Your search keyword '"Bedzhov I"' showing total 34 results

1. Agrobacterium- Mediated Transformation of Secondary Somatic Embryos fromRosa HybridaL. and Recovery of Transgenic Plants

Author

Borissova, A., primary, Hvarleva, T., additional, Bedzhov, I., additional, Kondakova, V., additional, Atanassov, A., additional, and Atanassov, I., additional

Published

2005

2. Agrobacterium- Mediated Transformation of Secondary Somatic Embryos from Rosa HybridaL. and Recovery of Transgenic Plants

Author

Borissova, A., Hvarleva, T., Bedzhov, I., Kondakova, V., Atanassov, A., and Atanassov, I.

Abstract

ABSTRACTA genetic transformation protocol, based on co-cultivation of Rosa hybrida L. secondary embryos with Agrobacterium was established. Transgenic phosphinothricin (ppt) - resistant plants were obtained through application of interrupted selection procedure. Following the Agrobacterium inoculation step, the somatic embryos were initially cultivated on ppt—free media containing cefatoxim for elimination of the bacteria and later transferred on media containing the selective agent. The ppt—resistant secondary somatic embryos were matured and regenerated on ppt—free media and the putative transgenic plants were subsequently selected on media contained ppt and chlorphenol red. The performed PCR—and PAT protein—assays demonstrated presence and expression of bar gene encoding the phosphinothricin acetyltransferase (PAT) in part of the selected plants. The possibilities for application of the established transformation protocol are discussed.

Published

2005

3. Agrobacterium - Mediated transformation of secondary somatic embryos from Rosa hybrida L. and recovery of transgenic plants

Author

Borissova, A., Hvarleva, T., Bedzhov, I., Violeta Kondakova, Atanassov, A., and Atanassov, I.

4. Analyzing embryo dormancy at single-cell resolution reveals dynamic transcriptional responses and activation of integrin-Yap/Taz prosurvival signaling.

Author

Chen R, Fan R, Chen F, Govindasamy N, Brinkmann H, Stehling M, Adams RH, Jeong HW, and Bedzhov I

Subjects

Animals, Mice, Cell Survival, Diapause, Embryonic Development genetics, Gene Expression Regulation, Developmental, Transcription Factors metabolism, Transcription Factors genetics, Transcription, Genetic, Transcriptional Coactivator with PDZ-Binding Motif Proteins, Adaptor Proteins, Signal Transducing metabolism, Adaptor Proteins, Signal Transducing genetics, Embryo, Mammalian metabolism, Integrins metabolism, Signal Transduction, Single-Cell Analysis, YAP-Signaling Proteins metabolism

Abstract

Embryonic diapause is a reproductive adaptation that enables some mammalian species to halt the otherwise continuous pace of embryonic development. In this dormant state, the embryo exploits poorly understood regulatory mechanisms to preserve its developmental potential for prolonged periods of time. Here, using mouse embryos and single-cell RNA sequencing, we molecularly defined embryonic diapause at single-cell resolution, revealing transcriptional dynamics while the embryo seemingly resides in a state of suspended animation. Additionally, we found that the dormant pluripotent cells rely on integrin receptors to sense their microenvironment and preserve their viability via Yap/Taz-mediated prosurvival signaling., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

5. Tissue-intrinsic beta-catenin signals antagonize Nodal-driven anterior visceral endoderm differentiation.

Author

Schumacher S, Fernkorn M, Marten M, Chen R, Kim YS, Bedzhov I, and Schröter C

Subjects

Animals, Mice, Germ Layers metabolism, Germ Layers cytology, Mouse Embryonic Stem Cells metabolism, Mouse Embryonic Stem Cells cytology, Gene Expression Regulation, Developmental, Embryo, Mammalian cytology, Endoderm cytology, Endoderm metabolism, Endoderm embryology, beta Catenin metabolism, Cell Differentiation, Nodal Protein metabolism, Nodal Protein genetics, Signal Transduction, Body Patterning

Abstract

The anterior-posterior axis of the mammalian embryo is laid down by the anterior visceral endoderm (AVE), an extraembryonic signaling center that is specified within the visceral endoderm. Current models posit that AVE differentiation is promoted globally by epiblast-derived Nodal signals, and spatially restricted by a BMP gradient established by the extraembryonic ectoderm. Here, we report spatially restricted AVE differentiation in bilayered embryo-like aggregates made from mouse embryonic stem cells that lack an extraembryonic ectoderm. Notably, clusters of AVE cells also form in pure visceral endoderm cultures upon activation of Nodal signaling, indicating that tissue-intrinsic factors can restrict AVE differentiation. We identify β-catenin activity as a tissue-intrinsic factor that antagonizes AVE-inducing Nodal signals. Together, our results show how an AVE-like population can arise through interactions between epiblast and visceral endoderm alone. This mechanism may be a flexible solution for axis patterning in a wide range of embryo geometries, and provide robustness to axis patterning when coupled with signal gradients., (© 2024. The Author(s).)

