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By
From the Department of Medicine University of Massachusetts Cancer Center, Worcester, MA; and Ontario Cancer Institute, Toronto, Ontario.
To better understand the molecular mechanism(s) by which growth and differentiation of the primitive hematopoietic stem cell is initiated, as well as the means by which the maturing cell can commit to development along a specific cell lineage, we elected to study the Id family of helix-loop-helix (HLH) transcriptional regulators. Some members of the HLH family are expressed in a stage-specific manner during hematopoietic development and can regulate the ability of immature hematopoietic cells to terminally differentiate. None of the four Id family genes were detected in the most primitive progenitors. Id-1 was widely expressed in proliferating bi- and unipotential progenitors, but its expression was downregulated in cells of increasing maturity; conversely, Id-2 and, to a limited extent, Id-3 gene expression increased as cells matured and lost proliferative capacity. Id-2 expression ran counter to that of Id-1 not only during maturation, but during periods of cell growth and arrest as well. This is quite distinct from the nonhematopoietic tissues, in which these two factors are coordinately expressed and suggests that Id-1 and Id-2 might be regulating very different events during hematopoiesis than they regulate in other cell types.
A POOL OF PRIMITIVE hematopoietic stem cells (PHSC) reside in the adult bone marrow as a reservoir of uncommitted and undifferentiated blood cell precursors. In order to maintain an appropriately balanced system, these cells must respond to cues from the extracellular environment by proliferation and subsequent differentiation into mature cell types. Each stage of this process, from the initial activation of the resting G0 stem cell through the critical event of lineage commitment to the final stages of differentiation is ultimately controlled by the amounts and types of transcriptional regulators expressed in the cell. Members of the helix-loop-helix (HLH),1 the homeobox (Hox),2-4 basic-zipper (bZ),5,6 LIM,7,8 and zinc finger9,10 transcription factor families have been detected in cells during some stage(s) of hematopoietic development. Thus, members of any of these groups could potentially play a role in the regulation of some or all of the key developmental switch points that must be negotiated in order for a normal blood cell to mature.
The HLH family of transcriptional regulators may play an important role in hematopoiesis. Members of this family have been shown to be key players in the regulation of neural development,11,12 sex determination,12 and myogenesis,13,14 as well as to contribute to regulation of development in the pancreas,15 bone,16,17 and fatty tissue.18 There is evidence to suggest that this family may control hematopoietic development as well.1,4,19-24 Numerous HLH regulators, including E47/E12,1,4,24 SCL,1,4,25 lyl-1,1,4,22 and most of the Id factors4,26-28 have been identified in at least a subset of normal hematopoietic tissues and cell lines. These regulators include both known transcriptional activators (eg, E12/E47 and SCL) as well as transdominant negative regulators (eg, the Id proteins).
The function of HLH transcriptional regulators is dictated by three structural elements: (1) the HLH protein dimerization interface, (2) a basic DNA binding region, and (3) an N-terminal transactivation domain. The HLH structure is a protein dimerization motif that is used to combine HLH monomer subunits into functionally important dimers.29 Upstream and extending from helix one there is usually a basic region, which is a DNA binding half-site. When these proteins dimerize they juxtapose the two half-sites into an active DNA-binding element that can then recognize and bind to specific sequence motifs called E-boxes. Finally, in some of these molecules, there is an N-terminal transactivation domain that affects transcriptional activation once the active dimer has been localized to its correct position in a promoter or enhancer regulatory unit.22,30,31 There are variants that function as negative regulators as well. In some instances, alternative splicing generates HLH monomers lacking the transactivation region; heterodimerization between this monomer and a full-length HLH activator would be expected to decrease or extinguish the activation potential of the resultant dimer.32 Alternately, there is a subclass of HLH forms that completely lack the basic DNA binding region. These proteins make up the Id (inhibitor of DNA binding) family, which can heterodimerize with HLH members to form dimers containing an incomplete DNA binding region, which then cannot bind to DNA.26,27,33,34 These Id family proteins act through sequestration of the HLH activators in nonfunctional complexes.
