(Received for publication, October 22, 1996, and in revised form, January 30, 1997)
From the Institut de Génétique et de
Biologie Moléculaire et Cellulaire, CNRS/INSERM/ULP,
Collège de France, B.P. 163-67404 Illkirch Cédex,
France and the § Laboratoire de Biologie Moléculaire
et de Génie Génétique, Institut de Chimie-B6,
Université de Liège, B-4000 Sart-Tilman, Belgium
We report the cloning of a cDNA encoding the human transcription factor hTEF-5, containing the TEA/ATTS DNA binding domain and related to the TEF family of transcription factors. hTEF-5 is expressed in skeletal and cardiac muscle, but the strongest expression is observed in the placenta and in placenta-derived JEG-3 choriocarcinoma cells. In correlation with its placental expression, we show that hTEF-5 binds to several functional enhansons of the human chorionic somatomammotropin (hCS)-B gene enhancer. We define a novel functional element in this enhancer comprising tandemly repeated sites to which hTEF-5 binds cooperatively. In the corresponding region of the hCS-A enhancer, which is known to be inactive, this element is inactivated by a naturally occurring single base mutation that disrupts hTEF-5 binding. We further show that the binding of the previously described placental protein f/chorionic somatomammotropin enhancer factor-1 to TEF-binding sites is disrupted by monoclonal antibodies directed against the TEA domain and that this factor is a proteolytic degradation product of the TEF factors. These results strongly suggest that hTEF-5 regulates the activity of the hCS-B gene enhancer.
Human transcriptional enhancer factor (hTEF)-11 is the prototype member of the family of transcription factors containing the TEA/ATTS (hereafter called TEA) DNA binding domain (DBD, Refs. 1-3). Transcription factors belonging to this family have been identified in several organisms, where they fulfill various developmental functions. For instance, in yeast the TEC1 protein is postulated to regulate transcription from the Ty1 transposon and is required for pseudohyphal growth (4-6), while in Aspergillus nidulans the AbaA factor controls a regulatory circuit in the terminal stages of conidiophore development (7, 8). The Drosophila scalloped gene is required for normal development of the central and peripheral nervous systems, taste behavior, and normal wing morphology (9, 10).
In chicks and in mammals, binding sites for TEA domain proteins have been described in diverse types of enhancers with different tissue specificities (Refs. 1 and 11-18 and references therein, and see below). The activity of these sites was originally attributed to the binding of TEF-1, the first cloned mammalian TEF factor, identified by its binding to the GT-IIC and Sph enhansons of the simian virus 40 (SV40) enhancer, where it regulates transcription from the early and late promoters (1, 19-26). TEF-1 is expressed widely, but not ubiquitously, from early stages of murine embryonic development and in many established cell lines (Refs. 27-29 and references therein). TEF-1 expression is particularly pronounced in developing skeletal and cardiac muscle and in mitotic neuroblasts. Despite this wide pattern of expression, TEF-1 null mice show defects only in the heart, leading to embryonic lethality (28).
The vertebrate genome encodes at least four related TEF factors with
the TEA DBD (TEF-1, -3, -4, and -5; Refs. 13, 28, and 30-35), all of
which bind to the consensus site
(5-(A/T)(A/G)(A/G)(A/T)ATG(C/T)(G/A)-3
), containing a conserved ATG
core. The TEF-3 factor (28), also called chick RTEF-1 (35) or mouse
TEFR1/FR-19 (Refs. 31 and 32; summarized in Table I) is
expressed in several cell lines, and its expression can be induced by
mitogenic stimulation of quiescent fibroblasts or by in
vitro differentiation of myoblasts to myotubes (28, 31, 32). In
contrast to TEF-1, the expression of TEF-3 during mouse embryonic
development is largely restricted to the skeletal muscle lineage, where
it can be clearly seen at 10.5 days postcoitum, although at later times
it is also expressed in the developing lung and liver (28). In adult
mice and chicken, TEF-3 is expressed also in cardiac muscle (31-33,
35). In addition to TEF-1 and TEF-3, DTEF-1, whose expression is also
enriched in cardiac muscle, has been described in chicken (Ref. 33; see Table I). The muscle-enriched expression of these TEFs correlates with
the expression of known target genes, such as
- and
-myosin heavy
chain,
-skeletal actin, and cardiac troponin C, whose enhancers contain the TEF-binding M-CAT motif (11-17, 36-41), pointing to a
potential role for these TEFs in skeletal and cardiac muscle development.
|
TEF-4 was first described as a neuron-specific factor in the mouse as ETF (Ref. 34; see Table I); however, we have shown that it is strongly expressed throughout the embryo as early as 6.5 days postcoitum, while at later times its expression becomes more restricted to mitotic neuroblasts and to various mesenchymes (28). At later stages of embryogenesis, TEF-4 is also expressed in a number of developing organs (e.g. in the nephrogenic region of the kidney). Thus, the TEF-4 expression pattern is distinct from that of TEF-3 but partially overlaps with that of TEF-1. Although no target genes for the TEF factors have been described in neural and mesenchymal tissues, these observations suggest that TEF-1 and TEF-4 may play a role in neurogenesis and in the development of several organs. Thus, considered together, the above results suggest that the TEFs may play partially redundant roles in several developmental processes.