Published

2024

6. Highly cooperative chimeric super-SOX induces naive pluripotency across species.

Author

MacCarthy CM, Wu G, Malik V, Menuchin-Lasowski Y, Velychko T, Keshet G, Fan R, Bedzhov I, Church GM, Jauch R, Cojocaru V, Schöler HR, and Velychko S

Subjects

Humans, Mice, Rats, Animals, Swine, Macaca fascicularis metabolism, Octamer Transcription Factor-3 genetics, Octamer Transcription Factor-3 metabolism, Cellular Reprogramming, SOXB1 Transcription Factors metabolism, Cell Differentiation, Mammals metabolism, Induced Pluripotent Stem Cells metabolism, Pluripotent Stem Cells metabolism

Abstract

Our understanding of pluripotency remains limited: iPSC generation has only been established for a few model species, pluripotent stem cell lines exhibit inconsistent developmental potential, and germline transmission has only been demonstrated for mice and rats. By swapping structural elements between Sox2 and Sox17, we built a chimeric super-SOX factor, Sox2-17, that enhanced iPSC generation in five tested species: mouse, human, cynomolgus monkey, cow, and pig. A swap of alanine to valine at the interface between Sox2 and Oct4 delivered a gain of function by stabilizing Sox2/Oct4 dimerization on DNA, enabling generation of high-quality OSKM iPSCs capable of supporting the development of healthy all-iPSC mice. Sox2/Oct4 dimerization emerged as the core driver of naive pluripotency with its levels diminished upon priming. Transient overexpression of the SK cocktail (Sox+Klf4) restored the dimerization and boosted the developmental potential of pluripotent stem cells across species, providing a universal method for naive reset in mammals., Competing Interests: Declaration of interests S.V., H.R.S., C.M.M., V.C., and G.W. filed a patent with Max Planck Innovation on highly cooperative Sox factors and SK naive reset. S.V. advises eGenesis. G.W. filed a patent on tetraploid complementation and leads MingCeler Biotech. R.J. filed patents on engineered Sox. G.M.C. founded and advises eGenesis., (Copyright © 2023 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

7. 3D biomimetic environment enabling ex utero trophoblast invasion and co-culture of embryos and somatic cells.

Author

Govindasamy N, Long H, Ranga A, Trappmann B, and Bedzhov I

Subjects

Coculture Techniques, Embryo, Mammalian, Trophoblasts, Biomimetics, Endothelial Cells

Abstract

The first direct contact between the embryo and the mother is established during implantation. This process is inaccessible for direct studies as the implanting embryo is concealed by the maternal tissues. Here, we present a protocol for establishing a 3D biomimetic environment based on synthetic hydrogels which harbor key biomechanical properties of the uterine stroma. We describe steps for isolating and culturing embryos in PEG/DexMA hydrogel. We then detail the co-culture of embryos and endothelial cells in a microfluidic device. For complete details on the use and execution of this protocol, please refer to Govindasamy et al. (2021) 1 and Ozguldez et al. (2023). 2 ., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2023 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2023

8. Polarity inversion reorganizes the stem cell compartment of the trophoblast lineage.

Author

Ozguldez HO, Govindasamy N, Fan R, Long H, Mildner K, Zeuschner D, Trappmann B, Ranga A, and Bedzhov I

Subjects

Pregnancy, Female, Mice, Animals, Stem Cells, Embryo Implantation, Placenta, Cell Lineage, Cell Differentiation, Trophoblasts, Blastocyst

Abstract

The extra-embryonic tissues that form the placenta originate from a small population of trophectoderm cells with stem cell properties, positioned at the embryonic pole of the mouse blastocyst. During the implantation stages, the polar trophectoderm rapidly proliferates and transforms into extra-embryonic ectoderm. The current model of trophoblast morphogenesis suggests that tissue folding reshapes the trophoblast during the blastocyst to egg cylinder transition. Instead of through folding, here we found that the tissue scale architecture of the stem cell compartment of the trophoblast lineage is reorganized via inversion of the epithelial polarity axis. Our findings show the developmental significance of polarity inversion and provide a framework for the morphogenetic transitions in the peri-implantation trophoblast., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2023 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2023

9. Early developmental plasticity enables the induction of an intermediate extraembryonic cell state.

Author

Sathyanarayanan A, Ing-Simmons E, Chen R, Jeong HW, Ozguldez HO, Fan R, Duethorn B, Kim KP, Kim YS, Stehling M, Brinkmann H, Schöler HR, Adams RH, Vaquerizas JM, and Bedzhov I

Abstract

Two fundamental elements of pre-implantation embryogenesis are cells' intrinsic self-organization program and their developmental plasticity, which allows embryos to compensate for alterations in cell position and number; yet, these elements are still poorly understood. To be able to decipher these features, we established culture conditions that enable the two fates of blastocysts' extraembryonic lineages-the primitive endoderm and the trophectoderm-to coexist. This plasticity emerges following the mechanisms of the first lineage segregation in the mouse embryo, and it manifests as an extended potential for extraembryonic chimerism during the pre-implantation embryogenesis. Moreover, this shared state enables robust assembly into higher-order blastocyst-like structures, thus combining both the cell fate plasticity and self-organization features of the early extraembryonic lineages.

Published

2022

10. Mechanisms of formation and functions of the early embryonic cavities.

Author

Kim YS and Bedzhov I

Subjects

Animals, Embryo Implantation, Embryo, Mammalian, Embryonic Development, Mice, Blastocyst, Endoderm

Abstract

As the early mouse embryo develops, fundamental steps include the sequential formation of the first lumens in the murine conceptus. The first cavity established in the pre-implantation embryo is the blastocoel, followed by the emergence of the proamniotic cavity during the peri-implantation stages. The mouse embryo is a dynamic system which switches its modes of lumenogenesis before and after implantation. The blastocoel emerges in between the basolateral membranes, whereas the proamniotic cavity is formed on the apical interface. Defects in the sculpting of these luminal spaces are associated with developmental abnormalities and embryonic lethality. Here, we review the mechanisms by which these early embryonic cavities are formed and discuss the cavities in terms of their common and stage-specific principles of lumenogenesis and their functions., Competing Interests: Declaration of Competing Interest The authors declare no conflict of interest., (Copyright © 2022 Elsevier Ltd. All rights reserved.)

