(Received for publication, June 25, 1996, and in revised form, September 13, 1996)
From the Institute for Molecular Biology and Genetics
and the § Department of Microbiology, Seoul National
University, Seoul 151-742, Korea
DnaA protein, the initiator protein for initiation of Escherichia coli chromosomal replication, has been shown to repress its own expression from two dnaA promoters, 1P and 2P. The sequence-specific binding of DnaA protein to the DnaA box, located between the two promoters, results in subsequent oligomerization of DnaA protein. Upon increasing the concentration of DnaA protein, the oligomerization proceeds to both dnaA promoters from the DnaA box and inhibits RNA polymerase binding to both promoters. This results in the repression of transcription, suggesting that the extent of oligomerization of DnaA proteins over two dnaA promoters contributes to the autoregulation of expression of the dnaA gene. When the two dnaA promoters were bound and repressed by DnaA protein, the interaction of RNA polymerase with IciA protein, which is a specific inhibitor of initiation of in vitro E. coli chromosomal replication, appeared to dissociate the oligomerized DnaA proteins from the 1P promoter and allowed RNA polymerase to be loaded for its transcription.
DnaA protein is essential for the initiation of Escherichia coli chromosomal DNA replication in vivo and in vitro (1, 2, 3, 4, 5). The binding of 20-30 molecules of DnaA protein to oriC (origin of chromosomal DNA replication) containing five DnaA boxes (or 9-mers), which are recognized by DnaA protein, forms an initial complex for the initiation of in vitro oriC plasmid DNA replication (4, 6, 7, 8). DnaA protein binds ATP, with a KD of 0.03 µM, and other nucleotides (9). Whereas the ADP- or AMP-bound form of DnaA protein is not active for oriC plasmid DNA replication, the ATP-bound form is active. Phospholipid exchanges ADP in the ADP form of DnaA protein with ATP. Also, ATP stabilizes DnaA protein. DnaA protein appears to exist as monomeric and aggregated forms in E. coli (2). The inactive and aggregated form of DnaA protein containing phospholipid was converted in an ATP-dependent manner to active monomeric forms by phospholipase or DnaK protein (10). The DNase I footprint of oriC bound by the nucleotide-bound form of DnaA protein was distinct from that bound by the nucleotide-free form of DnaA protein (7, 11). While DNase I cleavages in the footprint with the nucleotide-free form were widely distributed in oriC and its adjacent region, those with the nucleotide-bound form were in the regions containing the DnaA box. The localized binding of DnaA protein to the regions containing the DnaA box was similar to the in vivo footprint pattern of oriC (12).
The dnaA gene, encoding DnaA protein, contains two
promoters, 1P and 2P (see Fig. 1). One DnaA box is located between the two promoters. In vivo overproduction of DnaA protein
reduced the transcription from both promoters (13). Transformation of E. coli with a plasmid containing several DnaA boxes
resulted in an increase of dnaA expression due to the
titration out of intracellular DnaA proteins (14). In vitro
transcription of the dnaA gene was inhibited by DnaA protein
(15). These results supported the autoregulation of expression of the
dnaA gene (3, 16, 17). Also, DnaA protein functions as a
transcriptional repressor for the expression of other genes including
rpoH (18), mioC (19), the guaBA operon
(20), and uvrB (21), while the expression of the
nrd gene appeared to be enhanced by DnaA protein (22).
In the presence of a millimolar level of ATP, DnaA protein unwinds the AT-rich region (containing three 13-mers) of oriC for the next step of initiation of oriC replication. IciA protein has been shown to specifically inhibit this early step of in vitro E. coli chromosomal DNA replication (23, 24). The binding of IciA protein to the AT-rich region blocks the opening of the AT-rich region. Also, IciA protein binds to two sites, IciA I and IciA II, in the dnaA promoter region (25). The IciA I site is located upstream of dnaA promoter 1P, and the IciA II site is downstream of dnaA promoter 2P (see Fig. 1). Among the two dnaA promoters, transcription from the 1P promoter was specifically enhanced by in vivo overproduction of IciA protein or by the addition of IciA protein, regardless of the presence of DnaA protein, in the transcription assay of the dnaA gene in vitro.
