Your search keyword '"Trophectoderm"' showing total 897 results

151. Development of trophoblast cystic structures from human induced pluripotent stem cells in limited-area cell culture.

Author

Li, Zhuosi, Kurosawa, Osamu, and Iwata, Hiroo

Subjects

*ENGINEERING, *PLURIPOTENT stem cells, *CHORIONIC gonadotropins, *CYSTS (Pathology), *GENES

Abstract

Abstract We developed a novel engineering technique to induce differentiation of human induced pluripotent stem cells (hiPSCs) into organoids mimicking the trophectoderm (TE). Here, hiPSCs were cultured on a limited area of 2–4 mm in diameter. After 15–20 days, spherical cysts appeared on the surface of the limited area. Secretion of human chorionic gonadotrophin (hCG) began to increase after ∼ 20 days and remained dramatically elevated over the next 20 days. Limited-area-cultured cysts exhibited expression of hCG, which was a result of epithelial differentiation. Low expression levels of pluripotent genes and high expression levels of trophoblast lineage-specific genes were detected in the cells of spherical cysts. Multinucleated syncytia trophoblast was observed in the reseeded cystic cells. We observed hiPSC-derived cysts that morphologically resembled trophectoderm in vivo. The limited-area cell culture induced a three-dimensional (3D) trophectoderm organoid, which has potential for use in the study of human trophoblast differentiation and placental morphogenesis. Highlights • Limited-area culture of iPSs induced trophectoderm-like cyst structures. • Trophectoderm-like cyst structures exhibited trophoblast function. • These cysts provide a 3D model for the study of differentiation and morphogenesis. [ABSTRACT FROM AUTHOR]

Published

2018

152. Euploidy in relation to blastocyst sex and morphology.

Author

Wang, Ange, Kort, Jonathan, Behr, Barry, and Westphal, Lynn M.

Subjects

*BLASTOCYST, *CELL morphology, *PLOIDY, *HUMAN in vitro fertilization, *PREIMPLANTATION genetic diagnosis

Abstract

Purpose: The objective of our study is to assess the relationship of embryo ploidy status in relation to embryo sex, morphological characteristics, and transfer parameters.Methods: This is a retrospective cohort study at an academic medical center of patients who underwent in vitro fertilization with preimplantation genetic screening (PGS) from 2010 to 2015. Embryos were screened with 24-chromosome preimplantation genetic screening with day 5/6 trophectoderm biopsy. We investigated embryo euploidy in relation to morphology (expansion, inner cell mass, trophectoderm), embryo sex, biopsy day, and blastocyst cohort size. We used multivariate logistic regression to calculate odds ratios of euploidy in relation to these parameters.Results: A total of 1559 embryos from 316 cycles and 233 patients (mean maternal age = 37.8 ± 4.2 years) were included in the analysis. Six hundred and twenty-eight blastocysts (40.3%) were found to be euploid. Expansion (p < 0.001), inner cell mass (ICM) (p < 0.01), and trophectoderm grade (p < 0.001) were significantly associated with embryo ploidy in bivariate models controlling for maternal age, while embryo sex, biopsy day, and blastocyst cohort size were not associated with embryo ploidy. In a multivariate model, we found that maternal age (p < 0.001), higher grade of expansion (p < 0.01), and better quality trophectoderm (p < 0.001 for A compared to C grade) remained significantly associated with increased embryo euploidy, but ICM grade was no longer significant. Embryo sex was not associated with ploidy status, though male embryos were found to be associated with higher trophectoderm scores (p < 0.02).Conclusions: This is the largest study to date to investigate PGS-tested embryo sex and ploidy status. While maternal age and some morphological parameters (expansion, trophectoderm grade) are associated with euploidy in our cohort, other parameters such as embryo sex, biopsy day, and cohort size are not. Though embryo sex was not associated with euploidy, male embryos were found to be associated with higher trophectoderm grades. Additional investigation in larger studies is warranted. [ABSTRACT FROM AUTHOR]

Published

2018

153. Hypoxia-dependent accumulation of hypoxia-inducible factor-1 alpha induces transient cell cycle arrest in porcine trophectoderm cells.

Author

Jeong, Wooyoung, Jung, Seoungo, Bazer, Fuller W., and Kim, Jinyoung

Subjects

*HYPOXIA-inducible factor 1, *CELL cycle, *GENE expression, *CYCLINS, *TRANSCRIPTION factors

Abstract

In the uterine environment, the pre-implantation embryo adapts to low oxygen concentrations through intracellular responses including modification of gene expression, progression via the cell cycle and metabolism. In this study, we determined mechanisms underlying the adaptation of pig embryos to oxygen deficiency in the maternal-conceptus microenvironment in in vitro experiments using our established porcine trophectoderm (pTr) cells in culture. The transition from G 1 to S phase in pTr cells was reduced in response to 2% oxygen during a short period (<24 h), and the hypoxia-induced G 1 arrest was reversible during prolonged hypoxia exposure. Acute hypoxia up-regulated expression of transcription factors p21 and p27 and down-regulated cell cycle regulators associated with the G 1 /S phase transition including cyclin D1, cyclin E1 and E2F1 mRNAs and proteins. Furthermore, hypoxia exposure for 24 h markedly increased the abundance of HIF-1α protein. Even under acute hypoxia, by HIF-1α silencing reduced the hypoxia-induced transient G 1 arrest and expression of p21 and p27 genes was restored. Contrary to acute hypoxia, the accumulation of HIF-1α protein decreased as the length of the hypoxic period increased. Overall results of the present study suggest that increases in HIF-1α are responsible for initial response to hypoxia that results in a transient cell cycle arrest in pTr cells and cell cycle progression is restored by increasing degradation of HIF-1α during prolonged hypoxia. These findings advance understating of cellular adaptation of developing pre-implantation porcine conceptuses to hypoxic stress. [ABSTRACT FROM AUTHOR]

Published

2018

154. Chromosomal mosaicism in human blastocysts: the ultimate challenge of preimplantation genetic testing?

Author

Popovic, M., Dheedene, A., Christodoulou, C., Taelman, J., Dhaenens, L., Van Nieuwerburgh, F., Deforce, D., Van den Abbeel, E., De Sutter, P., Menten, B., and Heindryckx, B.

Subjects

*PREIMPLANTATION genetic diagnosis, *MOSAICISM, *BLASTOCYST, *MITOSIS, *HUMAN chromosomes

Abstract

Study Question: To what extent does a trophectoderm (TE) biopsy reliably reflect the chromosomal constitution of the inner cell mass (ICM) in human blastocysts?Summary Answer: Concordance between TE and ICM was established in 62.1% of the embryos analysed.What Is Known Already: Next generation sequencing (NGS) platforms have recently been optimised for preimplantation genetic testing for aneuploidies (PGT-A). However, higher sensitivity has led to an increase in reports of chromosomal mosaicism within a single TE biopsy. This has raised substantial controversy surrounding the prevalence of mosaicism in human blastocysts and the clinical implications of heterogeneity between the TE and ICM.Study Design, Size, Duration: To define the distribution and rate of mosaicism in human blastocysts, we assessed chromosomal profiles of the ICM and multiple TE portions obtained from the same embryo. We evaluated donated embryos with an unknown chromosomal profile (n = 34), as well as PGT-A blastocysts, previously diagnosed as abnormal or mosaic (n = 24). Our intra-embryo comparison included a total of 232 samples, obtained from 58 embryos.Participants/materials, Setting, Methods: Four embryo samples, including the ICM and three distinct TE portions, were acquired from good quality blastocysts by micromanipulation. Whole genome amplification (WGA), followed by NGS was performed on all embryo segments. Profiles were compared between samples from the same embryo, while the results from pretested blastocysts were further correlated to the original report. The embryos investigated in our untested group were obtained from good prognosis patients (n = 25), with maternal age ranging from 23 to 39 years. For the pretested embryo group, maternal age ranged from 23 to 40 years (n = 18).Main Results and the Role Of Chance: We uncover chromosomal mosaicism, involving both numerical and structural aberrations, in up to 37.9% of the blastocysts analysed. Within the untested group, the overall concordance between the ICM and all TE portions was 55.9%. A normal ICM was detected in 20.6% of blastocysts for which at least one TE portion showed a chromosomal aberration. Conversely, 17.6% of embryos presented with mosaic or uniform abnormalities within the ICM, while showing normal or mosaic TE profiles. For the pretested blastocysts, the overall concordance between the ICM and all TE samples was 70.8%. However, 50% of embryos previously diagnosed with mosaicism did not confirm the original diagnosis. Notably, 31.3% of embryos with a mosaic aberration reported in the original TE biopsy, revealed a euploid profile in the ICM and all three TE samples. Taken together, concordance between the ICM and all TE portions was established in 62.1% of blastocysts, across both embryo groups. Finally, we could not observe a significant effect of age on embryo mosaicism (P = 0.101 untested group; P = 0.7309 pretested group). Similarly, ICM and TE quality were not found to affect the occurrence of chromosomal mosaicism (P = 0.718 and P = 0.462 untested group; P = 1.000 and P = 0.2885 pretested group).Large Scale Data: All data that support the findings of this study are available online in Vivar (http://cmgg.be/vivar) upon request.Limitations, Reasons For Caution: Evaluating biological variation in some instances remains challenging. The technological limitations of sampling mitotic errors that lead to mosaicism, as well as WGA artefacts, warrant careful interpretation.Wider Implications Of the Findings: Our results highlight the complex nature of genetic (in)stability during early ontogenesis and indicate that blastocysts harbour a higher rate of chromosomal mosaicism than may have been anticipated. Moreover, our findings reveal an overall high diagnostic sensitivity and relatively low specificity in the context of PGT-A. This suggests that a considerable proportion of embryos are potentially being classified as clinically unsuitable. Ultimately, more precise quantification will benefit the clinical management of embryo mosaicism.Study Funding/competing Interest(s): M.P. is supported by the Special Research Fund, Bijzonder Onderzoeksfonds (BOF01D08114). J.T. and L.D. are supported by the agency for innovation through science (131673, 141441). B.H. and this research are supported by the Special Research Fund, Bijzonder Onderzoeksfonds (BOF15/GOA/011). The authors declare no competing interests.Trial Registration Number: Not applicable. [ABSTRACT FROM AUTHOR]

Published

2018

155. Effects of Bisphenol-A on proliferation and expression of genes related to synthesis of polyamines, interferon tau and insulin-like growth factor 2 by ovine trophectoderm cells.

Author

Elmetwally, Mohammed A., Halawa, Amal A., Lenis, Yasser Y., Tang, Wanjin, Wu, Guoyao, and Bazer, Fuller W.

Subjects

*BISPHENOL A, *GENE expression, *POLYAMINES, *ARGININE decarboxylase, *MESSENGER RNA

Abstract

This study evaluated the effects of bisphenol A (BPA) on proliferation of ovine trophectoderm (oTr1) cells, as well as expression of genes for transport of arginine and synthesis of polyamines. BPA reduced proliferation of oTr1 cells at concentrations of 1 × 10 −6 , 1 × 10 −5 , 1 × 10 −4  M compared to concentrations of 0, 1 × 10 −9 , and 1 × 10 −8  M at 24 and 96 h of culture. Lower concentrations of BPA significantly increased expression of mRNAs for agmatinase (AGMAT), arginine decarboxylase (ADC), ornithine decarboxylase (ODC1) and solute carrier family 7 member 1 (SLC7A1). Similarly, synthesis of polyamines by oTr1 cells was greatest at lower concentrations of BPA and decreased as the dose of BPA increased. Expression of mRNAs for interferon tau (IFNT) and insulin-like growth factor 2 (IGF2) by oTr1 cells was greater than for controls at 1 × 10 −9  M BPA. Overall, the effects of BPA on proliferation and gene expression by oTr1 cells were highly dose-dependent. [ABSTRACT FROM AUTHOR]

Published

2018

156. Self‐organization of human iPS cells into trophectoderm mimicking cysts induced by adhesion restriction using microstructured mesh scaffolds.

