The in vivo profile of transcription factors during neutrophil differentiation in human bone marrow

doi:10.1182/blood-2002-03-0835

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Prepublished online as a Blood First Edition Paper on January 30, 2003; DOI 10.1182/blood-2002-03-0835.

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Blood, 1 June 2003, Vol. 101, No. 11, pp. 4322-4332

HEMATOPOIESIS
The in vivo profile of transcription factors during neutrophil differentiation in human bone marrow
Malene Digmann Bjerregaard, Jesper Jurlander, Pia Klausen, Niels Borregaard, and Jack Bernard Cowland
From the the Granulocyte Research Laboratory and the Leukemia and Lymphoma Research Laboratory, Department of Hematology, Rigshospitalet, University of Copenhagen, Copenhagen, Denmark.

   Abstract

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

In vivo distribution of myeloid transcription factors duringgranulopoiesis was investigated by Northern and Western blottingin 3 neutrophil precursor populations from human bone marrow:immature (myeloblasts [MBs] and promyelocytes [PMs]); intermediatemature (myelocytes [MCs] and metamyelocytes [MMs]); and matureneutrophil cells (band cells [BCs] and segmented neutrophil cells [SCs]). Nonneutrophil cells were removed with magnetic-bead–coupledantibodies against CD2, CD3, CD14, CD19, CD56, CD61, glycophorin-A,and CD49d (BCs/SCs) before RNA and protein extraction. Polymorphonuclearneutrophils (PMNs) from peripheral blood depleted with anti-CD49dantibodies were also included. Expression of acute myeloid leukemia 1b (AML-1b), c-myb, GATA-1, and CCAAT/enhancer binding protein ${gamma}$ (C/EBP- ${gamma}$ ) was seen primarily in MBs/PMs, and little expressionwas found in more mature cells. The level of C/EBP- ${alpha}$ was constantin the bone marrow–derived cells and decreased in PMNs.C/EBP- ${epsilon}$ was found primarily in MCs/MMs and was almost absentin more mature cells. Expression of C/EBP- ${beta}$ , C/EBP- ${delta}$ , and C/EBP- ${zeta}$ was observed from the MC/MM stage onward, with peak levelsin the most mature cells. The amount of PU.1 increased throughoutmaturation whereas the level of Elf-1 reached a nadir in MCs/MMsThe PU.1 coactivator c-jun and c-jun's dimerization partnerc-fos were both detectable in MCs/MMs and increased in amountwith maturity. CCAAT displacement protein (CDP) was found atcomparable levels at all stages of differentiation. This demonstratesa highly individualized expression of the transcription factors,which can form the basis for the heterogeneous expression ofgranule proteins during granulopoiesis and cell cycle arrestin metamyelocytes.

   Introduction

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Differentiation of granulocytes (granulopoiesis) takes placein the bone marrow over a period of 10 to 14 days. The firstrecognizable myeloid precursor is the myeloblast (MB), whichdifferentiates to segmented neutrophils (SCs) through the morphologicallydistinct stages of promyelocytes (PMs), myelocytes (MCs), metamyelocytes(MMs), and band cells (BCs).¹ Granulopoiesis is a complexprocess, in which a number of transcription factors play critical roles.^2,3 This can be appreciated by recognizing that thedifferentiation stop associated with acute myeloid leukemiain most cases involves translocations or other mutations thatdisturb the function of a transcription factor.^4,5 Furtherdocumentation comes from experiments involving ectopic expressionof transcription factors in myeloid cell cultures^6,7 andtargeted disruption of genes encoding transcription factorsin mice.^{8, 9, 10, 11} Experimental evidence has shown thatsome transcription factors, such as CCAAT/enhancer binding protein ${alpha}$ (C/EBP- ${alpha}$ ) and acute myeloid leukemia 1 (AML-1),^8,9 are important during early granulopoiesis whereas others, suchas C/EBP- ${epsilon}$ and CCAAT displacement protein (CDP),^10,12 firstexert their function in more mature neutrophil precursors. This demonstrates that timing of transcription factor expressionand activation is also important for proper neutrophil differentiation.
To date, much of the information on the timed expression oftranscription factors during neutrophil differentiation comesfrom investigation of in vitro–differentiated CD34⁺ bonemarrow cells or myeloid cell lines.^{6,13, 14, 15, 16} Thesestudies, however, have some inherent shortcomings. First, itis difficult to reproduce the endogenous milieu and stimuliencountered by the neutrophil precursors in the bone marrow,which is a prerequisite for proper granulocytic differentiation.^6,14 Second, data have often been obtained from asynchronously differentiatingcell cultures, which may obscure the disappearance of an earlyexpressed transcription factor owing to a sustained presenceof immature cells in the differentiated cell population.^6,15,17 Third, many of the widely used neutrophil cell lines, suchas HL60 and NB4 cells,¹⁸ lack the ability to express specific-and gelatinase-granule proteins. As the expression of theseproteins is transcriptionally regulated,^{10,19, 20, 21} thisstrongly suggests that the transcriptional program is corruptedin these cells.
The physiologic role of transcription factors in granulopoiesishas also been analyzed by gene-targeting experiments.^{8, 9, 10, 11,22,23} Although the hematopoietic cells in these casesencounter the proper microenvironment, the nature of theseexperiments usually allows only the earliest effect of a knocked-outtranscription factor to be observed. Since some transcriptionfactors are required not only for hematopoiesis in general (eg, AML-1b and c-myb)^9,11 or commitment of a hematopoieticprecursor (eg, C/EBP- ${alpha}$ and PU.1)^8,22,23 but also for the developmentof the precursor along the neutrophil lineage, the specificexpression pattern of the factor during granulopoiesis may notbe observed owing to a lack of definitive hematopoiesis inthese mice. Furthermore, the phenotype of the mutation maynot always be a direct consequence of the targeted disruptionbut may instead be a secondary effect caused by the lack ofa gene product induced by the transactivator as exemplifiedby the reduced C/EBP- ${delta}$ expression in C/EBP- ${epsilon}$ knockout mice.²⁴Finally, the resulting phenotype may depend on the design ofthe targeted disruption,²⁵ as was observed for the 2 PU.1knockout mouse models.^22,23
To gain further insight into the in vivo expression of transcription factors during granulopoiesis, we have analyzed the mRNA andprotein profiles of 14 transcription factors in neutrophilprecursors from human bone marrow.

