Genome Architecture of the Human {beta}-Globin Locus Affects Developmental Regulation of Gene Expression

doi:10.1128/MCB.25.20.8765-8778.2005

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Molecular and Cellular Biology, October 2005, p. 8765-8778, Vol. 25, No. 20
0270-7306/05/$08.00+0 doi:10.1128/MCB.25.20.8765-8778.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.

Genome Architecture of the Human ß-Globin Locus Affects Developmental Regulation of Gene Expression

Susanna Harju,¹ Patrick A. Navas,² George Stamatoyannopoulos,² and Kenneth R. Peterson¹^,3^*

Department of Biochemistry and Molecular Biology,¹ Department of Anatomy and Cell Biology, University of Kansas Medical Center, Kansas City, Kansas 66160,³ Division of Medical Genetics, University of Washington, Seattle, Washington 98195²

Received 16 January 2005/ Returned for modification 10 February 2005/ Accepted 21 July 2005

ABSTRACT

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

To test the role of gene order in globin gene expression, mutanthuman ß-globin locus yeast artificial chromosome constructswere used, each having one additional globin gene encoding a"marked" transcript ( ${varepsilon}$ ^m, ${gamma}$ ^m, or ß^m) integrated at differentlocations within the locus. When a ß^m-globin genewas placed between the locus control region (LCR) and the ${varepsilon}$ -globingene, ß^m-globin expression dominated primitive anddefinitive erythropoiesis; only ß^m-globin mRNA wasdetected during the fetal and adult definitive stages of erythropoiesis.When an ^A ${gamma}$ ^m-globin gene was placed at the same location, ^A ${gamma}$ ^m-globinwas expressed during embryonic erythropoiesis and the fetalliver stage of definitive erythropoiesis but was silenced duringthe adult stage. The downstream wild-type ${gamma}$ -globin genes werenot expressed. When an ${varepsilon}$ ^m-globin gene was placed between the ${delta}$ - and ß-globin genes, it remained silent during embryonicerythropoiesis; only the LCR-proximal wild-type ${varepsilon}$ -globin genewas expressed. Placement of a ß^m-globin gene upstreamof the ^G ${gamma}$ -globin gene resulted in expression of ß^m-globinin embryonic cells and in a significant decrease in expressionof the downstream wild-type ß-globin gene. These resultsindicate that distance from the LCR, an inherent property ofspatial gene order, is a major determinant of temporal geneexpression during development.

INTRODUCTION

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

The human ß-globin locus consists of five functionalglobin genes, which are expressed during ontogeny in the orderin which they lie on the chromosome, 5'- ${varepsilon}$ -^G ${gamma}$ -^A ${gamma}$ - ${delta}$ -ß-3'.During development, two switches occur in globin gene expression,from embryonic to fetal, coinciding with the transition fromembryonic to definitive erythropoiesis, and from fetal to adultaround the perinatal period. High-level expression of the ß-likeglobin genes is dependent upon both gene-proximal and -distalcis-acting regulatory elements. The major distal regulatoryelement is the locus control region (LCR). It contains fiveDNase I-hypersensitive sites (5'HS1 to -5) (42) and is located6 to 22 kb upstream of the ${varepsilon}$ -globin gene. Functions of LCRs includetissue-specific enhancement of gene expression, chromatin-openingactivity, insulation of the locus from the effects of surroundingchromatin, and determination of replication timing and choiceof origin used (26, 27). It is currently assumed that LCR sequences,together with their cognate transcription factors and coactivators,form an active site "hub" that interacts with gene-proximalelements and their bound transcription factors to form a transcriptosomespecific for the globin gene(s) expressed at each developmentalstage (8, 20, 26, 34). Less-conserved sequences between theHS cores also may function in globin gene regulation (19), perhapsby acting to constrain the complex conformation.

Because the spatial arrangement of the ß-like globingenes parallels their temporal expression pattern, it has beenproposed that gene order or proximity to the LCR may be a determinantof the order of globin gene expression during development. Previousstudies have established an effect of either gene order or distancefrom the LCR (10, 18, 39, 44). Data from transgenic mice producedwith ${alpha}$ - and ß-globin genes linked at various distancesto the LCR demonstrated that proximity to the LCR increasedthe probability of interaction with the LCR (18). The effectof gene order on globin gene developmental regulation was testedby producing transgenic mice containing two tandemly arranged ${gamma}$ - or ß-globin or ${gamma}$ ß- and ß ${gamma}$ -globingenes linked to a µLCR (39). These studies showed thatthe trans-acting environment is the primary determinant forcorrect developmental control but that proximity to the LCRalso is involved in regulation. The effect of distance fromthe LCR was analyzed using a larger 70-kb ß-globinlocus in two linked cosmids (10). When the ${varepsilon}$ -globin gene wasreplaced with a marked ß-globin (ß^m) gene,ß-globin expression was sustained throughout development.In contrast, when the ß^m-globin gene was placed upstreamof the ${delta}$ -globin gene, ß^m-globin gene expression accountedfor 75% of total ß-globin gene expression (ß^m+ ß^wt). Inversion of the whole locus relative to theLCR in ß-globin locus yeast artificial chromosome(ß-YAC) transgenic mice resulted in ß-globingene expression throughout development, with no ${varepsilon}$ -globin geneexpression and limited ${gamma}$ -globin gene expression during primitiveerythropoiesis, again suggesting that proximity to the LCR isa determinant of globin gene expression (44).

In this study we sought to further test the role of spatialgene order in the control of globin gene expression using ß-YACtransgenic mice carrying constructs containing one additionalglobin gene encoding a "marked" transcript ( ${varepsilon}$ ^m, ${gamma}$ ^m, or ß^m)integrated at a different locations within the locus. Our resultsindicate that distance from the LCR as determined by gene order,in addition to gene-proximal cis-acting elements, determinesthe appropriate developmental expression of ß-likeglobin genes.

MATERIALS AND METHODS

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

YAC constructs. A 213-kb ß-YAC containing the human ß-globinlocus (Fig. 1) was utilized for all experiments (16, 36, 38).This ß-YAC was previously estimated to be 248 kb,but with a nearly complete sequence of the human ß-globinlocus region now available (http://globin.cse.psu.edu) (4),the size was more accurately determined. An approximately 6-kbsequence gap still exists downstream of 3'HS1 in the latestrelease of the human genome sequence. The numerical coordinatesused in construct descriptions below are based upon GenBankfile U01317 unless indicated otherwise. All of the YAC modificationswere introduced by yeast integrating plasmid (YIP)-mediated"pop-in," "pop-out" or two-step gene replacement methods ofhomologous recombination as previously described (1, 31, 38).Briefly, for the "pop-in," "pop-out" method, YIP clone DNA waslinearized with the indicated restriction enzyme and transformedinto spheroplasted Saccharomyces cerevisiae strain AB1380 containingthe 213-kb ß-YAC. Transformants were selected foruracil prototrophy on complete medium (CM), and correct recombinationwas determined by Southern blot hybridization analysis. Spontaneousexcision of the YIP was induced by overnight growth in nonselectiveCM. The yeast cells were plated on 5-fluoroorotic acid (5-FOA)CM plates to select for loss of the URA3 gene residing on theYIP vector, which results in 5-FOA resistance. The two-stepgene replacement protocol utilized the same selection stepsas the "pop-in," "pop-out" method, except two fragments withrecombinogenic ends were used in sequential transformations.The first fragment contained the target sequence and the markedglobin gene interrupted with the URA3 cassette; the second fragmentwas identical, but it lacked the URA3 gene. Correct recombinantswere confirmed by Southern blot hybridization analysis and PCR.

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FIG. 1. Gene order constructs. The human ß-globin locus is shown as a line, the genes are indicated as rectangles, and the DNase I-hypersensitive sites are marked with arrows. The various marked globin genes and their sites of integration are shown with arrows linking them to the site of integration.