The molecular mechanism of the DnaA protein-dependent transcriptional repression has not been reported. In this report, we show that the repression is due to the occlusion of RNA polymerase caused by oligomerization of DnaA proteins over two dnaA promoters. The binding of IciA protein to the IciA I site was also addressed to enhance the binding of RNA polymerase to dnaA promoter 1P covered by DnaA protein.
Sources were as follows:
[-32P]ATP and [
-32P]UTP (4000 Ci/mmol), Amersham Corp.; poly(dI)·poly(dC) and Fast Q, Pharmacia
Biotech Inc.; calf intestinal alkaline phosphatase, Boehringer
Mannheim; Long Ranger polyacrylamide, AT Biochem; T4 polynucleotide
kinase, New England Biolabs Inc.; and restriction and cloning enzymes, Promega. Unless otherwise indicated, other reagents were purchased from
Sigma.
Monomeric DnaA protein from MC1061(pDS596) (10), IciA protein from
MC1061(pISC1) (26), and the 70 subunit of RNA polymerase
from BL21(pGEMD) (27) were purified as described previously. RNA
polymerase from E. coli W3110 was purified as described
previously (28), except that Fast Q chromatography replaced Mono Q
chromatography at the final step of purification. RNA polymerase
holoenzyme was reconstituted by mixing the purified RNA polymerase with
a 3.5-fold molar excess of the
70 subunit.
The E. coli
strains W3110 (,
IN[rrnD-rrnE]1) and DH5
(29) were previously described.
E. coli DH5
was used for isolation of plasmid DNAs. The
plasmid DNAs pdnaA/dnaN (30), pBF1509 (31), pISC1 (26), pYS1
(25), and pBluescript SK(+) (Stratagene) were previously described. To
construct plasmid pHJ4, end-filling of the
165-bp1 BglII/BamHI
fragment, which was isolated from plasmid pBF1509, with the Klenow
fragment was followed by insertion into the EcoRV site of
vector pBluescript SK.
To end-label DNA fragments for gel-shift
and footprinting assays, DNA fragments were dephosphorylated with calf
intestinal alkaline phosphatase and radioactively labeled with T4
polynucleotide kinase and [-32P]ATP. Gel-shift assays
were performed as described previously (23) with minor modifications.
18 µl of gel-shift assay buffer (20 mM HEPES/KOH (pH
8.0), 5 mM magnesium acetate, 60 mM KCl, 1 mM EDTA, 4 mM dithiothreitol, 0.5 mg/ml bovine
serum albumin, 10 µM ATP, and 10% glycerol) contained 1 µg of poly(dI)·poly(dC) and 21.5 fmol of the
32P-end-labeled 228-bp XbaI/XhoI
fragment, which was isolated from plasmid pHJ4. The indicated amounts
of proteins were added and incubated for 10 min at 30 °C. Then, the
reactions were loaded onto a 4.5% polyacrylamide gel and subjected to
electrophoresis at 100 V for 2 h in 45 mM Tris borate
(pH 8.3) and 1 mM EDTA. The gel was dried and visualized by
autoradiography. If necessary, the radioactivities in each band were
quantitated using a FUJIX Bio-Imaging Analyzer (BAS1000).
1,10-Phenanthroline-copper(II) (OP·Cu(II)) footprinting was performed as described previously (32) with minor modifications. A gel-shift assay with 21.5 fmol of the 228-bp XbaI/XhoI fragment from plasmid pHJ4, which was 32P-end-labeled at the XhoI restriction site, was performed as described above. After finishing electrophoresis of the gel-shift assay, the gel was immersed in 200 ml of 10 mM Tris-HCl (pH 8.0), followed by the addition of 20 ml of OP·Cu(II) solution (6 mM 1,10-phenanthroline and 1.35 mM CuSO4). The cleavage reaction was initiated by the addition of 20 ml of 174 mM 3-mercaptopropionic acid, followed by incubation for 3 min at room temperature. Then, 20 ml of 28 mM 2,9-dimethyl-1,10-phenanthroline was added to quench the cleavage reaction. The quenched gel was exposed to x-ray film to localize each band. The DNAs in each band were eluted into diffusion buffer (0.5 M ammonium acetate, 10 mM magnesium acetate, 1 mM EDTA, and 0.1% SDS) by incubation for 1 h at 50 °C and recovered by phenol/chloroform extraction and ethanol precipitation. The pellet was resuspended in sequencing gel loading buffer and electrophoresed through 5% Long Ranger polyacrylamide sequencing gel containing 7 M urea. The gel was dried and visualized by autoradiography or by scanning of radioactivities in each lane with a FUJIX Bio-Imaging Analyzer (BAS1000).
