Gupta P S P, Nandi S, Ravindranatha B M, Sarma P V
National Institute of Animal Nutrition and Physiology, Adugodi, Bangalore, India.
Theriogenology. 2002 Apr 15;57(7):1839-54. doi: 10.1016/s0093-691x(02)00694-5.
Growth of buffalo preantral follicles in culture was studied to investigate the effect of size of preantral follicles, individual or group culture, long-term culture of preantral follicles for (40 days), addition of human follicle stimulating hormone (FSH), insulin-transferrin-selenium (ITS), growth factors (epidermal growth factor (EGF), fibroblast growth factor (FGF), vaso active intestinal polypeptide (VIP) in culture media, and substitution of pregnant mare serum gonadotrophin (PMSG) for FSH as gonadotrophin source in culture media. Preantral follicles were isolated mechanically from ovaries of matured, nonpregnant slaughtered buffaloes and cultured in droplets of culture media under mineral oil in a 35 mm petri dish in a CO2 incubator (38-39 degrees C, 5% CO2 in air, 90-95% relative humidity) for 15 days. Preantral follicle isolation and washing medium consisted of Minimum Essential Medium (MEM) supplemented with steer serum (10%), glutamine (2 mM), sodium pyruvate (0.23 mM), hypoxanthine (2 mM) and gentamycin (50 microg/ml), respectively. In Experiment 1, we placed isolated preantral follicles individually or in groups of 2-4 preantral follicles in 30 or 50 microl droplets, respectively, using two culture media: washing media and washing media + ITS (1%) + FSH (0.05 IU/ml), respectively. In Experiment 2, we grouped isolated preantral follicles were grouped into six different size classes: < or = 36, 37-54, 55-72, 73-90, 90-108 and > or = 109 microm. We cultured groups of 2-4 preantral follicles in washing media + ITS (1A) + FSH (0.05 IU/ml) in a CO2 incubator for 15 days. In Experiment 3, we allocated groups of 2-4 preantral follicles to 10 treatments: (1) only washing media, (2) washing media + FSH (0.05 IU/ml), (3) washing media + ITS (17%), (4) washing media + ITS (1%) + FSH (50 IU/ml), (5) washing media + ITS (1%) + EGF (50 ng/ml), (6) washing media + ITS (1%) + FSH (0.05 IU/ml) + EGF (50 ng/ml), (7) washing media + ITS (1%) + FGF (50 ng/ml), (8) washing media + ITS (1%) + FSH (0.05 IU/ml) + FGF (50 ng/ml), (9) washing media + ITS (1%) + VIP (50 ng/ml), and (10) washing media + ITS (1%) + FSH (0.05 IU/ml) + VIP (50 ng/ml). In Experiment 4, based on the results of Experiment 3, we incubated preantral follicles from those treatments showing significantly (P < 0.05) higher growth up to 40 days. In Experiment 5, we allocated groups of 2-4 preantral follicles to two treatments: (1) washing media + PMSG (50 IU/ml), and (2) washing media + ITS (1%) + PMSG (50 IU/ml) and cultured in a CO2 incubator for 15 days. The results indicated that the preantral follicles cultured in groups had a higher growth rate (P < 0.05) than those cultured as individuals. ITS, FSH, PMSG and growth factors significantly (P < 0.05) promoted the growth of the preantral follicles. Following 40 days of culture, follicular architecture was preserved in nearly 17% of the follicles though there was no antrum formation. The growth rate of preantral follicles was lower in buffalo than in cattle.
为研究水牛腔前卵泡在体外培养中的生长情况,本实验探讨了腔前卵泡大小、单独培养或分组培养、腔前卵泡长期培养(40天)、在培养基中添加人促卵泡激素(FSH)、胰岛素 - 转铁蛋白 - 硒(ITS)、生长因子(表皮生长因子(EGF)、成纤维细胞生长因子(FGF)、血管活性肠肽(VIP))以及用孕马血清促性腺激素(PMSG)替代FSH作为培养基中的促性腺激素来源对其的影响。从成熟、未孕屠宰水牛的卵巢中机械分离出腔前卵泡,在35毫米培养皿的矿物油下的培养基液滴中,于二氧化碳培养箱(38 - 39摄氏度,空气中5%二氧化碳,相对湿度90 - 95%)中培养15天。腔前卵泡分离和洗涤培养基由最低基本培养基(MEM)分别添加牛血清(10%)、谷氨酰胺(2 mM)、丙酮酸钠(0.23 mM)、次黄嘌呤(2 mM)和庆大霉素(50微克/毫升)组成。在实验1中,我们将分离的腔前卵泡分别以单个或2 - 4个腔前卵泡为一组,分别置于30或50微升的液滴中,使用两种培养基:洗涤培养基和洗涤培养基 + ITS(1%) + FSH(0.05国际单位/毫升)。在实验2中,我们将分离的腔前卵泡分为六个不同大小类别:≤36、37 - 54、55 - 72、73 - 90、90 - 108和≥109微米。我们将2 - 4个腔前卵泡为一组,在洗涤培养基 + ITS(1%) + FSH(0.05国际单位/毫升)中于二氧化碳培养箱中培养15天。在实验3中,我们将2 - 4个腔前卵泡为一组分为10种处理:(1)仅洗涤培养基,(2)洗涤培养基 + FSH(0.05国际单位/毫升),(3)洗涤培养基 + ITS(1%),(4)洗涤培养基 + ITS(1%) + FSH(50国际单位/毫升),(5)洗涤培养基 + ITS(1%) + EGF(50纳克/毫升),(6)洗涤培养基 + ITS(1%) + FSH(0.05国际单位/毫升) + EGF(50纳克/毫升),(7)洗涤培养基 + ITS(1%) + FGF(50纳克/毫升),(8)洗涤培养基 + ITS(1%) + FSH(0.05国际单位/毫升) + FGF(50纳克/毫升),(9)洗涤培养基 + ITS(1%) + VIP(50纳克/毫升),以及(10)洗涤培养基 + ITS(1%) + FSH(0.05国际单位/毫升) + VIP(50纳克/毫升)。在实验4中,根据实验3的结果,我们将那些显示出显著(P < 0.05)更高生长的处理组的腔前卵泡培养至40天。在实验5中,我们将2 - 4个腔前卵泡为一组分为两种处理:(1)洗涤培养基 + PMSG(50国际单位/毫升),以及(2)洗涤培养基 + ITS(1%) + PMSG(50国际单位/毫升),并在二氧化碳培养箱中培养15天。结果表明,分组培养的腔前卵泡比单独培养的具有更高的生长率(P < 0.05)。ITS、FSH、PMSG和生长因子显著(P < 0.05)促进了腔前卵泡的生长。培养40天后,尽管没有形成卵泡腔,但近17%的卵泡保留了卵泡结构。水牛腔前卵泡的生长率低于牛。
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