ß^m 5' ${varepsilon}$ ß-YAC. A 4.1-kb ß^m-globin HpaI-XbaI fragment (GenBank coordinates61340 to 65439) was inserted into an EcoRV site between 5'HS1and the ${varepsilon}$ -globin gene at GenBank coordinate 15182 (Fig. 1). Themark in the ß^m-globin gene was an 8-bp ClaI linkerligated into an S1 nuclease-blunted NcoI site of the ß-globinpromoter at GenBank coordinate 62185 (11). A net increase of4 bp resulted, and the linker was constructed in such a waythat the initiation methionine codon was preserved. A 3,139-bpBglII-HindIII fragment (GenBank coordinates 13769 to 16908)was isolated from pHSI (gift from Q. Li) and ligated into BamHI-HindIII-cutand calf intestinal alkaline-phosphatase-treated pUC19 to producepUC-5' ${varepsilon}$ . The 4.1-kb HpaI-XbaI ß^m-globin fragment wasisolated from pSP73ß^m (11), the XbaI overhang filledwith E. coli polymerase I Klenow enzyme and ligated into EcoRV-cutand phosphatase-treated pUC-5' ${varepsilon}$ , resulting in pUC ß^m5' ${varepsilon}$ . An 1,166-bp HindIII-cut and Klenow enzyme-filled URA3 fragmentwas isolated from YEP24-neo (gift from C. Huxley) and ligatedinto BamHI-cut, Klenow enzyme-filled and phosphatase-treatedpUC ß^m 5' ${varepsilon}$ to generate pUC ß^m::URA3 5' ${varepsilon}$ .This vector was digested with PvuII to yield an 8,282-bp fragmentencompassing the ß^m::URA3 5' ${varepsilon}$ insert and two smallerfragments bearing the pUC19 plasmid vector sequence. This 8.3-kbfragment was used to transform yeast; selection was for uracilprototrophy. For the second transformation and recombination,a 2,116-bp ClaI-PstI fragment containing a portion of the ß^m-globingene (GenBank coordinates 62202 to 64319) was purified fromdigested pUC ß^m 5' ${varepsilon}$ ; selection was for 5-FOA resistance.Wild-type and marked gene transcripts in ß-YAC transgenicmice were distinguished by RNase protection analysis (RPA) orreverse transcriptase-PCR (RT-PCR) coupled with restrictionfragment length polymorphism (RFLP) analysis.

ß^m 5' ^G ${gamma}$ ß-YAC. A 4.1-kb HpaI-XbaI ß^m fragment was inserted 5' ofthe ^G ${gamma}$ -globin gene into a BglII site at GenBank coordinate 32837(Fig. 1). A 3,167-bp XbaI fragment 5' to the ^G ${gamma}$ -globin gene (GenBankcoordinates 32011 to 35178) was purified from pA-36 (gift fromB. Forget) and ligated into the XbaI-digested and phosphatase-treatedYIP vector pRS406 (Stratagene, La Jolla, CA) to produce pRS-5'^G ${gamma}$ . The 4.1-kb HpaI-XbaI ß^m-globin fragment was preparedas described in the preceding section and ligated into BglII-cut,Klenow enzyme-filled and phosphatase-treated pRS-5' ^G ${gamma}$ to producepRS ß^m 5' ^G ${gamma}$ . This YIP was linearized with Tth111Iprior to transformation of ß-YAC-bearing yeast. Differentialanalysis of ß^m- and ß^wt-globin transcriptsin murine lines was as described in the preceding section forthe ß^m 5' ${varepsilon}$ ß-YAC construct.

^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YAC. A 5.4-kb ^A ${gamma}$ ^m-globin SspI fragment (GenBank coordinates 38683to 44077) was inserted at the same EcoRV site described forthe ß^m 5' ${varepsilon}$ ß-YAC construct (Fig. 1). The^A ${gamma}$ ^m-globin gene contains a six-base-pair deletion at +21 to +26relative to the ^A ${gamma}$ -globin translation start site (41). A 3,139-bpBglII-HindIII fragment (GenBank coordinates 13769 to 16908)was isolated from pHSI and ligated into BamHI-HindIII-cut andcalf intestinal alkaline phosphatase-treated pBluescript KS+(Stratagene, La Jolla, CA) to produce pBS-5' ${varepsilon}$ . The 5.4-kb SspI-SalIfragment encompassing the ^A ${gamma}$ ^m-globin gene was isolated from pUC19^A ${gamma}$ ^m (+) (39) and ligated into EcoRV-digested and phosphatase-treatedpBS-5' ${varepsilon}$ to produce pBS ^A ${gamma}$ ^m 5' ${varepsilon}$ . An 8.5-kb SalI-NotI fragmentencompassing the ^A ${gamma}$ ^m 5' ${varepsilon}$ insert was isolated from pBS ^A ${gamma}$ ^m 5' ${varepsilon}$ and subcloned into SalI-NotI-digested and phosphatase-treatedpRS406 to produce pRS ^A ${gamma}$ ^m 5' ${varepsilon}$ . This YIP construct was linearizedwith PshAI (GenBank coordinate 16300) prior to transformationof yeast and recombination into the ß-YAC. Differentialanalysis of ^A ${gamma}$ ^m- and ^A ${gamma}$ ^wt-globin transcripts in transgenic mouselines was as described for the ß^m 5' ${varepsilon}$ ß-YACconstruct.

${varepsilon}$ ^m 3' ${delta}$ ß-YAC. A 3.7-kb EcoRI ${varepsilon}$ ^m-globin fragment (GenBank coordinates 17482to 21233) was inserted between the ${delta}$ - and ß-globingenes in a HindIII site at GenBank coordinate 59641 (Fig. 1).The mark is an eight-base-pair XhoI linker inserted in a PvuIIsite at GenBank coordinate 19524 (Q. Li, personal communication).A 2,595-bp EcoRI fragment encompassing sequence 3' to the ${delta}$ -globingene (GenBank coordinates 58034 to 60629) was isolated fromp ${delta}$ BglII and ligated into EcoRI-digested and phosphatase-treatedpUC19, in which the HindIII site had been previously ablatedby digestion with HindIII, Klenow enzyme filling of the 5' overhangs,and religation to generate pUC-3' ${delta}$ . A 3,770-bp EcoRI fragmentencompassing the ${varepsilon}$ -globin gene was isolated from p ${varepsilon}$ 3.7 (2), Klenowenzyme filled, and ligated in HindIII-cut, Klenow enzyme-filledand phosphatase-treated pUC-3' ${delta}$ to produce pUC ${varepsilon}$ 3' ${delta}$ . A 1,516-bpClaI-SpeI fragment encompassing the ${varepsilon}$ -globin mark was purifiedfrom p ${varepsilon}$ 3.7^m (K. R. Peterson, unpublished construct) and ligatedinto ClaI-SpeI-cut and phosphatase-treated pUC ${varepsilon}$ 3' ${delta}$ to generatepUC ${varepsilon}$ ^m 3' ${delta}$ . The 6,370-bp EcoRI fragment containing the entireinsert from pUC ${varepsilon}$ ^m 3' ${delta}$ was subcloned into EcoRI-digested andphosphatase-treated pRS406 to produce pRS ${varepsilon}$ ^m 3' ${delta}$ . A PmlI site(GenBank coordinate 60366) was used to linearize this YIP vectorprior to transformation of yeast and "pop-in," "pop-out" recombination.Measurement of ${varepsilon}$ ^m- and ${varepsilon}$ ^wt-globin transcripts in transgenic micewas as described above for the ß^m 5' ${varepsilon}$ ß-YACconstruct.

YAC purification and transgenesis. Purification of ß-YAC DNAs for microinjection wasperformed as described previously (16, 35-38). Briefly, pulsed-fieldgel electrophoresis of preparative high-mass DNA agarose plugswas used to fractionate yeast chromosomes and the ß-YAC,followed by electrophoretic concentration of the YAC DNA ina 4% low-melting-point agarose gel, ß-agarase digestionof the concentrated YAC DNA plugs, and filtration of the liquefiedagarose solution through a 0.22-µm syringe filter in high-saltmicroinjection buffer. Purified and filtered YAC DNAs were microinjectedinto fertilized mouse oocytes (C57/Bl6) and then transferredto pseudopregnant foster mothers to produce transgenic mice.Transgenic animals were identified by PCR analysis of tail biopsyDNA. Founders were bred with nontransgenic mice to produce F₁progeny; these in turn were bred to obtain F₂ staged embryos,fetuses, and adults. All structure-function analyses were carriedout beginning with the F₂ generation.

