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人胎肝细胞类器官的建立及基于 CRISPR-Cas9 的基因敲入和敲除在人肝来源的类器官培养物中的应用。

Establishment of human fetal hepatocyte organoids and CRISPR-Cas9-based gene knockin and knockout in organoid cultures from human liver.

机构信息

Hubrecht Institute, Royal Netherlands Academy of Arts and Sciences, Utrecht, the Netherlands.

Oncode Institute, Utrecht, the Netherlands.

出版信息

Nat Protoc. 2021 Jan;16(1):182-217. doi: 10.1038/s41596-020-00411-2. Epub 2020 Nov 27.

Abstract

The liver is composed of two epithelial cell types: hepatocytes and liver ductal cells. Culture conditions for expansion of human liver ductal cells in vitro as organoids were previously described in a protocol; however, primary human hepatocytes remained hard to expand, until recently. In this protocol, we provide full details of how we overcame this limitation, establishing culture conditions that facilitate long-term expansion of human fetal hepatocytes as organoids. In addition, we describe how to generate (multi) gene knockouts using CRISPR-Cas9 in both human fetal hepatocyte and adult liver ductal organoid systems. Using a CRISPR-Cas9 and homology-independent organoid transgenesis (CRISPR-HOT) approach, efficient gene knockin can be achieved in these systems. These gene knockin and knockout approaches, and their multiplexing, should be useful for a variety of applications, such as disease modeling, investigating gene functions and studying processes, such as cellular differentiation and cell division. The protocol to establish human fetal hepatocyte organoid cultures takes ~1-2 months. The protocols to genome engineer human liver ductal organoids and human fetal hepatocyte organoids take 2-3 months.

摘要

肝脏由两种上皮细胞类型组成

肝细胞和胆管细胞。此前曾在一项方案中描述过体外扩增人胆管细胞类器官的培养条件;然而,直到最近,原代人肝细胞仍难以扩增。在本方案中,我们提供了克服这一限制的详细信息,建立了培养条件,可促进人胎肝细胞作为类器官的长期扩增。此外,我们还描述了如何在人胎肝细胞和成人胆管细胞类器官系统中使用 CRISPR-Cas9 生成(多)基因敲除。使用 CRISPR-Cas9 和非同源性类器官转基因(CRISPR-HOT)方法,可以在这些系统中实现高效的基因敲入。这些基因敲入和敲除方法及其多重化应该对各种应用有用,例如疾病建模、研究基因功能以及研究细胞分化和细胞分裂等过程。建立人胎肝细胞类器官培养物的方案需要 1-2 个月。基因组工程人胆管细胞类器官和人胎肝细胞类器官的方案需要 2-3 个月。

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