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猪雄性生殖干细胞的分离培养及鉴定 总被引:1,自引:0,他引:1
本试验旨在探索猪雄性生殖干细胞(mGSCs)体外分离、培养的适宜条件,建立猪雄性生殖干细胞体外培养体系。采用两步酶消化法对新生小猪睾丸生殖干细胞进行了体外分离和初步的培养鉴定,并利用层黏连蛋白和明胶的不同贴壁特性,比较2种差易贴壁分选方法的富集效果,并对传代后的干细胞培养1周后进行碱性磷酸酶染色鉴定,通过免疫荧光技术检测培养细胞是否表达干细胞标志蛋白OCT-4。试验结果表明,层黏连蛋白更适用于猪生殖干细胞的富集、培养,细胞分选效率及增殖生长明显优于采用明胶分选的方法。培养的mGSCs拥有与小鼠mGSCs相同的形态、增殖及表达特征。鉴定结果显示,生长细胞克隆碱性磷酸酶染色呈阳性,支持细胞碱性磷酸酶染色呈阴性;培养的生殖干细胞克隆表达转录蛋白OCT-4,而饲养层支持细胞OCT-4抗体染色则呈阴性。结果表明培养的干细胞克隆仍保持较好的干细胞活性,保持正常的自我复制和分化潜能,初步建立了生殖干细胞培养体系。 相似文献
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精原干细胞(spermatogonial stem cells,SSCs)位于睾丸曲细精管基底小室内,因其具有持续的自我更新能力和分化为精子的能力,被认为是雄性哺乳动物体内唯一能将自身遗传物质传递给后代的成体干细胞。对SSCs的研究已成为干细胞学科研究的热点之一,但目前SSCs的研究多集中于啮齿类动物,而猪SSCs(porcine SSCs,pSSCs)的研究进展相对落后,主要是由于存在以下几个问题:睾丸中pSSCs本身数量极少,且缺乏特异的分子标记;pSSCs的分离纯化技术仍不成熟;pSSCs体外培养体系仍不够完善。这些问题的存在导致pSSCs分离纯化效率低,并且难以在体外长期稳定培养及传代,以至于pSSCs的相关机理研究缺乏稳定的材料,为其体外研究及应用带来了不便。基于以上现状,文章总结了pSSCs体外分离培养及移植的研究进展,详细介绍了pSSCs的分子标记、分离纯化和体外培养的相关方法,以及pSSCs移植技术的研究现状,旨在为pSSCs研究提供参考,以期加快pSSCs在猪的遗传育种与繁殖领域以及男性生殖医学领域的研究和应用。 相似文献
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《中国畜牧兽医》2020,(8)
精原干细胞(spermatogonial stem cells,SSCs)位于睾丸曲细精管基底小室内,因其具有持续的自我更新能力和分化为精子的能力,被认为是雄性哺乳动物体内唯一能将自身遗传物质传递给后代的成体干细胞。对SSCs的研究已成为干细胞学科研究的热点之一,但目前SSCs的研究多集中于啮齿类动物,而猪SSCs (porcine SSCs,pSSCs)的研究进展相对落后,主要是由于存在以下几个问题:睾丸中pSSCs本身数量极少,且缺乏特异的分子标记;pSSCs的分离纯化技术仍不成熟;pSSCs体外培养体系仍不够完善。这些问题的存在导致pSSCs分离纯化效率低,并且难以在体外长期稳定培养及传代,以至于pSSCs的相关机理研究缺乏稳定的材料,为其体外研究及应用带来了不便。基于以上现状,文章总结了pSSCs体外分离培养及移植的研究进展,详细介绍了pSSCs的分子标记、分离纯化和体外培养的相关方法,以及pSSCs移植技术的研究现状,旨在为pSSCs研究提供参考,以期加快pSSCs在猪的遗传育种与繁殖领域以及男性生殖医学领域的研究和应用。 相似文献
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采用贴壁速率差法分离纯化的新生牛雄性生殖干细胞(Male germ stem cell,mGSCs)和支持细胞(Calf sertoli cell,CSCs);CSCs饲养层细胞一般维持时间不超过8d;新生牛雄性生殖干细胞在CSCs饲养层上1代培养至5~6d可形成类ES细胞集落,采用机械离散集落传代法有利于集落形成或存在,传代培养至少在前2代细胞集落存在;部分典型细胞集落的中心细胞AKP强阳性,周边细胞AKP弱阳性或阴性;免疫组化检测显示,细胞集落SSEA1强阳性、SSEA3弱阳性和Oct-4呈现阳性染色。表明mGSCs具有ES细胞的某些细胞特性。 相似文献
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牛精原干细胞的分离和纯化及体外培养的一般特性 总被引:4,自引:0,他引:4
采用两步酶消化法制备5月龄的牛生殖细胞悬液,用Percoll不连续密度梯度法分离精原细胞,接种于含10%胎牛血清的DMEM/F12培养基中,37℃,5%CO2饱和湿度培养,观察培养细胞的生长和形态变化。结果5月龄牛的曲细精管主要包含细胞为精原细胞、Sertoli细胞,每克睾丸实质收获生精上皮细胞总数平均为3.18×106个细胞,精原细胞纯化后纯度达69.27%,精原细胞主要分布于27%~35%的Percoll梯度中。牛精原干细胞体外培养6~7 d后开始分裂,20 d后精原干细胞形成小集落。结果表明用两步酶消化、Percoll不连续密度梯度法分离的精原细胞能满足体外培养的需要,可以存活并发生增殖。 相似文献
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《中国奶牛》2015,(16)
精原干细胞(SSCs)能够自我更新,产生大量分化的生殖细胞并在出生以后形成精子,将遗传信息传递给下一代。因为所有雌性生殖干细胞在出生前已停止增殖,所以SSCs是成年哺乳动物唯一的生殖干细胞。将有生育能力的雄性供体睾丸细胞移植到不育症雄性睾丸细胞中,不育症的雄性可以重新进行精子发生和恢复生育能力。这项移植技术已经用来研究SSCs的生物学特性。研究发现,精原干细胞可以在小鼠的曲细精管进行复制,然后迁移,精原干细胞所需自我更新的生长因子保存在哺乳动物中。因此相信该培养技术很快会被应用于人类的精原干细胞中。本文讨论了现有的和潜在的运用移植技术和体外培养精原干细胞的方法。由于辅助的生殖技术能使精子细胞进入卵母细胞使之受精,所以在体外培养分化精原干细胞使之成为成熟生殖细胞的技术,将会促使人的临床精原干细胞的应用得到长足发展。 相似文献
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《畜牧与生物技术杂志(英文版)》2016,(2)
Background: Male germline stem cells(MGSCs) are a subpopulation of germ cells in the testis tissue. MGSCs are capable of differentiation into spermatozoa and thus are perfect targets for genomic manipulation to generate transgenic animals.Method: The present study was to optimize a protocol of production of transgenic mice through transduction of MGSCs in vivo using lentiviral-based vectors. The recombinant lentiviral vectors with either EF-1 or CMV promoter to drive the expression of enhanced green fluorescent protein(e GFP) transgene were injected into seminiferous tubules or inter-tubular space of 7-day-old and 28-day-old mouse testes. At 5 or 6 wk post-surgery, these