mBim transfection and representative images. The cell viability and inhibition rate were also calculated (scale bar: 100 μm, ****P<0.0001). ( L ) Proliferation-inhibition ability of the DMP-mBim complex on SCC-VII cells evaluated by clonogenic assay (****P<0.0001). ( M ) Apoptosis-inducing ability of DMP-mBim complex in SCC-VII cells using Annexin V/PI staining by flow cytometry (****P<0.0001). ( N ) Live/dead staining evaluation of SCC-VII cells treated with the DMP-mBim complex (scale bar: 100 μm, ****P<0.0001).

    Techniques Used: In Vitro, Zeta Potential Analyzer, Transmission Assay, Electron Microscopy, Staining, MTT Assay, Positive Control, Saline, Negative Control, Concentration Assay, Electrophoresis, Electrophoretic Mobility Shift Assay, Transfection, Inhibition, Clonogenic Assay, Flow Cytometry

    Transfection efficiency and treatment effect of DMP-mBim complex after release from scaffold. ( A and B ) Representative fluorescence images of SCC-VII cells transfected with supernatants of the outer layer of the scaffold containing the DMP-EGFP complex in short-term release (scale bar: 50 μm) and detection of efficiency by flow cytometry. ( C and D ) Representative fluorescence images of SCC-VII cells transfected with supernatants of the outer layer of the scaffold containing the DMP-EGFP complex in long-term release (scale bar: 100 μm) and the calculated transfection efficiency. ( E ) Cumulative RNA-release rate in the outer layer scaffold. ( F ) Bim levels in SCC-VII cells after treatment with supernatants of the outer layer of the scaffold containing DMP-mBim complex (***P<0.001). ( G and H ) MTT assay of SCC-VII cells after treatment with the supernatants of the outer layer of the scaffold containing DMP-mBim complex (scale bar: 100 μm, ****P<0.0001, **P<0.01). ( I ) Live/dead staining evaluation of SCC-VII cells treated with the supernatants of the outer layer of the scaffold (scale bar: 100 μm, ****P<0.0001).
    Figure Legend Snippet: Transfection efficiency and treatment effect of DMP-mBim complex after release from scaffold. ( A and B ) Representative fluorescence images of SCC-VII cells transfected with supernatants of the outer layer of the scaffold containing the DMP-EGFP complex in short-term release (scale bar: 50 μm) and detection of efficiency by flow cytometry. ( C and D ) Representative fluorescence images of SCC-VII cells transfected with supernatants of the outer layer of the scaffold containing the DMP-EGFP complex in long-term release (scale bar: 100 μm) and the calculated transfection efficiency. ( E ) Cumulative RNA-release rate in the outer layer scaffold. ( F ) Bim levels in SCC-VII cells after treatment with supernatants of the outer layer of the scaffold containing DMP-mBim complex (***P<0.001). ( G and H ) MTT assay of SCC-VII cells after treatment with the supernatants of the outer layer of the scaffold containing DMP-mBim complex (scale bar: 100 μm, ****P<0.0001, **P<0.01). ( I ) Live/dead staining evaluation of SCC-VII cells treated with the supernatants of the outer layer of the scaffold (scale bar: 100 μm, ****P<0.0001).

    Techniques Used: Transfection, Fluorescence, Flow Cytometry, MTT Assay, Staining



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    Characteristics of DMP nanoparticles and the proliferation-inhibiting effect of the DMP-mBim complex in vitro. ( A ) Size distribution and zeta potential of DMP nanoparticles. ( B ) Transmission electron microscopy (TEM) photomicrographs of DMP stained with phosphotungstic acid solution (scale bar: 50 nm). ( C ) <t>Cell</t> viability MTT assay of DMP and PEI25K in 293T cells. ( D ) Hemolysis test of DMP nanoparticles, Triton X-100 was used as positive control, and normal saline was used as negative control (***P<0.001, ****P<0.0001). ( E ) Critical micelle concentration evaluation of DMP using pyrene as the fluorescent dye. ( F ) Murine Bim mRNA (mBim) obtained by the in vitro transcription method was detected by electrophoresis. ( G ) Gel-retardation assay of mRNA and DMP at different weight ratios. ( H ) RNase protection electrophoresis assay of the DMP-mRNA complex. ( I ) Transfection efficiency of DMP-EGFP in SCC-VII cells (scale bar: 100 μm). ( J ) Bim levels in SCC-VII cells after DMP-mBim complex transfection (***P<0.001). ( K ) MTT assay of SCC-VII cells after DMP-mBim transfection and representative images. The cell viability and inhibition rate were also calculated (scale bar: 100 μm, ****P<0.0001). ( L ) Proliferation-inhibition ability of the DMP-mBim complex on SCC-VII cells evaluated by clonogenic assay (****P<0.0001). ( M ) Apoptosis-inducing ability of DMP-mBim complex in SCC-VII cells using Annexin V/PI <t>staining</t> by flow cytometry (****P<0.0001). ( N ) <t>Live/dead</t> staining evaluation of SCC-VII cells treated with the DMP-mBim complex (scale bar: 100 μm, ****P<0.0001).
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    Biocompatibility and cell adhesion of the bone marrow mesenchymal stem cells (BMSCs) in different groups. (A) Cell viability at day 1, 4 and 7 via the CCK-8 assay. (B) Percentage of live cells at day 1 assessed by Live/Dead staining. (C) Proportion of adherent BMSCs. (D) Representative fluorescence images of BMSCs obtained by Live/Dead staining. (E) Representative fluorescence images of adherent BMSCs stained with phalloidin. ∗∗ p < 0.01, and ∗∗∗ p < 0.001, n = 3.