   Materials and methods

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Isolation of neutrophils and their precursors from bone marrow and peripheral blood
Bone marrow samples (15 mL) from healthy volunteers were usedfor isolation of neutrophil precursors by density centrifugationon a 2-layer Percoll (Amersham Biosciences, Little Chalfont,England) gradient, which resulted in the separation of bonemarrow cells into 3 bands containing neutrophil precursorsof different maturity: MBs/PMs, MCs/MMs, and BCs/SCs, as described previously.^19,26 Contaminating erythrocytes in the BC/SC cellpopulation were removed by 30 seconds of hypotonic lysis. Matureneutrophils from peripheral blood were isolated by centrifugationon Lymphoprep (Nygaard, Oslo, Norway) as described previously.^26,27 Remaining erythrocytes were lysed by hypotonic lysis.
Removal of nonneutrophil hematopoietic cells by MACS depletion
Nonneutrophil bone marrow cells were depleted from the 3 populationsof neutrophil precursors by incubation with mouse antibodiesagainst human CD2, CD3, CD14, CD19, CD56, CD61, glycophorin-A,and CD49d (only BCs/SCs). Lymphoprep-purified polymorphonuclearneutrophils (PMNs) from peripheral blood were depleted forcontaminating eosinophils by incubation with anti-CD49d antibodies.All antibodies were mouse immunoglobulin G (IgG) monoclonals(BD PharMingen, San Diego, CA). The antibodies were incubatedwith the cells according to the manufacturer's recommendations.Goat anti-mouse IgG microbeads (Miltenyi Biotech, BergischGladbach, Germany) were added; following incubation and washing,the cells were layered on a depletion column of the appropriatesize (AS or BS depletion columns; Miltenyi Biotech). The columnwas fixed in a magnet (VarioMACS; Miltenyi Biotech), and the flow-through collected. If isolation of immunopositive cellswas required, the column was washed with a higher flow rateand removed from the magnet for elution of the cells. Then,1 x 10⁶ cells were saved for cytospin preparations and flowcytometric analysis. The remaining cells were used for RNAor protein purification.
Flow cytometric analysis
For flow cytometric analysis, the following phycoerythrin (PE)–and fluorescein isothiocyanate (FITC)–labeled mouse monoclonalantibodies and isotype negative controls were used: CD16-PE,CD19-PE, CD33-PE, CD34-PE, CD56-PE, IgG₁-PE, and IgG₁-FITC(Becton Dickinson, San Jose, CA); CD49d-PE (BD PharMingen);CD5-PE, CD10-PE, CD61-FITC, and glycophorin-A–PE (DAKO,Glostrup, Denmark); and CD14-PE and IgM-PE (Beckman Coulter,Miami, FL). Cells were incubated with antibody for 15 minutesat room temperature for labeling, washed twice in 0.5% bovineserum albumin (BSA) in phosphate-buffered saline (PBS) andfixed in 1% paraformaldehyde in PBS. Flow cytometric analysiswas performed with the use of a FACScan (Becton Dickinson),for which settings and compensation were adjusted weekly bymeans of CaliBRITE Beads (Becton Dickinson). The data were analyzed by means of the CELLQuest and PAINT-A-GATE software(Becton Dickinson).
Staining of eosinophils
Cells resuspended in 1% BSA in PBS were cytocentrifuged ontoa glass slide. Following methanol fixation, cells were stained30 minutes in 0.2% Fast Green (Sigma-Aldrich, St Louis, MO),rinsed in water, and counter-stained in 1% Neutral Red (Sigma-Aldrich).
RNA isolation and Northern blotting
Total RNA was isolated with Trizol (Invitrogen, San Diego, CA).The RNA was ethanol-precipitated and resuspended in 0.1 mMEDTA (ethylenediami-netetraacetic acid). For Northern blotting,5 µg RNA was run on a 1% agarose gel and transferredto a Hybond-N membrane (Amersham Biosciences) as described.¹⁹ Filters were prehybridized for 1 to 2 hours at 42°C in6 mL ULTRAhyb (Ambion, Austin, TX) and hybridized overnightat 42°C after addition of a further 4 mL containing the³²P-labeled probe and sheared salmon sperm DNA (10 µg/mL).The membranes were washed as described¹⁹ and developed bya Fuji BAS2500 PhosphorImager (Tokyo, Japan). Membranes were stripped by boiling in 0.1% sodium dodecyl sulfate (SDS) before rehybridization. Probes used for hybridization were radiolabeledwith [ ${alpha}$ -³²P] deoxycytidine triphosphate (dCTP) by means of the Random Primers DNA Labeling System (Invitrogen). Sizes of thehybridizing bands were determined relative to 18S and 28S andfound to be in accordance with previous reports (Table 1).For quantitative assessments, the intensities of the transcriptionfactor signals were normalized to the hybridization intensity from a probe against 18S.

