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Mol Cell Biol, June 1998, p. 3340-3349, Vol. 18, No. 6
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Functional Replacement of the Mouse E2A Gene
with a Human HEB cDNA
Yuan
Zhuang,*
Robert
J.
Barndt,
Lihua
Pan,
Robert
Kelley, and
Meifang
Dai
Department of Immunology, Duke University
Medical Center, Durham, North Carolina 27710
Received 11 December 1997/Returned for modification 29 January
1998/Accepted 24 February 1998
 |
ABSTRACT |
The mammalian E2A, HEB, and E2-2 genes encode a unique class of
basic helix-loop-helix (bHLH) transcription factors that are evolutionarily conserved and essential for embryonic and postnatal development. While the structural and functional similarities among the
gene products are well demonstrated, it is not clear why deletion of
E2A, but not HEB or E2-2, leads to a complete arrest in B-lymphocyte
development. To understand the molecular basis of the
functional specificity between E2A and HEB/E2-2 in mammalian
development, we generated and tested a panel of E2A knockin mutations
including subtle mutations in the E12 and E47 exons and substitution of
both E12 and E47 exons with a human HEB cDNA. We find that the
alternatively spliced E12 and E47 bHLH proteins of the E2A gene play
similar and additive roles in supporting B lymphopoiesis.
Further, we find that HEB driven by the endogenous E2A promoter can
functionally replace E2A in supporting B-cell commitment and
differentiation toward completion. Finally, the postnatal lethality
associated with E2A disruption is fully rescued by the addition of HEB.
This study suggests that the functional divergence among E12, E47,
and HEB in different cell types is partially defined by the context of
gene expression.
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INTRODUCTION |
B lymphocytes in mammals are derived
from hematopoietic stem cells (HSC) present in the liver during fetal
development and bone marrow in adult life. The same HSC also generate T
lymphocytes, erythrocytes, macrophages, and other cell types in
blood and the lymphoid organs. Once committed to the B-cell
lineage, the HSC follow a stepwise differentiation pathway to become B
lymphocytes, which subsequently participate in diverse humoral immune
responses. It is not entirely known how and when B-lineage cells are
first specified from HSC and how B lymphopoiesis is maintained
throughout life.
B-lineage development can be divided roughly into three discrete
stages: progenitor (pro-B), precursor (pre-B), and mature B-cell
stages. Rearrangements of immunoglobulin (Ig) genes initiate at the
pro-B stage and proceed to completion at the pre-B stage. Pre-B cells
expressing functional but nonself-reactive B-cell receptors are
selected for survival and expansion to become mature B cells
(18). In addition, B cells at various stages of
development express lineage-specific markers, such as B220, CD43, and
CD19 surface antigens (9, 19). These lineage markers,
combined with the status of Ig rearrangements and expression, establish road signs of normal and abnormal progression of B lymphopoiesis (9).
Regulation at the transcriptional level is crucial in each step of
B-cell development. Indeed, recent studies have shown that E2A, EBF,
Pax5, Ikaros, and several other transcription factors play key roles in
the pro- and pre-B stages of development (2, 14, 29, 31,
35). Disruption of genes encoding each one of these
transcription factors arrests B-cell development at
either the pro- or pre-B-cell stage. Since deletion of
E2A blocks B-cell development prior to the initiation of Ig gene
rearrangement, E2A seems to play an extremely early role. Furthermore,
E2A is the only gene that has been shown to be capable of triggering Ig
gene D-J rearrangement in non-B cells, making E2A a key regulatory component for B-lineage commitment (6, 23).
E2A is a founding member of the basic-helix-loop-helix
(bHLH) gene family, which is defined by the conserved bHLH structure, a
protein domain involved in DNA binding and protein dimerization. E2A encodes two bHLH proteins, E12 and E47, which contain different bHLH domains resulting from alternative splicing (15,
27). E12 and E47, together with the gene products of the
E2-2 and HEB genes (10, 11), comprise a unique subfamily of
bHLH proteins, commonly known as the E-protein family. These E proteins
are ubiquitously, although not evenly, expressed and are capable of
forming heterodimers with a variety of bHLH proteins, including
tissue-specific bHLH proteins such as MyoD (13, 16)
and broadly expressed inhibitory proteins such as Id1 (4). A
large body of evidence indicates that E2A proteins participate in
tissue-specific regulation through heterodimer formation with the
tissue-specific bHLH proteins (13, 16). This activity of E2A
can be inhibited by Id proteins that dimerize with E2A and form a
non-DNA binding heterodimer (4, 32). Thus, E2A plays a
central role in tissue-specific gene regulation by mediating positive
and negative signals. However, gene knockout studies have shown
that this generic function of E2A may not be provided by E2A
alone, since most tissue types and organs can develop in the absence of
the E2A gene (2, 34, 35).
The function of E2A in B-cell development is thought to be mediated by
E2A protein homodimers. Studies have demonstrated that E47 is capable
of forming homodimers in the physiological conditions of B cells
but not other cell types (5, 25). E47 homodimerization is
regulated posttranslationally through at least two possible means: a
disulfide bond can covalently link two monomers and prevent dimer
dissociation (5), and hypophosphorylation at the
region upstream of the basic domain may enhance homodimer formation
(25). Therefore, it has been generally believed that
the initiation and maintenance of E47 homodimers in B cells underlies
the specificity of E2A function in B-cell development. E12, on the
other hand, does not form homodimers because of the inhibitory effect
of an acidic region adjacent to the bHLH domain (27).
Nonetheless, a recent study has suggested that E12 may collaborate with
E47 in supporting B-lineage commitment (3). The molecular
basis of this cooperation between E12 and E47 is not known.
The function of E2-2 and HEB in B-cell development has also been
investigated through targeted mutation in mice (36). Mice lacking either E2-2 or HEB, in contrast to the E2A mutation,
are still able to generate substantial amounts of B-lineage
cells, suggesting that neither E2-2 nor HEB is essential to B-cell
commitment and maturation. However, the number of pro-B cells produced
in E2-2 or HEB mutant mice is slightly reduced and can be reduced further in the compound-heterozygous background of E2A and E2-2 or
E2A and HEB (36). Based on these observations, we have
proposed that E2-2 and HEB can modulate, but may not replace, E2A
activity, and the interaction between E2A and E2-2 or HEB is due to
titration of the Id proteins, the common dimerization partners of all E proteins (28, 36).
To further explore the functional specificity of individual E proteins
in B-cell development, we generated and analyzed a panel of E2A
mutations. First, we used gene targeting to convert the endogenous E47
into a dominant negative form by introducing a point mutation into
the basic region of the bHLH domain of E47. This mutation, together
with a previously generated E12 knockout allele, demonstrated that
either E12 or E47 is sufficient to support a limited, but definitive,
B-lineage commitment. However, a sustained and optimal B-cell
production requires both E12 and E47. Second, we used a knockin
approach to replace the mouse E2A gene with a human HEB cDNA.
When the HEB cDNA was tested on the E2A-null background, we found
that two copies, but not one, of human HEB can support B-cell
development. This study demonstrates that E47, E12, and HEB have
similar structural features required for B-cell development. Further,
the results suggest that B-cell commitment and maturation are regulated
by a threshold level of E proteins.
