Nuclear transfer of sand cat cells into enucleated domestic cat oocytes is affected by cryopreservation of donor cells.

Martha C Gómez, C Earle Pope, Robert H Kutner, David M Ricks, Leslie A Lyons, Mark Ruhe, Cherie Dumas, Justine Lyons, Mónica López, Betsy L Dresser, Jakob Reiser
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引用次数: 97

Abstract

In the present study, we used the sand cat (Felis margarita) as a somatic cell donor to evaluate whether cryopreservation of donor cells alters viability and epigenetic events in donor cells and affects in vitro and in vivo developmental competence of derived embryos. In Experiment 1, flow cytometry analysis revealed that the percentage of necrosis and apoptosis in cells analyzed immediately after freezing/thawing (61 vs. 8.1%, respectively) was higher than that observed in frozen/thawed cells cultured for 18 h (6.9 vs. 3.3%, respectively) or 5 days (38 vs. 2.6%; respectively). The relative acetylation level of H3K9 was lower in frozen/thawed cells (5.4%) compared to that found in cultured cells (60.1%). In Experiment 2, embryos reconstructed with frozen/thawed cells had a lower cleavage rate (85%; day 2) than did embryos reconstructed with cultured cells (95%), while development to the blastocyst stage (day 8) was not affected by cell treatment (17.0% with frozen/thawed cells vs. 16.5% with cultured cells). In Experiment 3, pregnancy rates were similar between both cell treatments (32% with frozen/thawed cells vs. 30% with cultured cells), but the number of embryos that were implanted, and the number of fetuses that developed to term was lower for embryos reconstructed with frozen/thawed cells (1.2 and 0.3%, respectively) than those reconstructed with cultured cells (2.6 and 1.8%, respectively), while the number of fetuses reabsorbed by day 30 was higher (75%) for embryos reconstructed with frozen/thawed cells than those reconstructed with cultured cells (31%). A total of 11 kittens from cultured cells and three kittens from frozen/thawed cells were born between days 60 to 64 of gestation. Most kittens died within a few days after birth, although one kitten did survive for 2 months. In Experiment 4, POU5F1 mRNA expression was detected in 25% of blastocysts derived from frozen/thawed cells, whereas 88 and 87% of blastocysts derived from cultured cells and by in vitro fertilization, respectively, expressed POU5F1. We have shown that cell cryopreservation increased the incidence of necrosis and apoptosis and altered epigenetic events in donor cells. Consequently, the number of embryos that cleaved, implanted, and developed to term-gestation and POU5F1 expression in derived blastocysts indirectly was affected.

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沙猫细胞的核移植到去核的家猫卵母细胞受到供体细胞低温保存的影响。
在本研究中,我们以沙猫(Felis margarita)作为体细胞供体,评估供体细胞低温保存是否会改变供体细胞的活力和表观遗传事件,并影响衍生胚胎的体外和体内发育能力。实验1中,流式细胞术分析显示,冷冻/解冻后立即分析的细胞中坏死和凋亡的百分比(分别为61比8.1%)高于冷冻/解冻18 h(分别为6.9比3.3%)或5 d(分别为38比2.6%;分别)。冷冻/解冻细胞中H3K9的相对乙酰化水平(5.4%)低于培养细胞(60.1%)。在实验2中,用冷冻/解冻细胞重建的胚胎的卵裂率较低(85%;第2天)比用培养细胞重建的胚胎(95%),而发育到囊胚期(第8天)不受细胞处理的影响(17.0%的冷冻/解冻细胞对16.5%的培养细胞)。在实验3中,两种细胞处理之间的妊娠率相似(冷冻/解冻细胞处理32%,培养细胞处理30%),但植入的胚胎数量和发育至足月的胎儿数量,冷冻/解冻细胞处理的胚胎(分别为1.2和0.3%)低于培养细胞处理的胚胎(分别为2.6和1.8%)。而用冷冻/解冻细胞重建的胚胎在第30天重吸收的胎儿数量(75%)高于用培养细胞重建的胚胎(31%)。在妊娠第60天至第64天,培养细胞和冷冻/解冻细胞分别产生了11只和3只幼猫。大多数小猫在出生后几天内死亡,尽管有一只小猫存活了两个月。实验4中,25%的冷冻/解冻囊胚中检测到POU5F1 mRNA的表达,而培养囊胚和体外受精囊胚中分别有88%和87%的囊胚表达POU5F1。我们已经表明,细胞冷冻保存增加了供体细胞坏死和凋亡的发生率,并改变了表观遗传事件。因此,胚胎的分裂、植入和发育到妊娠期的数量和衍生囊胚中POU5F1的表达间接受到影响。
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