Stra 8基因的激活与精原干细胞的特异性分化研究

视黄酸对维持正常的雄性睾丸结构和功能起着重要的作用。近来的研究发现,在雄性生殖腺发育过程中有一组基因,它们可以被视黄酸特异性的诱导活化,称为Stra（Stimulated by Retinoic Acid）基因。从鼠源分离得到的Stra8 基因编码一种细胞质蛋白,该基因只特异性的在成熟雄性生殖细胞中表达,其功能被认为与精子形成有关。为研究Stra8 基因的表达特性,我们从小鼠的基因组中克隆了Stra8 基因的启动子序列（1.4kb）。将Stra8 基因的1.4kb启动子序列克隆到pEGFP-1载体的EGFP基因之前,构建成由Stra8 基因1.4kb启动子序列调控表达绿色荧光蛋白的pStra8-EGFP载体。将其分别转化到不同类型的细胞中,如小鼠ES-129细胞、人胎儿胰腺干细胞、小鼠骨髓间充质干细胞和小鼠精原干细胞等,通过荧光显微镜观察发现,绿色荧光蛋白只在小鼠精原干细胞中表达,表明Stra8基因是组织特异性表达的基因。将pStra8-EGFP转化小鼠骨髓间充质干细胞,经G418筛选2周后,用视黄酸诱导,12h培养后,有一部分转化pStra8-EGFP载体的细胞表达绿色荧光蛋白。RT-PCR证明这些细胞中有精原干细胞特异表达基因Stra8 的转录,还有生殖细胞特异表达基因CyclinA8 和Oct4的转录,这些结果说明小鼠骨髓间充质细胞经视黄酸的诱导可以向生殖细胞方向分化。     

Stra 8基因的激活与精原干细胞的特异性分化研究

视黄酸对维持正常的雄性睾丸结构和功能起着重要的作用。近来的研究发现,在雄性生殖腺发育过程中有一组基因,它们可以被视黄酸特异性的诱导活化,称为Stra（Stimulated by Retinoic Acid）基因。从鼠源分离得到的Stra8 基因编码一种细胞质蛋白,该基因只特异性的在成熟雄性生殖细胞中表达,其功能被认为与精子形成有关。为研究Stra8 基因的表达特性,我们从小鼠的基因组中克隆了Stra8 基因的启动子序列（1.4kb）。将Stra8 基因的1.4kb启动子序列克隆到pEGFP-1载体的EGFP基因之前,构建成由Stra8 基因1.4kb启动子序列调控表达绿色荧光蛋白的pStra8-EGFP载体。将其分别转化到不同类型的细胞中,如小鼠ES-129细胞、人胎儿胰腺干细胞、小鼠骨髓间充质干细胞和小鼠精原干细胞等,通过荧光显微镜观察发现,绿色荧光蛋白只在小鼠精原干细胞中表达,表明Stra8基因是组织特异性表达的基因。将pStra8-EGFP转化小鼠骨髓间充质干细胞,经G418筛选2周后,用视黄酸诱导,12h培养后,有一部分转化pStra8-EGFP载体的细胞表达绿色荧光蛋白。RT-PCR证明这些细胞中有精原干细胞特异表达基因Stra8 的转录,还有生殖细胞特异表达基因CyclinA8 和Oct4的转录,这些结果说明小鼠骨髓间充质细胞经视黄酸的诱导可以向生殖细胞方向分化。     

MiR-34c在奶山羊雄性生殖干细胞增殖分化过程中的作用

microRNA (miRNA)在奶山羊雄性生殖细胞和精子发生过程有重要的调控功能。为研究miR-34c对雄性生殖干细胞增殖与分化中的作用,本文利用视黄酸效应基因8（Stra8）在雄性生殖细胞中随年龄增长,以其表达量上调的表达特征为指针,使用实时定量PCR技术筛选分析miRNAs。结果发现,miR-34c与Stra8的表达规律基本一致。在无精症奶山羊的睾丸组织中,发现miR-34c在无精症奶山羊睾丸组织中表达缺失。利用miR-34c模拟物及抑制剂转染奶山羊雄性生殖干细胞,体外转染miR-34c模拟物及其抑制剂,发现miR-34c能够下调Rarg、Stra8与c-Myc基因的表达,减缓奶山羊雄性生殖干细胞的增殖。结果提示,miR-34c可能具有调控奶山羊雄性生殖干细胞的减数分裂的作用,同时抑制其增殖。     