Published

2022

11. Rap1 controls epiblast morphogenesis in sync with the pluripotency states transition.

Author

Kim YS, Fan R, Lith SC, Dicke AK, Drexler HCA, Kremer L, Kuempel-Rink N, Hekking L, Stehling M, and Bedzhov I

Subjects

Animals, Cell Differentiation, Gene Expression Regulation, Developmental, Mice, Morphogenesis, Embryo Implantation, Germ Layers

Abstract

The complex architecture of the murine fetus originates from a simple ball of pluripotent epiblast cells, which initiate morphogenesis upon implantation. In turn, this establishes an intermediate state of tissue-scale organization of the embryonic lineage in the form of an epithelial monolayer, where patterning signals delineate the body plan. However, how this major morphogenetic process is orchestrated on a cellular level and synchronized with the developmental progression of the epiblast is still obscure. Here, we identified that the small GTPase Rap1 plays a critical role in reshaping the pluripotent lineage. We found that Rap1 activity is controlled via Oct4/Esrrb input and is required for the transmission of polarization cues, which enables the de novo epithelialization and formation of tricellular junctions in the epiblast. Thus, Rap1 acts as a molecular switch that coordinates the morphogenetic program in the embryonic lineage, in sync with the cellular states of pluripotency., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2022 Elsevier Inc. All rights reserved.)

Published

2022

12. Tissue clearing may alter emission and absorption properties of common fluorophores.

Author

Eliat F, Sohn R, Renner H, Kagermeier T, Volkery S, Brinkmann H, Kirschnick N, Kiefer F, Grabos M, Becker K, Bedzhov I, Schöler HR, and Bruder JM

Subjects

Brain diagnostic imaging, Ionophores, Solvents, Fluorescent Dyes chemistry, Imaging, Three-Dimensional methods

Abstract

In recent years, 3D cell culture has been gaining a more widespread following across many fields of biology. Tissue clearing enables optical analysis of intact 3D samples and investigation of molecular and structural mechanisms by homogenizing the refractive indices of tissues to make them nearly transparent. Here, we describe and quantify that common clearing solutions including benzyl alcohol/benzyl benzoate (BABB), PEG-associated solvent system (PEGASOS), immunolabeling-enabled imaging of solvent-cleared organs (iDISCO), clear, unobstructed brain/body imaging cocktails and computational analysis (CUBIC), and ScaleS4 alter the emission spectra of Alexa Fluor fluorophores and fluorescent dyes. Clearing modifies not only the emitted light intensity but also alters the absorption and emission peaks, at times to several tens of nanometers. The resulting shifts depend on the interplay of solvent, fluorophore, and the presence of cells. For biological applications, this increases the risk for unexpected channel crosstalk, as filter sets are usually not optimized for altered fluorophore emission spectra in clearing solutions. This becomes especially problematic in high throughput/high content campaigns, which often rely on multiband excitation to increase acquisition speed. Consequently, researchers relying on clearing in quantitative multiband excitation experiments should crosscheck their fluorescent signal after clearing in order to inform the proper selection of filter sets and fluorophores for analysis., (© 2022. The Author(s).)

Published

2022

13. A balanced Oct4 interactome is crucial for maintaining pluripotency.

Author

Han D, Wu G, Chen R, Drexler HCA, MacCarthy CM, Kim KP, Adachi K, Gerovska D, Mavrommatis L, Bedzhov I, Araúzo-Bravo MJ, and Schöler HR

Abstract

Oct4 collaborates primarily with other transcriptional factors or coregulators to maintain pluripotency. However, how Oct4 exerts its function is still unclear. Here, we show that the Oct4 linker interface mediates competing yet balanced Oct4 protein interactions that are crucial for maintaining pluripotency. Oct4 linker mutant embryonic stem cells (ESCs) show decreased expression of self-renewal genes and increased expression of differentiation genes, resulting in impaired ESC self-renewal and early embryonic development. The linker mutation interrupts the balanced Oct4 interactome. In mutant ESCs, the interaction between Oct4 and Klf5 is decreased. In contrast, interactions between Oct4 and Cbx1, Ctr9, and Cdc73 are increased, disrupting the epigenetic state of ESCs. Control of the expression level of Klf5, Cbx1, or Cdc73 rebalances the Oct4 interactome and rescues the pluripotency of linker mutant ESCs, indicating that such factors interact with Oct4 competitively. Thus, we provide previously unidentified molecular insights into how Oct4 maintains pluripotency.

Published

2022

14. Induction of osteogenesis by bone-targeted Notch activation.

Author

Xu C, Dinh VV, Kruse K, Jeong HW, Watson EC, Adams S, Berkenfeld F, Stehling M, Rasouli SJ, Fan R, Chen R, Bedzhov I, Chen Q, Kato K, Pitulescu ME, and Adams RH

Subjects

Adaptor Proteins, Signal Transducing metabolism, Animals, Bone and Bones metabolism, Calcium-Binding Proteins metabolism, Chondrocytes metabolism, Endothelial Cells metabolism, Female, Human Umbilical Vein Endothelial Cells, Humans, Male, Mesenchymal Stem Cells metabolism, Mice, Mice, Inbred C57BL, Osteoblasts metabolism, Signal Transduction, Osteogenesis, Osteoporosis metabolism, Receptors, Notch metabolism

