Deriving Retinal Pigment Epithelium (RPE) from Induced Pluripotent Stem (iPS) Cells by Different Sizes of Embryoid Bodies

Alberto Mu&#241;iz; Kaini R. Ramesh; Whitney A. Greene; Jae-Hyek Choi; Heuy-Ching Wang

doi:10.3791/52262

JoVE Journal > Developmental Biology

Please note that all translations are automatically generated. Click here for the English version.

Gelişim Biyolojisi

从诱导多能干得出视网膜色素上皮（RPE）（IPS），由胚体大小不同的细胞

Published: February 04, 2015

doi:

10.3791/52262

Alberto Muñiz¹, Kaini R. Ramesh¹, Whitney A. Greene¹, Jae-Hyek Choi¹, Heuy-Ching Wang¹

¹Ocular Trauma,U.S. Army Institute of Surgical Research

Özet

此报告的目的是描述协议来导出从诱导的多能干（iPS细胞）使用不同尺寸的胚状体的视网膜色素上皮细胞（RPE）。

Abstract

Pluripotent stem cells possess the ability to proliferate indefinitely and to differentiate into almost any cell type. Additionally, the development of techniques to reprogram somatic cells into induced pluripotent stem (iPS) cells has generated interest and excitement towards the possibility of customized personal regenerative medicine. However, the efficiency of stem cell differentiation towards a desired lineage remains low. The purpose of this study is to describe a protocol to derive retinal pigment epithelium (RPE) from iPS cells (iPS-RPE) by applying a tissue engineering approach to generate homogenous populations of embryoid bodies (EBs), a common intermediate during in vitro differentiation. The protocol applies the formation of specific size of EBs using microwell plate technology. The methods for identifying protein and gene markers of RPE by immunocytochemistry and reverse-transcription polymerase chain reaction (RT-PCR) are also explained. Finally, the efficiency of differentiation in different sizes of EBs monitored by fluorescence-activated cell sorting (FACS) analysis of RPE markers is described. These techniques will facilitate the differentiation of iPS cells into RPE for future applications.

Introduction

诱导多能干细胞（iPS细胞）是由重编程体细胞与外在因素¹派生的类型的多能干细胞。与此相反，胚胎干细胞（ESCs），另一种类型的多能干细胞，从胚泡^2-3的内细胞团生成。尽管他们的不同的起源，iPS细胞和胚胎干细胞是可比在其无限的容量在体外和在其分化成任何细胞类型的能力^4-5进行复制。 iPS细胞的这些特性使其成为理想的候选人在个性化的再生医学应用。最近的研究工作集中在开发健壮的分化协议用于生产特殊成年细胞包括视网膜色素上皮^{（RPE）6-11。}

于iPS来源的细胞潜在的临床应用中，定向分化为特定的细胞类型是至关重要的。有多种方法公布为胚胎干细胞和iPS细胞定向分化为RPE的良莠不齐的工作效率^{6-7，12-16。}我们仍然不知道有多少，发展和分化过程中执政细胞/组织命运的分子事件。在最近几年，已经作出努力来开发该分化方案，可以模仿的胚胎发育尽可能。在胚泡阶段，干细胞的未提交的人口都一起在三维微环境。因此，采用了不同的策略，使ESC / iPS细胞聚集在一起，在三个维度成长他们。这些干细胞聚集体被称为胚体（EB）。有研究表明，干细胞的分化的EB模仿胚胎发育的早期阶段，并且可以自发地产生原始内胚层在其外表面上。后来，随着EB开发的进展，所有三个胚谱系分化细胞的表型出现^17-18。日erefore，胚基分化协议已经吸引了大量的关注在体外分化ESC / iPS细胞，是一个很好的候选人RPE代从多能干细胞^13。

胚可以使用多种方法从ESC / iPS细胞进行。最初，胚被刮去附着的菌落，并保持它们在非粘附悬浮培养制成。然而，这种方法产生的EB，导致低再现性的异质群体。悬滴细胞培养和微孔基EBS形成其他流行的技术胚形成而产生定义尺寸的高度重复性的同质胚。另外，微孔的技术可以产生大量的聚集体以较少的努力。

内的EB细胞分化是通过从细胞外和细胞内的微形态线索多路复用调节。与此相反，以分化的纹olayer格式的EB为细胞的复杂的组装和细胞间信号发生¹⁷的平台。有趣的是，观察到用来制作个别的EB多能干细胞的数量来影响细胞的命运。例如，在人类胚胎干细胞的造血分化的研究中，观察到500个细胞EB对促进髓系分化，而1000细胞EB推向红系^20。在另一项研究中，较小的EB青睐定形内胚层分化而促进向神经外胚层分化^11,17更大的EB。