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MATERIALS AND METHODS |
Construction of E47bm and E2Aheb
alleles.
The E47bm (basic-region mutation) targeting
construct was built on a 9-kb KpnI-BamHI fragment
of the E2A genomic DNA isolated from the 129/sv strain. A 2-kb subclone
covering the E47 exon was used in site-directed mutagenesis (Amersham
Sculptor kit) for introduction of the E47 basic-region mutation. The
mutation was verified by sequencing before subcloning into the
targeting construct. A phosphoglycerate kinase (PGK)-neomycin
phosphoryltransferase (Neo) cassette was inserted into the unique
XbaI site located downstream of the E2A gene. A
(PGK)-thymidine kinase (TK) cassette was placed outside the
targeting module and used as a negative selection marker to
eliminate the nonhomologous recombination events.
A separate and more generic targeting vector was made for introducing
any cDNA sequence into the E2A locus. This construct contains, from 5'
to 3', a 6-kb E2A homologous sequence, the Neo coding sequence fused in
frame with E2A, a unique cloning site for introduction of foreign cDNA,
and a short 3' homologous sequence to facilitate PCR detection of
recombination events. A full-length human HEB cDNA (11) was
inserted between the Neo marker and the 3' homologous sequence.
Translation of the HEB cDNA was provided by the encephalomyocarditis
virus internal ribosomal entry site (IRES) added in front of the HEB
cDNA (12). Transcription of the HEB cDNA was provided by the
endogenous E2A promoter when the construct was integrated into the E2A
locus.
Gene targeting was performed in an embryonic stem (ES) cell line (a
gift from A. Imamoto and P. Soriano) derived from a 129/sv
mouse.
Clones carrying targeting events were identified by PCR
and
subsequently confirmed by Southern analysis. Chimeric mice
were derived
by injecting ES cells into blastocysts harvested
from C57BL/6 mice.
Germ line transmission was tested by crossing
chimeric males with
C57BL/6 females, and the resulting heterozygous
mice were maintained
thereafter on the mixed background of 129/sv
and C57BL/6. All mice were
maintained in a specific-pathogen-free
environment throughout the
study.
PCR genotyping.
DNA used in genotyping was prepared from
toes cut at approximately 10 days of age. Toe tissue was digested at
50°C for more than 3 h in 0.1 ml of lysis buffer containing 100 mM NaCl, 10 mM Tris (pH 8.0), 25 mM EDTA, 0.5% sodium dodecyl sulfate,
and freshly added proteinase K (0.1 mg/ml). DNA was purified by
extraction with phenol once and chloroform once and addition of 2 volumes of 95% ethanol. After a wash with 70% ethanol, the DNA pellet was resuspended in 0.5 ml of Tris-EDTA buffer. PCR was performed by
adding 1 µl of DNA into 15 µl of the reaction cocktail, which consisted of 1× PCR buffer, 10% dimethyl sulfoxide, 1 mM
deoxynucleoside triphosphate, 0.1 µM each primer, and Taq
polymerase; 10× PCR buffer contained 166 mM ammonium sulfate, 670 mM
Tris (pH 8.8), 67 mM MgCl2, 50 mM 2-mercaptoethanol, and 67 µM EDTA. PCR was performed with an MJ thermocycler using the
following program: step 1, 93°C for 1.5 min; step 2, 93°C for 0.5 min; step 3, 57°C for 0.5 min; step 4, 65°C for 3 min; repetition
of steps 2 to 4 40 times. For each allele, three PCR primers were used
for simultaneous amplification of both mutant and wild-type alleles.
Sequences of PCR primers used in genotyping and the results expected
from use of each primer set are shown in Tables
1 and 2.
Western and RT-PCR analyses.
Western analysis was carried
out by first separating nuclear extracts on a sodium dodecyl
sulfate-10% polyacrylamide gel and then blotting the proteins
to a nitrocellulose membrane. Anti-E2A polyclonal sera (provided by T. Kadesch), anti-E2A monoclonal antibody (Yae; Santa Cruz
Biotechnology), and anti-HEB polyclonal sera (Santa Cruz) were used to
detect relevant E proteins. Horseradish peroxidase-conjugated secondary
antibodies were used in an enhanced chemiluminescence (ECL) reaction
(Amersham). Reverse transcription (RT)-PCR was carried out essentially
as described (20). Briefly, 0.1 µg of cytoplasmic RNA was
used in each RT reaction, and 1/10 of the reaction mixture was used for
each PCR. PCR was carried out for 22 cycles with elongation factor 1 alpha (EF1
) primers and 28 cycles with all of the E2A primers.
Flow cytometry.
Bone marrow, spleen, and fetal liver cells
were isolated from various age group mice and used immediately for
fluorescence-activated cell sorting (FACS) analysis. Cell suspensions
were stained with a combination of a fluorescein isothiocyanate
(FITC)-conjugated antibody and a phycoerythrin
(PE)-conjugated antibody plus 7-amino-actiomycin D (7AAD).
Live cells were analyzed on a FACScan (Becton Dickinson) for
simultaneous detection and recording of FITC, PE, and 7AAD signals.
Data were processed by using the CellQuest program (Becton Dickinson). 7AAD is a DNA dye that stains permeable or dead cells (Molecular Probes). The use of 7AAD was crucial for eliminating nonspecific staining of antibodies to dead cells. Anti-mouse CD19 antibody was provided by S. Sato and T. F. Tedder (21).
All other antibodies were purchased from Sigma, Jackson Immunology, and
Pharmingen.
Irradiation and stem cell reconstitution.
C57BL/6 mice
congenic for the Ly5A allotype marker were purchased from Jackson
Laboratories. Host mice at 8 to 12 weeks of age were irradiated with
1,100 rads 1 day before stem cell transfusion and maintained in sterile
bedding and antibiotics thereafter. Donor cells were prepared from
either frozen stocks or freshly isolated fetal liver or bone marrow
cells. From 0.1 × 106 to 0.5 × 106
total fetal liver or 0.5 × 105 to 2 × 105 bone marrow cells were delivered to the host in 0.2 ml
of phosphate-buffered saline through tail vein injection. For each
donor type, two to five recipients were used in the test. Mice were
bled at 1 month and sacrificed at 2 months after irradiation for FACS
analysis.
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RESULTS |
E2A alleles used in this study.
Table
3 lists the E2A alleles used in this
study. E2Ako and E2Agal are two independent
alleles with both E12 and E47 exons deleted from the gene. The
E2Ako allele (also known as E2A
bhlh) has
been thoroughly characterized and reported in an earlier study
(35). The phenotype of E2Agal is essentially the
same as E2Ako except that the former expresses a
-galactosidase marker driven by the endogenous E2A promoter. In this
report, both alleles are used interchangeably as E2A-null controls. The
E12ko allele has been generated and analyzed at the ES cell
level in a previous study (34). Essentially, the Neo
coding sequence was inserted into the E12 exon to produce a E2A-Neo
fusion protein and cause a disruption of E12 (34). The mouse
strain carrying this mutation was generated and characterized in this
study. E47bm and E2Aheb are newly created
alleles and are fully described in this report.
Disruption of the DNA binding domain of E47.