Abstract

Declining bone mass is associated with aging and osteoporosis, a disease characterized by progressive weakening of the skeleton and increased fracture incidence. Growth and lifelong homeostasis of bone rely on interactions between different cell types including vascular cells and mesenchymal stromal cells (MSCs). As these interactions involve Notch signaling, we have explored whether treatment with secreted Notch ligand proteins can enhance osteogenesis in adult mice. We show that a bone-targeting, high affinity version of the ligand Delta-like 4, termed Dll4 (E12) , induces bone formation in male mice without causing adverse effects in other organs, which are known to rely on intact Notch signaling. Due to lower bone surface and thereby reduced retention of Dll4 (E12) , the same approach failed to promote osteogenesis in female and ovariectomized mice but strongly enhanced trabecular bone formation in combination with parathyroid hormone. Single cell analysis of stromal cells indicates that Dll4 (E12) primarily acts on MSCs and has comparably minor effects on osteoblasts, endothelial cells, or chondrocytes. We propose that activation of Notch signaling by bone-targeted fusion proteins might be therapeutically useful and can avoid detrimental effects in Notch-dependent processes in other organs., Competing Interests: CX, VD, KK, HJ, EW, SA, FB, MS, SR, RF, RC, IB, QC, KK, MP, RA No competing interests declared, (© 2022, Xu et al.)

Published

2022

15. Lima1 mediates the pluripotency control of membrane dynamics and cellular metabolism.

Author

Duethorn B, Groll F, Rieger B, Drexler HCA, Brinkmann H, Kremer L, Stehling M, Borowski MT, Mildner K, Zeuschner D, Zernicka-Goetz M, Stemmler MP, Busch KB, Vaquerizas JM, and Bedzhov I

Subjects

Animals, Blastocyst, Cell Proliferation, Embryonic Development physiology, Embryonic Stem Cells cytology, Female, Male, Mice, Pluripotent Stem Cells cytology, Cytoskeletal Proteins genetics, Cytoskeletal Proteins metabolism, Embryonic Stem Cells metabolism, Pluripotent Stem Cells metabolism

Abstract

Lima1 is an extensively studied prognostic marker of malignancy and is also considered to be a tumour suppressor, but its role in a developmental context of non-transformed cells is poorly understood. Here, we characterise the expression pattern and examined the function of Lima1 in mouse embryos and pluripotent stem cell lines. We identify that Lima1 expression is controlled by the naïve pluripotency circuit and is required for the suppression of membrane blebbing, as well as for proper mitochondrial energetics in embryonic stem cells. Moreover, forcing Lima1 expression enables primed mouse and human pluripotent stem cells to be incorporated into murine pre-implantation embryos. Thus, Lima1 is a key effector molecule that mediates the pluripotency control of membrane dynamics and cellular metabolism., (© 2022. The Author(s).)

Published

2022

16. 3D biomimetic platform reveals the first interactions of the embryo and the maternal blood vessels.

Author

Govindasamy N, Long H, Jeong HW, Raman R, Özcifci B, Probst S, Arnold SJ, Riehemann K, Ranga A, Adams RH, Trappmann B, and Bedzhov I

Subjects

Animals, Biomimetics, Blastocyst cytology, Blood Vessels cytology, Cell Culture Techniques, Cell Movement, Embryo Implantation, Embryo, Mammalian cytology, Female, Giant Cells cytology, Giant Cells metabolism, Mice, Mice, Inbred C57BL, Mice, Inbred CBA, Pregnancy, Trophoblasts cytology, Blastocyst metabolism, Blood Vessels metabolism, Cell Communication, Embryo, Mammalian metabolism, Embryonic Development, Maternal-Fetal Exchange, Trophoblasts metabolism

Abstract

The process of implantation and the cellular interactions at the embryo-maternal interface are intrinsically difficult to analyze, as the implanting embryo is concealed by the uterine tissues. Therefore, the mechanisms mediating the interconnection of the embryo and the mother are poorly understood. Here, we established a 3D biomimetic culture environment that harbors the key features of the murine implantation niche. This culture system enabled direct analysis of trophoblast invasion and revealed the first embryonic interactions with the maternal vasculature. We found that implantation is mediated by the collective migration of penetrating strands of trophoblast giant cells, which acquire the expression of vascular receptors, ligands, and adhesion molecules, assembling a network for communication with the maternal blood vessels. In particular, Pdgf signaling cues promote the establishment of the heterologous contacts. Together, the biomimetic platform and our findings thereof elucidate the hidden dynamics of the early interactions at the implantation site., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2021 Elsevier Inc. All rights reserved.)

Published

2021

17. Ronin governs the metabolic capacity of the embryonic lineage for post-implantation development.

Author

Salewskij K, Gross-Thebing T, Ing-Simmons E, Duethorn B, Rieger B, Fan R, Chen R, Govindasamy N, Brinkmann H, Kremer L, Kuempel-Rink N, Mildner K, Zeuschner D, Stehling M, Dejosez M, Zwaka TP, Schöler HR, Busch KB, Vaquerizas JM, and Bedzhov I

Subjects

Animals, Blastocyst metabolism, Embryo Implantation physiology, Embryo, Mammalian metabolism, Mice, Embryonic Development genetics, Embryonic Stem Cells metabolism

Abstract

During implantation, the murine embryo transitions from a "quiet" into an active metabolic/proliferative state, which kick-starts the growth and morphogenesis of the post-implantation conceptus. Such transition is also required for embryonic stem cells to be established from mouse blastocysts, but the factors regulating this process are poorly understood. Here, we show that Ronin plays a critical role in the process by enabling active energy production, and the loss of Ronin results in the establishment of a reversible quiescent state in which naïve pluripotency is promoted. In addition, Ronin fine-tunes the expression of genes that encode ribosomal proteins and is required for proper tissue-scale organisation of the pluripotent lineage during the transition from blastocyst to egg cylinder stage. Thus, Ronin function is essential for governing the metabolic capacity so that it can support the pluripotent lineage's high-energy demands for cell proliferation and morphogenesis., (© 2021 The Authors. Published under the terms of the CC BY NC ND 4.0 license.)