这些过去的研究有力地表明，用于制造单个的EB ESC / iPS细胞的数量的影响根据分化成任何细胞类型的胚。然而，据我们所知，有一些已经阐明其倾向胚大小的影响，区分对RPE目前没有研究。这项研究的目的是表征的影响EB大小对诱导多能干细胞（iPS细胞） – 视网膜色素上皮细胞（IPS-RPE）的分化，并确定最佳的细胞数量，使胚的对RPE细胞系定向分化。

Protocol

1.准备培养试剂和培养皿通过加入100ml 5×无血清补充到400毫升干细胞基础培养基的制备无饲养干细胞培养基。该介质是稳定的，在4℃下进行最多2周，并在-20℃下6个月。加的Rho相关，卷曲螺旋包含蛋白激酶（岩）抑制剂（Y-27362），以市售胚状体（EB）形成介质10μM的溶液。通过加入0.1mMβ巯基乙醇，0.1mM非必需氨基酸，2mM的L-谷氨酰胺，10％敲除血清替代品（KSR）和10微克/毫升?…

Representative Results

在这个实验中，iPS细胞进行培养，分化成从胚的视网膜色素上皮谱系。利用微孔板形成控制大小胚。如从图1可见EB形成为同质的微孔板。这些胚然后收集并接种在6孔板（图2）。 RPE可以通过经典六角形态，色素沉着，及表达的视网膜色素上皮标志物来鉴定。 12周文化后，200细胞胚制定了星形胶质细胞和成纤维细胞的形态。无色素沉着，观察这些细胞…

Discussion

为了实现多能干细胞用于细胞疗法的充分承诺，有必要调节其分化以一致和可再现的方式。这份报告描述了协议，形成利用微孔板技术尺寸控制EBS，开始分化为RPE，并确定RPE的蛋白质和基因标记。同步在体外分化，胚的大小均匀已知数字的iPS细胞在微孔板强迫聚集离心的形成。免疫细胞化学和逆转录聚合酶链反应（RT-PCR），用于监视所述表达式的RPE的蛋白质和基因说明。最后，分化的不同?…

Açıklamalar

The authors have nothing to disclose.

Acknowledgements

The opinions or assertions contained herein are the private views of the authors and are not to be construed as official or as reflecting the views of the Department of the Army or the Department of Defense. This research was performed while the authors Alberto Muñiz, Ramesh R Kaini, Whitney A Greene and Jae-Hyek Choi held a National Research Council Postdoctoral Research Associateship at the USAISR. This work was supported by U.S. Army Clinical Rehabilitative Medicine Research Program (CRMRP) and Military Operational Medicine Research Program (MOMRP).

Materials

Name of Material/ Equipment	Company	Catalog Number	Comments/Description
mTeSR1 media + 5X supplement	Stem Cell Technologies	5850
Y-27632 (Rock Inhibitor)	Stem Cell Technologies	72304
DMEM/F12	Life Technologies	11330-032
2-Mercaptoethanol	Sigma	M-7154
Non essential amino acids	Hyclone(Fisher)	SH30853.01
Knockout serum replacement	Life Technologies	10828-028
Gentamicin	Life Technologies	15750-060
L-Glutamine	Life Technologies	25030-081
MEM media	Life Technologies	10370-021
N1 supplement	Sigma	N-6530-5ML
Taurine	Sigma	T-8691-25G
Hydrocortisone	Sigma	H0888-1G
Fetal bovine serum	Hyclone(Fisher)	SH3008803HI
Triiodo-l-thyronine sodium salt	Sigma	T6397
Sodium hydroxide	Sigma	S5881
Dispase	Life Technologies	17105-041
Matrigel	BD Biosciences	354277
Phosphate buffered saline	Hyclone(Fisher)	10010-023
Aggrewell 400 plate	Stem Cell Technologies	27940
AggreWell medium	Stem Cell Technologies	5893
Accutase	Stem Cell Technologies	7920
BD Cytofix/Cytoperm Fixation/Permeabilization Kit	BD Biosciences	554714
Mouse Anti-PAX6 antibody	Developmental Studies Hybridoma Bank
Rabbit Anti- RX antibody	Abcam	Ab23340
Mouse Anti-MITF antibody	Thermo Scientific	MS-772-P
Rabbit Anti-ZO-1 antibody	Invitrogen	40-2200
RNeasy plus mini kit	Qiagen	74134
PCR master mix	promega	M7502
High capacity RNA to c DNA kit	Life Technologies	4387406