Structural analysis of transgene integrity and copy number determination. Structural analysis of ß-YAC transgenes was performedto assess the integrity and colinearity of transgenes as describedpreviously (31, 38). High-molecular-weight DNA embedded in agarosewas prepared, and slices were digested with SfiI. Digested DNAwas fractionated by pulsed-field gel electrophoresis and transferredto a Zeta-probe charged nylon membrane (Bio-Rad, Hercules, CA)by capillary blotting. Strips representing individual lanesof the gel were cut from the blot, and each one was hybridizedwith one of the following ³²P-radiolabeled probes: 0.7-kb PstI5'HS3, 1.9-kb HindIII 5'HS2, 1.8-kb XbaI 5'HS1, 3.7-kb EcoRI ${varepsilon}$ -globin gene, 2.4-kb EcoRI fragment 3' ^A ${gamma}$ -globin gene, 1.0-kbEcoRV ${psi}$ ß region, 2.1-kb PstI fragment 5' ${delta}$ -globin gene,0.9-kb EcoRI-BamHI fragment 3' ß-globin gene, 1.4-kbXbaI DF10 (3'HS1), 1.9-kb BglII HPFH3, 0.5-kb HindIII H500,and 1.5-kb EcoRI-BglII HPFH6. DNA probes were labeled usingthe Decaprime II kit (Ambion, Austin, TX), following the manufacturer'sinstructions.

The presence of 5'HS4 and 5'HS5 was confirmed by Southern blothybridization using a ³²P-radiolabeled 3.2-kb BamHI fragment(Globin Gene Server human ß-globin locus coordinates215110 to 218333) as a probe (4). Digestion with SfiI (218055)and MluI (226095) produces a diagnostic 8.0-kb fragment for5'HS5 and 5'HS4. All lines contained 5'HS4 and -5 unless otherwiseindicated.

Transgene copy numbers were determined by Southern blot hybridizationusing LCR 5'HS3, ${gamma}$ -, and ß-globin gene fragment probescoradiolabeled with a mouse Thy 1.1 gene fragment as describedpreviously (15, 30). Probe-specific activity was corrected,and comparison of hybridization signal intensity between humanglobin transgenes and the endogenous diploid murine Thy1.1 genegave an estimate of transgene copy number. Radioactive signalswere quantitated using a phosphorimager (Packard Instruments,Meriden, CT).

RPA. Total RNA was isolated from yolk sac, fetal liver, and bloodof developmentally staged transgenic F₂, or later, embryos,fetuses, and adults by the method of Chomczynski and Sacchi(7) using the RNAgents total RNA isolation reagents (Promega,Madison, WI) as previously described (39). Human and murineglobin mRNAs were detected by RNase protections performed asdescribed previously (21, 39). Antisense RNA probes were preparedusing the MaxiScript II kit (Ambion, Austin, TX). Template DNAsused to prepare riboprobes to measure endogenous mouse ${alpha}$ - and ${zeta}$ -globins were pT7Mo ${alpha}$ and pT7Mo ${zeta}$ , respectively (28), and to measurehuman ${varepsilon}$ -, ${gamma}$ -, and ß-globins, the templates were pT7Hu ${varepsilon}$ (188),pT7^A ${gamma}$ ^m(170), and pT7ß^m, respectively (25, 43). Individualhuman ß-like globin gene expression levels were quantitatedas percentages of total human ß-like globin gene expressionor as percentages of murine ${alpha}$ - and ${zeta}$ -globin gene expression correctedfor transgene and endogenous murine gene copy number using datacollected on a Cyclone phosphorimager and OptiQuant analysissoftware (Packard Instruments, Meriden, CT). RPAs were doneseparately with each conceptus of each litter to minimize experimentalerror and determine variation in globin gene expression. Foreach construct, three transgenic lines were established, andwith rare exceptions, two or three conceptuses were analyzedat each developmental stage. Quantitative data include the meansand standard deviations from two or three experiments for eachline. Thus, averages at each developmental stage are indicativeof 4 to 9 experimental values for individual transgenic linesand 12 to 27 values for combined lines. Wild-type ß-YAClines 4 and 10 served as controls for RPA and RT-PCR RFLP (40).All experiments performed included a parallel set of wild-typeß-YAC samples (data not shown). In all instances theoutcome confirmed the data we have compiled in published orunpublished form over the past 12 years regarding expressionlevels in these lines. Wild-type ß-YAC control laneswere included in each figure for comparison purposes, for sizeor band location indicators only, or to demonstrate proper functionof riboprobes. For statistical analysis, the Student t testof comparison of means was performed, and differences were consideredsignificant at P values of <0.025.

Semiquantitative RT-PCR. cDNA was synthesized from 10-day embryonic yolk sac, 12-dayfetal liver, 14-day fetal liver, or adult mouse blood totalRNA using an oligo-dT primer (Promega Corp., Madison, WI) andSuperscriptase II reverse transcriptase (Invitrogen, Carlsbad,CA). One microgram of total RNA was mixed with 0.5 µgoligo-dT and sterile water in a final volume of 11 µl.The mixture was heated to 70°C for 10 min and then chilledon ice. Once cooled, 4 µl 5x first-strand buffer, 2 µl0.1 M dithiothreitol, 1 µl 10 mM deoxynucleoside triphosphatemix, and 1 µl RNasin (Promega Corp, Madison, WI) wereadded and the reaction mixture was heated at 42°C for 2min. One µl Superscript II RT was added, and the 20-µlreaction mixture was incubated at 42°C for 50 min. RT enzymewas heat inactivated by incubation for 15 min at 70°C.

PCR was performed essentially as described by Omori et al. (32)using Biolase Taq polymerase (Bioline USA, Randolph, MA) ina 25-µl reaction mix containing 1x NH₄ buffer [16 mM (NH₄)₂SO₄,67 mM Tris-HCl (pH 8.8), 0.01% Tween-20], 2 mM MgCl₂, 100 µMdeoxynucleoside triphosphates, 1 µCi [ ${alpha}$ -³²P]dCTP, 0.4 pmolforward primer, 0.4 pmol reverse primer, 1 U Taq polymerase,and globin gene-specific primers (Invitrogen, Carlsbad, CA).All primers were designed to cross an intron so that RNA-templatedreverse-transcribed DNA amplification products could be distinguishedfrom gene amplification products. For human ß-globinand mouse ${alpha}$ -globin, initial denaturation was at 95°C for5 min, followed by 18 cycles of 94°C for 30 s, 60°Cfor 30 s, and 72°C for 45 s; final extension was at 72°Cfor 10 min. Separate reactions were performed for human ß-globinand mouse ${alpha}$ -globin. Parallel titration reactions showed thatthis cycle number was within the exponential amplification range.The primer sequences for RT-PCR were as follows: ß^m5' ${varepsilon}$ ß-YAC or ß^m 5' ^G ${gamma}$ ß-YAC ß-globinforward, 5'-ACATTTGCTTCTGACACAACTG-3', and reverse, 5'-AGGAGCCTGAAGTTCTCAG-3'.The mouse ${alpha}$ -globin primers employed were as described previously(32). A similar scheme was used for the human ${varepsilon}$ -globin gene products.Amplification conditions were identical to those used for ß-globin.The primer sequences for RT-PCR were as follows: ${varepsilon}$ ^m 3' ${delta}$ ß-YACforward, 5'-CATATCTGCTTCCGACACAG-3', and reverse, 5'-GGGGTAAACAACGAGGAGTC-3'.Mouse ${alpha}$ -globin was included as a control in separate reactions.

A nonquantitative RT-PCR was employed for the ${gamma}$ -globins. Initialdenaturation was at 95°C for 5 min, followed by 20 to 40cycles of 1-min steps at 95°C, 60°C, and 72°C; finalextension was at 72°C for 10 min. The primer sequences forRT-PCR were as follows: ^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YAC ${gamma}$ -globin forward,5'-ACACTCGCTTCTGGAACGT-3', and reverse, 5'-TAGACAACCAGGAGCCTTCC-3'.