DNase I Protection AssayThe standard reaction (25 µl) contained 40 mM HEPES/KOH (pH 7.6), 50 mM potassium chloride, 10 mM magnesium acetate, 0.1 mM ATP, 2.5 µg of bovine serum albumin, 10% glycerol, 20 fmol of the indicated 32P-end-labeled DNA fragments, and the indicated amounts of proteins. After incubation at 32 °C for 10 min, DNase I (5 ng in 1.5 µl of H2O) was added and incubated for 30 s, and the reaction was stopped by the addition of 27 µl of 0.6 M sodium acetate, 0.4% sodium dodecyl sulfate, 25 mM EDTA, and 2.5 µg of yeast tRNA. Proteins were removed by phenol/chloroform extraction. DNA was precipitated by ethanol, followed by a 70% ethanol wash. DNA was subjected to electrophoresis through a 5% Long Ranger polyacrylamide sequencing gel containing 7 M urea. The gel was dried and visualized by autoradiography.
Run-off Transcription AssayRun-off transcription assays were performed as described previously (25).
Sequence-specific DNA binding of DnaA protein to the
dnaA promoter region (Fig. 1) was studied in
detail using a combined gel-shift and chemical footprinting assay to
determine the extent of DNA binding to the region flanking the
consensus DNA-binding site, the DnaA box. The 32P-labeled
228-bp XbaI/XhoI DNA fragment used for in
vitro DNA binding reactions was derived from plasmid pHJ4 and
contains the DnaA box, the dnaA promoter 1P region, and a
truncated region of dnaA promoter 2P (Fig.
2).
At the lowest level of DnaA protein added to the gel-shift assay, one DnaA protein-DNA complex predominated (complex A) (Fig. 2, second lane). Increasing amounts of DnaA protein added to the reactions produced more slowly migrating complexes (B, C, and D), which are presumably formed by binding of increasing numbers of DnaA molecules to the DNA fragment.
To analyze each individual protein-DNA complex in more detail, in
situ footprinting was performed using the OP·Cu(II) complex as a
chemical DNA cleavage agent (32). After electrophoresis of the
protein-DNA complexes, the polyacrylamide gel was treated with
OP·Cu(II). The DNA in each band was isolated and subjected to
electrophoresis through a 5% denaturing sequencing gel, followed by
autoradiography (Fig. 3A) or by scanning the
gel with a FUJIX Bio-Imaging Analyzer (BAS1000) (Fig. 3B).
OP·Cu(II) cleavage of complex A revealed that the protection by DnaA
protein is limited to a region encompassing ~20 bp within the DnaA
box and to a region encroaching upon dnaA promoter 2P (Fig.
3A, lane 2). In complexes B to D, which were
produced at higher amounts of DnaA protein, the protected regions
became more extended from the DnaA box toward the two dnaA
promoter start sites. As the DnaA protein used in this report was
monomeric and the binding reactions were performed in the presence of
ATP (see "Experimental Procedures"), the possibility of binding of
a contaminating aggregated form of DnaA protein can be excluded. These
results suggest that the initial binding of DnaA protein to the DnaA
box promotes cooperative binding of additional monomers extending
ultimately over the two dnaA promoters.
