Loss of Oct4 expression during the development of murine embryoid bodies

Abdulrahim A. Sajini; Lucas V. Greder; James R. Dutton; Jonathan M W Slack

doi:10.1016/j.ydbio.2012.08.008

Loss of Oct4 expression during the development of murine embryoid bodies

Abdulrahim A. Sajini, Lucas V. Greder, James R. Dutton, Jonathan M W Slack

Research output: Contribution to journal › Article › peer-review

23 Scopus citations

Abstract

We describe the internal organization of murine embryoid bodies (EBs) in terms of the structures and cell types formed as Oct4 expression becomes progressively lost. This is done by making the EBs from iPS cells carrying a novel Oct4 reporter (Oct4-MerCreMer;. mTmG) which is inducible, sensitive, and permanent in all cellular progeny. When these EBs are treated with tamoxifen, the Oct4 expressing cells switch from a red to a green fluorescence color, and this is maintained thereafter by all their progeny. We show that there is no specific pattern in which Oct4 is downregulated, rather it appears to be spatially random. Many of the earliest cells to lose Oct4 expression stain positive for markers of visceral endoderm (DAB2, α-fetoprotein (AFP), HNF4). These are randomly located, although if endoderm differentiation is allowed to commence before EB formation then an external layer is formed. This is true both of EBs made from the reporter iPS cells, or from an embryo-derived mouse ES line (R1 cells). Markers of the early body axis, Brachyury (BRA) and FOXA2, usually showed a concentration of positive cells in one region of the EB, but the morphology is not predictable and there are also scattered cells expressing these markers. These patterns are similar in R1 cells. Use of the Oct4 reporter showed a difference between BRA and FOXA2. BRA, which marks the early mesoderm, node and notochord, arises in Oct4 expressing cells on days 3-4. FOXA2, which marks the floor plate of the neural tube and definitive endoderm, as well as the node and notochord, arises at the same time but mostly in cells that have already lost Oct4 expression. Several clumps of cardiomyocytes are visible by days 7-8 of EB development, both in our iPS cells and in R1 cells. Using the Oct4 reporter we show that the cells forming these clumps lose Oct4 expression between days 3 and 5. Overall, our results indicate that EBs recapitulate normal development quite well in terms of the tempo of events and the appearance of specific markers, but they do not resemble embryos in terms of their morphology.

Original language	English (US)
Pages (from-to)	170-179
Number of pages	10
Journal	Developmental Biology
Volume	371
Issue number	2
DOIs	https://doi.org/10.1016/j.ydbio.2012.08.008
State	Published - Nov 15 2012

Bibliographical note

Funding Information:
We thank Randy Daughters, Ersin Akinci, Anannya Banga, Susan Keirstead, Nobuaki Kikyo and Sandeep Gupta for advice and support. This study was part funded by Grants U01HL100407 and R01DK080747 from the National Institutes of Health . A.S. was funded by a scholarship from the University of Tabuk, Saudi Arabia.

Keywords

Alpha-fetoprotein
Brachyury
Cardiac troponin T
Dab2
Embryoid body
Endoderm
FoxA2
HNF4
Induced pluripotent stem cells
Mesoderm
Oct4

Access

10.1016/j.ydbio.2012.08.008

OpenUrl availability

Full text

Cite this

@article{2185d11515294dc8940abe36cdf8351e,

title = "Loss of Oct4 expression during the development of murine embryoid bodies",