In addition to these structural classifications, HLH family regulators are subdivided according to their expression patterns. Some regulators are widely expressed, such as the universal E protein family (eg, E2A, E2-2, HEB; also called class I proteins); other class II factors are expressed in a tissue-restricted fashion (eg, MyoD and myogenin in muscle tissue; SCL and lyl-1 in hematopoietic cells).1,35 Class III proteins, such as the Id family of negative regulators, show an intermediate pattern of distribution.26,27,33,34 Most importantly, many of these regulators are highly expressed in normal hematopoietic tissues during the stage in which these cells must be able to respond to the external signaling that controls their ability to continue proliferation or commit to differentiate into a mature blood cell.1,4
Both class I and class II factors have been demonstrated to be essential for normal hematopoietic development. Mice lacking the class I gene E2A have a complete block in B cell development while other hematopoietic lineages remain largely normal.24,36 Blood development is profoundly limited in mice lacking the class II SCL gene; embryos suffer a complete block in early erythropoiesis with virtual absence of myeloid cells, suggesting that this gene is essential for normal growth and development of early myelo-erythroid progenitor cells.37 A working model for the role of HLH factors in differentiation proposes that the ability of a cell to differentiate may be controlled at the transcriptional level by a heterodimer between a class II tissue-specific HLH factor and a member of the class I E proteins.38 This heterodimer would then be able to activate expression of genes required for maturation. The action of this dimer is negatively regulated by the class III Id family, which can prevent differentiation by sequestration of class I E proteins in nonfunctional complexes.40 Since most tissue-specific class II proteins only function as heterodimeric complexes with the class I proteins,35,41-43 this prevents tissue-specific factors from initiating the maturation process.
In a previous study, we surveyed the expression patterns of several HLH transcriptional regulators (eg, E12/E47, SCL, ly1-1, and Id-1) in proliferating hematopoietic cells and cell lines.4 This work identified developmental stage-specific and cell cycle-related variations in expression of these genes, particularly Id-1. Since Id-1 belongs to a family of at least four similar transdominant negative regulators, we first needed to study the expression of Id-1 in the context of the other four family members in order to determine which Id family gene might be functionally important for regulating different aspects of hematopoietic growth and development. To do this, we first determined the range of expression of all four Id family genes in hematopoietic cells and tissues during growth and differentiation, then assayed whether the expression of some or all of these genes was specifically modulated in response to the defined environmental cues that stimulate normal hematopoietic growth and development.
Cell Lines and Cell Culture
Cell-Cycle Synchronization
Cytokine Starvation Experiments FDCPI cells were cultured in RPMI 1640 supplemented with 25% WEHIcm and 10% FCS. For cytokine-response studies, these cells were starved of growth factors by culture in RPMI plus 0.5% HI-FCS for 24 hours before transfer into fresh medium supplemented recombinant murine (rm) IL-3 (Collaborative Research, Waltham, MA) or rmGM-CSF (Amgen, Thousand Oaks, CA) at 100 U/mL each. In each case, maximal cell growth stimulation was predetermined by a dose-response titration of the individual growth factor (not shown); a concentration of each factor that gave maximal growth response was selected for use in each of these experiments. Samples were removed for RNA analysis at multiple time points after cytokine stimulation.RNA Isolation and Analysis Ten micrograms of unselected cytoplasmic RNA44 from each time point was separated by electrophoresis on a formaldehyde gel before transfer to Hybond N membrane. Each filter was hybridized to 32P-random labeled Id gene probes. After a high stringency wash, filters were exposed to film and the specific bands later quantitated on a PhosphorImager (Molecular Dynamics, Sunnyvale, CA). To normalize for loading efficiency each filter was stripped and rehybridized to a 28S ribosomal RNA probe46 or a GAPDH probe47 as indicated. Id-1 was quantitated after a 24-hour exposure; Id-2 quantitated after 3 to 5 days, Id-3 after 3 days; GAPDH after 3 hours; and 28S after 15 to 30 minutes.Isolation, Culture, and Analysis of Normal Murine Bone Marrow and Fetal Liver Cells Cells isolated from CBA/J bone marrow and day 12 fetal liver were used in this work.RT-PCR Analysis of Gene Expression in Single Cells and Small Populations Individual cells picked from colony starts were analyzed by RT-PCR.4 For small pools of cells, RT-PCR was performed using primers and conditions as previously described.48 Five micrograms of each amplified product was separated by agarose gel electrophoresis and transferred to Hybond N membrane. Each blot was subsequently probed with cDNA probes of the individual Id family genes. Due to the high degree of sequence conservation between human and murine Id genes at both the DNA and protein levels (Id-1 mRNA, 83% identity at the DNA level; Id-2, 88%; Id-3, 86%), our murine Id probes were also effective for detection of human Id family mRNAs. The Id-1 probe was a gift of H. Weintraub. pE:Id(S) is a BamHI/EcoR1 fragment consisting of the total cDNA sequence from pMH18DR blunt-ended into pEMSV-scribe 2 then released by Sma I. The Id-2 probe was a gift of X-H. Sun and consisted of a BamHI/XhoI fragment consisting of the full-length Id-2 cDNA. Id-3 is a 0.94-kb EcoRI fragment originally cloned as h1h462 (ATCC#63120). The Id-4 probes were a gift of F. Sablitzky: an EcoRI fragment containing the "full" 1.7 kb cDNA sequence and "probe b," an additional 0.7 kb of alternatively spliced Id-4, were used. Finally, a rat GAPDH probe was used for normalization of loading efficiency and RNA integrity.5 The isolated fragments were random labeled to 0.5 to 1 × 109 cpm/µg and hybridized to the filters at high stringency.48
The Id Family Genes Are Widely Expressed in Hematopoietic Cell Lines To determine the range of Id family gene expression in hematopoietic cells, we initially analyzed a panel of 18 cell lines. These cells included both murine and human lymphoid (P3X and T1165 plasmacytoma, Namalwa mature B, 22D6 and 18-81 preB, and EL4 and BW T-cell lines), monocyte/macrophage (M1 and RAW 246.7), megakaryotic (MO7E), erythroleukemia (K562 and MEL), mastocytoma (MC6), and myeloid (WEHI-3, MC6, FDCP1, NFS60, HL60) cells.
