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本文引用的文献

1
Non-invasive, label-free optical analysis to detect aneuploidy within the inner cell mass of the preimplantation embryo.应用非侵入性、无标记的光学分析技术,检测胚胎植入前内细胞团中的非整倍体。
Hum Reprod. 2021 Dec 27;37(1):14-29. doi: 10.1093/humrep/deab233.
2
Author Correction: Depletion of aneuploid cells in human embryos and gastruloids.作者更正:人类胚胎和原肠胚样结构中非整倍体细胞的耗尽。
Nat Cell Biol. 2021 Nov;23(11):1212. doi: 10.1038/s41556-021-00775-x.
3
The "mosaic" embryo: misconceptions and misinterpretations in preimplantation genetic testing for aneuploidy.“镶嵌型”胚胎:非整倍体植入前基因检测中的误解与误读
Fertil Steril. 2021 Nov;116(5):1205-1211. doi: 10.1016/j.fertnstert.2021.06.027. Epub 2021 Jul 23.
4
Intracellular pH Regulates Cancer and Stem Cell Behaviors: A Protein Dynamics Perspective.细胞内pH调节癌症和干细胞行为:蛋白质动力学视角
Front Oncol. 2020 Aug 26;10:1401. doi: 10.3389/fonc.2020.01401. eCollection 2020.
5
Autophagy-mediated apoptosis eliminates aneuploid cells in a mouse model of chromosome mosaicism.自噬介导的细胞凋亡可消除染色体嵌合体小鼠模型中的非整倍体细胞。
Nat Commun. 2020 Jun 11;11(1):2958. doi: 10.1038/s41467-020-16796-3.
6
The birth of a baby with mosaicism resulting from a known mosaic embryo transfer: a case report.一例因已知的嵌合胚胎移植导致的嵌合婴儿出生:病例报告
Hum Reprod. 2020 Mar 27;35(3):727-733. doi: 10.1093/humrep/dez309.
7
Need for choosing the ideal pH value for IVF culture media.需要选择理想的 pH 值用于 IVF 培养液。
J Assist Reprod Genet. 2020 May;37(5):1019-1028. doi: 10.1007/s10815-020-01726-5. Epub 2020 Mar 2.
8
Reconstituting the transcriptome and DNA methylome landscapes of human implantation.重建人类着床过程中的转录组和 DNA 甲基化组图谱。
Nature. 2019 Aug;572(7771):660-664. doi: 10.1038/s41586-019-1500-0. Epub 2019 Aug 21.
9
Embryonic POU5F1 is Required for Expanded Bovine Blastocyst Formation.胚胎 POU5F1 对于扩展牛囊胚的形成是必需的。
Sci Rep. 2018 May 17;8(1):7753. doi: 10.1038/s41598-018-25964-x.
10
Caspase 2 in mitotic catastrophe: The terminator of aneuploid and tetraploid cells.有丝分裂灾难中的半胱天冬酶2:非整倍体和四倍体细胞的终结者。
Mol Cell Oncol. 2017 Mar 10;4(3):e1299274. doi: 10.1080/23723556.2017.1299274. eCollection 2017.

在培养基中添加弱酸 5,5-二甲基-2,4-恶唑烷二酮(DMO)可以通过 Trp53 依赖的机制限制非整倍体小鼠胚胎的发育。

Supplementing culture medium with the weak acid, 5,5-dimethyl-2,4-oxazolidinedione (DMO) limits the development of aneuploid mouse embryos through a Trp53-dependent mechanism.

机构信息

Department of Cell Biology, University of Connecticut Health Center, 263 Farmington Ave., CT, 06030, Farmington, USA.

Department of Obstetrics and Gynecology, University of Connecticut Health Center, Farmington, CT, 06030, USA.

出版信息

J Assist Reprod Genet. 2023 May;40(5):1215-1223. doi: 10.1007/s10815-023-02788-x. Epub 2023 Apr 14.

DOI:10.1007/s10815-023-02788-x
PMID:37058262
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10239418/
Abstract

PURPOSE

This study was designed to determine if DMO limits in vitro development of aneuploid-enriched mouse embryos by activating a Trp53-dependent mechanism.

METHODS

Mouse cleavage-stage embryos were treated with reversine to induce aneuploidy or vehicle to generate controls, and then cultured in media supplemented with DMO to reduce the pH of the culture media. Embryo morphology was assessed by phase microscopy. Cell number, mitotic figures, and apoptotic bodies were revealed by staining fixed embryos with DAPI. mRNA levels of Trp53, Oct-4, and Cdx2 were monitored by quantitative polymerase chain reactions (qPCRs). The effect of Trp53 on the expression of Oct-4 and Cdx2 was assessed by depleting Trp53 using Trp53 siRNA.

RESULTS

Aneuploid-enriched late-stage blastocysts were morphologically indistinguishable from control blastocysts but had fewer cells and reduced mRNA levels of Oct-4 and Cdx2. Adding 1 mM DMO to the culture media during the 8-cell to blastocyst transition reduced the formation of aneuploid-enriched late-stage blastocysts but not control blastocysts and further suppressed the levels of Oct-4 and Cdx2 mRNA. Trp53 RNA levels in aneuploid-enriched embryos that were exposed to DMO were > twofold higher than controls, and Trp53 siRNA levels reduced the levels of Trp53 and increased levels of Oct-4 and Cdx2 mRNA by > twofold.

CONCLUSION

These studies suggest that the development of morphologically normal aneuploid-enriched mouse blastocysts can be inhibited by adding low amounts of DMO to the culture media, which results in elevated levels of Trp53 mRNA that suppresses Oct-4 and Cdx2 expression.

摘要

目的

本研究旨在通过激活 Trp53 依赖性机制,确定 DMO 限制体外发育非整倍体富集的小鼠胚胎的程度。

方法

用 reversine 处理小鼠卵裂期胚胎以诱导非整倍体或用载体生成对照,并在补充 DMO 的培养基中培养以降低培养基的 pH 值。通过相差显微镜评估胚胎形态。用 DAPI 固定胚胎染色显示细胞数量、有丝分裂图和凋亡小体。通过定量聚合酶链反应(qPCRs)监测 Trp53、Oct-4 和 Cdx2 的 mRNA 水平。通过使用 Trp53 siRNA 耗尽 Trp53 来评估 Trp53 对 Oct-4 和 Cdx2 表达的影响。

结果

非整倍体富集的晚期囊胚在形态上与对照囊胚无法区分,但细胞数量较少,Oct-4 和 Cdx2 的 mRNA 水平降低。在 8 细胞至囊胚过渡期间向培养基中添加 1 mM DMO 可减少非整倍体富集的晚期囊胚的形成,但不减少对照囊胚的形成,并进一步抑制 Oct-4 和 Cdx2 mRNA 的水平。暴露于 DMO 的非整倍体富集胚胎中的 Trp53 RNA 水平比对照高出两倍以上,Trp53 siRNA 水平降低了 Trp53 的水平,并将 Oct-4 和 Cdx2 mRNA 的水平提高了两倍以上。

结论

这些研究表明,通过向培养基中添加少量 DMO 可以抑制形态正常的非整倍体富集的小鼠囊胚的发育,导致 Trp53 mRNA 水平升高,从而抑制 Oct-4 和 Cdx2 的表达。