Sabet A, Azarpira N, Kohan L, Ghavami S
Department of Genetics, Fars Science and Research Branch, Islamic Azad University, Marvdasht, Iran.
Department of Genetics, Marvdasht Branch, Islamic Azad University, Marvdasht, Iran.
Int J Organ Transplant Med. 2022;13(2):4-13.
Autophagy is an intracellular self-degradative homeostasis process which eliminates undesirable and harmful macromolecules and organelles. Autophagy is also involved in self-renewal and differentiation of induced pluripotent stem cell (iPSCs).
In this study, we investigated the expression profile of autophagy marker genes in human iPSCs during their differentiation induction toward insulin producing β-like cells.
Human iPSC line, R1-hiPSC1, was used for differentiation induction toward β-like cells. The mRNA expression of Nanog, OCT4 (pluripotency markers), SOX17, FOXA2 (endodermic markers), PTF1A, NKX6.1 (exocrine/endocrine determinants), and PDX1 were measured during differentiation stages. Autophagy was monitored by genes expression study of four autophagy markers, MAP1LC3B, BECN1, SQSTM1/P62 and ATG5, along with protein expression profile of LC3b-II during differentiation stages.
The mRNA expression measurement of pluripotency, endoderm and exocrine/endocrine marker genes confirmed that hiPSCs skipped pluripotency, differentiated into endoderm, passed through the pancreatic lineage commitment stage and successfully generated insulin producing β-like cells. Expression profile of autophagy genes during differentiation stages indicated the decreased expression levels at the early stages (EB and MEI) and then increased at the definitive endoderm stages (DEI 1, DEI 2 and DE) followed by a subtractive pattern toward the end of differentiation. The results of protein expression of LC3b-II were consistent with gene expression data.
This study demonstrated the high contribution of key autophagy genes/proteins during the differentiation of hiPSC toward β-like cells. The enhanced autophagy levels were a prominent feature of early stages of differentiation and DE rather than the later stages.
自噬是一种细胞内自我降解的稳态过程,可清除不需要的和有害的大分子及细胞器。自噬也参与诱导多能干细胞(iPSC)的自我更新和分化。
在本研究中,我们调查了人类iPSC在向胰岛素分泌β样细胞分化诱导过程中自噬标记基因的表达谱。
使用人类iPSC系R1-hiPSC1向β样细胞进行分化诱导。在分化阶段测量Nanog、OCT4(多能性标记物)、SOX17、FOXA2(内胚层标记物)、PTF1A、NKX6.1(外分泌/内分泌决定因子)和PDX1的mRNA表达。通过研究四个自噬标记物MAP1LC3B、BECN1、SQSTM1/P62和ATG5的基因表达以及分化阶段LC3b-II的蛋白质表达谱来监测自噬。
多能性、内胚层和外分泌/内分泌标记基因的mRNA表达测量证实,hiPSC跳过了多能性阶段,分化为内胚层,经过胰腺谱系定向阶段,并成功产生了胰岛素分泌β样细胞。分化阶段自噬基因的表达谱表明,早期阶段(EB和MEI)表达水平降低,然后在确定内胚层阶段(DEI 1、DEI 2和DE)升高,随后在分化末期呈递减模式。LC3b-II的蛋白质表达结果与基因表达数据一致。
本研究证明了关键自噬基因/蛋白质在hiPSC向β样细胞分化过程中的重要作用。自噬水平增强是分化早期和确定内胚层阶段而非后期阶段的突出特征。