(Received for publication, September 6, 1996, and in revised form, October 28, 1996)
From the Centro Nacional de Biotecnología, Consejo Superior de Investigaciones Científicas, Campus de Cantoblanco, 28049 Madrid, Spain
This work reports a genetic analysis of the
interactions between NahR, the LysR-type regulator of the NAH operons
for biodegradation of naphthalene in Pseudomonas, and its
aromatic effectors. Six mutants encoding NahR variants responsive to
salicylate analogs such as benzoate, which is not an inducer for the
wild type regulator, were isolated with a polymerase chain
reaction-based saturation mutagenesis protocol. Most mutants displaying
a specific change of effector profile bore single amino acid
substitutions within a short protein segment of 60 residues located at
the central portion of the NahR sequence. Some of the protein variants
exhibited an increased affinity for salicylate and also for otherwise
suboptimal effectors, with apparent
Ks values 5-100-fold
lower than those of the wild type NahR protein. In addition, all
mutants were activated by inducers bearing novel substituents at
positions 1 or 2 of the aromatic ring and displayed also an enhanced
tolerance to changes at positions 3 and 4. Correlation between
mutations in NahR and the structures of the new effectors suggested
that protein sites Met116, Arg132,
Asn169, and Arg248 are involved in effector
recognition and binding during the earlier steps of the process leading
to transcriptional activation of cognate NAH promoters.
Transcriptional regulators belonging to the LysR-type family (hereafter referred to as LTTRs)1 have protein sizes ranging from 276 to 324 amino acids, and they are widely distributed among prokaryotes (1). Individual members of the family share their being responsive to chemical effectors, their being transcribed divergently from the genes that they regulate (frequently accompanying an autorepression mechanism), and their mode of transcriptional activation of target promoters. All LTTRs studied so far in this respect remain bound to equivalent promoter-proximal target DNA sequences regardless of the presence or absence of inducer. Effector binding and subsequent transcriptional activation seem to result in the relief of the DNA bending caused by LTTR binding under noninduced conditions (reviewed in Ref. 2). In fact, the most conserved portion of LTTRs is precisely the N-terminal segment that contains the helix-turn-helix DNA-binding motif that accounts for binding to DNA (3).
Apart from changes in DNA structure, the precise mechanism by which
inducer binding is ultimately translated in transcriptional activation
remains largely unknown. LTTRs contain a poorly conserved central
domain (see Fig. 1) believed to interact with the chemical inducers.
The divergence of the central portions of LTTRs seems to reflect the
variety of inducers to which these proteins respond (1). This notion is
supported by comparisons between various NodD proteins of
Rhizobium species. These LTTRs are similar and bind the same
target DNA sequences, but minor differences in their central domain
account for their responsiveness to distinct flavonoid derivatives (4,
5). Furthermore, constitutive, inducer-independent mutants of
various LTTRs have been found to bear changes in their central domain
(6-9). However, evidence of direct interactions between specific
residues of LTTRs and their cognate inducers is generally scarce. A
particularly useful LTTR to address this issue is the NahR protein of
Pseudomonas, the salicylate-responsive transcriptional
regulator of two operons for biodegradation of naphthalene by strains
carrying the catabolic plasmid NAH7 (Refs. 1, 3, and 10; see Fig. 1).
Because the native effector of NahR is a simple aromatic
compound, an entire variety of salicylate analogs is commercially
available to search for altered effector specificities. In this work,
we show that mutations at the central domain of NahR expand the range
of aromatic compounds that can activate the protein into a
transcriptionally competent form. On the basis of these results, we
have identified a region of the NahR protein that may interact with the
aromatic inducers and tentatively pinpoint those amino acid
residues involved in effector specificity.
The
bacterial strains and plasmids used in this work are listed in Table I.
Plasmids bearing an R6K origin of replication (i.e.
mini-Tn5 delivery vectors) were always propagated in
Escherichia coli CC118pir. Bacteria were grown
in rich LB medium (11) supplemented where required with 150 µg/ml
ampicillin (Ap), 50 µg/ml kanamycin (Km), 25 µg/ml streptomycin
(Sm), and 40 µg/ml 5-bromo-4-chloro-3-indolyl
-D-galactopyranoside (X-Gal). Recombinant DNA techniques
were made following published protocols (12). Insertion of hybrid mini-transposons into the chromosome of target bacteria was made as
described in detail elsewhere (13) using E. coli
S17-1
pir as the donor strain of suicide delivery
plasmids. DNA sequencing of NahR variants was carried out on
double-stranded templates with an automatic Applied Biosystems
instrument and a dye terminator cycle protocol with Taq
polymerase.
