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玻璃化冷冻后通过共聚焦激光扫描显微镜对人囊胚细胞骨架进行分析。

Cytoskeletal analysis of human blastocysts by confocal laser scanning microscopy following vitrification.

机构信息

Section of Reproductive Medicine, First Department of Obstetrics & Gynaecology, Aristotle University Medical School, Papageorgiou General Hospital, Thessaloniki 56403, Greece.

出版信息

Hum Reprod. 2012 Jan;27(1):106-13. doi: 10.1093/humrep/der344. Epub 2011 Oct 25.

Abstract

BACKGROUND

Vitrification of human blastocysts is being used increasingly to cryopreserve supernumerary embryos following IVF. In this study, we investigate the effects of aseptic vitrification on the cytoskeleton and development of human blastocysts, by analysing survival rates and spindle and chromosome configurations by fluorescence and confocal laser scanning microscopy.

METHODS

A total of 55 fresh blastocysts and 55 day 5 dimethylsulphoxide/ethylene glycol vitrified blastocysts, which were allowed to remain in culture for 24 h post-warming, were rapidly fixed in ice cold methanol, and immunostained with an a-tubulin antibody to visualize microtubules in combination with antibodies against acetylated tubulin (to visualize spindles, poles and mid bodies), gamma tubulin (to identify spindle poles) and 4(6-diamidino-2-phenylindole) to visualize DNA.

RESULTS

In total, 213 spindles were analysed in the control (fresh) group of which 183/213 (85.9%) were normal, 20/213 (9.4%) were abnormally shaped, 9/213 (4.2%) were multipolar and 1/213 (0.5%) was monopolar. A total of 175 spindles were analysed in the vitrified group, of which 120/175 (68.6%) were normal, 39/175 (22.3%) were abnormally shaped, 10/175 (5.7%) were multipolar and 6/175 (3.4%) were monopolar. The incidence of multipolar spindles was similar in the two groups, but the level of abnormally shaped spindles, often associated with chromosome lagging, or congression failure, was significantly higher in the vitrified group compared with the fresh group (P< 0.05).

CONCLUSIONS

The high survival rate following thawing and the large proportion of normal spindle/chromosome configurations suggests that vitrification at the blastocyst stage on Day 5 does not adversely affect the development of human embryos and the ability of spindles to form and continue normal cell divisions. However, there was a significantly higher incidence of abnormal spindles in the vitrified group compared with the fresh group, notably of spindles with a focused and an unfocused pole as well as chromosome bridging and disorganized middle spindle fibres at telophase. Further investigation is warranted to elucidate the mitotic stages that are more vulnerable to damage during vitrification, the fate of the abnormal spindles and any potential effects that may be reflected on the chromosomal constitution of the developing blastocysts.

摘要

背景

玻璃化冷冻保存技术被广泛应用于 IVF 后多余胚胎的冷冻保存。本研究通过荧光和共聚焦激光扫描显微镜分析存活率以及纺锤体和染色体形态,旨在研究无菌玻璃化对人类囊胚细胞骨架和发育的影响。

方法

共收集新鲜囊胚 55 枚和玻璃化冷冻后第 5 天解冻的囊胚 55 枚,胚胎解冻后 24 小时继续培养,迅速在冰甲醇中固定,并与 a-微管蛋白抗体进行免疫荧光染色,以可视化微管,同时用抗乙酰化微管蛋白(用于可视化纺锤体、极体和中体)、γ微管蛋白(用于鉴定纺锤体极体)和 4,6-二脒基-2-苯基吲哚(DAPI)进行免疫荧光染色,以可视化 DNA。

结果

在新鲜组(对照组)中,共分析了 213 个纺锤体,其中 183/213(85.9%)为正常,20/213(9.4%)为异常,9/213(4.2%)为多极,1/213(0.5%)为单极。在玻璃化组中,共分析了 175 个纺锤体,其中 120/175(68.6%)为正常,39/175(22.3%)为异常,10/175(5.7%)为多极,6/175(3.4%)为单极。两组多极纺锤体的发生率相似,但玻璃化组异常纺锤体的比例明显高于新鲜组,异常纺锤体常与染色体滞后或 congression 失败有关(P<0.05)。

结论

胚胎解冻后的高存活率和大量正常纺锤体/染色体形态表明,在第 5 天的囊胚阶段进行玻璃化冷冻保存不会对人类胚胎的发育和纺锤体形成及继续正常细胞分裂的能力产生不利影响。然而,玻璃化组异常纺锤体的发生率明显高于新鲜组,尤其是具有聚焦和非聚焦极体以及染色体桥和中间纺锤体纤维在末期排列紊乱的纺锤体。需要进一步研究以阐明在玻璃化过程中更易受损的有丝分裂阶段、异常纺锤体的命运以及可能对发育中的囊胚染色体组成产生的任何潜在影响。

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