In addition to muscle-specific enhancers, putative TEF-binding sites have been noted in the placenta-specific human chorionic somatomammotropin (hCS; also called placental lactogen) B gene enhancer (42-45). The hCS-B enhancer is active in the cytotrophoblast-derived JEG-3 cell line and is progressively activated during the differentiation of primary cytotrophoblasts to syncytiotrophoblast in vitro (46). This enhancer can be divided into two functional elements, DF-3 and DF-4, each of which have been postulated to contain TEF-binding sites. Point mutations affecting the putative TEF-binding site within DF-4 inactivate this element (46-48). The TEF-binding site in DF-4 is recognized by placental protein f (PPf) or chorionic somatomammotropin enhancer factor-1 (CSEF-1) (43, 46-48). This factor(s) has not yet been identified, but it is apparently unrelated to TEF-1 (48).
By analogy to myogenesis, where muscle-specific TEF factors and target genes have been identified, a TEF factor(s) contributing to the function of placenta-specific enhancers may also exist. Here we report the cloning of hTEF-5, which is homologous to the B isoform of chicken DTEF-1 (33) and is expressed mainly in skeletal muscle and placenta. In correlation with this restricted expression pattern, we show that hTEF-5 binds to the M-CAT motifs of several muscle genes and to the TEF-binding site in the hCS-B DF-4 element. Furthermore, we have characterized a novel functional enhanson within the hCS-B DF-3 element composed of tandemly repeated binding sites to which hTEF-5 binds cooperatively. In the DF-3 element of the hCS-A enhancer, which is inactive in JEG-3 cells and syncytiotrophoblast, this enhanson is mutated by a naturally occurring single base change, which disrupts one of the conserved ATG cores and consequently hTEF-5 binding. We further show that PPf/CSEF-1 is immunologically related to the TEA domain and most likely corresponds to a proteolytic product of the TEF factors. Consequently, all of the factors identified to date interacting with the TEF-binding sites in the hCS-B enhancer belong to the TEA domain family. Together, these observations suggest that hTEF-5 is an important regulatory factor in the human placenta.
Two degenerate oligonucleotides
5-CCCAAGCTTGGC(A/C)GGAA(C/T)GA(A/G)(C/T)TGAT(A/C)GC-3
and
5
-CCCAAGCTTC(A/G/C/T)A(G/A)(A/G/C/T)AC(C/T)TG(T/G/A)AT(G/A)TG-3
), corresponding to the TEA domain amino acid sequences GRNELIA and HIQVL, were used as polymerase chain reaction (PCR) primers with a
cDNA library of human placental tissue as template. 30 cycles (1 min at 94 °C, 1.5 min at 40 °C, and 1.5 min at 72 °C) of PCR were performed under standard conditions in a 100-µl reaction volume
with 200 pmol of each degenerate oligonucleotide primer, DNA from
>106 plaque-forming units of phage, and 2 units of
ampliTaq polymerase (Perkin-Elmer). Amplification products of the
correct size were gel-purified and cloned into the TA cloning vector
(Invitrogen). DNA sequencing was performed on an Applied Biosystems
automated sequencer. TEF-specific probes for screening the placental
cDNA library were generated by PCR using the degenerate primers
described above and the partial hTEF-5 or full-length hTEF-1, hTEF-3,
and hTEF-4 cDNAs as templates in the presence of
[
-32P]dCTP. The cDNA library was screened by
hybridization at 42 °C in 6 × SSC, 50% formamide. Filters
were washed at 55 °C in 3 × SSC. Positive clones were picked
and purified, and the cDNA was excised from
ExLox (Novagen) by
standard procedures. The DNA sequences of both strands of each clone
were determined using internal primers. DNA and protein sequence
analysis were performed using the GCG (Genetics Computer Group,
University of Wisconsin) software package.
The hTEF-5 open reading frame was amplified with appropriately positioned oligonucleotides containing a consensus Kozak sequence replacing the translation initiation isoleucine codon with ATG. The primers contained EcoRI or XhoI restriction sites, and the PCR fragment was cloned between the corresponding sites in pXJ41 (1). The DNA sequence of the expression vector was verified by automated DNA sequencing. The expression vectors for the other human and mouse TEFs were as described previously (28). Human and mouse TEF-3A cDNA clones encoding the alternatively spliced isoforms were PCR-amplified with primers containing EcoRI/XhoI restriction sites as described above and cloned into pXJ41. The hCS-B DF-3 reporter constructs were constructed by PCR using oligonucleotides bearing the appropriate mutations. The resulting fragments were cloned upstream of the thymidine kinase promoter as described previously (43).