建立对未分化细胞特异性标记的小鼠胚胎干细胞系

构建pRex-1-EGFP表达载体,电穿孔转染小鼠ES细胞,用增强绿色荧光蛋白对起源于3．5d胚泡内细胞团的小鼠胚胎干细胞进行特异性标记,用荧光显微观察EGFP的表达以及RT-PCR方法检测Rex-1基因在未分化和分化中ES细胞中的表达情况。结果显示,EGFP基因成功转入小鼠ES细胞,并在未分化的ES细胞中高效表达;细胞开始分化后,EGFP的表达开始下降。由Rex-1基因启动子控制下的EGFP稳定表达的小鼠ES细胞系,对哺乳动物早期发育过程的研究以及对筛选能够调节上述过程的小分子化合物具有重要意义。     

山羊生殖细胞特异报告载体pVASA-EGFP的构建及表达

为监测成体干细胞向生殖细胞分化的过程,分析生殖细胞特异性DEAD-box家族ATP依赖RNA解旋酶vasa在不同日龄山羊睾丸组织中的表达情况并构建山羊生殖细胞特异性报告载体p VASA-EGFP。通过免疫荧光及RT-PCR法监测vasa的表达情况,利用分子技术构建报告载体p VASA-EGFP,脂质体法转染山羊骨髓间充质干细胞(Bone mesenchymal stem cells,BMSCs),经过视黄酸(Retinoic acid,RA)诱导后,观察绿色荧光蛋白表达情况以鉴定该报告载体的有效性。免疫荧光结果显示,Vasa在性成熟不同阶段的山羊睾丸组织中均有表达,RT-PCR结果表明vasa基因在3月龄、10月龄山羊睾丸组织中显著高于10日龄组。测序及酶切鉴定结果表明,扩增的vasa基因启动子片段成功连至N1载体,转染BMSCs后经4 d的RA诱导,发现有绿色荧光蛋白表达,表明成功构建了山羊vasa基因启动子调控的报告载体p VASA-EGFP。以上结果表明,vasa基因在不同日龄山羊睾丸组织中均有表达,所构建的山羊生殖细胞特异性报告载体p VASA-EGFP具有示踪山羊成体干细胞向生殖细胞分化过程的能力,为下一步监测山羊BMSCs向生殖细胞分化的过程提供了鉴定和筛选方法。     

Figla基因过表达促进小鼠胚胎干细胞向雌性生殖细胞分化

生殖系a因子(Figla）是最早表达的生殖细胞特异性转录因子之一,对卵泡的发育、Zp基因的表达和透明带的形成具有调节作用. Figla基因异常会引起卵巢早衰的发生. 本研究通过 PCR自小鼠基因组中扩增出Figla基因,将其克隆到真核报告载体pDsRed1 N1,构建了携带609 bp 的Figla重组载体pDsRed1 N1 Figla. 用该载体转染小鼠胚胎干细胞（mESCs）系J1、小鼠成纤维细胞系NIH 3T3、小鼠畸胎瘤细胞P19和小鼠精原细胞系GC1,在荧光显微镜下观察红色荧光蛋白(RFP)在细胞中的表达,同时检测转染细胞中Figla基因及其它生殖细胞特异性基因的表达. 结果显示,转染2 d,mESCs内Figla总表达量明显增加,且内源性表达量亦有所提高,即转入的外源性Figla基因可以促进内源性Figla的启动和表达. 免疫荧光染色显示,表达RFP 的细胞同时表达生殖特异性基因Vasa,减数分裂特异性基因Stra8、Scp3及卵母细胞标志基因Zp3. 通过QRT PCR检测发现,在转染3 d的细胞中,Vasa、Scp3和Zp1的表达较对照组均有明显上调,而Oct4和Stra8的表达量下降. 研究表明,Figla基因对生殖特异性基因的表达具有调控作用,可以激活雌性生殖基因表达,为更清楚地了解Figla基因在生殖细胞生长发育过程中的调控机制,以及发现该基因在生殖细胞中的新功能奠定了基础.     

川芎嗪体外诱导小鼠骨髓间充质干细胞分化为神经元样细胞的研究

为了探讨川芎嗪体外诱导小鼠骨髓间质干细胞（BMSCs）分化为神经元样细胞的作用,以小鼠骨髓间充质干细胞为研究对象,实验分为空白对照组、β-巯基乙醇（BME）阳性对照组和川芎嗪诱导组。采用荧光免疫化学和Western blot方法,分别检测神经干细胞巢蛋白（nestin）和经元特异性烯醇化酶（NSE）的表达;RT-PCR检测诱导不同时间对神经细胞相关基因Nestin、NSE、β-微管蛋白III（β-Tubulin III）和核受体相关因子-1（Nurr1）mRNA表达的影响。结果显示川芎嗪诱导间充质干细胞24 h后,细胞形态发生显著改变,细胞突起形成且数目不等,形成神经元样细胞。细胞死亡率低于β-巯基乙醇诱导组。免疫荧光化学法和western blot结果显示：川芎嗪诱导后的细胞nes-tin和NSE蛋白表达呈阳性,且表达丰度显著高于β-巯基乙醇诱导组。川芎嗪作用不同时间的BMSCs表达神经细胞相关基因Nestin、β-Tubulin III、NSE和Nurrl。结果表明川芎嗪能定向诱导小鼠骨髓间充质干细胞分化为神经元样细胞,是较理想的诱导剂。     