Author

Okeyo, Kennedy O., Tanabe, Maiko, Kurosawa, Osamu, Oana, Hidehiro, and Washizu, Masao

Subjects

*HUMAN embryology, *INDUCED pluripotent stem cells, *SELF-organizing systems, *CELL adhesion, *TISSUE scaffolds, *MICROSTRUCTURE

Abstract

Cellular dynamics leading to the formation of the trophectoderm in humans remain poorly understood owing to limited accessibility to human embryos for research into early human embryogenesis. Compared to animal models, organoids formed by self‐organization of stem cells in vitro may provide better insights into differentiation and complex morphogenetic processes occurring during early human embryogenesis. Here we demonstrate that modulating the cell culture microenvironment alone can trigger self‐organization of human induced pluripotent stem cells (hiPSCs) to yield trophectoderm‐mimicking cysts without chemical induction. To modulate the adhesion microenvironment, we used the mesh culture technique recently developed by our group, which involves culturing hiPSCs on suspended micro‐structured meshes with limited surface area for cell adhesion. We show that this adhesion‐restriction strategy can trigger a two‐stage self‐organization of hiPSCs; first into stem cell sheets, which express pluripotency signatures until around day 8–10, then into spherical cysts following differentiation and self‐organization of the sheet‐forming cells. Detailed morphological analysis using immunofluorescence microscopy with both confocal and two‐photon microscopes revealed the anatomy of the cysts as consisting of a squamous epithelial wall richly expressing E‐cadherin and CDX2. We also confirmed that the cysts exhibit a polarized morphology with basal protrusions, which show migratory behavior when anchored. Together, our results point to the formation of cysts which morphologically resemble the trophectoderm at the late‐stage blastocyst. Thus, the mesh culture microenvironment can initiate self‐organization of hiPSCs into trophectoderm‐mimicking cysts as organoids with potential application in the study of early embryogenesis and also in drug development. [ABSTRACT FROM AUTHOR]

Published

2018

157. Fosl1 overexpression directly activates trophoblast-specific gene expression programs in embryonic stem cells.

Author

Lee, Bum-Kyu, Uprety, Nadima, Jang, Yu Jin, Tucker, Scott K., Rhee, Catherine, LeBlanc, Lucy, Beck, Samuel, and Kim, Jonghwan

Abstract

During early development in placental mammals, proper trophoblast lineage development is essential for implantation and placentation. Defects in this lineage can cause early pregnancy failures and other pregnancy disorders. However, transcription factors controlling trophoblast development remain poorly understood. Here, we utilize Fosl1, previously implicated in trophoblast giant cell development as a member of the AP-1 complex, to trans-differentiate embryonic stem (ES) cells to trophoblast lineage-like cells. We first show that the ectopic expression of Fosl1 is sufficient to induce trophoblast-specific gene expression programs in ES cells. Surprisingly, we find that this transcriptional reprogramming occurs independently of changes in levels of ES cell core factors during the cell fate change. This suggests that Fosl1 acts in a novel way to orchestrate the ES to trophoblast cell fate conversion compared to previously known reprogramming factors. Mapping of Fosl1 targets reveals that Fosl1 directly activates TE lineage-specific genes as a pioneer factor. Our work suggests Fosl1 may be used to reprogram ES cells into differentiated cell types in trophoblast lineage, which not only enhances our knowledge of global trophoblast gene regulation but also may provide a future therapeutic tool for generating induced trophoblast cells from patient-derived pluripotent stem cells. [ABSTRACT FROM AUTHOR]

Published

2018

158. Enhanced Antigen Processing or Immune Evasion? West Nile Virus and the Induction of Immune Recognition Molecules

Author

King, Nicholas J. C., Davison, Ariane, Getts, Daniel R., Lu, David Ping, Getts, Meghann Teague, Yeung, Amanda, Peterson, James K., Kesson, Alison M., Fong, I. W., editor, and Diamond, Michael S.

Published

2009

159. Single-cell transcriptomic characterization of sheep conceptus elongation and implantation.

Author

Jia, Gong-Xue, Ma, Wen-Ji, Wu, Zhao-Bo, Li, Shuang, Zhang, Xiao-Qian, He, Zhen, Wu, Shi-Xin, Tao, Hai-Ping, Fang, Yi, Song, Yong-Wu, Xu, Shang-Rong, Wang, Xiao-Qun, and Yang, Qi-En

Abstract

Bidirectional communication between the developing conceptus and endometrium is essential for pregnancy recognition and establishment in ruminants. We dissect the transcriptomic dynamics of sheep conceptus and corresponding endometrium at pre- and peri-implantation stages using single-cell RNA sequencing. Spherical blastocysts contain five cell types, with 68.62% trophectoderm cells. Strikingly, elongated conceptuses differentiate into 17 cell types, indicating dramatic cell fate specifications. Cell-type-specific gene expression delineates the features of distinctive trophectoderm lineages and indicates that the transition from polar trophectoderm to trophoblast increases interferon-tau expression and likely drives elongation initiation. We identify 13 endometrium-derived cell types and elucidate their molecular responses to conceptus development. Integrated analyses uncover multiple paired transcripts mediating the dialogues between extraembryonic membrane and endometrium, including IGF2 - IGF1R , FGF19 - FGFR1 , NPY - NPY1R , PROS1 - AXL , and ADGRE5 - CD55. These data provide insight into the molecular regulation of conceptus elongation and represent a valuable resource for functional investigations of pre- and peri-implantation ruminant development. [Display omitted] • Transcriptome-based cell types are classified in sheep developing embryo/conceptus • Trophectoderm transition drives interferon-tau production and conceptus elongation • Cell-type-specific endometrial responses to conceptus development are elucidated • Ligand-receptor interactions between the conceptus and endometrium are demonstrated Jia et al. perform single-cell RNA sequencing analyses of sheep conceptus and corresponding endometrium at pre- and peri-implantation stages to elucidate the cell fate specifications and gene expression dynamics in conceptus elongation and implantation. Embryonic cell differentiation and uterine molecular responses to conceptus development are discussed. [ABSTRACT FROM AUTHOR]

Published

2023

160. The metaboloepigenetic regulation of preimplantation embryo development and fetal programming by ketone bodies

Author

Whatley, Emma Grace and Whatley, Emma Grace

Abstract

Diet-induced nutritional changes in the maternal reproductive tract elicit embryonic adaptations to maintain growth and survival, changes which nonetheless compromise long-term child and adult health via developmental programming. This is plausibly facilitated by metaboloepigenetic mechanisms, whereby metabolic sensing of nutrient availability coordinates epigenetic regulation of gene expression in a developmentally persistent manner, affecting short- and long-term embryo physiology and health. Despite little evidence for its efficacy and developmental safety, the very high fat, low carbohydrate ketogenic diet (KD) is increasing in popularity as a ‘fertility diet’ worldwide. In line with the hypothesis that metaboloepigenetics links diet with embryo health, KD consumption elevates systemic concentrations of the ketones beta-hydroxybutyrate (BOHB) and acetoacetate (AcAc), which in addition to their role as oxidative fuels, are epigenetic modifiers and may consequently affect embryo development. Therefore, to investigate the safety of a periconceptional KD for offspring health, it is necessary to determine the impact of ketones on the development, physiology, and viability of the preimplantation embryo. Using a mouse model, the impact of in vitro ketone exposure on preimplantation embryo development, physiology and viability was assessed. Exposure to BOHB alone perturbed blastocyst development, decreased glucose metabolism, and increased histone acetylation, predominantly impacting the trophectoderm cell lineage. This was further associated with implantation failure and delayed female fetal development post-transfer, suggesting preimplantation BOHB exposure is detrimental to development in a female-specific manner via a trophectoderm-mediated mechanism. Similarly, in vitro exposure to AcAc alone or AcAc + BOHB in combination did not impair morphological development of the blastocyst, however impacted glucose metabolism and cumulatively increased histone acetylation. P

Published

2022

161. Developmental stage and morphology of the competent blastocyst are associated with sex of the child but not with other obstetric outcomes:a multicenter cohort study

Author

Borgstrøm, M. B., Kesmodel, U. S., Klausen, T. W., Danielsen, A. K., Thomsen, T., Gabrielsen, A., Englund, A. L.M., Zedeler, A., Povlsen, B. B., Troest, B., Almind, G. J., Fedder, J., Kirk, J., Hindkjær, J., Lemmen, J. G., Petersen, K., Haahr, K., Petersen, M. R., Laursen, S., Knudsen, U. B., Bentin-Ley, U., Larsen, T., Grøndahl, M. I., Borgstrøm, M. B., Kesmodel, U. S., Klausen, T. W., Danielsen, A. K., Thomsen, T., Gabrielsen, A., Englund, A. L.M., Zedeler, A., Povlsen, B. B., Troest, B., Almind, G. J., Fedder, J., Kirk, J., Hindkjær, J., Lemmen, J. G., Petersen, K., Haahr, K., Petersen, M. R., Laursen, S., Knudsen, U. B., Bentin-Ley, U., Larsen, T., and Grøndahl, M. I.

Abstract

STUDY QUESTION: Are transfer day, developmental stage and morphology of the competent blastocyst in pregnancies leading to live birth associated with preterm birth, birthweight, length at birth and sex of the child? SUMMARY ANSWER: A high score in blastocyst developmental stage and in trophectoderm (TE) showed a significant association with the sex of the child, while no other associations with obstetric outcomes were observed. WHAT IS KNOWN ALREADY: The association between blastocyst assessment scores and obstetric outcomes have been reported in small single-center studies and the results are conflicting. STUDY DESIGN, SIZE, DURATION: Multicenter historical cohort study based on exposure data (transfer day (blastocyst developmental stage reached by Day 5 or Day 6)) blastocyst developmental stage (1–6) and morphology (TE and inner cell mass (ICM): A, B, C)) and outcome data (preterm birth, birthweight, length at birth, and sex of the child) from women undergoing single blastocyst transfer resulting in a singleton pregnancy and live birth. PARTICIPANTS/MATERIALS, SETTING, METHODS: Data from 16 private and university-based facilities for clinical services and research were used. A total of 7246 women, who in 2014–2018 underwent fresh-embryo transfer with a single blastocyst or frozen-thawed embryo transfer (FET) with a single blastocyst resulting in a singleton pregnancy were identified. Linking to the Danish Medical Birth Registry resulted in a total of 4842 women with a live birth being included. Cycles with pre-implantation genetic testing and donated gametes were excluded. The analyses were adjusted for female age (n ¼ 4842), female BMI (n ¼ 4302), female smoking (n ¼ 4290), parity (n ¼ 4365), infertility diagnosis (n ¼ 4765), type of treatment (n ¼ 4842) and center (n ¼ 4842); some analyses additionally included gestational age (n ¼ 4368) and sex of the child (n ¼ 4833). MAIN RESULTS AND THE ROLE OF CHANCE: No statistically significant associations between bla

Published

2022

162. Mesenchymal Stem Cells in Embryo-Maternal Communication under Healthy Conditions or Viral Infections: Lessons from a Bovine Model

Author

Ministerio de Ciencia e Innovación (España), Ministerio para la Transición Ecológica y el Reto Demográfico (España), Fundación Biodiversidad, European Commission, Ramírez, Miguel Ángel [0000-0002-5868-2134], Calle, Alexandra, Ramírez, Miguel Ángel, Ministerio de Ciencia e Innovación (España), Ministerio para la Transición Ecológica y el Reto Demográfico (España), Fundación Biodiversidad, European Commission, Ramírez, Miguel Ángel [0000-0002-5868-2134], Calle, Alexandra, and Ramírez, Miguel Ángel

Abstract

Bovine mesenchymal stem cells are a relevant cell population found in the maternal reproductive tract that exhibits the immunomodulation capacity required to prevent embryo rejection. The phenotypic plasticity showed by both endometrial mesenchymal stem cells (eMSC) and embryonic trophoblast through mesenchymal to epithelial transition and epithelial to mesenchymal transition, respectively, is essential for embryo implantation. Embryonic trophoblast maintains active crosstalk via EVs and soluble proteins with eMSC and peripheral blood MSC (pbMSC) to ensure the retention of eMSC in case of pregnancy and induce the chemotaxis of pbMSC, critical for successful implantation. Early pregnancy-related proteins and angiogenic markers are detected as cargo in EVs and the soluble fraction of the embryonic trophectoderm secretome. The pattern of protein secretion in trophectoderm-EVs changes depending on their epithelial or mesenchymal phenotype and due to the uptake of MSC EVs. However, the changes in this EV-mediated communication between maternal and embryonic MSC populations infected by viruses that cause abortions in cattle are poorly understood. They are critical in the investigation of reproductive viral pathologies.

Published

2022

163. A developmental insurance policy

Author

Nestor Saiz and Anna-Katerina Hadjantonakis

Subjects

inner cell mass, trophectoderm, cell fate, preimplantation, cell plasticity, Medicine, Science, Biology (General), QH301-705.5

Abstract

Why does a totipotent state linger within the inner cell mass of mouse embryos?

Published

2017

164. Position- and Hippo signaling-dependent plasticity during lineage segregation in the early mouse embryo

Author

Eszter Posfai, Sophie Petropoulos, Flavia Regina Oliveira de Barros, John Paul Schell, Igor Jurisica, Rickard Sandberg, Fredrik Lanner, and Janet Rossant

Subjects

inner cell mass, trophectoderm, cell fate, preimplantation, cell plasticity, Medicine, Science, Biology (General), QH301-705.5

Abstract

The segregation of the trophectoderm (TE) from the inner cell mass (ICM) in the mouse blastocyst is determined by position-dependent Hippo signaling. However, the window of responsiveness to Hippo signaling, the exact timing of lineage commitment and the overall relationship between cell commitment and global gene expression changes are still unclear. Single-cell RNA sequencing during lineage segregation revealed that the TE transcriptional profile stabilizes earlier than the ICM and prior to blastocyst formation. Using quantitative Cdx2-eGFP expression as a readout of Hippo signaling activity, we assessed the experimental potential of individual blastomeres based on their level of Cdx2-eGFP expression and correlated potential with gene expression dynamics. We find that TE specification and commitment coincide and occur at the time of transcriptional stabilization, whereas ICM cells still retain the ability to regenerate TE up to the early blastocyst stage. Plasticity of both lineages is coincident with their window of sensitivity to Hippo signaling.