We used a
dominant negative strategy to investigate the function of E47 and its
potential dimerization partner(s). In principle, a point mutation in
the E47 basic region disrupts the DNA binding but not the protein
dimerization activities of E47. Such a mutation not only abolishes the
function of E47 homodimer but can inhibit the function of putative E47
heterodimers and thus may help reveal the identity and function of E47
dimerization partner(s).
The mutation of E47 was introduced into the E2A locus by gene targeting
(Fig.
1A). This change replaced two conserved arginines
with glycines
in the protein and added a new
BamHI site in the
DNA.
Mutation at the identical positions has been shown previously
to be a
true dominant negative mutation in gel shift assays (
30).
In
addition to the mutation in the basic region, the gene targeting
construct also contained PGK-Neo as a positive selection marker
and
PGK-TK as a negative selection marker. Integration of PGK-Neo
into the
E2A locus was determined by PCR analysis with primers
YZ-29 and YZ-104,
which specifically detects homologous recombination
at the 3' region.
The positive clones were subsequently analyzed
by a second round of PCR
using primers E21 and YZ-24. An integration
of the basic region
mutation was scored by restriction enzyme
digestion of the PCR
products, which should contain a
BamHI site
if the E47 basic
mutation is retained after recombination. The
frequency of gene
targeting after the double selection was approximately
30%. About half
of the targeted clones carried the basic mutation.
This mutant allele
was named E47
bm. The E47
bm mouse strain used in
the subsequent experiments was derived from
two independently targeted
clones and bred in the 129/sv and C57BL/6
mixed background.
To determine whether the expression of E2A is affected by the PGK-Neo
marker inserted downstream of the E2A gene, RT-PCR was
used to evaluate
the RNA levels of E12 and E47 in E47
bm mice (Fig.
1C). The newly
introduced
BamHI site served as an
allelic marker to
distinguish the mutant allele and the wild-type
allele in
E47
bm heterozygous mice. Because of a severe impairment of
B-cell development
in E47
bm mice, thymocyte RNA were used
in this assay. Four sets of PCR
primers, including EF1
as an
internal control, were used for
each sample. This semiquantitative
RT-PCR assay showed that the
expression levels of E2A in
E47
bm homozygous mice was reduced to about 60% of the
wild-type level
(comparing E2A with EF1
), and the ratio of E47/E12
splicing was
increased approximately 80% (comparing E47
bm
with E12). Although the cause of the change in splicing is still
under
investigation, the analysis clearly demonstrates the presence
of the
E12 transcript in the E47
bm mice.
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FIG. 1.
(A) The 3' portion of the mouse E2A genomic DNA (from
KpnI to BamHI) was used in the gene targeting
experiment. The exons contained within this piece of genomic DNA are
shown as shaded boxes. The direction of the E2A gene, positions of E12
and E47 exons, and the 3' polyadenylation site of the E2A gene are
shown. The structures of E12ko and E47bm
alleles are shown according to the scale of the wild type
(wt). The E12ko allele was generated by
insertion of a promoterless neo gene into the E12 exon
(34). The E47bm allele was generated by
cointegration of a point mutation and a selection marker into the E2A
gene. "B" above the E47 exon of the E47bm allele
indicates the position of the basic-region mutation and the addition of
a BamHI site. A PGK-Neo cassette running in the same
direction as the E2A gene is inserted into the unique XbaI
site downstream of the E2A gene. The names, positions, and directions
of PCR primers used in the experiment are shown below the constructs.
RV, EcoRV. (B) Detailed structure of the E47-specific exon.
Sequences of the basic region of E47 wild-type and E47bm
alleles are shown. Underlines indicate amino acid residues that are
conserved in the bHLH gene family, and boldface indicates the changes
made in E47bm. (C) RT-PCR analysis of thymocyte RNA
prepared from E47bm homozygous, E47bm
heterozygous, and wild-type animals. For each reverse-transcribed RNA
sample, four sets of PCRs were performed with primers specific to (i)
EF1 gene, (ii) E2A exons common to both E12 and E47, (iii) the
E12-specific exon, and (iv) the E47-specific exon. To differentiate E47
wild-type and the E47bm alleles, PCR product generated with
E47 primers was digested with BamHI, which is present in the
E47bm but not the wild-type allele (in lanes
E47bm +/ and E47bm /). Results are
representative of three repeated experiments with multiple individuals
from each genotype. (D) Western analysis of E2A proteins in the thymus isolated from the wild-type,
E2Ako, E47bm, and E12ko mice.
Genotypes of the samples are indicated at the top. Size markers in
kilodaltons are shown at the left, and positions of the full-length E2A
proteins are indicated at the right.
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Western analysis of thymus extracts showed that the expression level of
total E2A proteins in the E47
bm homozygous animals is
approximately the same as in wild-type
controls (Fig.
1D). Although
separate anti-E2A antibodies have
been used to verify this result, we
cannot yet distinguish E12
and E47 with the reagents available.
E47 is not essential for survival and reproduction.
Previous
studies on the E2A knockout mice have shown that deletion of the E2A
gene resulted in a high frequency of postnatal death and deficiency in
B-lineage formation (2, 35). Subsequent studies also show
that the surviving E2Ako females are sterile, while males
are fertile (data not shown). In contrast to the E2Ako
mice, the survival rates of E47bm mice are
indistinguishable from those of their wild-type or heterozygous littermates, and both males and females are fertile. This result indicates that the DNA binding activity of E47 is not essential for
postnatal survival and reproduction. Furthermore,
E47bm may play a dominant role in keeping these mice
alive and fertile, perhaps by keeping Id levels in check
(33). Although the dominant negative effect of
E47bm cannot be completely understood before a true
E47-null allele is available (experiment is under way), the improved
viability and fertility already makes the E47bm mice a
valuable strain (see below).
Mice without normal E47 proteins are able to produce B cells in
neonatal but not adult life.
The earliest committed B-lineage
cells are characterized by surface expression of B220, CD43, and CD19
antigens (9, 19). As cells mature from pro-B to pre-B cells,
both B220 and CD19 are gradually upregulated, whereas CD43 is
downregulated. Mature B cells in the bone marrow and spleen express, in
addition to B220 and CD19, surface IgM. When these markers are used to
analyze E47bm neonates, we find a 10-fold reduction of pro-
and pre-B-cell numbers in the bone marrow and more than a 20-fold
reduction of B-cell numbers in the spleen (Fig. 2A and
C). B cells found in E47bm
bone marrow are further verified by PCR analysis of the Ig heavy-chain locus, which detects substantial DH-JH
rearrangement (Fig. 3). No B cells are
detected by either flow cytometry or PCR analysis of
DH-JH rearrangements in the same age group of
E2A-null mice. This result indicates that in the absence of normal E47
protein, E12 is sufficient to support a limited but definitive B-cell
commitment at the neonatal stage.
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FIG. 2.
(A) Three-channel FACS analysis of live bone marrow (top
two panels) and spleen B cells (bottom panel) prepared from 10- to
20-day-old pups carrying various E2A mutations. The genotype of each
animal is indicated above each vertical panel, which is composed of
three FACS analyses of the same animal. B220-FITC and 7AAD were
included in all the stainings. In addition, CD19-PE or CD43-PE was used
in the bone marrow samples, and IgM-PE was used in the spleen samples.
