Extracellular vesicles secreted by human aneuploid embryos present a distinct transcriptomic profile and upregulate MUC1 transcription in decidualised endometrial stromal cells.

IF 8.3 Q1 OBSTETRICS & GYNECOLOGY

Human reproduction open Pub Date : 2024-03-12 eCollection Date: 2024-01-01 DOI:10.1093/hropen/hoae014

Sofia Makieva, Elisa Giacomini, Giulia Maria Scotti, Dejan Lazarevic, Valentina Pavone, Jessica Ottolina, Ludovica Bartiromo, Matteo Schimberni, Marco Morelli, Alessandra Alteri, Sabrina Minetto, Giovanni Tonon, Massimo Candiani, Enrico Papaleo, Paola Viganò

{"title":"Extracellular vesicles secreted by human aneuploid embryos present a distinct transcriptomic profile and upregulate MUC1 transcription in decidualised endometrial stromal cells.","authors":"Sofia Makieva, Elisa Giacomini, Giulia Maria Scotti, Dejan Lazarevic, Valentina Pavone, Jessica Ottolina, Ludovica Bartiromo, Matteo Schimberni, Marco Morelli, Alessandra Alteri, Sabrina Minetto, Giovanni Tonon, Massimo Candiani, Enrico Papaleo, Paola Viganò","doi":"10.1093/hropen/hoae014","DOIUrl":null,"url":null,"abstract":"Study question: Do extracellular vesicles (EVs) secreted by aneuploid human embryos possess a unique transcriptomic profile that elicits a relevant transcriptomic response in decidualized primary endometrial stromal cells (dESCs)?Summary answer: Aneuploid embryo-derived EVs contain transcripts of PPM1J, LINC00561, ANKRD34C, and TMED10 with differential abundance from euploid embryo-derived EVs and induce upregulation of MUC1 transcript in dESCs.What is known already: We have previously reported that IVF embryos secrete EVs that can be internalized by ESCs, conceptualizing that successful implantation to the endometrium is facilitated by EVs. Whether these EVs may additionally serve as biomarkers of ploidy status is unknown.Study design size duration: Embryos destined for biopsy for preimplantation genetic testing for aneuploidy (PGT-A) were grown under standard conditions. Spent media (30 μl) were collected from euploid (n = 175) and aneuploid (n = 140) embryos at cleavage (Days 1-3) stage and from euploid (n = 187) and aneuploid (n = 142) embryos at blastocyst (Days 3-5) stage. Media samples from n = 35 cleavage-stage embryos were pooled in order to obtain five euploid and four aneuploid pools. Similarly, media samples from blastocysts were pooled to create one euploid and one aneuploid pool. ESCs were obtained from five women undergoing diagnostic laparoscopy.Participants/materials setting methods: EVs were isolated from pools of media by differential centrifugation and EV-RNA sequencing was performed following a single-cell approach that circumvents RNA extraction. ESCs were decidualized (estradiol: 10 nM, progesterone: 1 µM, cAMP: 0.5 mM twice every 48 h) and incubated for 24 h with EVs (50 ng/ml). RNA sequencing was performed on ESCs.Main results and the role of chance: Aneuploid cleavage stage embryos secreted EVs that were less abundant in RNA fragments originating from the genes PPM1J (log2fc = -5.13, P = 0.011), LINC00561 (log2fc = -7.87, P = 0.010), and ANKRD34C (log2fc = -7.30, P = 0.017) and more abundant in TMED10 (log2fc = 1.63, P = 0.025) compared to EVs of euploid embryos. Decidualization per se induced downregulation of MUC1 (log2fc = -0.54, P = 0.0028) in ESCs as a prerequisite for the establishment of receptive endometrium. The expression of MUC1 transcript in decidualized ESCs was significantly increased following treatment with aneuploid compared to euploid embryo-secreted EVs (log2fc = 0.85, P = 0.0201).Large scale data: Raw data have been uploaded to GEO (accession number GSE234338).Limitations reasons for caution: The findings of the study will require validation utilizing a second cohort of EV samples.Wider implications of the findings: The discovery that the transcriptomic profile of EVs secreted from aneuploid cleavage stage embryos differs from that of euploid embryos supports the possibility to develop a non-invasive methodology for PGT-A. The upregulation of MUC1 in dESCs following aneuploid embryo EV treatment proposes a new mechanism underlying implantation failure.Study funding/competing interests: The study was supported by a Marie Skłodowska-Curie Actions fellowship awarded to SM by the European Commission (CERVINO grant agreement ID: 79620) and by a BIRTH research grant from Theramex HQ UK Ltd. The authors have no conflicts of interest to declare.","PeriodicalId":73264,"journal":{"name":"Human reproduction open","volume":"2024 2","pages":"hoae014"},"PeriodicalIF":8.3000,"publicationDate":"2024-03-12","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10980593/pdf/","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Human reproduction open","FirstCategoryId":"1085","ListUrlMain":"https://doi.org/10.1093/hropen/hoae014","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"2024/1/1 0:00:00","PubModel":"eCollection","JCR":"Q1","JCRName":"OBSTETRICS & GYNECOLOGY","Score":null,"Total":0}

