ART altered DNA methylation of the imprinted gene H19 in fetal tissue after multifetal pregnancy reduction

IF 4.3 3区 材料科学 Q1 ENGINEERING, ELECTRICAL & ELECTRONIC ACS Applied Electronic Materials Pub Date : 2024-09-10 DOI:10.1007/s10815-024-03218-2
Wenbin Wu, Menglu Ji, Jingjing Yang, Meng Zhang, Dayong Hao, Xinyan Zhao, Saisai Li, Yichun Guan, Xingling Wang
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Abstract

Purpose

This study aimed to assess whether assisted reproductive technology alters DNA methylation levels at the H19 promoter and H19 imprinting control element (ICE) in fetal tissues obtained after multifetal pregnancy reduction.

Methods

Fetal tissues from multiple pregnancies were obtained, including fresh and frozen-thawed embryos: nine from conventional in vitro fertilization (c-IVF), four from intracytoplasmic sperm injection (ICSI), ten from cryopreserved IVF embryos (cryo-IVF), and six from cryopreserved ICSI (cryo-ICSI) embryos. Next-generation sequencing-based bisulfite PCR was used to determine the DNA methylation status of three CpG islands (H19-1, H19-2, and H19-3) in the H19 promoter and H19 ICE. The primary outcome was H19-1 DNA methylation status, whereas secondary outcomes assessed H19-2, H19-3, and ICE methylation.

Results

The ICSI (β = -3.189, 95% CI = -5.034 to -1.345, p = 0.0026), cryo-IVF (β = -2.150, 95% CI = -3.706 to -0.593, p = 0.0129), and cryo-ICSI (β = -2.238, 95% CI = -3.817 to -0.659, p = 0.0110) groups exhibited significantly lower methylation levels in the primary outcome H19-1 region than the c-IVF group after adjustment. For the secondary outcome H19-2 region, significant decreases were observed in the cryo-IVF (β = -2.132, 95% CI = -4.071 to -0.192, p = 0.0425) and cryo-ICSI groups (β = -2.598, 95% CI = -4.566 to -0.630, p = 0.0168).

Conclusions

These findings further indicate that embryo cryopreservation and potentially ICSI can lower the methylation level of the H19 promoter, advocating for careful use of these techniques when necessary.

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ART 改变了多胎妊娠减胎后胎儿组织中印记基因 H19 的 DNA 甲基化
目的 本研究旨在评估辅助生殖技术是否会改变多胎妊娠减胎后胎儿组织中H19启动子和H19印记控制元件(ICE)的DNA甲基化水平。方法获得了多胎妊娠的胎儿组织,包括新鲜和冷冻解冻的胚胎:9个来自常规体外受精(c-IVF),4个来自卵胞浆内单精子注射(ICSI),10个来自低温保存的体外受精胚胎(cryo-IVF),6个来自低温保存的ICSI胚胎(cryo-ICSI)。研究人员利用基于下一代测序的亚硫酸氢盐 PCR 技术确定了 H19 启动子和 H19 ICE 中三个 CpG 岛(H19-1、H19-2 和 H19-3)的 DNA 甲基化状态。结果ICSI(β = -3.189,95% CI = -5.034 to -1.345, p = 0.0026)、冷冻-体外受精(β = -2.150,95% CI = -3.706到-0.593,p = 0.0129)和冷冻-ICSI(β = -2.238,95% CI = -3.817到-0.659,p = 0.0110)组在主要结果H19-1区域的甲基化水平在调整后显著低于c-IVF组。对于次要结果 H19-2 区域,在冷冻IVF 组(β = -2.132,95% CI = -4.071 至 -0.192,p = 0.0425)和冷冻卵胞浆内单精子显微注射组(β = -2.598,95% CI = -4.566 至 -0.结论这些研究结果进一步表明,胚胎冷冻保存和潜在的 ICSI 可降低 H19 启动子的甲基化水平,提倡在必要时谨慎使用这些技术。
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7.20
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4.30%
发文量
567
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