RÉSUMÉ
During vertebrate development, progenitor cells give rise to tissues and organs through a complex choreography that commences at gastrulation. A hallmark event of gastrulation is the formation of the primitive streak, a linear assembly of cells along the anterior-posterior (AP) axis of the developing organism. To examine the primitive streak at a single-cell resolution, we measured the transcriptomes of individual chick cells from the streak or the surrounding tissue (the rest of the area pellucida) in Hamburger-Hamilton stage 4 embryos. The single-cell transcriptomes were then ordered by the statistical method Wave-Crest to deduce both the relative position along the AP axis and the prospective lineage of single cells. The ordered transcriptomes reveal intricate patterns of gene expression along the primitive streak.
Sujet(s)
Gastrulation/génétique , Ligne primitive/embryologie , Analyse sur cellule unique/méthodes , Animaux , Embryon de poulet , Poulets , Analyse de profil d'expression de gènes/méthodes , Régulation de l'expression des gènes au cours du développement/génétique , Ligne primitive/physiologie , Analyse spatio-temporelle , Transcriptome/génétiqueRÉSUMÉ
Arterial diseases continue to pose a major health concern but in vitro studies are limited because explanted cells can exhibit poor proliferative capacity and a loss of specificity. Here, we find that two transcription factors, MYCN and SOX17, induce and indefinitely expand in culture precursors of human arterial endothelial cells (expandable arterial endothelial precursors [eAEPs]). The eAEPs are derived from CD34+ cells found in umbilical cord blood or adult bone marrow. Independent eAEP lines differ in their proclivity to undergo an endothelial-to-mesenchymal transition (EndoMT), a hallmark event in a broad array of vascular diseases and disorders. Some cell lines spontaneously become mesenchymal over time in culture, an effect exacerbated by inhibition of the fibroblast growth factor receptor, while others do not readily convert. These distinctions were exploited to identify genes that correlate with resistance to an EndoMT and to elucidate transcriptional changes that underpin the transition.
Sujet(s)
Antigènes CD34/métabolisme , Cellules de la moelle osseuse/métabolisme , Différenciation cellulaire , Progéniteurs endothéliaux/métabolisme , Sang foetal/métabolisme , Cellules de la moelle osseuse/cytologie , Progéniteurs endothéliaux/cytologie , Sang foetal/cytologie , Humains , Protéine du proto-oncogène N-Myc/métabolisme , Spécificité d'organe , Facteurs de transcription SOX-F/métabolismeRÉSUMÉ
BACKGROUND: Human pluripotent stem cells offer the best available model to study the underlying cellular and molecular mechanisms of human embryonic lineage specification. However, it is not fully understood how individual stem cells exit the pluripotent state and transition towards their respective progenitor states. RESULTS: Here, we analyze the transcriptomes of human embryonic stem cell-derived lineage-specific progenitors by single-cell RNA-sequencing (scRNA-seq). We identify a definitive endoderm (DE) transcriptomic signature that leads us to pinpoint a critical time window when DE differentiation is enhanced by hypoxia. The molecular mechanisms governing the emergence of DE are further examined by time course scRNA-seq experiments, employing two new statistical tools to identify stage-specific genes over time (SCPattern) and to reconstruct the differentiation trajectory from the pluripotent state through mesendoderm to DE (Wave-Crest). Importantly, presumptive DE cells can be detected during the transitory phase from Brachyury (T) (+) mesendoderm toward a CXCR4 (+) DE state. Novel regulators are identified within this time window and are functionally validated on a screening platform with a T-2A-EGFP knock-in reporter engineered by CRISPR/Cas9. Through loss-of-function and gain-of-function experiments, we demonstrate that KLF8 plays a pivotal role modulating mesendoderm to DE differentiation. CONCLUSIONS: We report the analysis of 1776 cells by scRNA-seq covering distinct human embryonic stem cell-derived progenitor states. By reconstructing a differentiation trajectory at single-cell resolution, novel regulators of the mesendoderm transition to DE are elucidated and validated. Our strategy of combining single-cell analysis and genetic approaches can be applied to uncover novel regulators governing cell fate decisions in a variety of systems.
