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首页> 外文期刊>Reports of Biochemistry and Molecular Biology >The Effect of Caffeic Acid on Spermatogonial Stem Cell-type A Cryopreservation
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The Effect of Caffeic Acid on Spermatogonial Stem Cell-type A Cryopreservation

机译:咖啡酸对精原干细胞A型冷冻保存的影响

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Background: Cancer treatment methods can lead to male infertility .in this regard, cryopreservation of spermatogonial stem cells (SSC) and cell-to-person transplantation after the course of treatment to resolve the problem of infertility is a good one. The cryopreservation of SSC is an important process as it can help on the return of spermatogenesis. However, during this process, the stem cells often become damaged which degrades their value for experiments and treatments. Caffeic acid (CA) is an antioxidant that has been shown to increase the viability of cells under stress. The aim of this study was to investigate the effect of CA has on spermatogonial stem cell (SSC) cryopreservation. Methods: Spermatogonial stem cells isolated from the testes of Balb/c mice pups were cultured in laminin-coated dishes, purified using CD90.1 microbeads, then cryopreserved in vitrification media supplemented with 10 μM CA either through a slow or rapid freezing process. After thawing, cell viability was evaluated. Expression of Bax, Fas, Bcl-2 and P53 genes was determined by real-time PCR. Gel electrophoresis was used to confirm the results of the real-time PCR. Results: The viability of the SSCs that were rapidly frozen and treated with CA was observed to be significantly reduced compared to the control group (p 0.003). The viability SSCs that received CA and underwent the slow freezing treatment was significantly reduced compared to controls (p 0.002). The expression levels of BAX, BCL-2, and Fas in the rapid freeze-thaw group didn’t significantly change. However, the levels of P53 expression were shown to increase. In the group of SSCs that underwent the slow freezing process, the BAX gene expression levels increased, while the levels of BCL-2 gene expression decreased. No significant changes in the level of Fas and P53 expression were detected. When comparing the groups that received CA treatment, SSCs that were rapidly frozen showed an up-regulation of Fas and P53 expression and a down-regulation of Bcl-2 and Bax expression. Conclusions: Caffeic acid may protect intact SCCs during the cryopreservation process through stimulating the induction of apoptosis in injured SSCs. Supplementing the vitrification media with CA has a superior effect on the preservation of SSCs.
机译:背景:癌症的治疗方法会导致男性不育,在这方面,冷冻保存精原干细胞(SSC)和经过治疗过程的细胞移植解决不育问题是一个很好的方法。 SSC的冷冻保存是一个重要的过程,因为它可以帮助恢复精子的生成。但是,在此过程中,干细胞通常会受损,从而降低其在实验和治疗中的价值。咖啡酸(CA)是一种抗氧化剂,已被证明可以增加细胞在压力下的活力。这项研究的目的是调查CA对精原干细胞(SSC)冷冻保存的影响。方法:将从Balb / c小鼠幼崽的睾丸中分离的精原干细胞在层粘连蛋白包被的培养皿中培养,用CD90.1微珠纯化,然后通过缓慢或快速冷冻过程在补充有10μMCA的玻璃化培养基中冷冻保存。解冻后,评估细胞活力。通过实时PCR确定Bax,Fas,Bcl-2和P53基因的表达。凝胶电泳用于确认实时PCR的结果。结果:与对照组相比,快速冷冻并用CA处理的SSC的生存能力显着降低(p <0.003)。与对照组相比,接受了CA并进行了慢速冷冻处理的SSC的存活力显着降低(p <0.002)。快速冻融组中BAX,BCL-2和Fas的表达水平没有明显变化。然而,显示P53表达水平增加。在经历缓慢冷冻过程的SSC组中,BAX基因表达水平升高,而BCL-2基因表达水平降低。没有检测到Fas和P53表达水平的显着变化。当比较接受CA治疗的组时,快速冷冻的SSC显示Fas和P53表达上调,而Bcl-2和Bax表达下调。结论:咖啡酸可能通过刺激受损SSCs的凋亡诱导作用而在冷冻保存过程中保护完整的SCCs。用CA补充玻璃化介质对SSC的保存具有优异的效果。

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