TAUi002-A

General

Cell Line
hPSCreg name	TAUi002-A
Cite as:	TAUi002-A (RRID:CVCL_RN25)
Alternative name(s)	UTA.04602.WT
Cell line type	Human induced pluripotent stem cell (hiPSC)
Similar lines	No similar lines found.
Last update	19th April 2022
User feedback	Written by on No feedback available yet. Login to share your feedback, experiences or results with the research community.
Provider
Generator	Tampere University (TAU)
Derivation country	Finland
External Databases
BioSamples	SAMEA6880676
Cellosaurus	CVCL_RN25
Wikidata	Q54992209
General Information
Publications	(unknown author). Electrophysiological Evaluation of Human Induced Pluripotent Stem Cell- Derived Cardiomyocytes Obtained by Different Methods. . . Kujala K et al. Cell model of catecholaminergic polymorphic ventricular tachycardia reveals early and delayed afterdepolarizations. PloS one. 2012;7(9):e44660. Ojala M et al. Culture conditions affect cardiac differentiation potential of human pluripotent stem cells. PloS one. 2012;7(10):e48659. Lahti AL et al. Model for long QT syndrome type 2 using human iPS cells demonstrates arrhythmogenic characteristics in cell culture. Disease models & mechanisms. 2012 Mar;5(2):220-30. Ahola A et al. Video image-based analysis of single human induced pluripotent stem cell derived cardiomyocyte beating dynamics using digital image correlation. Biomedical engineering online. 2014 Apr 7;13:39. Penttinen K et al. Novel Analysis Software for Detecting and Classifying Ca2+ Transient Abnormalities in Stem Cell-Derived Cardiomyocytes. PloS one. 2015;10(8):e0135806. Penttinen K et al. Antiarrhythmic Effects of Dantrolene in Patients with Catecholaminergic Polymorphic Ventricular Tachycardia and Replication of the Responses Using iPSC Models. PloS one. 2015;10(5):e0125366. Kiviaho AL et al. Distinct electrophysiological and mechanical beating phenotypes of long QT syndrome type 1-specific cardiomyocytes carrying different mutations. International journal of cardiology. Heart & vasculature. 2015 Sep 1;8:19-31. Ojala M et al. Mutation-Specific Phenotypes in hiPSC-Derived Cardiomyocytes Carrying Either Myosin-Binding Protein C Or α-Tropomyosin Mutation for Hypertrophic Cardiomyopathy. Stem cells international. 2016;2016:1684792. Kuusela J et al. The Effects of Pharmacological Compounds on Beat Rate Variations in Human Long QT-Syndrome Cardiomyocytes. Stem cell reviews and reports. 2016 Dec;12(6):698-707. Ahola A et al. Simultaneous Measurement of Contraction and Calcium Transients in Stem Cell Derived Cardiomyocytes. Annals of biomedical engineering. 2018 Jan;46(1):148-158. Pölönen RP et al. Mutation-specific differences in arrhythmias and drug responses in CPVT patients: simultaneous patch clamp and video imaging of iPSC derived cardiomyocytes. Molecular biology reports. 2020 Feb;47(2):1067-1077.
* Is the cell line readily obtainable for third parties?	Yes Cell line can only be used in: Fit4purpose-OOC project Research use: allowed Clinical use: not allowed Commercial use: allowed

Donor Information

General Donor Information

Sex

female

Ethnicity

Caucasian

Phenotype and Disease related information (Donor)

Diseases

No disease was diagnosed.

Karyotyping (Donor)

Has the donor karyotype been analysed?

No

Other Genotyping (Donor)

Is there genome-wide genotyping or functional data available?

