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J. Biol. Chem., Vol. 275, Issue 49, 38160-38169, December 8, 2000
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From the
Received for publication, July 6, 2000, and in revised form, August 21, 2000
The archaeal transcriptional initiation machinery
closely resembles core elements of the eukaryal polymerase II system.
However, apart from the established basal archaeal transcription
system, little is known about the modulation of gene expression in
archaea. At present, no obvious eukaryal-like transcriptional
regulators have been identified in archaea. Instead, we have previously
isolated an archaeal gene, the Pyrococcus furiosus lrpA,
that potentially encodes a bacterial-like transcriptional regulator. In
the present study, we have for the first time addressed the actual
involvement of an archaeal Lrp homologue in transcription modulation.
For that purpose, we have produced LrpA in Escherichia
coli. In a cell-free P. furiosus transcription system
we used wild-type and mutated lrpA promoter fragments to
demonstrate that the purified LrpA negatively regulates its own
transcription. In addition, gel retardation analyses revealed a single
protein-DNA complex, in which LrpA appeared to be present in (at least)
a tetrameric conformation. The location of the LrpA binding site was
further identified by DNaseI and hydroxyl radical footprinting,
indicating that LrpA binds to a 46-base pair sequence that overlaps the
transcriptional start site of its own promoter. The molecular basis of
the transcription inhibition by LrpA is discussed.
Recent studies have revealed that the archaeal transcriptional
machinery represents a simplified version of the eukaryal RNA polymerase II transcription apparatus, which involves homologues of the
TATA-binding protein (TBP),1
the transcription factor IIB (TFIIB; the archaeal homologue is called
TFB), and the multi-subunit RNA polymerase II (for a recent review, see
Ref. 1). The initiation process starts when the TBP interacts
specifically with the core promoter element, the TATA box, which is
located at positions Analysis of the available archaeal genomic sequences shows that the
majority of the identified homologues of regulators are bacterial-like
(12). Recently a mechanism by which a bacterial-like regulator affects
the archaeal transcriptional machinery was described. It was shown that
MDR1 from Archaeoglobus fulgidus, a homologue of the
iron-dependent bacterial repressor DxtR, represses
transcription by binding to its own promoter in a
metal-dependent manner. Upon binding of MDR1 to the
promoter, RNA polymerase recruitment is prevented but not binding of
TBP or TFB (13).
One particular group of bacterial-like regulators present in all
available archaeal genomes is the family of Lrp/AsnC regulators. Members of this family have been identified in more than a dozen different bacterial species, in which they generally appear to be
involved in regulation of amino acid metabolism. The most extensively studied example is the leucine-responsive regulatory protein (Lrp) from
Escherichia coli (14, 15). Lrp is a global regulator that
controls the expression of approximately 75 genes, many of which are
involved in transport, degradation, or biosynthesis of amino acids. Lrp
can either activate or repress transcription, and this action can be
modulated by the effector leucine, which either decreases or increases
its particular action. In some cases, like the negative autoregulation,
leucine has no effect at all. The paralogous E. coli AsnC
appears to be a specific transcriptional activator of asparagine
synthetase A. Activation is reduced in the presence of the effector
asparagine, but again, the negative autoregulation of AsnC itself is
not affected by asparagine (16, 17). Two Lrp/AsnC homologues from
Sulfolobus solfataricus have been studied in more detail.
One of these was cloned, sequenced, and shown to be expressed during
growth on complex medium (18). The other Lrp/AsnC homologue, called
Lrs14, was studied in more detail (19). It was shown that the purified
recombinant protein binds to its promoter at a region overlapping the
TATA box. In addition, it was shown that the lrs14
transcript accumulates in the late growth stages of S. solfataricus.
In the genome sequence of Pyrococcus furiosus (Center of
Marine Biotechnology, University of Utah) at least 10 homologues of genes encoding Lrp/AsnC-like proteins can be
identified.2 The
lrpA gene, encoding one of these homologues, was previously identified downstream of the gdh gene that encodes glutamate
dehydrogenase (20, 21). In this paper, we describe the cloning,
functional expression, and characterization of LrpA and show that LrpA
binds to its own promoter and specifically inhibits in vitro
transcription from this promoter. Using the combined data of gel
mobility shift assays, in vitro transcription analyses, and
footprinting, we identified the sequence elements responsible for LrpA
binding and propose a mechanism by which LrpA binds its promoter.
DNA Sequence Analysis--
Identification of LrpA homologues was
done using the Advanced BLAST program at NCBI. Alignments were made
using the program ClustalX. Motif searches were performed using the
PROSITE Pattern and Profile Searches program at the ExPaSy Molecular
Biology Server and the program HELIX-TURN-HELIX (32). Inverted repeats
were identified using the GeneQuest program, which is part of the DNA Star package.
Plasmid and Strain Construction--
The gene encoding
lrpA was PCR-amplified using primers BG240 and BG241 (see
Table I, italic and underlined sequences
indicate the restriction sites BspHI and BamHI,
respectively). The resulting 444-bp PCR fragment was cloned into pGEM-T
(Promega Corp.), resulting in pLUW600, and the sequence of the insert
was verified by DNA sequencing. Subsequently, pLUW600 was digested with
BspHI and BamHI, and the resulting 428-bp
fragment was cloned into the T7 expression vectors pGEF+ (22), pET9d,
and pET24d (23) (Novagen, Inc.), resulting in the constructs pLUW601,
pLUW604, and pLUW605, respectively. These constructs were transformed
into E. coli BL21(DE3), BL21(DE3) (pLysS), and BL21(DE3)
(pLysE) (Novagen, Inc.) and tested for expression (not shown). The
optimal result was obtained with E. coli BL21(DE3) in
combination with the pET9d-derivative pLUW604. This combination was
used for further expression experiments. pLUW613 was made by cloning
fragment A into pGEM-T (Promega, Corp.). Mutations in fragment A were
introduced using Pfu polymerase in the PCR-based overlap
extension method (24). For each mutation a sense/antisense primer pair
was designed. BG730 and BG731 introduced mutation 621; BG759 and BG760
introduced mutation 623; BG792 and BG793 introduced mutation 629; BG794
and BG795 introduced mutation 630 (see Table I). BG289 and BG290 were
used as flanking primers for the PCR of fragment A (see below). All
mutant fragments A were cloned into pGEM-T (Promega) and sequenced,
resulting in pLUW621, pLUW623, pLUW629, and pLUW630.