Sujet(s)
Différenciation cellulaire/génétique , Séquençage nucléotidique à haut débit , Cellules souches embryonnaires humaines/cytologie , ARN/génétique , Techniques de culture cellulaire , Endoderme/croissance et développement , Endoderme/métabolisme , Régulation de l'expression des gènes au cours du développement , Hépatocytes/cytologie , Humains , Cellules souches pluripotentes/cytologie , Analyse sur cellule unique/méthodesRÉSUMÉ
In this study, we demonstrate a newly derived mouse model that supports engraftment of human hematopoietic stem cells (HSCs) in the absence of irradiation. We cross the NOD.Cg-Prkdc(scid)Il2rg(tm1Wjl)/SzJ (NSG) strain with the C57BL/6J-Kit(W-41J)/J (C57BL/6.Kit(W41)) strain and engraft, without irradiation, the resulting NBSGW strain with human cord blood CD34+ cells. At 12-weeks postengraftment in NBSGW mice, we observe human cell chimerism in marrow (97% ± 0.4%), peripheral blood (61% ± 2%), and spleen (94% ± 2%) at levels observed with irradiation in NSG mice. We also detected a significant number of glycophorin-A-positive expressing cells in the developing NBSGW marrow. Further, the observed levels of human hematopoietic chimerism mimic those reported for both irradiated NSG and NSG-transgenic strains. This mouse model permits HSC engraftment while avoiding the complicating hematopoietic, gastrointestinal, and neurological side effects associated with irradiation and allows investigators without access to radiation to pursue engraftment studies with human HSCs.
Sujet(s)
Différenciation cellulaire , Survie du greffon , Transplantation de cellules souches hématopoïétiques , Cellules souches hématopoïétiques/cytologie , Cellules souches hématopoïétiques/métabolisme , Sous-unité gamma commune aux récepteurs des interleukines/génétique , Protéines proto-oncogènes c-kit/génétique , Animaux , Lignage cellulaire , Génotype , Hétérogreffes , Humains , Immunophénotypage , Mâle , Souris , Souris de lignée C57BL , Souris de lignée NOD , Souris knockout , Souris SCID , Phénotype , Facteurs temps , Chimère obtenue par transplantationRÉSUMÉ
During development, the hematopoietic and vascular lineages are thought to descend from common mesodermal progenitors called hemangioblasts. Here we identify six transcription factors, Gata2, Lmo2, Mycn, Pitx2, Sox17, and Tal1, that "trap" murine cells in a proliferative state and endow them with a hemangioblast potential. These "expandable" hemangioblasts (eHBs) are capable, once released from the control of the ectopic factors, to give rise to functional endothelial cells, multilineage hematopoietic cells, and smooth muscle cells. The eHBs can be derived from embryonic stem cells, from fetal liver cells, or poorly from fibroblasts. The eHBs reveal a central role for fibroblast growth factor, which not only promotes their expansion, but also facilitates their ability to give rise to endothelial cells and leukocytes, but not erythrocytes. This study serves as a demonstration that ephemeral progenitor states can be harnessed in vitro, enabling the creation of tractable progenitor cell lines.
Sujet(s)
Facteurs de croissance fibroblastique/métabolisme , Hémangioblastes/cytologie , Hémangioblastes/métabolisme , Animaux , Cellules sanguines/cytologie , Cellules sanguines/métabolisme , Différenciation cellulaire , Lignage cellulaire , Prolifération cellulaire , Cellules endothéliales/cytologie , Cellules endothéliales/métabolisme , Facteurs de croissance fibroblastique/pharmacologie , Analyse de profil d'expression de gènes , Hémangioblastes/effets des médicaments et des substances chimiques , Séquençage nucléotidique à haut débit , Immunophénotypage , Souris , Myocytes du muscle lisse/cytologie , Myocytes du muscle lisse/métabolisme , Phénotype , TranscriptomeRÉSUMÉ
Gene-corrected patient-specific induced pluripotent stem (iPS) cells offer a unique approach to gene therapy. Here, we begin to assess whether the mutational load acquired during gene correction of iPS cells is compatible with use in the treatment of genetic causes of retinal degenerative disease. We isolated iPS cells free of transgene sequences from a patient with gyrate atrophy caused by a point mutation in the gene encoding ornithine-δ-aminotransferase (OAT) and used homologous recombination to correct the genetic defect. Cytogenetic analysis, array comparative genomic hybridization (aCGH), and exome sequencing were performed to assess the genomic integrity of an iPS cell line after three sequential clonal events: initial reprogramming, gene targeting, and subsequent removal of a selection cassette. No abnormalities were detected after standard G-band metaphase analysis. However, aCGH and exome sequencing identified two deletions, one amplification, and nine mutations in protein coding regions in the initial iPS cell clone. Except for the targeted correction of the single nucleotide in the OAT locus and a single synonymous base-pair change, no additional mutations or copy number variation were identified in iPS cells after the two subsequent clonal events. These findings confirm that iPS cells themselves may carry a significant mutational load at initial isolation, but that the clonal events and prolonged cultured required for correction of a genetic defect can be accomplished without a substantial increase in mutational burden.