The variation in the levels of CD19-PE staining is due to batch
difference in the antibody used. To enrich lymphocytes and to exclude
dead cells in the analysis, size gate and 7AAD gate were used for all
the dot plots displayed. The relative percentages of pro-B, pre-B, and
mature B cells in total live cells are given in each plot. FACS
analysis of B cells in adult mice. Wild-type control, E47bm
homozygous and E47bm/E12ko transheterozygous
mice were analyzed with B220 and 7AAD plus CD19 for bone marrow, IgM
for spleen, and CD5 for peritoneum samples. Presentation of data is as
described for panel A. (C) Average B-cell numbers as a percentage of
total nucleated bone marrow or spleen populations. Both sample size and
standard deviation are shown with each data bar. Four genotype groups
of animals, wild-type (wt), E47bm homozygous,
E12ko homozygous, and E47bm/E12ko
transheterozygous, are included. Pup is equivalent to 10 to 20 days
old; adult is more than 2 months old.
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FIG. 3.
PCR analysis of Ig heavy-chain gene D-J rearrangements.
Genomic DNA was purified from bone marrow of either 10- to 20-day-old
neonates or 2-month-old adults. PCR was carried out with a J4-specific
primer (24) and a D-segment-specific primer that hybridizes
to the upstream sequence of most D segments (8). PCR
products representing specific D-J rearrangements were revealed by a
radiolabeled oligonucleotide that hybridizes to the internal side of
the J4 primer. The running positions of DNA size markers and J segments
are indicated on the left and right side, respectively. WT, wild
type.
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This limited B lymphopoiesis in E47
bm mice, however, is
observed only during the first few weeks of postnatal life. Analysis
of
2- to 4-month-old-mice failed to detect B cells in bone marrow,
spleen,
and peritoneum (Fig.
2B and C). Although less than 1%
of
B220
+ CD19
cells were detected in bone
marrow, PCR analysis did not show
any D
H-J
H
rearrangement in these cells, indicating that these
B220
+
CD19
cells had not yet committed to the B-cell lineage
(Fig.
3). Recent
studies by several groups have shown that bone marrow
B220
+ CD19
cells contain progenitors of
B-lymphoid, natural killer, and
other undetermined cell types
(
19).
Mice without E12 have limited capacity to generate B cells.
Parallel to the analysis of E47bm mutation, we also tested
an E12-specific mutation, which had been generated and analyzed
previously at the ES cell level (34). This mutant allele was
made by inserting the Neo coding region into the bHLH domain of the
E12-specific exon. This mutation was introduced recently into mice
through blastocyst injection, and the resulting mice were subsequently bred into 129/sv and C57BL/6 backgrounds. The expression of E47 in the
E12ko homozygous background was verified by RT-PCR analysis
(34) and by Western analysis in this study (Fig. 1D). In
contrast to mice with the E47bm mutation, the survival rate
for E12ko mice was lower than normal but significantly
higher than that of E2A knockout mice (data not shown). With limited
breeding, E12ko males were found to be normal in
reproduction, while females were sterile.
At the neonatal stage, E12
ko mice showed limited capacity
to produce B cells. Similar to the phenotype of E47
bm mice,
a small number of B cells were found in the bone marrow
and spleens of
neonatal E12
ko mice. The bone marrow B cells were mostly
B220
+ CD19
+ CD43
+ and
D
H-J
H-rearranged pro-B cells, and the splenic B
cells were
B220
+ IgM
+ mature B cells (Fig.
2A
and C; Fig.
3). This result indicates
that in the absence of E12, E47
alone is capable of supporting
B-cell commitment. However, since the
number of B cells produced
in E12
ko mice is less than 10%
of the wild-type level, the function of
E47 must be limited. A noted
difference between E12
ko and E47
bm mice is that
small numbers of B cells are frequently, but not
always, found in the
spleens of adult E12
ko mice (Fig.
2C). Although the number
of B cells is about 1 to
5% of the wild-type level, they can produce a
substantial amount
of serum Igs (data not shown).
E47bm/E12ko transheterozygous mice
are phenotypically similar to the E47bm
or E12ko homozygous mice.
It was not clear why
E47bm and E12ko mice had only limited capacity
to produce B cells. One possible interpretation is that the levels of
functional E12 or E47 proteins in E47bm or
E12ko mice are reduced below a threshold level which is
required for maintaining normal B lymphopoiesis. RT-PCR analysis
clearly showed a small but detectable reduction of E12 and E47
messages in E47bm and E12ko mice, respectively.
In the E47bm mice, the level of functional E12 proteins may
be reduced even further by a dominant negative effect from the
E47bm allele, but we cannot say if this suboptimal gene
expression is sufficient to account for the impairment of B
lymphopoiesis in these mice.
Alternatively, the lack of sustained B lymphopoiesis in
E47
bm and E12
ko mice may be due to the
disruption of synergy between the two
E proteins, a possibility
suggested by Bain et al. (
3). To
evaluate this
scenario, we analyzed the E47
bm/E12
ko
transheterozygous mice. The transheterozygous mice were born
and
lived to adulthood without any superficial difference from
the control
littermates. Although both E12 and E47 messages are
present in
these transheterozygous mice (data not shown), their
capacity to
produce B-lineage cells is about the same as that
of homozygous
E12
ko or E47
bm mice (Fig.
2A and C); i.e.,
small numbers of B-lineage cells
are detected in neonates but not in
adults. This result indicates
that coexpression of wild-type E47 and
E12 proteins in the same
animal is sufficient to initiate B
lymphopoiesis in the neonates
but not sufficient to maintain B
lymphopoiesis in the adult. Given
the potential dominant negative
effect from the E47
bm allele, we cannot say how much of the
functional E12 and E47
proteins are available to support B
lymphopoiesis in the E47
bm/E12
ko mice. However,
the phenotypic similarity among E47
bm homozygous,
E12
ko homozygous, and E47
bm/E12
ko
transheterozygous mice indicates an underlying common defect
in
these mice.
Stem cell transfusion confirms a B-cell-specific role for E12 and
E47.
E12ko and E47bm mice have a limited
capacity to generate B-lineage cells. This suppression of B
lymphopoiesis could be due to an intrinsic defect within the B-cell
lineage, a nonsupportive stromal environment, or both. To test this
possibility, we performed a stem cell transfusion test. HSC from either
the fetal livers of E12ko mice or the bone marrow of
E47bm neonates were used as donors to complement lethally
irradiated wild-type hosts. As shown in Fig.
4A, HSC from both E12ko and
E47bm mice are capable of providing radioprotection and
giving rise to T-lymphoid, myeloid cells but not B cells. Meanwhile, a
normal number of B cells can be generated when wild-type fetal liver or
bone marrow is used as the donor. This result confirms the transfusion
test with the E2A-null cells as donors (36) and indicates
that disruption of either E12 or E47 specifically limits the potential
of hematopoietic stem cells to give rise to B-lineage cells.
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FIG. 4.