RT-PCR RFLP analysis. RT-PCR primers were designed to amplify regions of the wild-typeand marked globin gene products that were distinguished by RFLPanalysis. Following semiquantitative RT-PCR, 5 µl of theRT-PCR products were digested overnight with restriction enzymesand fractionated on an 8% native polyacrylamide gel, which wasdried and subjected to phosphorimager analysis (Typhoon, GEHealthcare, Waukesha, WI). In the ß^m-globin gene constructs,the normal NcoI site was replaced with a ClaI site by virtueof introduction of the mark. Thus, the ß^wt-globinproduct was digested with NcoI but not ClaI, and the conversewas true for the ß^m-globin product. For the ß^m5' ${varepsilon}$ ß-YAC and ß^m 5' ^G ${gamma}$ ß-YAC mice,the full-length PCR product was 370 bp. Digestion of the wild-typeproduct with NcoI produced 320-bp plus 50-bp bands, whereasthe ß^m-globin product was not digested. ClaI digestedthe ß^m-globin product but not the ß^wt-globinproduct to produce 324-bp plus 50-bp fragments. All experimentswere run twice using the samples indicated in the figures.

The ${varepsilon}$ ^m 3' ${delta}$ ß-YAC samples were similarly processed,except that XhoI was used to distinguish the ${varepsilon}$ ^wt- and ${varepsilon}$ ^m-globinRT-PCR products. The 164-bp ${varepsilon}$ ^wt-globin product was not digestedwith XhoI, whereas the 172-bp ${varepsilon}$ ^m-globin product was cut into155-bp and 17-bp fragments.

For the ^A ${gamma}$ ^m-globin construct, following RT-PCR, portions of thePCR product were subjected to overnight digestion with appropriaterestriction enzymes, fractionated on a 2 to 3% agarose gel,and visualized by ethidium bromide staining. DdeI digestionwas used to analyze the ^A ${gamma}$ ^m- and ^A ${gamma}$ ^wt-globin gene products. The^A ${gamma}$ ^wt-globin RT-PCR product from ^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YAC mice wascut with DdeI into 130-bp plus 19-bp fragments, whereas the^A ${gamma}$ ^m-globin RT-PCR product remained as the full-length 159-bpfragment.

RESULTS

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

The goal of our studies was to analyze the effect of gene orderon the temporal expression of the human ß-like globinsusing ß-YAC transgenic mice. Towards this purpose,four modified ß-YAC constructs were made (Fig. 1).Each of the constructs contained an additional marked ß-likeglobin gene inserted in a nonnative location within a 213-kbß-YAC. For the construct ß^m 5' ${varepsilon}$ ß-YAC,a ß^m-globin gene was inserted 1.6 kb 3' to 5'HS1 and4.4 kb 5' to the ${varepsilon}$ -globin gene CAP site. The ß^m 5'^G ${gamma}$ ß-YAC construct bore a ß^m-globin geneinserted 1.7 kb 5' to the ^G ${gamma}$ -globin CAP site. For the ^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YAC construct, an ^A ${gamma}$ ^m-globin gene was inserted atthe same location as the ß^m-globin gene in the ß^m5' ${varepsilon}$ ß-YAC construct. The ${varepsilon}$ ^m 3' ${delta}$ ß-YAC constructcontained an ${varepsilon}$ ^m-globin gene inserted 4.3 kb 3' to ${delta}$ -globin exon2 and 2.5 kb 5' to the ß-globin CAP site.

An adult ß-globin gene located proximally to the LCR is preferentially expressed throughout development. Three ß^m 5' ${varepsilon}$ ß-YAC transgenic lines wereestablished. Each line harbored at least one intact human ß-globinlocus transgene extending from 5'HS5 through the ß-globingene enhancer (see Fig. S1 in the supplemental material). Expressionstudies were done by RNase protection assay using embryonic,fetal, and adult erythroid cells of F₂ progeny of the transgeniclines.

As shown in Fig. 2, the ß^m-globin gene was expressedthroughout development, beginning as early as detectable (day8) and continuing through adulthood. ${varepsilon}$ -Globin mRNA was not detectedand ${gamma}$ -globin gene expression was reduced during embryonic erythropoiesis.At day 10 postconception, the ${gamma}$ -globin level was 15% of totalhuman globin expression [ ${gamma}$ /( ${gamma}$ +ß)] versus 90% in wild-typeß-YAC transgenic mice [ ${gamma}$ /( ${varepsilon}$ + ${gamma}$ )].

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FIG. 2. Developmental profile of ß-like globin gene expression in ß^m 5' ${varepsilon}$ ß-YAC transgenic mice. Total RNA was isolated from the blood of staged fetuses and subjected to RNase protection analysis. Representative data from line 1 are shown. The days after conception are shown at the top of the autoradiograph. The numbers indicate individuals of the same developmental stage. Antisense RNA probes for human ${varepsilon}$ -, ${gamma}$ -, and ß-globin mRNAs were utilized. Protected fragments are displayed on the right. The protected fragment sizes are as follows: human ß-globin exon 2 (ß ex 2), 205 bp; ${varepsilon}$ -globin exon 2 ( ${varepsilon}$ ), 188 bp; ${gamma}$ -globin exon 2 ( ${gamma}$ ), 170 bp; marked ß-globin exon 1 (ß^m ex 1), 145 bp; wild-type ß-globin exon 1 (ß^wt ex 1), 91 and 50 bp. The ß-globin antisense probe hybridizes with exons 1 and 2 of both the ß^wt- and ß^m-globin mRNAs. Thus, the exon 2 protected fragment is the sum of these two gene products, and the exon 1 protected fragments distinguish the two mRNAs. The marker (M) in the left lane is a radiolabeled MspI digest of plasmid pBR322; fragment sizes are shown in base pairs. FL, fetal liver; Bl, blood; wt ß-YAC, wild-type 213-kb human ß-globin locus YAC transgenic mouse line 4 (42). Lines 2 and 3 showed an identical phenotype.

Mean ${gamma}$ -globin expression in the day 10 yolk sac for all lines(nine embryos), calculated as a percentage of murine ${alpha}$ -like globingenes and corrected for endogenous and transgene copy numbers,was 30.7% ± 21.5% compared to 59.9 ± 2.4% (P <0.025) in wild-type ß-YAC lines. No ${gamma}$ -globin mRNA wasdetected in the liver during fetal definitive erythropoiesisby RNase protection assay or antibody staining for globin chains(data not shown), although ${gamma}$ -globin mRNA was detected in theperipheral circulation, which still contains high numbers ofembryonic erythroblasts, through day 14 (Fig. 2). Only ß^m-globinwas detected during adult definitive erythropoiesis; no wild-typeß-globin mRNA was observed.

Semiquantitative RT-PCR coupled with restriction enzyme digestionanalysis (RT-PCR RFLP) was performed using primers for the ß-globin5' untranslated region (UTR) and exon 1/exon 2 boundary. cDNAswere synthesized from adult blood RNA and amplified by PCR,and the PCR products were digested overnight with restrictionenzymes ClaI or NcoI. These data confirmed that only the ß^m-globingene was expressed in adult mice carrying the ß^m 5' ${varepsilon}$ ß-YAC construct (Fig. 3). This analysis also demonstratedthat the wild-type ß-globin gene was not expressedat any stage of development. ClaI treatment showed completedigestion of the 370-bp fragment, whereas NcoI did not digestthe PCR product at all, demonstrating that all of the ß-globinmRNA synthesis in these lines was ß^m-globin. Furthermore,ß^wt-globin protected fragments were not observed inFig. 2, nor were they observed in RNase protection assays usingonly a ß-globin exon 1 antisense riboprobe to exclusivelydetect and distinguish ß^m- and ß^wt-globinmRNAs (data not shown).