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Table 1.. Synthesis of cDNA probes for Northern blot hybridization

Construction of probes for Northern blot
The probes were constructed by polymerase chain reaction (PCR) amplification with the use of a human bone marrow cDNA library(Clontech, Palo Alto, CA) or cDNA from HL60 cells as template (Table 1) and were cloned in pCRII (Invitrogen). Correctnessof the inserts was confirmed by sequencing. Inserts were excisedand gel-purified before use. The cDNA probes for AML-1 and ${beta}$ -actin were kindly donated by Dr Kim Theilgaard-Mönch, Rigshospitalet (University of Copenhagen, Denmark). The C/EBP- ${alpha}$ probe was kindly provided by Dr Daniel Tenen, Harvard MedicalSchool (Boston, MA), and the probe for CLC protein was kindlyprovided by Dr Steven Ackerman, University of Illinois, Chicago.
Protein isolation and Western blotting
The cells were pretreated with diisopropyl fluorophosphate (DFP)and subsequently isolated by a guadinium-hydrochloride–basedmethod to rapidly inactivate cellular proteases according tothe manufacturer's recommendations (Trizol; Invitrogen). Equalamount of protein lysate was applied on 7% to 14% SDS gelsand transferred to nitrocellulose membranes (Amersham Biosciences).The source of the antibodies and the reaction conditions areshown in Table 2. The immune complexes were visualized by theenhanced chemiluminiscence (ECL) reaction (Amersham Biosciences).Equal loading was assessed by probing with an antibody against ${alpha}$ -tubulin.

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Table 2.. Source and reaction conditions of antibodies for Western blot analysis

   Results

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Isolation of neutrophil precursor populations
Previously, our laboratory developed a method for purificationof neutrophil precursors from human bone marrow by Percolldensity centrifugation to study the expression of neutrophil-specificgranule proteins.^19,26 By this method, the neutrophil precursorswere separated into 3 cell populations enriched in MBs/PMs,MCs/MMs, or BCs/SCs.^19,26 For the investigation of neutrophiltranscription factors it was, however, important that contaminationwith nonneutrophil cells be minimized since some transcriptionfactors are shared among different hematopoietic lineages.^9,11,28 An immuno-magnetic isolation step was therefore applied tothe cells purifed on Percoll density gradients. Since no neutrophil-specificmembrane marker that is expressed at all stages of granulopoiesisexists, we decided to use a depletion protocol with antibodiesdirected against plasma membrane proteins present on the erythroid(glycophorin-A), B-lymphoid (CD19), T-lymphoid (CD2 and CD3),monocytic (CD14), megakaryocytic (CD61), and natural killer(NK) cell (CD56) lineages. The membrane marker CD49d is expressedon mature eosinophils and on neutrophil precursors up to themetamyelocyte stage.²⁹ Antibodies against CD49d were thereforeincluded when purifying the BC/SC population to remove contaminatingeosinophils. Neutrophil granulocytes from peripheral blood(PMNs) were also included in the study as they represent themost mature form of this cell. The PMNs were isolated by Lymphoprepdensity centrifugation and further purified by removal of contaminatingeosinophils on a magnetically activated cell sorter (MACS)column with the use of anti-CD49d antibodies.
By inclusion of the immunobead purification step, the mean percentageof contaminating cells was reduced from 68%, 22%, 16%, and4.0% to 7.7%, 2.0%, 2.2%, and 0.7% for the MBs/PMs, MCs/MMs,BCs/SCs, and PMNs, respectively, as determined by flow cytometricanalysis (Figures 1, 2A; Table 3).

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Figure 1.. Flow cytometric analysis of the 4 neutrophil cell populations before and after MACS purification. (A) MBs/PMs. (B) MCs/MMs. (C) BCs/SCs. (D) PMNs. Separations are from Percoll-separated human bone marrow cells before (Ai,Bi,Ci,Di) and after (Aii,Bii,Cii,Dii) depletion of nonneutrophil cells.

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Figure 2.. Cytospin and Northern blot analysis of the neutrophil cell populations before and after MACS purification. (A) Cytospin preparations of cells from the 3 Percoll-separated bone marrow populations (MBs/PMs, MCs/MMs, and BCs/SCs) and peripheral blood granulocytes (PMNs) before and after MACS depletion of nonneutrophil cells. Cells were stained with May-Grünwald-Giemsa. (B) Cytospins of granulocytic populations from peripheral blood stained with May-Grünwald-Giemsa (MGG) and Fast Green/Nuclear Red. (Top) Total granulocytes isolated from peripheral blood by means of Lymphoprep. Neutrophils are dominant, but eosinophils are visible (characterized by their bilobed nucleus, intense red granules in MGG staining, and green granules in Fast Green staining,⁸⁴ respectively). (Middle) Total granulocytes depleted for CD49d-expressing cells. (Bottom) The CD49d⁺ fraction from total granulocytes highly enriched in eosinophils. (C) Northern blot of RNA from the 3 granulocytic populations. The blot was hybridized to C/EBP- ${epsilon}$ , CLC, and 18S.