Transfections, Preparation of Cell Extracts, and Cloramphenicol Acetyltransferase (CAT) AssaysFor EMSA, COS cells were transfected by the calcium phosphate coprecipitation technique as described previously (26, 28). 48 h after transfection, the cells were harvested (from 60-mm diameter dishes), and extracts prepared by three cycles of freeze-thaw in 100 µl of buffer A (50 mM Tris-HCl, pH 7.9, 20% glycerol, 0.5 mM EDTA, 1 mM phenylmethylsulfonyl fluoride, 0.1% Nonidet P-40, and 1 mM dithiothreitol) containing 0.5 M KCl and 2.5 µg/ml of leupeptin, pepstatin, aprotinin, antipain, and chymostatin as described (28, 49). Generally, between 1 and 5 µl of the extracts were then used in EMSA. For CAT assays, 2 µg of reporter constructs and 1 µg of the Rous sarcoma virus-luciferase vector as an internal standard were introduced into JEG-3 cells by lipofection. 48 h after transfection, cell extracts were prepared and luciferase values were determined. After correction for the luciferase values, CAT assays were performed and quantitated on a Fujix BAS 2000 apparatus as described (50). JEG-3 whole cell extracts were prepared as described previously (46, 47).
Electrophoretic Mobility Shift AssaysThe oligonucleotides
containing the wild-type or mutated GT-IIC enhanson and the tandemly
repeated GT-IIC or Sph enhansons were as described previously (1, 26).
The oligonucleotides were 32P-5-end-labeled using
polynucleotide kinase and separated from unincorporated
[
-32P]ATP by chromatography on G50-Sepharose. The
hCS-A and hCS-B DF-3 and DF-4 fragments were generated by PCR using
32P-5
-end-labeled oligonucleotides 7 and 8 or 2 and 5, respectively, as described (Ref. 43, and see boundaries
(arrows) in Fig. 6B) using the appropriate DNA
templates. EMSAs were performed essentially as described previously (1,
26, 28) on 5% polyacrylamide gels in 0.5 × standard TBE buffer.
Where indicated, 1-2 µg of the monoclonal antibodies were
preincubated with the extracts for 30 min at 25 °C prior to the
addition of the oligonucleotides. Immunodepletions were performed by
incubating 50 µl of the JEG-3 whole cell extract with 3 µg of the
antibodies for 1 h at 4 °C. 50 µl of protein G-Sepharose was
then added to the mixture, and incubation was continued for a further
hour. The extract was then centrifuged, and aliquots of the supernatant
were used for EMSA.
Northern Blot and Reverse Transcription-PCR (RT-PCR)
A
Northern blot containing immobilized total RNA from human tissues
(CLONTECH) was hybridized with a continuously
labeled full-length hTEF-5 probe generated by PCR in the presence of
[-32P]dCTP. Hybridization was performed overnight at
42 °C in buffer containing 6 × SSC and 50% formamide. The
blot was washed with 0.3 × SSC at 50 °C and subjected to
autoradiography. After exposure, the blot was stripped and hybridized
to a probe for cytoskeletal
-actin to verify that each lane
contained RNA. For RT-PCR, total cytoplasmic RNA was isolated from the
human cell lines by lysis with buffer B (50 mM Tris-HCl, pH
7.9, 0.1 M KCl, 0.5 mM EDTA, and 0.2% Nonidet
P-40) and subsequent phenol/chloroform extractions and ethanol
precipitations. To test the integrity of the RNA preparations, RT-PCR
was performed using primers in the hRBP17 subunit common to all three
RNA polymerases, generating a 630-nucleotide fragment (Ref. 51 and data
not shown). Reverse transcription was performed with 2.5 µg of RNA
for 30 min at 40 °C with 5 units of Moloney murine leukemia virus
reverse transcriptase using the following TEF-specific antisense
primers: hTEF-4, 5
-CTTGGACTGGATTTCCCT-3; and hTEF-5,
5
-ACCTGGTACTCCCGCACC-3
. The products of reverse transcription were
then amplified using the same antisense primers and the following sense
primers: hTEF-4, 5
-GGGGGTGACGGGGGCCCG-3
; and hTEF-5,
5
-AACGCCAGCAGCAGCCCC-3
. The 5
and 3
primers were chosen in separate
exons to distinguish the cDNA product from possible contaminating
genomic DNA. RT-PCR generated a 255-nucleotide fragment for hTEF-4 and
a 302-nucleotide fragment for hTEF-5. Control PCR reactions were
performed using 10 pg of the appropriate expression vectors or no DNA
template. 30 cycles of PCR were performed with 1 min at 94 °C, 1.5 min at 53 °C, and 1.5 min at 72 °C in a 60-µl volume. 15 µl
of the reaction was then electrophoresed, transferred to
nitrocellulose, and hybridized to the homologous 32P-5
-end-labeled TEA domain probes generated by PCR using
the degenerate oligonucleotide primers shown in Fig. 1A.
