Hepatocyte heterogeneity in bile formation and hepatobiliary transport of drugs.

Enzyme Pub Date : 1992-01-01 DOI:10.1159/000468780
G M Groothuis, D K Meijer
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引用次数: 31

Abstract

In the past two decades many studies have been devoted to the involvement of the periportal (zone-1) and perivenous (zone-3) hepatocytes in bile formation and hepatobiliary transport of endogenous and exogenous compounds. It became clear that such a heterogeneity in transport function can, in principle, be due to the different localization of the cells in the acinus with respect to the incoming blood, to intrinsic differences between the cells or to both. In this review we first discuss the techniques used to study hepatocyte heterogeneity in hepatobiliary transport function. Combinations of such techniques can be used to discriminate between cellular heterogeneity due to acinar localization as opposed to intrinsic differences. These techniques include: normal and retrograde perfusions of isolated perfused livers; autoradiographic, fluorimetric and histochemical localization of injected substrates; separation of isolated hepatocytes into fractions enriched in periportal and perivenous cells; measurements of fluorescent surface signals with microlight guides; selective zonal toxicity, and pharmacokinetic modelling and analysis. Subsequently, for each of the rate-limiting steps in the hepatobiliary transport of organic compounds, the basic mechanisms are summarized and the available knowledge on the involvement of the cells from the various zones in these transport steps is discussed. The available literature data indicate that heterogeneity in transport function is often due to the localization of the cells in the acinus: the periportal cells are the first to come into contact with the portal blood and are thus exposed to the highest substrate concentration. Consequently they obtain the most prominent task in further disposition of the particular compound. It follows that the extent of involvement of the perivenous cells in drug disposition is implicitly determined by the activity of the periportal cells. Because of the potential saturation of elimination processes in the periportal cells, the involvement of perivenous cells may vary with the input concentration. In addition, real intrinsic differences have been established in the hepatobiliary transport of some substrates. These are probably based on differences in the cellular content of carrier- and receptor-binding and/or metabolizing proteins. In some cases these intrinsic differences may be secondary to existing sinusoidal gradients of endogenous compounds, such as O2, amino acids, bile acids or monosaccharides. Yet, data on the heterogeneity of hepatocytes in the various transport steps are far from complete or are even totally lacking, especially for human liver. A multi-experimental approach and advanced technology will be needed in the future to gain more insight into the acinar organization of bile formation and hepatobiliary transport of drugs in the human.

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胆汁形成和药物肝胆转运中的肝细胞异质性。
在过去的二十年中,许多研究致力于门周(1区)和静脉周(3区)肝细胞参与胆汁形成和内源性和外源性化合物的肝胆运输。很明显,这种运输功能的异质性原则上可能是由于腺泡中细胞相对于传入血液的不同定位,细胞之间的内在差异或两者兼而有之。在这篇综述中,我们首先讨论了用于研究肝胆运输功能中肝细胞异质性的技术。这些技术的组合可用于区分由于腺泡定位引起的细胞异质性,而不是内在差异。这些技术包括:正常和逆行灌注离体肝脏;注射底物的放射自显影、荧光和组织化学定位;分离肝细胞成门静脉周围和门静脉周围细胞富集的部分;用微光导测量荧光表面信号选择性区域毒性,以及药代动力学建模和分析。随后,对于有机化合物肝胆运输中的每个限速步骤,总结了基本机制,并讨论了来自不同区域的细胞参与这些运输步骤的现有知识。现有的文献资料表明,运输功能的异质性通常是由于细胞在腺泡中的定位:门静脉周围细胞首先与门静脉血液接触,因此暴露于最高的底物浓度。因此,它们在进一步处理特定化合物方面获得了最突出的任务。因此,静脉周围细胞参与药物处置的程度隐含地由门静脉周围细胞的活性决定。由于门静脉周围细胞消除过程的潜在饱和,静脉周围细胞的参与可能随输入浓度而变化。此外,在一些底物的肝胆运输中已经建立了真正的内在差异。这可能是基于载体和受体结合和/或代谢蛋白的细胞含量的差异。在某些情况下,这些内在差异可能继发于内源性化合物(如氧、氨基酸、胆汁酸或单糖)现有的正弦梯度。然而,关于肝细胞在各个转运步骤中的异质性的数据远不完整,甚至完全缺乏,特别是对于人类肝脏。未来需要多实验的方法和先进的技术来更深入地了解人类胆汁形成和药物肝胆转运的腺泡组织。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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Functional hepatocellular heterogeneity for the production of plasma proteins. Liver cell heterogeneity: functions of non-parenchymal cells. Hepatocyte heterogeneity in the metabolism of carbohydrates. Zonal liver cell heterogeneity. Hepatocyte heterogeneity in the metabolism of amino acids and ammonia.
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