Overproduction of LrpA--
The P. furiosus LrpA
protein was produced in 2-liter Erlenmeyer flasks containing 1 liter of
LB medium with 50 µg/ml kanamycin. The culture was inoculated with
E. coli BL21(DE3) containing pLUW604. Cells were grown in a
rotary shaker at 37 °C until an A600 of 0.5 was reached, and 0.4 mM
isopropyl-1-thio- Gel Mobility Shift Experiments--
DNA probes used for gel
mobility shift experiments were generated using PCR. The following
primers were used: BG289 and BG290 for fragment A; BG367 and BG290 for
fragment B; BG289 and BG431 for fragment C; BG430 and BG290 for
fragment D; BG638 and BG498 for fragment E; BG638 and BG615 for
fragment F; BG427 and BG109 for fragment G (see Table I). PCR reactions
consisted of a 5-min denaturation step at 95 °C, 30 cycles
consisting of 95, 45, and 72 °C, with 30 s for each step,
followed by a 7-min final extension step at 72 °C. PCR products were
end-labeled using T4 kinase and radioactive [ DNaseI and Hydroxyl Radical Footprinting--
DNaseI and
hydroxyl radical footprinting was performed using non-radioactive
probes containing the IRD800 label in combination with a Li-Cor
sequencer (Li-Cor, Inc.). For this purpose DNA probes were prepared as
follows. Fragments B and G (see Fig. 1B) were cloned into
pGEM-T (Promega), and clones were selected containing the insert in
both orientations. These constructs were used as a template in PCR
reactions with a IRD800-labeled T7 primer (MWG-Biotech, GmbH) in
combination with BG290, BG367, BG427, or BG109. These PCR reactions
produced fragments B or G carrying the IRD800 label on a 68-bp
extension originating from pGEM-T at the 5' end of either the
non-template or the template strand. 10 ng of this DNA was used per
reaction. Binding reactions for DNaseI and hydroxyl radical
footprinting were identical to the binding reaction conditions in gel
mobility shift experiments (see above) except that glycerol and
poly(dI·dC)·poly(dI·dC) were omitted. DNaseI cleavage was done by
adding 20 µl of a solution containing 5 mM
CaCl2, 10 mM MgCl2, and 2 milliunits of DNaseI. After 1 min the DNaseI reaction was stopped by
the addition of 20 µl of 4 M ammonium acetate and 30 mM EDTA. The DNA was extracted with 60 µl of phenol,
precipitated with 96% ethanol in the presence of 20 µg of glycogen,
and washed with 70% ethanol. The pellet was dissolved in 1 µl of
formamide loading buffer, heated at 95 °C for 5 min, and chilled on
ice. Subsequently, 0.8 µl was analyzed on a Li-Cor 4000 sequencer
using a 5.5% KBPlus 41-cm denaturing sequence gel (Li-Cor)
with 0.2-mm spacers and settings 2000 V, 25 mA, 50 watt, and
45 °C.
Hydroxyl radicals were generated by adding 3 µl of 40 mM
sodium ascorbate, 3 µl of 1.2% H2O2, and 3 µl of 4 mM
(NH4)2Fe(SO4)2·6H2O, 8 mM EDTA. After 2 min the reaction was stopped by the
addition of 26 µl of 0.1 M thiourea, 20 mM
EDTA. DNA was extracted with phenol, precipitated as described above,
and analyzed on a Li-Cor 4000L sequencer (Li-Cor) using a 66-cm
denaturing sequencing gel with 0.25-mm spacers and settings 2250 V,
30.6 mA, 68 watt, and 45 °C. Images of the footprints were analyzed
using the program Scion Image for Windows, available from the National
Institutes of Health.
In Vitro Transcription--
Transcription reactions were
performed essentially as described previously (26) except that 300 mM KCl was used instead of 250 mM. A standard
reaction mixture (50 µl) contained 1 µg of linearized template DNA
(pLUW479 (26), pLUW613, pLUW621, pLUW623, pLUW629, pLUW629, or piC31/2
(27)), 250 ng of recombinant TBP, 280 ng of recombinant TFB, 135 ng of
native RNA polymerase, and varying concentrations of LrpA. This
reaction mixture was incubated for 30 min at 70 °C. RNA purification
and electrophoresis was performed as described previously (28).
Primer Extension--
For analysis of the in vitro
transcriptional start site, cell-free transcription reactions were
performed as described above but with unlabeled precursors. In a
control reaction, nucleotides were omitted from cell-free transcription
reactions. The end-labeled DNA primer 5'-GTATAATTTTGTCTCTCTCATCA-3' was
used complementary to nucleotides +20 to +42 relative to the
transcriptional start of lrpA. The primer extension assay
was performed as described previously (26, 28). For
determination of the in vivo transcriptional start site,
primer extension was performed with total RNA of P. furiosus, which was isolated as described previously (29).
Chemical Cross-linking and Western Blot Analysis--
Chemical
cross-linking was performed as described by Davies and Stark (30), with
the following modifications. For cross-linking experiments with free
LrpA, different concentrations of LrpA were diluted in cross-linking
buffer (80 mM triethanolamine-HCl, pH 8.0, 100 mM NaCl, 1 mM EDTA, 0.1 mM
dithiothreitol), and the final volume was adjusted to 16 µl.
Dimethylsuberimidate (DMSI, 25 mg/ml freshly made in cross-linking
buffer) was added to a final concentration of 5 mg/ml so that the final
volume was 20 µl. After a 1-h incubation at room temperature,
SDS-PAGE loading buffer (25) was added, and 100 ng of each sample was
separated on a 10% Tricine SDS-PAGE gel (31). The separated proteins
were transferred to a nitrocellulose membrane by electroblotting in 10 mM CAPS, pH 11.0, and 10% methanol and detected
immunologically using a polyclonal antiserum raised against purified
LrpA (25). For cross-linking experiments with LrpA-DNA complexes, about
2 µg of purified LrpA was incubated with 500 ng of DNA (fragment B,
see Fig. 1B) in cross-linking buffer in a final volume of 64 µl. DMSI was added as described above so that the final volume was 80 µl. The samples were loaded on a non-denaturing 5% acrylamide gel,
buffered in 1× Tris borate EDTA buffer (25). The gel was stained with
ethidium bromide, bands representing specific DNA-LrpA complexes were
excised and crushed, and SDS-PAGE loading buffer was added. The
recovered samples were heated for 10 min at 100 °C and loaded on a
10% Tricine SDS-PAGE gel and analyzed as described above.