引用次数: 0

Abstract

Study question: Do extracellular vesicles (EVs) secreted by aneuploid human embryos possess a unique transcriptomic profile that elicits a relevant transcriptomic response in decidualized primary endometrial stromal cells (dESCs)?

Summary answer: Aneuploid embryo-derived EVs contain transcripts of PPM1J, LINC00561, ANKRD34C, and TMED10 with differential abundance from euploid embryo-derived EVs and induce upregulation of MUC1 transcript in dESCs.

What is known already: We have previously reported that IVF embryos secrete EVs that can be internalized by ESCs, conceptualizing that successful implantation to the endometrium is facilitated by EVs. Whether these EVs may additionally serve as biomarkers of ploidy status is unknown.

Study design size duration: Embryos destined for biopsy for preimplantation genetic testing for aneuploidy (PGT-A) were grown under standard conditions. Spent media (30 μl) were collected from euploid (n = 175) and aneuploid (n = 140) embryos at cleavage (Days 1-3) stage and from euploid (n = 187) and aneuploid (n = 142) embryos at blastocyst (Days 3-5) stage. Media samples from n = 35 cleavage-stage embryos were pooled in order to obtain five euploid and four aneuploid pools. Similarly, media samples from blastocysts were pooled to create one euploid and one aneuploid pool. ESCs were obtained from five women undergoing diagnostic laparoscopy.

Participants/materials setting methods: EVs were isolated from pools of media by differential centrifugation and EV-RNA sequencing was performed following a single-cell approach that circumvents RNA extraction. ESCs were decidualized (estradiol: 10 nM, progesterone: 1 µM, cAMP: 0.5 mM twice every 48 h) and incubated for 24 h with EVs (50 ng/ml). RNA sequencing was performed on ESCs.

Main results and the role of chance: Aneuploid cleavage stage embryos secreted EVs that were less abundant in RNA fragments originating from the genes PPM1J (log2fc = -5.13, P = 0.011), LINC00561 (log2fc = -7.87, P = 0.010), and ANKRD34C (log2fc = -7.30, P = 0.017) and more abundant in TMED10 (log2fc = 1.63, P = 0.025) compared to EVs of euploid embryos. Decidualization per se induced downregulation of MUC1 (log2fc = -0.54, P = 0.0028) in ESCs as a prerequisite for the establishment of receptive endometrium. The expression of MUC1 transcript in decidualized ESCs was significantly increased following treatment with aneuploid compared to euploid embryo-secreted EVs (log2fc = 0.85, P = 0.0201).

Large scale data: Raw data have been uploaded to GEO (accession number GSE234338).

Limitations reasons for caution: The findings of the study will require validation utilizing a second cohort of EV samples.