Expression of the TEF-1 TEA Domain and Monoclonal Antibody Production
The region of TEF-1 encoding the TEA domain (amino
acids 28-104) was PCR-amplified with primers containing
BamHI and EcoRI restriction sites, and the PCR
product was cloned into the vector pGEX2T. The plasmid was transformed
into the Escherichia coli DH5 strain, and expression of the
fusion protein was induced by the addition of
isopropyl-1-thio--D-galactopyranoside for 2 h. The
fusion protein was purified by chromatography on glutathione-Sepharose (Pharmacia Biotech Inc.), eluted with reduced glutathione, and analyzed
by SDS-polyacrylamide gel electrophoresis. Immunizations and monoclonal
antibody production were performed as described previously (52-54).
Briefly, mice were injected intraperitoneally three times at 2-week
intervals with the purified GST-TEA fusion protein. Spleen cells were
fused with Sp2/O AG 14 myeloma cells, and culture supernatants at day
10 were tested on COS cells transfected with pXJ40-TEF-1 by
immunofluorescence or by enzyme-linked immunosorbent assay. The
antibodies were also characterized by Western blotting against the
GST-TEA domain fusion protein and the 6-His-tagged TEA domain protein
(28). After generation of ascites fluid, the antibodies were purified
by caprylic acid and ammonium sulfate precipitation as described
previously (52, 53). mAbs 3G3, 22TA, and 2GV3 are as described
previously (52-56).
To isolate TEF factors expressed in human placenta,
degenerate oligonucleotides corresponding to the conserved amino acids GRNELIA and the complement of HIQVL in -helices 2 and 3 of the TEA
domain (see Fig. 1A) were used for PCR
amplification of a human placental cDNA library (see "Materials
and Methods"). PCR products of the expected size were cloned, and
their DNA sequences were determined. All of the TEA domain sequences
analyzed encoded hTEF-5, which contained a TEA domain of identical
amino acid sequence to that of hTEF-1 but with a different codon usage
(Fig. 1A). The partial cDNA was used to isolate a
full-length hTEF-5 cDNA. Full-length hTEF-5 initiates at an ATA
codon and comprises 435 amino acids (Fig. 1B). The TEA
domain is identical to that of hTEF-1 except for a conservative Arg to
Lys change at amino acid 100. Comparison of the sequence of hTEF-5 with
that of the other TEF factors cloned to date showed that hTEF-5 is most
closely related to the B isoform of chicken DTEF-1 (93% homology
compared with 84% for hTEF-1, 83% for hTEF-3, and 79% for hTEF-4;
see also Fig. 2). As previously noted for the other
TEFs, the TEA domain and C-terminal regions are best conserved, while
the N-terminal region and the region following the TEA domain are the
most variable.
To determine whether hTEF-5 was the only TEF expressed in placenta, the
cDNA library was also screened at low stringency with a mixture of
probes for hTEF-1, hTEF-3, and hTEF-5, and 32 clones were analyzed. Of
these, 30 encoded hTEF-5, while two encoded TEF-1. Remarkably, these
two independent clones encoded splice variants of TEF-1, where the
sequence GKTRTRKQ in the TEA domain is followed by an unrelated
sequence comprising VK and a stop codon resulting in a truncated
protein, which cannot bind DNA. In addition to the full-length hTEF-5,
one clone encoding an alternatively spliced isoform of hTEF-5 was
isolated. This isoform contained the sequence GKTRTRKQ of the TEA
domain fused directly to a downstream exon beginning AMNLDQSV. The
protein encoded by this splice variant lacks -helix three of the TEA
domain and consequently does not bind DNA (data not shown). These
results show that hTEF-5 is the only full-length TEF protein encoded in
the placental cDNA library.
The expression pattern of hTEF-5 in adult human tissues
was investigated by Northern blot analysis. Strong expression of a 3.2-kilobase mRNA was detected in placenta and skeletal muscle and
more weakly in heart (Fig. 3A, lanes
3, 6, and 1, respectively). In addition to
the 3.2-kilobase mRNA, an 8.1-kilobase mRNA was detected only
in placenta, while a shorter 1.7-kilobase transcript was detected only
in skeletal muscle.
We next compared the expression patterns of hTEF-5 and hTEF-4, which also has a restricted expression pattern (28), in cultured cell lines. Exon-specific oligonucleotides in hTEF-4 and hTEF-5 were used in an RT-PCR assay (see "Materials and Methods"). As described previously, hTEF-4 transcripts were readily detected in intestine (In) 407 and ovarian OVCAR-3 cells and weakly in 293 and JEG-3 cells (Fig. 3B, lanes 6, 13, 7, and 12, respectively). In contrast, hTEF-5 was expressed only in JEG-3 choriocarcinoma cells (Fig. 3B, lane 12). Together with the results of the Northern blot analysis, this indicates that hTEF-5 is strongly expressed in placenta and placenta-derived cells.
hTEF-5 Binds to TEF-binding Sites in the SV40 Enhancer and in Muscle PromotersThe hTEF-5 coding sequence was inserted into the
pXJ41 (1) eukaryotic expression vector and transfected into COS cells. The transfected cell extracts were then used in EMSAs. Both TEF-1 and
hTEF-5 bound specifically to the GT-IIC enhanson of the SV40 enhancer
(Fig. 4A, lanes 1-4). Both
proteins also bound cooperatively to the tandemly repeated GT-IIC and
Sph enhansons as evidenced by the preferential formation of complex A,
where both enhansons are occupied (Fig. 4A, lanes
5-8).
