Measuring oxygen levels in Caco-2 cultures

Nathalie E. Zeitouni, J. Fandrey, H. Naim, M. von Köckritz-Blickwede
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引用次数: 23

Abstract

Purpose Measuring oxygen levels in three different systems of Caco-2 cell culture. Methods Caco-2 cells were cultured in three different systems, using conventional polystyrene 24-well plates, special 24-well gas permeable plates, or on membrane inserts in conventional plates. Optical sensor spots were used to measure dissolved O2 levels in these cultured cells over the course of 6 days under normoxia (143 mmHg) and for 6 hours under hypoxia (7 mmHg). Western blot analysis was used to determine the protein levels of hypoxia-inducible factor 1α (HIF-1α) in the different cultures. Results All culture systems displayed lower O2 levels over time than expected when cultured under normoxia conditions. On average, O2 levels reached as low as 25 mmHg in 24-well plates but remained at 97 and 117 mmHg in gas permeable plates and membrane inserts, respectively. Under hypoxia, 1 mL cell cultures equilibrated to 7 mmHg O2 within the first 60 minutes and dropped to 0.39 and 0.61 mmHg O2 in 24-well and gas permeable plates, respectively, after the 6-hour incubation period. Cultures in membrane inserts did not equilibrate to 7 mmHg by the end of the 6-hour incubation period, where the lowest O2 measurements reached 23.12 mmHg. Western blots of HIF-1α protein level in the whole cell lysates of the different Caco-2 cultures revealed distinct stabilization of HIF-1α after hypoxic incubation for 1, 2, and 4 hours in 24-well plates as well as gas permeable plates. For membrane inserts, notable HIF-1α was seen after 4 hours of hypoxic incubation. Conclusion Cellular oxygen depletion was achieved in different hypoxic Caco-2 culture systems. However, different oxygen levels comparing different culture systems indicate that O2 level should be carefully considered in oxygen-dependent experiments.
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测量Caco-2培养物中的氧含量
目的测定三种不同Caco-2细胞培养体系中的氧含量。方法Caco-2细胞在常规聚苯乙烯24孔板、特殊24孔透气板和常规板中插入膜三种不同体系中培养。在正常缺氧(143毫米汞柱)和缺氧(7毫米汞柱)下6小时,使用光学传感器点测量这些培养细胞中的溶解氧水平。Western blot检测不同培养物中缺氧诱导因子1α (HIF-1α)蛋白水平。结果在常氧条件下,所有培养系统的氧含量随时间的推移均低于预期。平均而言,24孔板的O2水平低至25 mmHg,而透气板和插入膜的O2水平分别保持在97和117 mmHg。在缺氧条件下,1 mL细胞培养物在前60分钟内平衡到7 mmHg O2,在24孔板和透气板中,6小时孵育后分别降至0.39和0.61 mmHg O2。在6小时的孵育期结束时,膜插入物中的培养物没有平衡到7 mmHg,其中最低的O2测量值达到23.12 mmHg。Western blot检测不同Caco-2培养物全细胞裂解物中HIF-1α蛋白水平显示,在24孔板和透气板中缺氧孵育1、2和4小时后,HIF-1α明显稳定。对于膜插入,缺氧培养4小时后观察到显著的HIF-1α。结论不同低氧Caco-2培养体系均可实现细胞耗氧。然而,不同培养体系的不同氧水平表明,在氧依赖实验中应仔细考虑氧水平。
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