LrpA Sequence Analysis--
A 2.7-kilobase HindIII
fragment including the gene encoding glutamate dehydrogenase
(gdh) was previously isolated from a genomic library of
P. furiosus (Fig.
1B) (20). Downstream of the
gdh gene, an open reading frame was found with a high degree
of similarity to bacterial transcription regulators of the Lrp/AsnC
family (21). Sequence analysis of the lrpA gene identified a
frame-shift in the previously published sequence (GenBankTM
accession number P42180), which introduced a stop codon after lysine
120 in the predicted protein sequence. The corrected P. furiosus
lrpA gene is predicted to encode a 141-amino acid protein with a
predicted molecular mass of 15.9 kDa. Subsequent BLAST analysis
revealed that LrpA shares a high degree of similarity with many
(hypothetical) regulatory proteins from a number of archaea including
Pyrococcus horikoshii (93% identity), Pyrococcus abyssi (98% identity), Methanococcus jannaschii (54%
identity), A. fulgidus (49% identity), M. thermoautotrophicum (37% identity), and S. solfataricus (32% identity, Fig.
2). In addition, all of these archaea
contain a number of more distantly related homologues, e.g.
in P. horikoshii a total of 9 genes appear to encode LrpA homologues, whereas P. furiosus itself contains at least 10 LrpA homologues. The best characterized LrpA homologues are from
bacterial origin, in particular E. coli AsnC (33% identity)
and E. coli Lrp (28% identity). A PROSITE pattern search
with P. furiosus LrpA identified a putative helix-turn-helix
motif of the Lrp/AsnC family (Fig. 2). This motif was also predicted by
the program HELIX-TURN-HELIX (32).
Overexpression and Purification of LrpA--
Using a PCR approach
we cloned the lrpA gene into a pET9d vector, resulting in
pLUW604. Production of LrpA was achieved after transformation of
pLUW604 to E. coli BL21( Analysis of the lrpA Promoter--
We used primer extension
analysis to map the transcriptional start site for lrpA.
Using in vitro generated run-off transcript RNA (see below),
we found that the transcriptional start was located at an adenosine
located 14 bp upstream the translational start (see Fig.
1A). We compared the lrpA promoter sequence to
other known promoter sequences from P. furiosus. Although
only 14 Pyrococcus promoters have been mapped to date, a
clear consensus sequence can be derived for the Pyrococcus
BRE and TATA elements: AAAnnTTTWWWWW (
We used total isolated RNA from P. furiosus grown on
cellobiose, pyruvate, and tryptone to determine the transcriptional
start in vivo. In all cases the transcriptional start was
identical to that found with in vitro generated RNA (not
shown); however, relatively weak signals were obtained. Although the
results showed that lrpA is expressed during growth on the
above-mentioned substrates, they indicate that lrpA
transcript levels are not very abundant under these conditions.
In Vitro Transcription of lrpA and gdh in the Presence of
LrpA--
Several bacterial members of the Lrp/AsnC family are
negatively autoregulated (16, 33, 34). Hence, it was anticipated that
P. furiosus LrpA could also be a repressor of its own
expression. In the previously established cell-free transcription
system (26), the P. furiosus purified transcription factors
TBP, TFB, and RNA polymerase direct efficient transcription from a DNA
template containing the (partial) gdh-encoding sequence and
its promoter. We used this in vitro transcription system to
study the effect of LrpA on lrpA and gdh
transcription (Fig. 5). The template used in this experiment is PstI-linearized pLUW613, which carried
fragment A (Fig. 1B). Transcription from this template
results in a 160-nucleotide lrpA run-off transcript. With
increasing amounts of LrpA present in the reactions, the signal of the
radiolabeled lrpA PstI run-off transcripts drastically
decreased (Fig. 5A). This indicated that LrpA had a negative
effect on its own transcription in vitro. A similar
experiment was performed using BamHI-digested pLUW479 as the
DNA template (26). This plasmid carried the partial P. furiosus
gdh gene including its 200-bp upstream sequence. Transcription from this template resulted in a 173-nucleotide gdh run-off
transcript. There was no effect on gdh transcription when
LrpA was added (Fig. 5B). Likewise, transcription from the
Methanococcus vannielii tRNAVal promoter (26)
was not inhibited by LrpA (Fig. 5B).
LrpA Binds Specifically to Its Own Promoter--
To test whether
LrpA binds to its own promoter, we performed gel mobility shift
experiments with purified LrpA and DNA fragments containing the LrpA
promoter sequence. Three different DNA fragments (C, D, and E) were
used that contained sequences upstream of lrpA (Fig.
1B). Fragment C contained the upstream lrpA
promoter region including the TATA element (Fig. 1B). LrpA
did not shift this fragment, indicating that no interaction occurred
between LrpA and the upstream promoter region (Fig.
6). Fragment D contained the TATA
element, the transcriptional start site, and the sequence downstream
thereof (Fig. 1B). The addition of LrpA to this fragment resulted in a shifted band (Fig. 6). Using LrpA concentrations of up to
810 nM (as calculated for an LrpA monomer), we observed only one shifted band in gel mobility shift experiments, indicating that only one complex is formed when LrpA binds to the lrpA
promoter. This binding was specific, since the addition of 2 µg of
poly(dI·dC)·poly(dI·dC) as nonspecific competitor DNA did not
prevent LrpA-DNA binding.
As mentioned above, we observed dimer, tetramer, and octamer
configurations of LrpA in gel filtration chromatography experiments. We
tested fractions of all these different forms in gel mobility shift
experiments; however, there was no obvious difference in DNA binding
activity between the fractions (not shown).
To determine the affinity of LrpA for its promoter DNA, we performed a
gel mobility shift experiment with fragment D and increasing LrpA
concentrations (not shown). The concentration of LrpA, as calculated
for an LrpA monomer, that caused half of the DNA to become complexed
under the experimental conditions used was taken as the dissociation
constant (Kd) of the LrpA-DNA complex (35). We
determined a Kd of 0.3 nM, which is
about 4-10-fold lower compared with values measured for E. coli Lrp (36, 37) and several orders of magnitude lower than that
of S. solfataricus Lrs14 (19).
We tested several smaller fragments to locate the boundaries of the
LrpA binding sequence more precisely. Fragment E (43 bp) was the
smallest fragment to which LrpA bound efficiently (Figs. 6 and
7C). LrpA also bound to
fragments smaller than 43 bp, such as fragment F (30 bp), but the
affinity for these fragments was drastically decreased (Fig. 6 and
7C). LrpA binding to fragment E was specific, since the
addition of increasing amounts of unlabeled fragment E prevented LrpA
binding to labeled fragment D (not shown). Altogether, these results
indicated that LrpA bound specifically to its own promoter at a
position around the transcriptional start site. Since P. furiosus grows optimally at 100 °C we performed binding
reactions for gel mobility experiments at several temperatures. Binding
experiments performed at 0, 4, 25, 50, and 80 °C resulted in
identical gel mobility shift patterns (not shown).