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Table 3.. Flow cytometric determination of contaminating cells in the neutrophil cell preparations

A differential count of the 3 neutrophil precursor cell populationsshowed a distribution profile similar to that reported previously,^19,26 only demonstrating a slightly higher percentage of band cellsin the MC/MM fraction in this study (Table 4). To furtherensure that the distribution profile of the neutrophil precursorswas not biased by the MACS purification step, cells from the3 bone marrow populations and PMNs were analyzed for the presenceof granule protein mRNAs known to be found specifically inMBs/PMs (myeloperoxidase); MCs/MMs (lactoferrin); and BCs/SCsand PMNs (the fMLP-receptor).^19,26,30 As shown in Figure 3A-B,the distribution profile of the granule markers was as expectedand in accordance with previously published distribution profiles.^19,26,30

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Table 4.. Distribution of neutrophil precursors in the 3 Percoll-separated and MACS-depleted bone marrow populations

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Figure 3.. Northern blot analysis of the 4 neutrophil cell populations after MACS purification. (A) Northern blot of total RNA from the 4 MACS-depleted cell populations. The blot was hybridized with probes against the granule proteins MPO, lactoferrin, and fMLP-R, which are expressed specifically in MBs/PMs, MCs/MMs, and BCs/SCs and PMNs, respectively. (B) Schematic representation of the hybridization intensities from panel A. For each probe, the cell population showing maximal expression is given the value 1; the expression levels in the other cell populations are shown relative to this. All expression levels are normalized to the 18S level. (C) Relative hybridization intensities of 18S and ${beta}$ -actin in the 4 cell populations. Data are based on 12 (18S) or 17 ( ${beta}$ -actin) filters blotted with 5 µg RNA from each cell population. For each hybridization, the cell population with the strongest signal was given the value 1, and the other signal intensities were related to this.

To normalize transcript levels in Northern blots, hybridizationto glyceraldehyde-3-phosphate dehydrogenase (GAPDH), ${beta}$ -actin,or 18S transcripts is usually performed. Previously, we foundthat the level of GAPDH mRNA decreases with neutrophil maturation,and we therefore examined ${beta}$ -actin and 18S RNA levels to determinewhether they were a better choice. Relative hybridization intensitiesof 12 (18S) and 17 ( ${beta}$ -actin) Northern filters, each containing5 µg total RNA from the 4 neutrophil cell populations,are shown in Figure 3C. Levels of ${beta}$ -actin mRNA were approximately45% lower in MBs/PMs and PMNs than in the 2 other cell populations,whereas 18S appeared to be more evenly expressed, demonstrating,at most, 25% difference between any 2 cell populations. Forthis reason, we chose 18S for normalization of our transcripts.All data presented are the combined result of 3 hybridizations, each normalized to 18S. The distribution of transcription factorswas also examined by Western blotting. In this case, equalloading was assured by probing with an antibody against ${alpha}$ -tubulin.
When analyzing transcript levels, one should bear in mind thatonly the relative hybridization intensities of one probe withthe RNA on a single filter can be compared. Comparison of hybridizationlevels of one transcript with another (eg, PU.1 with C/EBP- ${alpha}$ )is not possible, as a stronger signal for one of the transcriptsdoes not necessarily reflect a higher level of that particularmRNA population, but may instead reflect differences in the size and labeling efficiency of the probe used. The same considerationsapply for immunoblots where the immune complexes are visualizedby ECL.
Transcript profiles for c-myb, AML-1, CDP, and GATA-1
Studies have demonstrated that c-myb, AML-1, CDP, and GATA-1are involved in neutrophil gene regulation prior to the promyelocyte-myelocytetransition. AML-1 and c-myb are required for hematopoietic development^9,11 and expression of early neutrophil markerssuch as the azurophil granule proteins MPO and elastase.^{31, 32, 33} GATA-1 is important for erythroid and eosinophil developmentbut can also be found in early myeloid precursors.^34,35 CDPis a transcriptional repressor that blocks expression of thegenes encoding specific granule proteins and glycoprotein 91^phox (gp91^phox) in MBs and PMs.¹²
A similar distribution profile was found for the AML1b (approximately7 kilobase [kb]) and AML1c (approximately 6.5 kb) transcripts,which arise from the AML1 gene by use of 2 different promoters,³⁶with highest mRNA levels in MBs/PMs and lower levels in moremature cells (Figure 4A-B). Also for c-myb, transcripts of2 different sizes were observed (Figure 4A). The 3.8-kb mRNA encodes a transcriptional activator, and the 2.5-kb mRNA an inhibitor.^37,38 Both splice products were abundant in the2 most immature cell populations and almost undetectable fromthe band cell stage onward. The amount of the largest c-mybtranscript (3.8 kb) was 3- to 4-fold larger in the MBs/PMs relativeto the MCs/MMs, whereas the opposite was the case for the 2.5-kbc-myb transcript, which increased 3-fold in the MCs/MMs comparedwith the MB/PM population. In contrast, a strong hybridizationsignal was measured for CDP mRNA in all 4 cell populationsand demonstrated no significant change in the transcript levelwith maturity (Figure 4A-B). The approximately 3.4-kb alternativelyspliced transcript encoding the protein CASP, which lacks theDNA-binding domains of CDP,³⁹ is most prominent in the MBs/PMsand decreases with maturity of the neutrophil granulocyte.Transcripts for GATA-1 were detected in MBs/PMs, but not inmore mature granulocytic cells. The signal was not due to contaminatingerythroid cells, which strongly express GATA-1,³⁴ as no hybridizationto the erythroid-specific transcript glycophorin-A was observed in the granulocytic precursors, whereas RNA from bone marrowcells depleted of neutrophil cells (but still containing erythrocyticprecursors) hybridized strongly (Figure 4A-B). Contaminationof MBs/PMs by eosinophils, which also express GATA-1 throughout differentiation,³⁵ cannot be ruled out. The nondetection ofGATA-1 in the other cell populations, however, demonstratesthat the more mature neutrophilic cells are uncontaminatedby eosinophils.