pre-founders were mated with wild-type C57BL/6J female mice(1.5 to 2.0-month-old).Results: Sixty-seven percent of F1 generation and 55.56 % of F2 offspring were positive for eG FP transgene under the control of EF-1 promoter via PCR analysis. The transgenic pups were generated in an injection site-and age-independent manner. The expression of transgene was displayed in the progeny derived from lentiviral vector containing CMV promoter to drive transgene, but it was silenced or undetectable in the offspring derived from lentiviral vector with transgene under EF-1 promoter. The methylation level of g DNA in the promoter region of transgene was much higher in the samples derived lentiviral vectors with EF-1 promoter than that with CMV promoter,suggesting e GFP transgene was suppressed by DNA methylation in vivo.Conclusion: This research reported here an effective strategy for generation of transgenic mice through transduction of MGSCs in vivo using lentivirus vectors with specific promoters, and the transgenic offspring were obtained in an injection site-and age-independent manner. This protocol could be applied to other animal species, leading to advancement of animal transgenesis in agricultural and biomedical fields. 相似文献
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建立高效的原生质体再生体系是通过原生质体融合技术培育草地早熟禾(Poa pratensis)新品种的重要前提。以甘肃陇西野生草地早熟禾(LX)和定西野生草地早熟禾(DX)胚性愈伤组织为材料,探索其原生质体游离和培养条件。结果表明,LX和DX原生质体分离的最佳酶液组合为1.5%纤维素酶R-10+0.5%果胶酶Y-23+1.0%离析酶R-10+0.3%崩溃酶;酶解时间为16 h;LX原生质体最适宜的甘露醇浓度为0.6 mol·L-1,而DX原生质体的最适甘露醇浓度为0.5 mol·L-1。LX原生质体的产量最高可达6.59×106个·g-1,DX可达5.95×106个·g-1。DX原生质体培养的最适密度为3.0×105个·m L-1,最适2,4-D浓度为1.0 mg·L-1,此时,DX原生质体再生细胞的分裂频率可达9.56%,植板率为4.62%。 相似文献
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Spermatogonial stem cells transplantation provides a unique approach for studying spermatogenesis. Initially developed in mice, this technique has now been extended in farm animals and provides an alternative means to preserve valuable male germ line and to produce transgenic animals. The aim of this study was to enrich type A spermatogonial cells amongst the isolated cells from goat testis, to cryopreserve these enriched populations of cells and their subsequent transplantation in unrelated recipient goats under ultrasound guidance. The cells were isolated enzymatically and enriched by differential plating and separation on discontinuous percoll gradient. Ultrasound guided injection of trypan blue dye into rete testis resulted in 20–30% filling of the seminiferous tubules. Prior to transplantation, the cells were labelled with a fluorescent dye to trace donor cells in recipient seminiferous tubules after transplantation. The fluorescent‐labelled cells were observed up to 12 weeks after transplantation. 相似文献
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High levels of estrogen produced by boar testes and the presence of estrogen receptors in both interstitial and tubular compartments are consistent with a direct role for estrogen in regulation of testicular cell function. This study investigated the importance of estrogen on hormone production by Leydig cells and seminiferous tubules in the developing boar. Thirty-six 1-week-old littermate pairs of boars were treated weekly with vehicle or 0.1 mg/kg BW Letrozole, an aromatase inhibitor, until castration at 2, 3, 4, 5, 6, 7, or 8 months. Tissue was collected and Leydig cells and seminiferous tubules were isolated. In a separate study, five untreated boars (ages 1.5-4 months) were