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METHYLATION SIGNATURE FOR REPLICATIVE SENESCENCE OF CELLS IN CULTURE

机译:甲基化信号用于培养细胞的替代性敏感性

摘要

The invention concerns methods and kits for determining the replicative senescence status of a cell, for identifying a cell culture which is suitable for therapeutic use, and for quantifying the reprogramming efficiency of induced pluripotent stem cells, wherein the methylation status of at least one of the CpG-dinucleotides within a region of about 50,000 bp upstream and/or downstream of at least one of the CpG-dinucleotides selected from the group consisting of GRM7-CpG-site #1, CASR-CpG-site #1, PRAMEF2-CpG-site #1, SELP-CpG- site #1, CASP14-CpG-site #1 and KRTAP13-3-CpG-site #1 for multiple corresponding DNA molecules is determined and compared to a reference methylation status.
机译:本发明涉及用于确定细胞的复制性衰老状态,用于鉴定适合治疗用途的细胞培养物以及用于量化诱导的多能干细胞的重编程效率的方法和试剂盒,其中至少一种在选自GRM7-CpG-位点#1,CASR-CpG-位点#1,PRAMEF2-CpG-的至少一个CpG-二核苷酸的上游和/或下游约50,000 bp的区域内的CpG-二核苷酸。确定多个相应DNA分子的位点#1,SELP-CpG位点#1,CASP14-CpG位点#1和KRTAP13-3-CpG位点#1,并将其与参考甲基化状态进行比较。

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