The relative binding efficiencies of hTEF-5 and the other TEF factors
to sites present in several muscle-specific promoters were
investigated. As described previously, hTEF-1, hTEF-3, hTEF-5, mTEF-3,
and mTEF-4 all bound to the GT-IIC enhanson (Fig. 4B, lanes 2, 6, 7, 3, and
8, respectively). Similarly, binding of an alternatively
spliced isoform of mouse and hTEF-3 lacking the exon after the TEA
domain (TEF-3A; Refs. 31 and 32), was observed (Fig. 4B,
lanes 4 and 5). Using the same amounts of
transfected cell extracts that gave equivalent binding to the GT-IIC
site, similar relative binding efficiencies to the M-CAT1 motif of the cardiac troponin T (cTNT) promoter were observed (Fig.
4B, lanes 17-24; Ref. 11). However, all of these
factors bound with lower affinity to the proximal enhancer core motif
of the rat -myosin heavy chain (MHC) gene promoter (Fig
4B, lanes 9-16; Ref. 37), whose sequence differs
from the consensus (5
-ATG GC-3
; consensus 5
-ATG(C/T)(G/A)-3
). Quantitative PhosphorImager analysis indicated that the binding of hTEF-1 and mTEF-4 to this site was at least 2-3-fold weaker than that of mTEF-3, hTEF-3, and hTEF-5. These results
show that all of the TEF factors bind to the TEF-binding sites in
several muscle-specific promoters, albeit with slightly different
affinities to the
-myosin heavy chain site.
We next examined the binding of hTEF-5 to the enhansons
of the placenta-specific hCS-B enhancer. Radiolabeled probes containing the DF-3 and DF-4 elements (Ref. 43; see Fig.
5B) were generated by PCR and used in EMSA.
hTEF-5 bound specifically to the consensus TEF-binding site in the
wild-type DF-4 (Refs. 42, 43, and 45; see Fig. 5, A and
B) but not to a DF-4 in which this site had been mutated
(Fig. 5A, lanes 1 and 2). This same
mutation inactivates the DF-4 element in JEG-3 cells and
syncytiotrophoblast (46, 47).
A, binding of hTEF-5 to the hCS-B DF-4 and hCS-A and hCS-B DF-3 elements. EMSA was performed with PCR fragments containing the hCS-B DF-4 element (lanes 1 and 2) or the DF-3 element from the hCS-B or A enhancers (lanes 3 and 4). The sequences of the TEF-binding sites in each enhancer are indicated at the bottom of the panel. In lanes 5-8, EMSA was performed with the wild-type or mutated oligonucleotides whose sequences are indicated at the bottom of the panel. The positions of the specific complexes A and B are indicated along with that of the free probe (F). B, the sequence of the human hCS-B enhancer. The boundaries of the DF-3 and DF-4 elements are indicated by arrows. The potential hTEF-5 binding sites I-IV in DF-3 and the binding site in DF-4 are boxed. C, functional analysis of the hCS-B DF-3 hTEF-5 binding sites. The graph shows a quantitative PhosphorImager analysis of CAT assays performed after lipofection of the constructs shown into placental JEG-3 cells. The activity of the wild-type DF-3 element has been taken as 100%. The sequences of the DF-3 hTEF-5 binding sites in each construct are shown below the graph. An alignment of the sequences of the hCS-B and GT-IIC sites is also shown below the graph.
A comparison of the activities of the closely related hCS-A and hCS-B
DF-3 elements has shown that the hCS-A element is inactive in JEG-3
cells and syncytiotrophoblast (46, 47). These DF-3 elements differ by
two nucleotide changes (Fig. 5A). In EMSA, hTEF-5 binds to
the hCS-B DF-3 fragment to generate two complexes, A and B
, which are
not formed on the equivalent fragment from the hCS-A enhancer (Fig.
5A, lanes 3 and 4). This observation suggests that one or both of the nucleotide changes disrupt an hTEF-5
binding site(s). Several potential TEF binding sites have already been
pointed out in this region (Ref. 45; Fig. 5, A and
B, sites III and IV); however, our
inspection of the DF-3 sequence revealed two additional potential
TEF-binding sites containing an ATG core (Fig. 5, A and
B, sites I and II) arranged as a
tandem repeat analogous to the Sph motifs in the SV40 enhancer. One of the base changes in the hCS-A enhancer mutates the ATG core of site II
(Fig. 5A). To investigate the binding of hTEF-5 to these sites, oligonucleotides containing wild-type or mutated versions of
sites I-IV were used in EMSA. The binding of hTEF-5 to the wild-type
oligonucleotide generated two retarded complexes, A and
B (Fig. 5A, lane 5), analogous to
those formed with the Sph enhansons, where complex A, in which both
binding sites are occupied, is preferentially formed. Formation of
these complexes was unaffected by mutation of site III (lane
8), whereas formation of both complexes was abolished by mutations
in site I or II (lanes 6 and 7). These results
show that hTEF-5 binds cooperatively to the tandemly repeated sites I
and II but not to site III or IV (data not shown). These results define
novel tandemly repeated TEF-binding sites within the DF-3 element of
the hCS-B enhancer.
