|本期目录/Table of Contents|

[1]汪存利,姜 宏,孙静波.曲细精管片段培养法和混合细胞共培养法对小鼠生精细胞的增殖分化效应[J].医学研究与战创伤救治(原医学研究生学报),2014,16(06):569-571,596.[doi:10.3969/j.issn.1672-271X.2014.06.003]
 WANG Cun-li,JIANG Hong,SUN Jing-bo..Proliferation and differentiation effects between seminiferous tubule segments culture and mixed cells coculture on mouse spermatogenic cells in vitro[J].JOURNAL OF MEDICALRESEARCH —COMBAT TRAUMA CARE,2014,16(06):569-571,596.[doi:10.3969/j.issn.1672-271X.2014.06.003]
点击复制

曲细精管片段培养法和混合细胞共培养法对小鼠生精细胞的增殖分化效应()
分享到62.8K

《医学研究与战创伤救治》(原医学研究生学报)[ISSN:1672-271X/CN:32-1713/R]

卷:
第16卷
期数:
2014年06期
页码:
569-571,596
栏目:
出版日期:
2014-11-20

文章信息/Info

Title:
Proliferation and differentiation effects between seminiferous tubule segments culture and mixed cells coculture on mouse spermatogenic cells in vitro
作者:
汪存利1姜 宏1孙静波2
1.230031 安徽合肥,解放军105医院生殖医学中心;2.230031 安徽合肥,合肥市第二人民医院妇产科
Author(s):
WANG Cun-li1JIANG Hong1SUN Jing-bo2.
1.Center of Reproductive Medicine,105 Hospital of PLA,Hefei,Anhui 230031,China;2.Department of Gynecology and Obstetrics,the Second People’s Hospital of Hefei,Hefei,Anhui 230031,China
关键词:
生精细胞曲细精管片段培养混合细胞共培养流式细胞术
Keywords:
spermatogenic cells seminiferous tubules fragment culture mixed cells coculture flow cytometry
分类号:
R321.1
DOI:
10.3969/j.issn.1672-271X.2014.06.003
文献标志码:
A
摘要:
目的 探讨曲细精管片段培养法和混合细胞共培养法对体外培养生精细胞的增殖、分化效应。方法 采用曲细精管片段培养法和生精细胞-支持细胞共培养法对7~8 d 小鼠 生精细胞进行体外培养,通过细胞形态学观察、细胞存活率和精母细胞特异性基因P19、单倍体精子细胞特异性基因TP1检测及染色体倍性分析,比较两种培养法生精细胞的存活、 增殖以及分化情况。结果 两种培养方法均可见生精细胞增殖,P19/TP1比值呈降低趋势,并可获得少量带鞭毛的精子细胞和长形精子,但共培养法生精细胞增殖速度及存活时间均 优于片段法。体外培养各阶段,共培养法所获细胞数和存活率及单倍体精子细胞形成率均显著高于片段培养法(P<0.05);P19/TP1比值显著低于组织片段培养法(P<0.05)。结论 生 精细胞-支持细胞共培养法的细胞增殖速度、存活率、存活时间及单倍体精子细胞形成率均优于曲细精管片段培养法,是较为理想的小鼠生精细胞体外培养方法。
Abstract:
Objective To investigate the proliferation and differentiation effects for mouse spermatogenic cells between seminiferous tubule segments culture and mixed cells coculture in vitro.Methods Spermatogenic cells of 7-8 days mouse were separated and cultured by the methods of seminiferous tubule segments culture and mixed cells coculture,the survival rates,proliferation and differentiation rates in two culture methods were evaluated by morphological observation,viability testing,pachytene-specific phosphoprotein gene (P19) and haploid sperm cell-specific transition protein gene (TP1) detecting and ploidy analysis of cells.Results In both culture methods,the rate of P19/TP1 were on a declining curve,round spermatid and a small number of sperm cells with flagella or elongating spermatid could be observed.But the proliferation rate and survival time of mixed cells coculture was superior to seminiferous tubule fragments.Compared mixed cells coculture with seminiferous tubule fragments,cell numbers,survival rate,rate of haploid sperm cells was significantly higher (P<0.05),the rate of P19/TP1 was significantly lower (P<0.05).Conclusion Mixed cells coculture is better method than seminiferous tubules fragment culture with superior proliferation rate,survival time,and the rate of haploid sperm cells.

参考文献/References:

[1]Hamra FK,Chapman KM,Wu Z,et al.Isolating highly pure rat spermatogonial stem cells in culture[J].Methods Mol Biol,2008,450:163-179.
[2]朱培元,黄宇烽.精子细胞显微受精技术的研究进展[J].中华男科学,2003,9(7):532-535.
[3]He X,Cao Y,Zhang Z,et al.Spermatogenesis affects the outcome of ICSI for azoospermic patients rather than sperm retrieval method[J].Syst Biol Reprod Med,2010,56(6):457-464.
[4]Griswold MD.The central role of sertoli cells in spermatogenesis[J].Semin Cell Dev Biol,1998,9(4):411-416.
[5]Oatley JM,Brinster RL.Regulation of spermatogonial stem cell self-renewal in mammals[J].Annu Rev Cell Dev Biol,2008,24:263-286.
[6]Reuter K,Schlatt S,Ehmcke J,et al.Fact or fiction in vitro spermatogenesis[J].Spermatogenesis,2012,2(4):245-252.
[7]Mruk DD,Cheng CY.In search of suitable in vitro models to study germ cell movement across the blood-testis barrier[J].Spermatogenesis,2012,2(1):11-15.
[8]Gourdon JC,Travis AJ.Spermatogenesis in ferret testis xenografts:a new model[J].Comp Med,2011,61(2):145-149.
[9]Lim JJ,Seol DW,Choi KH,et al.Spermatogonial stem cell enrichment using simple grafting of testis and in vitro cultivation[J].Sci Rep,2014,1(4):5923-5932.
[10]Tesarik J.Overcoming maturation arrest by in vitro spermatogenesis:search for the optimal culture system[J].Fertil Steril,2004,81(5):1417-1419.
[11]于 洁, 叶 静,张芳婷,等.睾丸组织异体异位移植生成成熟精子的动物模型建立[J].北京大学学报:医学版,2004,36(6):591-594.
[12]Liu SX,Tang ZW,Xiong T,et al.Isolation and characterization of human spermatogonial stem cells[J].Reprod Biol Endocrinol,2011,9(1):141-149.
[13]Kala S,Kaushik K,Singh KP,et al.In vitro culture and morphologyical characterizeation of prepubertal buffalo (Bubalus bubalis) putative spermatogonial stem cell[J].J Assist Reprod Genet,2012,29(12):1335-1342.
[14]Xie B,Qin Z,Huang B,et al.In vitro culture and differentiation of buffalo (Bubalus bubalis) spermatogonia[J].Reprod Domest Anim,2010,45(2):275-282.

相似文献/References:

备注/Memo

备注/Memo:
安徽省自然科学基金项目(090413271X)
更新日期/Last Update: 2014-11-20