(A) FACS analysis of spleen samples from stem cell
transfusion experiments. Sources of donor stem cells are indicated at
the top (BM, bone marrow; wt, wild type; FL, fetal liver). Each
vertical panel represents separate FACS analysis for B cells (IgM), T
cells (CD5), and myeloid cells (Mac1) from the same splenic sample.
CD45.2 (Pharmingen) is an allotype marker that is present on the donor
cells and absent on host cells. To eliminate nonspecific staining and
dead cells, 7AAD was also included in all the staining reactions.
Percentages of cells given in the quadrants are calculated based on
total live cells rather than the size-gated population. Data are
representative of two to five independent transfusion tests for each
donor type. (B) FACS analysis of an E47bm mouse
(representative of three mice) reconstituted with the wild-type HSC.
Cells from bone marrow, spleen, and blood were analyzed with a B-cell
marker (B220) and a myeloid cell marker (Mac1). Donor cells were
derived from wild-type C57BL/6Ly5A mice and were negative for CD45.2,
whereas host cells were positive for the CD45.2 marker. Gating and data
presentation are as in panel A.
|
|
Adoptive transfer in the reverse direction has been impossible in the
past because of the lethality of E2A knockout. The E47
bm
mice generated in this study provided excellent hosts for transfusion
tests. We now know that wild-type HSC can provide complete
radioprotection
and give rise to B-lineage cells in the lethally
irradiated E47
bm hosts (Fig.
4B), demonstrating a
permissive stromal environment
for B lymphopoiesis in E47
bm
mice. Therefore, the lack of B lymphopoiesis in adult E47
bm
mice is almost exclusively due to a B-lineage autonomous defect.
Replacement of E2A with a human HEB cDNA.
Analyses of
E47bm and E12ko mice suggest that the
B-cell-specific function of E2A has at least two features: it requires
a structural domain shared by both E12 and E47, and it demands a
minimal dosage of functional E2A proteins. To further explore the
molecular basis of these phenomena, we compared the functions of E2A
proteins and HEB protein, which is encoded by a separate E-protein
gene. The sequence similarity at the amino acid level between HEB and E2A is 82% (for E47) and 89% (for E12) within the bHLH domain and is
significantly lower outside the bHLH domain (11). We had
shown previously by gene disruption that HEB is not essential for
B-cell commitment and differentiation. However, mice
compound-heterozygous for E2A and HEB disruption have reduced
capacity for producing pro-B cells in fetal liver, suggesting the
involvement of HEB in B lymphopoiesis.
To allow a direct comparison of the function of E2A and HEB in the
context of B-cell development, we introduced an HEB cDNA
into the
E2A locus through gene targeting. A full-length human
HEB cDNA
driven by an IRES (see Materials and Methods) was used
to replace the
E12 and E47 exons. Selection of targeting events
was achieved by adding
the
neo gene in frame with the E2A coding
sequence (Fig.
5A). Gene-targeting events with this HEB
insertional
construct were obtained at a frequency of 65% after G418
selection,
demonstrating the selection efficiency of the construct. The
validity
of this targeting strategy for expression of an inserted cDNA
under the endogenous E2A promoter has been demonstrated by the
construction and analysis of the E2A
gal allele, in which
inactivation of the E2A gene is concomitant
with the expression of a
-galactosidase marker by the endogenous
E2A promoter (
34,
35). We have since shown that this E2A
gal allele
drives
-galactosidase expression in a broad pattern throughout
embryogenesis (data not shown).
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FIG. 5.
(A) Gene targeting construct for generating the
E2Aheb allele. The Neo marker was introduced in the E2A
gene as a fusion protein. IRES-driven human HEB cDNA was inserted
downstream of the Neo cassette but in front of the E2A translation
termination site. Both E12 and E47 exons are completely deleted from
the targeting construct. Primers used for PCR genotyping the
mutant and wild-type (wt) alleles are indicated (see
Materials and Methods). Designations are as in Fig. 1A. (B) Western
blot analysis of thymus (lanes 1 to 4) and spleen (lanes 5 to 8)
nuclear extracts from 10-day-old neonatal mice of indicated
genotypes. Wild-type, E2Ako heterozygote,
E2Aheb heterozygote, and E2Aheb
homozygote samples are included in the assay as indicated. The anti-HEB
polyclonal sera used in this assay (Santa Cruz) cross-react with both
human and mouse HEB proteins. Size markers in kilodaltons and the HEB
band are indicated on the left and right, respectively. (C) Gel shift
analysis of E-protein complex formation, using µE5 radiolabeled
probe. µE5 probe (25) was incubated with nuclear extracts
from splenocytes (lanes 1 to 6) or thymocytes (lanes 7 to 11) derived
from wild-type (lanes 1, 2, 3, 7, 8, and 9) or E2Aheb
(lanes 4, 5, 6, 10, and 11) animals. Anti-E2A antibody (Yae) was added
in lanes 2, 5, and 8, and anti-HEB antibody (Santa Cruz) was added in
lanes 3, 6, 9, and 11. The E2A- and HEB-dependent supershifts are
indicated by arrows on the left and right sides, respectively. Assay
conditions are as described by Sawada and Littman (22).
|
|
Mice carrying the newly created gene replacement allele, named
E2A
heb, were tested by Western analysis for expression of
the human
HEB protein. Whole-cell extracts from spleen and thymus
were probed
with anti-HEB antibodies, which cross-react with both
human and
mouse HEB proteins. As shown in Fig.
5B, the level of
the endogenous
HEB proteins is low in the spleen and high in the thymus
in wild-type
animals. Replacement of the E2A gene with the HEB cDNA
leads to
a moderate increase of HEB proteins in the thymus and a
dramatic
increase of HEB proteins in the spleen. Disruption of the E2A
proteins was verified by anti-E2A antibodies (data not shown).
Because no increase of HEB expression is seen in E2A
ko
heterozygous mice, we conclude that the increased HEB proteins
are derived from the human HEB cDNA rather than from upregulation
of
the endogenous mouse HEB gene.
A gel shift assay with the Ig µE5 enhancer was used to evaluate
the activity of HEB proteins produced from the E2A locus.
It has been
well documented that µE5 is specifically recognized
by
E2A-containing protein dimers in B-cell extracts (
1). As
shown in Fig.
5C, the E2A-µE5 complex can be seen as a supershift
with anti-E2A antibody in wild-type splenocytes (lane 2) but not
in
E2A
heb/ splenocytes (lane 5). In contrast, an HEB-µE5
complex is seen
as a supershift with anti-HEB antibody in the
E2A
heb splenocytes (lane 6) but not in the wild-type
splenocytes (lane
3), suggesting that the E2A-dependent µE5 binding
activity has
been replaced by HEB. However, HEB may have a lower
affinity for
the µE5 site than E2A does in the splenocytes since the
HEB-µE5
complex can only be seen as a supershift (lane 6). The
activity
of HEB proteins was also tested in thymocyte extracts, where a
replacement of the HEB-E2A heterodimers (lane 7 to 9) by HEB homodimers
(lane 10, 11) was observed in the E2A
heb mice. This result
is consistent with an observation made by Sawada
and Littman
(
22) that E proteins in wild-type T cells were
heterodimers
between E2A and HEB.
A copy number-dependent rescue of B-cell development by
E2Aheb.
