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Cell-Type-Specific Quantification of a Scaffold-Based 3D Liver Co-Culture

机译:基于支架的3D肝共培养的细胞类型特异性定量

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摘要

In order to increase the metabolic activity of human hepatocytes and liver cancer cell lines, many approaches have been reported in recent years. The metabolic activity could be increased mainly by cultivating the cells in 3D systems or co-cultures (with other cell lines). However, if the system becomes more complex, it gets more difficult to quantify the number of cells (e.g., on a 3D matrix). Until now, it has been impossible to quantify different cell types individually in 3D co-culture systems. Therefore, we developed a PCR-based method that allows the quantification of HepG2 cells and 3T3-J2 cells separately in a 3D scaffold culture. Moreover, our results show that this method allows better comparability between 2D and 3D cultures in comparison to the often-used approaches based on metabolic activity measurements, such as the conversion of resazurin.
机译:为了增加人肝细胞和肝癌细胞系的代谢活性,近年来据报道了许多方法。 可以主要通过培养3D系统或共培养物(与其他细胞系)中的细胞来增加代谢活性。 然而,如果系统变得更复杂,则会变得更加困难,以量化单元的数量(例如,在3D矩阵上)。 到目前为止,在3D共同培养系统中,不可能量化不同的细胞类型。 因此,我们开发了一种基于PCR的方法,其允许在3D支架培养物中分别定量HepG2细胞和3T3-J2细胞。 此外,我们的结果表明,与基于代谢活性测量的经常使用的方法相比,该方法在2D和3D培养物之间允许更好的可比性,例如使用的方法,例如转塔脲的转化。

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