Gene Expression Profiling of Embryo-Derived Stem Cells Reveals Candidate Genes Associated With Pluripotency and Lineage Specificity

Tanaka, Tetsuya; Kunath, Tilo; Kimber, Wendy L.; Jaradat, Saied; Stagg, Carole A.; Usuda, Masayuki; Yokota, Takashi; Niwa, Hitoshi; Rossant, Janet; Ko, Minoru S.H.

doi:10.1101/gr.670002

Cited by 208 publications

(168 citation statements)

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“…We then attempted to identify candidate genes that are expressed more highly in the ICM than in TE cells. Due to difficulty of collecting the ICM and TE from blastocysts separately, we exploited the cultured cells derived from these cell types in our previous study (Tanaka et al, 2002). Mouse ES cells are cultured from the ICM (Evans and Kaufman, 1981;Martin, 1981), whereas mouse TS cells are cultured from the TE (Tanaka et al, 1998) (Fig.…”

Section: Informatics Selection Of Candidate Genesmentioning

confidence: 99%

“…To supplement the data (Tanaka et al, 2002) and update to the latest microarray platform, we performed hybridizations of ES and TS RNAs onto the NIA 22K 60-mer oligonucleotide microarrays in triplicate (Carter et al, 2003a). This glass-slide microarray platform contains genes from preimplantation and stem cells (for experimental design, see ref (Tanaka et al, 2002); for all the array data set, see http://lgsun.grc.nia.nih.gov/data, and also Supplementary Material 3).…”

Section: Informatics Selection Of Candidate Genesmentioning

confidence: 99%

“…This glass-slide microarray platform contains genes from preimplantation and stem cells (for experimental design, see ref (Tanaka et al, 2002); for all the array data set, see http://lgsun.grc.nia.nih.gov/data, and also Supplementary Material 3). By this criterion, we identified 1388 genes that were expressed more highly in ES cells than in TS cells.…”

Section: Informatics Selection Of Candidate Genesmentioning

confidence: 99%

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High-throughput screen for genes predominantly expressed in the ICM of mouse blastocysts by whole mount in situ hybridization

Yoshikawa

Piao

Zhong

et al. 2006

Gene Expression Patterns

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Mammalian preimplantation embryos provide an excellent opportunity to study temporal and spatial gene expression in whole mount in situ hybridization (WISH). However, large-scale studies are made difficult by the size of the embryos (∼60 μm diameter) and their fragility. We have developed a chamber system that allows parallel processing of embryos without the aid of a microscope. We first selected 91 candidate genes that were transcription factors highly expressed in blastocysts, and more highly expressed in embryonic (ES) than in trophoblast (TS) stem cells. We then used the WISH to identify 48 genes expressed predominantly in the ICM and to follow several of these genes in all seven preimplantation stages. The ICM-predominant expressions of these genes suggest their involvement in the pluripotency of embryonic cells. This system provides a useful tool to a systematic genome-scale analysis of preimplantation embryos.

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Section: Informatics Selection Of Candidate Genesmentioning

confidence: 99%

Section: Informatics Selection Of Candidate Genesmentioning

confidence: 99%

Section: Informatics Selection Of Candidate Genesmentioning

confidence: 99%

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High-throughput screen for genes predominantly expressed in the ICM of mouse blastocysts by whole mount in situ hybridization

Yoshikawa

Piao

Zhong

et al. 2006

Gene Expression Patterns

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“…Although previous reports have suggested that Esg1 is not expressed after the preimplantation and peri-implantation stages [11,12], we examined Esg1 expression during germ cell development. A unique quality of segregating PGCs is the expression of many pluripotency-associated genes, which are downregulated in somatic cells.…”

Section: Esg1 Oct4 and Sox2 Coexpression In Es And Germ Cellsmentioning

confidence: 99%

Analysis of Esg1 Expression in Pluripotent Cells and the Germline Reveals Similarities with Oct4 and Sox2 and Differences Between Human Pluripotent Cell Lines

et al. 2005

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Establishment of pluripotent epiblast cells is a critical event during early mammalian development because all somatic lineages and the primordial germ cells (PGCs) are derived from them. The epiblast and PGCs are in turn the precursors of pluripotent embryonic stem cells and embryonic germ cells, respectively. Although PGCs are specialized cells, they express several key pluripotency-related genes, such as Oct4 and Sox2. We have analyzed Esg1 expression in mouse and human cells and shown that in the mouse the gene is specifically expressed in preimplantation embryos, stem cells, and the germline. Moreover, Esg1 coexpresses with Oct4 and Sox2, confirming its identity as a marker of the pluripotent cycle. Esg1 is also expressed with Oct4 and Sox2 by human embryonic stem cells and in germ cell carcinoma tissue but not by all human embryonal carcinoma cell lines. These data suggest that together with Oct4 and Sox2, Esg1 plays a conserved role in the pluripotent pathway of mouse and human stem and germ cells.