Published

2017

165. The role of BMP4 signaling in trophoblast emergence from pluripotency

Author

R. Michael Roberts, Toshihiko Ezashi, Jasmine Temple, Joseph R. Owen, Francesca Soncin, and Mana M. Parast

Subjects

Pluripotent Stem Cells, Biochemistry & Molecular Biology, Physiology, Placenta, Trophoblast stem cells, 1.1 Normal biological development and functioning, Clinical Sciences, Bone Morphogenetic Protein 4, Regenerative Medicine, Article, Cellular and Molecular Neuroscience, Mice, Pregnancy, Underpinning research, Animals, Humans, Naive pluripotency, Molecular Biology, Cytotrophoblast, Pharmacology, Pediatric, Epiblast, Bone Morphogenetic Protein, Cell Differentiation, Cell Biology, Stem Cell Research, Naïve pluripotency, Trophoblasts, Primed pluripotency, Molecular Medicine, Trophectoderm, Female, Inner cell mass, Stem Cell Research - Nonembryonic - Non-Human, Biochemistry and Cell Biology, Signal Transduction

Abstract

The Bone Morphogenetic Protein (BMP) signaling pathway has established roles in early embryonic morphogenesis, particularly in the epiblast. More recently, however, it has also been implicated in development of extraembryonic lineages, including trophectoderm (TE), in both mouse and human. In this review, we will provide an overview of this signaling pathway, with a focus on BMP4, and its role in emergence and development of TE in both early mouse and human embryogenesis. Subsequently, we will build on these in vivo data and discuss the utility of BMP4-based protocols for in vitro conversion of primed vs. naïve pluripotent stem cells (PSC) into trophoblast, and specifically into trophoblast stem cells (TSC). PSC-derived TSC could provide an abundant, reproducible, and ethically acceptable source of cells for modeling placental development.

Published

2022

166. Requirement for expression of WW domain containing transcription regulator 1 in bovine trophectoderm development

Author

Shota Yamamura, Masashi Takahashi, Hanako Bai, Shun Saito, Nanami Kohri, and Manabu Kawahara

Subjects

0301 basic medicine, Hippo pathway, Biophysics, Embryonic Development, WWTR1, Biology, Biochemistry, WW Domains, WW domain, 03 medical and health sciences, 0302 clinical medicine, medicine, Animals, Inner cell mass, RNA, Messenger, Blastocyst, RNA, Small Interfering, Molecular Biology, Adaptor Proteins, Signal Transducing, Hippo signaling pathway, Gene knockdown, Cell growth, Gene Expression Regulation, Developmental, Cell Differentiation, Embryo, Cell Biology, Trophoblasts, Cell biology, 030104 developmental biology, medicine.anatomical_structure, Differentiation, 030220 oncology & carcinogenesis, embryonic structures, Oocytes, biology.protein, Trophectoderm, Cattle, Female

Abstract

WW domain-containing transcription regulator 1 (WWTR1) is one of the primary effectors in the Hippo pathway, which plays essential roles in cell differentiation into trophectoderm (TE) and inner cell mass cell lineages at the blastocyst stage. However, little is known about the roles of WWTR1 in preimplantation development. The present study aimed to explore the significance of WWTR1 expression in preimplantation development using an mRNA knockdown (KD) system in bovine embryos. We first quantitated WWTR1 expression at protein and mRNA levels from fertilization to blastocyst stage. WWTR1 proteins gradually shifted from extranuclear localization during the 16-cell stage to nuclear localization by morula stage. WWTR1 mRNA expression was also transiently upregulated at the 16-cell stage. WWTR1 KD efficiently repressed WWTR1 expression at protein and mRNA levels. The WWTR1 KD embryos developed to the blastocyst stage at rates equivalent to those of controls, but TE cell numbers were significantly decreased. Representative TE-expressed genes, including CDX2 and IFNT were also significantly decreased in WWTR1 KD blastocysts. These results provide the first demonstration that WWTR1 expression is responsible for normal TE cell development in preimplantation embryos. (c) 2021 Elsevier Inc. All rights reserved.

Published

2021

167. Trophectoderm

Author

Gross, Isabelle and Schwab, Manfred, editor

Published

2017

168. GATA2/3-TFAP2A/C transcription factor network couples human pluripotent stem cell differentiation to trophectoderm with repression of pluripotency.

Author

Krendl, Christian, Shaposhnikov, Dmitry, Rishko, Valentyna, Ori, Chaido, Ziegenhain, Christoph, Sass, Steffen, Simon, Lukas, Müller, Nikola S., Straub, Tobias, Brooks, Kelsey E., Chavez, Shawn L., Enard, Wolfgang, Theis, Fabian J., and Drukker, Micha

Subjects

*PLURIPOTENT stem cells, *GATA proteins, *EPIGENOMICS, *GENETIC transcription, *EMBRYOLOGY, *CPG nucleotides, *DNA methylation

Abstract

To elucidate the molecular basis of BMP4-induced differentiation of human pluripotent stem cells (PSCs) toward progeny with trophectoderm characteristics, we produced transcriptome, epigenome H3K4me3, H3K27me3, and CpG methylation maps of trophoblast progenitors, purified using the surface marker APA. We combined them with the temporally resolved transcriptome of the preprogenitor phase and of single APA+ cells. This revealed a circuit of bivalent TFAP2A, TFAP2C, GATA2, and GATA3 transcription factors, coined collectively the "trophectoderm four" (TEtra), which are also present in human trophectoderm in vivo. At the onset of differentiation, the TEtra factors occupy multiple sites in epigenetically inactive placental genes and in OCT4. Functional manipulation of GATA3 and TFAP2A indicated that they directly couple trophoblast-specific gene induction with suppression of pluripotency. In accordance, knocking down GATA3 in primate embryos resulted in a failure to form trophectoderm. The discovery of the TEtra circuit indicates how trophectoderm commitment is regulated in human embryogenesis. [ABSTRACT FROM AUTHOR]

Published

2017

169. Stem cell factor-induced AKT cell signaling pathway: Effects on porcine trophectoderm and uterine luminal epithelial cells.

Author

Jeong, Wooyoung, Jung, Seoungo, Bazer, Fuller W., and Kim, Jinyoung

Subjects

*STEM cell factor, *PROTEIN kinase B, *CELL communication, *EPITHELIAL cells, *ENDOMETRIUM

Abstract

Stem cell factor (SCF) is a multipotent growth factor that elicits diverse biological actions in various aspects of embryogenesis and animal development. The aim of the present study was to assess SCF-induced intracellular signaling and cellular activities in porcine trophectoderm (pTr) and uterine luminal epithelial (pLE) cells which are well known as useful to elucidate developmental events. SCF induced abundances of p-AKT, p-P70RSK and RPS6 proteins in pTr cells reached to their maximum, and then returned to basal levels by 120 min. In pLE cells, SCF induced protracted effect to increase AKT phosphorylation which was well correlated with the time course for P70RSK and RPS6 phosphorylation. LY294002 (an inhibitor of AKT) decreased SCF-induced p-AKT, p-P70RSK and p-RPS6 proteins. Also, immunofluorescence analyses revealed that p-RPS6 was abundant within the cytoplasm of SCF-treated cells, but p-RPS6 was present only at basal levels in cells treated with LY294002. In the presence of LY294002, both SCF-stimulated transient and sustained AKT phosphorylation were inhibited in pLE cells. Furthermore, SCF increased migration of pTr and pLE cells, but LY294002 significantly reduced this effect of SCF. In conclusion, results of the present study suggest that SCF secreted by the endometrium induces autocrine/paracrine signaling responses that stimulate migration of pTr and pLE cells through activation of the AKT cell signaling pathway. Those results support the hypothesis that SCF is a critical regulatory factor for conceptus development and implantation during pregnancy in pigs. [ABSTRACT FROM AUTHOR]

Published

2017

170. Isolation and characterization of the trophectoderm from the Arabian camel (Camelus dromedarius).

Author

Saadeldin, Islam M., Swelum, Ayman Abdel-Aziz, Elsafadi, Mona, Moumen, Abdullah F., Alzahrani, Faisal A., Mahmood, Amer, Alfayez, Musaad, and Alowaimer, Abdullah N.

Abstract

We isolated and characterized trophoblast from in vivo-derived camel embryos and compared with embryonic stem-like cells. Camel embryos were flushed on day 8 post-insemination and used to derive trophectoderm and embryonic stem-like cells under feeder-free culture conditions using a basement membrane matrix. Embryos were evaluated for the expression of POU5F1, MYC, KLF4, SOX2, CDX2, and KRT8 mRNA transcripts by relative quantitative polymerase chain reaction. Camel embryos grew and expanded to ∼4.5 mm and maintained their vesicular shape in vitro for 21 days post-insemination. Trophoblast and embryonic stem-like cell lines grew under feeder-free culture conditions and showed distinct morphological criteria and normal chromosomal counts. Embryonic stem-like cells showed positive staining in the alkaline phosphatase reaction. Trophoblast cells showed a significant increase in CDX2, KRT8, KLF4, and SOX2 expression compared with embryonic stem-like cells and whole embryos. Embryonic stem-like cells showed a significant decrease in CDX2 expression and increase in SOX2 and KRT8 expression compared to embryonic expression. POU5F1 and MYC expression showed no difference between embryos and both cell lines. We characterized embryo survival in vitro, particularly the derivation of trophectoderm and embryonic stem-like cells, providing a foundation for further analysis of early embryonic development and placentation in camels. [ABSTRACT FROM AUTHOR]

Published

2017

171. Actions of activin A, connective tissue growth factor, hepatocyte growth factor and teratocarcinoma-derived growth factor 1 on the development of the bovine preimplantation embryo.

Author

Kannampuzha-Francis, Jasmine, Tribulo, Paula, and Hansen, Peter J.

Subjects

*ACTIVIN, *HEPATOCYTE growth factor, *TERATOCARCINOMA, *BOS, *BLASTOCYST, *GENE expression, *REPRODUCTION, *CATTLE

Abstract

The reproductive tract secretes bioactive molecules collectively known as embryokines that can regulate embryonic growth and development. In the present study we tested four growth factors expressed in the endometrium for their ability to modify the development of the bovine embryo to the blastocyst stage and alter the expression of genes found to be upregulated (bone morphogenetic protein 15 (BMP15) and keratin 8, type II (KRT8)) or downregulated (NADH dehydrogenase 1 (ND1) and S100 calcium binding protein A10 (S100A10)) in embryos competent to develop to term. Zygotes were treated at Day 5 with 0.01, 0.1 or 1.0nM growth factor. The highest concentration of activin A increased the percentage of putative zygotes that developed to the blastocyst stage. Connective tissue growth factor (CTGF) increased the number of cells in the inner cell mass (ICM), decreased the trophectoderm : ICM ratio and increased blastocyst expression of KRT8 and ND1. The lowest concentration of hepatocyte growth factor (HGF) reduced the percentage of putative zygotes becoming blastocysts. Teratocarcinoma-derived growth factor 1 increased total cell number at 0.01nM and expression of S100A10 at 1.0 nM, but otherwise had no effects. Results confirm the prodevelopmental actions of activin A and indicate that CTGF may also function as an embryokine by regulating the number of ICM cells in the blastocyst and altering gene expression. Low concentrations of HGF were inhibitory to development. [ABSTRACT FROM AUTHOR]

Published

2017

172. Identification of Novel Placentally Expressed Aspartic Proteinase in Humans.

Author

Majewska, Marta, Lipka, Aleksandra, Panasiewicz, Grzegorz, Gowkielewicz, Marek, Jozwik, Marcin, Krzysztof Majewski, Mariusz, and Szafranska, Bozena

Subjects

*ASPARTIC proteinases, *ANTISENSE DNA, *PLACENTA, *RNA sequencing, *GENOMES

Abstract

This study presents pioneering data concerning the human pregnancy-associated glycoprotein-Like family, identified in the genome, of the term placental transcriptome and proteome. RNA-seq allowed the identification of 1364 bp hPAG-L/pep cDNA with at least 56.5% homology with other aspartic proteinases (APs). In silico analyses revealed 388 amino acids (aa) of full-length hPAG-L polypeptide precursor, with 15 aa-signal peptide, 47 aa-blocking peptide and 326 aa-mature protein, and two Asp residues (D), specific for a catalytic cleft of the APs (VVFDTGSSNLWV91-102 and AIVDTGTSLLTG274-285). Capillary sequencing identified 9330 bp of the hPAG-L gene (Gen Bank Acc. No. KX533473), composed of nine exons and eight introns. Heterologous Western blotting revealed the presence of one dominant 60 kDa isoform of the hPAG-L amongst cellular placental proteins. Detection with anti-pPAG-P and anti-Rec pPAG2 polyclonals allowed identification of the hPAG-L proteins located within regions of chorionic villi, especially within the syncytiotrophoblast of term singleton placentas. Our novel data extend the present knowledge about the human genome, as well as placental transcriptome and proteome during term pregnancy. Presumably, this may contribute to establishing a new diagnostic tool for examination of some disturbances during human pregnancy, as well as growing interest from both scientific and clinical perspectives. [ABSTRACT FROM AUTHOR]

Published

2017

173. Tissue organization alters gene expression in equine induced trophectoderm cells.

Author

Reinholt, Brad M., Bradley, Jennifer S., Jacobs, Robert D., Ealy, Alan D., and Johnson, Sally E.