Gel mobility shift experiments were also performed with DNA fragments
containing gdh promoter sequences. Under similar conditions as the experiments with the lrpA promoter fragments, we
observed very weak LrpA binding with fragment G (not shown). This
fragment contained 386 bp of the gdh promoter, including the
TATA element (Fig. 1B). However, this binding appeared
to be rather weak and nonspecific since the observed shift
disappeared upon the addition of poly(dI·dC)·poly(dI·dC). This
indicates that, under the tested conditions, LrpA binds specifically to
its own promoter but not to the gdh promoter. With promoter
fragments of both lrpA and gdh, several compounds
were tested for their ability to act as an effector for LrpA. Among
those tested were L-leucine, L-alanine, L-glutamate, DNaseI and Hydroxyl Radical Footprinting--
To study LrpA
binding at its own promoter in more detail, we performed DNaseI
footprinting with purified LrpA and fragment B containing the
lrpA promoter (Fig. 1B). The addition of LrpA resulted in DNaseI protection at a region of
To further characterize the LrpA binding site(s) at its own promoter,
hydroxyl radical footprinting was performed with the lrpA
promoter fragment B (Fig. 1B). Using this technique
information can be obtained about the interactions between LrpA and the
DNA sugar-phosphate backbone. The plot profiles of the relative band intensities from these experiments revealed the presence of four regions with decreased band intensities in both the non-template and
the template strand (Fig. 7B). These regions are all located between positions Mutational Analysis of the LrpA Binding Sequence--
Because most
of the protection against DNaseI cleavage occurred within the
We used different approaches to design mutations. In the first approach
we mutated four of the eight bp of the palindromic sequence ACCTAGGT
present within the
In the second approach we compared putative lrpA promoter
sequences of P. horikoshii (41) and P. abyssi
with that of P. furiosus. All these Pyrococcus
species have a similar organization of gdh and
lrpA genes, and putative promoter sequences of
lrpA share a high degree of homology. In Fig. 8A,
the bases that are conserved among the three Pyrococcus
species are indicated with a gray background. Upstream from
the TATA boxes there is little conservation, whereas a higher degree of
conservation is present around the TATA elements and the sequence
downstream thereof. We mutated two conserved sequence blocks present
within the
Finally, we focused on the right half of the substituted bases in
promoter mutant 629, since bases at the left half did not cause a
drastic effect on LrpA binding (mutant 621). Therefore, we constructed
promoter mutant 630, in which GGTTC is substituted by TTGGA (Fig.
8A). This substitution caused the same effect as in mutant
629. LrpA did not bind the mutant promoter DNA, and in agreement with
this, transcription inhibition by LrpA was decreased to 44% compared
with wild-type DNA (Fig. 8B). The observation that there was
still an effect in in vitro transcription, although there
was no detectable binding to mutant fragments 629 and 630, can be
explained by the fact that nonspecific competitor DNA was only added in
gel mobility shift experiments. In the absence of competitor DNA, very
weak LrpA binding still occurred (not shown).
Chemical Cross-linking--
Results from gel filtration
chromatography suggested that LrpA existed as a dimer, tetramer, and
octamer in solution. To further characterize the configuration of LrpA
as a free protein or in complex with lrpA promoter DNA, we
performed chemical cross-linking experiments. DMSI was used as a
cross-linking agent that acts by forming covalent amide linkages
between lysine residues. This results in cross-links primarily between
the subunits of oligomeric proteins (30). Cross-linked LrpA was
analyzed by SDS-PAGE, followed by Western blotting using an antiserum
raised against purified LrpA. First, cross-linking experiments were
performed with LrpA as a free protein in solution. For that purpose,
LrpA was incubated with DMSI, and cross-linking was analyzed using
SDS-PAGE. DMSI caused the appearance of three bands in addition to the
LrpA monomer (I, Fig. 9)
corresponding to molecular masses of an LrpA dimer (II), trimer (III)
and tetramer (IV). Although the band corresponding with the dimer form
(II) appears to be the predominant species, a band corresponding with
the tetrameric form (IV) is present as well. Although the results from
gel filtration chromatography showed that LrpA also exists as an
octamer in solution, this configuration was not observed in
cross-linking experiments. We tested several concentrations of LrpA
(200 nM to 40 µM) under identical
cross-linking conditions but did not observe an obvious change in the
intensities of the individual bands (not shown). This suggests that the
degree of multimerization of LrpA is not
concentration-dependent under the tested conditions.
We also performed cross-linking experiments with LrpA bound to its
target DNA. LrpA was incubated with lrpA promoter DNA, DMSI
was added, and the samples were separated on a non-denaturing acrylamide gel. Subsequently the bands representing specific LrpA-DNA complexes were excised and analyzed by SDS-PAGE. The pattern of cross-linked LrpA in complex with DNA was almost similar to that of
free LrpA (Fig. 9). In both cases bands with molecular masses corresponding to the dimer, trimer and tetramer or LrpA were present in
addition to the monomer. However, in cross-linked LrpA that is
complexed with DNA the tetrameric form appeared to be the more dominant
species. Therefore, these results suggest that at least four LrpA
monomers are in complex with the lrpA promoter fragment.
The present study describes the characterization of the LrpA
transcriptional regulator from the hyperthermophilic archaeon P. furiosus. Comparison of the amino acid sequence of LrpA reveals that it belongs to the Lrp/AsnC family of transcriptional regulators, which consists of many bacterial proteins as well as a growing number
of putative archaeal proteins (Fig. 2). Although gel filtration experiments showed that the purified recombinant LrpA exists as a
mixture of dimer, tetramer, and octamer in solution, chemical cross-linking experiments suggest that the tetrameric form of the
protein was the highest quaternary structure, both in solution and in
complex with DNA (Fig. 9). In comparison, E. coli Lrp exists as a dimer, both in solution and in complex with a single binding site.
Pseudomonas putida BkdR exists as a tetramer in solution, and three tetramers are proposed to bind to its target DNA
(42-45).
In vitro analyses revealed that P. furiosus LrpA
binds to its own promoter and represses its transcription. We tested
potential effectors for their ability to alter the effect of LrpA on
lrpA transcription; however, both in vitro
transcription analyses and gel mobility shift assays revealed that
these compounds had no effect on the LrpA autoregulation efficiency.
Negative autoregulation is a common characteristic within the Lrp/AsnC
family of regulatory proteins, and in general this repression is
independent of effectors (16, 34, 46).