Published

2021

18. Deciphering epiblast lumenogenesis reveals proamniotic cavity control of embryo growth and patterning.

Author

Kim YS, Fan R, Kremer L, Kuempel-Rink N, Mildner K, Zeuschner D, Hekking L, Stehling M, and Bedzhov I

Abstract

During the peri-implantation stages, the mouse embryo radically changes its appearance, transforming from a hollow-shaped blastocyst to an egg cylinder. At the same time, the epiblast gets reorganized from a simple ball of cells to a cup-shaped epithelial monolayer enclosing the proamniotic cavity. However, the cavity's function and mechanism of formation have so far been obscure. Through investigating the cavity formation, we found that in the epiblast, the process of lumenogenesis is driven by reorganization of intercellular adhesion, vectoral fluid transport, and mitotic paracellular water influx from the blastocoel into the emerging proamniotic cavity. By experimentally blocking lumenogenesis, we found that the proamniotic cavity functions as a hub for communication between the early lineages, enabling proper growth and patterning of the postimplantation embryo., (Copyright © 2021 The Authors, some rights reserved; exclusive licensee American Association for the Advancement of Science. No claim to original U.S. Government Works. Distributed under a Creative Commons Attribution NonCommercial License 4.0 (CC BY-NC).)

Published

2021

19. In Vitro Culture of Mouse Blastocysts to the Egg Cylinder Stage via Mural Trophectoderm Excision.

Author

Ozguldez HO and Bedzhov I

Subjects

Animals, Blastocyst cytology, Blastocyst ultrastructure, Embryonic Development, Female, Ovum cytology, Ovum ultrastructure, Blastocyst physiology, Embryo Culture Techniques methods, Mice embryology, Ovum physiology

Abstract

The developmental transition from the blastocyst to the egg cylinder stage is associated with stark changes in the overall shape of the embryo, as well as with reorganization of the transcriptional network and epigenetic landscape in the pluripotent and the supportive extraembryonic lineages. To directly analyze this pre- to postimplantation switch, culture conditions are needed that can support mouse embryogenesis beyond the blastocyst stage without maternal input. Here we provide a step-by-step protocol describing an experimental pipeline for isolating late blastocysts, excising (manually or via laser assistance) the mural trophectoderm, and, finally, culturing the embryo to the egg cylinder stage.

Published

2021

20. Wnt/Beta-catenin/Esrrb signalling controls the tissue-scale reorganization and maintenance of the pluripotent lineage during murine embryonic diapause.

Author

Fan R, Kim YS, Wu J, Chen R, Zeuschner D, Mildner K, Adachi K, Wu G, Galatidou S, Li J, Schöler HR, Leidel SA, and Bedzhov I

Subjects

Animals, Embryonic Development, Female, Germ Layers metabolism, Male, Membrane Proteins metabolism, Mice, Mice, Inbred C57BL, Mice, Knockout, Morphogenesis, Protein Serine-Threonine Kinases metabolism, Receptors, Estrogen genetics, beta Catenin genetics, Diapause physiology, Embryonic Stem Cells metabolism, Receptors, Estrogen metabolism, Wnt Signaling Pathway physiology

Abstract

The epiblast, which provides the foundation of the future body, is actively reshaped during early embryogenesis, but the reshaping mechanisms are poorly understood. Here, using a 3D in vitro model of early epiblast development, we identify the canonical Wnt/β-catenin pathway and its central downstream factor Esrrb as the key signalling cascade regulating the tissue-scale organization of the murine pluripotent lineage. Although in vivo the Wnt/β-catenin/Esrrb circuit is dispensable for embryonic development before implantation, autocrine Wnt activity controls the morphogenesis and long-term maintenance of the epiblast when development is put on hold during diapause. During this phase, the progressive changes in the epiblast architecture and Wnt signalling response show that diapause is not a stasis but instead is a dynamic process with underlying mechanisms that can appear redundant during transient embryogenesis.

Published

2020

21. Placental gene editing via trophectoderm-specific Tat-Cre/loxP recombination.

Author

Ozguldez HO, Fan R, and Bedzhov I

Subjects

Animals, Blastocyst cytology, Female, Gene Editing, Humans, Integrases genetics, Integrases metabolism, Mice, Pregnancy, Trophoblasts cytology, Blastocyst metabolism, Placenta metabolism, Trophoblasts metabolism

Abstract

The ways in which placental defects affect embryonic development are largely overlooked because of the lack of a trophoblast-specific approach for conditional gene ablation. To tackle this, we have established a simple, fast and efficient method for trophectodermal Tat-Cre/loxP recombination. We used the natural permeability barrier in mouse blastocysts in combination with off-the-shelf Tat-Cre recombinase to achieve editing of conditional alleles in the trophoblast lineage. This direct approach enables gene function analysis during implantation and placentation in mice, thereby crucially helping to broaden our understanding of human reproduction and development., Competing Interests: Competing interestsThe authors declare no competing or financial interests., (© 2020. Published by The Company of Biologists Ltd.)

Published

2020

22. Functional and clinical characterization of the alternatively spliced isoform AML1-ETO9a in adult patients with translocation t(8;21)(q22;q22.1) acute myeloid leukemia (AML).