To address the functional importance of these sites, a wild-type DF-3 element or DF-3 elements mutated in sites I, II, and IV were inserted upstream of the thymidine kinase promoter driving expression of the bacterial CAT gene. These reporter constructs were transfected into JEG-3 cells, and the resulting CAT activity was quantified by PhosphorImager analysis. The wild-type DF-3 element strongly stimulated CAT activity compared with the native thymidine kinase promoter (Fig. 5C, bars 1 and 2). The mutations in sites I and II that disrupted hTEF-5 binding resulted in an almost complete loss of DF-3 activity (bars 3 and 4). Mutation of site IV also resulted in a significant loss of activity (bar 5), while simultaneous mutation of sites I and IV completely abolished activity (bar 6). These results indicate that the hTEF-5 binding sites I and II are critical for the activity of the DF-3 element. Although site IV does not bind hTEF-5, the factor(s) that binds to this site cooperates with the TEF-binding sites I and II to generate DF-3 activity.
PPf/CSEF-1 Is Immunologically Related to the TEF FactorsThe above results indicate that hTEF-5 is expressed in placenta and binds to several functional enhansons in the hCS-B enhancer. However, it has previously been reported that the DF-4 TEF-binding site is recognized by the low molecular mass PPf/CSEF-1, which in EMSA generates a complex with a different electrophoretic mobility from that of hTEF-5 (43, 46-48; see Fig. 6A). PPf recognizes the same sequence as hTEF-5, suggesting that this protein is either a TEF isoform or degradation product or an unrelated protein with the same binding specificity. Although it has been reported that CSEF-1/PPf is not related to the TEFs (48), we reasoned that due to its reported low molecular mass it may comprise little more than the TEA domain and the immediately surrounding sequences. To test this possibility, we generated monoclonal antibodies to the TEA domain (mAbs 4G4 and 5F6; see "Materials and Methods") and used these antibodies in EMSA.
Incubation of oligonucleotides comprising the GT-IIC enhanson with JEG-3 whole cell extracts (WCE) generated specific PPf complexes (Fig. 6, A and B, lanes 1 and 2; Ref. 43) of much higher electrophoretic mobility than those observed with extracts of cells transfected with hTEF-5 (Fig. 6A, lane 8). Preincubation of the JEG-3 WCE or transfected COS cell extracts with mAbs 4G4 and 5F6 inhibited binding of hTEF-5 (Fig. 6A, lanes 9 and 10) and the formation of the PPf complexes (Fig. 6A, lanes 4 and 5). In contrast, control mAbs against the TATA-binding protein (mAb 3G3 (52-54)) had no effect on the binding of hTEF-5 or PPf (Fig. 6A, lanes 6 and 7 and lanes 11 and 12). Similarly, the anti-TEA domain antibodies did not inhibit the binding of a fusion protein containing the GAL4 DBD (in this case GAL-VDR(DE) (50)) to oligonucleotides containing a GAL4 binding site (Fig. 6A, lanes 13 and 14), while the GAL-VDR(DE)-DNA complexes were supershifted by the anti-GAL4 DBD mAb 2GV3 (Ref. 56; Fig. 6A, lane 15).
In an alternative assay, the JEG-3 WCE was immunodepleted with mAbs 4G4 and 5F6 or with an mAb directed against human TATA-binding protein-associated factor 20 (mAb 22TA; Ref. 55), and aliquots of the immunodepleted extracts were used in EMSA. Using JEG-3 WCE immunodepleted with mAb 4G4 or 5F6, no PPf complexes were formed (Fig. 6B, lane 5), whereas these complexes were formed in extracts immunodepleted with the control mAb 22TA (Fig. 6B, lane 6). These results demonstrate that the PPf/CSEF-1 protein(s) are immunologically related to the TEA domain.
One explanation for the above results is that PPf is a proteolytic
breakdown product of hTEF-5 or another TEF generated by a protease
present in the JEG-3 WCE. To test this possibility, we incubated the
transfected COS cell extracts either alone or with the JEG-3 WCE for 30 min at 37 °C prior to EMSA. When incubated alone, only minor
proteolytic degradation was observed with the hTEF-5-transfected COS
cell extract, and the resulting faster migrating complex
(B) had an electrophoretic mobility different from that of
the PPf complexes (Fig. 6C, lane 3). In contrast, when incubated with an aliquot of the JEG-3 WCE the amount of complex B
generated by the binding of full-length hTEF-5 was significantly decreased with a concomitant increase in the PPf complexes (Fig. 6C, lanes 1 and 2). Thus, a protease
present in JEG-3 WCE, but not in transfected COS cell extract, degrades
hTEF-5, generating proteolytic fragments that form the PPf
complexes.
