ARX-T2A-H2B-CFP x C-PEP-mCherry -hiPSC, ARX-CFPxC-PEP-mCherry-hiPSC, ARXCFP/CFP x C-PEPmCherry/+ hiPSC
HMGUi001-A-54
General
Cell Line |
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hPSCreg name | HMGUi001-A-54 |
Cite as: | HMGUi001-A-54 |
Alternative name(s) |
ARX-T2A-H2B-CFP x C-PEP-mCherry -hiPSC, ARX-CFPxC-PEP-mCherry-hiPSC, ARXCFP/CFP x C-PEPmCherry/+ hiPSC
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Cell line type | Human induced pluripotent stem cell (hiPSC) |
Similar lines | No similar lines found. |
Last update | 16th September 2024 |
Notes | This line is a subclone of HMGUi001-A-4. |
User feedback | |
Provider |
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Generator | Institute of Diabetes and Regeneration Research (IDR) |
Owner | Institute of Diabetes and Regeneration Research (IDR) |
Distributors | |
Derivation country | Germany |
External Databases |
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BioSamples | SAMEA116049440 |
General Information |
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* Is the cell line readily obtainable for third parties? |
No |
Subclone of |
Donor Information
General Donor Information |
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Sex | female |
Ethnicity | Caucasian |
Phenotype and Disease related information (Donor) |
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Diseases | No disease was diagnosed.
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Family history | no |
Is the medical history available upon request? | no |
Is clinical information available? | no |
Other Genotyping (Donor) |
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Is there genome-wide genotyping or functional data available? |
No
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Donor Relations |
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Other cell lines of this donor | |
External Databases (Donor) |
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BioSamples | SAMEA5696688 |
Ethics
Also have a look at the ethics information for the parental line
HMGUi001-A
.
Is there an MTA available for the cell line? | No |
For generation of the cell line, who was the supplier of any recombined DNA vectors or commercial kits used? | Vectors were generated at IDR, pU6-(BbsI)-sgRNA-CAG-Cas9-Venus-bpA plasmid (Addgene plasmid #86986) was used. |
Are you aware of any constraints on the use or distribution of the cell line from the owner or any parties identified in the query above? | Yes |
Constraints for use or distribution | According to donor consent the line must not be used for commercial purposes. For research purposes project-specific review by a medical Ethics Committee is obligatory. |
hIPSC Derivation
General |
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The source cell information can be found in the parental cell line
HMGUi001-A.
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Passage number reprogrammed | 26 |
Reprogramming method |
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Vector type | Non-integrating |
Vector | HMGUi001-A-4 was targeted with two vectors. For the first vector, the Cas9-Venus-sgRNA vector, a sgRNA was cloned into the pU6-(BbsI)-sgRNA-CAG-Cas9-Venus-bpA plasmid (Addgene plasmid #86986). Cas9 and a targeting site specific sgRNA were expressed from this vector to induce a double strand break at the targeting region. The second vector contained the template for the intended homology directed repair: the mCherry coding sequence flanked by a 1111 bp left homology arm (5’ HA) and a 901 bp right homology arm (3’ HA). Silent mutations in the sgRNA binding site were introduced to avoid cutting of the correctly inserted sequences. |
Vector free reprogramming |
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Other |
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Selection criteria for clones | Transfected cells expressed Venus and were sorted by FACS. The genotype of the clones was screened by PCR and verified by Sanger sequencing. |
Derived under xeno-free conditions |
Yes |
Derived under GMP? |
No |
Available as clinical grade? |
No |
Culture Conditions
Surface coating | Matrigel/Geltrex |
Feeder cells |
No |
Passage method | EDTA |
O2 Concentration | 21 % |
CO2 Concentration | 5 % |
Medium |
Other medium:
Base medium: StemMACS iPS-Brew XF medium
Main protein source: xeno-free Serum concentration: 0 % |
Has Rock inhibitor (Y27632) been used at passage previously with this cell line? | Yes |
Has Rock inhibitor (Y27632) been used at cryo previously with this cell line? | Yes |
Has Rock inhibitor (Y27632) been used at thaw previously with this cell line? | Yes |
Characterisation
Analysis of Undifferentiated Cells
Marker | Expressed | Immunostaining | RT-PCR | Flow Cytometry | Enzymatic Assay | Expression Profiles |
SOX2 |
Yes |
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POU5F1 (OCT-4) |
Yes |
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SSEA-4 |
Yes |
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TRA 1-60 |
Yes |
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Oct-3 |
Yes |
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Differentiation Potency
Microbiology / Virus Screening |
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Mycoplasma | Negative |
Genotyping
Karyotyping (Cell Line) |
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Has the cell line karyotype been analysed? |
Yes
46,XX
Karyotyping method:
G-Banding
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Other Genotyping (Cell Line) |
Genetic Modification
Genetic modifications not related to a disease |
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