It has been reported that the RNA polymerase of the archaeon
Methanococcus thermolithotrophicus protects a region of In analogy with E. coli Lrp, it is tempting to speculate
that the archaeal homologues may also act as global regulators (18) and
thereby act both as transcriptional repressors and activators. Activation of transcription would probably require binding upstream of
the Hydroxyl radical footprinting analysis confirmed that LrpA
protects its promoter from position The 46-bp binding sequence has been analyzed for sequence motifs that
could serve as targets for DNA-binding proteins (e.g. palindromes, inverted or direct repeats). An obvious 8-bp palindrome ACCTAGGT is present (Fig. 8A), but the possibility that this
is a specific recognition element for LrpA can be ruled out because LrpA binds well to promoter mutant 621, in which the palindrome has
partly been substituted (Fig. 8B). Moreover, the consensus binding sequence for E. coli Lrp consists of at least 15 bp.
Assuming that LrpA binds to two sites, it might be expected that the
two sites share similar sequence elements. Overall, however, there is
very little sequence homology between the two halves of the 46-bp
fragment. Although a CTAG motif is present in the left part of both of
these halves (position The appearance of DNaseI hypersensitive sites in the proximity of
DNaseI-protected regions is a very common phenomenon when DNA-binding
proteins interact with their target DNA and is generally interpreted as
a result of DNA bending. In some cases this bending occurs when DNA is
looped out through interaction between proteins bound to sites spaced
(far) apart (38). In many other cases, binding of a protein to a single
binding site causes bending of DNA (49-51). DNaseI footprinting
studies with these proteins, however, revealed only a small number of
hypersensitive sites, generally located within the area protected
against cleavage (2, 52-62). DNaseI footprints of E. coli
Lrp with several target promoter fragments show protection from DNaseI
over a range of 100 bp or even longer, due to multiple binding sites.
Hypersensitive sites are located between the protected regions (37,
63-67). Similar patterns are generated by the Lrp homologs BkdR from
P. putida (44) and PutR from Agrobacterium
tumefaciens (46). In the case of P. furiosus LrpA,
however, two distinct footprinting techniques indicate only a
significant protection of a 46-bp fragment of the lrpA
promoter, whereas DNaseI-hypersensitive sites are extended in both
directions, in total covering approximately 88 bp (Fig. 7). Hence, at
least under the conditions used for the DNaseI footprinting (elevated
LrpA concentrations), LrpA appears to affect the DNA conformation over
a relatively long distance. In the case of E. coli Lrp and
A. tumefaciens PutR, it has been suggested that DNA is
somehow wrapped around the regulators (66, 68). Analysis of PutR-DNA
complexes by atomic force microscopy supports the idea that PutR
condenses DNA into globular nucleoprotein complexes (46). Although a
similar looping or wrapping of DNA around P. furiosus LrpA
is possible, we cannot rule out the possibility that the observed
hypersensitivity pattern is a result of some nonspecific phenomenon in
the in vitro analysis.
In conclusion, we have described for the first time the actual
involvement of an archaeal Lrp homolog in transcription modulation by
in vitro analyses. The P. furiosus LrpA interacts
specifically with the lrpA promoter in the proximity of the
transcriptional start site. Hence, the observed transcription
inhibition is most likely a consequence of preventing RNA polymerase
recruitment similar to that reported for the A. fulgidus
MDR1 (13). In addition, LrpA binds to lrpA promoter
fragments in a single configuration, most likely as a tetramer.
Alternatively, such a configuration may also be referred to as a dimer
of dimers, but we do not have any indication of cooperativity, as has
been reported for E. coli Lrp (Calvo et al.
(14) and Newman and Lin (15)). Gel retardation analysis revealed
that the DNA binding efficiency of LrpA is reduced significantly when
the DNA fragments were reduced in size below 46 bp. The interaction
with this fragment was confirmed in two distinct footprinting
experiments. The actual binding site could at least in part be
identified, but as in many bacterial Lrp-target promoters, no obvious
palindromic motif(s) appear to be involved. Recent progress with
crystallization of P. furiosus
LrpA,3 may be
very important to confirm molecular details of the archaeal and
bacterial Lrp homologues, and as such, LrpA may be a model for further
understanding of structure-function relations of this widely
distributed class of transcription regulators.
*
This research was supported by Council for Chemical Sciences
(CW) of the Netherlands Organization for Scientific Research (NWO)
Grant 700-35-101 and by grants of the Deutsche Forschungsgemeinschaft and the Fonds der Chemischen Industrie to (to M. T.).The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
§
To whom correspondence should be addressed: Laboratory of
Microbiology, Dept. of Agrotechnology and Food Sciences, Wageningen University, Hesselink van Suchtelenweg 4, 6703 CT Wageningen, The
Netherlands. Tel.: 0031-317-483110; Fax: 0031-317-483829; E-mail:
arjen.brinkman@algemeen.micr.wau.nl.
Published, JBC Papers in Press, September 5, 2000, DOI 10.1074/jbc.M005916200
2
A. B. Brinkman and J. van der Oost,
unpublished information.
3
S. E. Sedelnikova, S. H. J. Smits, P. M. Leonard, A. B. Brinkman, J. van der Oost, J. B. Rafferty, and D. W. Rice, submitted for publication.
The abbreviations used are:
TBP, TATA-binding protein;
TFB, archaeal homologue of transcription factor
IIB;
BRE, TFB-responsive element;
bp, base pair(s);
PCR, polymerase
chain reaction;
PAGE, polyacrylamide gel electrophoresis;
DMSI, dimethylsuberimidate;
CAPS, 3-(cyclohexylamino)propanesulfonic
acid.