The Id Family Genes Are Differentially Expressed During the Early Stages of Normal Hematopoietic Development
Differential Expression of Id Family Genes During Cell Cycle
(D) Raw data.
Id-1 and Id-2 Are Differentially Regulated in Response to Cytokine Stimulation of FDCP1 Cells
Although the PHSC is a dormant (G0 ) cell,58-60 it retains the capacity to respond to external signaling by entering cell cycle and continuing to proliferate until its progeny differentiate into mature blood cells. For this to happen, gene programs that maintain the quiescent state of the stem cell need to be extinguished or modified and genes that support proliferation must be induced. Later, the gene program that supports proliferation of these undifferentiated progenitor cells needs to be repressed and expression of a new set of differentiation-specific genes increased in turn. Candidate regulators of this process must meet certain criteria: they should be differentially expressed during a relevant period of development, respond to cytokine stimulation by appropriate up- or down-regulation of their expression, and participate in control of a developing cell's ability to initiate and/or maintain proliferation or to mediate terminal differentiation. The Id family regulators of the HLH transcription factor family are excellent candidates for regulators of this process. This is the first comprehensive study describing the expression of the four Id family genes during growth and differentiation in the hematopoietic system. Several important findings are revealed in this work: (1) Id-1 is not highly expressed until normal progenitors have matured to the bipotential and unipotential stage, after which time its expression decreases withmaturation; (2) Id-2 expression does not parallel that of Id-1 as it does in other tissue types; these two Ids are expressed reciprocally during growth and differentiation; and (3) Id-2 and, to a limited extent, Id-3 are upregulated as cells mature.
Submitted September 16, 1996;
accepted December 5, 1996.
The publication costs of this article were defrayed in part by page
charge payment. This article must therefore be hearly marked
``advertisment'' in accordance with 18 U.S.C. section 1734 solely to
indicate this fact. Thanks to Drs Christopher Roman, Ellen Kittler, and Gary Stein for their thoughtful comments on this manuscript. We also wish to acknowledge and thank Drs Harold Weintraub, Xiao-Hong Sun, and Fred Sablitzky for their gifts of Id-1, Id-2, and Id-4 cDNA clones, respectively.
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Abstract
Introduction
Abstract
), while the other half were transferred into fresh medium without WEHIcm (
). Cells were allowed to grow for 48 hours, during which time samples were removed for RNA isolation and northern hybridization to (A) Id-1 and (B) Id-2 probes. Signal intensity was quantitated by phosphorimage analysis before the blots were normalized by rehybridization to a 28S RNA oligonucleotide. Values were plotted as the relative intensity (pixel number) of the specific bands above background for each probe. Values are comparable only within the group of samples hybridized to a single probe; different exposure times were used for each probe to maximize clarity of the phosphorimage. (C) Cell cycle progression was monitored by 3H-thymidine uptake of the cytokine-replete, proliferating population.
) or medium containing 100 U/mL of either rIL-3 (
) or rGM-CSF (
treated cells, which responded with only minimal growth, showed an intermediate depression in Id-2 gene expression. A similar, reciprocal, pattern of Id-1 and Id-2 gene expression was also seen in factor-starved NFS60 cells when compared with cells proliferating in the presence of cytokines (Cooper, manuscript in preparation). Thus expression of Id-2 consistently runs counter to that of Id-1, during periods of cytokine-stimulated growth (Fig 
promoter, 
-globin enhancer, the erythroid promoters of the carbonic anhydrase II, band 3 and GATA-1 genes, and the enhancer elements of the immunoglobulin locus.