    Journal: Materials Today Bio

    Article Title: 3D-printed titanium scaffolds coated with a multifunctional photothermal-responsive hydrogel promote osteoporotic bone defect repair

    doi: 10.1016/j.mtbio.2026.102879

    Figure Lengend Snippet: Biocompatibility and cell adhesion of the bone marrow mesenchymal stem cells (BMSCs) in different groups. (A) Cell viability at day 1, 4 and 7 via the CCK-8 assay. (B) Percentage of live cells at day 1 assessed by Live/Dead staining. (C) Proportion of adherent BMSCs. (D) Representative fluorescence images of BMSCs obtained by Live/Dead staining. (E) Representative fluorescence images of adherent BMSCs stained with phalloidin. ∗∗ p < 0.01, and ∗∗∗ p < 0.001, n = 3.

    Article Snippet: A live/dead cell double-staining kit (KGA9501-100) was obtained from KeyGENBiotech (Nanjing, China), and a CCK-8 assay kit (TM772) was purchased from Dojindo (Tokyo, Japan).

    Techniques: CCK-8 Assay, Staining, Fluorescence

    Characteristics of DMP nanoparticles and the proliferation-inhibiting effect of the DMP-mBim complex in vitro. ( A ) Size distribution and zeta potential of DMP nanoparticles. ( B ) Transmission electron microscopy (TEM) photomicrographs of DMP stained with phosphotungstic acid solution (scale bar: 50 nm). ( C ) Cell viability MTT assay of DMP and PEI25K in 293T cells. ( D ) Hemolysis test of DMP nanoparticles, Triton X-100 was used as positive control, and normal saline was used as negative control (***P<0.001, ****P<0.0001). ( E ) Critical micelle concentration evaluation of DMP using pyrene as the fluorescent dye. ( F ) Murine Bim mRNA (mBim) obtained by the in vitro transcription method was detected by electrophoresis. ( G ) Gel-retardation assay of mRNA and DMP at different weight ratios. ( H ) RNase protection electrophoresis assay of the DMP-mRNA complex. ( I ) Transfection efficiency of DMP-EGFP in SCC-VII cells (scale bar: 100 μm). ( J ) Bim levels in SCC-VII cells after DMP-mBim complex transfection (***P<0.001). ( K ) MTT assay of SCC-VII cells after DMP-mBim transfection and representative images. The cell viability and inhibition rate were also calculated (scale bar: 100 μm, ****P<0.0001). ( L ) Proliferation-inhibition ability of the DMP-mBim complex on SCC-VII cells evaluated by clonogenic assay (****P<0.0001). ( M ) Apoptosis-inducing ability of DMP-mBim complex in SCC-VII cells using Annexin V/PI staining by flow cytometry (****P<0.0001). ( N ) Live/dead staining evaluation of SCC-VII cells treated with the DMP-mBim complex (scale bar: 100 μm, ****P<0.0001).

    Journal: International Journal of Nanomedicine

    Article Title: Sequential Release of mRNA Complex and T Cells by a Double-Layered Implantable Scaffold for Combination Therapy of Head and Neck Squamous Cell Carcinoma

