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体外成熟前将马卵母细胞置于无减数分裂抑制剂培养基中以及保存温度对减数分裂抑制和线粒体能量/氧化还原电位的影响。

Effect of holding equine oocytes in meiosis inhibitor-free medium before in vitro maturation and of holding temperature on meiotic suppression and mitochondrial energy/redox potential.

作者信息

Martino Nicola A, Dell'Aquila Maria E, Filioli Uranio Manuel, Rutigliano Lucia, Nicassio Michele, Lacalandra Giovanni M, Hinrichs Katrin

机构信息

Veterinary Clinics and Animal Productions Unit-Dipartimento dell'Emergenza e Trapianti D'Organo (DETO), Università di Bari Aldo Moro, Str, Prov, Casamassima Km 3°, Valenzano 70010, Bari, Italy.

出版信息

Reprod Biol Endocrinol. 2014 Oct 11;12:99. doi: 10.1186/1477-7827-12-99.

Abstract

BACKGROUND

Evaluation of mitochondrial function offers an alternative to evaluate embryo development for assessment of oocyte viability, but little information is available on the relationship between mitochondrial and chromatin status in equine oocytes. We evaluated these parameters in immature equine oocytes either fixed immediately (IMM) or held overnight in an Earle's/Hank's' M199-based medium in the absence of meiotic inhibitors (EH treatment), and in mature oocytes. We hypothesized that EH holding may affect mitochondrial function and that holding temperature may affect the efficiency of meiotic suppression.

METHODS

Experiment 1 - Equine oocytes processed immediately or held in EH at uncontrolled temperature (22 to 27°C) were evaluated for initial chromatin configuration, in vitro maturation (IVM) rates and mitochondrial energy/redox potential. Experiment 2 - We then investigated the effect of holding temperature (25°C, 30°C, 38°C) on initial chromatin status of held oocytes, and subsequently repeated mitochondrial energy/redox assessment of oocytes held at 25°C vs. immediately-evaluated controls.

RESULTS

EH holding at uncontrolled temperature was associated with advancement of germinal vesicle (GV) chromatin condensation and with meiotic resumption, as well as a lower maturation rate after IVM. Holding did not have a significant effect on mitochondrial distribution within chromatin configurations. Independent of treatment, oocytes having condensed chromatin had a significantly higher proportion of perinuclear/pericortical mitochondrial distribution than did other GV configurations. Holding did not detrimentally affect oocyte energy/redox parameters in viable GV-stage oocytes. There were no significant differences in chromatin configuration between oocytes held at 25°C and controls, whereas holding at higher temperature was associated with meiosis resumption and loss of oocytes having the condensed chromatin GV configuration. Holding at 25°C was not associated with progression of mitochondrial distribution pattern and there were no significant differences in oocyte energy/redox parameters between these oocytes and controls.

CONCLUSIONS

Mitochondrial distribution in equine GV-stage oocytes is correlated with chromatin configuration within the GV. Progression of chromatin configuration and mitochondrial status during holding are dependent on temperature. EH holding at 25°C maintains meiotic arrest, viability and mitochondrial potential of equine oocytes. This is the first report on the effects of EH treatment on oocyte mitochondrial energy/redox potential.

摘要

背景

评估线粒体功能为评估卵母细胞活力以评价胚胎发育提供了一种替代方法,但关于马属动物卵母细胞中线粒体与染色质状态之间的关系,目前所知甚少。我们评估了未成熟马属动物卵母细胞(立即固定(IMM)或在不含减数分裂抑制剂的基于Earle's/Hank's的M199培养基中过夜保存(EH处理))以及成熟卵母细胞中的这些参数。我们假设EH保存可能会影响线粒体功能,并且保存温度可能会影响减数分裂抑制的效率。

方法

实验1 - 评估立即处理或在不受控制的温度(22至27°C)下在EH中保存的马属动物卵母细胞的初始染色质构型、体外成熟(IVM)率和线粒体能量/氧化还原电位。实验2 - 然后我们研究了保存温度(25°C、30°C、38°C)对保存卵母细胞初始染色质状态的影响,随后重复对在25°C保存的卵母细胞与立即评估的对照进行线粒体能量/氧化还原评估。

结果

在不受控制的温度下进行EH保存与生发泡(GV)染色质浓缩的进展和减数分裂恢复相关,并且IVM后的成熟率较低。保存对染色质构型内的线粒体分布没有显著影响。与处理无关,具有浓缩染色质的卵母细胞中核周/皮质周线粒体分布的比例明显高于其他GV构型。保存对存活的GV期卵母细胞的能量/氧化还原参数没有不利影响。在25°C保存的卵母细胞与对照之间的染色质构型没有显著差异,而在较高温度下保存与减数分裂恢复和具有浓缩染色质GV构型的卵母细胞损失相关。在25°C保存与线粒体分布模式的进展无关,并且这些卵母细胞与对照之间的卵母细胞能量/氧化还原参数没有显著差异。

结论

马属动物GV期卵母细胞中的线粒体分布与GV内的染色质构型相关。保存过程中染色质构型和线粒体状态的进展取决于温度。在25°C进行EH保存可维持马属动物卵母细胞的减数分裂停滞、活力和线粒体电位。这是关于EH处理对卵母细胞线粒体能量/氧化还原电位影响的首次报道。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/318b/4209075/df0704543f06/12958_2014_1269_Fig1_HTML.jpg

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