Author

Agrawal M, Schwarz P, Giaimo BD, Bedzhov I, Corbacioglu A, Weber D, Gaidzik VI, Jahn N, Rücker FG, Schroeder T, Kindler T, Wattad M, Götze K, Lübbert M, Salwender H, Ringhoffer M, Lange E, Koller E, Thol F, Heuser M, Ganser A, Bullinger L, Paschka P, Döhner H, Geiger H, Borggrefe T, Döhner K, and Oswald F

Subjects

Adolescent, Adult, Aged, Female, Humans, Male, Middle Aged, Young Adult, Alternative Splicing genetics, Chromosomes, Human, Pair 21 genetics, Chromosomes, Human, Pair 8 genetics, Core Binding Factor Alpha 2 Subunit genetics, Leukemia, Myeloid, Acute genetics, Oncogene Proteins, Fusion genetics, Protein Isoforms genetics, RUNX1 Translocation Partner 1 Protein genetics, Translocation, Genetic genetics

Published

2020

23. Isolation and Culture of Periimplantation and Early Postimplantation Mouse Embryos.

Author

Govindasamy N and Bedzhov I

Subjects

Animals, Blastocyst cytology, Mice, Blastocyst metabolism, Cell Differentiation, Embryo Culture Techniques methods, Embryonic Development

Abstract

Key developmental processes of cell fate decisions and morphogenetic transformations take place during the periimplantation and early postimplantation stages of mouse embryogenesis. However analysing these fundamental events relies on direct observations of cultured embryos, which are challenging to obtain. To address this challenge, here we provide a detailed protocol describing a workflow for isolating early implanted embryos, removing of redundant extraembryonic tissues and describing the culture conditions that support further embryo development in vitro.

Published

2019

24. Test-tube embryos - mouse and human development in vitro to blastocyst stage and beyond.

Author

Govindasamy N, Duethorn B, Oezgueldez HO, Kim YS, and Bedzhov I

Subjects

Animals, Embryo Culture Techniques, Embryo Implantation immunology, Embryonic Development physiology, Female, Fertilization in Vitro, Humans, Mice, Blastocyst physiology, Embryo Implantation physiology

Abstract

Mammalian embryogenesis is intrauterine and depends on support from the maternal environment. Therefore, in order to directly study and manipulate early mouse and human embryos, fine-tuned culture conditions have to be provided to maintain embryo growth in vitro. Over time, the establishment and implementation of embryo culture methods have come a long way, initially enabling the development of few pre-implantation stages, expanding later to support in vitro embryogenesis from fertilization until blastocyst and even ex utero development beyond the implantation stages. Designing culture conditions that enable near physiological development of early embryos without maternal input, especially during the peri- and post-implantation stages, requires overcoming numerous experimental challenges, and it is still far from optimal. Nevertheless, embryo culture methods are an essential cornerstone of both assisted reproductive technologies and basic research, and these methods provide a platform to understand life's greatest miracle - the development of a new organism.

Published

2019

25. Development of the anterior-posterior axis is a self-organizing process in the absence of maternal cues in the mouse embryo.

Author

Bedzhov I, Bialecka M, Zielinska A, Kosalka J, Antonica F, Thompson AJ, Franze K, and Zernicka-Goetz M

Subjects

Animals, Embryo, Mammalian cytology, Endoderm cytology, Endoderm embryology, Endoderm metabolism, Mice, Body Patterning, Embryo, Mammalian embryology, Embryo, Mammalian metabolism

Published

2015

26. Cell death and morphogenesis during early mouse development: are they interconnected?

Author

Bedzhov I and Zernicka-Goetz M

Subjects

Animals, Apoptosis physiology, Blastocyst cytology, Embryo Implantation physiology, Embryonic Development physiology, Female, Germ Layers physiology, Mice, Pregnancy, Germ Layers cytology, Morphogenesis physiology

Abstract

Shortly after implantation the embryonic lineage transforms from a coherent ball of cells into polarized cup shaped epithelium. Recently we elucidated a previously unknown apoptosis-independent morphogenic event that reorganizes the pluripotent lineage. Polarization cues from the surrounding basement membrane rearrange the epiblast into a polarized rosette-like structure, where subsequently a central lumen is established. Thus, we provided a new model revising the current concept of apoptosis-dependent epiblast morphogenesis. Cell death however has to be tightly regulated during embryogenesis to ensure developmental success. Here, we follow the stages of early mouse development and take a glimpse at the critical signaling and morphogenic events that determine cells destiny and reshape the embryonic lineage., (© 2015 The Authors. Bioessays published by WILEY Periodicals, Inc.)

Published

2015

27. Correction to: 'Developmental plasticity, cell fate specification and morphogenesis in the early mouse embryo'.

Author

Bedzhov I, Graham SJ, Yan Leung C, and Zernicka-Goetz M

Published

2015

28. Applying the proximity ligation assay (PLA) to mouse preimplantation embryos for identifying protein-protein interactions in situ.

Author

Bedzhov I and Stemmler MP

Subjects

Animals, Antibodies, Monoclonal chemistry, Antibodies, Monoclonal metabolism, Blastocyst ultrastructure, Cadherins genetics, Embryo, Mammalian, Fluorescent Antibody Technique methods, Gene Expression Regulation, Developmental, Mice, Nucleic Acid Amplification Techniques, Nucleic Acid Hybridization, Protein Interaction Mapping, Receptor, IGF Type 1 genetics, beta Catenin genetics, Blastocyst metabolism, Cadherins metabolism, Receptor, IGF Type 1 metabolism, Staining and Labeling methods, beta Catenin metabolism

Abstract

Analysis of protein-protein interactions in mouse preimplantation embryos is hindered by the low cell number of the embryo. Here we describe the use of the proximity ligation assay to overcome these limitations and outline how protein-protein interactions can be visualized in situ. The method is based on a normal immunofluorescence labeling protocol of preimplantation embryos. Events of binding of the two primary antibodies directed against two individual proteins close to each other are visualized. If the two primary antibodies and the corresponding oligo-linked secondary antibodies bind in close proximity a cascade of events is initiated. This includes oligo ligation, DNA amplification, and hybridization with a fluorescent probe that allows visualization of this close proximity. In contrast to normal immunofluorescence labeling, here detection of red fluorescent dots reflects protein-protein interaction.