Subjects

*PREGNANCY, *GENE expression, *BLASTOCYST, *CELLULAR signal transduction, *LIGAND binding (Biochemistry), *PHYSIOLOGY

Abstract

Rapid morphological and gene expression changes occur during the early formation of a mammalian blastocyst. Critical to successful retention of the blastocyst and pregnancy is a functional trophectoderm (TE) that supplies the developing embryo with paracrine factors and hormones. The contribution of TE conformational changes to gene expression was examined in equine induced trophoblast (iTr) cells. Equine iTr cells were cultured as monolayers or in suspension to form spheres. The spheres are hollow and structurally reminiscent of native equine blastocysts. Total RNA was isolated from iTr monolayers and spheres and analyzed by RNA sequencing. An average of 32.2 and 31 million aligned reads were analyzed for the spheres and monolayers, respectively. Forty-four genes were unique to monolayers and 45 genes were expressed only in spheres. Conformation did not affect expression of CDX2 , POU5F1 , TEAD4 , ETS2 , ELF3 , GATA2 or TFAP2A , the core gene network of native TE. Bioinformatic analysis was used to identify classes of genes differentially expressed in response to changes in tissue shape. In both iTr spheres and monolayers, the majority of the differentially expressed genes were associated with binding activity in cellular, developmental and metabolic processes. Inherent to protein:protein interactions, several receptor-ligand families were identified in iTr cells with enrichment of genes coding for PI3-kinase and MAPK signaling intermediates. Our results provide evidence for ligand initiated kinase signaling pathways that underlie early trophectoderm structural changes. [ABSTRACT FROM AUTHOR]

Published

2017

174. Sex differences in rat placental development: from pre-implantation to late gestation.

Author

Kalisch-Smith, J. I., Simmons, D. G., Pantaleon, M., and Moritz, K. M.

Subjects

*PLACENTA development, *SEXUAL dimorphism, *GESTATIONAL age

Abstract

Background: A male fetus is suggested to be more susceptible to in utero and birth complications. This may be due in part to altered morphology or function of the XY placenta. We hypothesised that sexual dimorphism begins at the blastocyst stage with sex differences in the progenitor trophectoderm (TE) and its derived trophoblast lineages, as these cells populate the majority of cell types within the placenta. We investigated sex-specific differences in cell allocation in the pre-implantation embryo and further characterised growth and gene expression of the placental compartments from the early stages of the definitive placenta through to late gestation. Methods: Naturally mated Sprague Dawley dams were used to collect blastocysts at embryonic day (E) 5 to characterise cell allocation; total, TE, and inner cell mass (ICM), and differentiation to downstream trophoblast cell types. Placental tissues were collected at E13, E15, and E20 to characterise volumes of placental compartments, and sex-specific gene expression profiles. Results: Pre-implantation embryos showed no sex differences in cell allocation (total, TE and ICM) or early trophoblast differentiation, assessed by outgrowth area, number and ploidy of trophoblasts and P-TGCs, and expression of markers of trophoblast stem cell state or differentiation. Whilst no changes in placental structures were found in the immature E13 placenta, the definitive E15 placenta from female fetuses had reduced labyrinthine volume, fetal and maternal blood space volume, as well as fetal blood space surface area, when compared to placentas from males. No differences between the sexes in labyrinth trophoblast volume or interhaemal membrane thickness were found. By E20 these sex-specific placental differences were no longer present, but female fetuses weighed less than their male counterparts. Coupled with expression profiles from E13 and E15 placental samples may suggest a developmental delay in placental differentiation. Conclusions: Although there were no overt differences in blastocyst cell number or early placental development, reduced growth of the female labyrinth in mid gestation is likely to contribute to lower fetal weight in females at E20. These data suggest sex differences in fetal growth trajectories are due at least in part, to differences in placenta growth. [ABSTRACT FROM AUTHOR]

Published

2017

175. Overexpression of Trophoblast Stem Cell-Enriched MicroRNAs Promotes Trophoblast Fate in Embryonic Stem Cells.

Author

Nosi, Ursula, Lanner, Fredrik, Huang, Tsu, and Cox, Brian

Abstract

Summary The first cell fate choice of the preimplantation embryo generates the extraembryonic trophoblast and embryonic epiblast lineages. Embryonic stem cells (ESCs) and trophoblast stem cells (TSCs) can be utilized to investigate molecular mechanisms of this first cell fate decision. It has been established that ESCs can be induced to acquire trophoblast lineage characteristics upon manipulation of lineage-determining transcription factors. Here, we have interrogated the potential of microRNAs (miRNAs) to drive trans-differentiation of ESCs into the trophoblast lineage. Analysis of gene expression data identified a network of TSC-enriched miRNAs that were predicted to target mRNAs enriched in ESCs. Ectopic expression of these miRNAs in ESCs resulted in a stable trophoblast phenotype, supported by gene expression changes and in vivo contribution potential. This process is highly miRNA-specific and dependent on Hdac2 inhibition. Our experimental evidence suggests that these miRNAs promote a mural trophectoderm (TE)-like cell fate with physiological properties that differentiate them from the polar TE. [ABSTRACT FROM AUTHOR]

Published

2017

176. Current experience concerning mosaic embryos diagnosed during preimplantation genetic screening.

Author

Harton, Gary L., Cinnioglu, Cengiz, and Fiorentino, Francesco

Subjects

*MOSAIC diseases, *EMBRYOS, *PREIMPLANTATION genetic diagnosis, *CELL lines, *ANEUPLOIDY, *PREIMPLANTATION genetic diagnosis & ethics, *GENETIC testing & ethics, *CHROMOSOME abnormalities, *EMBRYO transfer, *GENETIC counseling, *MOSAICISM, *EVIDENCE-based medicine, *GENETIC testing, *FETAL development, *ETHICS, *PREVENTION

Abstract

The concept of embryos containing multiple cell lines (mosaicism) is not new, but much attention has been paid to this concept recently owing to recent advances in molecular techniques to analyze human embryos. Mosaicism in embryos has been known and reported for some time, originally in early cleavage-stage embryos diagnosed with the use of fluorescence in situ hybridization (FISH). However, the early data have come under attack owing to the limited ability of FISH to reliably detect the actual copy number count of chromosomes as well as potential ascertainment bias of those early studies, which were all performed on already analyzed embryos found to be aneuploid. More recent molecular techniques for analyzing embryos have allowed scientists to really begin to understand mosaic embryos, and to now transfer and follow this class of embryo. Indeed, it could be said that three classes of embryos now exist after preimplantation genetic screening: euploid, aneuploid, and mosaic aneuploid. This paper attempts to bring to light the latest data on mosaic embryos and to understand how clinicians and others will deal with this issue today and in the future. Finally, an attempt is made to look to other fields of genetics to understand how this important issue can be dealt with as a group much better than any one individual group may be able to. [ABSTRACT FROM AUTHOR]

Published

2017

177. Mosaicism between trophectoderm and inner cell mass.

Author

Capalbo, Antonio and Rienzi, Laura

Subjects

*MOSAICISM, *ECTODERM, *DISEASE prevalence, *BLASTOCYST, *ANEUPLOIDY, *CHROMOSOME abnormalities, *EMBRYO transfer, *GENETIC counseling, *PREIMPLANTATION genetic diagnosis, *GENETIC testing, *FETAL development, *PREVENTION

Abstract

Defining the actual incidence and prevalence of mosaicism in human blastocysts still remains a difficult task. The small amount of evidence generated by animal and human studies does not support the existence of mechanisms involved in developmental arrest, clonal depletion, or aneuploidy rescue for abnormal cells in euploid/aneuploid embryos during preimplantation development. However, studies in humans are mainly descriptive and lack functional evidence. Understanding the biological mechanisms that beset preimplantation differentiation holds the potential to reveal the role of aneuploidies and gene dosage imbalances in cell fate decision, providing important clues on the origin and evolution of embryonic mosaicism. The evidence on human blastocysts suggests that a mosaic euploid/aneuploid configuration is detected in around 5% of embryos. This figure supports the extremely low level of mosaicism reported in natural and IVF pregnancies. Similarly, the clinical management of patterns consistent with the presence of mosaicism in a trophectoderm biopsy during preimplantation genetic diagnosis cycles (PGD-A) is still a controversial issue. Despite the facts that some contemporary comprehensive chromosomal screening platforms can detect mosaic samples in cell mixture models with variable accuracy and many reproductive genetics laboratories are now routinely including embryonic mosaicism on their genetic reports, a diagnosis of certainty for mosaicism in PGD-A cycles is conceptually impracticable. Indeed, several technical and biological sources of errors clearly exist when trying to estimate mosaicism from a single trophectoderm biopsy in PGD-A cycles and must be understood to adequately guide patients during clinical care. [ABSTRACT FROM AUTHOR]

Published

2017

178. Magnesium chloride and polyamine can differentiate mouse embryonic stem cells into trophectoderm or endoderm.

Author

Tanase, Jun-ichi, Yokoo, Takehiro, Matsumura, Yuuki, Kinoshita, Makoto, Kikuchi, Yo, Suemori, Hirofumi, and Ohyama, Takashi

Subjects

*EMBRYONIC stem cells, *CELL differentiation, *ENDODERM, *MAGNESIUM chloride, *POLYAMINES, *CHROMATIN, *LABORATORY mice

Abstract

Magnesium chloride and polyamines stabilize DNA and chromatin. Furthermore, they can induce nucleosome aggregation and chromatin condensation in vitro . To determine the effects of elevating the cation concentrations in the nucleus of a living cell, we microinjected various concentrations of mono-, di- and polyvalent cation solutions into the nuclei of mouse embryonic stem (ES) cells and traced their fates. Here, we show that an elevation of either MgCl 2 , spermidine or spermine concentration in the nucleus exerts a significant effect on mouse ES cells, and can differentiate a certain population of the cells into trophectoderm, a lineage that mouse ES cells do not normally generate, or endoderm. It is hypothesized that the cell differentiation was most probably caused by the condensation of chromatin including the Oct3/4 locus, which was induced by the elevated concentrations of these cations. [ABSTRACT FROM AUTHOR]

Published

2017

179. Activities for leptin in bovine trophoblast cells.

Author

Hughes, C.K., Xie, M.M., McCoski, S.R., and Ealy, A.D.

Subjects

*CATTLE physiology, *LEPTIN, *TROPHOBLAST, *METALLOPROTEINASES, *CELL proliferation

Abstract

Leptin is involved in various reproductive processes in humans and rodents, including placental development and function. The specific ways that leptin influences placental development and function in cattle are poorly understood. This work was completed to explore how leptin regulates hormone, cytokine and metalloprotease transcript abundance, and cell proliferation in cultured bovine trophoblast cells. In the first set of studies, cells were cultured in the presence of graded recombinant bovine leptin concentrations (0, 10, 50, 250 ng/mL) for 6 or 24 h. Transcript profiles were examined from extracted RNA. Leptin supplementation did not affect abundance of the maternal recognition of pregnancy factor, interferon-tau ( IFNT ), but leptin increased ( P < 0.05) abundance of chorionic somatomammotropin hormone 2 ( CSH2 ; ie, placental lactogen) at both 6 and 24 h at each concentration tested. At 24 h, the greatest CSH2 abundance ( P < 0.05) was detected in cells supplemented with 50 ng/mL leptin. Transcript abundance of the remodeling factor, metalloprotease 2 ( MMP2 ), was greater ( P < 0.05) in leptin-treated cells at 24 h but not at 6 h. The 24 h MMP2 response was greatest ( P < 0.05) at 250 ng/mL. Transcript abundance for MMP9 was not altered by leptin treatment. In a separate set of studies, cell proliferation assays were completed. Leptin supplementation did not affect bovine trophoblast cell line proliferation at any dose tested. In conclusion, leptin supplementation did not affect bovine trophoblast cell proliferation or IFNT expression, but leptin increases CSH2 and MMP2 transcript abundance. Both of these factors are involved with peri-implantation and postimplantation placental development and function, and this implicates leptin as a potential mediator of early placental development and function in cattle. [ABSTRACT FROM AUTHOR]

Published

2017

180. hnRNPL expression dynamics in the embryo and placenta.

Author

Mathew, Vineetha, Mei, Ariel, Giwa, Hamida, Cheong, Agnes, Chander, Ashmita, Zou, Aaron, Blanton, Robert M., Kashpur, Olga, Cui, Wei, Slonim, Donna, Mahmoud, Taysir, O'Tierney-Ginn, Perrie, Mager, Jesse, Draper, Isabelle, and Wallingford, Mary C.