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FIG. 3. Semiquantitative RT-PCR RFLP analysis of ß-globin expression in ß^m 5' ${varepsilon}$ ß-YAC transgenic mouse lines. RT-PCRs were performed to amplify the 5' end of the ß-globin transcript in adult mouse blood total RNA samples from ß^m 5' ${varepsilon}$ ß-YAC lines 1, 2, and 3 (See Materials and Methods). Representative data from two adult individuals for each line are shown. The 4-bp insertion in the ß^m-globin gene created a diagnostic ClaI restriction enzyme site and destroyed an NcoI site. ClaI digestion of the ß^m-globin produces 324-bp and 50-bp fragments, whereas NcoI does not cut (ß^m control lane). The reverse occurs for wild-type ß-globin; NcoI produces 320-bp and 50-bp fragments, whereas ClaI does not cut (ß^wt control lane). Both enzymes digest proportionately to gene product levels as shown in the ß^mß^wt control lane, where the majority of expression in these µLCRß^mß^wt mice is ß^m-globin. Top panel, controls: ß^mß^wt, µLCRß^mß^wt transgenic mouse adult blood (39); ß^m, µLCRß^mA ${gamma}$ transgenic mouse adult blood (39); ß^wt, wild-type 213-kb ß-YAC transgenic mouse line 4 adult blood (40). Bottom panel: ßm 5' ${varepsilon}$ ß-YAC lines 1, 2, and 3. Digest fragment sizes are shown on the left, along with the location and size of the mouse ${alpha}$ -globin product used to normalize our data. Molecular weight marker (M) sizes are listed on the right side of the panels.

Midlocus localization of an adult ß-globin gene alters its expression pattern. Three ß^m 5' ^G ${gamma}$ ß-YAC transgenic lines wereestablished. All lines contained at least one ß-globinlocus copy that encompassed the LCR and the ß^m-globingene (see Fig. S2 in the supplemental material). However, line3 ( ${Delta}$ ß^wt) contained a deletion of the normally locatedß^wt-globin gene but contained sequences through the ${psi}$ ß-globin gene. Globin gene expression was measuredby RPA in embryonic, fetal, and adult erythroid cells of F₂animals.

Representative results by RNase protection assay are shown inFig. 4. ß^m-Globin expression was detected in the embryonicyolk sac, and expression continued through definitive erythropoiesisin both fetal liver and adult blood (Fig. 4B). Nearly all ofthe ß-globin expressed was ß^m-globin, althoughß^wt-globin expression was detectable in day 14 fetalliver and adult blood by RPA using only a ß-globinantisense riboprobe to reduce background (Fig. 4C). In the full-lengthß-YAC mice (lines 1 and 2), mean ${varepsilon}$ -globin expressionin the day 10 yolk sac was 2.5-fold higher than in wild-typeß-YAC lines (P < 0.01), whereas ${gamma}$ -globin expressionwas 45% lower than in control mice (P < 0.01) (Table 1; Fig.5A). During day 12 and 14 fetal definitive erythropoiesis, mean ${gamma}$ -globin expression was approximately 28% of the wild-type ß-YACexpression level (Fig. 5A; Table 1).

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FIG. 4. Globin gene expression during development in ß^m 5' ^G ${gamma}$ ß-YAC transgenic mice. RPAs of samples from line 1 are shown. (A) Human ß-like globin expression in blood. (B) Expression of human and murine globin genes in hematopoietic tissues. (C) ß^m- versus ß^wt-globin mRNA expression in blood. Labeling is as for Fig. 2. Developmental days are indicated above the images; ß-like globin gene fragments are indicated on the right or left side, as are markers. The protected fragment sizes are the same as for Fig. 2 with the addition of mouse ${alpha}$ -globin (Mo ${alpha}$ ), 128 bp, and mouse ${zeta}$ -globin (Mo ${zeta}$ ), 151-bp doublet. YS, yolk sac; +, wild-type 213-kb ß-YAC transgenic mouse line 4 (40) positive controls.

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TABLE 1. Human globin mRNA levels per copy of transgene and copy of endogenous murine ${alpha}$ - and ${zeta}$ -globin in ß^m 5' ^G ${gamma}$ ß-YAC transgenic mice and wild-type ß-YAC control mice

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FIG. 5. Human ${gamma}$ - and ß-globin mRNA levels in ß^m 5' ^G ${gamma}$ ß-YAC transgenic mice during embryonic and definitive erythropoiesis. ${gamma}$ - or ß-globin gene expression levels were quantitated from RNase protection analyses of RNAs derived from the indicated tissues at the developmental stages shown by phosphorimaging. Levels were calculated as percentages of murine ${alpha}$ - and ${zeta}$ -globin gene expression corrected for transgene and endogenous murine gene copy number. The average and standard deviation for all individuals within all lines are plotted on the x axis. The number of conceptuses tested for each genotype is indicated in Materials and Methods; the range was from 9 to 27. (A) ${gamma}$ -Globin mRNA expression. (B) ß-Globin mRNA expression. Black bars, full-length ß^m 5' ^G ${gamma}$ ß-YAC lines 1 and 2; hatched bars, ß^m 5' ^G ${gamma}$ ${Delta}$ ß^wt ß-YAC line 3; white bars, wild-type ß-YAC line 4 (40). Other abbreviations are as described in previous figure legends.

In the day 10 yolk sac of the full-length lines (1 and 2), 12%of the human globin mRNA was ß-globin (Fig. 5; Table1). At day 12 in the fetal liver, the total ß-globinmRNA (ß^wt+ß^m) was similar to that of thewild-type ß-YAC mice. Thereafter, ß-globinmRNA declined to 56% of the control level in day 14 fetal liverand to 25% in adult blood. To confirm the pattern and levelof ß^m- versus ß^wt-globin mRNA expression,semiquantitative RT-PCR RFLP was performed as described in Materialsand Methods. For these experiments, cDNAs were synthesized fromday 10 embryonic yolk sac, day 12 fetal liver, day 14 day fetalliver, and adult blood RNA. Wild-type ß-globin PCRproduct was digested by NcoI in wild-type ß-YAC transgenicmice that do not have a ß^m-globin gene but not byClaI (Fig. 6, top left panel, wild-type ß-YAC mice).The reverse was true for the ß^m-globin product inß^m 5' ^G ${gamma}$ ß-YAC mice lacking the ß^wt-globingene, which was digested by ClaI but not by NcoI [Fig. 6, bottomright panel, ß^m 5' ^G ${gamma}$ ß-YAC mouse line 3( ${Delta}$ ß^wt)]. In ß^m 5' ^G ${gamma}$ ß-YAC mouselines 1 and 2, which contain both the ß^m- and ß^wt-globingenes, only ß^m-globin expression was observed in theday 10 yolk sac, but both ß^wt- and ß^m-globinswere detected in day 12 fetal liver, day 14 fetal liver, andadult blood (Fig. 6, top right and bottom left panels, ß^m5' ^G ${gamma}$ ß-YAC mouse lines 1 and 2). ß^wt-globinconstituted 7.3% ± 0.7% of total human ß-globingene expression [ß^wt/(ß^m+ß^wt)]in day 12 fetal liver, 10.6% ± 1.2% in day 14 fetal liver,and 16.1% ± 2.2% in adult blood (means and standard deviationsof lines 1 and 2 combined, two conceptuses per line, duplicateexperiments).

