HVRDe001-A

General

Cell Line
hPSCreg name	HVRDe001-A
Cite as:	HVRDe001-A (RRID:CVCL_B139)
Alternative name(s)	HuES1
Cell line type	Human embryonic stem cell (hESC)
Similar lines	HVRDe001-A-1
Last update	4th September 2022
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Provider
Generator	Harvard University (HVRD) Contact: Melton Lab (MLB)
Derivation country	United States
External Databases
Cellosaurus	CVCL_B139
NIHhESC	NIHhESC-09-0014
Wikidata	Q54896736
General Information
Publications	Cowan CA et al. Derivation of embryonic stem-cell lines from human blastocysts. The New England journal of medicine. 2004 Mar 25;350(13):1353-6. International Stem Cell Initiative et al. Characterization of human embryonic stem cell lines by the International Stem Cell Initiative. Nature biotechnology. 2007 Jul;25(7):803-16. Braam SR et al. Feeder-free culture of human embryonic stem cells in conditioned medium for efficient genetic modification. Nature protocols. 2008;3(9):1435-43. Chen AE et al. Optimal timing of inner cell mass isolation increases the efficiency of human embryonic stem cell derivation and allows generation of sibling cell lines. Cell stem cell. 2009 Feb 6;4(2):103-6. Bock C et al. Reference Maps of human ES and iPS cell variation enable high-throughput characterization of pluripotent cell lines. Cell. 2011 Feb 4;144(3):439-52. Ramirez JM et al. Brief report: benchmarking human pluripotent stem cell markers during differentiation into the three germ layers unveils a striking heterogeneity: all markers are not equal. Stem cells (Dayton, Ohio). 2011 Sep;29(9):1469-74. Guhr A et al. Recent Trends in Research with Human Pluripotent Stem Cells: Impact of Research and Use of Cell Lines in Experimental Research and Clinical Trials. Stem cell reports. 2018 Aug 14;11(2):485-496.
Projects	ESNATS: Embryonic stem cell-based novel alternative testing strategies StemProteostasis: Mediation of stem cell identity and aging by proteostasis SCR&TOX: Stem Cells for Relevant Efficient Extended and Normalized Toxicology
* Is the cell line readily obtainable for third parties?	Yes
Subclones	HVRDe001-A-1

Donor Information

General Donor Information
Sex	female
Phenotype and Disease related information (Donor)
Diseases

Ethics

Was the embryo established purely for research purposes?	No
Have both parents consented to the use of the embryo for ESC derivation?	No
Has informed consent been obtained from the donor of the embryo/tissue from which the pluripotent stem cells have been derived?	Yes
Was the consent voluntarily given?	Yes
Alternatives to consent are available?	Yes
Alternatives to consent	lease see the NIH hESC Registry https://grants.nih.gov/stem_cells/registry/current.htm?id=40 HUES 9 was given the NIH Approval Number NIHhESC-09-0014
Alternative consent approval number	NIHhESC-09-0014
Please indicate whether the data associated with the donated material has been pseudonymised or anonymised.	anonymised
Does consent explicitly allow the derivation of pluripotent stem cells?	Yes
Does consent expressly prevent the derivation of pluripotent stem cells?	No
How may genetic information associated with the cell line be accessed?
Will the donor expect to receive financial benefit, beyond reasonable expenses, in return for donating the biosample?	No
Has a favourable opinion been obtained from a research ethics committee, or other ethics review panel, in relation to the Research Protocol including the consent provisions?	Yes
Name of accrediting authority involved?	Harvard University IRB
Approval number	unknown/check http://stemcelldistribution.harvard.edu/content/view/21#hues-lines

hESC Derivation

Embryo stage	Blastula with ICM and Trophoblast
Supernumerary embryos from IVF treatment?	Yes
PGD Embryo?	No
Expansion status	4 Stephenson 2007
ICM morphology	A Stephenson 2007
Trophectoderm morphology	b Stephenson 2007
ZP removal technique	Chemical
Cell isolation	Immunosurgery
Cell seeding	Isolated ICM

Culture Conditions

Feeder cells

Mouse Embryonic Fibroblast Cell
Cellfinder Ont Id: EFO_0004040

CO2 Concentration

5 %

Medium

Other medium:

Base medium: Knockout-DMEM
Main protein source: Knock-out serum replacement
Serum concentration: 10 %

Supplements

Supplement	Amount	Unit
bFGF		%

Characterisation

Analysis of Undifferentiated Cells

Marker Expression

Marker	Expressed	Immunostaining	RT-PCR	Flow Cytometry	Enzymatic Assay	Expression Profiles
Alkaline Phosphatase	Yes
POU5F1 (OCT-4)	Yes
SSEA-3	Yes
SSEA-4	Yes
TRA 1-60	Yes
TRA 1-81	Yes
DNMT3B	Yes
GABRB3	Yes
GDF3	Yes
NANOG	Yes
ZFP42 (REX-1)	Yes
SOX2	Yes
TDGF1	Yes

Differentiation Potency

Endoderm

Endoderm
Ont Id: UBERON_0000925

In vivo teratoma

In vitro spontaneous differentiation

Mesoderm

Mesoderm
Ont Id: UBERON_0000926

In vivo teratoma

In vitro spontaneous differentiation

Ectoderm

Ectoderm
Ont Id: UBERON_0000924

In vivo teratoma

In vitro spontaneous differentiation

Genotyping

Karyotyping (Cell Line)
Has the cell line karyotype been analysed?	Yes 46XX Passage number: 29
Other Genotyping (Cell Line)

HuES1

General

Cell Line

Provider

External Databases

General Information

Donor Information

General Donor Information

Phenotype and Disease related information (Donor)

Ethics

hESC Derivation

Culture Conditions

Characterisation

Analysis of Undifferentiated Cells

Differentiation Potency

Genotyping

Karyotyping (Cell Line)

Other Genotyping (Cell Line)