Subjects

*TROPHOBLAST, *EMBRYO implantation, *PLACENTA, *RNA-binding proteins, *ALTERNATIVE RNA splicing, *EMBRYOS

Abstract

Heterogeneous nuclear ribonucleoprotein L (hnRNPL) is a conserved RNA binding protein (RBP) that plays an important role in the alternative splicing of gene transcripts, and thus in the generation of specific protein isoforms. Global deficiency in hnRNPL in mice results in preimplantation embryonic lethality at embryonic day (E) 3.5. To begin to understand the contribution of hnRNPL-regulated pathways in the normal development of the embryo and placenta, we determined hnRNPL expression profile and subcellular localization throughout development. Proteome and Western blot analyses were employed to determine hnRNPL abundance between E3.5 and E17.5. Histological analyses supported that the embryo and implantation site display distinct hnRNPL localization patterns. In the fully developed mouse placenta, nuclear hnRNPL was observed broadly in trophoblasts, whereas within the implantation site a discrete subset of cells showed hnRNPL outside the nucleus. In the first-trimester human placenta, hnRNPL was detected in the undifferentiated cytotrophoblasts, suggesting a role for this factor in trophoblast progenitors. Parallel in vitro studies utilizing Htr8 and Jeg3 cell lines confirmed expression of hnRNPL in cellular models of human trophoblasts. These studies [support] coordinated regulation of hnRNPL during the normal developmental program in the mammalian embryo and placenta. [ABSTRACT FROM AUTHOR]

Published

2023

181. Establishment of bovine trophoblast stem cells.

Author

Wang, Yinjuan, Ming, Hao, Yu, Leqian, Li, Jie, Zhu, Linkai, Sun, Hai-Xi, Pinzon-Arteaga, Carlos A., Wu, Jun, and Jiang, Zongliang

Abstract

Here, we report that a chemical cocktail (LCDM: leukemia inhibitory factor [LIF], CHIR99021, dimethinedene maleate [DiM], minocycline hydrochloride), previously developed for extended pluripotent stem cells (EPSCs) in mice and humans, enables de novo derivation and long-term culture of bovine trophoblast stem cells (TSCs). Bovine TSCs retain developmental potency to differentiate into mature trophoblast cells and exhibit transcriptomic and epigenetic (chromatin accessibility and DNA methylome) features characteristic of trophectoderm cells from early bovine embryos. The bovine TSCs established in this study will provide a model to study bovine placentation and early pregnancy failure. [Display omitted] • LCDM enables the derivation of bovine TSCs from blastocysts • Bovine TSCs have the capacity to give rise to two types of functional trophoblast cells • Bovine TSCs exhibit transcriptomic and epigenetic features of primary trophoblast cells Wang et al. establish bovine trophoblast stem cells (bTSCs) from blastocysts. They show that bTSCs retain developmental potency to differentiate into mature trophoblast cells and exhibit transcriptomic and epigenetic features characteristic of trophectoderm cells from early bovine embryos. [ABSTRACT FROM AUTHOR]

Published

2023

182. Uterine WNTS modulates fibronectin binding activity required for blastocyst attachment through the WNT/CA 2+ signaling pathway in mice.

Author

Lou Y, Pinel L, and Dufort D

Subjects

Animals, Mice, Female, Phosphatidylinositol 3-Kinases, Blastocyst, Wnt Signaling Pathway, Integrins, Fibronectins, Calcium-Calmodulin-Dependent Protein Kinase Type 2

Abstract

Adhesion of the implanting blastocyst involves the interaction between integrin proteins expressed by trophoblast cells and components present in the basement membrane of the endometrial luminal epithelium. Although several factors regulating integrins and their adhesion to fibronectin are already known, we showed that Wnt signaling is involved in the regulation of blastocyst adhesion through the trafficking of integrins expressed by trophoblast cells. Localization of Itgα5β1 by immunofluorescence and FN-binding assays were conducted on peri-implantation blastocysts treated with either Wnt5a or Wnt7a proteins. Both Wnt5a and Wnt7a induced a translocation of Itgα5β1 at the surface of the blastocyst and an increase in FN-binding activity. We further demonstrated that uterine fluid is capable of inducing integrin translocation and this activity can be specifically inhibited by the Wnt inhibitor sFRP2. To identify the Wnt signaling pathway involved in this activity, blastocysts were incubated with inhibitors of either p38MAPK, PI3K pathway or CamKII prior to the addition of Wnts. Whereas inhibition of p38MAPK and PI3K had not effect, inhibition of CamKII reduced FN-binding activity induced by Wnts. Finally, we demonstrated that inhibition of Wnts by sFRP2 reduced the binding efficiency of the blastocyst to uterine epithelial cells. Our findings provide new insight into the mechanism that regulates integrin trafficking and FN-binding activity and identifies Wnts as a key player in blastocyst attachment to the uterine epithelium., (© 2023. BioMed Central Ltd., part of Springer Nature.)

Published

2023

183. insideOutside: an accessible algorithm for classifying interior and exterior points, with applications in embryology.

Author

Strawbridge SE, Kurowski A, Corujo-Simon E, Fletcher AN, Nichols J, and Fletcher AG

Subjects

Animals, Mice, Cell Nucleus, Blastocyst, Cell Differentiation, Algorithms, Biological Science Disciplines

Abstract

A crucial aspect of embryology is relating the position of individual cells to the broader geometry of the embryo. A classic example of this is the first cell-fate decision of the mouse embryo, where interior cells become inner cell mass and exterior cells become trophectoderm. Fluorescent labelling, imaging, and quantification of tissue-specific proteins have advanced our understanding of this dynamic process. However, instances arise where these markers are either not available, or not reliable, and we are left only with the cells' spatial locations. Therefore, a simple, robust method for classifying interior and exterior cells of an embryo using spatial information is required. Here, we describe a simple mathematical framework and an unsupervised machine learning approach, termed insideOutside, for classifying interior and exterior points of a three-dimensional point-cloud, a common output from imaged cells within the early mouse embryo. We benchmark our method against other published methods to demonstrate that it yields greater accuracy in classification of nuclei from the pre-implantation mouse embryos and greater accuracy when challenged with local surface concavities. We have made MATLAB and Python implementations of the method freely available. This method should prove useful for embryology, with broader applications to similar data arising in the life sciences., Competing Interests: Competing interests The authors declare no competing or financial interests., (© 2023. Published by The Company of Biologists Ltd.)

Published

2023

184. 3D-cultured blastoids model human embryogenesis from pre-implantation to early gastrulation stages.

Author

Karvas RM, Zemke JE, Ali SS, Upton E, Sane E, Fischer LA, Dong C, Park KM, Wang F, Park K, Hao S, Chew B, Meyer B, Zhou C, Dietmann S, and Theunissen TW

Subjects

Humans, Embryo, Mammalian, Blastocyst, Epithelial Cells, Gastrulation, Embryo Implantation

Abstract

Naive human pluripotent stem cells have the remarkable ability to self-organize into blastocyst-like structures ("blastoids") that model lineage segregation in the pre-implantation embryo. However, the extent to which blastoids can recapitulate the defining features of human post-implantation development remains unexplored. Here, we report that blastoids cultured on thick three-dimensional (3D) extracellular matrices capture hallmarks of early post-implantation development, including epiblast lumenogenesis, rapid expansion and diversification of trophoblast lineages, and robust invasion of extravillous trophoblast cells by day 14. Extended blastoid culture results in the localized activation of primitive streak marker TBXT and the emergence of embryonic germ layers by day 21. We also show that the modulation of WNT signaling alters the balance between epiblast and trophoblast fates in post-implantation blastoids. This work demonstrates that 3D-cultured blastoids offer a continuous and integrated in vitro model system of human embryonic and extraembryonic development from pre-implantation to early gastrulation stages., Competing Interests: Declaration of interests R.M.K. and T.W.T. are co-inventors on a patent application related to the extended culture of human blastoids on 3D matrices., (Copyright © 2023 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2023

185. CircKDM5B sponges miR-128 to regulate porcine blastocyst development by modulating trophectoderm barrier function.

Author

Gao D, Wang X, Yan YL, Li C, Tan YP, Liu QC, Zhang MY, Zhang JV, Sun QY, Cao ZB, and Zhang YH

Subjects

Animals, Humans, Mice, Embryo, Mammalian, Embryonic Development genetics, Gene Expression Regulation, Developmental, Mammals genetics, Swine, Jumonji Domain-Containing Histone Demethylases genetics, Blastocyst metabolism, MicroRNAs genetics, MicroRNAs metabolism, RNA, Circular genetics, RNA, Circular metabolism

Abstract

Circular RNAs (circRNAs), which exert critical functions in the regulation of transcriptional and post-transcriptional gene expression, are found in mammalian cells but their functions in mammalian preimplantation embryo development remain poorly understood. Here, we showed that circKDM5B mediated miRNA-128 (miR-128) to regulate porcine early embryo development. We screened circRNAs potentially expressed in porcine embryos through an integrated analysis of sequencing data from mouse and human embryos, as well as porcine oocytes. An authentic circRNA originating from histone demethylase KDM5B (referred to as circKDM5B) was abundantly expressed in porcine embryos. Functional studies revealed that circKDM5B knockdown not only significantly reduced blastocyst formation but also decreased the number of total cells and trophectoderm (TE) cells. Moreover, the knockdown of circKDM5B resulted in the disturbance of tight junction assembly and impaired paracellular sealing within the TE epithelium. Mechanistically, miR-128 inhibitor injection could rescue the early development of circKDM5B knockdown embryos. Taken together, the findings revealed that circKDM5B functions as a miR-128 sponge, thereby facilitating early embryonic development in pigs through the modulation of gene expression linked to tight junction assembly., (© The Author(s) 2023. Published by Oxford University Press on behalf of European Society of Human Reproduction and Embryology. All rights reserved. For permissions, please email: journals.permissions@oup.com.)

Published

2023

186. Conjugated linoleic acid supplementation changes prostaglandin concentration ratio and alters the expression of genes involved in maternal-fetal recognition from bovine trophoblast cells in vitro.

Author

Bueno Cordeiro Maldonado M, de Castro Lourenço V, de Oliveira Bezerra L, Feltrin IR, Mendes AF, Rocha CC, Pugliesi G, Ealy AD, Membrive CMB, and Nogueira MFG

Subjects

Pregnancy, Female, Cattle, Animals, Dinoprost pharmacology, Dinoprost metabolism, Trophoblasts metabolism, Dinoprostone metabolism, Dietary Supplements, Prostaglandins, Linoleic Acids, Conjugated pharmacology

Abstract

Early embryonic mortality caused by maternal-fetal recognition failure in the three weeks after fertilization represents a major cause of reproductive inefficiency in the cattle industry. Modifying the amounts and ratios of prostaglandin (PG) F 2α and PGE 2 can benefit the establishment of pregnancy in cattle. Adding conjugated linoleic acid (CLA) to endometrial and fetal cells culture affects PG synthesis, but its effect on bovine trophoblast cells (CT-1) is unknown. The aim of this study was to determine the effects of CLA (a mixture of cis- and trans-9, 11- and -10,12-octadecadienoic acids) on PGE 2 and PGF 2α synthesis and the expression of transcripts involved with maternal-fetal recognition of bovine trophectoderm. Cultures of CT-1 were exposed to CLA for 24, 48 and 72 h. Transcript abundance was determined by qRT-PCR and hormone profiles were quantified by ELISA. The PGE 2 and PGF 2α concentrations were reduced in the culture medium of CLA-exposed CT-1 compared to that of unexposed cells. Furthermore, CLA supplementation increased the PGE 2 :PGF 2α ratio in CT-1 and had a quadratic effect (P < 0.05) on the relative expression of MMP9, PTGES2, and PTGER4. The relative expression levels of PTGER4 were reduced (P < 0.05) in CT-1 cultured with 100 μM CLA than in the unsupplemented and 10 μM-CLA groups. Treatment of CT-1 with CLA decreased PGE 2 and PGF 2α synthesis but a biphasic effect of CLA was observed on the PGE 2 :PGF 2α ratio and relative abundance of transcripts with 10 μM CLA providing maximal improvements in each endpoint. Our data suggest that CLA may influence eicosanoid metabolic process and extracellular matrix remodeling., Competing Interests: Declaration of competing interest The authors have declared that no competing interests exist., (Copyright © 2023 Elsevier Inc. All rights reserved.)

