Characterization of transcription factor networks involved in umbilical cord blood CD34+ stem cells-derived erythropoiesis

Fetal stem cells isolated from umbilical cord blood (UCB) possess a great capacity for proliferation and differentiation and serve as a valuable model system to study gene regulation. Expanded knowledge of the molecular control of hemoglobin synthesis will provide a basis for rational design of ther...

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Bibliographic Details
Published in:PloS one 2014-09, Vol.9 (9), p.e107133-e107133
Main Authors: Li, Biaoru, Ding, Lianghao, Yang, Chinrang, Kang, Baolin, Liu, Li, Story, Michael D, Pace, Betty S
Format: Article
Language:English
Subjects:
Antigens, CD34 - genetics
beta-Globins - biosynthesis
beta-Globins - genetics
Biology and life sciences
Blood
Bone marrow
Cancer
CD34 antigen
Cell culture
Cell Differentiation - genetics
Chemical synthesis
Cord blood
Differentiation
DNA microarrays
Erythroblasts
Erythroblasts - cytology
Erythroblasts - metabolism
Erythroid Precursor Cells - cytology
Erythropoiesis
Erythropoiesis - genetics
Fetal Blood - cytology
Fetal Blood - metabolism
Fetuses
gamma-Globins - biosynthesis
gamma-Globins - metabolism
GATA-1 protein
Gene expression
Gene Expression Regulation
Gene regulation
Gene set enrichment analysis
Genomics
Hematology
Hemoglobin
Humans
KLF4 protein
Leukemia
Liquid culture
Medicine and Health Sciences
Molecular chains
Molecular modelling
Mutation
Oncology
Pediatrics
Proteins
Ribonucleic acid
RNA
Sickle cell disease
Stem cells
Stem Cells - cytology
Stem Cells - metabolism
Switching theory
Transcription factors
Transcription Factors - genetics
Transcription Factors - metabolism
Umbilical cord
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Summary:Fetal stem cells isolated from umbilical cord blood (UCB) possess a great capacity for proliferation and differentiation and serve as a valuable model system to study gene regulation. Expanded knowledge of the molecular control of hemoglobin synthesis will provide a basis for rational design of therapies for β-hemoglobinopathies. Transcriptome data are available for erythroid progenitors derived from adult stem cells, however studies to define molecular mechanisms controlling globin gene regulation during fetal erythropoiesis are limited. Here, we utilize UCB-CD34+ stem cells induced to undergo erythroid differentiation to characterize the transcriptome and transcription factor networks (TFNs) associated with the γ/β-globin switch during fetal erythropoiesis. UCB-CD34+ stem cells grown in the one-phase liquid culture system displayed a higher proliferative capacity than adult CD34+ stem cells. The γ/β-globin switch was observed after day 42 during fetal erythropoiesis in contrast to adult progenitors where the switch occurred around day 21. To gain insights into transcription factors involved in globin gene regulation, microarray analysis was performed on RNA isolated from UCB-CD34+ cell-derived erythroid progenitors harvested on day 21, 42, 49 and 56 using the HumanHT-12 Expression BeadChip. After data normalization, Gene Set Enrichment Analysis identified transcription factors (TFs) with significant changes in expression during the γ/β-globin switch. Forty-five TFs were silenced by day 56 (Profile-1) and 30 TFs were activated by day 56 (Profile-2). Both GSEA datasets were analyzed using the MIMI Cytoscape platform, which discovered TFNs centered on KLF4 and GATA2 (Profile-1) and KLF1 and GATA1 for Profile-2 genes. Subsequent shRNA studies in KU812 leukemia cells and human erythroid progenitors generated from UCB-CD34+ cells supported a negative role of MAFB in γ-globin regulation. The characteristics of erythroblasts derived from UCB-CD34+ stem cells including prolonged γ-globin expression combined with unique TFNs support novel mechanisms controlling the γ/β-globin switch during UCB-derived erythropoiesis.
ISSN:1932-6203
1932-6203
DOI:10.1371/journal.pone.0107133