abstract = "We describe the internal organization of murine embryoid bodies (EBs) in terms of the structures and cell types formed as Oct4 expression becomes progressively lost. This is done by making the EBs from iPS cells carrying a novel Oct4 reporter (Oct4-MerCreMer;. mTmG) which is inducible, sensitive, and permanent in all cellular progeny. When these EBs are treated with tamoxifen, the Oct4 expressing cells switch from a red to a green fluorescence color, and this is maintained thereafter by all their progeny. We show that there is no specific pattern in which Oct4 is downregulated, rather it appears to be spatially random. Many of the earliest cells to lose Oct4 expression stain positive for markers of visceral endoderm (DAB2, α-fetoprotein (AFP), HNF4). These are randomly located, although if endoderm differentiation is allowed to commence before EB formation then an external layer is formed. This is true both of EBs made from the reporter iPS cells, or from an embryo-derived mouse ES line (R1 cells). Markers of the early body axis, Brachyury (BRA) and FOXA2, usually showed a concentration of positive cells in one region of the EB, but the morphology is not predictable and there are also scattered cells expressing these markers. These patterns are similar in R1 cells. Use of the Oct4 reporter showed a difference between BRA and FOXA2. BRA, which marks the early mesoderm, node and notochord, arises in Oct4 expressing cells on days 3-4. FOXA2, which marks the floor plate of the neural tube and definitive endoderm, as well as the node and notochord, arises at the same time but mostly in cells that have already lost Oct4 expression. Several clumps of cardiomyocytes are visible by days 7-8 of EB development, both in our iPS cells and in R1 cells. Using the Oct4 reporter we show that the cells forming these clumps lose Oct4 expression between days 3 and 5. Overall, our results indicate that EBs recapitulate normal development quite well in terms of the tempo of events and the appearance of specific markers, but they do not resemble embryos in terms of their morphology.",

keywords = "Alpha-fetoprotein, Brachyury, Cardiac troponin T, Dab2, Embryoid body, Endoderm, FoxA2, HNF4, Induced pluripotent stem cells, Mesoderm, Oct4",

author = "Sajini, {Abdulrahim A.} and Greder, {Lucas V.} and Dutton, {James R.} and Slack, {Jonathan M W}",

note = "Funding Information: We thank Randy Daughters, Ersin Akinci, Anannya Banga, Susan Keirstead, Nobuaki Kikyo and Sandeep Gupta for advice and support. This study was part funded by Grants U01HL100407 and R01DK080747 from the National Institutes of Health . A.S. was funded by a scholarship from the University of Tabuk, Saudi Arabia. ",

year = "2012",

month = nov,

day = "15",

doi = "10.1016/j.ydbio.2012.08.008",

language = "English (US)",

volume = "371",

pages = "170--179",

journal = "Developmental Biology",

issn = "0012-1606",

publisher = "Academic Press Inc.",

number = "2",

}

TY - JOUR

T1 - Loss of Oct4 expression during the development of murine embryoid bodies

AU - Sajini, Abdulrahim A.

AU - Greder, Lucas V.

AU - Dutton, James R.

AU - Slack, Jonathan M W

N1 - Funding Information: We thank Randy Daughters, Ersin Akinci, Anannya Banga, Susan Keirstead, Nobuaki Kikyo and Sandeep Gupta for advice and support. This study was part funded by Grants U01HL100407 and R01DK080747 from the National Institutes of Health . A.S. was funded by a scholarship from the University of Tabuk, Saudi Arabia.

