ŠIMARA, Pavel, Lenka TESAŘOVÁ, Daniela ŘEHÁKOVÁ, Pavel MATULA a Irena KRONTORÁD KOUTNÁ. Genomic Stability of the Cells during hiPSC Reprogramming and Endothelial Differentiation. In 12th International Congress of Cell Biology. 2016.
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Základní údaje
Originální název Genomic Stability of the Cells during hiPSC Reprogramming and Endothelial Differentiation
Autoři ŠIMARA, Pavel (203 Česká republika, garant, domácí), Lenka TESAŘOVÁ (203 Česká republika, domácí), Daniela ŘEHÁKOVÁ (203 Česká republika, domácí), Pavel MATULA (203 Česká republika, domácí) a Irena KRONTORÁD KOUTNÁ (203 Česká republika, domácí).
Vydání 12th International Congress of Cell Biology, 2016.
Další údaje
Originální jazyk angličtina
Typ výsledku Konferenční abstrakt
Obor 10601 Cell biology
Stát vydavatele Česká republika
Utajení není předmětem státního či obchodního tajemství
WWW 12th International Congress of Cell Biology
Kód RIV RIV/00216224:14330/16:00088049
Organizační jednotka Fakulta informatiky
Klíčová slova anglicky human induced pluripotent stem cells (hiPSCs); DNA double-strand breaks (DSBs); CGH microarrays; endothelial differentiation
Příznaky Mezinárodní význam, Recenzováno
Změnil Změnil: Mgr. Pavel Šimara, Ph.D., učo 67594. Změněno: 2. 3. 2018 09:56.
Anotace
Studies of endothelial biology at genetic and molecular level are limited by the availability of relevant endothelial cells (ECs). Human induced pluripotent stem cells (hiPSCs) offer a potentially unlimited source of ECs. hiPSC-derived ECs (hiPSC-ECs) provide a robust and reproducible patient-specific model system for (1) tissue engineering, (2) drug development, (3) toxicity screening, and (4) disease modeling. However, one of the main concerns is the maintenance of genomic integrity of the cells throughout the processes of hiPSC reprogramming and differentiation in vitro. In our study we generated hiPSCs from various cell-type sources, including human umbilical vein ECs (HUVECs) and adult vein ECs. After phenotypical and functional characterization, hiPSC lines were differentiated into the hiPSC-ECs using previously published protocol (Orlova et al., 2014). Upon magnetic beads-based purification, the hiPSC-EC population displayed endothelial surface markers and functions consistent with primary ECs. In order to provide with global overview of the genome stability and integrity level of the cells throughout the in vitro manipulation, we focused on occurrence of spontaneous double strand DNA breaks (DSBs), functionality of reparation mechanisms, appearance of sub-chromosomal aberrations and differentiation potential of hiPSC sample set. The cells in each stage of the process (source cells – hiPSCs – hiPSC-ECs) were subjected to genomic analysis. Levels of DSBs were assessed using fluorescence microscope in 3D and sub-chromosomal aberrations were analyzed with comparative genomic hybridization (CGH) microarrays. Our study aims to contribute to efforts to eliminate or minimize chromosomal aberrations before hiPSCs will fully realize their scientific and therapeutic potential.
Návaznosti
GBP302/12/G157, projekt VaVNázev: Dynamika a organizace chromosomů během buněčného cyklu a při diferenciaci v normě a patologii
Investor: Grantová agentura ČR, Dynamika a organizace chromosomů během buněčného cyklu a při diferenciaci v normě a patologii
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