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The experimental model of intestinal epithelial cell growth established by real time cell analysis / 中国药理学通报
Chinese Pharmacological Bulletin ; (12): 290-294, 2018.
Article in Chinese | WPRIM | ID: wpr-705033
ABSTRACT
Aim To observe the effect of epidermal growth factor (EGF) on cell growth under different culture conditions using the real-time cell analyzer and EGF as a tool medicine to promote cell growth,and to provide reference for establishing pharmacokinetic model of IEC-6 cell growth (proliferation).Methods IEC-6 cell was inoculated on E-Plate 16 plate at a density of 1 × 104 cell/well and cultured in DMEM with 10% serum for 24 h,then replaced by serum-free DMEM culture (serum starvation)for 20 h,then the effects of different culture conditions on cell growth as well as EGF efficacy were observed.Results ① When the serum concentration was 10%,the cell growth index of EGF group(1,10,100 μg · L-1) after drug administration 24 h,48 h and 72 h was P > 0.05 compared with the blank group,suggesting that 10% serum culture could not reflect the efficacy of EGF.② When the serum concentration was 0%,EGF (1,10 μg · L-1) improved cell growth inhibition caused by serum-free cultivation,but could not recover it to normal level (the EGF group after drug administration 24 h,48 h and 72 h was P <0.01 compared with 5% serum),which suggested that serum-free culture could not reflect the EGF efficacy.③ 0%,0.5%,1% serum had different effects on cell growth,of which 0.5% serum could neither have obvious inhibition on cell growth,nor reflect the EGF effect due to promoting cell growth for a long time.④When the serum concentration was 0.5 %,the cell growth index of EGF groups after drug administration 24h,48h and 72h was P <0.01 compared with the blank group,suggesting that 0.5% serum culture could better reflect EGF efficacy.⑤The efficacy of EGF (10 μg· L-1) in promoting cell growth was confirmed by repeated validation of 0.5 % serum.Condusions A reference scheme of the IEC-6 cell growth (proliferative) pharmacological experimental model is established in the real-time cell analyzercells are cultured in DMEM with 10% serum for 24h,then in serum-free DMEM (serum starvation) for 20h,then after the adding of reagent,cells are cultured in DMEM with 0.5% serum for 48-72 h to observe its effect on cell growth (proliferation).

Full text: Available Index: WPRIM (Western Pacific) Type of study: Prognostic study Language: Chinese Journal: Chinese Pharmacological Bulletin Year: 2018 Type: Article

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Full text: Available Index: WPRIM (Western Pacific) Type of study: Prognostic study Language: Chinese Journal: Chinese Pharmacological Bulletin Year: 2018 Type: Article