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优化培养条件以促进小鼠和人类结肠类器官的生长及功能分化

Optimized Culture Conditions for Improved Growth and Functional Differentiation of Mouse and Human Colon Organoids.

作者信息

Wilson Sarah S, Mayo Martha, Melim Terry, Knight Heather, Patnaude Lori, Wu Xiaoming, Phillips Lucy, Westmoreland Susan, Dunstan Robert, Fiebiger Edda, Terrillon Sonia

机构信息

Foundational Immunology, AbbVie, Cambridge Research Center, Cambridge, MA, United States.

Immunology Pharmacology, AbbVie, AbbVie Bioresearch Center, Worcester, MA, United States.

出版信息

Front Immunol. 2021 Feb 12;11:547102. doi: 10.3389/fimmu.2020.547102. eCollection 2020.

Abstract

BACKGROUND & AIMS: Diligent side-by-side comparisons of how different methodologies affect growth efficiency and quality of intestinal colonoids have not been performed leaving a gap in our current knowledge. Here, we summarize our efforts to optimize culture conditions for improved growth and functional differentiation of mouse and human colon organoids.

METHODS

Mouse and human colon organoids were grown in four different media. Media-dependent long-term growth was measured by quantifying surviving organoids imaging and a cell viability readout over five passages. The impact of diverse media on differentiation was assessed by quantifying the number of epithelial cell types using markers for enterocytes, stem cells, Goblet cells, and enteroendocrine cells by qPCR and histology upon removal of growth factors.

RESULTS

In contrast to Wnt3a-conditioned media, media supplemented with recombinant Wnt3a alone did not support long-term survival of human or mouse colon organoids. Mechanistically, this observation can be attributed to the fact that recombinant Wnt3a did not support stem cell survival or proliferation as demonstrated by decreased LGR5 and Ki67 expression. When monitoring expression of markers for epithelial cell types, the highest level of organoid differentiation was observed after combined removal of Wnt3a, Noggin, and R-spondin from Wnta3a-conditioned media cultures.

CONCLUSION

Our study defined Wnt3a-containing conditioned media as optimal for growth and survival of human and mouse organoids. Furthermore, we established that the combined removal of Wnt3a, Noggin, and R-spondin results in optimal differentiation. This study provides a step forward in optimizing conditions for intestinal organoid growth to improve standardization and reproducibility of this model platform.

摘要

背景与目的

尚未对不同方法如何影响肠道类器官的生长效率和质量进行细致的并列比较,这使得我们目前的知识存在空白。在此,我们总结了为优化培养条件以促进小鼠和人类结肠类器官的生长及功能分化所做的努力。

方法

小鼠和人类结肠类器官在四种不同培养基中培养。通过在五个传代过程中对存活类器官进行定量成像和细胞活力读数来测量培养基依赖性长期生长。在去除生长因子后,通过qPCR和组织学,使用肠细胞、干细胞、杯状细胞和肠内分泌细胞的标志物来量化上皮细胞类型的数量,从而评估不同培养基对分化的影响。

结果

与Wnt3a条件培养基相比,单独添加重组Wnt3a的培养基不支持人类或小鼠结肠类器官的长期存活。从机制上讲,这一观察结果可归因于重组Wnt3a不支持干细胞存活或增殖,这通过LGR5和Ki67表达降低得以证明。在监测上皮细胞类型标志物的表达时,从Wnta3a条件培养基培养物中联合去除Wnt3a、Noggin和R-spondin后,观察到类器官分化水平最高。

结论

我们的研究确定含Wnt3a的条件培养基是人类和小鼠类器官生长和存活的最佳培养基。此外,我们确定联合去除Wnt3a、Noggin和R-spondin可实现最佳分化。这项研究在优化肠道类器官生长条件以提高该模型平台的标准化和可重复性方面向前迈进了一步。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/77c8/7906999/723d7f0d643c/fimmu-11-547102-g001.jpg

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