Oligomerized DnaA Protein-DNA Complexes Occlude RNA Polymerase from the dnaA Promoter
DnaA protein has been shown to repress the
transcription of the dnaA gene in vivo (13) and
in vitro (15). However, the mechanism of the repression has
not been addressed. Two possible mechanisms involve either an
inactivation of RNA polymerase-DNA initiation complexes through direct
protein-protein interactions or the inhibition of RNA polymerase
binding to the promoter. The effect of DnaA protein on the stable
binding of RNA polymerase to dnaA promoter 1P was examined
using a gel-shift assay with the 32P-labeled 228-bp
XbaI/XhoI fragment from plasmid pHJ4 (Fig.
4).
RNA polymerase bound stably to the 1P promoter and shifted ~30% of the input DNA (Fig. 4). With increasing amounts of DnaA protein added to the reaction, RNA polymerase binding was inhibited at levels that also inhibited in vitro run-off transcription. These results suggest that competition for promoter binding is responsible for DnaA protein inhibition of transcription.
Small amounts of DnaA protein (38 ng or less) did not significantly inhibit the binding of RNA polymerase to the dnaA promoter, nor did these low levels of DnaA protein inhibit in vitro transcription (Fig. 4). At 19 ng of DnaA protein (Fig. 2), the ratios of free DNA and complex A over the input DNA were 0.54 and 0.38, respectively. At 38 ng of DnaA protein, the ratios of free DNA and complexes A, B, C, and D were 0.20, 0.36, 0.20, 0.19 and 0.05, respectively. At these lower levels of DnaA protein, the major form of DnaA protein is in complexes A and B (Fig. 2), where the binding of DnaA protein was limited to the DnaA box (Fig. 3). The significant inhibition of RNA polymerase binding to the 1P promoter was only apparent at 75 ng or more of DnaA protein, where the formation of DnaA protein-DNA complexes C and D was proportional to the rate of inhibition of RNA polymerase binding (Fig. 4). These observations indicate that the inhibition of binding of RNA polymerase to the dnaA promoters is dependent upon the oligomerization of DnaA protein to regions flanking the DnaA box and that the binding of one or two DnaA monomers to the DnaA box is not sufficient for occlusion of RNA polymerase from the dnaA promoters.
The inhibition of the binding of RNA polymerase to dnaA
promoters 1P and 2P was also confirmed using a DNase I protection assay
(Fig. 5). The region bound by RNA polymerase alone was
localized within promoters 1P and 2P. As the amounts of DnaA protein
increased, the protection of both promoters from DNase I cleavage by
RNA polymerase was reduced dramatically, and the DNase I footprinting pattern of the two promoters became similar to that for protection by
DnaA protein alone. The less efficient binding of RNA polymerase to the
dnaA promoter in gel-shift assays compared with the binding in DNase I protection assays was caused by the presence of
poly(dI)·poly(dC) in the gel-shift assays. The amount of
poly(dI)·poly(dC) used abolished the nonspecific binding of RNA
polymerase to DNA fragments, but did not significantly affect the
binding of DnaA protein to the DNA fragments containing the DnaA
box.
IciA Protein Counteracts the Repression of DnaA Protein by Stabilizing RNA Polymerase DNA Binding to dnaA Promoter 1P
IciA protein binds to two sites in the dnaA promoter region, which are located upstream of dnaA promoter 1P (IciA I) and downstream of dnaA promoter 2P (IciA II) (Fig. 1) (25). Between the two dnaA promoters, transcription from the 1P promoter was specifically activated by IciA protein in vivo and in vitro. The binding of two dimers of IciA protein to the IciA I site is responsible for the activation of dnaA promoter 1P.2 When the two dnaA promoters were repressed by DnaA protein, IciA protein was able to restore transcription from the 1P promoter with little effect on transcription from the 2P promoter (25). The mechanism of IciA protein stimulation of transcription from dnaA promoter 1P in the presence of inhibitory amounts of DnaA protein was examined.
Using a gel-shift assay (Fig. 6A), RNA
polymerase-DNA binding activity (lane 2) was inhibited by
the addition of DnaA protein (lane 3). However, the binding
of RNA polymerase to the DNA fragment in the presence of DnaA protein
was restored by the addition of IciA protein (lanes
4-6).
Similar results were also observed using DNase I footprinting (Fig.