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FIG. 6. Semiquantitative RT-PCR RFLP analysis of ß-globin gene expression in ß^m 5' ^G ${gamma}$ ß-YAC transgenic mice. RT-PCRs were performed for wild-type ß-YAC and three ß^m 5' ^G ${gamma}$ ß-YAC mouse lines. Total mRNAs from 10 day embryonic yolk sac (lanes 1), 12-day fetal liver (lanes 2), 14-day fetal liver (lanes 3), and adult blood (lanes 4) were analyzed using primers for the 5' UTR and exon 1/exon 2 boundary of the ß-globin gene (See Materials and Methods). The full-length product is 370 bp. Digestion of the wild-type ß-globin product with NcoI produces 320-bp and 50-bp fragments, whereas the ß^m-globin product is not digested. ClaI digests the ß^m-globin product, but not the ß^wt-globin product, to produce 324-bp and 50-bp fragments. Top panel: left, wild-type 213-kb ß-YAC transgenic mouse line 4 (Wild-type ß-YAC [40]); right, ß^m 5' ^G ${gamma}$ ß-YAC mouse line 1 (Line 1). Bottom panel: left, ß^m 5' ^G ${gamma}$ ß-YAC line 2 (Line 2); right, ß^m 5' ^G ${gamma}$ ${Delta}$ ß^wt-globin ß-YAC mouse line 3, which bears a deletion of the normally located wild-type ß-globin gene [Line 3 ( ${Delta}$ ß^wt)]. NcoI completely digested the ß^wt-globin product, whereas ClaI did not, in the wild-type ß-YAC mouse line. ClaI digested the ß^m-globin PCR product, whereas NcoI did not, in ß^m 5' ^G ${gamma}$ ${Delta}$ ß^wt-globin ß-YAC line 3.

For line 3 ( ${Delta}$ ß^wt) mice, which carried a ß-globinlocus lacking the wild-type ß-globin gene, ${varepsilon}$ -globinexpression was 4.7-fold higher than that for controls, but ${gamma}$ -globinexpression was essentially the same as for wild-type ß-YACmice (Table 1; Fig. 5A). ${gamma}$ -Globin gene expression was not detectedduring fetal or adult definitive erythropoiesis. ß^m-Globingene expression in the yolk sac was twofold higher than thatfor lines 1 and 2 (P < 0.01), suggesting that the absenceof the ß^wt-globin gene resulted in a higher levelof expression from the ß^m-globin gene (Fig. 5B; Table1). However, ß-globin expression was consistentlylower than in lines 1 and 2 during all stages of definitiveerythropoiesis (Table 1; Fig. 5B).

Together, these data suggest that the LCR-proximal ß^m-globingene is expressed exclusively early in development (Fig. 4 and6), and low-level expression of the more distal ß^wt-globingene occurs beginning on day 12. Although there was a declinein ß^m-globin gene expression during adult erythropoiesis,the ß^m-globin gene was never completely silenced inspite of its location in the ${gamma}$ -globin gene domain. The elevated ${varepsilon}$ -globin gene expression during embryonic erythropoiesis suggeststhat location of the ß^m-globin gene 5' to the ^G ${gamma}$ -globingene may give the ${varepsilon}$ -globin gene an expression advantage by downregulating ${gamma}$ -globin expression, especially in the absence of the ß^wt-globingene. In day 12 fetal erythropoiesis, no ${gamma}$ -globin was observedin line 3 ( ${Delta}$ ß^wt) mice, whereas in lines 1 and 2, ${gamma}$ -globinexpression gradually declined, suggesting that the distal ß^wt-globingene may exert a repressive effect on ${gamma}$ -globin expression.

A fetal ${gamma}$ -globin gene located proximally to the LCR is autonomously silenced during adult definitive erythropoiesis. Five ^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YAC transgenic mouse lines were established;each contained at least one intact copy of the ß-YACthrough the ${gamma}$ -globin genes (see Fig. S3 in the supplemental material).Three lines (1 to 3) carried at least one ß-YAC extendingfrom 5'HS3 through the ß-globin gene, and two lineshad deletions of the ${delta}$ - and ß-globin genes and downstreamsequences ( ${Delta}$ ß line 1 and ${Delta}$ ß line 2). Representativeresults of RNase protection assays are shown for line 3 (Fig.7). ${varepsilon}$ - and ${gamma}$ ^wt-globins were not expressed at any time during ontogeny.^A ${gamma}$ ^m-Globin expression was initiated during primitive erythropoiesisand continued through fetal definitive erythropoiesis, as indicatedby the presence of a 138-bp ^A ${gamma}$ ^m-globin exon 1 band. ^A ${gamma}$ ^m-Globinexpression was not detected during adult definitive erythropoiesisin blood. ß-Globin was expressed during fetal definitiveerythropoiesis and continued throughout adulthood. Analysisof lines lacking the ß^wt-globin gene also demonstratedthat ${varepsilon}$ -, ^G ${gamma}$ -, and ^A ${gamma}$ ^wt-globins were not expressed at any stage(see Fig. S3 in the supplemental material, ${Delta}$ ß lines1 and 2; data not shown). Interestingly, ^A ${gamma}$ ^m-globin expressionwas down-regulated even in the absence of the ß-globingene, suggesting that the 5.4-kb SspI fragment carrying the^A ${gamma}$ ^m-globin gene contains a silencer region. In addition, thesedata demonstrate that ${gamma}$ -globin expression may be autonomouslysilenced, independently from competition with the ß-globingene for interaction with the LCR.

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FIG. 7. ^A ${gamma}$ ^m-Globin is silenced in adult ^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YAC transgenic mice. RPAs of developmentally staged fetuses from ^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YAC line 3. (A) Human ß-like globin expression in blood. (B) Human and murine globin gene expression in hematopoietic tissues. Labeling is as for Fig. 2 and 4 with the addition of human ^A ${gamma}$ ^m-globin exon 1 (^A ${gamma}$ ^m ex 1), 138 bp, and ^G ${gamma}$ /^A ${gamma}$ ^wt-globin exon 1 (^G ${gamma}$ /^A ${gamma}$ ^wt ex 1), 118 bp. The ^A ${gamma}$ -globin antisense probe hybridizes with exon 2 of the ^A ${gamma}$ ^wt-, ^A ${gamma}$ ^m-, these and ^G ${gamma}$ -globin mRNAs; it also hybridizes with exon 1 of mRNAs. Thus, the exon 2 protected fragment is the sum of these three gene products, and the exon 1 protected fragments distinguish ^A ${gamma}$ ^m-globin mRNA from ^G ${gamma}$ - and ^A ${gamma}$ ^wt-globin mRNAs.

Qualitative RT-PCR RFLP analysis was used to confirm whether ${gamma}$ -globin expression was exclusively ^A ${gamma}$ ^m-globin or whether it representeda mixture of ^A ${gamma}$ ^wt- and ^A ${gamma}$ ^m-globins. RNA derived from day 14 fetalliver was subjected to RT-PCR using primers encompassing the ${gamma}$ -globin gene 5' UTR and exon 1 sequences. The mark in the ^A ${gamma}$ ^m-globingene is a six-basepair deletion in the 5' UTR of the ^A ${gamma}$ -globingene (41). The deletion removes a DdeI restriction enzyme sitewithin the 5' UTR. RT-PCR followed by digestion with DdeI confirmedthat all of the ${gamma}$ -globin expressed in the ^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YACmice originated with the ^A ${gamma}$ ^m-globin gene (data not shown).

${gamma}$ - and ß-globin gene expression was quantitated andcompared to expression in wild-type ß-YAC mice (Table2). In all lines, mean ${gamma}$ -globin expression was approximatelythe same as that measured in wild-type ß-YAC miceduring primitive erythropoiesis, but expression varied widelybetween the mutant lines. Similarly, during fetal definitiveerythropoiesis, ${gamma}$ -globin expression was variable between thedifferent lines. The difference between the mutant and wild-typeß-YAC lines in day 12 fetal liver erythropoiesis (40%versus 24%, respectively) is not statistically significant. ${gamma}$ -Globin expression was essentially the same in mutant and wild-typemice by day 14, and it was absent in adult definitive erythropoiesis.ß-Globin was not detected during primitive erythropoiesisin either ^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YAC mice or wild-type ß-YACmice. In day 12 and day 14 fetal liver, ß-globin inthe mutant line was 14% and 11% of the wild-type ß-YAClevel, respectively, reflecting delayed activation of ß-globingene transcription. During adult definitive erythropoiesis,mean ß-globin expression was 61% of that measuredin wild-type ß-YAC mice. Analysis of the globin geneexpression switching profile in blood confirmed that the switchfrom ${gamma}$ - to ß-globin expression was delayed comparedto results for wild-type ß-YAC mice and occurred onapproximately day 16 instead of on day 12 (data not shown).

