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使用肠类器官模型研究顶端特异性相互作用的培养方法。

Culture Methods to Study Apical-Specific Interactions using Intestinal Organoid Models.

机构信息

STEMCELL Technologies Ltd.

STEMCELL Technologies Inc.

出版信息

J Vis Exp. 2021 Mar 23(169). doi: 10.3791/62330.

Abstract

The lining of the gut epithelium is made up of a simple layer of specialized epithelial cells that expose their apical side to the lumen and respond to external cues. Recent optimization of in vitro culture conditions allows for the re-creation of the intestinal stem cell niche and the development of advanced 3-dimensional (3D) culture systems that recapitulate the cell composition and the organization of the epithelium. Intestinal organoids embedded in an extracellular matrix (ECM) can be maintained for long-term and self-organize to generate a well-defined, polarized epithelium that encompasses an internal lumen and an external exposed basal side. This restrictive nature of the intestinal organoids presents challenges in accessing the apical surface of the epithelium in vitro and limits the investigation of biological mechanisms such as nutrient uptake and host-microbiota/host-pathogen interactions. Here, we describe two methods that facilitate access to the apical side of the organoid epithelium and support the differentiation of specific intestinal cell types. First, we show how ECM removal induces an inversion of the epithelial cell polarity and allows for the generation of apical-out 3D organoids. Second, we describe how to generate 2-dimensional (2D) monolayers from single cell suspensions derived from intestinal organoids, comprised of mature and differentiated cell types. These techniques provide novel tools to study apical-specific interactions of the epithelium with external cues in vitro and promote the use of organoids as a platform to facilitate precision medicine.

摘要

肠上皮的衬里由一层简单的特化上皮细胞组成,这些细胞将其顶端暴露于腔中,并对外界信号做出反应。最近,体外培养条件的优化使得能够重新创建肠干细胞龛,并开发先进的三维(3D)培养系统,以再现细胞组成和上皮组织。嵌入细胞外基质(ECM)中的肠类器官可以长期维持,并自我组织以生成具有明确极性的上皮组织,包括内部腔和外部暴露的基底侧。肠类器官的这种限制性质在体外访问上皮的顶端表面方面带来了挑战,并限制了对营养物质摄取和宿主-微生物群/宿主-病原体相互作用等生物学机制的研究。在这里,我们描述了两种方法,可促进对类器官上皮顶端表面的访问,并支持特定肠细胞类型的分化。首先,我们展示了 ECM 去除如何诱导上皮细胞极性的反转,并允许生成顶端向外的 3D 类器官。其次,我们描述了如何从肠类器官的单细胞悬浮液中生成由成熟和分化细胞类型组成的 2 维(2D)单层。这些技术提供了研究体外上皮与外部信号的顶端特异性相互作用的新工具,并促进了将类器官用作促进精准医学的平台。

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