We next determined whether the PPf breakdown products were the
predominant TEF species present in JEG-3 cells or whether they were
artefactually formed during the extraction procedure. To answer this
question, extracts from JEG-3 cells transfected with pXJ41 or
pXJ41-hTEF-5 were prepared, not by the WCE procedure, but by the
simpler freeze-thaw protocol, and EMSA was performed. When extracts
were prepared in this way from the hTEF-5-transfected cells, the
predominant specific complex (B) was formed by the binding
of full-length hTEF-5 (Fig. 6D, lanes 2 and
4). Strikingly, this complex was also the predominant
specific complex formed in extracts from mock-transfected cells, while
no PPf complexes were observed (lanes 1 and 3).
Thus, the extracts made using the freeze thaw procedure, either from
JEG-3 or COS cells, do not contain an active form of the protease that
cleaves TEF-5 into the PPf product, although the B product is still
observed. These two proteolytic products are therefore likely to be
generated by distinct proteases. These results further show that the
TEF factors in JEG-3 cells are mainly full-length.
We report here the cloning of hTEF-5, related to the previously described human and murine TEF-1, -3, and -4 factors. Analysis of the amino acid sequence of hTEF-5 shows that, similar to TEF-1 and TEF-3 (1, 28), the protein initiates with a non-ATG codon, in this case ATA. The TEA domain of hTEF-5 contains only one amino acid substitution compared with that of TEF-1, and, as observed with the other TEFs, the C-terminal region is also highly conserved, but the N-terminal region and the region following the TEA domain are more divergent (28).
Comparison of the hTEF-5 amino acid sequence with other cloned TEFs indicated that hTEF-5 is most closely related to the B isoform of chicken DTEF-1 (84% identity). The TEA domain of the DTEF-1 B isoform contains the R100K amino acid substitution found in hTEF-5; however, none of the hTEF-5 clones analyzed contained the R87K and I94L substitutions found in the DTEF-1 A isoform (33). These results show that the vertebrate genome contains at least four highly related TEF genes conserved from chickens to humans.
The expression patterns of hTEF-5 and DTEF-1 may be somewhat different. In chickens, DTEF-1 is most strongly expressed in embryonic cardiac muscle, while very low levels are observed in skeletal muscle (33). On the other hand, in adults, hTEF-5 is expressed at approximately equivalent levels in both of these tissues. DTEF-1 is also expressed at moderate levels in the lung, whereas only trace levels of expression are detected for hTEF-5. Most strikingly, however, the predominant site of hTEF-5 expression is the placenta, a tissue that has no equivalent in chicken.
The expression of several TEFs is enriched in skeletal and cardiac muscle, and a variety of TEF target genes have been described in these tissues. This report together with previous results from our own and other laboratories (13, 17, 31-37, 57) show that all of the TEF factors can bind with similar relative affinities to sites present in the regulatory regions of several target genes. In adult skeletal muscle, TEF-1, TEF-3, and hTEF-5 are all expressed, suggesting that they may play redundant roles. In keeping with this idea, TEF-1 null mice show defects only in cardiogenesis, although this does not exclude the possibility that each TEF factor plays a specific role in skeletal muscle development and that additional functions of TEF-1 would have become evident only at stages subsequent to that at which the TEF-1 null embryos die. Moreover, we proposed (28) that the phenotype of the TEF-1 null mice reflected the fact that TEF-1 was the only TEF expressed in the developing myocardium. Since our present results show that hTEF-5 is expressed in adult cardiac muscle, further in situ hybridizations comparing the expression of TEF-1 and TEF-5 in the developing mouse embryo will be required to determine whether these two genes are coexpressed or are expressed at different stages of cardiogenesis.
A Potential Role for hTEF-5 in Placenta-specific Gene ExpressionThe predominant site of hTEF-5 expression is the placenta. This observation is consistent with the restricted expression of hTEF-5 in JEG-3 cells. We have previously reported that TEF-1, TEF-3, and TEF-4 were also expressed in JEG-3 cells (28); however, our present results suggest that this is not the case in the placenta. Low stringency screening of a placental cDNA library with probes for each TEF resulted in isolation of many independent hTEF-5 clones, two clones encoding truncated splice variants of hTEF-1, but no clones for hTEF-3 or hTEF-4. Although the splice variants of TEF-1 do not bind DNA, we cannot formally rule out the possibility that they perform some other function. Nevertheless, hTEF-5 is the predominant TEF expressed in the placenta.