    doi: 10.2147/IJN.S582078

    Figure Lengend Snippet: Characteristics of DMP nanoparticles and the proliferation-inhibiting effect of the DMP-mBim complex in vitro. ( A ) Size distribution and zeta potential of DMP nanoparticles. ( B ) Transmission electron microscopy (TEM) photomicrographs of DMP stained with phosphotungstic acid solution (scale bar: 50 nm). ( C ) Cell viability MTT assay of DMP and PEI25K in 293T cells. ( D ) Hemolysis test of DMP nanoparticles, Triton X-100 was used as positive control, and normal saline was used as negative control (***P<0.001, ****P<0.0001). ( E ) Critical micelle concentration evaluation of DMP using pyrene as the fluorescent dye. ( F ) Murine Bim mRNA (mBim) obtained by the in vitro transcription method was detected by electrophoresis. ( G ) Gel-retardation assay of mRNA and DMP at different weight ratios. ( H ) RNase protection electrophoresis assay of the DMP-mRNA complex. ( I ) Transfection efficiency of DMP-EGFP in SCC-VII cells (scale bar: 100 μm). ( J ) Bim levels in SCC-VII cells after DMP-mBim complex transfection (***P<0.001). ( K ) MTT assay of SCC-VII cells after DMP-mBim transfection and representative images. The cell viability and inhibition rate were also calculated (scale bar: 100 μm, ****P<0.0001). ( L ) Proliferation-inhibition ability of the DMP-mBim complex on SCC-VII cells evaluated by clonogenic assay (****P<0.0001). ( M ) Apoptosis-inducing ability of DMP-mBim complex in SCC-VII cells using Annexin V/PI staining by flow cytometry (****P<0.0001). ( N ) Live/dead staining evaluation of SCC-VII cells treated with the DMP-mBim complex (scale bar: 100 μm, ****P<0.0001).

    Article Snippet: Cells were dual-stained for the plasma membrane and tubulin using DiI (Cell Plasma Membrane Staining Kit; Beyotime, China) and Tubulin-Tracker Green (Live Cell Staining Kit; Beyotime, China).

    Techniques: In Vitro, Zeta Potential Analyzer, Transmission Assay, Electron Microscopy, Staining, MTT Assay, Positive Control, Saline, Negative Control, Concentration Assay, Electrophoresis, Electrophoretic Mobility Shift Assay, Transfection, Inhibition, Clonogenic Assay, Flow Cytometry

    Transfection efficiency and treatment effect of DMP-mBim complex after release from scaffold. ( A and B ) Representative fluorescence images of SCC-VII cells transfected with supernatants of the outer layer of the scaffold containing the DMP-EGFP complex in short-term release (scale bar: 50 μm) and detection of efficiency by flow cytometry. ( C and D ) Representative fluorescence images of SCC-VII cells transfected with supernatants of the outer layer of the scaffold containing the DMP-EGFP complex in long-term release (scale bar: 100 μm) and the calculated transfection efficiency. ( E ) Cumulative RNA-release rate in the outer layer scaffold. ( F ) Bim levels in SCC-VII cells after treatment with supernatants of the outer layer of the scaffold containing DMP-mBim complex (***P<0.001). ( G and H ) MTT assay of SCC-VII cells after treatment with the supernatants of the outer layer of the scaffold containing DMP-mBim complex (scale bar: 100 μm, ****P<0.0001, **P<0.01). ( I ) Live/dead staining evaluation of SCC-VII cells treated with the supernatants of the outer layer of the scaffold (scale bar: 100 μm, ****P<0.0001).

    Journal: International Journal of Nanomedicine

    Article Title: Sequential Release of mRNA Complex and T Cells by a Double-Layered Implantable Scaffold for Combination Therapy of Head and Neck Squamous Cell Carcinoma

    doi: 10.2147/IJN.S582078

    Figure Lengend Snippet: Transfection efficiency and treatment effect of DMP-mBim complex after release from scaffold. ( A and B ) Representative fluorescence images of SCC-VII cells transfected with supernatants of the outer layer of the scaffold containing the DMP-EGFP complex in short-term release (scale bar: 50 μm) and detection of efficiency by flow cytometry. ( C and D ) Representative fluorescence images of SCC-VII cells transfected with supernatants of the outer layer of the scaffold containing the DMP-EGFP complex in long-term release (scale bar: 100 μm) and the calculated transfection efficiency. ( E ) Cumulative RNA-release rate in the outer layer scaffold. ( F ) Bim levels in SCC-VII cells after treatment with supernatants of the outer layer of the scaffold containing DMP-mBim complex (***P<0.001). ( G and H ) MTT assay of SCC-VII cells after treatment with the supernatants of the outer layer of the scaffold containing DMP-mBim complex (scale bar: 100 μm, ****P<0.0001, **P<0.01). ( I ) Live/dead staining evaluation of SCC-VII cells treated with the supernatants of the outer layer of the scaffold (scale bar: 100 μm, ****P<0.0001).

    Article Snippet: Cells were dual-stained for the plasma membrane and tubulin using DiI (Cell Plasma Membrane Staining Kit; Beyotime, China) and Tubulin-Tracker Green (Live Cell Staining Kit; Beyotime, China).

    Techniques: Transfection, Fluorescence, Flow Cytometry, MTT Assay, Staining