PY - 2012/11/15

Y1 - 2012/11/15

N2 - We describe the internal organization of murine embryoid bodies (EBs) in terms of the structures and cell types formed as Oct4 expression becomes progressively lost. This is done by making the EBs from iPS cells carrying a novel Oct4 reporter (Oct4-MerCreMer;. mTmG) which is inducible, sensitive, and permanent in all cellular progeny. When these EBs are treated with tamoxifen, the Oct4 expressing cells switch from a red to a green fluorescence color, and this is maintained thereafter by all their progeny. We show that there is no specific pattern in which Oct4 is downregulated, rather it appears to be spatially random. Many of the earliest cells to lose Oct4 expression stain positive for markers of visceral endoderm (DAB2, α-fetoprotein (AFP), HNF4). These are randomly located, although if endoderm differentiation is allowed to commence before EB formation then an external layer is formed. This is true both of EBs made from the reporter iPS cells, or from an embryo-derived mouse ES line (R1 cells). Markers of the early body axis, Brachyury (BRA) and FOXA2, usually showed a concentration of positive cells in one region of the EB, but the morphology is not predictable and there are also scattered cells expressing these markers. These patterns are similar in R1 cells. Use of the Oct4 reporter showed a difference between BRA and FOXA2. BRA, which marks the early mesoderm, node and notochord, arises in Oct4 expressing cells on days 3-4. FOXA2, which marks the floor plate of the neural tube and definitive endoderm, as well as the node and notochord, arises at the same time but mostly in cells that have already lost Oct4 expression. Several clumps of cardiomyocytes are visible by days 7-8 of EB development, both in our iPS cells and in R1 cells. Using the Oct4 reporter we show that the cells forming these clumps lose Oct4 expression between days 3 and 5. Overall, our results indicate that EBs recapitulate normal development quite well in terms of the tempo of events and the appearance of specific markers, but they do not resemble embryos in terms of their morphology.

AB - We describe the internal organization of murine embryoid bodies (EBs) in terms of the structures and cell types formed as Oct4 expression becomes progressively lost. This is done by making the EBs from iPS cells carrying a novel Oct4 reporter (Oct4-MerCreMer;. mTmG) which is inducible, sensitive, and permanent in all cellular progeny. When these EBs are treated with tamoxifen, the Oct4 expressing cells switch from a red to a green fluorescence color, and this is maintained thereafter by all their progeny. We show that there is no specific pattern in which Oct4 is downregulated, rather it appears to be spatially random. Many of the earliest cells to lose Oct4 expression stain positive for markers of visceral endoderm (DAB2, α-fetoprotein (AFP), HNF4). These are randomly located, although if endoderm differentiation is allowed to commence before EB formation then an external layer is formed. This is true both of EBs made from the reporter iPS cells, or from an embryo-derived mouse ES line (R1 cells). Markers of the early body axis, Brachyury (BRA) and FOXA2, usually showed a concentration of positive cells in one region of the EB, but the morphology is not predictable and there are also scattered cells expressing these markers. These patterns are similar in R1 cells. Use of the Oct4 reporter showed a difference between BRA and FOXA2. BRA, which marks the early mesoderm, node and notochord, arises in Oct4 expressing cells on days 3-4. FOXA2, which marks the floor plate of the neural tube and definitive endoderm, as well as the node and notochord, arises at the same time but mostly in cells that have already lost Oct4 expression. Several clumps of cardiomyocytes are visible by days 7-8 of EB development, both in our iPS cells and in R1 cells. Using the Oct4 reporter we show that the cells forming these clumps lose Oct4 expression between days 3 and 5. Overall, our results indicate that EBs recapitulate normal development quite well in terms of the tempo of events and the appearance of specific markers, but they do not resemble embryos in terms of their morphology.

KW - Alpha-fetoprotein

KW - Brachyury

KW - Cardiac troponin T

KW - Dab2

KW - Embryoid body

KW - Endoderm

KW - FoxA2

KW - HNF4

KW - Induced pluripotent stem cells

KW - Mesoderm

KW - Oct4

UR - http://www.scopus.com/inward/record.url?scp=84867143463&partnerID=8YFLogxK

UR - http://www.scopus.com/inward/citedby.url?scp=84867143463&partnerID=8YFLogxK

U2 - 10.1016/j.ydbio.2012.08.008

DO - 10.1016/j.ydbio.2012.08.008

M3 - Article

C2 - 22960235

AN - SCOPUS:84867143463

SN - 0012-1606

VL - 371

SP - 170

EP - 179

JO - Developmental Biology

JF - Developmental Biology

IS - 2

ER -

Loss of Oct4 expression during the development of murine embryoid bodies

Abstract

Bibliographical note

Keywords

Access

OpenUrl availability

Other files and links

Fingerprint

Cite this