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Figure 4.. Northern and Western blot of AML-1, c-myb, CDP, CASP, GATA-1, and glycophorin-A. (A) Northern blot of total RNA from mature neutrophils and the 3 MACS-depleted populations of neutrophil precursors. The blot was hybridized with probes against AML-1, c-myb, CDP, GATA-1, and glycophorin-A. CASP is a splice variant of CDP. RNA from erythrocytes (ERY) was included as a positive control for glycophorin-A and GATA-1. (B) Schematic representation of the hybridization intensities from panel A. For each probe, the cell population showing maximal expression is given the value 1; the expression levels in the other cell populations are shown relative to this. All expression levels are mean values of 18S-normalized transcript levels from 3 different subjects. Standard deviations (SDs) are shown as error bars. (C) Western blot of AML-1, c-myb, and CDP. Equal loading was assessed by probing with an antibody against ${alpha}$ -tubulin. The arrows indicate the bands of the target proteins.

Transcript profiles for the family of C/EBP transcription factors
Members of the C/EBP transcription factor family are requiredfor proper neutrophil differentiation. Since homodimerizationand heterodimerization of different C/EBP family members aswell as functional substitution of one C/EBP dimer with anothercan occur,⁴⁰ we decided to examine the transcript profileof the entire C/EBP family (ie, C/EBP- ${alpha}$ , - ${beta}$ , - ${delta}$ , - ${epsilon}$ , - ${gamma}$ , and - ${zeta}$ ).⁴⁰Owing to high homology in the coding region, C/EBP probes weredesigned toward the 3'-region of the mRNA. The specificityof the probes was confirmed by a BLAST search (http://www.ncbi.nlm.nih.gov/blast/), which demonstrated that cross-reaction with other genes shouldnot be possible. The amount of C/EBP- ${alpha}$ transcript was highestin MBs/PMs and then declined to a 50% lower level in the moremature cells (Figure 5A-B). The 2 transcripts for C/EBP- ${gamma}$ ,which probably encode the same protein,⁴¹ had identical distributionprofiles with strong expression in MBs/PMs and barely detectablelevels from myelocytes onward (Figure 5A-B). The peak level of the C/EBP- ${epsilon}$ mRNA was found in MCs/MMs, with a considerablylower level in the other cell populations (Figure 5A-B). Transcriptsfor C/EBP- ${beta}$ , C/EBP- ${delta}$ , and C/EBP- ${zeta}$ were only abundant in the mostmature neutrophil precursors of the bone marrow and in peripheralblood granulocytes (Figure 5A-B). A 5000-nucleotide (nt) bandwas observed following prolonged exposure of the C/EBP- ${beta}$ blot.The distribution profile of this band was similar to that ofC/EBP- ${alpha}$ (data not shown).

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Figure 5.. Northern and Western blot of C/EBP- ${alpha}$ ,- ${beta}$ ,- ${delta}$ ,- ${epsilon}$ ,- ${gamma}$ , and - ${zeta}$ . (A) Northern blot of total RNA from mature neutrophils and the 3 MACS-depleted populations of neutrophil precursors. The blot was hybridized with probes against C/EBP- ${alpha}$ , - ${beta}$ , - ${delta}$ , - ${epsilon}$ ,- ${gamma}$ , and - ${zeta}$ . (B) Schematic representation of the hybridization intensities from panel A as in Figure 4. (C) Western blot of C/EBP- ${alpha}$ ,- ${beta}$ ,- ${delta}$ ,- ${epsilon}$ ,- ${gamma}$ , and - ${zeta}$ . Equal loading was assessed by probing with an antibody against ${alpha}$ -tubulin (not shown). The arrows indicate the bands of the target proteins. The asterisk denotes an unspecific band in the C/EBP- ${gamma}$ blot.

The 2 C/EBPs examined most extensively with regard to theirrole in granulocytic differentiation are C/EBP- ${alpha}$ and C/EBP- ${epsilon}$ .The data presented here for C/EBP- ${alpha}$ fit those of earlier reports,^17,42 whereas the expression profile of C/EBP- ${epsilon}$ contrasts with previous findings in which an expression of C/EBP- ${epsilon}$ in peripheral blood granulocytes was demonstrated.^15,43 Since the only majorcellular contaminant of standard Lymphoprep-isolated granulocytesis eosinophils, we examined whether the previously reported C/EBP- ${epsilon}$ expression in the PMN fraction could result from thesecells. As shown in Figure 2B-C, this was indeed the case:RNA from CD49⁺ cells (ie, eosinophils) hybridized stronglyto the C/EBP- ${epsilon}$ probe, whereas no C/EBP- ${epsilon}$ transcript was detectedin the CD49^– cells (ie, neutrophils). The presence ofeosinophils only in the CD49⁺ and PMN cell populations, andnot in the CD49^– cells, was confirmed by the strong expressionof the eosinophil-specific transcript CLC only in the formercell populations.⁴⁴
Transcript profiles for PU.1, Elf-1, c-jun, and c-fos
The ets factors PU.1 and Elf-1 are both found in neutrophils,and a requirement for PU.1 in early granulopoiesis has been demonstrated.^20,22,23 We therefore chose to examine the expressionprofile of these 2 transcription factors. As c-jun acts asa coactivator of PU.1 in monocytic differentiation,⁴⁵ we decidedto include this factor, as well as c-fos, a well-documented dimerization partner of c-jun.⁴⁶ PU.1 transcript was foundat all stages of granulopoiesis and increased gradually withmaturity, reaching the highest level in peripheral blood PMNs (Figure 6A-B). The transcript profile of Elf-1 was more complex,with a lower mRNA level in MCs/MMs compared with the othercell populations. A similar pattern was observed for the c-jun mRNA, where the transcript level also diminishes at the MC/MMstage. The c-fos transcript, on the other hand, was prominentonly in BCs/SCs and peripheral blood granulocytes (Figure 6A-B).

