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羰基氰化物4-(三氟甲氧基)苯腙(FCCP)预暴露可确保家猫模型中卵巢组织体外培养期间的卵泡完整性,但在冷冻保存期间则不能。

Carbonyl cyanide 4-(trifluoromethoxy)phenylhydrazone (FCCP) pre-exposure ensures follicle integrity during in vitro culture of ovarian tissue but not during cryopreservation in the domestic cat model.

作者信息

Tanpradit Nae, Chatdarong Kaywalee, Comizzoli Pierre

机构信息

Department of Obstetrics, Gynaecology and Reproduction, Faculty of Veterinary Science, Chulalongkorn University, Bangkok, 10330, Thailand.

Smithsonian Conservation Biology Institute, National Zoological Park, Washington, DC, 20008, USA.

出版信息

J Assist Reprod Genet. 2016 Dec;33(12):1621-1631. doi: 10.1007/s10815-016-0810-5. Epub 2016 Sep 17.

Abstract

PURPOSE

Temporary and reversible downregulation of metabolism may improve the survival of tissues exposed to non-physiological conditions during transport, in vitro culture, and cryopreservation. The objectives of the study were to (1) optimize the concentration and duration of carbonyl cyanide 4-(trifluoromethoxy)phenylhydrazone (FCCP-a mitochondrial uncoupling agent) exposures for biopsies of domestic cat ovarian tissue and (2) examine the effects of FCCP pre-exposures on follicle integrity after tissue culture and/or cryopreservation.

METHODS

Biopsies of cat ovarian tissue were first treated with various concentrations of FCCP (0, 10, 40, or 200 nM) for 10 or 120 min to determine the most suitable pre-exposure conditions. Based on these results, tissues were pre-exposed to 200 nM FCCP for 120 min for the subsequent studies on culture and cryopreservation. In all experiments and for each treatment group, tissue activity and integrity were measured by mitochondrial membrane potential (relative optical density of rhodamine 123 fluorescence), follicular viability (calcein assay), follicular morphology (histology), granulosa cell proliferation (Ki-67 immunostaining), and follicular density.

RESULTS

Ovarian tissues incubated with 200 nM FCCP for 120 min led to the lowest mitochondrial activity (1.17 ± 0.09; P < 0.05) compared to control group (0 nM; 1.30 ± 0.12) while maintaining a constant percentage of viable follicles (75.3 ± 7.8 %) similar to the control group (71.8 ± 11.7 %; P > 0.05). After 2 days of in vitro culture, percentage of viable follicles (78.8 ± 8.9 %) in similar pre-exposure conditions was higher (P < 0.05) than in the absence of FCCP (61.2 ± 12.0 %) with percentages of morphologically normal follicles (57.6 ± 17.3 %) not different from the fresh tissue (70.2 ± 7.1 %; P > 0.05). Interestingly, percentages of cellular proliferation and follicular density were unaltered by the FCCP exposures. Based on the indicators mentioned above, the FCCP-treated tissue fragments did not have a better follicle integrity after freezing and thawing.

CONCLUSIONS

Pre-exposure to 200 nM FCCP during 120 min protects and enhances the follicle integrity in cat ovarian tissue during short-term in vitro culture. However, FCCP does not appear to exert a beneficial or detrimental effect during ovarian tissue cryopreservation.

摘要

目的

代谢的暂时且可逆下调可能会提高在运输、体外培养和冷冻保存等非生理条件下的组织存活率。本研究的目的是:(1)优化羰基氰4-(三氟甲氧基)苯腙(FCCP,一种线粒体解偶联剂)对家猫卵巢组织活检样本的暴露浓度和持续时间;(2)研究FCCP预先暴露对组织培养和/或冷冻保存后卵泡完整性的影响。

方法

首先用不同浓度的FCCP(0、10、40或200 nM)处理猫卵巢组织活检样本10或120分钟,以确定最合适的预先暴露条件。基于这些结果,在后续的培养和冷冻保存研究中,将组织预先暴露于200 nM FCCP 120分钟。在所有实验和每个处理组中,通过线粒体膜电位(罗丹明123荧光的相对光密度)、卵泡活力(钙黄绿素测定)、卵泡形态(组织学)、颗粒细胞增殖(Ki-67免疫染色)和卵泡密度来测量组织活性和完整性。

结果

与对照组(0 nM;1.30±0.12)相比,用200 nM FCCP孵育120分钟的卵巢组织线粒体活性最低(1.17±0.09;P<0.05),同时保持与对照组相似的存活卵泡恒定百分比(75.3±7.8%)(对照组为71.8±11.7%;P>0.05)。在体外培养2天后,类似预先暴露条件下的存活卵泡百分比(78.8±8.9%)高于未使用FCCP的情况(61.2±12.0%)(P<0.05),形态正常卵泡的百分比(57.6±17.3%)与新鲜组织(70.2±7.1%)无差异(P>0.05)。有趣的是,FCCP暴露对细胞增殖和卵泡密度百分比没有影响。基于上述指标,FCCP处理的组织碎片在冻融后卵泡完整性并未更好。

结论

在120分钟内预先暴露于200 nM FCCP可在短期体外培养期间保护并增强猫卵巢组织中的卵泡完整性。然而,FCCP在卵巢组织冷冻保存期间似乎未产生有益或有害影响。

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