A simple approach for mouse embryonic stem cells isolation and differentiation inducing embryoid body formation

Fagundez, Carol B; Loresi, Monica; Quintana, Marcos E Ojea; Delcourt, S.; Testa, Roberto; Gogorza, S.; Argibay, Pablo

doi:10.1016/j.cellbi.2009.08.001

Cited by 4 publications

(7 citation statements)

References 14 publications

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“…When staining of mESCs with the cell surface marker SSEA-1 was carried out in our laboratory, the extensions projected to the MEFs mentioned above were observed, supporting this information (Fig. 2E) (Fagundez et al, 2009). …”

Section: Wwwintechopencomsupporting

confidence: 59%

“…Reichert-like basement membrane deposits are often seen during the first days of EB culture and its presence can be identified by Periodic Acid Shiff (PAS) reaction (Fig. 4A,B) (Fagundez et al, 2009;Zhou et al, 2005). There are different types of culture media that can be employed to induce formation of EBs and results vary according to the medium chosen and whether they are supplemented either with FBS or Ko-SR. As mentioned earlier, FBS contains pro-differentiation factors which make it a useful tool in differentiation protocols (Fagundez et al, 2009).…”

Section: Differentiation Of Mescsmentioning

confidence: 99%

“…Some authors have attempted supplementation of ES medium with a FBS-KoSR mixture in different ratios to improve the isolation and the subsequent establishment of ESCs (Lee et al, 2006;Tanimoto et al, 2008). However, culture in ES medium without complete or partial FBS replacement do not always support ESCs derivation, but could be beneficial to increase cell growth rate of the colonies already established, while preserving the stemness state (Fagundez et al, 2009;Lee et al, 2006). The use of KoSR could be useful to easily isolate mESCs from cultures of whole blastocyst embryos, since it prevents development of trophoblastic cells which tend to colonize the culture, avoiding also the application of immunosurgery, a complex technique involving the use of cytotoxic antibodies, that is not always efficient at the moment of eliminating all the trophoblastic cell population of the embryo (Fagundez et al, 2009;Gardner, 1985).…”

Section: Considerations At the Moment Of Working With Mescsmentioning

confidence: 99%

“…The cells do not attach to the plastic surface of the dish; instead they stick to each other forming aggregates that will give rise to EBs (Kurosawa, 2007). Another way to form EBs employing these plates is to culture the whole colonies of mESCs during varying periods of time (Fagundez et al, 2009). Unfortunately, both of these methods produce heterogeneous EBs with distinct degrees of differentiation.…”

Section: Differentiation Of Mescsmentioning

confidence: 99%

“…In our laboratory we were not able to form EBs with HD technique, as cells were unable to group and failed to produce three-dimensional aggregates. Although generation of EBs in suspension culture employing whole ESCs colonies has some disadvantages, it seems possible that the proximity established among cells when growing together could be an important factor favouring the differentiation process, since cell to cell contact plays a major role in the early stages of embryonic development (Choi et al, 2005;Fagundez et al, 2009). Semisolid suspension culture.…”

Section: Differentiation Of Mescsmentioning

confidence: 99%

See 4 more Smart Citations

Mouse Embryonic Stem Cells Basics from a Fertilized Zygote to These Promising Pluripotent Stem Cells

Fagundez¹,

Loresi²,

Delcourt³

et al. 2011

Methodological Advances in the Culture, Manipulation and Utilization of Embryonic Stem Cells for Basic and Practical Applicatio

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Section: Wwwintechopencomsupporting

confidence: 59%

Section: Differentiation Of Mescsmentioning

confidence: 99%

Section: Considerations At the Moment Of Working With Mescsmentioning

confidence: 99%

Section: Differentiation Of Mescsmentioning

confidence: 99%

Section: Differentiation Of Mescsmentioning

confidence: 99%

See 3 more Smart Citations

Mouse Embryonic Stem Cells Basics from a Fertilized Zygote to These Promising Pluripotent Stem Cells

Fagundez¹,

Loresi²,

Delcourt³

et al. 2011

Methodological Advances in the Culture, Manipulation and Utilization of Embryonic Stem Cells for Basic and Practical Applicatio

View full text Add to dashboard Cite

SSSPTA is essential for serine palmitoyltransferase function during development and hematopoiesis

Parthibane

Acharya

Abimannan

et al. 2021

Journal of Biological Chemistry

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Serine palmitoyltransferase complex (SPT) mediates the first and rate-limiting step in the de novo sphingolipid biosynthetic pathway. The larger subunits SPTLC1 and SPTLC2/SPTLC3 together form the catalytic core while a smaller third subunit either SSSPTA or SSSPTB has been shown to increase the catalytic efficiency and provide substrate specificity for the fatty acyl-CoA substrates. The in vivo biological significance of these smaller subunits in mammals is still unknown. Here, using two null mutants, a conditional null for ssSPTa and a null mutant for ssSPTb, we show that SSSPTA is essential for embryogenesis and mediates much of the known functions of the SPT complex in mammalian hematopoiesis. The ssSPTa null mutants are embryonic lethal at E6.5 much like the Sptlc1 and Sptlc2 null alleles. Mx1-Cre induced deletion of ssSPTa leads to lethality and myelopoietic defect. Chimeric and competitive bone marrow transplantation experiments show that the defect in myelopoiesis is accompanied by an expansion of the Lin − Sca1 + c-Kit + stem and progenitor compartment. Progenitor cells that fail to differentiate along the myeloid lineage display evidence of endoplasmic reticulum stress. On the other hand, ssSPTb null mice are homozygous viable, and analyses of the bone marrow cells show no significant difference in the proliferation and differentiation of the adult hematopoietic compartment. SPTLC1 is an obligatory subunit for the SPT function, and because Sptlc1 −/− and ssSPTa −/− mice display similar defects during development and hematopoiesis, we conclude that an SPT complex that includes SSSPTA mediates much of its developmental and hematopoietic functions in a mammalian model.

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iPSCs: A Minireview from Bench to Bed, including Organoids and the CRISPR System

Orqueda¹,

Giménez²,

Pereyra-Bonnet³

2016

Stem Cells International

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When Dolly the sheep was born, the first probe into an adult mammalian genome traveling back in time and generating a whole new animal appeared. Ten years later, the reprogramming process became a defined method of producing induced pluripotent stem cells (iPSCs) through the overexpression of four transcription factors. iPSCs are capable of originating virtually all types of cells and tissues, including a whole new animal. The reprogramming strategies based on patient-derived cells should make the development of clinical applications of cell based therapy much more straightforward. Here, we analyze the current state, opportunities, and challenges of iPSCs from bench to bed, including organoids and the CRISPR system.

show abstract

A simple approach for mouse embryonic stem cells isolation and differentiation inducing embryoid body formation

Cited by 4 publications

References 14 publications

Mouse Embryonic Stem Cells Basics from a Fertilized Zygote to These Promising Pluripotent Stem Cells

Mouse Embryonic Stem Cells Basics from a Fertilized Zygote to These Promising Pluripotent Stem Cells

SSSPTA is essential for serine palmitoyltransferase function during development and hematopoiesis

iPSCs: A Minireview from Bench to Bed, including Organoids and the CRISPR System

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