Celltox green cytotoxicity assay kit

Manufactured by Promega

Sourced in United States

The CellTox Green Cytotoxicity Assay kit is a cell-based assay used to measure cytotoxicity. The kit utilizes a proprietary dye that selectively stains the DNA of dead cells, providing a quantitative measure of cytotoxicity in cell populations.

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Lab products found in correlation

Cholesterol, by Thermo Fisher Scientific (2 mentions) Trypsin, by Thermo Fisher Scientific (2 mentions) Hepes buffer, by MP Biomedicals (2 mentions) Diacetyl phosphate, by Thermo Fisher Scientific (2 mentions) Animal endothelial cell medium, by Cell Biologics (2 mentions) Murine endothelial growth factor, by Cell Biologics (2 mentions) Fetal bovine serum (fbs), by Cell Biologics (2 mentions) L glutamine, by Cell Biologics (2 mentions) Antibiotic antimycotic, by Cell Biologics (2 mentions) Hank s buffered salt solution hbss, by Thermo Fisher Scientific (2 mentions) D luciferin fluorescence dye, by BD (2 mentions) Polystyrene nonpyrogenic 96 well plates, by BD (2 mentions) 24 well trans inserts, by Corning (2 mentions) Peg 600, by Croda (2 mentions) Modulus 2 microplate multimode reader, by Promega (1 mentions) Heracell 240i, by Thermo Fisher Scientific (1 mentions) Fetal calf serum (fcs), by Harvard Bioscience (1 mentions) Ethanol, by Merck Group (1 mentions) Penicillin, by GE Healthcare (1 mentions) Streptomycin, by GE Healthcare (1 mentions)

18 protocols using celltox green cytotoxicity assay kit

Cytotoxicity Assay for AM404 Treatment

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Cytotoxicity assay was performed using CellTox™ Green Cytotoxicity assay kit (Promega, Mannheim, Germany). Briefly, cells were cultured in 96-well plates at the density of 25 × 10³ cells/well in DMEM medium containing 10% fetal calf serum (Biochrom AG, Berlin, Germany) and antibiotics (40 U/mL penicillin and 40 μg/mL streptomycin, both from PAA Laboratories, Linz, Austria). Cells were pre-treated with different concentrations of AM404 (0.1–10 μM) or DMSO 0.1% for 30 min. Thereafter, cells were incubated with or without LPS for the next 24 h. Ethanol (10% end conc., Sigma-Aldrich, Taufkirchen, Germany) was used as positive control to induce the cell death. After incubation (10% CO₂ at 37 °C - Heracell 240i, Thermo Scientific), 100 μl of CellTox™ Green reagent were added in each well. The plate was mixed for 1 min and incubated for 15 min at room temperature, and the fluorescence was measured at 490 nm_Ex/530 nm_Em using a Modulus™ II Microplate Multimode Reader (Turner BioSystems, USA).
The principle of the assay is to evaluate the alterations in the membrane integrity, using the cyanine dye. The dye binds in the dead-cell DNA and enhanced the fluorescent property, which is excluded from viable cells. The fluorescence intensity values obtained were normalized and presented as the percentage of untreated controls.

Saliba S.W., Marcotegui A.R., Fortwängler E., Ditrich J., Perazzo J.C., Muñoz E., de Oliveira A.C, & Fiebich B.L. (2017). AM404, paracetamol metabolite, prevents prostaglandin synthesis in activated microglia by inhibiting COX activity. Journal of Neuroinflammation, 14, 246.

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Cytotoxicity Evaluation of Bar

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A CellTox™ Green Cytotoxicity Assay kit (Promega, Madison, WI, USA) was used to assess the toxicity of Bar by measuring the changes in membrane integrity that occur as a result of cell death using an asymmetric cyanine dye. A concentration of 1 μM Bar was selected for all experiments.

Liu C., Arnold R., Henriques G, & Djabali K. (2019). Inhibition of JAK-STAT Signaling with Baricitinib Reduces Inflammation and Improves Cellular Homeostasis in Progeria Cells. Cells, 8(10), 1276.

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In Vitro BBB Endothelial Cell Assay

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Hydrogenated phosphatidylcholine (95%-hydrogenated phosphatidylcholine and 0.5%hydrogenated lyso phosphatidylcholine) was gifted from American Lecithin Company (Oxford, CT). Cit-HBr was kindly donated by Lund beck A/S (Copenhagen, Denmark). Diacetyl phosphate, NAG, and cholesterol were purchased from Fisher Scientific (Pittsburgh, PA). PEG 600 was purchased from Croda Inc. (Columbus Circle Edison, NJ). All other solvents were purchased as HPLC grade. Rat Primary Brain Microvascular Endothelial Cells (RPBMECs), Animal Endothelial cell medium supplemented with murine Endothelial Growth Factor (mEGF), fetal bovine serum (FBS), L-glutamine, Antibiotic-Antimycotic and gelatin-based coating solutions were purchased from Cell Biologics (Chicago, IL). Hank’s Buffered Salt Solution (HBSS) was purchased from Thermo Scientific (South Logan, UT). CellTox Green Cytotoxicity Assay kit was gifted by Promega Corporation (Madison, WI). D-Luciferin fluorescence dye was purchased from BD Bioscience (Bedford, MA). Trypsin was purchased from Gibco (Grand Island, NY). HEPES buffer was purchased from MP Biomedical (Solon, OH). Polystyrene nonpyrogenic 96-well plates were obtained from BD Bioscience (Bedford,MA). 24-well trans inserts obtained from Corning Life Sciences (Lowell, MA.).