No

External Databases (Donor)

BioSamples

SAMEA6880677

Ethics

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
Has the donor been informed that participation will not directly influence their personal treatment?	Yes
Can you provide us with a copy of the Donor Information Sheet provided to the donor?	Yes
Do you (Depositor/Provider) hold the original Donor Consent Form?	Yes
Please indicate whether the data associated with the donated material has been pseudonymised or anonymised.	pseudonymised
Does consent explicitly allow the derivation of pluripotent stem cells?	Yes
Does consent pertain to a specific research project?	No
Does consent permit unforeseen future research, without further consent?	Yes
Does the consent permit uses of donated embryo/tissue or derived cell line intended for clinical treatment or human applications?	No
Does consent expressly prevent development of commercial products?	No
Does consent expressly prevent financial gain from any use of the donated embryo/tissue, including any product made from it?	No
Does consent prevent CELLS DERIVED FROM THE DONATED BIOSAMPLE from being made available to researchers anywhere in the world?	No
Does consent permit research by
an academic institution?	Yes
a public organisation?	Yes
a non-profit company?	Yes
a for-profit corporation?	Yes

How may genetic information associated with the cell line be accessed?	No information
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?	Ethics Committee of Pirkanmaa Hospital District
Approval number	R08070
Has a favourable opinion been obtained from a research ethics committee, or other ethics review panel, in relation to the PROPOSED PROJECT, involving use of donated embryo/tissue or derived cells?	No
For generation of the cell line, who was the supplier of any recombined DNA vectors or commercial kits used?

hIPSC Derivation

General
Source cell type	Skin fibroblast
Collected in	2010
Reprogramming method
Vector type	Integrating
Vector	Virus (Retrovirus)
Genes	POU5F1 SOX2 KLF4 MYC
Is the used vector excisable?	Unknown
Absence of reprogramming vector(s)?	Unknown
Reprogramming vectors silenced?
Vector free reprogramming
Type of used vector free reprogramming factor(s)	None
Other
Selection criteria for clones	Morphology
Derived under xeno-free conditions	No
Derived under GMP?	No
Available as clinical grade?	No

Culture Conditions

Surface coating

Gelatin

Feeder cells

CF-1 MEF MITC
Cellfinder Ont Id: CELDA_00007731

Passage method

Enzymatically

Collagenase

CO2 Concentration

5 %

Medium

Other medium:

Base medium: KO-DMEM
Main protein source: Knock-out serum replacement
Serum concentration: 20 %

Supplements

Supplement	Amount	Unit
NEA		%
Glutamax
Pen/Strep
FGF
β-mercaptoethanol

Has Rock inhibitor (Y27632) been used at passage previously with this cell line?

No

Has Rock inhibitor (Y27632) been used at cryo previously with this cell line?

No

Has Rock inhibitor (Y27632) been used at thaw previously with this cell line?

No

Characterisation

Analysis of Undifferentiated Cells

Marker Expression

Marker	Expressed	Immunostaining	RT-PCR	Flow Cytometry	Enzymatic Assay	Expression Profiles
NANOG	Yes	–
POU5F1 (OCT-4)	Yes	–
SOX2	Yes	–
SSEA-4	Yes	–
TRA 1-60	Yes	–
TRA 1-81	Yes	–

Differentiation Potency

Endoderm

Endoderm
Ont Id: UBERON_0000925

In vitro spontaneous differentiation

Marker	Expressed
AFP	Yes

Protocol or reference

eb 04602.WT.jpg

EB PCR

Mesoderm

Mesoderm
Ont Id: UBERON_0000926

In vitro spontaneous differentiation

Marker	Expressed
KDR	Yes

Protocol or reference

eb 04602.WT.jpg

Ectoderm

Ectoderm
Ont Id: UBERON_0000924

In vitro spontaneous differentiation

Marker	Expressed
nestin	Yes

Protocol or reference

eb 04602.WT.jpg

Genotyping

Karyotyping (Cell Line)
Has the cell line karyotype been analysed?	Yes 46XX karyotype_UTA.04602_.WT_.jpg Karyotyping method: G-Banding
Other Genotyping (Cell Line)

UTA.04602.WT

General

Cell Line

Provider

External Databases

General Information

Donor Information

General Donor Information

Phenotype and Disease related information (Donor)

Karyotyping (Donor)

Other Genotyping (Donor)

External Databases (Donor)

Ethics

Does consent permit research by

hIPSC Derivation

General

Reprogramming method

Vector free reprogramming

Other

Culture Conditions

Characterisation

Analysis of Undifferentiated Cells

Differentiation Potency

Genotyping

Karyotyping (Cell Line)

Other Genotyping (Cell Line)