Published

2015

29. Developmental plasticity, cell fate specification and morphogenesis in the early mouse embryo.

Author

Bedzhov I, Graham SJ, Leung CY, and Zernicka-Goetz M

Subjects

Animals, Mice, Models, Biological, Body Patterning physiology, Cell Differentiation physiology, Cell Lineage physiology, Embryo Implantation physiology, Embryo, Mammalian embryology, Morphogenesis physiology

Abstract

A critical point in mammalian development is when the early embryo implants into its mother's uterus. This event has historically been difficult to study due to the fact that it occurs within the maternal tissue and therefore is hidden from view. In this review, we discuss how the mouse embryo is prepared for implantation and the molecular mechanisms involved in directing and coordinating this crucial event. Prior to implantation, the cells of the embryo are specified as precursors of future embryonic and extra-embryonic lineages. These preimplantation cell fate decisions rely on a combination of factors including cell polarity, position and cell-cell signalling and are influenced by the heterogeneity between early embryo cells. At the point of implantation, signalling events between the embryo and mother, and between the embryonic and extraembryonic compartments of the embryo itself, orchestrate a total reorganization of the embryo, coupled with a burst of cell proliferation. New developments in embryo culture and imaging techniques have recently revealed the growth and morphogenesis of the embryo at the time of implantation, leading to a new model for the blastocyst to egg cylinder transition. In this model, pluripotent cells that will give rise to the fetus self-organize into a polarized three-dimensional rosette-like structure that initiates egg cylinder formation.

Published

2014

30. In vitro culture of mouse blastocysts beyond the implantation stages.

Author

Bedzhov I, Leung CY, Bialecka M, and Zernicka-Goetz M

Subjects

Animals, Blastocyst physiology, Cell Adhesion, Ectoderm cytology, Embryo Culture Techniques instrumentation, Embryo Implantation, Female, Mice, Inbred C57BL, Blastocyst cytology, Embryo Culture Techniques methods

Abstract

The implanting mouse blastocyst invades the uterine stroma and undergoes a dramatic transformation into an egg cylinder. The morphogenetic and signaling events during this transition are largely unexplored, as the uterine tissues engulf the embryo. Here we describe a protocol supporting the development of the mouse embryo beyond the blastocyst stage in vitro. We established two types of medium to be applied sequentially, and we used a substrate permitting high-resolution imaging of the transition from blastocyst to egg cylinder. We developed two variants of this protocol: the first starts with intact early blastocysts that upon zona removal can attach to the substrate and develop into egg cylinders after 5 d, and the second starts with late blastocysts that upon dissection of the mural trophectoderm form egg cylinders in only 3 d. This method allows observation of a previously hidden period of development, and it provides a platform for novel research into peri-implantation embryogenesis and beyond.

Published

2014

31. Self-organizing properties of mouse pluripotent cells initiate morphogenesis upon implantation.

Author

Bedzhov I and Zernicka-Goetz M

Subjects

Animals, Apoptosis, Blastocyst metabolism, Embryo, Mammalian metabolism, Embryonic Stem Cells cytology, Embryonic Stem Cells metabolism, Extracellular Matrix metabolism, Female, Integrins metabolism, Male, Mice, Mice, Inbred C57BL, Mice, Inbred CBA, Morphogenesis, Signal Transduction, Blastocyst cytology, Embryo Implantation, Embryo, Mammalian cytology, Germ Layers cytology

Abstract

Transformation of pluripotent epiblast cells into a cup-shaped epithelium as the mouse blastocyst implants is a poorly understood and yet key developmental step. Studies of morphogenesis in embryoid bodies led to the current belief that it is programmed cell death that shapes the epiblast. However, by following embryos developing in vivo and in vitro, we demonstrate that not cell death but a previously unknown morphogenetic event transforms the amorphous epiblast into a rosette of polarized cells. This transformation requires basal membrane-stimulated integrin signaling that coordinates polarization of epiblast cells and their apical constriction, a prerequisite for lumenogenesis. We show that basal membrane function can be substituted in vitro by extracellular matrix (ECM) proteins and that ES cells can be induced to form similar polarized rosettes that initiate lumenogenesis. Together, these findings lead to a completely revised model for peri-implantation morphogenesis in which ECM triggers the self-organization of the embryo's stem cells., (Copyright © 2014 Elsevier Inc. All rights reserved.)

Published

2014

32. Adhesion, but not a specific cadherin code, is indispensable for ES cell and induced pluripotency.

Author

Bedzhov I, Alotaibi H, Basilicata MF, Ahlborn K, Liszewska E, Brabletz T, and Stemmler MP

Subjects

Animals, Cadherins deficiency, Cadherins genetics, Cell Adhesion, Cell Differentiation, Cells, Cultured, Embryonic Stem Cells metabolism, Epithelial-Mesenchymal Transition, Gene Knock-In Techniques, Genetic Loci, Homeodomain Proteins metabolism, Induced Pluripotent Stem Cells cytology, Induced Pluripotent Stem Cells metabolism, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Mice, Nude, Nanog Homeobox Protein, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Cadherins metabolism, Embryonic Stem Cells cytology