Published

2023

187. Lineage segregation in human pre-implantation embryos is specified by YAP1 and TEAD1.

Author

Regin M, Essahib W, Demtschenko A, Dewandre D, David L, Gerri C, Niakan KK, Verheyen G, Tournaye H, Sterckx J, Sermon K, and Van De Velde H

Subjects

Pregnancy, Female, Humans, Mice, Animals, Embryonic Development physiology, Transcription Factors genetics, Embryo, Mammalian metabolism, TEA Domain Transcription Factors, Actins metabolism, Blastocyst metabolism

Abstract

Study Question: Which processes and transcription factors specify the first and second lineage segregation events during human preimplantation development?, Summary Answer: Differentiation into trophectoderm (TE) cells can be initiated independently of polarity; moreover, TEAD1 and YAP1 co-localize in (precursor) TE and primitive endoderm (PrE) cells, suggesting a role in both the first and the second lineage segregation events., What Is Known Already: We know that polarity, YAP1/GATA3 signalling and phospholipase C signalling play a key role in TE initiation in compacted human embryos, however, little is known about the TEAD family of transcription factors that become activated by YAP1 and, especially, whether they play a role during epiblast (EPI) and PrE formation. In mouse embryos, polarized outer cells show nuclear TEAD4/YAP1 activity that upregulates Cdx2 and Gata3 expression while inner cells exclude YAP1 which upregulates Sox2 expression. The second lineage segregation event in mouse embryos is orchestrated by FGF4/FGFR2 signalling which could not be confirmed in human embryos; TEAD1/YAP1 signalling also plays a role during the establishment of mouse EPI cells., Study Design, Size, Duration: Based on morphology, we set up a development timeline of 188 human preimplantation embryos between Day 4 and 6 post-fertilization (dpf). The compaction process was divided into three subgroups: embryos at the start (C0), during (C1), and at the end (C2) of, compaction. Inner cells were identified as cells that were entirely separated from the perivitelline space and enclosed by cellular contacts on all sides. The blastulation process was divided into six subgroups, starting with early blastocysts with sickle-cell shaped outer cells (B0) and further on, blastocysts with a cavity (B1). Full blastocysts (B2) showed a visible ICM and outer cells referred to as TE. Further expanded blastocysts (B3) had accumulated fluid and started to expand due to TE cell proliferation and zona pellucida (ZP) thinning. The blastocysts then significantly expanded further (B4) and started to hatch out of the ZP (B5) until they were fully hatched (B6)., Participants/materials, Setting, Methods: After informed consent and the expiration of the 5-year cryopreservation duration, 188 vitrified high quality eight-cell stage human embryos (3 dpf) were warmed and cultured until the required stages were reached. We also cultured 14 embryos that were created for research until the four- and eight-cell stage. The embryos were scored according to their developmental stage (C0-B6) displaying morphological key differences, rather than defining them according to their chronological age. They were fixed and immunostained for different combinations of cytoskeleton (F-actin), polarization (p-ERM), TE (GATA3), EPI (NANOG), PrE (GATA4 and SOX17), and members of the Hippo signalling pathway (YAP1, TEAD1 and TEAD4). We choose these markers based on previous observations in mouse embryos and single cell RNA-sequencing data of human embryos. After confocal imaging (LSM800, Zeiss), we analysed cell numbers within each lineage, different co-localization patterns and nuclear enrichment., Main Results and the Role of Chance: We found that in human preimplantation embryos compaction is a heterogeneous process that takes place between the eight-cell to the 16-cell stages. Inner and outer cells are established at the end of the compaction process (C2) when the embryos contain up to six inner cells. Full apical p-ERM polarity is present in all outer cells of compacted C2 embryos. Co-localization of p-ERM and F-actin increases steadily from 42.2% to 100% of the outer cells, between C2 and B1 stages, while p-ERM polarizes before F-actin (P < 0.00001). Next, we sought to determine which factors specify the first lineage segregation event. We found that 19.5% of the nuclei stain positive for YAP1 at the start of compaction (C0) which increases to 56.1% during compaction (C1). At the C2 stage, 84.6% of polarized outer cells display high levels of nuclear YAP1 while it is absent in 75% of non-polarized inner cells. In general, throughout the B0-B3 blastocyst stages, polarized outer/TE cells are mainly positive for YAP1 and non-polarized inner/ICM cells are negative for YAP1. From the C1 stage onwards, before polarity is established, the TE marker GATA3 is detectable in YAP1 positive cells (11.6%), indicating that differentiation into TE cells can be initiated independently of polarity. Co-localization of YAP1 and GATA3 increases steadily in outer/TE cells (21.8% in C2 up to 97.3% in B3). Transcription factor TEAD4 is ubiquitously present throughout preimplantation development from the compacted stage onwards (C2-B6). TEAD1 displays a distinct pattern that coincides with YAP1/GATA3 co-localization in the outer cells. Most outer/TE cells throughout the B0-B3 blastocyst stages are positive for TEAD1 and YAP1. However, TEAD1 proteins are also detected in most nuclei of the inner/ICM cells of the blastocysts from cavitation onwards, but at visibly lower levels as compared to that in TE cells. In the ICM of B3 blastocysts, we found one main population of cells with NANOG+/SOX17-/GATA4- nuclei (89.1%), but exceptionally we found NANOG+/SOX17+/GATA4+ cells (0.8%). In seven out of nine B3 blastocysts, nuclear NANOG was found in all the ICM cells, supporting the previously reported hypothesis that PrE cells arise from EPI cells. Finally, to determine which factors specify the second lineage segregation event, we co-stained for TEAD1, YAP1, and GATA4. We identified two main ICM cell populations in B4-6 blastocysts: the EPI (negative for the three markers, 46.5%) and the PrE (positive for the three markers, 28.1%) cells. We conclude that TEAD1 and YAP1 co-localise in (precursor) TE and PrE cells, indicating that TEAD1/YAP1 signalling plays a role in the first and the second lineage segregation events., Limitations, Reasons for Caution: In this descriptive study, we did not perform functional studies to investigate the role of TEAD1/YAP1 signalling during the first and second lineage segregation events., Wider Implications of the Findings: Our detailed roadmap on polarization, compaction, position and lineage segregation events during human preimplantation development paves the way for further functional studies. Understanding the gene regulatory networks and signalling pathways involved in early embryogenesis could ultimately provide insights into why embryonic development is sometimes impaired and facilitate the establishment of guidelines for good practice in the IVF lab., Study Funding/competing Interests: This work was financially supported by Wetenschappelijk Fonds Willy Gepts (WFWG) of the University Hospital UZ Brussel (WFWG142) and the Fonds Wetenschappelijk Onderzoek-Vlaanderen (FWO, G034514N). M.R. is doctoral fellow at the FWO. The authors have no conflicts of interest to declare., Trial Registration Number: N/A., (© The Author(s) 2023. Published by Oxford University Press on behalf of European Society of Human Reproduction and Embryology. All rights reserved. For permissions, please email: journals.permissions@oup.com.)

Published

2023

188. Systematic mapping and modeling of 3D enhancer-promoter interactions in early mouse embryonic lineages reveal regulatory principles that determine the levels and cell-type specificity of gene expression.

Author

Murphy D, Salataj E, Di Giammartino DC, Rodriguez-Hernaez J, Kloetgen A, Garg V, Char E, Uyehara CM, Ee LS, Lee U, Stadtfeld M, Hadjantonakis AK, Tsirigos A, Polyzos A, and Apostolou E

Abstract

Mammalian embryogenesis commences with two pivotal and binary cell fate decisions that give rise to three essential lineages, the trophectoderm (TE), the epiblast (EPI) and the primitive endoderm (PrE). Although key signaling pathways and transcription factors that control these early embryonic decisions have been identified, the non-coding regulatory elements via which transcriptional regulators enact these fates remain understudied. To address this gap, we have characterized, at a genome-wide scale, enhancer activity and 3D connectivity in embryo-derived stem cell lines that represent each of the early developmental fates. We observed extensive enhancer remodeling and fine-scale 3D chromatin rewiring among the three lineages, which strongly associate with transcriptional changes, although there are distinct groups of genes that are irresponsive to topological changes. In each lineage, a high degree of connectivity or "hubness" positively correlates with levels of gene expression and enriches for cell-type specific and essential genes. Genes within 3D hubs also show a significantly stronger probability of coregulation across lineages, compared to genes in linear proximity or within the same contact domains. By incorporating 3D chromatin features, we build a novel predictive model for transcriptional regulation (3D-HiChAT), which outperformed models that use only 1D promoter or proximal variables in predicting levels and cell-type specificity of gene expression. Using 3D-HiChAT, we performed genome-wide in silico perturbations to nominate candidate functional enhancers and hubs in each cell lineage, and with CRISPRi experiments we validated several novel enhancers that control expression of one or more genes in their respective lineages. Our study comprehensively identifies 3D regulatory hubs associated with the earliest mammalian lineages and describes their relationship to gene expression and cell identity, providing a framework to understand lineage-specific transcriptional behaviors., Competing Interests: Conflict of interest statement The authors declare that the above study was conducted in the absence of any commercial, financial, or personal relationships that could have appeared to influence the work reported in this article. All authors have approved the submitted version.

Published

2023

189. Inconclusive results in preimplantation genetic testing: go for a second biopsy?

Author

Parriego, Monica, Coll, Lluc, Vidal, Francesca, Boada, Montserrat, Devesa, Marta, Coroleu, Buenaventura, and Veiga, Anna

Subjects

*GENETIC testing, *BIOPSY, *BLASTOCYST, *CHILDBIRTH

Abstract

The transition in biopsy timing from blastomere to trophectoderm biopsy has led to a remarkable decrease in the percentage of undiagnosed blastocysts. However, patients with few or no euploid blastocysts can be affected by this residual percentage of diagnosis failure. The aim of this study is to assess whether blastocyst rebiopsy and revitrification is an efficient and safe procedure to be applied in cases of no results after analysis. Fifty-three patients agreed to the warming of 61 blastocysts to perform a second biopsy and PGT-A by aCGH. Only 75.4% of the blastocysts survived, reexpanded, and could be rebiopsied. After the second biopsy and analysis, 95.6% of the blastocysts were successfully diagnosed with an euploidy rate of 65.9%. Eighteen euploid blastocysts were warmed and transferred to 18 patients with a 100% survival and reexpansion rate. Seven clinical pregnancies have been achieved with 4 live births, 1 ongoing pregnancy, and 2 miscarriages. Thus, although few transfers of rebiopsied and revitrified blastocysts have been performed till date, our preliminary results show that this approach is efficient and safe to be applied for undiagnosed blastocysts, as it ultimately allows the transfer of euploid blastocysts and good clinical outcomes. [ABSTRACT FROM AUTHOR]

Published

2019

190. The role of RHOA signaling in trophectoderm cell-fate decision in cattle

Author

Hiroki Akizawa, Manabu Kawahara, Nanami Kohri, Sakie Iisaka, Hanako Bai, and Masashi Takahashi

Subjects

0301 basic medicine, RHOA activity, RHOA, Biophysics, Fertilization in Vitro, Cell fate determination, Biochemistry, Embryo Culture Techniques, 03 medical and health sciences, 0302 clinical medicine, Pregnancy, Ectoderm, medicine, Animals, Inner cell mass, Blastocyst, Hippo signaling pathway, Molecular Biology, Transcription factor, YAP1, biology, Bovine, Cell Biology, Embryonic stem cell, Cell biology, 030104 developmental biology, medicine.anatomical_structure, Differentiation, 030220 oncology & carcinogenesis, embryonic structures, biology.protein, Trophectoderm, Cattle, Female, rhoA GTP-Binding Protein, Signal Transduction

Abstract

Mammalian blastocysts are composed of two distinct cell lineages, namely the inner cell mass (ICM) and trophectoderm (TE). TE cells that give rise to the embryonic placenta are marked by an exclusive expression of the key determinant transcription factor, CDX2. Although Hippo signaling pathway is known to be responsible for this TE-specific expression of CDX2, the upstream regulator of this pathway in mammalian embryos is still controversial. In the present study, the involvement of the small molecular G protein, RHOA, in TE cell-fate decision in cattle was investigated. Inhibition of RHOA by the specific inhibitor, C3 transferase (C3), severely impaired the blastocyst formation. Further, C3 treatment significantly decreased the number of blastomeres with nuclearized YAP1, the prominent effector of Hippo pathway. An artificial isolation of ICM cells from blastocysts followed by the continuing culture to regenerate TE cells was conducted and showed that TE re-emergence from the isolated ICM is governed by Hippo pathway and suppressed by C3 treatment like that observed in developing embryos. Finally, the long-term exposure to C3 suggests the presence of alternative regulators of CDX2 expression other than RHOA signaling because there were still CDX2-positive cells after C3 treatment. These results demonstrated that RHOA signaling plays a significant role in TE cell-fate decision by regulating Hippo pathway in cattle. (C) 2020 Elsevier Inc. All rights reserved.