The activity of E2Aheb in B
lymphopoiesis was tested by analyzing B-cell contents in the bone
marrow and spleens of preweaning-age animals, a stage when B
lymphopoiesis is sensitive to the E2A protein dosage. Even in
heterozygous animals, a contribution to B-cell development from the
E2Aheb allele can be readily seen by comparison of
E2Aheb heterozygous mice with E2Ako
heterozygous mice. As shown in Fig. 6B,
E2Aheb heterozygous mice generate twice as many B cells as
E2Ako heterozygous mice do. The number of B cells found in
E2Aheb heterozygous mice is no less, and perhaps
slightly higher, than the B-cell number in the
wild-type controls. We then tested E2Aheb activity on the
E2A-null background by crossing E2Aheb heterozygous mice
with E2Ako heterozygous mice. Genotyping analysis of 1- to
3-week-old pups showed that the survival rate of transheterozygous
offspring is slightly lower than expected (16 wild type, 36 heterozygous, and 11 transheterozygous) but significantly improved
from age-matched E2A-null homozygous mice (33). FACS
analysis with B-cell lineage markers showed that the
E2Aheb/E2Ako mice generate extremely low
numbers of pro-B cells (B220+ CD43+
CD19+) in the bone marrow of neonatal mice (Fig. 6). This
result indicates that one copy of E2Aheb is insufficient to
completely rescue E2A-null defects.
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FIG. 6.
(A) FACS analysis of mice carrying one or two copies of
E2Aheb. Bone marrow (top two panels) and spleens (bottom
panel) from 10-day-old wild-type (WT),
E2Ako/E2Aheb transheterozygous, and
E2Aheb homozygous mice were analyzed with B-cell markers.
Plots were gated on live lymphocytes based on cell size and 7AAD
staining. Percentages of cells shown in the quadrants represent the
fractions of total live cells analyzed. (B) B-cell contents as a
percentage of total live suspension cells for the five genotypes.
Percentages of B cells in bone marrow and spleen are calculated based
on the analysis of multiple litters with ages ranging from 1 to 3 weeks. Sample size and standard deviation are shown with each data bar.
Relatively large standard deviations for most spleen samples are due to
a sharp increase of B-cell content in the first 3 weeks of postnatal
life.
|
|
E2A
heb homozygous mice are recovered with expected
frequency (14 +/+, 35 +/
, and 22
/
) from E2A
heb
heterozygous intercross. These E2A
heb homozygous mice are
superficially indistinguishable from their
wild-type and heterozygous
littermates, indicating a general rescue
of E2A-null defects by two
copies of E2A
heb. Further, interbreeding of
E2A
heb homozygous mice has produced healthy offspring. In
contrast to
the E2A
heb/E2A
ko transheterozygous
mice, a substantial number of B-lineage cells,
including pro- and pre-B
cells and mature B cells, were detected
in bone marrow and spleen,
respectively (Fig.
6). This result
indicates a functional replacement
of E2A by HEB in both the commitment
and maturation processes of B
lymphopoiesis. The number of bone
marrow B cells in these
E2A
heb mice is about 40% of the number in the
wild-type littermates,
nearly reaching the B-cell number in
age-matched E2A
ko heterozygous mice (Fig.
6B). Such a log
scale increase of B-cell
numbers from mice carrying one copy of
E2A
heb to mice carrying two copies of E2A
heb
strongly argues that a threshold level of E proteins is critical
and
essential for B-cell commitment.
| |
DISCUSSION |
E2A encodes two broadly expressed bHLH proteins that play specific
and essential roles in B lymphopoiesis. How functional specificity is
achieved by the E2A gene is central to our understanding of
E2A-mediated regulatory pathways in B lymphopoiesis. B-cell-specific posttranslational modification of E47 has been postulated as a major
event in regulating E2A protein activity, which in principle provides
the needed functional specificity. This model suggests that the
functional specificity of E2A is mediated by E47 homodimerization, which is detected exclusively in B-lineage cells. Further, the model
suggests that the structure of the E47-specific exon provides the
functional specificity and excludes any functional significance of E12
and other E proteins in B lymphopoiesis. This model is challenged by a
transgenic rescuing test carried out by Bain et al. (3) and
is further questioned by two pieces of genetic evidence reported here.
First, we have shown that either E12 or E47 alone is capable of
supporting limited but definitive B lymphopoiesis. Second, we have
shown by gene replacement that HEB can replace the function of E2A in
driving B-cell commitment and maturation. Both findings favor the
notion that the functional specificity of E2A is largely determined at
the transcription level of the E2A gene.
Functional requirement of E47 and E12 throughout B-cell
development.
Although E47 or E12 alone is sufficient to
support B-cell commitment and differentiation into mature B
cells, the entire process is extremely inefficient. Pro-B, pre-B, and
mature B cells are generated in both E47bm and
E12ko mice but at levels more than 10-fold lower than in
their wild-type littermates. In wild-type mice, pro-B cells represent
only a small fraction of the total population of B-lineage cells in the
bone marrow. In contrast, most B-lineage cells detected in the
bone marrow of E47 and E12 knockout mice are B220+
CD43+ CD19+ pro-B cells. The unbalanced ratio
of pro-B versus pre-B cells suggests a role for E2A proteins in
differentiation from pro-B to pre-B cells. It has been well established
that transition from pro-B to pre-B stage is dependent on
proper expression and selection of the B-cell receptor genes.
Indeed, the Ig heavy-chain and light-chain genes, the terminal
deoxynucleotide transferase gene, and surrogate light-chain
genes lambda 5 and V-pre-B are among the demonstrated targets of
E2A (6, 23, 26). Therefore, E2A proteins, in addition to
their unique role in supporting B-lineage commitment, may play a much
broader role in later stages of B-cell development.
The combined dosage of E47 and E12 is required for B-cell
development.
We have shown that
E47bm/E12ko transheterozygous mice have no
better capacity to generate B cells than E12ko or
E47bm homozygous mice. Therefore, the mere presence of both
E12 and E47 proteins is not sufficient to support normal B
lymphopoiesis. Comparison with E2Ako heterozygous mice
which also carry a single copy of E47 and E12 shows that
transheterozygous E47bm/E12ko is composed of an
E47bm allele. However, the E2Ako heterozygous
mice can produce 50% wild-type levels of pro- and pre-B cells in fetal
and neonatal life and near normal levels of B cells in adult life
(35). The phenotypic discrepancy between E47bm/E12ko and E2Ako heterozygous
mice may be partially due to inadvertent reduction of E12 and E47
expression from the mutated E47bm and E12ko
alleles, respectively. Alternatively, the discrepancy may be attributed
to a dominant negative effect from the E47bm allele; e.g.,
E47bm may inhibit the activity of E12 and E47 through
competitive dimerization. In either case, the end result is a further
reduction of functional E proteins below one-half of the wild-type
level in the E47bm/E12ko mice. Perhaps this
subtle difference in the level of functional E2A proteins is
sufficient to trigger a threshold effect, leading to inefficient B
lymphopoiesis in the E47bm/E12ko mice.
Function by context rather than by a unique structure.