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Figure 6.. Northern and Western blot of PU.1, Elf-1, c-jun, and c-fos. (A) Northern blot of total RNA from mature neutrophils and the 3 MACS-depleted populations of neutrophil precursors. The blot was hybridized with probes against PU.1, Elf-1, c-jun, and c-fos (B) Schematic representation of the hybridization intensities from panel A as in Figure 4. (C) Western blot of PU.1, Elf-1, c-jun, and c-fos. Equal loading was assessed by probing with an antibody against ${alpha}$ -tubulin (not shown). The arrows indicate the bands of the target proteins.

Protein profiles of transcription factors
To examine whether the protein profiles matched the mRNA profilesfor the 14 transcription factors, we also performed Westernblot analysis. The protein profiles of AML-1, PU.1, Elf-1,c-jun, c-fos, CDP, C/EBP- ${gamma}$ , and C/EBP- ${delta}$ were very similar totheir mRNA profiles (Figures 4, 5, 6). For c-myb, only thelarge (75-kDa) activator form³⁷ was observed, indicatingeither that the 2.5-kb mRNA also encodes the 75-kDa activatoror that the concentration of the inhibitory form is below the detection limit of our antibody (Figure 4C). Although somemRNA for c-myb is found in MCs/MMs, we were able to detecta strong c-myb signal only by Western blotting in MBs/PMs. We were unable to detect CASP with our CDP antibody as the antibodywas directed against a part of CDP that is not contained inCASP.
Both the 42- and 30-kDa isoforms of C/EBP- ${alpha}$ , representing the transactivation-competent full-length and the N-truncated transdominant repressor forms of the protein, respectively,⁴⁷ were detected(Figure 5C). The larger isoform was most prominent in all cellpopulations, indicating that the transactivating competenceof C/EBP- ${alpha}$ was maintained thoughout granulopoiesis. Two formsof C/EBP- ${beta}$ have been reported in liver cells (a 43-kDa activatorand a 20-kDa form that attenuates transcriptional activation of the 43-kDa isoform).⁴⁸ Our antibody should detect bothproteins, but only the 43-kDa type was seen, indicating thatonly the transactiving type of C/EBP- ${beta}$ is present in the neutrophilprecursors. Three isoforms of C/EBP- ${epsilon}$ , of 32, 27, and 14 kDa, were seen in the neutrophil precursors. As for the mRNA, thevast majority of C/EBP- ${epsilon}$ protein was found in MCs/MMs (Figure 5C).The 32-kDa transactivation-competent form was the mostprominent of the 3 C/EBP- ${epsilon}$ isoforms, and the 27- and 14-kDaforms, which lack transactivating potential, constituted onlya very minor portion of the C/EBP- ${epsilon}$ proteins.^43,49 The 14-kDaform was seen only following prolonged exposure. The same expressionpattern of C/EBP- ${epsilon}$ was found with another C/EBP- ${epsilon}$ antibody (Table 2).

   Discussion

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

It is well established that a finely tuned timing of transcriptionfactor expression is pivotal for correct neutrophil differentiation.Expression of the receptors for granulocyte colony-stimulatingfactor (G-CSF) and interleukin 6 (IL-6),⁵⁰ the azurophiland specific granule proteins,^{10,20,31, 32, 33} and transcriptional regulators such as PU.1, C/EBP- ${delta}$ , and C/EBP- ${epsilon}$ ^7,24,51 is governedby the emergence and/or disappearance of key transcription factors. Current knowledge about the expression pattern of transcription factors during granulopoiesis has been obtained primarily fromwork with neutrophil cell lines, bone marrow–derivedCD34⁺ cells, and murine knockout models. Although much informationcan be gained from such experiments, the data may not alwaysbe a true representation of the in vivo situation owing tothe previously mentioned limitations of these model systems.For this reason, we decided to examine the in vivo profile of transcription factors during granulopoiesis in 4 distinct cellpopulations of different maturity from human bone marrow andperipheral blood.
It is possible to obtain a finely tuned transcription factorprofile in relation to neutrophil maturation on the basis ofthe mRNA and protein levels in the 4 neutrophil cell populationsif the following assumptions are fulfilled: First, it is assumedthat the relative level of 18S mRNA is constant in the cellsin such a way that it can be used to normalize the levels ofmRNA for the transcription factors (Figure 3C). Second, ifthe level of a specific mRNA is low in one cell populationand increases in the next cell population, which contains moremature cells, then it is assumed that the low mRNA level inthe more immature cells is not due to a uniformly low levelin all the cells, but instead to a high level in the most mature cells of this cell population, resulting in a gradual increasein the mRNA level. The alternative interpretation would bethat uniform transcript levels exist in all cells of the population,despite the fact that these cover a span of maturation artificiallysampled into the same population by the limitations set bythe density of the separating Percoll medium,⁵² and that steepchanges in the mRNA level occur at the transition between thedifferent cell populations. Third, although the presence ofa particular transcript does not necessarily imply the synthesisof the concurrent protein and, conversely, the disappearanceof a given mRNA does not always mean that the protein it encodesalso disappears, coexpression of an mRNA and its cognate proteinis usually observed for cytosolic proteins.⁵³ Our proteinexpression data demonstrate that this indeed is the case forthe transcription factors investigated here. This is in contrastto granular proteins such as MPO and lactoferrin, which arestored in granules (and thus protected from degradation) until exocytosed.³⁰ In this case, the protein can be detected longafter the transcript has disappeared.^19,26 If the assumptionis made that gradual changes of mRNA and protein levels occur,then the hypothetical distribution profile depicted in Figure 7can be made. Although alternative splicing and translation,as well as posttranslational modifications such as phosphorylation,acetylation, and proteolytic processing, may also influencethe activity of a transcriptional regulator and thus have tobe taken into consideration, we believe that the in vivo expressionpattern of the 14 transcription factors presented here can toa large extent explain the temporal regulation of stage-specificallyexpressed genes during granulopoiesis.