起搏基因体外调控骨髓间充质干细胞分化为类起搏细胞的研究

目的本研究旨在通过体外构建起搏基因质粒pIRES2-EGFP-HCN2,电穿孔转染骨髓间充质干细胞,检测其在体外的表达情况。方法对含mHCN2 cDNA的PTR载体进行转化和扩增,将所得mHCN2基因定向克隆到含有增强型绿色荧光蛋白的真核表达载体pIRES2-EGFP中,进行双酶切来鉴定克隆的正确性。将重组质粒及空白质粒用电穿孔法转染骨髓间充质干细胞,并在体外与心肌细胞共培养,观察搏动频率变化及mHCN2的表达,并检测其电生理和组织学特征。结果构建了重组质粒pIRES2-EGFP-HCN2。荧光显微镜下可见转染后的骨髓间充质干细胞呈绿色荧光,细胞中mHCN2的阳性表达率为98.2%。免疫荧光显示转染起搏基因的骨髓间充质干细胞mHCN2的表达,而对照组无表达。实验组共培养的心肌细胞搏动频率较对照组干细胞共培养的明显增快(140±11次/分VS 100±13次/分,P0.05),动作电位显示实验组最大舒张期电位值小于对照组(-62±2mv VS-71±2mv,P0.05)。免疫荧光显示干细胞与心肌细胞间形成间隙连接。结论成功构建了重组质粒pIRES2-EGFP-HCN2,转染后的骨髓间充质干细胞可在体外成功表达功能性mH-CN2通道,提供起搏电流,具有类起搏细胞的功能,为进一步构建生物起搏器提供依据。     

猪bmp15基因报告载体的构建及其特异性

为了研究骨形态发生蛋白15(bmp15)基因的表达和调控特性,通过克隆猪bmp15基因2.2 kb启动子片段,构建pBMP15-EGFP报告载体,实现监测干细胞向类卵母细胞分化的过程。以猪卵巢组织和中国仓鼠卵巢细胞(CHO)、成肌细胞(C2C12)、猪羊水干细胞(pAFSC)为材料,通过RT-PCR、免疫荧光、细胞转染、显微注射检测bmp15组织特异性表达,并且通过单层细胞诱导检测该基因体外示踪类卵母细胞获得过程的能力。RT-PCR结果显示bmp15在猪的卵巢组织中特异表达,在CHO中表达,而在C2C12和pAFSC中不表达。卵巢组织切片免疫荧光检测结果显示bmp15表达于卵泡发育的各个阶段。瞬时转染不同细胞发现启动子只在CHO中有活性,而在C2C12和pAFSC中均无活性。显微注射重组质粒片段结果显示增强绿色荧光蛋白(Enhanced Green Fluorecence Protein,EGFP)在卵母细胞体外成熟18 h启动表达,并能够持续至4-细胞期胚胎。单层细胞诱导结果显示诱导12 d的pAFSC出现携带EGFP的圆形细胞团。说明bmp15具有表达特异性和示踪干细胞诱导分化为类卵母细胞的潜能。     

Stella基因真核表达载体的构建及其对小鼠胚胎干细胞多能性的影响

构建Stella基因真核表达质粒,转染小鼠胚胎干细胞(Embryonic stem cells,ESC)并初步探讨Stella对减数分裂起始相关基因(Stra8)及胚胎干细胞多能性的影响。通过RT-PCR扩增目的基因,并连接至真核表达载体pEGFP-C1,利用重组质粒转染小鼠胚胎干细胞。对转染细胞进行荧光检测,确认Stella的表达,并利用免疫荧光及PCR检测转染细胞基因表达情况。酶切鉴定及测序分析表明成功构建含Stella基因的重组真核表达质粒,过表达Stella对ES细胞的增殖和形态学特征、进入减数分裂阶段的相关基因及其多能性基因的表达影响并不显著。故此得出结论:Stella在小鼠胚胎干细胞中能够正确表达,但对ES细胞的分化、Stra8基因的表达及其多能性基因的表达并无显著影响。     

Stem cell protein Piwil2 modulates expression of murine spermatogonial stem cell expressed genes

