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Viability of primordial follicles derived from cryopreserved ovine ovarian cortex tissue.

机译:冷冻保存的绵羊卵巢皮质组织来源的原始卵泡的活力。

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OBJECTIVE: To develop an efficient technique to preserve primordial follicles from cryopreserved ovarian tissue. DESIGN: Frozen-thawed and fresh preantral follicles were mechanically isolated for viability testing, and their morphology was histologically analyzed. SETTING: Laboratory of Animal Reproduction, Faculty of Veterinary Medicine and Zootechny, University State of Sao Paulo, Brazil. ANIMAL(S): Lambs 12-24 months of age. INTERVENTION(S): Ovarian cortical fragments were prepared for cryoprotectant toxicity testing, freezing and thawing procedures, and in vitro culture. MAIN OUTCOME MEASURE(S): Histologic structure and follicular viability. RESULT(S): On day zero, no morphologic differences were observed between follicles isolated from fresh tissue and those treated with the cryopreservatives ethylene glycol (EG) and dimethyl sulfoxide (DMSO) and subjected to freezing. Even so, frozen follicles treated with DMSO + EG showed dark staining, indicating degeneration. On day zero, the follicular viability was similar between the control group (78.9%) and those treated with EG (77%) and frozen with EG (75%). After 10 days in culture, a reduced percentage of follicles was considered viable in all groups. This decrease was accentuated in those treated with DMSO (37.5% and 35.2% in those exposed to and frozen with DMSO, respectively) and DMSO + EG (33.9% and 30% in those exposed to and frozen with DMSO + EG, respectively) as compared with the control group (45%) and EG-treated groups (40.1% and 40% for those exposed to and frozen with EG, respectively). CONCLUSION(S): Ethylene glycol seems to be the best cryoprotectant for the cryopreservation of ovine ovarian tissue.
机译:目的:开发一种有效的技术来保存冷冻保存的卵巢组织中的原始卵泡。设计:将冻融和新鲜的窦前卵泡机械分离以进行活力测试,并对其组织学进行形态学分析。地点:巴西圣保罗大学动物医学与动物科技学院动物繁殖实验室。动物:12-24个月大的羔羊。干预措施:准备卵巢皮质片段进行冷冻保护剂毒性测试,冷冻和解冻步骤以及体外培养。主要观察指标:组织学结构和卵泡生存力。结果:在第0天,从新鲜组织中分离出的卵泡与用冷冻保存剂乙二醇(EG)和二甲基亚砜(DMSO)处理并冷冻的卵泡之间没有观察到形态学差异。即使这样,用DMSO + EG处理的冷冻卵泡仍显示深色,表明变性。在第0天,对照组(78.9%)与用EG处理(77%)并用EG冷冻(75%)的那些之间的卵泡生存力相似。培养10天后,所有组中的卵泡百分比均降低。 DMSO处理组(分别暴露于DMSO和冷冻的DMSO中分别为37.5%和35.2%)和DMSO + EG(暴露于DMSO + EG并冷冻的DMSO中分别为33.9%和30%)加剧了这种下降与对照组(45%)和EG治疗组相比(分别与EG接触和冷冻的组分别为40.1%和40%)。结论:乙二醇似乎是绵羊卵巢组织冷冻保存的最佳冷冻保护剂。

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