The
existence of functional specificity among different E-protein genes is
supported by gene knockout studies (36). However, it is not
clear how functional specificity for each E-protein gene is defined and
regulated. Because all three E-protein genes are broadly,
although not evenly, expressed in different tissues, transcriptional regulation has been generally discounted as a way to
achieve functional specificity. All of the evidence accumulated prior
to this study favors the notion that functional specificity of E2A in
B-cell development is determined mainly by a unique structure of E2A,
in particular the E47 protein (5, 25). HEB and E2-2 can
modulate E2A activity in two possible ways: they can interact
directly with E12 and E47 through heterodimerization (1, 22)
or indirectly affect E2A activity through interactions with the
Id proteins (28, 36). Since mice lacking either HEB or E2-2
can still generate a substantial number of B cells (36), these presumed functions of HEB and E2-2 are apparently nonessential. A
functional replacement of E2A with HEB, shown in this study, argues
that HEB, E2A, and perhaps E2-2 as well share a common protein
structure necessary and sufficient to support B-cell commitment and
maturation. This finding challenges the existing hypothesis and
suggests that the functional specificity of E2A is determined primarily
by transcriptional regulation of the E2A gene.
Threshold regulation
from Drosophila to mice.
The
high degree of conservation among different E proteins at both
structural and functional levels argues that E proteins must play
fundamental roles during development. In fact, this conservation of E
proteins can be traced back to invertebrates such as
Drosophila, in which a single E-protein-equivalent bHLH gene
known as daughterless was found. It has been shown that
daughterless is involved in regulating
differentiation events such as sex determination in a dosage-dependent
manner (7, 17). The regulation of differentiation events by
daughterless in invertebrates is reminiscent of the dosage-dependent regulation of B-cell development by the E
proteins in mammals. In both cases a critical level of bHLH
proteins is required to trigger a binary switch leading to irreversible
differentiation events, namely, establishment of the female body
plan in Drosophila and the B-cell lineage in mice. This
structural and functional conservation between the fly
daughterless gene and the mouse E2A gene suggests that the
threshold mechanism may be more generally used by transcription factors
in the regulation of other cell lineages.
Why three functionally equivalent E-protein genes?
This study
also poses an important question: why do mammals need three
functionally equivalent E-protein genes? For simplicity, we discuss
only the common roles shared by these E proteins, although subtle
differences, such as dimerization specificity and affinity to specific
DNA sites, clearly exist. It may be argued that a functional
diversification at the protein level may not be tolerated if the
ancestor E protein plays a fundamental role which has been fixed in
evolution. Our study suggests that the function of the E proteins,
although fixed, is subject to tissue specific regulation. The
transcriptional regulation of the E2A gene in B cells is, perhaps, only
one of many tissue-specific regulation events that have occurred during
embryonic and tissue development; each event may be regulated by a
unique enhancer (or a unique set of enhancers) attached to the gene.
Intuitively, there may be a limit for how many tissue-specific
enhancers can be added to a single gene. We argue that gene duplication
may be a simple way to accommodate the increasing need for
tissue-specific regulation of the conserved function provided by the
ancestor E-protein gene. This interpretation predicts that as important
as transcriptional regulation of the E2A gene is to B-cell development,
transcriptional regulation of the HEB and E2-2 genes may be important
to other cell types.
| |
ACKNOWLEDGMENTS |
We thank Peifeng Cheng for assistance in generating the
E47bm mutation, Mike Krangel and Mike Krause for critical
reading of the manuscript, and Billie Maciunas for editorial
assistance. We are grateful to Duke Cancer Center Flow Cytometry
Facility for technical support.
This work was initiated with a fellowship award from the Leukemia
Society of America to Y.Z. and supported by a Whitehead Scholarship and
an NCI grant (R01CA72433-01) to Y.Z.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Immunology, Duke University Medical Center, Durham, NC 27710. Phone: (919) 613-7824. Fax: (919) 684-8982. E-mail:
yzhuang{at}acpub.duke.edu.
| |
REFERENCES |
| 1.
|
Bain, G.,
S. Gruenwald, and C. Murre.
1993.
E2A and E2-2 are subunits of B-cell-specific E2-box DNA-binding proteins.
Mol. Cell. Biol.
13:3522-3529[Abstract/Free Full Text].
|
| 2.
|
Bain, G.,
E. C. Robanus Maandag,
D. J. Izon,
D. Amsen,
A. M. Kruisbeek,
B. C. Weintraub,
I. Krop,
M. S. Schlissel,
A. J. Feeney,
M. van Roon,
M. van der Valk,
H. P. J. te Riele,
A. Berns, and C. Murre.
1994.
E2A proteins are required for proper B cell development and initiation of immunoglobulin gene rearrangements.
Cell
79:885-892[Medline].
|
| 3.
|
Bain, G.,
E. C. Robanus Maandag,
H. P. te Riele,
A. J. Feeney,
A. Sheehy,
M. Schlissel,
S. A. Shinton,
R. R. Hardy, and C. Murre.
1997.
Both E12 and E47 allow commitment to the B cell lineage.
Immunity
6:145-154[Medline].
|
| 4.
|
Benezra, R.,
R. L. Davis,
D. Lockshon,
D. L. Turner, and H. Weintraub.
1990.
The protein Id: a negative regulator of helix-loop-helix DNA binding proteins.
Cell
61:49-59[Medline].
|
| 5.
|
Benezra, R.
1994.
An intermolecular disulfide bond stabilizes E2A homodimers and is required for DNA binding at physiological temperatures.
Cell
79:1057-1067[Medline].
|
| 6.
|
Choi, J. K.,
C. P. Shen,
H. S. Radomska,
L. A. Eckhardt, and T. Kadesch.
1996.
E47 activates the Ig-heavy chain and TdT loci in non-B cells.
EMBO J.
15:5014-5021[Medline].
|
| 7.
|
Cline, T. W.
1989.
The affairs of daughterless and the promiscuity of developmental regulation.
Cell
59:231-234[Medline].
|
| 8.
|
Gu, H.,
D. Kitamura, and K. Rajewsky.
1991.
B cell development regulated by gene rearrangement: arrest of maturation by membrane-bound D mu protein and selection of DH element reading frames.
Cell
65:47-54[Medline].
|
| 9.
|
Hardy, R. R.,
C. E. Carmack,
S. A. Shinton,
J. D. Kemp, and K. Hayakawa.
1991.
Resolution and characterization of pro-B and pre-pro-B-cell stages in normal mouse bone marrow.
J. Exp. Med.
173:1213-1225[Abstract/Free Full Text].
|
| 10.
|
Henthorn, P.,
M. Kiledjian, and T. Kadesch.
1990.
Two transcription factors that bind the immunoglobulin enhancer µE5/kE2 motif.
Science
247:467-470[Abstract/Free Full Text].
|
| 11.
|
Hu, J.-S.,
E. N. Olson, and R. E. Kingston.
1992.
HEB, a helix-loop-helix protein related to E2A and ITF2 that can modulate the DNA-binding ability of myogenic regulatory factors.
Mol. Cell. Biol.
12:1031-1042[Abstract/Free Full Text].
|
| 12.
|
Jang, S. K., and E. Wimmer.
1990.
