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双酚A 干扰大鼠生精过程时TJ 渗透性屏障的体外研究
引用本文:冯友亮尹营营王新生王沛涛.双酚A 干扰大鼠生精过程时TJ 渗透性屏障的体外研究[J].现代生物医学进展,2012,12(8):1430-1434.
作者姓名:冯友亮尹营营王新生王沛涛
作者单位:青岛大学医学院附属医院泌尿外科 山东青岛266003
摘    要:目的:研究体外大鼠睾丸支持细胞紧密连接蛋白(SCJP)在类雌激素-双酚A(BPA)干扰下的损伤机制。方法:对Wistar大鼠睾丸支持细胞(Sertoli细胞)离体原代培养4-5d,通过双室培养模型建立体外紧密连接(TJ)渗透性屏障,并测量其跨上皮电阻值(TER)反应紧密连接结构的形成及BPA对紧密连接的损害程度。设溶剂(DMSO)做阴性对照,以终浓度为25μM、100μM的BPA作用于支持细胞24h,MTT法测不同浓度BPA作用的Sertoli细胞增殖活性。Western bloting观察occludin、ZO-1、Cx43表达的变化。结果:成功分离并培养Wistar大鼠睾丸支持细胞,并建立良好的体外TJ屏障模型。双室培养支持细胞上皮TER值在培养的d4达到顶峰,然后在d4-9维持相对较稳定的状态,d4以200μM,100μM,25μM BPA染毒,分别于染毒后24,48,72,96和120h测TER:与DMSO溶剂对照组相比,200μM,100μM的BPA组TER值明显下降(P<0.05),而25μM的BPA组在染毒后TER值无明显变化(P>0.05)。MTT结果显示:经不同浓度BPA作用24h后,Sertoli细胞的吸光度(OD值)随着染毒剂量的增加而逐渐降低。102、103μM浓度组与溶剂对照组有显著性差异(P<0.05),而10-2、10-1、100、101μM组和溶剂对照组无显著性差异(P>0.05)。Western blot结果显示:occludin、ZO-1、Cx43在各剂量组均有表达,与溶剂对照组相比,occludin、ZO-1表达均分别随作用剂量的增加而降低:25μM组、100μM组与溶剂对照组相比,差异均存在显著性(P<0.05);100μM组与25μM组相比,差异亦存在显著性(P<0.05)。Cx43的表达却随染毒剂量的增加而增加,与溶剂对照组相比,25μM组表达无明显增加(P>0.05),而100μM组则明显增加(P<0.05);与25μM组相比,100μM组表达明显增加(P<0.05)。结论:双酚A可通过损伤支持细胞连接蛋白正常表达,破坏了TJ屏障渗透性,从而影响正常的精子形成过程。

关 键 词:双酚A  精子形成  紧密连接  支持细胞连接蛋白

BPA Disturb TJ- Permiablity of Rat Sertoli Cells During Spermatogenesis in Vitro
FENG You-liang,YIN Ying-ying,WANG Xin-sheng,WANG Pei-tao.BPA Disturb TJ- Permiablity of Rat Sertoli Cells During Spermatogenesis in Vitro[J].Progress in Modern Biomedicine,2012,12(8):1430-1434.
Authors:FENG You-liang  YIN Ying-ying  WANG Xin-sheng  WANG Pei-tao
Institution:(Department of Urinary Surgery,The Affiliated Hospital of Qingdao University,Qingdao,266003,China)
Abstract:Objective: To investigate the effects of BPA exposure on the testicular expression of Sertoli cell junctional proteins(SCJP) in male rats during spermatogenesis.Methods: Primary sertoli cells were isolated and cultured from Wistar rat for 4-5 days,and the tight junction-permeability barrier was established by dual-chamber culture model.The effect of BPA on tight junctions was measured by the method of transepithelial electrical resistance(TER) assay.With a series of concentration BPA(0,25,and 100μM) co-incubating the Sertoli cells in vitro for 24h,cell proliferative activity was assessed with MTT assay,and the expression of occludin,ZO-1,Cx43 were determined by Western blotting.Results: BPA perturbs the integrity of the TJ-permeablity in Sertoli cells in vitro,which was associated with the decline of selected proteins at the tight junction,and gap junction at the blood-testis barrier.The expression of Cx43 increased while the expression of occludin and ZO-1 reduced in the Sertoli cell following BPA treatment.Conclusion: The present study showed that occludin,ZO-1 and specifically Cx43 could be early targets for BPA,which may be one of the contributing factors leading to impairment in spermatogenesis.
Keywords:Bisphenol A  Spermatogenesis  Tight junction  Sertoli cell junctional proteins
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