Published

2020

191. An economic analysis of preimplantation genetic testing for aneuploidy by polar body biopsy in advanced maternal age

Author

J.P.M. Geraedts, Wolfgang Rudolph-Rothfeld, V. Goossens, K van der Ven, Mònica Parriego, Andreas G. Schmutzler, K Neumann, Georg Griesinger, Patrick M.M. Bossuyt, Joanne Traeger-Synodinos, Karen Sermon, Reinhard Vonthein, Epidemiology and Data Science, APH - Methodology, APH - Personalized Medicine, Basic (bio-) Medical Sciences, Reproduction and Genetics, Materials and Chemistry, Faculty of Physical Education and Physical Therapy, Klinische Genetica, and RS: FHML non-thematic output

Subjects

Adult, medicine.medical_specialty, Cost effectiveness, Cost-Benefit Analysis, Population, Polar Bodies, ESTEEM trial, Miscarriage, Genetic Testing/economics, Polar Bodies/transplantation, medicine, Humans, array CGH, TROPHECTODERM, Polar body biopsy, Abortion, Spontaneous/genetics, Genetic Testing, Advanced maternal age, education, cost-effectiveness, Preimplantation Diagnosis, health care economics and organizations, Genetic testing, education.field_of_study, medicine.diagnostic_test, Obstetrics, business.industry, Obstetrics and Gynecology, Aneuploidy, medicine.disease, abortion, Abortion, Spontaneous, EXPECTANT, Pregnancy rate, polar body biopsy, PREGNANCY, IVF, Preimplantation Diagnosis/economics, Female, preimplantation genetic testing, business, Live birth, Maternal Age

Abstract

Objective: What are the cost per live birth and the incremental cost of preventing a miscarriage with preimplantation genetic testing for aneuploidy (PGT-A) by polar body biopsy and array-based comprehensive genome hybridisation (aCGH) versus regular IVF/ICSI without PGT-A for infertility treatment in women 36–40 years of age?. Design: Decision tree model. Population: A randomised clinical trial on PGT-A (ESTEEM study). Methods: Two treatment strategies were compared: one cycle of IVF/ICSI with or without PGT-A. Costs and effects were analysed with this model for four different cost scenarios: high-, higher medium, lower medium and low-cost. Base case, sensitivity, threshold, and probabilistic sensitivity analyses were used to examine the cost-effectiveness implications of PGT-A. Results: PGT-A increased the cost per live birth by approximately 15% in the high-cost scenario to approximately 285% in the low-cost scenario. Threshold analysis revealed that PGT-A would need to be associated with an absolute increase in pregnancy rate by 6% to >39% or, alternatively, would need to be US$2,969 (high-cost scenario) to US$4,888 (low-cost scenario) cheaper. The incremental cost to prevent one miscarriage by PGT-A using the base case assumptions was calculated to be US$34,427 (high-cost scenario) to US$51,146 (low-cost scenario). A probabilistic sensitivity analysis showed cost-effectiveness for PGT-A from 1.9% (high-cost scenario) to 0.0% (low-cost scenario) of calculated samples. Conclusions: While avoiding unnecessary embryo transfers and miscarriages are important goals, patients and doctors need to be aware of the high-cost implications of applying PGT-A using aCGH on polar bodies. Tweetable abstract: PGT-A by polar body biopsy and comprehensive genome hybridisation increases cost per live birth and requires high financial spending per miscarriage averted.

Published

2020

192. Cell differentiation events in pre-implantation mouse and bovine embryos

Author

Carreiro, Letícia Escobar, dos Santos, Gabriel Siqueira, Luedke, Felipe Eduardo, and Goissis, Marcelo Demarchi

Subjects

General Veterinary, blastocyst, embryonic structures, Animal Science and Zoology, embryogenesis, Review Article, EMBRIOGÊNESE ANIMAL, inner cell mass, trophectoderm, early development

Abstract

Early mammal embryogenesis starts with oocyte fertilization, giving rise to the zygote. The events that the newly formed zygote surpasses are crucial to the embryo developmental success. Shortly after activation of its genome, cells of the embryo segregate into the inner cell mass (ICM) or the trophectoderm (TE). The first will give rise to the embryo while the latter will become the placenta. This first segregation involves cellular and molecular processes that include cell polarity linked to intracellular pathway activation, which will regulate the transcription of trophectoderm-related genes. Then, cells of the ICM undergo the second event of mammalian cell differentiation, which consists of the separation between epiblast (EPI) and hypoblast or primitive endoderm (PrE). This second segregation involves paracrine signaling, leading to differential expression of key genes that will dictate the fate of the cell. Although these processes are described in detail in the mouse, recent studies suggest that the bovine embryo could also be an interesting model for early development, since there are differences to the mouse and similarities with early human embryogenesis. In this review, we gathered the main data available in the literature upon bovine and mouse early development events, suggesting that both models should be analyzed and studied in a complementary way, to better model early events occurring in human development.

Published

2022

193. The trophectoderm acts as a niche for the inner cell mass through C/EBPα-regulated IL-6 signaling

Author

Marcos Plana-Carmona, Gregoire Stik, Romain Bulteau, Carolina Segura-Morales, Noelia Alcázar, Chris D.R. Wyatt, Antonios Klonizakis, Luisa de Andrés-Aguayo, Maxime Gasnier, Tian V. Tian, Guillem Torcal Garcia, Maria Vila-Casadesús, Nicolas Plachta, Manuel Serrano, Mirko Francesconi, Thomas Graf, Institut Català de la Salut, [Plana-Carmona M, Stik G, Segura-Morales C] Gene Regulation, Stem Cells and Cancer Program, Centre for Genomic Regulation (CRG), The Barcelona Institute of Science and Technology (BIST), Barcelona, Spain. Universitat Pompeu Fabra (UPF), Barcelona, Spain. [Bulteau R] Laboratoire de Biologie et Modélisation de la Cellule, Université de Lyon, Lyon, France. [Alcázar N] Institute for Research in Biomedicine (IRB Barcelona), The Barcelona Institute of Science and Technology, Barcelona, Spain. Vall d’Hebron Institute of Oncology (VHIO), Barcelona, Spain. [Wyatt CDR] Gene Regulation, Stem Cells and Cancer Program, Centre for Genomic Regulation (CRG), The Barcelona Institute of Science and Technology (BIST), Barcelona, Spain. Universitat Pompeu Fabra (UPF), Barcelona, Spain. Department of Genetics, Evolution & Environment, University College London, London, UK. [Tian TV] Gene Regulation, Stem Cells and Cancer Program, Centre for Genomic Regulation (CRG), The Barcelona Institute of Science and Technology (BIST), Barcelona, Spain. Universitat Pompeu Fabra (UPF), Barcelona, Spain. Vall d’Hebron Institute of Oncology (VHIO), Barcelona, Spain. [Vila-Casadesús M] Gene Regulation, Stem Cells and Cancer Program, Centre for Genomic Regulation (CRG), The Barcelona Institute of Science and Technology (BIST), Barcelona, Spain. Vall d’Hebron Institute of Oncology (VHIO), Barcelona, Spain, and Vall d'Hebron Barcelona Hospital Campus

Subjects

Embryology, factores biológicos::péptidos y proteínas de señalización intercelular::citocinas::interleucinas::interleucina-6 [COMPUESTOS QUÍMICOS Y DROGAS], INNER CELL MASS, Embryonic Development, Pre-implantation embryo development, Biochemistry, Morula, Interleucina-6, Genetics, CCAAT-Enhancer-Binding Protein-alpha, TRANSDIFFERENTIATION, Gene Regulation, Physiological Phenomena::Growth and Development::Morphogenesis::Embryonic and Fetal Development::Embryonic Development [PHENOMENA AND PROCESSES], Fisiologia cel·lular, Transdifferentiation, C/EBP transcription factor, Embriologia, Interleukin-6, somatic cell reprogramming, Cell Biology, Gene regulation, Blastocyst, pre-implantation embryo development, Biological Factors::Intercellular Signaling Peptides and Proteins::Cytokines::Interleukins::Interleukin-6 [CHEMICALS AND DRUGS], estructuras embrionarias::mórula [ANATOMÍA], Trophectoderm, IL-6 signaling, Inner cell mass, Embryonic Structures::Morula [ANATOMY], fenómenos fisiológicos::crecimiento y desarrollo::morfogénesis::desarrollo embrionario y fetal::desarrollo embrionario [FENÓMENOS Y PROCESOS], Somatic cell reprogramming, Developmental Biology

Abstract

Gene regulation; Somatic cell reprogramming; Trophectoderm Regulación de genes; Reprogramación de células somáticas; Trofoectodermo Regulació de gens; Reprogramació de cèl·lules somàtiques; Trofectoderma IL-6 has been shown to be required for somatic cell reprogramming into induced pluripotent stem cells (iPSCs). However, how Il6 expression is regulated and whether it plays a role during embryo development remains unknown. Here, we describe that IL-6 is necessary for C/EBPα-enhanced reprogramming of B cells into iPSCs but not for B cell to macrophage transdifferentiation. C/EBPα overexpression activates both Il6 and Il6ra genes in B cells and in PSCs. In embryo development, Cebpa is enriched in the trophectoderm of blastocysts together with Il6, while Il6ra is mostly expressed in the inner cell mass (ICM). In addition, Il6 expression in blastocysts requires Cebpa. Blastocysts secrete IL-6 and neutralization of the cytokine delays the morula to blastocyst transition. The observed requirement of C/EBPα-regulated IL-6 signaling for pluripotency during somatic cell reprogramming thus recapitulates a physiologic mechanism in which the trophectoderm acts as niche for the ICM through the secretion of IL-6. We thank C. Berenguer for help with B cell reprogramming and bone marrow collection; S. Nakagawa and B. Pernaute for advice on pre-implantation embryo culture and manipulation, and Kyle M. Loh for his valuable discussions; the flow cytometry and microscopy units of UPF-CRG for technical assistance; the CRG genomics core facility for sequencing and Graf laboratory members for critical discussions. Work in the laboratory of T.G. was supported by the Spanish Ministry of Economy, Industry and Competitiveness (Plan Estatal PID2019-109354GB-I00), the CRG, AGAUR (SGR 726), and a European Research Council Synergy grant (4D-Genome). M.P.-C. was supported by an FPI fellowship (BES-2016-076900). Work in the laboratory of M.S. was funded by the IRB and by grants from the Spanish Ministry of Economy co-funded by the European Regional Development Fund (SAF2017-82613-R), ERC (ERC-2014-AdG/669622), la Caixa Foundation, and Secretaria d’Universitats i Recerca del Departament d’Empresa i Coneixement of Catalonia (Grup de Recerca consolidat 2017 SGR 282).

Published

2022

194. mTOR-regulated translation during first the wave of inner cell generation in mouse preimplantation embryos

Author

ČERNÁ, Pavlína

Subjects

mTOR signalling pathway, epiblast, mouse preimplantation development, trophectoderm, primitive endoderm

Abstract

The aim of this master thesis was to investigate the role of mTOR and connected pathways in early mouse preimplantation development.

Published

2022

195. NuRD-dependent DNA methylation prevents ES cells from accessing a trophectoderm fate

Author

Paulina A. Latos, Christine Helliwell, Olukunbi Mosaku, Dominika A. Dudzinska, Bryony Stubbs, Maria Berdasco, Manel Esteller, and Brian Hendrich

Subjects

Stem cells, NuRD, DNA methylation, Trophectoderm, Chromatin, Science, Biology (General), QH301-705.5

Abstract

Summary Embryonic Stem (ES) cells are able to give rise to the three germ layers of the embryo but are prevented from contributing to the trophoblast. The molecular nature of this barrier between embryonic and trophectodermal cell fates is not clear, but is known to involve DNA methylation. Here we demonstrate that the Nucleosome Remodeling and Deacetylation (NuRD) co-repressor complex maintains the developmental barrier between embryonic and trophectodermal cell fates by maintaining transcriptional silencing of trophectoderm determinant genes in ES cells. We further show that NuRD activity facilitates DNA methylation of several of its target promoters, where it acts non-redundantly with DNA methylation to enforce transcriptional silencing. NuRD-deficient ES cells fail to completely silence expression of the trophectoderm determinant genes Elf5 and Eomes, but this alone is not sufficient to induce transdifferentiation towards the trophectoderm fate. Rather this leaves ES cells capable of activating expression of trophectoderm-specific genes in response to appropriate extracellular signals, enabling them to commit to a trophectodermal cell fate. Our findings clarify the molecular nature of the developmental barrier between the embryonic and trophoblast cell fates, and establish a role for NuRD activity in specifying sites for de novo DNA methylation.

Published

2012

196. The function of BMP signaling and dynamic transcription factor gene expression in pre-implantation mouse development

Author

Reyes de Mochel, Nabora Soledad

Subjects

Developmental biology, Blastocyst, BMP signaling, Expression noise, Inner Cell Mass, Pre-implantation, Trophectoderm

Abstract

Mammals are tasked with the unique process of forming trophectodermal lineages that are essential for in utero implantation. During pre-implantation stages the fertilized egg becomes the blastocyst by dividing and subsequently segregating cells into two distinct lineages, the inner cell mass (ICM) and the trophectoderm (TE). This apparently simple developmental process is sophisticated, with transcription factors, signaling networks, cell shape and relative position within the embryo each contributing to normal development of the pre-implantation embryo. Much of our current understanding of the molecular control of blastocyst formation is based on manipulating single genes, such as transcription factors and components of signaling networks, to explore their function in the process. The focus of the experiments described in this thesis was to investigate the function of bone morphogenetic protein (BMP) signaling in development of the mouse blastocyst. I demonstrate that BMP signaling is active beginning at the 4-cell stage of mouse development and persists until late blastocyst stage. Importantly, functional analysis using genetic and pharmacologic approaches identified a novel role for the regulation of the cell cycle by BMP signaling during mouse pre-implantation development. A second major question addressed in this dissertation is how robustness is generated in the developmental process of the pre-implantation mouse embryo. A systems biology approach was used to perform computational simulations of pre-implantation stages that uncover novel design principles employed by the early mouse embryo. These models support the hypothesis that expression noise improves the ability of the cells of the early pre-implantation mouse embryo to differentiate in an appropriate manner.

