Proliferation and Differentiation of Mouse Spermatogonial Stem Cells on a Three-Dimensional Surface Composed of PCL/Gel Nanofibers

被引:13
|
作者
Talebi, Ali [1 ]
Gilani, Mohanunad Ali Sadighi [2 ]
Koruji, Morteza [3 ,4 ]
Ai, Jafar [5 ]
Navidi, Shadan [1 ]
Rezaie, Mohammad Jafar [6 ]
Jabari, Ayob [1 ]
Movassagh, Sepideh Ashouri [1 ]
Khadivi, Farnaz [1 ]
Salehi, Majid [7 ]
Hoshino, Yumi [8 ]
Abbasi, Mehdi [1 ]
机构
[1] Univ Tehran Med Sci, Sch Med, Dept Anat, Tehran, Iran
[2] Univ Tehran Med Sci, Shariati Hosp, Dept Urol, Tehran, Iran
[3] Iran Univ Med Sci, Cellular & Mol Res Ctr, Tehran, Iran
[4] Iran Univ Med Sci, Dept Anat Sci, Tehran, Iran
[5] Univ Tehran Med Sci, Sch Adv Technol Med, Dept Tissue Engn, Tehran, Iran
[6] Kurdistan Univ Med Sci, Fac Med, Dept Embryol, Sanandaj, Iran
[7] Shahroud Univ Med Sci, Sch Med, Dept Tissue Engn, Shahroud, Iran
[8] Hiroshima Univ, Grad Sch Biosphere Sci, Hiroshima, Japan
来源
INTERNATIONAL JOURNAL OF MORPHOLOGY | 2019年 / 37卷 / 03期
关键词
Adult germline stem cell; Male infertility; Cell differentiation; Polycaprolactone; Nanofibers; IN-VITRO SPERMATOGENESIS; SERTOLI-CELLS; TESTICULAR TISSUE; DRUG-DELIVERY; CULTURE; CRYOPRESERVATION; BIOMATERIALS; PRESERVATION; COCULTURE; MONKEY;
D O I
10.4067/S0717-95022019000301132
中图分类号
R602 [外科病理学、解剖学]; R32 [人体形态学];
学科分类号
100101 ;
摘要
Spermatogonial stem cells (SSCs) have self-renewal and differentiation capacity essential for sperm production throughout the male reproductive life. The electrospun polycaprolactone/gelatin (PCL/Gel) nanofibrous scaffold mimics important features of the extracellular matrix (ECM), which can provide a promising technique for the proliferation and differentiation of SSCs in vitro. The goal of the present study was to investigate the effects of PCL/Gel nanofibrous scaffold on the propagation and differentiation of neonate mouse SSCs (mSSCs). mSSCs were enzymatically isolated, and the cells were purified by differential plating method and seeded on scaffold. After 2 weeks, viability, colony number and diameter, and expression of specific spermatogonial cell genes were investigated. After mSSCs propagation, the cells were cultivated in a differentiation medium on the scaffold for another 2 weeks, and differentiating cells were analyzed by real-time PCR. The number of mSSC colony (P<0.01) and expression levels of specific spermatogonial genes Plzf and Inga6 (P<0.01) and also differentiation genes c-Kit, Tp1 and Ptm1 (P<0.05) were higher in scaffold group compared with control during the culture period. We conclude that mSSCs can be expanded and can differentiate toward spermatid cells on PCL/Gel nanofibrous scaffold with improved developmental parameters.
引用
收藏
页码:1132 / 1141
页数:10
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