Wider implications of the findings: The discovery that the transcriptomic profile of EVs secreted from aneuploid cleavage stage embryos differs from that of euploid embryos supports the possibility to develop a non-invasive methodology for PGT-A. The upregulation of MUC1 in dESCs following aneuploid embryo EV treatment proposes a new mechanism underlying implantation failure.

Study funding/competing interests: The study was supported by a Marie Skłodowska-Curie Actions fellowship awarded to SM by the European Commission (CERVINO grant agreement ID: 79620) and by a BIRTH research grant from Theramex HQ UK Ltd. The authors have no conflicts of interest to declare.

查看原文本刊更多论文

人类非整倍体胚胎分泌的胞外囊泡呈现出独特的转录组特征，并上调蜕膜化子宫内膜基质细胞中的 MUC1 转录。

研究问题：非畸形人类胚胎分泌的细胞外囊泡（EVs）是否具有独特的转录组特征，能在蜕膜化的原代子宫内膜基质细胞（dESCs）中引起相关的转录组反应？非整倍体胚胎衍生的EV含有PPM1J、LINC00561、ANKRD34C和TMED10的转录本，其丰度与整倍体胚胎衍生的EV不同，并能诱导dESCs中MUC1转录本的上调：我们以前曾报道过体外受精胚胎分泌的EVs可被ESCs内化，并认为EVs可促进胚胎成功植入子宫内膜。这些EV是否还能作为倍性状态的生物标志物尚不清楚：在标准条件下培育胚胎，对胚胎进行活检以进行植入前非整倍体基因检测（PGT-A）。从处于卵裂期（第 1-3 天）的优合体胚胎（n = 175）和非整倍体胚胎（n = 140）以及处于囊胚期（第 3-5 天）的优合体胚胎（n = 187）和非整倍体胚胎（n = 142）中收集用过的培养基（30 μl）。将来自 n = 35 个卵裂期胚胎的培养基样本集中在一起，以获得 5 个优倍体池和 4 个非整倍体池。同样，囊胚的培养基样本也集中在一起，形成一个优倍体池和一个非整倍体池。造血干细胞来自五名接受腹腔镜诊断的女性：通过差速离心从培养基池中分离出EV，并采用单细胞方法进行EV-RNA测序，从而避免了RNA提取。ESC蜕膜（雌二醇：10 nM，孕酮：1 µM，cAMP：0.5 mM，每48小时两次）并与EVs（50 ng/ml）孵育24小时。对 ESCs 进行了 RNA 测序：非整倍体分裂期胚胎分泌的 EVs 中，源自基因 PPM1J（log2fc = -5.13，P = 0.011）、LINC00561（log2fc = -7.87，P = 0.010）和 ANKRD34C（log2fc = -7.30，P = 0.017），与优倍体胚胎的 EV 相比，TMED10 的含量更高（log2fc = 1.63，P = 0.025）。蜕膜本身会诱导 ESC 中 MUC1 的下调（log2fc = -0.54，P = 0.0028），这是建立可接受子宫内膜的先决条件。用非整倍体胚胎分泌的EVs处理蜕膜化的ESCs后，MUC1转录本的表达量比用整倍体胚胎分泌的EVs处理后显著增加（log2fc = 0.85，P = 0.0201）：原始数据已上传至 GEO（登录号 GSE234338）：该研究的发现需要利用第二批 EV 样本进行验证：发现非整倍体分裂期胚胎分泌的EV的转录组特征不同于优倍体胚胎，这为开发PGT-A的非侵入性方法提供了可能。非整倍体胚胎EV处理后dESCs中MUC1的上调提出了植入失败的新机制：该研究得到了欧盟委员会（CERVINO grant agreement ID: 79620）授予SM的Marie Skłodowska-Curie行动奖学金以及Theramex HQ UK Ltd.的BIRTH研究基金的支持。作者无利益冲突需要声明。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

求助全文

约1分钟内获得全文求助全文

来源期刊

Human reproduction open

CiteScore

15.50

自引率

0.00%

发文量

审稿时长

12 weeks