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TABLE 2. Human globin mRNA levels per copy of transgene and copy of endogenous murine ${alpha}$ - and ${zeta}$ -globin in ^A ${gamma}$ ^m 5' ${varepsilon}$ ß-YAC transgenic mice and wild-type ß-YAC control mice

These data demonstrate that the LCR-proximal ^A ${gamma}$ ^m-globin geneis preferentially expressed during development and that it repressesdownstream ${varepsilon}$ -, ^G ${gamma}$ -, and ^A ${gamma}$ ^wt-globin transcription, perhaps by moreeffectively competing for interaction with the LCR during primitiveand fetal definitive erythropoiesis. The ^A ${gamma}$ ^m-globin gene fragmentcontains an autonomous silencer element that functions in repressionof ^A ${gamma}$ ^m-globin gene expression even in the absence of competitionwith the ß-globin gene for LCR interaction duringadult definitive erythropoiesis.

An embryonic globin gene inserted between two adult globin genes is not expressed. Three ${varepsilon}$ ^m 3' ${delta}$ ß-YAC lines were obtained (see Fig. S4in the supplemental material). Analysis of ${varepsilon}$ -globin gene expressionrevealed that only wild-type ${varepsilon}$ -globin was expressed during primitiveerythropoiesis; no signal was observed from the ${varepsilon}$ ^m-globin geneat any stage of development (Fig. 8A). These data were confirmedby semiquantitative RT-PCR RFLP analysis as described in Materialsand Methods (Fig. 9). ${varepsilon}$ ^wt-Globin synthesis detected in day 12and 14 fetal liver is due to the presence of primitive erythrocytesfrom earlier yolk sac erythropoiesis in the fetal circulation(31). Although transcription was not observed, the integrityof the inserted ${varepsilon}$ ^m-globin gene was confirmed by Southern blothybridization and PCR analyses (see Fig. S4 in the supplementalmaterial; also data not shown). Expression of the gene was confirmedby RPA of erythroid cells containing an ${varepsilon}$ ^m-globin plasmid (datanot shown). The insertion of an ${varepsilon}$ ^m-globin gene between the ${delta}$ -and ß-globin genes had no effect on either the temporalor spatial pattern of globin gene expression within the locus(Fig. 8B). More recently, a derivative of the ${varepsilon}$ ^m 3' ${delta}$ ß-YACconstruct was synthesized that lacks the normally located ${varepsilon}$ ^wt-globingene. Transgenic lines produced from this construct also didnot display ${varepsilon}$ ^m-globin gene expression at any stage of developmentas measured by semiquantitative RT-PCR (data not shown).

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FIG. 8. ${varepsilon}$ ^m-Globin is not expressed in ${varepsilon}$ ^m 3' ${delta}$ ß-YAC transgenic mice. RPAs of developmentally staged fetuses from ${varepsilon}$ ^m 3' ${delta}$ ß-YAC lines. Labeling is as for Fig. 2, 4, and 7. (A) Wild-type ${varepsilon}$ -globin mRNA is detected as a 127-bp exon 1 protected fragment, whereas ${varepsilon}$ ^m-globin mRNA is detected as a 152-bp exon 1 protected fragment. (B) The temporal pattern of globin transgene expression.

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FIG. 9. Semiquantitative RT-PCR RFLP analysis of ${varepsilon}$ -globin gene expression in ${varepsilon}$ ^m 3' ${delta}$ ß-YAC transgenic mice. RT-PCRs were performed for wild-type ß-YAC and three ${varepsilon}$ ^m 3' ${delta}$ ß-YAC mouse lines. Total mRNAs from 10 day embryonic yolk sac (lanes 1), 12-day fetal liver (lanes 2), 14-day fetal liver (lanes 3), and adult blood (lanes 4) were analyzed using primers for the 5' UTR and exon 1/exon 2 boundary of the ${varepsilon}$ -globin gene (see Materials and Methods). The full-length ${varepsilon}$ ^wt-globin product is 164 bp; the ${varepsilon}$ ^m-globin product is 172 bp. The wild-type ${varepsilon}$ -globin product is not digested with XhoI, whereas the ${varepsilon}$ ^m-globin product is digested and generates 155-bp and 17-bp fragments. Left panel, wild-type 213-kb ß-YAC transgenic mouse line 4 (wild-type ß-YAC) (40); right panel, ${varepsilon}$ ^m 3' ${delta}$ ß-YAC mouse line 2 (Line 2). Results were the same for ${varepsilon}$ ^m 3' ${delta}$ ß-YAC transgenic mouse lines 1 and 3.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Many mammalian loci show a correlation between spatial arrangementof genes in the DNA sequence (gene order) and the temporal orderof expression during development. Such an arrangement may facilitatecis regulatory mechanisms, allowing fine-tuning of gene activationand repression circuitry and maintenance of the delicate balancebetween these developmentally controlled processes. Examplesinclude the human ß-globin locus, the homeobox (hox)gene loci of Drosophila and mammals, and mammalian ${alpha}$ -fetoproteinand albumin genes (5, 20, 29).

The question of the role of gene order in developmental regulationhas been previously addressed with various approaches. We demonstratedthat when two globin genes from the same developmental stagewere arranged tandemly and linked to the LCR, the gene moreproximal to the LCR was expressed preferentially throughoutdevelopment, indicating that proximity to the LCR was a determinantof globin gene expression, perhaps due to the increased frequencyof interaction of the proximal gene with the LCR (39). One sucharrangement occurs naturally within the human ß-globinlocus. The ^G ${gamma}$ - and ^A ${gamma}$ -globin coding sequences are nearly identical,but the ^G ${gamma}$ -globin gene is expressed at higher level than the^A ${gamma}$ -globin gene early in fetal erythropoiesis; the ratio invertsas development proceeds (22). When the ${gamma}$ - and ß-globingenes were linked tandemly to the LCR, ${gamma}$ -globin was expressedat a higher level than ß-globin during fetal definitiveerythropoiesis, and the ratio was reversed during adult definitiveerythropoiesis (39). This result occurred regardless of theorder of the ${gamma}$ - and ß-globin genes with respect tothe LCR, indicating that the trans-acting environment was theprimary determinant of globin gene expression, overcoming othermotifs, including proximity to the LCR. Although these experimentssuggest that proximity to the LCR plays a role in correct geneexpression, the distances between the LCR and linked genes wereartificially shortened, leaving open the question as to whethergene order was important.

Another experimental system utilized two cosmid constructs encompassingportions of the human ß-globin locus that were ligatedtogether just prior to producing transgenic mice (10). One setof mouse lines contained a locus in which a ß^m-globingene was placed upstream of the ${delta}$ -globin gene; in another setof lines the ${varepsilon}$ -globin gene was replaced with the ß^m-globingene. In the lines where the ß^m-globin gene replacedthe ${varepsilon}$ -globin gene, ß^m-globin was expressed throughoutdevelopment; ß^wt-globin comprised only a small percentageof expression in adult tissues. In addition, ${gamma}$ -globin gene expressionwas silenced. In the lines where the ß^m-globin genewas located near the ${delta}$ -globin gene, ß^m-globin accountedfor 75% of total ß-globin synthesis and ß^wt-globinfor 25%. In a third set of experiments, the genes of the humanß-globin locus were inverted with respect to the LCRin ß-YAC transgenic mice (44). In this instance theß-globin gene was proximal, and it was constitutivelyexpressed. The ${varepsilon}$ -globin gene was most distal; it was not expressedat all, and ${gamma}$ -globin expression was restricted to primitive erythropoiesis.These data suggested that any gene located near the LCR willbe strongly expressed throughout ontogeny.

In this study, we used complete, intact locus constructs containingall potential regulatory elements and all the wild-type genesof the locus in their normal spatial configuration. The 213-kbhuman ß-globin locus YAC contains 187 kb of the locus,and mice generated with this YAC have been shown to displaycorrect tissue-specific and temporal expression patterns (36,38). A marked ß-globin gene was placed upstream ofeither the ${varepsilon}$ -globin gene or the ^G ${gamma}$ -globin gene. A marked ^A ${gamma}$ -globingene was placed upstream of the ${varepsilon}$ -globin gene. A marked ${varepsilon}$ -globingene was placed between the ${delta}$ - and ß-globin genes.Several conclusions can be drawn from the expression patternswe observed.