An Lrp-like Transcriptional Regulator from the Archaeon
Pyrococcus furiosus Is Negatively Autoregulated*
§,,,,,, and
Laboratory of Microbiology, Department of
Agrotechnology and Food Sciences, Wageningen University, Hesselink van
Suchtelenweg 4, 6703 CT Wageningen, The Netherlands and ¶ Institut
für Allgemeine Mikrobiologie, Cristian-Albrechts
Universität zu Kiel,
Am Botanischen Garten 1-9, 24118 Kiel, Germany
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
25 to 30 relative to the transcriptional start
site (+1). This complex is stabilized by TFB, which interacts with TBP
as well as with the nucleotides 42 to 19 that flank the TATA box
(2). In particular, a sequence upstream of the TATA box (called the
TFB-responsive element or BRE) is essential for transcriptional
polarity (3, 4). Formation of this pre-initiation complex results in
recruitment of the RNA polymerase complex (1). Although important
progress has recently been made with the elucidation of the archaeal
transcriptional mechanism, very little is yet known about the actual
regulation of this process. A limited number of studies reported that
expression of genes involved in nitrogen metabolism, methanogenesis,
and sugar metabolism are subject to substrate-dependent
regulation at the transcriptional level (5-9). Unfortunately, data
about the molecular mechanisms underlying this regulation are still scarce. One of the few transcriptional regulators that have recently been studied in more detail concerns GvpE, an activator that is required for the expression of genes involved in gas vesicle synthesis in halophilic archaea. In a molecular modeling study, GvpE has been
proposed to resemble a eukaryal leucine-zipper dimer that might
interact with a palindrome sequence of its target promoter centered
40-50 bp upstream of the transcriptional start site (10). Another
putative transcriptional regulator that has been studied in more detail
is Tfx from Methanobacterium thermoautotrophicum (11). The
tfx-encoding gene is located upstream of the operon encoding
molybdenum formylmethanofuran dehydrogenase (fmdECB). Tfx
binds to a site located 167 bp downstream of the transcriptional start
site of fmdE. It was proposed that Tfx is a transcriptional activator required for the expression of fmdECB. Obvious
homologues of Tfx can only be found within the domain of the archaea.
EXPERIMENTAL PROCEDURES
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EXPERIMENTAL PROCEDURES
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DISCUSSION
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DNA oligonucleotides used in this study
-D-galactopyranoside was added to
induce expression. After overnight incubation, the cells were
harvested, washed in 125 mM citrate buffer, pH 5.0 and
resuspended in 90 ml of the same buffer. Cells were lysed by a triple
passage through a French pressure cell at 1000 p.s.i. After lysis,
MgCl2 and DNaseI were added to final concentrations of 10 mM and 10 µg/ml, respectively. The sample was left at
room temperature for 15 min. Subsequently, the cell-free extract was incubated at 80 °C for 30 min and centrifuged at 20,000 rpm for 30 min. The remaining soluble fraction was loaded on a 60-ml cation exchange column (S-Sepharose, Amersham Pharmacia Biotech) that had been
equilibrated with 125 mM citrate buffer, pH 5.0. The column
was eluted with the same buffer using a flow rate of 3 ml/min and a
linear gradient of NaCl from 0 to 1 M. Fractions containing
LrpA, as determined by SDS-PAGE, were pooled and concentrated by
centrifugation in Centricon units (10-kDa cut off) until a volume of
0.5 ml was reached. A 200-µl sample was loaded on a gel filtration
column (Superdex 200, Amersham Pharmacia Biotech) with 20 mM Tris, pH 8.0, and 100 mM NaCl with a flow
rate of 0.5 ml/min. The elution pattern from this gel filtration showed
three peaks corresponding to molecular masses of approximately 30, 60, and 120 kDa, respectively. Approximately 14 mg of purified LrpA was
obtained from one liter of culture.
-32P]ATP.
Binding reactions were performed in a total volume of 20 µl
containing 40 mM HEPES-NaOH, pH 7.3, 200 mM
KCl, 2.5 mM MgCl2, 2 mM
dithiothreitol, 1 mM CaCl2, 100 mM
EDTA, 10% glycerol, and varying concentrations of purified LrpA.
Standard reactions contained 2 µg of poly(dI·dC)·poly(dI·dC) as
nonspecific competitor DNA, but this was omitted from reactions with
smaller fragments (fragment E and F) and during determination of the
dissociation constant (Kd) for the LrpA-DNA complex.
Each reaction contained 1 to 10 ng of [-32P]ATP
end-labeled DNA. Reactions were incubated at room temperature for at
least 10 min and separated on a non-denaturing 8% acrylamide gel
buffered in 1× Tris borate EDTA buffer (25). In the case of fragment
E, a 20% gel was used. Gels were dried, exposed to phosphor screens,
and analyzed. Quantification was done using ImageQuant software
(Molecular Dynamics, Inc.).
RESULTS
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ABSTRACT
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EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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Fig. 1.
A, sequence of the
lrpA promoter. The transcriptional start (+1) is indicated
with a horizontal arrow. Underline, BRE element;
box, TATA element; bold italics, ATG start codon
of lrpA. B, the gdh-lrpA locus and DNA
fragments used in this study. HindIII restriction sites
indicate the genomic fragment carrying the glutamate
dehydrogenase-encoding gene (gdh) and the gene encoding the
Lrp-like regulator (LrpA). Filled squares show the TATA
boxes of the gdh and lrpA promoters. Dotted
lines display the enlarged intergenic region between
gdh and lrpA with the TATA boxes of the
lrpA promoter, the lrpA transcriptional start
site (+1), and DNA fragments (A-G) used in experiments.
kb, kilobases.
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Fig. 2.
Alignment of P. furiosus
LrpA with (putative) archaeal and bacterial Lrp/AsnC
homologues. Homologues of the Lrp/AsnC family of transcriptional
regulators can be identified in all sequenced archaeal genomes. From
each sequenced archaeon the deduced amino acid sequence of a putative
Lrp/AsnC-like regulator with highest homology to P. furiosus
LrpA is aligned with that of P. furiosus LrpA using the
program ClustalX. In addition, the amino acid sequences of Lrp and AsnC
from E. coli are aligned. Amino acids were grouped in four
clusters: I, L, V, and M; R and K; F, Y, and W; and E, D, N, and Q. Black-shaded symbols indicate completely conserved amino
acid residues or amino acids belonging to the same cluster.
Gray-shaded symbols indicate seven or eight residues
belonging to one cluster. The helix-turn-helix DNA binding motif is
boxed. P.f. LrpA, P. furiosus
GenBankTM accession number P42180; P.h. PH1592,
P. horikoshii GenBankTM accession number
AP000006, 93% identity (132/141); P.a. PAB0392, P. abyssi GenBankTM accession number CAB49492, 98%
identity (139/141); M.j. MJ0723, M. jannaschii
GenBankTM accession number Q58133, 54% identity (77/141);
A.f. AF1723, A. fulgidus GenBankTM
accession number AE000984, 49% identity (69/140); M.t.
MTH1193, M. thermoautotrophicum GenBankTM
accession number AE000887, 37% identity (27/72), S.s.
c01007, S. solfataricus GenBankTM accession
number Y08256, 32% identity (46/141); E.c. AsnC, E. coli GenBankTM accession number P03809, 33% identity
(46/139); E.c. Lrp, E. coli GenBankTM
accession number P19494, 28% identity (41/143).