To relate the placental expression of hTEF-5 to that of potential target genes, we show that hTEF-5 binds to multiple functional sites in the hCS-B enhancer. The DF-4 site, which is identical to the GT-IIC enhanson, binds hTEF-5, and mutations that inhibit hTEF-5 binding inactivate the DF-4 element. Other potential TEF binding sites have been pointed out in the DF-3 element. Several of these (see, for example, EM_6 in Ref. 45) are unlikely to be bona fide TEF-binding sites, since they lack the conserved ATG core sequence. However, two other sites identified in that study (see EM_4, designated sites III and IV in this study) contain an ATG core, but despite this homology, no binding of hTEF-5 (or TEF-1)2 was observed. Nevertheless, adjacent to sites III and IV we identified two other binding sites, organized as a tandem repeat reminiscent of the Sph enhansons, to which hTEF-5 binds cooperatively as shown by the preferential formation of complex A. When either of the two sites was mutated, no binding to the remaining site was observed, showing that individually these are low affinity binding sites and that the integrity of both sites and cooperativity is required for efficient binding to this element. In correlation with these observations, mutations in either of the two sites that disrupt hTEF-5 binding also inactivate the DF-3 element. These results clearly define a novel functional element in the hCS-B enhancer comprising tandemly repeated hTEF-5 binding sites.
In contrast to the hCS-B DF-3 element, the hCS-A DF-3 element is
inactive in placenta-derived cell lines and syncytiotrophoblast (46,
47). This differential activity correlates with hTEF-5 binding, since
the hCS-B DF-3 binds hTEF-5, but the hCS-A DF-3 does not. The lack of
hTEF-5 binding can be ascribed to the fact that one of the mutations in
the hCS-A DF-3 element affects the ATG core sequence of binding site
II. It has been reported that back-mutation of this nucleotide to the
hCS-B sequence (i.e. G A) results in a gain of function
(58). These authors have shown that sequences in this region bind two
unidentified proteins present in JEG-3 extracts. However, in these
experiments the oligonucleotides used did not contain the complete
nucleotide sequences of sites I and II and, consequently, probably do
not bind hTEF-5. Thus, although our results do not exclude the
possibility that other proteins bind to this region, we show that the
placentally expressed hTEF-5 binds cooperatively to tandemly repeated
sites in this region and that this binding correlates with the function
of the DF-3 element.
At first sight, a more direct approach to determine the role of hTEF-5 in hCS enhancer function would be to express hTEF-5 with an appropriate reporter construct in HeLa cells that do not express hTEF-5 and where the hCS enhancer is inactive. However, overexpression of hTEF-5 does not activate transcription from the hCS-B enhancer either in HeLa or in JEG-3 cells.2 These observations may be explained in two ways. First, as previously proposed (44, 58), the hCS enhancer contains negative regulatory sequences, which repress its activity in nonplacental cells; thus, expression of hTEF-5 alone would not be sufficient to activate this enhancer. Second, even in JEG-3 cells, overexpression of hTEF-5 does not further activate, but rather represses, hCS enhancer activity due to a transcriptional interference/squelching effect previously observed with TEF-1 (1, 26). Expression of hTEF-5 in HeLa cells represses the activity of endogenous HeLa cell TEF-1 showing that these two factors compete for a common limiting intermediary factor.2 To unambiguously determine the role of hTEF-5 in placental gene expression, it will be necessary to inactivate this gene in the mouse and analyze the resulting phenotype. Experiments of this type are currently in progress.
In contrast to previous reports (48), we show here that the PPf/CSEF-1 proteins are immunologically related to the TEF factors, since formation of the PPf complexes is inhibited by mAbs against the TEA domain. It is probable that PPf corresponds to a proteolytic breakdown product of hTEF-5, since incubation of hTEF-5 with JEG-3 WCE results in the disappearance of the full-length hTEF-5 and the appearance of PPf complexes. The resulting proteolytic fragment is considerably smaller than the full-length protein, explaining the previously reported differences in chromatographic properties and thermal stability between PPf/CSEF-1 and TEF-1 (48). The lack of cross-reaction with anti-cTEF-3 antibodies may be explained if the corresponding epitope is either not conserved between cTEF-3 and hTEF-5 and/or if the epitope is not present in the proteolytic fragment. Together these results show that the previously described PPf/CSEF-1 factor is in fact a selective proteolytic degradation product of the TEF factors.
Previous studies have highlighted the correlation between hCS-B enhancer activity and the presence of the PPf proteolysis products, raising the possibility that proteolysis of the TEF factors may be important for their function. However, this idea is not supported by the observation that, when an alternative extraction procedure is used, predominantly full-length TEF factors are detected, showing that an artefactual, but selective proteolysis occurs during extract preparation. In conclusion, our results demonstrate that all of the factors described to date that interact with the TEF-binding elements of the hCS-B enhancer belong to the TEF family of transcription factors, further highlighting the potential role of these factors in placental transcription.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) X94439[GenBank].
We thank M. Vigneron, J. Acker, and K. Yamamoto for different materials used in this study; P. Chambon for support; R. Fraser for critical reading of the manuscript; L. Carré for technical assistance; Y. Lutz and the monoclonal antibody facility; J-M. Garnier and T. Lerouge for providing the cDNA library; S. Vicaire and P. Hamman for DNA sequencing; the oligonucleotide facility; the staff of the cell culture facility for providing the cell lines; and B. Boulay, J. M. Lafontaine, R. Buchert, S. Metz, and C. Werlé for figures.