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Activation of Cyp1a1 and Cyp1a2 Genes in Adult Mouse Hepatocytes in Primary Culture

机译:在原代培养的成年小鼠肝细胞中Cyp1a1和Cyp1a2基因的激活

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摘要

Expression of Cyp1a1 and Cyp1a2 genes was investigated in adult C57BL/6NCrj mouse hepatocytes in primary culture for up to 5 days. When the cells were cultivated as monolayers on collagen‐coated dishes, CYP1A1 mRNA species were prominently induced after treatment with 3‐methylcholanthrene (MCA) throughout the observation period. Substantial induction of CYP1A2 mRNA by MCA was also observed at day 1 of cultivation, followed by a decrease to very low levels thereafter. In contrast, when cultivated on non‐coated dishes, the hepatocytes formed multicellular aggregates (spheroids) and prominent induction of both mRNA species was found for up to 5 days. Constitutive expression of CYP1A2 mRNA in spheroid culture was maintained throughout the observation period, whereas that in monolayer culture decreased rapidly. The time‐course of the induced CYP1A2 mRNA amounts after the treatment with MCA or 2,3,7,8‐tetrachlorodibenzo‐p‐dioxin (TCDD) followed the same pattern as that of CYP1A1 mRNA. Expressed amounts of CYP1A1 or CYP1A2 mRNA in spheroid culture were higher than or similar to the levels in the case of in vivo production, respectively. Induction of both mRNA species was also observed in hepatocytes from nonresponsive DBA/2NCrj mouse in spheroid culture, but the expressed amount after MCA treatment was far smaller than for C57BL/6NCrj cells, despite equivalent expression in the two strains after TCDD. Activities of aryl hydrocarbon hydroxylase (AHH) and acetanilide 4‐hydroxylase (AAH) were elevated with either type of cultivation after treatment with MCA or TCDD, Ratios of AAH to AHH were not changed between the two cultures after 24 h treatment. However, the ratios in spheroid culture after 48 h treatment increased, whereas they did not change in monolayer culture. The present observations indicate that the spheroid culture is more suitable than the monolayer system for studying the mechanism of Cyp1a2 gene expression in adult mouse hepatocytes.
机译:研究了在原代培养中长达5天的成年C57BL / 6NCrj小鼠肝细胞中Cyp1a1和Cyp1a2基因的表达。当细胞在胶原蛋白包被的培养皿上单层培养时,在整个观察期中,用3-甲基胆红素(MCA)处理后,CYP1A1 mRNA物种被显着诱导。在培养的第1天,MCA也大量诱导了CYP1A2 mRNA的诱导,随后又降至非常低的水平。相反,当在无涂层培养皿上培养时,肝细胞会形成多细胞聚集体(球状体),并且在长达5天的时间内都发现了这两种mRNA的显着诱导。 CYP1A2 mRNA的组成型表达在整个观察期间保持不变,而在单层培养中则迅速下降。用MCA或2,3,7,8-四氯二苯并-二恶英(TCDD)处理后,诱导的CYP1A2 mRNA的时间变化遵循与CYP1A1 mRNA相同的模式。 CYP1A1或CYP1A2 mRNA在球状培养物中的表达量分别高于或相似于体内生产的水平。在球状培养的无反应性DBA / 2NCrj小鼠的肝细胞中也观察到了这两种mRNA的诱导,但是尽管在TCDD之后在这两种菌株中表达均相同,但MCA处理后的表达量远小于C57BL / 6NCrj细胞。用MCA或TCDD处理后,无论哪种培养方式,芳烃羟化酶(AHH)和对乙酰苯胺4-羟化酶(AAH)的活性均升高,处理24小时后两种培养物中AAH与AHH的比例没有变化。但是,处理48小时后球状培养物中的比例增加,而在单层培养中则没有变化。目前的观察结果表明,对于研究成年小鼠肝细胞中Cyp1a2基因表达的机制,球状培养比单层培养更合适。

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