Additional file 1: Figure S1. of Rapid, efficient, and simple motor neuron differentiation from human pluripotent stem cells ShimojoDaisuke OnoderaKazunari Doi-ToriiYukiko IshiharaYasuharu HattoriChinatsu MiwaYukino TanakaSatoshi OkadaRina OhyamaManabu ShojiMasanobu NakanishiAtsushi DoyuManabu OkanoHideyuki OkadaYohei 2015 Evaluation of hiPSCs, TIGE-9 and YFE-16 cells. a The genomic integration of episomal vectors was detected through quantitative genomic PCR with primers specific for EBNA-1. EBNA-1 copy numbers are normalized to the β-ACTIN copy number. The EBNA-1 copy numbers were presented as the relative copy numbers to those in fibroblasts transfected with three plasmid vectors for reprogramming and cultured for 6 days (fibroblast-TF day6) (see Materials and methods). b Transgene expression in established hiPSC clones was examined via quantitative RT-PCR and is presented as the copy number normalized to that of β-ACTIN. The expressions of indicated genes are presented as the relative expressions to those in fibroblast-TF day6. c The expression levels of the pluripotency markers OCT4 and NANOG in established hiPSC clones were determined through quantitative RT-PCR analysis. d Immunocytochemical analysis of TIGE-9 and YFE-16 hiPSCs for OCT4, NANOG, Tra-1–60, and SSEA-4. Scale bar, 300 μm. e Hematoxylin and eosin staining of teratomas derived from TIGE-9 and YFE-16 hiPSCs. Scale bar, 200 μm. f Karyotype analysis of TIGE-9 and YFE-16 hiPSCs via G-banding analysis. (PNG 5285 kb)