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不同冷冻保护剂对冻融后未成熟秦川牛犊牛睾丸组织质量的影响。

Effects of various cryoprotectants on the quality of frozen-thawed immature bovine (Qinchuan cattle) calf testicular tissue.

作者信息

Zhang X-G, Li H, Hu J-H

机构信息

College of Animal Science and Technology, Northwest A&F University, Yangling, Shaanxi, China.

出版信息

Andrologia. 2017 Nov;49(9). doi: 10.1111/and.12743. Epub 2017 Mar 15.

DOI:10.1111/and.12743
PMID:28295478
Abstract

To investigate the effects of different concentrations of various cryoprotectants (CPs) on the cell viability as well as expression of spermatogenesis-related genes, such as CREM, Stra8 and HSP70-2 in frozen-thawed bovine calf testicular tissue, immature bovine (Qinchuan cattle) calf testicular tissue was collected and cryopreserved in the cryomedia containing different concentrations (5%, 10%, 15% and 20%) of the following three CPs: glycerol, ethylene glycol (EG) and dimethyl sulphoxide (DMSO) respectively. After 1 month cryopreservation in liquid nitrogen, cell viability was evaluated using Trypan blue exclusion under a bright-field microscope. The mRNA expression of the three genes was also evaluated using qRT-PCR. The results indicated that different concentrations of glycerol, EG and DMSO in cryomedia during cryopreservation could protect bovine calf testicular tissue in various ways to avoid freezing or cryopreservation-induced expression changes in spermatogenesis-related genes. The highest cell viability and the three spermatogenesis-related genes (CREM, Stra8 and HSP70-2) expression level came from the cryomedia containing glycerol, EG and DMSO at 10% concentration respectively (p < .05). Meanwhile, compared with the other CPs, the frozen-thawed bovine calf testicular tissue treated with 10% DMSO exhibited the highest cell viability and mRNA expression level of the spermatogenesis-related genes (CREM, Stra8 and HSP70-2).

摘要

为了研究不同浓度的各种冷冻保护剂(CPs)对冻融后的犊牛睾丸组织中细胞活力以及精子发生相关基因(如CREM、Stra8和HSP70-2)表达的影响,采集了未成熟的秦川牛犊牛睾丸组织,并分别保存在含有不同浓度(5%、10%、15%和20%)的以下三种CPs的冷冻培养基中:甘油、乙二醇(EG)和二甲基亚砜(DMSO)。在液氮中冷冻保存1个月后,在明场显微镜下使用台盼蓝排斥法评估细胞活力。还使用qRT-PCR评估了这三个基因的mRNA表达。结果表明,冷冻保存期间冷冻培养基中不同浓度的甘油、EG和DMSO可以通过多种方式保护犊牛睾丸组织,以避免冷冻或冷冻保存诱导的精子发生相关基因表达变化。最高的细胞活力以及三个精子发生相关基因(CREM、Stra8和HSP70-2)的表达水平分别来自含有10%浓度甘油、EG和DMSO的冷冻培养基(p < .05)。同时,与其他CPs相比,用10%DMSO处理的冻融后犊牛睾丸组织表现出最高的细胞活力和精子发生相关基因(CREM、Stra8和HSP70-2)的mRNA表达水平。

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