ipsc lines (Jackson Laboratory)
86
Structured Review
Jackson Laboratory
ipsc lines
Ipsc Lines, supplied by Jackson Laboratory, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/ipsc lines/product/Jackson Laboratory
Average 86 stars, based on 1 article reviews
Ipsc Lines, supplied by Jackson Laboratory, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/ipsc lines/product/Jackson Laboratory
Average 86 stars, based on 1 article reviews
ipsc lines - by Bioz Stars,
2026-06
86/100 stars
Images
1) Product Images from "Molecular and genetic heterogeneity in iPSCs derived from an outbred laboratory mouse population"
Article Title: Molecular and genetic heterogeneity in iPSCs derived from an outbred laboratory mouse population
Journal: bioRxiv
doi: 10.64898/2026.05.02.722403
Figure Legend Snippet: Tail tip fibroblasts from non-sibling Diversity Outbred mice were cultured on gelatin-coated plates and reprogrammed by lentiviral transduction of a doxycycline-inducible mouse OKSM cassette. Twenty-four hours after transduction, virus-containing medium was replaced with mESM + 2i/LIF supplemented with doxycycline to induce expression of the reprogramming factors. Emerging iPSC colonies were pooled and expanded as polyclonal lines. After three passages, lines were cryopreserved at P3. One vial per line was subsequently expanded to P5 for quality control screening and genotyping. Finalized lines were banked with associated metadata in The Jackson Laboratory Biobank (see Supplemental Table 1).
Techniques Used: Cell Culture, Transduction, Virus, Expressing, Control
Figure Legend Snippet: (A) Founder haplotype frequencies across chromosomes were estimated from GigaMUGA genotypes. Contributions from each of the eight DO founder strains are shown for chromosomes 1–19 and X. Deviations from the expected 0.125 founder contribution are summarized in Supplemental Table 2. (B) Pairwise kinship coefficients were calculated from GigaMUGA-derived genotypes to assess relatedness among iPSC lines. Eight pairs of lines showed high kinship (kin_raw > 0.4; highlighted in green and arrows), and one member of each pair was flagged in the final panel . All remaining line pairs showed kinship values consistent with non-sibling Diversity Outbred mice.
Techniques Used: Derivative Assay
Figure Legend Snippet: (A) Example of growth profiling of male and female DO iPSC lines. Cells were cultured for 96 hours and cell counts were used to calculate doubling time. Lines were assayed across multiple experimental batches. Representative colony morphologies are shown, including flattened morphology observed in some lines (e.g., line 5387, XX, 72 hours). (B) Embryoid body (EB) formation from 12 randomly selected iPSC lines. All lines formed EBs, with variation in EB morphology, some smooth and spherical and some rough and irregular, depending on the line. (C) Gene expression analysis before and after EB differentiation. RNA was collected from undifferentiated iPSCs and from EBs. Expression of pluripotency markers and early lineage markers representing ectoderm, mesoderm, and endoderm was quantified. Undifferentiated lines showed high pluripotency marker expression and low lineage marker expression, whereas EBs showed reduced pluripotency marker expression and increased lineage marker expression.
Techniques Used: Cell Culture, Gene Expression, Expressing, Marker
Figure Legend Snippet: (A) Gene expression of core pluripotency genes and early lineage markers in 218 DO iPSC lines. (B) Variance component analysis showing contributing factors to the variance in gene expression. Genotype is represented by the top 10 principal components informed by genotype probabilities.
Techniques Used: Gene Expression
Figure Legend Snippet: Quantile–quantile (Q–Q) plots of per-sample chromosome expression scores (median gene-level z-scores) were generated for each chromosome using the data from 218 DO iPSC lines. Observed values were statistically compared to the expected normal distribution. Deviation from the diagonal reflects broad chromosome-scale expression shifts. (A, B) Two examples are shown, one for a chromosome without gains or losses (Chromosome 2, A) and one for which there were frequent copy number gains (Chromosome 11, B). (C) To provide an overview for all chromosomes, the chromosome Z score was plotted for each iPSC line. Potential copy number gains were observed for Chromosomes 1, 6, 8, 11, 12, 13, and 14. Potential copy number losses were found for Chromosomes 7, 12, and 19.
Techniques Used: Expressing, Generated
![( A ) Schematic overview of the in vitro experimental design to test the Alu insertion’s functional impact in the human induced pluripotent stem cell (iPSC) line, <t>KOLF2.1J.</t> ( B ) Expression of OCA2 and melanocyte marker genes across seven stages of melanocyte differentiation (days 0, 2, 8, 16, 19, 25, and 30). Each dot represents a technical replicate (heterozygous insertion carriers, red; wildtype, gray). Lines indicate the mean across two replicates at each time point. Two OCA2 amplicons are shown: exon 11-13 and exon 16-18 (exon numbering from RefSeq NM_000275.3 as displayed in the UCSC Genome Browser). ( C ) Representative image illustrating pigmentation differences between wild-type (WT; homozygous reference) and heterozygous (HET; one Alu insertion allele) melanocyte cultures. ( D ) Enrichment of histone marks, H3K4me1 and H3K27ac, at days 19 and 30. “IgG” and “Control” indicate negative controls for the enrichment assay and locus-specific signal, respectively. The locus “Control” is derived from the B2M gene. Fold enrichment values were normalized to 1% of the input control. [Figure created with BioRender]](https://bio-rxiv-images-cdn.bioz.com/dois_ending_with_81/10__64898_slash_2026__03__18__712481/10__64898_slash_2026__03__18__712481___F5.large.jpg)