DE3). After overnight growth in the presence of 0.4 mM
isopropyl-1-thio--D-galactopyranoside, cells were
harvested and disrupted. Tricine-SDS-PAGE analysis of membrane and
soluble fractions indicated that 50% of the produced LrpA was present
as soluble protein (Figs. 3, lane
3, and 4). The soluble fraction
containing LrpA was further subjected to a heat incubation of 30 min at
80 °C, resulting in the denaturation of most of the E. coli proteins (Fig. 3, lane 5). This heat-stable cell
free extract was used for further purification by cation exchange
chromatography and gel filtration chromatography (Fig. 3, lanes
6 and 7). The calculated molecular mass of LrpA is 15.9 kDa, which is in good agreement with its migration on SDS-PAGE (Fig.
3). Elution patterns from gel filtration showed peaks corresponding to
molecular masses of approximately 30, 60, and 120 kDa. This suggests
that LrpA exists as a dimer, tetramer, and octamer in solution. We
performed several independent gel filtration experiments with LrpA, and
the apparent oligomeric heterogeneity was always observed.
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Fig. 3.
Overexpression and purification of LrpA.
10% Tricine-SDS-PAGE (31) showing extracts of E. coli
BL21(DE3) after several steps of purification. Lanes 1 and
2, insoluble and soluble fraction of extract from
pET9d-containing strain, respectively; lanes 3 and
4, insoluble and soluble fraction of extract from
pLUW604-containing strain, respectively. These extracts clearly show
overexpression of P. furiosus LrpA (arrow). The
extract shown in lane 4 was subjected to a 30-min heat
treatment at 80 °C and was subsequently centrifuged to separate
denatured proteins from heat-stable proteins, resulting in a
heat-stable cell-free extract (lane 5). This heat-stable
cell-free extract was used for further purification consisting of
cation exchange chromatography (lane 6) and gel filtration
(lane 7). M, molecular mass markers.
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Fig. 4.
Analysis of the transcription start site of
the lrpA promoter in vitro by primer
extension. The sequence of the template DNA strand is shown left
of the primer extension product (marked G, A,
T, C). Lane 1, control experiment
(nucleotides omitted from transcription reaction); lane 2,
analysis of the primer extension product.
35 to 23 sequence relative to
the transcriptional start (+1), where n = any base, and
W = A or T). The putative BRE and TATA elements of the
lrpA promoter match well with the consensus sequence mentioned above (see Fig. 1A).
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Fig. 5.
A, inhibition of lrpA
transcription by LrpA. Linearized pLUW613 DNA containing the P. furiosus lrpA promoter was used as the template in cell-free
transcription experiments. The 160-nucleotide (nt) run-off
transcripts are indicated by arrows. B, effects
of LrpA on cell-free transcription from the lrpA and
gdh promoter of Pyrococcus and the
tRNAVal promoter of Methanococcus. Transcripts
from the M. vannielii promoter were analyzed in the in
vitro transcription system of Pyrococcus as shown
previously (26). The addition of recombinant LrpA (0.8 µg) is
indicated (+/ ). The run-off transcripts are indicated by
arrows, and their respective sizes are shown.
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Fig. 6.
LrpA binds specifically to lrpA
promoter DNA. 0, 30, 90, 270, or 810 nM purified
LrpA was added to fragments C and D. 2 µg of
poly(dI·dC)·poly(dI·dC) was present in these reactions. 0, 10, 25, 50, 100, or 200 nM purified LrpA was added to fragments
E and F. No aspecific competitor DNA was present in these
reactions.
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Fig. 7.
A, DNaseI footprint analysis using
purified LrpA and lrpA promoter DNA. 0, 30, 90, 270, 810, 2430, and 0 nM purified LrpA was incubated with labeled
fragment B (see Fig. 1B). After DNaseI treatment, the DNA
was analyzed in parallel with a sequencing reaction. Left,
5'-labeled non-template strand; right, 5'-labeled template
strand. Brackets indicate DNaseI protection, and
arrows refer to hypersensitive sites. B, profile
plots of hydroxyl radical footprinting. Panel I,
non-template strand; panel II, template strand. Nucleotide
positions are given relative to the lrpA transcriptional
start (+1). Upper traces, no LrpA added; lower
traces (bold), 2.4 µM LrpA added, as
calculated for monomeric protein. Profile plots at the bottom indicate
sequence reactions that were run in parallel with hydroxyl radical
cleavage reactions. Brackets indicate protection against
hydroxyl radical cleavage in the presence of LrpA. C,
schematic summary of results obtained from gel mobility shift
experiments, DNaseI footprinting, and hydroxyl radical footprinting. A
double-helical representation of the lrpA promoter region is
given along the sequence of the non-template strand. Filled
circles, protection against hydroxyl radical cleavage;
filled arrows, protection against DNaseI cleavage;
open arrows, DNaseI hypersensitive sites. Sequence positions
are relative to the lrpA transcriptional start (+1).
Boxed sequences indicate the BRE element, TATA element, and
ATG start codon, respectively.
-ketoglutarate, pyruvate, cellobiose, and
ammonium. However, none of these compounds affected LrpA binding at
either the lrpA or the gdh promoter.
19 to +21 relative to
the lrpA transcriptional start (+1, Fig. 7A).
This indicated that this region contained the LrpA binding sequence.
Additionally, sites hypersensitive to DNaseI cleavage were observed.
Such an effect is common when DNA-binding proteins bind to their target DNA and can be explained as protein-induced DNA bending (38). In the
case of LrpA, however, apparent hypersensitivity appeared mainly at
positions outside of the 19 to +21 region, suggesting that binding of
LrpA affected the DNA conformation upstream and downstream of its
binding site (see "Discussion"). DNaseI footprinting experiments
were also performed with purified LrpA and fragment G containing the
gdh promoter. As in gel mobility shift experiments, no
interaction between LrpA and gdh promoter DNA could be
detected (not shown).
22 and +24. A spacing of approximately 10 bp was
present between disappearing bands, which indicated that interactions took place along the same face of the double helix. A schematic summary
of the data obtained from gel mobility shifts, DNaseI, and hydroxyl
radical footprinting is given in Fig. 7C.
19 to
+11 region, we tested whether LrpA was able to shift a 30-bp fragment
(F, Fig. 7C) containing only this 19 to +11
sequence. This fragment is only partly shifted, even at higher LrpA
concentrations (Fig. 6). Although binding to this fragment was, thus,
much weaker than to larger fragments like E or D, sequence elements
specifically recognized by LrpA are present within this region.
Therefore, we designed mutations in this particular region for a more
detailed analysis of the sequence elements required for the LrpA-DNA
interaction. The effects of these mutations were tested in gel mobility
shift experiments and in the cell-free transcription system mentioned
above. In gel mobility experiments we used mutants of fragment B (Fig.