Kamal N.S., Habib M.J., Zidan A.S, & Karla P.K. (2020). NAG-PEGylated multilamellar liposomes for BBB-GLUT transporter targeting. Cogent medicine, 6(1), 1701343.

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Cell Cytotoxicity Detection Protocol

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Cell mortality was detected by a CellTox Green Cytotoxicity Assay Kit (Promega, Wisconsin, United States). The detection system uses a proprietary asymmetric cyanine dye, which is blocked by living cells but can stain the DNA of dead cells. When the dye binds with DNA, it emits fluorescence. Therefore, the fluorescence signal produced by the dye bound to the dead cell DNA is directly proportional to the cytotoxicity. We operated strictly according to the protocol, adding 50 μL cells with a concentration of 1 × 10⁵/mL to the 96-well cell culture plate. Then, we added 100 μL CellTox^TM Green reagent (Madison, WI, USA), and after incubation for 15 min, it was put into a fluorescence enzyme labeling instrument. After 1 min of simple oscillation, the fluorescence signal value was detected at 485–500 nm Ex/520~530 nm Em wavelength.

Chu J., Guo Y., Xu G., Zhang Q., Zuo Z., Li Q., Wang Y, & He C. (2020). Chlamydia psittaci Triggers the Invasion of H9N2 Avian Influenza Virus by Impairing the Functions of Chicken Macrophages. Animals : an Open Access Journal from MDPI, 10(4), 722.

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Multiplex Assay for Intestinal Organoids

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CellTox Green Cytotoxicity Assay kit (G8742) was from Promega (MyBio, Ireland). Tetramethylrhodamine methyl ester (TMRM) (T-668), cholera toxin (CTX) subunit B Alexa Fluor 488 conjugate (C34775) and secondary Alexa Fluor 488-conjugated anti-mouse antibodies (A10680) were from Invitrogen (GE Healthcare, Ireland). Mouse monoclonal anti-BrdU antibody (clone BU-1, 05–633) was from Millipore (Cork, Ireland). Intesticult Organoid Growth Medium (mouse) kit (06005) and ‘gentle cell dissociation reagent’ (07174) were from Stem Cell Technologies (UK). Matrigel® with reduced growth factors (356231) was from Corning. Phosphorescent O₂-sensitive probe Pt-Glc was synthesized as previously described [18 ]. Bis-benzimide Hoechst 33342 (B2261), 5-bromo-2’-deoxyuridine (B5002), aphidicolin from Nigrospora sphaerica (A4487), metformin hydrochloride (PHR1084), phosphate buffered saline (P4417), albumin from bovine serum (A4503), penicillin-streptomycin solution (P0781) and all the other reagents were from Sigma-Aldrich (Dublin, Ireland).

Okkelman I.A., Dmitriev R.I., Foley T, & Papkovsky D.B. (2016). Use of Fluorescence Lifetime Imaging Microscopy (FLIM) as a Timer of Cell Cycle S Phase. PLoS ONE, 11(12), e0167385.

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Synergistic Drug Screening for KL-2

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The library of clinically used drugs (Selleck, L1300) was used for screening synergistic drugs with KL-2. Kelly cells were seeded at a density of 3000 cells per well in 96-well plates and then treated with KL-2 (2 μM) alone or in combination with each compound (500 nM) for 24 hours. Cell death was measured by the CellTox Green Cytotoxicity Assay kit (Promega, #G8743). Fluorescence readings were collected with an automatic microplate reader (Molecular Devices). CI values were calculated using the CalcuSyn software (Biosoft) based on the Chou-Talalay method (32 (link)).

Wang D., Yin Z., Wang H., Wang L., Li T., Xiao R., Xie T., Han R., Dong R., Liu H., Liang K, & Qing G. (2023). The super elongation complex drives transcriptional addiction in MYCN-amplified neuroblastoma. Science Advances, 9(13), eadf0005.

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Cytotoxicity Assay for Calu-3 Cells

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As an additional assay to measure the cytotoxic response from human bronchial Calu-3 cells, the CellTox Green Cytotoxicity Assay Kit from Promega was performed using a modified version of the Endpoint Step Protocol. Calu-3 cells grown in a 96-well microplate (Costar) were washed three times with PBS and infected with Spn at a density of ~2.75 × 10⁷ CFU/mL. CellTox Green Reagent was added to wells, as recommended by the manufacturer, and placed in a fluorometer (BMG LabTech Flustra Omega) with incubation at 37°C. Relative fluorescence unit readings were collected every 20 min for 24 h. In some experiments, infected Calu-3 cells that had been treated with CellTox Green Reagent were imaged in the green fluorescence channel using a Nikon Eclipse TSR inverted microscope.