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“…For example, during erythropoiesis nuclei become smaller and heterochromatic as many genes are silenced; concurrently, globin genes become active by associating with specific nuclear sites known as "factories" or "active chromatin hubs" (Cook, 1999(Cook, , 2002de Laat and Grosveld, 2003;Osborne et al, 2004). Although microarrays provide detailed information on changes in steady-state mRNA levels during differentiation (Kelly and Rizzino, 2000;Harris and Childs, 2002;Tanaka et al, 2002;Sperger et al, 2003), there is little information on how primary rates of transcription change. For example, we do not know by how much global rates vary as any mammalian cell differentiates.…”

mentioning

confidence: 99%

A Conserved Organization of Transcription during Embryonic Stem Cell Differentiation and in Cells with High C Value

Faro-Trindade

Cook

2006

MBoC

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Although we have detailed information on the alterations occurring in steady-state levels of all cellular mRNAs during differentiation, we still know little about more global changes. Therefore, we investigated the numbers of molecules of RNA polymerase II that are active-and the way those molecules are organized-as two mouse cells (aneuploid F9 teratocarcinoma, and euploid and totipotent embryonic stem cells) differentiate into parietal endoderm. Quantitative immunoblotting shows the number of active molecules roughly halves. Transcription sites (detected by light and electron microscopy after allowing engaged polymerases to extend nascent transcripts in bromouridine-triphosphate) are uniformly distributed throughout the nucleoplasm. The numbers of such sites fall during differentiation as nuclei become smaller, but site density and diameter remain roughly constant. Similar site densities and diameters are found in salamander (amphibian) cells with 11-fold larger genomes, and in aneuploid HeLa cells. We conclude that active polymerases and their nascent transcripts are concentrated in a limited number of discrete nucleoplasmic sites or factories, and we speculate that the organization of transcription is conserved during both differentiation and evolution to a high C value. INTRODUCTIONDifferentiation involves the repression of some genes and the activation of others. For example, during erythropoiesis nuclei become smaller and heterochromatic as many genes are silenced; concurrently, globin genes become active by associating with specific nuclear sites known as "factories" or "active chromatin hubs" (Cook, 1999(Cook, , 2002de Laat and Grosveld, 2003;Osborne et al., 2004). Although microarrays provide detailed information on changes in steady-state mRNA levels during differentiation (Kelly and Rizzino, 2000;Harris and Childs, 2002;Tanaka et al., 2002;Sperger et al., 2003), there is little information on how primary rates of transcription change. For example, we do not know by how much global rates vary as any mammalian cell differentiates. Eukaryotic genomes also differ in size more than 200,000-fold in a way unrelated to organismal complexity; there is no consensus as to the basis of this C-value enigma (Hartl, 2000;Gregory, 2001), or on how transcription might be organized in such differently sized genomes.Against this background, we investigated the changes that occur in the rates and organization of transcription as two mouse cells differentiate. Mouse F9 teratocarcinoma cells are a well-studied aneuploid line that can be induced to differentiate into parietal endoderm, which is characterized by flattened cells that secrete tissue-type plasminogen activator, laminin, and type IV collagen (Strickland and Mahdavi, 1978;Strickland et al., 1980;Hogan et al., 1983). ESF/48 -1 cells are totipotent embryonic stem (ES) cells with a normal karyotype; when transferred into host blastocysts, they contribute to all tissues (including germ lines) of the resulting chimeras (Brook and Gardner, 1997), and they can be induc...

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Gene Expression Profiling of Embryo-Derived Stem Cells Reveals Candidate Genes Associated With Pluripotency and Lineage Specificity

Cited by 208 publications

References 38 publications

High-throughput screen for genes predominantly expressed in the ICM of mouse blastocysts by whole mount in situ hybridization

High-throughput screen for genes predominantly expressed in the ICM of mouse blastocysts by whole mount in situ hybridization

Analysis of Esg1 Expression in Pluripotent Cells and the Germline Reveals Similarities with Oct4 and Sox2 and Differences Between Human Pluripotent Cell Lines

A Conserved Organization of Transcription during Embryonic Stem Cell Differentiation and in Cells with High C Value

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