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Oxaliplatin

SKU: orb1310880

Description

Oxaliplatin

Research Area

Cell Biology, Molecular Biology

Images & Validation

Key Properties

CAS Number61825-94-3
MW397.29
Purity98.96%
FormulaC8H14N2O4Pt
SMILESO=C1O[Pt]OC1=O.N[C@@H]1CCCC[C@H]1N
TargetDNA/RNA Synthesis,DNA Alkylator/Crosslinker,Apoptosis,Autophagy
SolubilityDMSO:50 mg/mL (125.85 mM);Ethanol:< 1 mg/mL (insoluble);H2O:2.5 mg/mL (6.29 mM);DMF:1.67 mg/mL (4.2 mM)

Bioactivity

Target IC50
RT4 cells:11 μM|WiDr cells:0.13 μg/mL|A2780 cells:0.17 μM|U-87MG cells:17.6 μM|HT29 cells:0.97 μM|TCCSUP cells:15 μM|HT144 cells:7.85 μM|HT29 cells:0.33 μg/mL|LS174T cells:0.19 μg/mL|SW620 cells:1.13 μg/mL|SK-MEL-2 cells:30.9 μM|U-373MG cells:2.95 μM
In Vivo
METHODS: To detect anti-tumor activity in vivo, Oxaliplatin (5 mg/kg) and piperlongumine (2.5 mg/kg) were administered intraperitoneally once a day for twenty-four days to BALB/c nu/nu mice bearing human colorectal carcinoma tumor HCT-116. RESULTS: The combination of Oxaliplatin and piperlongumine significantly inhibited tumor growth, and piperlongumine sensitized tumors to Oxaliplatin through ROS-mediated apoptosis in vivo. METHODS: To model platinum-induced painful peripheral neuropathy, Oxaliplatin (3 mg/kg/day) was injected intraperitoneally into C57BL6J mice for five days with five days of rest for two cycles. RESULTS: Mice in the Oxaliplatin-treated group exhibited significant mechanical anomalous pain. the Oxaliplatin group exhibited significant cold nociceptive hypersensitivity in the hindfoot.
In Vitro
METHODS: Human colon cancer cells HT29, SW620, WiDr and LS174T were treated with Oxaliplatin (0.001 ng/ml-100 µg/mL) for 24 h, and cytotoxicity was detected using MTT method. RESULTS: Oxaliplatin was cytotoxic to HT29, SW620, WiDr and LS174T cells, with IC50s of 0.33, 1.13, 0.13 and 0.19 μg/mL, respectively. METHODS: Human colon cancer cells HCT116 WT and CHK2 KO were treated with Oxaliplatin (40 µM) for 24-96 h. Apoptosis was detected by Flow Cytometry. RESULTS: Oxaliplatin treatment for 24-96 h increased apoptosis levels in WT and CHK2-KO cell lines. From 24-72 h, the apoptosis level of WT cells was consistently twofold lower than that of CHK2 KO cells. However, treatment for 96 h resulted in the same level of apoptosis in WT and CHK2-KO cells (85%). METHODS: Human oral squamous cell carcinoma cells CAL27 and SCC25 were treated with Oxaliplatin (31.25-125 μM) and Oxaliplatin (25-100 μM) for 12-36 h. Cell migration was detected using the Wound-healing method. RESULTS: Oxaliplatin inhibited the migration of CAL27 and SCC25 cells in a dose-dependent manner.
Cell Research
The cytotoxicity studies are carried out with the sulforhodamine-B microculture colorimetrie assay. Typically, cells are plated into 96-well plates on day 0 and exposed to Oxaliplatin on day 1; the sulforhodamine-B assay is carried out 48 h after Oxaliplatin exposure. The plates are incubated at 37 °C in 5% CO2 and 100% relative humidity at all times except when adding Oxaliplatin and during the final assay period. The initial number of cells plated for the assay ranged from 2-20 × 103 cells/50 /nL/well. The numbers of cells for plating and the drug exposure time are based on pilot studies using the criteria that (a) the cells in control wells are still in the log phase of growth on the day of the assay; (b) the maximum absorbance for the untreated controls on the day of the assay is in the range of 1.0 to 1.5; and (c) cells go through >2 doublings during the drug exposure. Eight wells are used per concentration. The plates are read at 570 and/or 540 nm using a Biotek Instruments model EL309 microplate reader interfaced with an IBM PC-compatible computer. The data are transferred and transformed into a LOTUS 1-2-3 format by the computer program DATALOG, and survival fractions are calculated by comparing the drug treated with control(Only for Reference)

Storage & Handling

Storagekeep away from direct sunlight | Powder: -20°C for 3 years | In solvent: -80°C for 1 year | Shipping with blue ice/Shipping at ambient temperature.
Expiration Date12 months from date of receipt.
DisclaimerFor research use only

Alternative Names

Inhibitor, Oxaliplatin, inhibit, L-OHP, DNA Alkylator, DNA Alkylator/Crosslinker, DNA cross-links, DNASynthesis, DNAAlkylator, DNA Synthesis, DNA/RNA Synthesis, DNA synthesis, Crosslinker, Autophagy, anticancer, apoptosis, RNA Synthesis, RNASynthesis

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Key Properties

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Oxaliplatin (orb1310880)

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