Scasny A., Alibayov B., Khan F., Rao S.J., Murin L., Jop Vidal A.G., Smith P., Li W., Edwards K., Warncke K, & Vidal J.E. (2023). Oxidation of hemoproteins by Streptococcus pneumoniae collapses the cell cytoskeleton and disrupts mitochondrial respiration leading to the cytotoxicity of human lung cells. Microbiology Spectrum, 12(1), e02912-23.

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Cytotoxicity Assay of Neural Cell Lines

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After 24 h of treatments, we used the CellTox™ Green Cytotoxicity Assay kit (G8742, Promega Corporation, Maddison, WI, USA) to assess the survival of NIH-3T3, PC12, HEK293T and P7 hippocampal NSCs under conditions of serum and EGF/FGF deprivation, respectively. NPCs were studied after 48 h. Cells were plated in 96-well plates, starved for 4 h and treated with NGF (100 ng/mL) and/or BDNF (500 ng/mL) and compound ENT-A044(500 nM) in the presence or absence of p75NTR inhibitor MC-192 (2.5 ng/mL, ab6172, Abcam, plc., Cambridge, UK) and TrkB inhibitor 100 μM of ANA-12 (SML0209, Sigma-Aldrich, Burlington, MA, US) for 24 h. CellTox assay reagents and Hoescht (1:10,000, H3570, Invitrogen, Waltham, MA, USA) were added to each well for 30 min, and cells were imaged using a fluorescent microscope (Zeiss AXIO Vert A1, Zeiss, Jena, Germany). Positive cells for cell tox reagent were normalized to reflect the total number of cells per image. We also refreshed the examined compound, as well as BDNF or/and NGF and HEK293T cells and P7 hippocampal NSCs, and they were imaged again after 48 h.

Papadopoulou M.A., Rogdakis T., Charou D., Peteinareli M., Ntarntani K., Gravanis A., Chanoumidou K, & Charalampopoulos I. (2023). Neurotrophin Analog ENT-A044 Activates the p75 Neurotrophin Receptor, Regulating Neuronal Survival in a Cell Context-Dependent Manner. International Journal of Molecular Sciences, 24(14), 11683.

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Intracellular ATP Measurement in Sperm

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To determine intracellular ATP, sperm cells from the spermathecae of C. osakensis queens were introduced to 40 µL of 39.44 mM sodium sulfite in PBS (anoxic condition) and PBS (aerobic condition) for 1 min. Thereafter, the sperm samples were centrifuged at 5000 rpm for 5 min, after which the supernatants were removed, and CellTiter-Glo® Luminescent Cell Viability Assay buffer (Promega) was added. The sperm suspension was then divided into two samples: one for measuring relative luminescence unit (RLU) to determine ATP levels using a CellTiter-Glo Luminescent Cell Viability Assay kit (Promega) and the other for measuring relative fluorescence unit (RFU) to assess DNA content using CellTox™ Green Cytotoxicity Assay kit (Promega). After the samples were prepared according to the manufacturer’s protocol, their luminescence and fluorescence were detected using the GloMax® system (Promega). We confirmed that the values were neither too low to detect nor saturated by checking whether they were within the linear range of the standard curve. To calibrate the ATP content by the number of sperm cells, we calculated values of RLU/RFU.

Gotoh A., Takeshima M, & Mizutani K.I. (2023). Near-anoxia induces immobilization and sustains viability of sperm stored in ant queens. Scientific Reports, 13, 3029.

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Reactive Oxygen Species and HIF-1α Assays

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The ROS content after different treatments was tested by using ROS-Glo™ H₂O₂ Assay kit (Promega, Milan, Italy). HIF-1α activity was measured on lysates through Luciferase Biochemical assay, using GloMax-Multi Detection System (Promega, Milan, Italy), and normalized for protein content [26 (link)]. The cytotoxicity of treatments was tested utilizing Cell Tox™ Green Cytotoxicity Assay kit (Promega, Milan, Italy) and Cell Titer-Glo^® Luminescent Cell Viability Assay (Promega). Detection and quantification of Glutathione (GSH) was performed after treatment by the commercially available GSH-Glo™ Glutathione Assay (Promega). Data were expressed as Glutathione concentration. All the assays performed by using commercially available kits were carried out according to the manufacturer’s instructions.

Lo Dico A., Salvatore D., Martelli C., Ronchi D., Diceglie C., Lucignani G, & Ottobrini L. (2019). Intracellular Redox-Balance Involvement in Temozolomide Resistance-Related Molecular Mechanisms in Glioblastoma. Cells, 8(11), 1315.

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