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猪诱导多能干细胞(iPSCs)源自支持细胞和成纤维细胞的比较分析。

Comparative analysis of porcine iPSCs derived from Sertoli cells and fibroblasts.

机构信息

College of Veterinary Medicine, Shaanxi Centre of Stem Cells Engineering & Technology, Northwest A&F University, Yangling, China.

College of Veterinary Medicine, Yangzhou University, Yangzhou, China.

出版信息

J Cell Physiol. 2022 Dec;237(12):4531-4543. doi: 10.1002/jcp.30903. Epub 2022 Oct 26.

DOI:10.1002/jcp.30903
PMID:36288570
Abstract

Porcine embryonic fibroblasts (PEFs) can be directly reprogrammed into porcine induced pluripotent stem cells (piPSCs). However, the reprogramming process is generally lengthy and inefficient. Here, we established a fast and efficient induction system of piPSCs from porcine Sertoli cells (SCs) via forced expression of pig Yamanaka factors. The alkaline phosphatase (AP)-positive colonies from SCs developed on Day 3 after lentivirus infection, and were expanded and then picked up on Day 7, whereas reprogramming process from PEFs did not show any colonies in the same period. The picked piPSCs strongly expressed pluripotent genes, had the differentiation capacity to three germ layers, and could be also induced into primordial germ cell-like cells. Screening for transcription factor combinations showed that POU class 5 homeobox 1 (OCT4) is the core factor for AP-positive colony formation, and two factors (OCT4 and c-MYC) could successfully reprogram SCs into piPSCs. We then compared the RNA-sequencing data of piPSCs derived from SCs and PEFs, and found that the most significant difference was the activation of Transforming Growth Factor β signaling pathway. We also compared the RNA levels of SCs and PEFs, and found that SCs exhibited higher Wnt signaling activity and Bone Morphogenetic Protein 4 expression than PEFs, which might be correlated with higher cell proliferation rate and reprogramming efficiency. In summary, the data demonstrated that starting cell sources of piPSCs significantly affect reprogramming dynamics and SCs could serve as cell sources for efficient reprogramming.

摘要

猪胚胎成纤维细胞(PEFs)可以直接被重编程为猪诱导多能干细胞(piPSCs)。然而,重编程过程通常耗时较长且效率低下。在这里,我们通过强制表达猪 Yamanaka 因子,建立了一种从猪睾丸支持细胞(SCs)快速有效地诱导 piPSCs 的系统。感染慢病毒后第 3 天,SCs 上出现碱性磷酸酶(AP)阳性集落,并在第 7 天被扩增和挑取,而在同一时期,来自 PEFs 的重编程过程没有出现任何集落。挑取的 piPSCs 强烈表达多能基因,具有向三个胚层分化的能力,并且可以被诱导为原始生殖细胞样细胞。筛选转录因子组合表明,POU 类 5 同源框 1(OCT4)是 AP 阳性集落形成的核心因子,两个因子(OCT4 和 c-MYC)可以成功地将 SCs 重编程为 piPSCs。然后,我们比较了来源于 SCs 和 PEFs 的 piPSCs 的 RNA 测序数据,发现最显著的差异是转化生长因子 β 信号通路的激活。我们还比较了 SCs 和 PEFs 的 RNA 水平,发现 SCs 比 PEFs 表现出更高的 Wnt 信号活性和骨形态发生蛋白 4 的表达,这可能与更高的细胞增殖率和重编程效率有关。综上所述,这些数据表明 piPSCs 的起始细胞来源显著影响重编程动力学,SCs 可以作为高效重编程的细胞来源。

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