A synthetic mRNA cell reprogramming method using CYCLIN D1 promotes DNA repair generating improved genetically stable human induced pluripotent stem cells
| Autor: | Michael J. Edel, Carme Grau-Bove, Francisco Vidal Pérez, Manel Juan Otero, Raul Delgado-Morales, Maria A. Blasco, Carlos Hobeich Naya, Agueda M. Tejera, Alejandro Vaquero, C. Barrot, Irene Santos-Barriopedro, Iris Garcia-Martínez, Ana Belén Alvarez-Palomo, Manel Esteller, Jovita Mezquita-Pla, Sebastian Moran, Victoria Moreno-Manzano, Jordi Requena-Osete |
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| Rok vydání: | 2021 |
| Předmět: |
0301 basic medicine
DNA Repair DNA repair induced pluripotent stem cells neural stem cells (NSCs) Induced Pluripotent Stem Cells Biology clinical translation Cell therapy 03 medical and health sciences Mice 0302 clinical medicine Cyclin D1 SOX2 Animals Humans RNA Messenger Induced pluripotent stem cell Cell Differentiation Cell Biology cellular therapy Cell cycle Cellular Reprogramming Cell biology 030104 developmental biology KLF4 Molecular Medicine cell cycle Reprogramming 030217 neurology & neurosurgery Developmental Biology |
| Zdroj: | STEM CELLS r-CIPF. Repositorio Institucional Producción Científica del Centro de Investigación Principe Felipe (CIPF) instname r-CIPF: Repositorio Institucional Producción Científica del Centro de Investigación Principe Felipe (CIPF) Centro de Investigación Principe Felipe (CIPF) |
| ISSN: | 1066-5099 |
| Popis: | A key challenge for clinical application of induced pluripotent stem cells (iPSC) to accurately model and treat human pathologies depends on developing a method to generate genetically stable cells to reduce long-term risks of cell transplant therapy. Here, we hypothesized that CYCLIN D1 repairs DNA by highly efficient homologous recombination (HR) during reprogramming to iPSC that reduces genetic instability and threat of neoplastic growth. We adopted a synthetic mRNA transfection method using clinically compatible conditions with CYCLIN D1 plus base factors (OCT3/4, SOX2, KLF4, LIN28) and compared with methods that use C-MYC. We demonstrate that CYCLIN D1 made iPSC have (a) lower multitelomeric signal, (b) reduced double-strand DNA breaks, (c) correct nuclear localization of RAD51 protein expression, and (d) reduced SNP changes per chromosome, compared with the classical reprogramming method using C-MYC. CYCLIN D1 iPSC have reduced teratoma Ki67 cell growth kinetics and derived neural stem cells successfully engraft in a hostile spinal cord injury (SCI) microenvironment with efficient survival, differentiation. We demonstrate that CYCLIN D1 promotes double-stranded DNA damage repair predominantly through HR during cell reprogramming to efficiently produce iPSC. CYCLIN D1 reduces general cell stress associated with significantly lower SIRT1 gene expression and can rescue Sirt1 null mouse cell reprogramming. In conclusion, we show synthetic mRNA transfection of CYCLIN D1 repairs DNA during reprogramming resulting in significantly improved genetically stable footprint in human iPSC, enabling a new cell reprogramming method for more accurate and reliable generation of human iPSC for disease modeling and future clinical applications. © AlphaMed Press 2021 A key challenge for clinical application of induced pluripotent stem cells (iPSC) to accurately model and treat human pathologies lies in developing a method for their generation that are genetically stable to reduce long-term risks of cell transplant therapy. The authors show synthetic mRNA transfection of CYCLIN D1 repairs DNA during reprogramming resulting in significantly improved genetically stable footprint in human iPSC, enabling more accurate and reliable generation of human iPSC for disease modeling and future clinical applications. |
| Databáze: | OpenAIRE |
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