Placement of the marked ß-globin gene upstream tothe ${varepsilon}$ -globin gene resulted in predominantly ß^m-globinexpression during yolk sac erythropoiesis. ${gamma}$ -Globin expressionin embryonic cells was decreased by 50% compared to that forthe wild-type ß-YAC ${gamma}$ -globin gene control, and therewas no detectable ${varepsilon}$ -globin gene expression. Only ß^m-globingene expression could be detected during definitive erythropoiesisin fetal liver and adult erythroid cells. Similar results wereobserved in a previous study in which a ß^m-globingene replaced the ${varepsilon}$ -globin gene (10). The most likely explanationfor these results is preferential interaction of the ß^m-globingene with the LCR due to its proximity to this regulatory element.The absence of downstream ß^wt-globin gene expressioncan be attributed to competition. It is of interest that althoughthere was ${gamma}$ -globin gene expression in the embryonic cells, ${varepsilon}$ -globingene expression was absent. This finding suggests that structural(or distance) constraints exist that determine (or influence)the interaction between the LCR and the downstream globin genes.Perhaps the distance between the ß^m- and ${varepsilon}$ -globin genesis too short and prohibits the interaction of the LCR with thenearby downstream ${varepsilon}$ -globin gene. Similarly, Dillon et al. (10)showed that ${gamma}$ -globin was expressed during embryonic erythropoiesiswhen the ß^m-globin gene replaced the ${varepsilon}$ -globin gene,but expression was completely suppressed in the fetal liver.Thus, the distance between the ${varepsilon}$ -globin gene (or the ß^m-globingene in this case) and the ${gamma}$ -globin gene is sufficient to allowinteraction of either of these genes with the LCR.

Another conclusion from this study is that it is not so muchthe placement of a gene within the locus that determines globingene switching but rather the presence of silencing sequencesand their interactions with repressor complexes. Because theß-globin gene lacks developmentally controlled silencingelements in its promoter, switching is abolished when that geneis located at the beginning of the locus. Conversely, when an^A ${gamma}$ ^m-globin gene was placed at the same location upstream of the ${varepsilon}$ -globin gene, the ^A ${gamma}$ ^m-globin gene was turned off during definitiveerythropoiesis and the switch from ${gamma}$ - to ß-globin geneexpression occurred. These results provide support for the conceptthat to a major degree, globin gene switching is controllednegatively by the presence of silencing elements in the embryonicand fetal globin gene promoters and the interaction of theseelements with the prevailing trans-acting environment. For the ${gamma}$ -globin genes, the silencing mechanism is leaky and can be overcomeby several physiological manipulations, acquired pathologicalconditions, and mutations in vivo in humans. Also of note hereis the fact that the level of ß^m-globin gene expressionin the adult stage of development decreased to about 50% ofthat in the embryonic stage. As will be discussed later, thisfinding may reflect a change (in chromatin modification?) ofthe embryonic gene chromatin domain in which the ß^m-globingene is located.

The placement of the ß^m-globin gene upstream of the^G ${gamma}$ -globin gene resulted in phenotypes that could have been predictedon the basis of the hypothesis that gene order and proximityto the LCR determine globin gene expression. Thus, in the embryoniccells there was ${varepsilon}$ -, ß^m-, and ${gamma}$ -globin gene expression,but there was no expression of the distal wild-type ß-globingene. ${varepsilon}$ -Globin expression switched off at the onset of fetalerythropoiesis; ${gamma}$ -globin gene expression subsequently switchedoff later. The distal ß^wt-globin gene was expressedat 1/10 the level of the upstream ß^m-globin gene duringfetal or adult definitive erythropoiesis. All of these observationswere expected based on the hypothesis. Significantly, however,instead of the expected increase of ß-globin geneexpression as development proceeded, a consistent decrease ofß^m-globin gene expression was observed, so that totalß-globin gene expression (ß^wt+ß^m)in the adult cells was about 25% of that in the embryonic cells.As mentioned earlier, a decrease of ß^m-globin expressionto 50% of that in embryonic cells was noted in adult erythropoiesiswhen the ß^m-globin gene was located upstream of the ${varepsilon}$ -globin gene. How can these unexpected declines in ß^m-and ß^wt-globin gene expression be explained? Changesin the transcriptional environment cannot be the reason, becausethe environment of the adult erythroid cells is expected tobe more conducive to the interaction between the LCR and theß-globin gene promoter. Perhaps, as suggested, thewhole architecture of the ß-globin locus chromatinchanges during development, so that an initial embryonic chromatindomain is succeeded by a fetal and finally an adult domain (17).Although this change in the chromatin domain still remains hypothetical,it could provide an explanation for our observations. For example,chromatin modification in the embryonic domain might affectthe efficiency of looping of the LCR and decrease its interactionwith the ß^m-globin gene placed in that domain. Chromatinmodification studies may provide further insight into this question.

The control of ${gamma}$ -globin gene expression during development hasbeen the subject of considerable discussion. Initial studiesby two laboratories suggested that competition between the ${gamma}$ -and ß-globin genes for interaction with the LCR, coupledwith the preferential interaction of the ß-globingene with the LCR during the adult stage of development, areresponsible for the silencing of the ${gamma}$ -globin gene in adult erythropoiesis(3, 6, 12). When the ${gamma}$ -globin gene was linked to a µLCRcassette, it was not silenced in the adult stage (13); it was,however, silenced in a cosmid containing the ^G ${gamma}$ - to ß-globingene region with these genes in their normal chromosomal location(11). On the other hand, studies with transgenic mice carryinga mini-LCR linked to a ${gamma}$ -globin gene suggested that silencingcould be autonomous, since several (but not all) of these transgenicsdid not express ${gamma}$ -globin in adult cells (9). The results of ourstudy in which the ^A ${gamma}$ ^m-globin gene was placed upstream of the ${varepsilon}$ -globin gene provide support for the possibility of autonomoussilencing, since the ${gamma}$ -globin gene, even that close to the LCR,was turned off in adult erythropoiesis. This experiment alsoprovided information on the relative roles of gene order andtranscriptional environment in determining globin gene expression,because only the upstream ^A ${gamma}$ ^m-globin gene was expressed in thesetransgenic mice; the distal ${gamma}$ -globin genes remained silent. Sincethe downstream ${gamma}$ -globin genes remained totally silent duringthe embryonic/fetal stage of development, it is unlikely thata fetal environment alone is sufficient for ${gamma}$ -globin gene expression.The results are best explained by assuming that proximity tothe LCR is the major determinant of the order of ${gamma}$ -globin geneexpression during development.

As mentioned earlier, some evidence suggests that the ß-globinlocus may be divided into developmental stage-specific chromatinsubdomains that have a role in determining gene expression (14,17, 23). Our data show that an open adult chromatin subdomaindoes not activate ${varepsilon}$ ^m-globin gene expression when this gene isplaced in the adult chromatin subdomain, between the ${delta}$ - and ß-globingenes. More-recent data from our laboratory support this notion,because an ${varepsilon}$ ^m-globin gene located between the ${delta}$ - and ß-globingenes was not expressed even in the absence of the wild-type ${varepsilon}$ -globin gene (unpublished data).

Three major conclusions may be drawn from our data. First, anygene located near the LCR will be strongly expressed throughoutontogeny, unless some gene-specific silencing mechanism exists.Second, the ^A ${gamma}$ -globin gene is autonomously silenced. Third, bothgene order and gene-proximal cis regulatory elements are importantfor correct developmental expression of the globin genes. Geneorder, per se, may not be a direct determinant of gene expression,but ultimately an inherent property of spatial gene order isthe maintenance of the necessary distance between the LCR andthe globin genes to avoid aberrant gene expression. Thus, geneorder constrains distance and LCR proximity. To some extent,alteration of normal LCR proximity supersedes the dominanceof the trans-acting environment, particularly when the genedoes not have a mechanism of autonomous silencing.