Cap-independent translation of encephalomyocarditis virus RNA: structural elements of the internal ribosomal entry site and involvement of a cellular 57-kD RNA-binding protein.
Genes Dev.
4:1560-1572[Abstract/Free Full Text].
|
| 13.
|
Lassar, A. B.,
C. Murre,
R. L. Davis,
A. Voronova,
W. E. Wright,
D. Baltimore,
T. Kadesch, and H. Weintraub.
1991.
Functional activity of myogenic HLH proteins requires hetero-oligomerization with E12/E47-like proteins in vivo.
Cell
66:305-315[Medline].
|
| 14.
|
Lin, H., and R. Grosschedl.
1995.
Failure of B-cell differentiation in mice lacking the transcription factor EBF.
Nature
376:263-267[Medline].
|
| 15.
|
Murre, C.,
P. S. McCaw, and D. Baltimore.
1989.
A new DNA binding and dimerization motif in immunoglobulin enhancer binding, daughterless, MyoD, and myc proteins.
Cell
56:777-783[Medline].
|
| 16.
|
Murre, C.,
P. S. McCaw,
H. Vaessin,
M. Caudy,
L. Y. Jan,
Y. N. Jan,
C. V. Cabrera,
J. N. Buskin,
S. D. Hauschka,
A. B. Lassar,
H. Weintraub, and D. Baltimore.
1989.
Interactions between heterodimeric helix-loop-helix proteins generate complexes that bind specifically to a common DNA sequence.
Cell
58:537-544[Medline].
|
| 17.
|
Parkhurst, S. M.,
H. D. Lipshitz, and D. Ish-Horowicz.
1993.
Achaete-scute feminizing activities and Drosophila sex determination.
Development
117:737-749[Abstract].
|
| 18.
|
Rolink, A., and F. Melchers.
1993.
B lymphopoiesis in the mouse.
Adv. Immunol.
53:123-156[Medline].
|
| 19.
|
Rolink, A.,
E. ten Boekel,
F. Melchers,
D. T. Fearon,
I. Krop, and J. Andersson.
1996.
A subpopulation of B220+ cells in murine bone marrow does not express CD19 and contains natural killer cell progenitors.
J. Exp. Med.
183:187-194[Abstract/Free Full Text].
|
| 20.
|
Rupp, R. A., and H. Weintraub.
1991.
Ubiquitous MyoD transcription at the midblastula transition precedes induction-dependent MyoD expression in presumptive mesoderm of X. laevis.
Cell
65:927-937[Medline].
|
| 21.
|
Sato, S.,
N. Ono,
D. A. Steeber,
D. S. Pisetsky, and T. F. Tedder.
1996.
CD19 regulates B lymphocyte signaling thresholds critical for the development of B-1 lineage cells and autoimmunity.
J. Immunol.
15:4371-4378.
|
| 22.
|
Sawada, S., and D. R. Littman.
1993.
A heterodimer of HEB and an E12-related protein interacts with the CD4 enhancer and regulates its activity in T-cell lines.
Mol. Cell. Biol.
13:5620-5628[Abstract/Free Full Text].
|
| 23.
|
Schlissel, M.,
A. Voronova, and D. Baltimore.
1991.
Helix-loop-helix transcription factor E47 activates germ-line immunoglobulin heavy-chain gene transcription and rearrangement in a pre-T-cell line.
Genes Dev.
5:1367-1376[Abstract/Free Full Text].
|
| 24.
|
Schlissel, M. S.,
L. M. Corcoran, and D. Baltimore.
1991.
Virus-transformed pre-B cells show ordered activation but not inactivation of immunoglobulin gene rearrangement and transcription.
J. Exp. Med.
173:711-720[Abstract/Free Full Text].
|
| 25.
|
Shen, C.-P., and T. Kadesch.
1995.
B-cell-specific DNA binding by an E47 homodimer.
Mol. Cell. Biol.
15:4518-4524[Abstract].
|
| 26.
|
Sigvardsson, M.,
M. O'Riordan, and R. Grosschedl.
1997.
EBF and E47 collaborate to induce expression of the endogenous immunoglobulin surrogate light chain genes.
Immunity
7:25-36[Medline].
|
| 27.
|
Sun, X.-H., and D. Baltimore.
1991.
An inhibitory domain of E12 transcription factor prevents DNA binding in E12 homodimers but not in E12 heterodimers.
Cell
64:459-470[Medline].
|
| 28.
|
Sun, X.-H.
1994.
Constitutive expression of the Id1 genes impairs mouse B cell development.
Cell
79:893-900[Medline].
|
| 29.
|
Urbanek, P.,
Z.-Q. Wang,
I. Fetka,
E. Wagner, and M. Busslinger.
1994.
Complete block of early B cell differentiation and altered patterning of the posterior midbrain in mice lacking Pax5/BSAP.
Cell
79:901-912[Medline].
|
| 30.
|
Voronova, A., and D. Baltimore.
1990.
Mutations that disrupt DNA binding and dimer formation in the E47 helix-loop-helix protein map to distinct domains.
Proc. Natl. Acad. Sci. USA
87:4722-4726[Abstract/Free Full Text].
|
| 31.
|
Wang, J. H.,
A. Nichogiannopoulou,
L. Wu,
L. Sun,
A. H. Sharpe,
M. Bigby, and K. Georgopoulos.
1996.
Selective defects in the development of the fetal and adult lymphoid system in mice with an Ikaros null mutation.
Immunity
5:537-549[Medline].
|
| 32.
|
Wilson, R. B.,
M. Kiledjian,
C. P. Shen,
R. Benezra,
P. Zwollo,
S. M. Dymecki,
S. V. Desiderio, and T. Kadesch.
1991.
Repression of immunoglobulin enhancers by the helix-loop-helix protein Id: implications for B lymphoid development.
Mol. Cell. Biol.
11:6185-6191[Abstract/Free Full Text].
|
| 33.
|
Yan, W.,
A. Z. Young,
Y. C. Soares,
R. Kelley,
R. Benezra, and Y. Zhuang.
1997.
High incidence of T-cell tumors in E2A-null mice and E2A/Id1 double knockout mice.
Mol. Cell. Biol.
17:7317-7327[Abstract].
|
| 34.
|
Zhuang, Y.,
C. G. Kim,
S. Bartelmez,
P. Cheng,
M. Groudine, and H. Weintraub.
1992.
Helix-loop-helix transcription factors E12 and E47 are not essential for skeletal or cardiac myogenesis, erythropoiesis, chondrogenesis, or neurogenesis.
Proc. Natl. Acad. Sci. USA
89:12132-12136[Abstract/Free Full Text].
|
| 35.
|
Zhuang, Y.,
P. Soriano, and H. Weintraub.
1994.
The helix-loop-helix gene E2A is required for B cell formation.
Cell
79:875-884[Medline].
|
| 36.
|
Zhuang, Y.,
P. F. Cheng, and H. Weintraub.
1996.
B-lymphocyte development is regulated by the combined dosage of three bHLH genes, E2A, E2-2, and HEB.
Mol. Cell. Biol.
16:2898-2905[Abstract].
|
Mol Cell Biol, June 1998, p. 3340-3349, Vol. 18, No. 6
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Copyright © 1998, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
