Department of Cell and Developmental Biology, Epigenetics Institute, Perelman School of Medicine, University of Pennsylvania, Philadelphia, PA, USA.
Center for Research on Reproduction and Women's Health, University of Pennsylvania, Philadelphia, PA, USA.
Hum Reprod. 2024 Jan 5;39(1):154-176. doi: 10.1093/humrep/dead238.
Does trophectoderm biopsy (TEBx) of blastocysts for preimplantation genetic testing in the clinic affect normal placental and embryo development and offspring metabolic outcomes in a mouse model?
TEBx impacts placental and embryonic health during early development, with some alterations resolving and others worsening later in development and triggering metabolic changes in adult offspring.
Previous studies have not assessed the epigenetic and morphological impacts of TEBx either in human populations or in animal models.
STUDY DESIGN, SIZE, DURATION: We employed a mouse model to identify the effects of TEBx during IVF. Three groups were assessed: naturally conceived (Naturals), IVF, and IVF + TEBx, at two developmental timepoints: embryonic day (E)12.5 (n = 40/Naturals, n = 36/IVF, and n = 36/IVF + TEBx) and E18.5 (n = 42/Naturals, n = 30/IVF, and n = 35/IVF + TEBx). Additionally, to mimic clinical practice, we assessed a fourth group: IVF + TEBx + Vitrification (Vit) at E12.5 (n = 29) that combines TEBx and vitrification. To assess the effect of TEBx in offspring health, we characterized a 12-week-old cohort (n = 24/Naturals, n = 25/IVF and n = 25/IVF + TEBx).
PARTICIPANTS/MATERIALS, SETTING, METHODS: Our mouse model used CF-1 females as egg donors and SJL/B6 males as sperm donors. IVF, TEBx, and vitrification were performed using standardized methods. Placenta morphology was evaluated by hematoxylin-eosin staining, in situ hybridization using Tpbpa as a junctional zone marker and immunohistochemistry using CD34 fetal endothelial cell markers. For molecular analysis of placentas and embryos, DNA methylation was analyzed using pyrosequencing, luminometric methylation assay, and chip array technology. Expression patterns were ascertained by RNA sequencing. Triglycerides, total cholesterol, high-, low-, and very low-density lipoprotein, insulin, and glucose were determined in the 12-week-old cohort using commercially available kits.
We observed that at E12.5, IVF + TEBx had a worse outcome in terms of changes in DNA methylation and differential gene expression in placentas and whole embryos compared with IVF alone and compared with Naturals. These changes were reflected in alterations in placental morphology and blood vessel density. At E18.5, early molecular changes in fetuses were maintained or exacerbated. With respect to placentas, the molecular and morphological changes, although different compared to Naturals, were equivalent to the IVF group, except for changes in blood vessel density, which persisted. Of note is that most differences were sex specific. We conclude that TEBx has more detrimental effects in mid-gestation placental and embryonic tissues, with alterations in embryonic tissues persisting or worsening in later developmental stages compared to IVF alone, and the addition of vitrification after TEBx results in more pronounced and potentially detrimental epigenetic effects: these changes are significantly different compared to Naturals. Finally, we observed that 12-week IVF + TEBx offspring, regardless of sex, showed higher glucose, insulin, triglycerides, lower total cholesterol, and lower high-density lipoprotein compared to IVF and Naturals, with only males having higher body weight compared to IVF and Naturals. Our findings in a mouse model additionally support the need for more studies to assess the impact of new procedures in ART to ensure healthy pregnancies and offspring outcomes.
Data reported in this work have been deposited in the NCBI Gene Expression Omnibus under accession number GSE225318.
LIMITATIONS, REASONS FOR CAUTION: This study was performed using a mouse model that mimics many clinical IVF procedures and outcomes observed in humans, where studies on early embryos are not possible.
This study highlights the importance of assaying new procedures used in ART to assess their impact on placenta and embryo development, and offspring metabolic outcomes.
STUDY FUNDING/COMPETING INTEREST(S): This work was funded by a National Centers for Translational Research in Reproduction and Infertility grant P50 HD068157-06A1 (M.S.B., C.C., M.M.), Ruth L. Kirschstein National Service Award Individual Postdoctoral Fellowship F32 HD107914 (E.A.R.-C.) and F32 HD089623 (L.A.V.), and National Institutes of Health Training program in Cell and Molecular Biology T32 GM007229 (C.N.H.). No conflict of interest.