Referanslar

Takahashi, K., et al. Induction of pluripotent stem cells from fibroblast cultures. Nat Protoc. 2 (12), 3081-3089 (2007).
Reubinoff, B. E., et al. Embryonic stem cell lines from human blastocysts: somatic differentiation in vitro. Nat Biotechnol. 18 (4), 399-404 (2000).
Thomson, J. A., et al. Embryonic stem cell lines derived from human blastocysts. Science. 282 (5391), 1145-1147 (1998).
Takahashi, K., Yamanaka, S. Induction of pluripotent stem cells from mouse embryonic and adult fibroblast cultures by defined factors. Cell. 126 (4), 663-676 (2006).
Yu, J., et al. Induced pluripotent stem cell lines derived from human somatic cells. Science. 318 (5858), 1917-1920 (2007).
Buchholz, D. E., et al. Derivation of functional retinal pigmented epithelium from induced pluripotent stem cells. Stem Cells. 27 (10), 2427-2434 (2009).
Ukrohne, T. U., et al. Generation of retinal pigment epithelial cells from small molecules and OCT4 reprogrammed human induced pluripotent stem cells. Stem Cells Transl Med. 1 (2), 96-109 (2012).
Subba, R. M., Sasikala, M., Nageshwar, R. D. Thinking outside the liver: induced pluripotent stem cells for hepatic applications. World J Gastroenterol. 19 (22), 3385-3396 (2013).
Yoshida, Y., Yamanaka, S. iPS cells: a source of cardiac regeneration. J Mol Cell Cardiol. 50 (2), 327-332 (2011).
Mak, S. K., et al. Small molecules greatly improve conversion of human-induced pluripotent stem cells to the neuronal lineage. Stem Cells Int. 2012, 140427 (2012).
Bauwens, C. L., et al. Control of human embryonic stem cell colony and aggregate size heterogeneity influences differentiation trajectories. Stem Cells. 26 (9), 2300-2310 (2008).
Cour la, M., Tezel, T. The Retinal Pigment Epithelium. Advances in Organ Biology. 10, 253-273 (2006).
Vaajassari, V., et al. Toward the defined and xeno-free differentiation of functional human pluripotent stem cell-derived retinal pigment epithelial cells. Mol Vis. 17, 558-575 (2011).
Carr, A. J., et al. Protective effects of human iPS-derived retinal pigment epithelium cell transplantation in the retinal dystrophic rat. PLoS One. 4 (12), e8152 (2009).
Muniz, A., et al. Retinoid uptake, processing, and secretion in human iPS-RPE support the visual cycle. Invest Ophthalmol Vis Sci. 55 (1), 198-209 (2014).
Meyer, J. S., et al. Modeling early retinal development with human embryonic and induced pluripotent stem cells. Proc Natl Acad Sci U S A. 106 (39), 16698-16703 (2009).
Bratt-Leal, A. M., Carpenedo, R. L., McDevitt, T. C. Engineering the embryoid body microenvironment to direct embryonic stem cell differentiation. Biotechnol Prog. 25 (1), 43-51 (2009).
Kurosawa, H. Methods for inducing embryoid body formation: in vitro differentiation system of embryonic stem cells. J Biosci Bioeng. 103 (5), 389-398 (2007).
Itskovitz-Eldor, J., et al. Differentiation of human embryonic stem cells into embryoid bodies compromising the three embryonic germ layers. Mol Med. 6 (2), 88-95 (2000).
Ng, E. S., et al. Forced aggregation of defined numbers of human embryonic stem cells into embryoid bodies fosters robust, reproducible hematopoietic differentiation. Blood. 106 (5), 1601-1603 (2005).
Maminishkis, A., et al. Confluent monolayers of cultured human fetal retinal pigment epithelium exhibit morphology and physiology of native tissue. Invest Ophthalmol Vis Sci. 47 (8), 3612-3624 (2006).

Etiketler

Induced Pluripotent Stem Cells Retinal Pigment Epithelium Embryoid Bodies Differentiation Microwell Plates Immunocytochemistry RT-PCR FACS Analysis

Play Video

PDF

DOI

DOWNLOAD MATERIALS LIST

Bu Makaleden Alıntı Yapın

Muñiz, A., Ramesh, K. R., Greene, W. A., Choi, J., Wang, H. Deriving Retinal Pigment Epithelium (RPE) from Induced Pluripotent Stem (iPS) Cells by Different Sizes of Embryoid Bodies. J. Vis. Exp. (96), e52262, doi:10.3791/52262 (2015).