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用于 ADME 和毒理学应用的大鼠十二指肠类器官的开发和特性鉴定。

Development and characterization of rat duodenal organoids for ADME and toxicology applications.

机构信息

Bristol-Myers Squibb R&D, Pharmaceutical Candidate Optimization, Rt. 206 and Province Line Road, Princeton, NJ, 08648, United States.

Bristol-Myers Squibb R&D, Pharmaceutical Candidate Optimization, Rt. 206 and Province Line Road, Princeton, NJ, 08648, United States.

出版信息

Toxicology. 2020 Dec 15;446:152614. doi: 10.1016/j.tox.2020.152614. Epub 2020 Oct 24.

DOI:10.1016/j.tox.2020.152614
PMID:33199268
Abstract

Many in vitro gastrointestinal models have been developed with the hope that they will continue to improve in their similarity to the organs from which they were isolated. Intestinal organoids isolated from various species are now being used to investigate physiology and pathophysiology. In this study, intestinal stem cells were isolated from adult rat duodenum and culture conditions were optimized to promote the growth, differentiation and development of 3D organoids. We optimized and characterized rat duodenal organoids with light and electron microscopy, immunofluorescence and notably, global mRNA expression. The metabolic capacity of these cultures was investigated using probe substrates for multiple phase I and phase II drug metabolizing enzymes and found to be in line with previous results from intestinal primary cultures and a significant improvement over immortalized cell lines. Over the course of differentiation, the gene expression profiles of the rat duodenal organoids were consistent with expected trends in differentiation to various cell lineages reflecting the duodenum in vivo. Further, incubations of these cultures with naproxen and celecoxib resulted in cytotoxicity consistent with the direct cytotoxic effects of these drugs to duodenum in vivo. Based on these characteristics, the rat duodenal organoids described herein will provide a novel platform for investigating a wide variety of mechanistic questions.

摘要

许多体外胃肠道模型已经开发出来,希望它们在与分离器官的相似性方面能够不断改进。现在,各种物种分离的肠类器官正在被用于研究生理学和病理生理学。在这项研究中,从成年大鼠十二指肠中分离出肠干细胞,并优化培养条件以促进 3D 类器官的生长、分化和发育。我们通过光镜和电镜、免疫荧光,特别是全局 mRNA 表达,对大鼠十二指肠类器官进行了优化和特征描述。使用多种 I 相和 II 相药物代谢酶的探针底物研究了这些培养物的代谢能力,结果与肠道原代培养物的先前结果一致,并且明显优于永生化细胞系。在分化过程中,大鼠十二指肠类器官的基因表达谱与向各种细胞谱系分化的预期趋势一致,反映了体内十二指肠的情况。此外,这些培养物与萘普生和塞来昔布孵育导致细胞毒性,与这些药物对体内十二指肠的直接细胞毒性作用一致。基于这些特征,本文所述的大鼠十二指肠类器官将为研究广泛的机制问题提供一个新的平台。

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