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Nedaplatin

    
99.95%

Nedaplatin

源葉(MedMol)
S81166 一鍵復制產品信息
95734-82-0
C2H8N2O3Pt
303.17
順糖氨鉑;奈達鉑
貨號 規格 價格 上海 北京 武漢 南京 購買數量
S81166-10mg
99.95% ¥69.00 6 - - -
S81166-50mg
99.95% ¥245.00 6 - - -
S81166-100mg
99.95% ¥425.00 2 - - -
S81166-250mg
99.95% ¥595.00 3 - - -
S81166-1g
≥98% ¥1700.00 貨期:2-3天 - - -
產品介紹 參考文獻(1篇) 質檢證書(COA) 摩爾濃度計算器 相關產品

產品介紹

The inhibition of cell (including human SCLC cell line SBC-3 and human NSCLC cell line PC-14) proliferation after drug treatments as the antitumor activity using a regrowth assay is messured. Briefly, cells are exposed to drugs alone or in combination for 6 days at 37°C in an atmosphere of 100% humidity with 5% CO2; the cells are then pipetted six to eight times until almost all cells appeared as single cells and counted with a counter. For each drug, concentration-effect curves are drawn as plots of the fraction of surviving cells (unaffected cell fraction, fu) versus drug concentration. The cell proliferation ratio of the treated:control cultures (T:C%) is calculated as follows: [(the number of treated cells on day 6)/(the number of treated cells on day 0)]/[(the number of control cells on day 6)/(the number of control cells on day 0)] × 100%. The IC50 is defined as the drug concentration required for a 50% reduction in the number of cells. Four or five independent experiments are carried out for each. To check the effect of the drug treatment schedule on the effect of the combination, the cells are treated either by simultaneous exposure to the two drugs or by sequential exposure to Nedaplatin followed by irinotecan (Nedaplatin→irinotecan) and vice versa (irinotecan→Nedaplatin) for 3 hours. For the sequential exposure treatment, cells are exposed to the first drug for 3 hours, ished in fresh medium once, and then immediately exposed to the second drug for 3 hours. The treated cells are cultured in drug-free medium until evaluation.(Only for Reference)

產品描述: The inhibition of cell (including human SCLC cell line SBC-3 and human NSCLC cell line PC-14) proliferation after drug treatments as the antitumor activity using a regrowth assay is messured. Briefly, cells are exposed to drugs alone or in combination for 6 days at 37°C in an atmosphere of 100% humidity with 5% CO2; the cells are then pipetted six to eight times until almost all cells appeared as single cells and counted with a counter. For each drug, concentration-effect curves are drawn as plots of the fraction of surviving cells (unaffected cell fraction, fu) versus drug concentration. The cell proliferation ratio of the treated:control cultures (T:C%) is calculated as follows: [(the number of treated cells on day 6)/(the number of treated cells on day 0)]/[(the number of control cells on day 6)/(the number of control cells on day 0)] × 100%. The IC50 is defined as the drug concentration required for a 50% reduction in the number of cells. Four or five independent experiments are carried out for each. To check the effect of the drug treatment schedule on the effect of the combination, the cells are treated either by simultaneous exposure to the two drugs or by sequential exposure to Nedaplatin followed by irinotecan (Nedaplatin→irinotecan) and vice versa (irinotecan→Nedaplatin) for 3 hours. For the sequential exposure treatment, cells are exposed to the first drug for 3 hours, ished in fresh medium once, and then immediately exposed to the second drug for 3 hours. The treated cells are cultured in drug-free medium until evaluation.(Only for Reference)
靶點: DNA/RNA Synthesis;DNA/RNASynthesis
體內研究: Nedaplatin (Aqupla)是順鉑衍生物,能抑制腫瘤克隆集落形成(IC50:28.5 μg/mL)。0.005-0.5 μg/mL的Nedaplatin對SBC-3細胞增殖的抑制效果為2%-98%(IC50:0.053 μg/mL)
細胞實驗: The inhibition of cell (including human SCLC cell line SBC-3 and human NSCLC cell line PC-14) proliferation after drug treatments as the antitumor activity using a regrowth assay is messured. Briefly, cells are exposed to drugs alone or in combination for 6 days at 37°C in an atmosphere of 100% humidity with 5% CO2; the cells are then pipetted six to eight times until almost all cells appeared as single cells and counted with a counter. For each drug, concentration-effect curves are drawn as plots of the fraction of surviving cells (unaffected cell fraction, fu) versus drug concentration. The cell proliferation ratio of the treated:control cultures (T:C%) is calculated as follows: [(the number of treated cells on day 6)/(the number of treated cells on day 0)]/[(the number of control cells on day 6)/(the number of control cells on day 0)] × 100%. The IC50 is defined as the drug concentration required for a 50% reduction in the number of cells. Four or five independent experiments are carried out for each. To c
參考文獻: 1.Alberts DS, et al. Cancer Chemother Pharmacol, 1997, 39(6), 493-497. 2.Matsumoto M, et al. Jpn J Cancer Res, 2001, 92(1), 51-58. 3.Kanzawa F, et al. Clin Cancer Res, 2001, 7(1), 202-209. 4.Wheate NJ et al. Dalton Trans, 2010, 39(35), 8113-8127. 5.Uchida N, et al.Eur J Cancer, 1998, 34(11), 1796-1801.
溶解性: DMSO:Insoluble    H2O:10  mM
保存條件: -20℃
配置溶液濃度參考:
1mg 5mg 10mg
1 mM 3.298 ml 16.492 ml 32.985 ml
5 mM 0.66 ml 3.298 ml 6.597 ml
10 mM 0.33 ml 1.649 ml 3.298 ml
50 mM 0.066 ml 0.33 ml 0.66 ml
注意: 部分產品我司僅能提供部分信息,我司不保證所提供信息的權威性,僅供客戶參考交流研究之用。

質檢證書(COA)

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請輸入貨號和一個與之匹配的批號。
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批號:JS298415 貨號:S20001-25g
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摩爾濃度計算器

質量 (mg) = 濃度 (mM) x 體積 (mL) x 分子摩爾量 (g/mol)

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