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Figure 7.. Hypothetical distribution scheme of neutrophil transcription factors during granulopoiesis. Theoretical distribution scheme of the transcription factors examined in this work based on the data presented in Figures 4, 5, and 6.

In accordance with previous reports,^31,54 AML-1 and c-mybwere found to be strongly expressed at the early stages of neutrophil differentiation, which fits with the requirementof both these transcription factors for the expression of azurophilgranule proteins such as MPO and elastase.^{31, 32, 33} Down-regulationof c-myb after the myelocyte stage was anticipated since c-mybblocks differentiation and induces proliferation and was thereforeexpected to disappear at the stage of differentiation wherecell cycle arrest and initiation of terminal neutrophil differentiationtakes place.¹ The same consideration is likely to apply toAML-1, as it also stimulates proliferation (in part by repressingtranscription of the cell cycle inhibitor p21^Cip1).⁵⁵
The level of CDP remained almost unaltered during neutrophil differentiation, which was surprising since CDP activity wasexpected to disappear at the myelocyte stage where expressionof specific granule proteins is initiated. The repressive effectof CDP in granulopoiesis has been demonstrated in HL60 cellsand murine 32Dcl3 cells where transcription of the genes encoding gp91phox⁵⁶ and specific granule proteins was inhibited bya continued expression of CDP—both by direct inhibitionof the genes^12,57 and indirectly by inhibiting the synthesisof C/EBP- ${epsilon}$ ,⁵¹ which is essential for specific granule proteingene expression.^10,21 Recently, it has been shown that CDPprotein is synthesized in HL60 cells during the entire processof granulocytic differentiation. However, the binding capabilityof CDP disappears in the more mature cells owing to phosphorylationof the protein.⁵⁸ A similar inactivation of CDP may occurin myelocytes in vivo. This suggests that the observed repressionof specific granule gene activity in cell cultures that overexpressCDP is due to an overload of the phosphorylating capacity ofthese cells rather than to a continued CDP synthesis. No function has been ascribed to CASP, but it has been speculated thatit may regulate CDP activity since CDP and CASP are able to heterodimerize.^39,59
C/EBP- ${alpha}$ is required for granulopoiesis, as demonstrated by the selective block in neutrophil differentiation in mice witha targeted disruption of the C/EBP- ${alpha}$ gene⁸ and the inductionof terminal granulocytic differentiation in 32Dcl3 cells inresponse to induced expression of C/EBP- ${alpha}$ .⁷ C/EBP- ${alpha}$ is alsoneeded for gene expression of both the early neutrophil markersMPO and elastase^33,60 and of the receptors for IL-6 and G-CSF,which are also expressed at later stages of neutrophil development.^7,50 In agreement with these requirements, C/EBP- ${alpha}$ is found throughout neutrophil differentiation. A similar expression pattern forC/EBP- ${alpha}$ has been observed for HL60 cells and NB4 cells inducedto granulocytic differentiation by retinoic acid.⁴² This isin contrast to the transcript levels found during differentiationof adipocytes and hepatocytes, where a steep increase in theC/EBP- ${alpha}$ mRNA level is observed when proliferation ceases andterminal differentiation is initiated.⁶¹ The proposed antiproliferativeeffect of C/EBP- ${alpha}$ seen in the latter cell types⁶² is thereforenot likely to be relevant in neutrophils.
The levels of both C/EBP- ${beta}$ , C/EBP- ${delta}$ , and C/EBP- ${zeta}$ increased dramaticallyat the stage where proliferation ceases in neutrophils (ie, metamyelocytes¹). Since in other cell systems these proteinsare associated with termination of proliferation,^63,64 a rolefor these C/EBPs (rather than C/EBP- ${alpha}$ ) in neutrophil cell cycle arrest can be envisaged. It is, however, also possible thatC/EBP- ${beta}$ , C/EBP- ${delta}$ , and/or C/EBP- ${zeta}$ are required for transcriptionalinitiation of late neutrophil markers such as gelatinase, fMLP-receptor,CD35, and Toll-like receptor 4 (TLR4).^19,26,65 C/EBP- ${gamma}$ lacksa transactivating domain and can inhibit the transactivatingpotential of other C/EBPs.^40,66 A high expression of C/EBP- ${gamma}$ has been associated with proliferation although the mechanismby which it governs this is unknown.^66,67 The strong expressionof C/EBP- ${gamma}$ in only the highly proliferative immature neutrophilprecursors supports such a function also in granulopoiesis.
Previous publications have demonstrated peak levels of C/EBP- ${epsilon}$ mRNA in promyelocyte and late myeloblast-like cell lines anda sustained expression in PMNs from peripheral blood.^15,43 This is in contrast to the findings in this report in whichthe peak C/EBP- ${epsilon}$ level is found in MCs/MMs. Our data, however,fit the phenotype of C/EBP- ${epsilon}$ knockout mice¹⁰ and patients with specific granule deficiency,²¹ where the earliest stepsof neutrophil differentiation are unaffected whereas expressionof specific granules at the myelocytic stage is completely abolished owing to the lack of C/EBP- ${epsilon}$ . The peak expression of C/EBP- ${epsilon}$ in MCs/MMs and its disappearance in more mature cellscould thus explain the confined expression of the specificgranule genes in myelocytes and metamyelocytes.