胚胎种植前遗传学检测中对囊胚的滋养外胚层活检(TEBx)是否会影响小鼠模型中正常胎盘和胚胎的发育以及后代的代谢结局?
TEBx 在早期发育过程中会影响胎盘和胚胎的健康,一些改变会在后期得到解决,而另一些则会恶化,并引发成年后代的代谢变化。
之前的研究要么没有在人类群体中,要么没有在动物模型中评估 TEBx 的表观遗传和形态影响。
研究设计、大小和持续时间:我们采用了一种小鼠模型来确定 IVF 过程中 TEBx 的影响。评估了三组:自然受孕(Naturals)、IVF 和 IVF+TEBx,在两个发育时间点:胚胎日(E)12.5(n=40/Naturals,n=36/IVF,n=36/IVF+TEBx)和 E18.5(n=42/Naturals,n=30/IVF,n=35/IVF+TEBx)。此外,为了模拟临床实践,我们评估了第四组:IVF+TEBx+Vit 组在 E12.5 时(n=29),该组结合了 TEBx 和玻璃化。为了评估 TEBx 对后代健康的影响,我们对 12 周龄的队列进行了特征描述(n=24/Naturals,n=25/IVF 和 n=25/IVF+TEBx)。
参与者/材料、设置、方法:我们的小鼠模型使用 CF-1 雌性作为卵子供体,SJL/B6 雄性作为精子供体。IVF、TEBx 和玻璃化都是用标准化的方法进行的。胎盘形态通过苏木精-伊红染色、使用 Tpbpa 作为连接区标记物的原位杂交和使用 CD34 胎儿内皮细胞标记物的免疫组织化学进行评估。为了分析胎盘和胚胎的分子变化,使用焦磷酸测序、发光甲基化测定和芯片阵列技术分析 DNA 甲基化。通过 RNA 测序确定表达模式。使用市售试剂盒测定 12 周龄队列的甘油三酯、总胆固醇、高低密度脂蛋白、胰岛素和葡萄糖。
我们观察到,在 E12.5 时,与 IVF 相比,IVF+TEBx 导致胎盘和整个胚胎的 DNA 甲基化和差异基因表达发生变化,其结果更糟,与 Naturals 相比也更糟。这些变化反映在胎盘形态和血管密度的改变上。在 E18.5 时,胎儿的早期分子变化得到了维持或加剧。就胎盘而言,尽管与 Naturals 相比,分子和形态变化不同,但与 IVF 组相当,除了血管密度的变化仍然存在。值得注意的是,大多数差异都是性别特异性的。我们的结论是,TEBx 在中期妊娠胎盘和胚胎组织中具有更大的破坏性影响,与 IVF 相比,胚胎组织的变化在后期发育阶段持续存在或恶化,并且在 TEBx 后添加玻璃化会导致更明显和潜在的有害的表观遗传影响:这些变化与 Naturals 相比有显著差异。最后,我们观察到,无论性别如何,12 周龄的 IVF+TEBx 后代的葡萄糖、胰岛素、甘油三酯较高,总胆固醇和高密度脂蛋白较低,与 IVF 和 Naturals 相比,只有雄性的体重比 IVF 和 Naturals 高。我们在小鼠模型中的研究结果进一步支持了需要进行更多的研究,以评估新的 ART 程序对确保健康妊娠和后代结局的影响。
本研究中报告的数据已在 NCBI 基因表达综合数据库中以 GSE225318 号存档。
局限性、谨慎的原因:这项研究是使用模拟人类许多临床 IVF 程序和结果的小鼠模型进行的,在这种模型中不可能对早期胚胎进行研究。
这项研究强调了评估新程序在 ART 中的应用以评估其对胎盘和胚胎发育以及后代代谢结局的影响的重要性。
研究资金/利益冲突:这项工作得到了转化生殖与不孕国家研究中心的 P50 HD068157-06A1 赠款(M.S.B.、C.C.、M.M.)、Ruth L. Kirschstein 国家服务奖个人博士后奖学金 F32 HD107914(E.A.R.-C.)和 F32 HD089623(L.A.V.)以及细胞和分子生物学 T32 GM007229 国家研究所培训计划(C.N.H.)的资助。没有利益冲突。
