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Volume 7, Issue 1, Pages (July 2010)

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1 Volume 7, Issue 1, Pages 20-24 (July 2010)
Reprogramming of Human Peripheral Blood Cells to Induced Pluripotent Stem Cells  Judith Staerk, Meelad M. Dawlaty, Qing Gao, Dorothea Maetzel, Jacob Hanna, Cesar A. Sommer, Gustavo Mostoslavsky, Rudolf Jaenisch  Cell Stem Cell  Volume 7, Issue 1, Pages (July 2010) DOI: /j.stem Copyright © 2010 Elsevier Inc. Terms and Conditions

2 Figure 1 Characterization of Peripheral Blood-Derived iPSCs
(A) Schematic drawing demonstrating the strategy to derive iPSCs from human peripheral blood. (B) Immunostaining for pluripotency markers Oct4, Nanog, and Tra1-81 in one representative T-iPSCs and M-iPSC line. (C) Southern blot analyses showing that telomeres are elongated in T-iPSCs and MiPSCs compared to mononuclear (D1MNC, D3MNC) and myeloid (D3myeloid) cells. (D) Quantitative RT-PCR assay for expression analyses of mesodermal (Brachyury), endodermal (AFP), and ectodermal (NCAM) lineage markers in differentiated embryoid bodies and iPSCs. Data are relative to GAPDH. (E) Teratoma analysis from one representative T-iPSC and M-iPSC line. (F) Methylation analyses of the Oct4 promoter region in human ESC, T-iPSC, M-iPSC, and peripheral blood cells. See also Table S1 and Figure S1. Cell Stem Cell 2010 7, 20-24DOI: ( /j.stem ) Copyright © 2010 Elsevier Inc. Terms and Conditions

3 Figure 2 Analyses of TCR Gene Rearrangements in T-iPSCs
(A) PCR analyses of TCRB Vβ-Jβ gene rearrangements in six iPSC lines derived from peripheral blood of donor 4. PCR products within the indicated valid size range were cloned and sequenced. (B) PCR analyses of TCRG Vγ-Jγ gene rearrangements in six iPSC lines derived from donor 4. PCR products within the indicated valid size range were cloned and sequenced. (C) PCR analyses showing that all iPSC clones from donor 4 tested negative for Vδ-Jδ TCRD gene rearrangements. (D) Sequencing analyses of PCR products obtained in (A) and (B). Shown are productive TCRB and productive (D4 #4) and unproductive (D4 #1) TCRG gene rearrangements in selected T-iPSC clones of donor 4. Genomic DNA from human ESC line BGO2 was used as negative control in all PCR assays; clonal positive controls were purchased from InVivoScribe Technologies. See also Table S1 and Figures S1 and S2. Cell Stem Cell 2010 7, 20-24DOI: ( /j.stem ) Copyright © 2010 Elsevier Inc. Terms and Conditions

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