castrated and Letrozole was added in vitro to Leydig cell and seminiferous tubule cultures. Leydig cells were cultured for 24h with and without porcine LH. Media were assayed for estradiol (E(2)) and testosterone (T) concentrations by RIA. Seminiferous tubules were cultured for 4h with and without porcine FSH; media were assayed for E(2) and immunoreactive inhibin (INH). In vivo aromatase inhibition decreased basal E(2) and increased basal T production by cultured Leydig cells. Basal seminiferous tubule production of E(2) but not INH was reduced. Decreasing estrogen synthesis in vivo did not alter LH-induced Leydig cell E(2) production or FSH-induced seminiferous tubule INH production. INH production decreased with advancing age regardless of treatment. In conclusion, in vivo aromatase inhibition altered baseline steroid production by cultured Leydig cells and seminiferous tubules but had little effect on response to gonadotropins. 相似文献
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Isolation of porcine, canine and feline IgG by affinity chromatography using protein A 总被引:1,自引:0,他引:1
Isolation of porcine, canine and feline IgG has hitherto been achieved usually by DEAE-ion exchange chromatography and gel filtration. These procedures, however, are rather time-consuming, as they involve purification of IgG. Isolation of IgG by affinity chromatography on a column of protein A-Sepharose was attempted. IgG of all three animal species was very easily isolated with a high yield. In the absence of any other method that allows isolation of IgG of three animal species from a single column, the procedure proposed would be very useful. 相似文献
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Xinpeng Yang Yue Feng Yang Li Dake Chen Xuanyan Xia Jialian Li Fenge Li 《Reproduction in domestic animals》2021,56(3):416-426
Sertoli cells are the only somatic cells in the seminiferous epithelium which directly contact with germ cells. Sertoli cells exhibit polarized alignment at the basal membrane of seminiferous tubules to maintain the microenvironment for growth and development of germ cells, and therefore play a crucial role in spermatogenesis. Androgens exert their action through androgen receptor (AR) and AR signalling in the testis is essential for maintenance of spermatogonial numbers, blood–testis barrier integrity, completion of meiosis, adhesion of spermatids and spermiation. In the present study, we demonstrated that AR gene could promote the proliferation of immature porcine Sertoli cells (ST cells) and the cell cycle procession, and accelerate the transition from G1 phase into S phase in ST cells. Meanwhile, miR-124a could affect the proliferation and cell cycle procession of ST cells by targeting 3′-UTR of AR gene. Furthermore, AR bound to the RNF4 via AR DNA-binding domain (DBD) and we verified that RNF4 was necessary for AR to regulate the growth of ST cells. Above all, this study suggests that AR regulates ST cell growth via binding to RNF4 and miR-124a, which may help us to further understand the function of AR in spermatogenesis. 相似文献
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细胞系是动物病毒分离培养的重要载体。本研究以现代商品化仔猪肾脏为原始材料,拟培育新的细胞系用于动物病毒的分离和培养。利用胰酶消化法和差速贴壁相结合方法,分离纯化仔猪肾上皮细胞,并在体外进行传代培养和筛选。结果显示,试验成功得到一株可以连续传代的细胞株,命名为SDPK-D,且已在体外连续传代90代。SDPK-D细胞株F33和F83代倍增时间分别为40.9和32.7 h,细胞活率分别为97.55%和98.86%,8 h细胞贴壁率分别为91.67%和97.06%。在该细胞株接种猪伪狂犬病病毒(PRV)、猪流感病毒(SIV)、猪流行性腹泻病毒(PEDV)阳性病料均出现明显的细胞病变。本研究首次针对现代商品猪培育出一株可以在体外连续传代的细胞株,并对多种动物病毒敏感,为相关动物病毒的分离培养提供了新的细胞系选择。 相似文献