Abstract

Embryonic stem (ES) cell pluripotency and induced pluripotent stem (iPS) cell generation is dependent on a core transcriptional network and proper cell-cell adhesion mediated by E-cadherin (E-cad). Whereas E-cad is associated with pluripotency, N-cadherin (N-cad) expression is correlated with differentiation into mesodermal and neuroectodermal lineages. We investigated whether E-cad harbors unique molecular features in establishing or maintaining pluripotency. By using a gene replacement knock-in (ki) approach to express N-cadherin (N-cad) or E-cad/N-cad chimeric cadherins under the control of the E-cad locus, we show that all E-cad-depleted ki/ki ES cells are maintained in an undifferentiated state. Surprisingly, these cells retained key features of pluripotency, such as Nanog expression and full differentiation capacity in vitro and in vivo, whereas E-cad knockout (ko) ES cells irreversibly lost most of these features. Moreover, our results indicate that E-cad mediated adhesion is essential for iPS cell generation, since E-cad depleted fibroblasts were not reprogrammed. In contrast, N-cad efficiently supports somatic reprogramming similar to E-cad, and permits initiation of the crucial initial step of mesenchymal-epithelial transition. Thus, we show that cell adhesion and a robust pluripotent phenotype are ultimately connected. Since N-cad properly compensates for loss of E-cad, no specific 'cadherin code' is required., (© 2013.)

Published

2013

33. Igf1r signaling is indispensable for preimplantation development and is activated via a novel function of E-cadherin.

Author

Bedzhov I, Liszewska E, Kanzler B, and Stemmler MP

Subjects

Animals, Apoptosis, Cell Adhesion genetics, Cell Communication genetics, Cell Survival, Embryonic Stem Cells, Gene Expression Regulation, Developmental, Homozygote, Ligands, Mice, Mutation, Protein Structure, Tertiary genetics, Blastocyst cytology, Blastocyst metabolism, Cadherins genetics, Cadherins metabolism, Embryonic Development genetics, Receptor, IGF Type 1 genetics, Receptor, IGF Type 1 metabolism, Signal Transduction genetics

Abstract

Insulin-like growth factor I receptor (Igf1r) signaling controls proliferation, differentiation, growth, and cell survival in many tissues; and its deregulated activity is involved in tumorigenesis. Although important during fetal growth and postnatal life, a function for the Igf pathway during preimplantation development has not been described. We show that abrogating Igf1r signaling with specific inhibitors blocks trophectoderm formation and compromises embryo survival during murine blastocyst formation. In normal embryos total Igf1r is present throughout the membrane, whereas the activated form is found exclusively at cell contact sites, colocalizing with E-cadherin. Using genetic domain switching, we show a requirement for E-cadherin to maintain proper activation of Igf1r. Embryos expressing exclusively a cadherin chimera with N-cadherin extracellular and E-cadherin intracellular domains (NcEc) fail to form a trophectoderm and cells die by apoptosis. In contrast, homozygous mutant embryos expressing a reverse-structured chimera (EcNc) show trophectoderm survival and blastocoel cavitation, indicating a crucial and non-substitutable role of the E-cadherin ectodomain for these processes. Strikingly, blastocyst formation can be rescued in homozygous NcEc embryos by restoring Igf1r signaling, which enhances cell survival. Hence, perturbation of E-cadherin extracellular integrity, independent of its cell-adhesion function, blocked Igf1r signaling and induced cell death in the trophectoderm. Our results reveal an important and yet undiscovered function of Igf1r during preimplantation development mediated by a unique physical interaction between Igf1r and E-cadherin indispensable for proper receptor activation and anti-apoptotic signaling. We provide novel insights into how ligand-dependent Igf1r activity is additionally gated to sense developmental potential in utero and into a bifunctional role of adhesion molecules in contact formation and signaling., Competing Interests: The authors have declared that no competing interests exist.

Published

2012

34. A Cdh1HA knock-in allele rescues the Cdh1-/- phenotype but shows essential Cdh1 function during placentation.

Author

Stemmler MP and Bedzhov I

Subjects

Animals, Apoptosis, Blastocyst physiology, Cdh1 Proteins, Cell Proliferation, Embryo, Mammalian anatomy & histology, Embryo, Mammalian physiology, Female, Gene Expression Regulation, Developmental, Genetic Complementation Test, Mice, Mice, Inbred C57BL, Mice, Knockout, Morphogenesis, Placenta abnormalities, Placenta physiology, Pregnancy, Alleles, Cell Cycle Proteins genetics, Cell Cycle Proteins metabolism, Gene Knock-In Techniques, Phenotype, Placentation physiology

Abstract

The specific roles of classical cadherins at key morphogenetic events during development are still not fully understood. As part of a project to study cadherin function during early mammalian development, we generated mice carrying an HA-epitope tagged Cdh1 (E-cadherin) cDNA knocked into the Cdh1 locus, similar to the previously described mouse mutants in which we forced Cdh2 (N-cadherin) expression in the Cdh1 expression domain. As expected and in contrast to Cdh1(Cdh2/Cdh2) and Cdh1(-/-), our Cdh1(HA/HA) mutant embryos form proper trophectoderm, implant and undergo both gastrulation and neurulation. However, Cdh1(HA/HA) mice display an unexpected phenotype at embryonic day 10.5. Cdh1(HA/HA) embryos are smaller, paler and suffer from an insufficient nutrient supply. We detected a reduced expression of Cdh1(HA) specifically in the extraembryonic ectoderm and in the labyrinth layer, whereas expression in the embryo proper was normal. With this approach, we show for the first time that Cdh1 is essential for the correct formation of the placenta. Placentas without Cdh1 expression are impaired and incapable of establishing a proper connection between the embryonic and the maternal blood vessels for efficient nutrient and oxygen transport., (Developmental Dynamics 239:2330-2344, 2010. © 2010 Wiley-Liss, Inc.)

Published

2010