1B), and for the cell-free transcription experiments, we
cloned mutants of fragment A (Fig. 1B) into pGEM-T. Although
transcriptional activities or transcriptional start sites were slightly
altered for some mutant promoters, it was possible to study the effect of LrpA on transcription from the mutated templates.
19 to +11 sequence (Fig. 8A, 621). In a gel
mobility shift experiment, however, a DNA fragment containing this
mutation shifted with an efficiency almost identical to that of the
wild-type DNA fragment (Fig. 8B). It was impossible, however, to analyze the effect of this mutation by in vitro
transcription, since no transcript was formed using this mutant DNA as
a template. A sequence element crucial for transcription is apparently
disturbed in this mutant. Most likely this element corresponds to (part of) the initiator element (INR, previously referred to as box B) (39,
40), since it is located around the transcriptional start site.
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Fig. 8.
A, analysis of mutant lrpA
promoters by mobility shift experiments and in vitro
transcription. Black arrows, 8-bp palindromic sequence;
sequence with gray background, conserved sequence between
lrpA promoters of P. furiosus, P. horikoshii, and P. abyssi. The 19 to +11 region
protected from DNaseI cleavage is indicated (see Fig. 7). B,
LrpA-DNA binding and in vitro transcription with mutant
lrpA promoter DNA. Wild type (w.t.) and mutants
of fragment B (Fig. 1B) were used in gel mobility shift
experiments. LrpA concentrations were 0, 30, 90, 270, and 810 nM, as calculated for monomeric protein. 2 µg of
poly(dI·dC)·poly(dI·dC) was present in each reaction. To
determine the percentage of shift, the bands were quantified using
PhosphorImager. The plasmids pLUW613 (wild type), pLUW623,
pLUW629, and pLUW630 were linearized with PstI and analyzed
in in vitro transcription in the presence of 0, 1.1, and 2.2 µM LrpA. The arrow indicates the
160-nucleotide run-off transcript from the wild type. Transcription
activities were calculated using phosphorimaging. Binding efficiency
indicates the percentage of shift relative to the wild type that was
obtained in gel mobility shift experiments upon the addition of 30 nM LrpA. Transcription inhibition indicates the inhibition
of transcription by LrpA relative to the wild type observed in the
presence of 1.1 µM LrpA. nt,
nucleotides.
19 to +11 region (Fig. 8A, 623 and
629). When we substituted TTATAC into GGCGCA (623) we found
that the affinity of LrpA for this mutant DNA was in fact higher than
for the wild-type DNA sequence. In accordance, LrpA inhibited in
vitro transcription more efficiently (125%, Fig. 8B).
When we substituted TAGGTGGTT into GCTTGTTGG (629), there was no
binding of LrpA in a gel mobility shift experiment. This was in
agreement with the affected transcription inhibition, which was only
52% compared with wild-type DNA (Fig. 8B).
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Fig. 9.
SDS-PAGE analysis of cross-linking
experiments with and free LrpA (left) or LrpA in
complex with DNA (right). Numbers I to IV
indicate molecular masses corresponding to an LrpA monomer, dimer,
trimer, and tetramer, respectively.
DISCUSSION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
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30
to +20 at a number of promoters in DNaseI footprinting experiments (47). In a similar approach, Hausner et al. (2) demonstrate that TBP and TFB together protect the 42 to 19 region of the P. furiosus gdh promoter. Assuming that these proteins bind
the same region at the lrpA promoter, LrpA binding occurs
immediately downstream of the bound TBP-TFB complex (22 to +24, Fig.
7C). In this way, LrpA blocks at least the binding of the
RNA polymerase, thereby inhibiting completion of the archaeal
transcription initiation complex. Such a mechanism of repression has
recently been demonstrated for the A. fulgidus
metal-dependent transcriptional repressor MDR1 (13).
Repression occurs when MDR1 binds to the 18 to +67 sequence of its
target promoter, thereby preventing RNA polymerase recruitment but not
binding of the TBP-TFB complex. Since the 5' border of the LrpA binding
sequence (24) is comparable with that of MDR1 (18), a similar
mechanism of repression is anticipated.
42 to 19 region involved in binding of the TBP-TFB complex, as
has been suggested for the Haloferax GvpE transcriptional
activator (10). In addition, a probable requirement would be a specific interaction between the bacterial-like LrpA protein and one or more
components of the eukaryal-like (pre-)initiation complex. Although many
genes encoding Lrp/AsnC homologues can be found within archaea, their
role as transcriptional global regulators or activators remains speculative.
22 to +24 (Fig. 7B).
We compared the size of the protected sequence (46 bp) to hydroxyl
radical footprints obtained from E. coli Lrp in complex with
ilvIH and ilvGMEDA (36, 37). In these cases two
E. coli Lrp dimers bind to a dual binding site of about 45 bp. In addition, it has been shown that one Lrp dimer binds to a single
binding site of about 15 bp (43). It is not unlikely that the P. furiosus LrpA binding sequence consists of two adjacent binding
sites. In gel mobility shift experiments only one distinct LrpA-DNA
complex is present. This suggests either binding of an LrpA tetramer or
the highly co-operative binding of two LrpA dimers. In both cases four
LrpA monomers are in complex with DNA, as was detected using chemical cross-linking of LrpA in a specific LrpA-DNA complex. Both of the above
mentioned configurations (tetramer or two dimers) would explain why a
fragment of at least 43 bp is necessary for a stable LrpA-DNA complex
in gel mobility shift experiments (see Fig. 6). In contrast, for a
stable interaction between an E. coli Lrp dimer and a single
binding site, a DNA fragment of only 21 bp is necessary (43).
20 and 2), the combined results from our
mutational analysis suggest that the GGTTC sequence and not the CTAG
sequence is specifically recognized by LrpA (Fig. 8). No similar
sequence is present in the other half of the 46-bp fragment. Although
the LrpA binding sequence is very well conserved between P. furiosus, P. horikoshii, and P. abyssi, we
found that substitutions in some of these conserved sequences
(e.g. promoter mutant 623) had no effect on LrpA binding. It
is therefore possible that LrpA does not recognize a limited number of
specific bases but rather a relatively long sequence with a specific
secondary structure. Indeed, certain protein-DNA interactions have been reported to be the result of a specific DNA structure and/or
flexibility (48). In addition, it should be noted that a consensus
sequence for E. coli Lrp is in many cases not obvious at all.
FOOTNOTES
ABBREVIATIONS
REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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