Published

2016

197. Developmental stage and morphology of the competent blastocyst are associated with sex of the child but not with other obstetric outcomes:a multicenter cohort study

Author

M B Borgstrøm, U S Kesmodel, T W Klausen, A K Danielsen, T Thomsen, A Gabrielsen, A L M Englund, A Zedeler, B B Povlsen, B Troest, G J Almind, J Fedder, J Kirk, J Hindkjær, J G Lemmen, K Petersen, K Haahr, M R Petersen, S Laursen, U B Knudsen, U Bentin-Ley, T Larsen, and M I Grøndahl

Subjects

length at birth, Male, sex of the child, Cohort Studies, Pregnancy, morphology, Humans, Embryo Transfer/methods, reproductive and urinary physiology, obstetric outcome, Retrospective Studies, Rehabilitation, Infant, Newborn, Obstetrics and Gynecology, preterm birth, inner cell mass, Embryo Transfer, developmental stage, Blastocyst, Reproductive Medicine, birthweight, embryonic structures, Premature Birth, competent blastocyst, Female, trophectoderm

Abstract

STUDY QUESTION Are transfer day, developmental stage and morphology of the competent blastocyst in pregnancies leading to live birth associated with preterm birth, birthweight, length at birth and sex of the child? SUMMARY ANSWER A high score in blastocyst developmental stage and in trophectoderm (TE) showed a significant association with the sex of the child, while no other associations with obstetric outcomes were observed. WHAT IS KNOWN ALREADY The association between blastocyst assessment scores and obstetric outcomes have been reported in small single-center studies and the results are conflicting. STUDY DESIGN, SIZE, DURATION Multicenter historical cohort study based on exposure data (transfer day (blastocyst developmental stage reached by Day 5 or Day 6)) blastocyst developmental stage (1–6) and morphology (TE and inner cell mass (ICM): A, B, C)) and outcome data (preterm birth, birthweight, length at birth, and sex of the child) from women undergoing single blastocyst transfer resulting in a singleton pregnancy and live birth. PARTICIPANTS/MATERIALS, SETTING, METHODS Data from 16 private and university-based facilities for clinical services and research were used. A total of 7246 women, who in 2014–2018 underwent fresh-embryo transfer with a single blastocyst or frozen-thawed embryo transfer (FET) with a single blastocyst resulting in a singleton pregnancy were identified. Linking to the Danish Medical Birth Registry resulted in a total of 4842 women with a live birth being included. Cycles with pre-implantation genetic testing and donated gametes were excluded. The analyses were adjusted for female age (n = 4842), female BMI (n = 4302), female smoking (n = 4290), parity (n = 4365), infertility diagnosis (n = 4765), type of treatment (n = 4842) and center (n = 4842); some analyses additionally included gestational age (n = 4368) and sex of the child (n = 4833). MAIN RESULTS AND THE ROLE OF CHANCE No statistically significant associations between blastocyst assessment scores (transfer day, developmental stage, TE, ICM) and preterm birth (8.3%) or birthweight (mean 3461.7 g) were found. The adjusted association between blastocysts with a TE score of C and a TE score of A and length at birth (mean 51.6 cm) were statistically significant (adjusted mean difference 0.4 cm (95% CI: 0.02; 0.77)). Blastocysts transferred with developmental stage score 5 compared to blastocysts transferred with score 3 had a 34% increased probability of being a boy (odds ratio (OR) 1.34 (95% CI: 1.09; 1.64). Further, TE score B blastocysts compared to TE score A blastocysts had a 31% reduced probability of being a boy (OR 0.69 (95% CI: 0.60; 0.80)). LIMITATIONS, REASONS FOR CAUTION It is possible that some residual confounding remains. WIDER IMPLICATIONS OF THE FINDINGS Blastocyst selection during ART does not appear to introduce any negative effects on obstetric outcome. Therefore, clinicians and patients can be reassured that the assessment scores of the selected blastocyst will not in themselves pose a risk of preterm birth or affect birthweight and the length at birth. STUDY FUNDING/COMPETING INTEREST(S) Unrestricted grant from Gedeon Richter Nordics AB, Sweden. None of the authors have any competing interest to declare. TRIAL REGISTRATION NUMBER N/A.

Published

2021

198. Early differentiation and gene expression characteristics of trophoblast lineages†.

Author

Qin J, Li W, Lv B, Xue Z, and Xue J

Subjects

Animals, Pregnancy, Female, Humans, Placenta metabolism, Placentation genetics, Cell Differentiation genetics, Gene Expression, Mammals, Trophoblasts metabolism, Pluripotent Stem Cells

Abstract

With the development of the embryo, the totipotent blastomere undergoes the first lineage decision to the inner cell mass (ICM) and the trophectoderm (TE). The ICM forms the fetus while the TE forms the placenta, which is one of the unique organs in mammals serving as the interface between maternal and fetal bloodstreams. Proper trophoblast lineage differentiation is crucial for correct placental and fetal development, including the TE progenitor self-renewal and its differentiation toward mononuclear cytotrophoblast, which later either develops into invasive extravillous trophoblast, remodeling the uterine vascular, or fuses into multinuclear syncytiotrophoblast, secreting pregnancy-sustaining hormone. Aberrant differentiation and gene expression of trophoblast lineage is associated with severe pregnancy disorders and fetal growth restriction. This review focuses on the early differentiation and key regulatory factors of trophoblast lineage, which have been poorly elucidated. Meanwhile, the recent development of trophoblast stem cells, trophectoderm stem cells, and blastoids derived from pluripotent stem cells bring the accessible model to investigate the profound mystery of embryo implantation and placentation and were also summarized., (© The Author(s) 2023. Published by Oxford University Press on behalf of Society for the Study of Reproduction. All rights reserved. For permissions, please e-mail: journals.permissions@oup.com.)

Published

2023

199. The use of copy number loads to designate mosaicism in blastocyst stage PGT-A cycles: fewer is better.

Author

Girardi L, Figliuzzi M, Poli M, Serdarogullari M, Patassini C, Caroselli S, Pergher I, Cogo F, Coban O, Boynukalin FK, Bahceci M, Navarro R, Rubio C, Findikli N, Simón C, and Capalbo A

Subjects

Pregnancy, Female, Humans, DNA Copy Number Variations, Blastocyst metabolism, Genetic Testing methods, Aneuploidy, Mosaicism, Preimplantation Diagnosis methods

Abstract

Study Question: How well can whole chromosome copy number analysis from a single trophectoderm (TE) biopsy predict true mosaicism configurations in human blastocysts?, Summary Answer: When a single TE biopsy is tested, wide mosaicism thresholds (i.e. 20-80% of aneuploid cells) increase false positive calls compared to more stringent ones (i.e. 30-70% of aneuploid cells) without improving true detection rate, while binary classification (aneuploid/euploid) provides the highest diagnostic accuracy., What Is Known Already: Next-generation sequencing-based technologies for preimplantation genetic testing for aneuploidies (PGT-A) allow the identification of intermediate chromosome copy number alterations potentially associated with chromosomal mosaicism in TE biopsies. Most validation studies are based on models mimicking mosaicism, e.g. mixtures of cell lines, and cannot be applied to the clinical interpretation of TE biopsy specimens., Study Design, Size, Duration: The accuracy of different mosaicism diagnostic thresholds was assessed by comparing chromosome copy numbers in multiple samples from each blastocyst. Enrolled embryos were donated for research between June 2019 and September 2020. The Institutional Review Board at the Near East University approved the study (project: YDU/2019/70-849). Embryos showing euploid/aneuploid mosaicism (n = 53), uniform chromosomal alterations (single or multiple) (n = 25), or uniform euploidy (n = 39) in their clinical TE biopsy were disaggregated into five portions: the inner cell mass (ICM) and four TE segments. Collectively, 585 samples from 117 embryos were analysed., Participants/materials, Setting, Methods: Donated blastocysts were warmed, allowed to re-expand, and disaggregated in TE portions and ICM. PGT-A analysis was performed using Ion ReproSeq PGS kit and Ion S5 sequencer (ThermoFisher). Sequencing data were blindly analysed with Ion Reporter software to estimate raw chromosome copy numbers. Intra-blastocyst comparison of copy number data was performed employing different thresholds commonly used for mosaicism detection. From copy number data, different case scenarios were created using more stringent (30-70%) or less stringent criteria (20-80%). Categorical variables were compared using the two-sample z test for proportions., Main Results and the Role of Chance: When all the five biopsies from the same embryo were analysed with 30-70% thresholds, only 8.4% (n = 14/166) of patterns abnormal in the original analysis revealed a true mosaic configuration, displaying evidence of reciprocal events (3.6%, n = 6/166) or confirmation in additional biopsies (4.8%, n = 8/166), while most mosaic results (87.3% of total predicted mosaic patterns) remained confined to a single TE specimen. Conversely, uniform whole chromosome aneuploidies (28.3% of total patterns, n = 47/166) were confirmed in all subsequent biopsies in 97.9% of cases (n = 46/47). When 20-80% thresholds were employed (instead of 30-70%), the overall mosaicism rate per biopsy increased from 20.2% (n = 114/565) to 40.2% (n = 227/565). However, the use of a wider threshold range did not contribute to the detection of additional true mosaic patterns, while significantly increasing false positive mosaic patterns from 57.8% to 79.5% (n = 96/166; 95% CI = 49.9-65.4 vs n = 271/341; 95% CI = 74.8-83.6, respectively) (P < 0.00001). Moreover, the shift of the aneuploid cut-off from 70% to 80% of aneuploid cells resulted in mosaicism overcalling in the high range (50-80% of aneuploid cells), impacting the accuracy of uniform aneuploid classification. Parametric analysis of thresholds, based on multifocal analysis, revealed that a binary classification scheme with a single cut-off at a 50% level provided the highest sensitivity and specificity rates. Further analysis on technical noise distribution at the chromosome level revealed a greater impact on smaller chromosomes., Limitations, Reasons for Caution: While enrolment of a population enriched in embryos showing intermediate chromosome copy numbers enhanced the evaluation of the mosaicism category compared with random sampling such study population selection is likely to lead to an overall underestimation of PGT-A accuracy compared to a general assessment of unselected clinical samples. This approach involved the analysis of aneuploidy chromosome copy number thresholds at the embryo level; future studies will need to evaluate these criteria in relation to clinical predictive values following embryo transfers for different PGT-A assays. Moreover, the study lacked genotyping-based confirmation analysis. Finally, aneuploid embryos with known meiotic partial deletion/duplication were not included., Wider Implications of the Findings: Current technologies can detect low-intermediate chromosome copy numbers in preimplantation embryos but their identification is poorly correlated with consistent propagation of the anomaly throughout the embryo or with negative clinical consequences when transferred. Therefore, when a single TE biopsy is analysed, diagnosis of chromosomal mosaicism should be evaluated carefully. Indeed, the use of wider mosaicism thresholds (i.e. 20-80%) should be avoided as it reduces the overall PGT-A diagnostic accuracy by increasing the risk of false positive mosaic classification and false negative aneuploid classification. From a clinical perspective, this approach has negative consequences for patients as it leads to the potential deselection of normal embryos for transfer. Moreover, a proportion of uniform aneuploid embryos may be inaccurately categorized as high-level mosaic, with a consequent negative outcome (i.e. miscarriage) when inadvertently selected for transfer. Clinical outcomes following PGT-A are maximized when a 50% threshold is employed as it offers the most accurate diagnostic approach., Study Funding/competing Interest(s): The study was supported by Igenomix. The authors not employed by Igenomix have no conflicts of interest to declare., Trial Registration Number: N/A., (© The Author(s) 2023. Published by Oxford University Press on behalf of European Society of Human Reproduction and Embryology. All rights reserved. For permissions, please email: journals.permissions@oup.com.)

Published

2023

200. Picolinafen exposure induces ROS accumulation and calcium depletion, leading to apoptosis in porcine embryonic trophectoderm and uterine luminal epithelial cells during the peri-implantation period.

Author

Park W, Park J, Park S, Lim W, and Song G

Subjects

Pregnancy, Female, Swine, Animals, Reactive Oxygen Species metabolism, Apoptosis, Epithelial Cells metabolism, Cell Proliferation, Mammals, Calcium metabolism, Embryo Implantation

Abstract

The global use of herbicides accounts for more than 48% of total pesticide usage. Picolinafen is a pyridine carboxylic acid herbicide that is predominantly used to control broadleaf weeds in wheat, barley, corn, and soybeans. Despite its widespread use in agriculture, its toxicity in mammals has rarely been studied. In this study, we first identified the cytotoxic effects of picolinafen on porcine trophectoderm (pTr) and luminal epithelial (pLE) cells, which are involved in the implantation process during early pregnancy. Picolinafen treatment significantly decreased the viability of pTr and pLE cells. Our results demonstrate that picolinafen increased the number of sub-G1 phase cells and early/late apoptosis. In addition, picolinafen disrupted mitochondrial function and resulted in the accumulation of intracellular ROS, leading to a reduction in calcium levels in both the mitochondria and cytoplasm of pTr and pLE cells. Moreover, picolinafen was found to significantly inhibit the migration of pTr. These responses were accompanied by the activation of the MAPK and PI3K signal transduction pathways by picolinafen. Our data suggest that the deleterious effects of picolinafen on the viability and migration of pTr and pLE cells might impair their implantation potential., Competing Interests: Declaration of competing interest The authors declare that there are no conflicts of interest that could be perceived as prejudicing the impartiality of the research reported., (Copyright © 2023 Elsevier Inc. All rights reserved.)

Published

2023