Efficient and cost-effective differentiation of induced neural crest cells from induced pluripotent stem cells using laminin 211

IF 3.4 3区环境科学与生态学 Q3 CELL & TISSUE ENGINEERING

Regenerative Therapy Pub Date : 2024-06-01 DOI:10.1016/j.reth.2024.08.024

Kazuma Takahashi, Shizuka Aritomi, Fumie Honkawa, Sayaka Asari, Ken Hirose, Atsushi Konishi

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引用次数: 0

Abstract

Introduction

Neural crest cells (NCCs) are cell populations that originate during the formation of neural crest in developmental stages. They are characterized by their multipotency, self-renewal and migration potential. Given their ability to differentiate into various types of cells such as neurons and Schwann cells, NCCs hold promise for cell therapy applications. The conventional method for obtaining NCCs involves inducing them from stem cells like induced pluripotent stem cells (iPSCs), followed by a long-term passage or purification using fluorescence-activated cell sorting (FACS). Although FACS allows high purity induced neural crest cells (iNCCs) to be obtained quickly, it is complex and costly. Therefore, there is a need for a simpler, cost-effective and less time-consuming method for cell therapy application.

Methods

To select differentiated iNCCs from heterogeneous cell populations quickly without using FACS, we adopted the use of scaffold material full-length laminin 211 (LN211), a recombinant, xeno-free protein suitable for cell therapy. After fist passage on LN211, iNCCs characterization was performed using polymerase chain reaction and flow cytometry. Additionally, proliferation and multipotency to various cells were evaluated.

Result

The iNCCs obtained using our new method expressed cranial NCC- related genes and exhibited stable proliferation ability for at least 57 days, while maintaining high expression level of the NCCs marker CD271. They demonstrated differentiation ability into several cell types: neurons, astrocytes, melanocytes, smooth muscle cells, osteoblasts, adipocytes and chondrocytes. Furthermore, they could be induced to differentiate into induced mesenchymal stem cells (iMSCs) which retain the essential functions of somatic MSCs.

Conclusion

In this study, we have developed novel method for obtaining high purity iNCCs differentiated from iPSCs in a short time using LN211 under xeno-free condition. Compared with traditional methods, like FACS or long-term passage, this approach enables the acquisition of a large amount of cells at a lower cost and labor, and it is expected to contribute to stable supply of large scale iNCCs for future cell therapy applications.

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利用层粘连蛋白 211 从诱导多能干细胞高效、经济地分化诱导神经嵴细胞

导言神经嵴细胞（NCC）是起源于神经嵴形成发育阶段的细胞群。它们具有多潜能、自我更新和迁移潜力等特点。鉴于它们能分化成神经元和许旺细胞等各种类型的细胞，NCC 在细胞治疗应用中大有可为。获得 NCCs 的传统方法包括从诱导多能干细胞（iPSCs）等干细胞中诱导 NCCs，然后使用荧光激活细胞分拣（FACS）进行长期传代或纯化。虽然荧光激活细胞分拣技术能快速获得高纯度的诱导神经嵴细胞（iNCCs），但其操作复杂且成本高昂。方法为了在不使用 FACS 的情况下从异质细胞群中快速筛选出分化的 iNCCs，我们采用了支架材料全长层粘连蛋白 211（LN211），这是一种适合细胞治疗的重组无异种蛋白。iNCCs 在 LN211 上经过拳头大小的通道后，使用聚合酶链式反应和流式细胞术进行了表征。结果使用我们的新方法获得的 iNCCs 表达了颅骨 NCC 相关基因，并在至少 57 天内表现出稳定的增殖能力，同时保持了 NCCs 标志物 CD271 的高表达水平。它们具有分化成多种细胞类型的能力：神经元、星形胶质细胞、黑色素细胞、平滑肌细胞、成骨细胞、脂肪细胞和软骨细胞。此外，它们还能被诱导分化为诱导间充质干细胞（iMSCs），后者保留了体细胞间充质干细胞的基本功能。与 FACS 或长期通道等传统方法相比，这种方法能以较低的成本和人力获取大量细胞，有望为未来细胞治疗应用中大规模 iNCCs 的稳定供应做出贡献。

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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来源期刊

Regenerative Therapy Engineering-Biomedical Engineering

CiteScore

6.00

自引率

2.30%

发文量

106

审稿时长

49 days

期刊介绍： Regenerative Therapy is the official peer-reviewed online journal of the Japanese Society for Regenerative Medicine. Regenerative Therapy is a multidisciplinary journal that publishes original articles and reviews of basic research, clinical translation, industrial development, and regulatory issues focusing on stem cell biology, tissue engineering, and regenerative medicine.