The piwi family genes are highly conserved during evolution and play essential roles in stem cell self-renewal, gametogenesis, and RNA interference in diverse organisms ranging from Arabidopsis to human. Piwil2, known also as Mili gene, is one of three mouse homologues of piwi. Piwil2 was found in germ cells of adult testis, suggesting that this gene functions in spermatogonial stem cell self-renewal. In order to find molecular mechanisms underlying stem cell activity mediated by Piwil2 gene, an in vitro gain of function cell culture model was established. Messenger RNAs isolated from cells expressing Piwil2 and mRNAs isolated from cells without Piwil2 expression were compared using a stem cell array technique. It was shown that Piwil2 modulates expression of stem cell specific genes, including platelet-derived growth factor receptor, beta polypeptide (Pdgfrb), solute carrier family 2 member 1 (Slc2a1), gap junction membrane channel protein alpha 7 (Gja7), and spermatogonial cell surface markers Thy-1 (CD90), integrin alpha 6 (Itga6), CD9, and spermatogonia specific markers heat shock protein 90 alpha (Hsp90a), and stimulated by retinoic acid gene 8 (Stra8). These molecules play essential role in stem cells proliferation (Pdgfrb), energy metabolism (Slc2a1), cell adhesion, cell-cell interaction (Itga6, Gja7, Thy-1, and CD9), and germ cell differentiation (Stra8). The expression of these markers in spermatogonial stem cells and other nongerminal stem cells suggests that these cells share elements of common molecular machinery with stem cells in other tissues which are modulated by stem cell protein Piwil2.     

Transgenic Stra8-EYFP pigs: a model for developing male germ cell technologies

The male germ line in mammals is composed of self-renewing cells, spermatogonia, the meiotic spermatocytes and spermiogenic spermatids. Identification of these cell stages in vitro has been problematic. Transgenic animals expressing a marker gene with a promoter specific to certain cell stages in the testis would be a useful approach to identifying these cells in a viable state. Towards this end, we have produced transgenic pigs expressing mitochondrial localized enhanced yellow fluorescent protein (EYFP-mito) under control of the germ cell specific Stimulated by Retinoic Acid 8 (Stra8) promoter. Stra8 has been shown to be expressed in pre-meiotic germ cells of mice. Twelve clones harboring the Stra8-EYFP-mito transgene were produced. Analysis by Western blot indicated that expression of the transgene was limited to testicular tissue in the transgenic pigs. Single cells and seminiferous tubules were cultured in vitro and subsequently examined with epifluorescent microscopy. Expression of EYFP was noted in cells cultured for up to 5 days. Both EYFP-mito and STRA8 antibodies were shown to bind and co-localize in seminiferous tubule cells in whole mounts and in histological sections. EYFP-mito in the transgenic pigs co-localized with the endogenous stem cell marker, NANOG. Expression of the Stra8-EYFP transgene in spermatogenic cells indicates that these pigs will be useful by providing labelled cells for use in such technologies such as germ cell transplantation and in vitro spermatogenic studies.     

Cre recombinase activity specific to postnatal, premeiotic male germ cells in transgenic mice

We have generated a transgenic mouse line,Tg(Stra8-cre)1Reb (Stra8-cre), which expresses improved Cre recombinase under the control of a 1.4 Kb promoter region of the germ cell-specific stimulated by retinoic acid gene 8 (Stra8). cre is expressed only in males beginning at postnatal day (P)3 in early-stage spermatogonia and is detected through preleptotene-stage spermatocytes. To further define when cre becomes active, we crossed Stra8-cre males with Tg(ACTB-Bgeo/GFP)21Lbe (Z/EG) reporter females and compared the expression of enhanced green fluorescent protein (EGFP) with the protein encoded by the zinc finger and BTB domain containing 16 (Zbtb16) gene, PLZF-a marker for undifferentiated spermatogonia. Co-expression of EGFP is observed in the majority of PLZF+ cells. We also tested recombination efficiency by mating Stra8-cre;Z/EG males and females with wild-type mice and examining EGFP expression in the offspring. Recombination is detected in >95% of Z/EG+ pups born to Stra8-cre;Z/EG fathers but in none of the offspring born to transgenic mothers, a verification that cre is not functional in females. The postnatal, premeiotic, male germ cell-specific activity of Stra8-cre makes this mouse line a unique resource to study testicular germ cell development.     

Characterization of a premeiotic germ cell-specific cytoplasmic protein encoded by Stra8, a novel retinoic acid-responsive gene

The full-length cDNA corresponding to Stra8, a novel gene inducible by retinoic acid (RA) in P19 embryonal carcinoma cells, has been isolated and shown to encode a 45-kD protein. Both Stra8 mRNA and protein were induced in cells treated by all-trans and 9-cis retinoic acids. Two- dimensional gel analysis and dephosphorylation experiments revealed that the two stereoisomers of RA differentially regulate the phosphorylation status of the Stra8 protein, which was shown to exist in differently phosphorylated forms. Subcellular fractionation and immunocytochemistry studies showed that the Stra8 protein is cytoplasmic. During mouse embryogenesis, Stra8 expression was restricted to the male developing gonads, and in adult mice, the expression of Stra8 was restricted to the premeiotic germ cells. Thus, Stra8 protein may play a role in the premeiotic phase of spermatogenesis.