7). RNA polymerase binding to the region containing
dnaA promoter 1P (lane 3) was inhibited by DnaA
protein (lane 4). Under these conditions, IciA protein
restored RNA polymerase binding to dnaA promoter 1P
(lanes 5 and 6). As all three proteins were present in the same reaction and as the promoter binding of both IciA
protein and DnaA protein remained the same in the absence or presence
of each other (lanes 2 and 7), these results
suggest that IciA protein may establish protein-protein contacts with RNA polymerase that are dominant over the occlusion and inhibition promoted by DnaA protein.
Physically and functionally heterogeneous complexes containing DnaA protein bound to the dnaA promoter were isolated and analyzed in order to address the mode of binding of DnaA protein to DNA containing a single DnaA box and how this binding inhibits transcription by RNA polymerase. First, by recognition of its consensus sequence, a DnaA protein monomer specifically binds to the DnaA box. Second, either through the intrinsic aggregation property of DnaA protein (2, 10) or by random and nonspecific nucleation to DNA surrounding the first DnaA protein, cooperative binding of DnaA protein monomers surrounds the DnaA Box and extends to regions containing promoters 1P and 2P (Fig. 3). Although we did not accurately define the number of DnaA protein molecules present at the dnaA promoter, a monomer is the minimal stable active unit for sequence-specific binding to a DnaA box (33). The formation of up to four major protein-DNA complexes at 150 ng of DnaA protein (Fig. 2) suggests that four monomers bind. This number of DnaA proteins per one DnaA box is within the range of 20-30 molecules of DnaA protein bound to the oriC region containing five DnaA boxes, the number that was deduced from the electron microscopic structure of the initial complex (7, 31, 34).
Previous genetic studies have suggested that RNA polymerase and DnaA protein may form direct complexes (35, 36), although biochemical evidence for this does not exist. We investigated whether DnaA protein and RNA polymerase can coexist at the dnaA promoter by gel-shift and footprinting analyses and whether a direct protein-protein interaction between DnaA protein and RNA polymerase is the mechanism of inhibition of transcription. Our results indicate that the repression of transcription from the two dnaA promoters (1P and 2P) by DnaA protein is promoted by the oligomerization of DnaA protein over dnaA promoters 1P and 2P and that this binding directly prevents RNA polymerase binding to the two promoters. The extent of oligomerization of DnaA protein at its own promoter, which depends upon the concentration of DnaA protein, could determine the rate of binding of RNA polymerase to the dnaA promoters and transcription of the dnaA gene.
IciA protein is a dimer of a single polypeptide (26). The binding of
two dimers of IciA protein to the IciA I site, which is located 50 to
63 nucleotides from the transcription start site of dnaA
promoter 1P, is required to stimulate RNA polymerase binding to the 1P
promoter.2 IciA protein may directly interact with the
-subunit of RNA polymerase to stimulate transcription. The presumed
interaction enhances the capability of RNA polymerase to be loaded onto
the 1P promoter, resulting in the activation of transcription from dnaA promoter 1P. Other transcriptional activators including
CRP (cAMP receptor protein), OxyR, Ada, and OmpR, which bind to the
40 to
60 region from the transcription start site, have been shown
to interact with the
-subunit of RNA polymerase to enhance the
binding of RNA polymerase to the corresponding promoters (reviewed in
Ref. 37). Our previous experiments have shown that when both dnaA promoters 1P and 2P were repressed by DnaA protein,
IciA protein specifically activated transcription from dnaA
promoter 1P, while dnaA promoter 2P was still repressed
(25). Analysis of the IciA and DnaA protein promoter-binding sites was
combined to determine the mechanism of this activation, and it was
found that the interaction of RNA polymerase with IciA protein is
sufficient to dissociate oligomerized DnaA proteins from the 1P
promoter for the activation of transcription. Once RNA polymerase is
bound to the 1P promoter, the oligomerized DnaA proteins over the 2P promoter do not block the movement of RNA polymerase for transcription from the 1P promoter, while the oligomerized DnaA proteins inhibit the
binding of RNA polymerase to the 2P promoter.
We thank Dr. Theodore R. Hupp for critical reading of the manuscript and Dr. Akira Ishihama for the gift of plasmid pGEMD.