Sujet(s)
Atrophie gyrée/enzymologie , Atrophie gyrée/génétique , Ornithine-oxo-acid transaminase/génétique , Ornithine-oxo-acid transaminase/métabolisme , Cellules souches pluripotentes/enzymologie , Cellules cultivées , Ciblage de gène/méthodes , Étude d'association pangénomique , Instabilité du génome/génétique , Atrophie gyrée/anatomopathologie , Atrophie gyrée/thérapie , Humains , Cellules souches pluripotentes/anatomopathologie , Recombinaison génétiqueRÉSUMÉ
Epstein-Barr virus (EBV) encodes oncogenic information and, oftentimes concomitant with host immunosuppression, gives rise to malignancies in all major categories of lymphoma defined by the World Health Organization. Here, we conditionally evicted the viral extrachromosomal genome from tumor cells in vitro to examine the role of EBV in different lymphomas, including Burkitt lymphoma (BL) and posttransplant lymphoproliferative disorder. Cells derived from 2 canonical BLs were found to have the least dependence on the virus; some required EBV to prevent the inefficient induction of apoptosis. In contrast, cells derived from a subset of BL, Wp-restricted BL, required EBV to block a robust apoptotic program that involves the up-regulation of the proapoptotic protein Bim. Wp-restricted BL cells also relied on the virus to promote efficient proliferation, a distinction that highlights the multiple contributions EBV makes to affect proliferation of its host cells. Like Wp-BL cells, posttransplant lymphoproliferative disorder cells depended on the virus to inhibit apoptosis. They furthermore required the virus to drive them out of G(1)/G(0). Together, these results reveal a graded dependence on EBV among tumor cells that directly correlates with the number of viral genes expressed in the tumor cell.
Sujet(s)
Infections à virus Epstein-Barr/génétique , Infections à virus Epstein-Barr/virologie , Herpèsvirus humain de type 4/génétique , Herpèsvirus humain de type 4/pathogénicité , Lymphomes/génétique , Lymphomes/virologie , Apoptose/génétique , Protéines régulatrices de l'apoptose/génétique , Protéine-11 analogue à Bcl-2 , Lymphome de Burkitt/génétique , Lymphome de Burkitt/anatomopathologie , Lymphome de Burkitt/virologie , Lignée cellulaire tumorale , Prolifération cellulaire , Infections à virus Epstein-Barr/anatomopathologie , Gènes myc , Génome viral , Humains , Lymphomes/anatomopathologie , Syndromes lymphoprolifératifs/étiologie , Syndromes lymphoprolifératifs/génétique , Syndromes lymphoprolifératifs/anatomopathologie , Syndromes lymphoprolifératifs/virologie , Protéines membranaires/génétique , Modèles biologiques , Oncogènes , Protéines proto-oncogènes/génétique , Transplants/effets indésirablesRÉSUMÉ
We identified binding sites for Epstein-Barr virus (EBV) nuclear antigen 1 (EBNA1) in the human genome using chromatin immunoprecipitation and microarrays. The sequences for these newly identified sites were used to generate a position-weighted matrix (PWM) for EBNA1's DNA-binding sites. This PWM helped identify additional DNA-binding sites for EBNA1 in the genomes of EBV, Kaposi's sarcoma-associated herpesvirus, and cercopithecine herpesvirus 15 (CeHV-15) (also called herpesvirus papio 15). In particular, a homologue of the Rep* locus in EBV was predicted in the genome of CeHV-15, which is notable because Rep* of EBV was not predicted by the previously developed consensus sequence for EBNA1's binding DNA. The Rep* of CeHV-15 functions as an origin of DNA synthesis in the EBV-positive cell line Raji; this finding thus builds on a set of DNA-binding sites for EBNA1 predicted in silico.