¹⁹ The disparitybetween the C/EBP- ${epsilon}$ mRNA profiles in bone marrow–derivedneutrophil precursors and in cell cultures may be due to anerroneous induction of C/EBP- ${epsilon}$ transcription by retinoic acid¹⁴or G-CSF⁶ as both these substances are commonly added to thegrowth media to induce neutrophil differentiation of cell cultures.Our data furthermore indicate that the previously reportedpresence of C/EBP- ${epsilon}$ transcript in peripheral blood neutrophilsis caused by contaminating eosinophils since a complete lackof measurable C/EBP- ${epsilon}$ signal by Northern blot analysis was demonstrated following removal of the eosinophils from this cell population (Figure 2B-C). We only detected a C/EBP- ${epsilon}$ mRNA of approximately1.4 kb by Northern blotting and were not able to identify theearlier reported C/EBP- ${epsilon}$ splice variant at 2.4 kb, even followingprolonged exposure of the Northern blot.⁴³ As our probe wasdesigned to recognize the 3'-end of the C/EBP- ${epsilon}$ mRNA, whichis included in all splice variants, our data indicate eitherthat the 2.4 kb-splice product is not made in vivo or thatthe amount produced is so low that a more sensitive detectionmethod such as reverse transcriptase–PCR (RT-PCR) isrequired for its identification.
Targeted disruption of PU.1 abolishes or severely impairs theproduction of neutrophils.^22,23 The few neutrophils formedin the PU.1 knockout mice are able to differentiate morphologicallyto PMNs but fail to express specific granule genes and gp91^phox.²⁰ Although mRNAs for azurophil granule proteins were detectedin the PU.1 null mice, demonstrating that PU.1 was not essentialfor their transcription, other experiments have shown thatPU.1 is required for optimal gene expression of early neutrophilmarkers such as MPO, proteinase-3, and elastase^33,60,68,69 as well as of very late markers such as TLR4.^65,70 Together,these data fit the transcript pattern observed here where PU.1is found at all stages of neutrophil differentiation. The expressionprofile of the second ets factor included in this study, Elf-1,was quite different from that of PU.1, demonstrating that etsfactors are also expressed in an individual manner. Elf-1 isunable to functionally substitute for PU.1 and has been foundto cooperate with PU.1 in the expression of the nicotinamideadenine dinucleotide phosphate (NADPH)–oxidase component gp91^phox, indicating an individual regulatory specificity ofthis transcription factor.^71,72
Transcriptional competence of PU.1 during monocytic differentiationis dependent upon c-jun as a non–DNA-binding coactivator.⁷³The same may apply to neutrophil differentiation, and the expressionpattern demonstrated here indicates that c-jun would be availablefor such a function during late granulopoiesis. Expressionof c-fos, which is often found heterodimerized with c-jun inthe transcriptional transactivator complex AP-1,⁴⁶ is also primarily found at the late stages of development and in PMNsfrom peripheral blood. It is possible that c-fos, through heterodimerizationwith c-jun, can modulate the transcriptional capacity of c-jun—eitherby reducing the transactivating potential of PU.1 or by forminga transcriptional active AP-1 complex or by both.⁷³ Sincethe "active concentration of PU.1" in the cell is criticalfor its transactivating potential,²⁸ a careful titrationof the c-jun/PU.1 level may be required for proper transcriptionalregulation by PU.1.
On the basis of the data presented here and in the literature,the following course of events during granulopoiesis can beenvisaged: In myeloblasts, low concentrations of PU.1 and highamounts of C/EBP- ${alpha}$ favor granulocytic differentiation over monocytic differentiation.^42,73 AML-1 and c-myb direct the expressionof azurophil granule protein genes such as MPO and NE. Followingonset of granulopoiesis, C/EBP- ${alpha}$ may stimulate additional PU.1transcription, which, when initiated, increases further, owing to a positive-feedback mechanism.⁷⁴ In myelocytes, the decreasein AML-1 and c-myb levels halts expression of azurophil granuleprotein genes. Furthermore, reduction of the active CDP levelcauses its repression of the genes for C/EBP- ${epsilon}$ , gp91^phox, andthe specific granule proteins to be relieved. C/EBP- ${epsilon}$ then inducestranscription of the specific granule protein genes and of C/EBP- ${delta}$ .²⁴ In band cells, down-regulation of C/EBP- ${epsilon}$ causesthe cessation of specific granule protein gene transcription.Cell cycle arrest and initiation of terminal neutrophil differentiationin metamyelocytes may be a result of the combined disappearanceof the pro-proliferative transcription factors c-myb, AML-1,C/EBP- ${gamma}$ , and CDP (which inhibits p21^cip1)⁷⁵ and the emergenceof potential antiproliferative factors such as C/EBP- ${delta}$ and C/EBP- ${zeta}$ .At present, it is unknown which transcription factors regulatethe timed onset of very late neutrophil markers such as the fMLP-receptor, TLR2, TLR4, and CD35, which are all preferentiallyexpressed in band cells, segmented cells, and PMNs. The datapresented in this work indicate that C/EBP- ${beta}$ , C/EBP- ${delta}$ , and C/EBP- ${zeta}$ may play a role. In conclusion, the transcription factor profilesdescribed here may to a large extent explain the timed geneexpression of granule protein genes and cell cycle arrest duringgranulocytic differentiation.