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Activity of
NahR was monitored in all cases by following its ability to cause
accumulation of -galactosidase in an E. coli strain
bearing a transcriptional Psal::lacZ fusion. To
this end, a hybrid between nahG (the first gene transcribed
from Psal; see Fig. 1) and lacZ was made by
cloning a 0.5-kb SalI-PstI fragment of pMS15
(spanning the Psal promoter; Ref. 3) in the corresponding sites of lacZ vector pNM482 plasmid (14). This fused the
first 70 codons of nahG to the eighth codon of
lacZ. The same fusion was recloned in pUJ9 (13) by exchange
of EcoRI-SacI segments between the two plasmids.
The entire Psal::nahG
-
lacZ fusion (simplified,
Psal::lacZ) was then excised as a NotI
fragment from the resulting plasmid and placed into the NotI
site of pUT/mini-Tn5Sm (15). This gave rise to pTSAL1, a
delivery vector for a hybrid mini-transposon bearing the
Psal::lacZ fusion, which was placed into the
chromosome of E. coli CC118 as explained in de Lorenzo and
Timmis (13). Such an arrangement places strong transcriptional terminators upstream and downstream of the reporter cassette (see Fig.
1) to prevent readthrough transcription from nearby chromosomal promoters after insertion. The resulting strain (E. coli
SAL1) was used as the recipient of plasmids bearing the nahR
variants as described below. Induction of the Psal promoter
in E. coli cells bearing Psal::lacZ
fusions was made by growing the corresponding cultures in LB medium at
37 °C up to an A600 of 0.4, after which inducers were added at the concentrations indicated in each case. Incubation was then continued for 5 h, and the accumulation of
-galactosidase was measured in cells permeabilized with chloroform and sodium dodecyl sulfate as described by Miller (11).
-Galactosidase activity values given throughout this paper represent
the average of at least three independent experiments, each of which
was conducted in duplicate samples, with deviations being less than
15-20%.
The plasmid pNR, used as the
DNA template for the protocol described below, was produced by
transferring an 1.2-kb NcoI-HindIII fragment from
pMS15 (3) bearing the entire nahR sequence to the same sites
of vector pFH2 (16). For mutagenesis, the DNA regions of interest
within pNR were amplified with the polymerase chain reaction (PCR)
using the oligos NRBgl (5-ACCGACATTGGCGAGATCT-3
) and
NRSph (5
-CTTGTGGTACTTCGCATGC-3
) under conditions favoring errors of the Taq DNA polymerase. 100-µl PCR reactions
were set up in a buffer containing 0.1 mM
MgCl2, 0.5 mM MnCl2, 1 mM dGTP, 1 mM dTTP, 1 mM dCTP, 0.25 mM dATP, 0.5 µg of each of the primers, and 5 units of
Taq DNA polymerase. 1-50 ng of pNR template was added to
the reactions, the amount depending on the rate of mutations desired.
The resulting 0.6-kb amplification products were digested with
BglII and SphI, purified, and used to replace the
equivalent segment of pNR. A second DNA template, namely plasmid
pUC/NR, was alternatively employed for mutagenesis of a different
nahR portion (see Fig. 2). pUC/NR bears also the entire
nahR gene assembled as the result of a tripartite ligation
between NotI-digested pUC18Not (17), a 0.6-kb
NotI-BglII fragment of pUC/NRC (see Table I) and
a 0.4-kb BglII-NotI fragment of pNR. pUC/NR has
an unique HindIII site that simplifies insertion when
required of the 0.6-kb HindIII-SphI segment of
nahR sequence resulting from error-prone PCR with primers
NRH5 (5
-ATCTGGCCGAGCCCGTC-3
) and NRSph. As before, the mutated HindIII-SphI DNA segments
were purified and cloned in the same sites of the larger fragment of
pUC/NR. After mutagenesis, screening for NahR variants with altered
effector specificity included the individual culture of each of the
E. coli SAL1 transformants with the reconstructed
nahR+ plasmids in microtiter plates, followed by
their replication on separate LB plates amended with Ap, X-Gal, and 1 mM of each of the aromatic compounds under scrutiny.
Differences in the intensity of the color developed in equivalent spots
in each plate after incubation was considered an indication of altered
NahR activity.
Construction of nahR/Psal-lacZ Insertions
Mini-Tn5 derivatives bearing not only a
Psal-lacZ fusion but also the mutant nahR
variants named nahR3 and nahR4 were made as
follows. pNR derivatives encoding the mutated genes (pNR3 and pNR4,
respectively) were partially digested with HindIII and
ligated to a 2.1-kb HindIII -Km fragment (18). The
location and orientation selected was the same than that present in the
reference wild type nahR/Psal-lacZ mini-transposon bore by
pCNB4lacZ plasmid (Ref. 19; see Fig. 1). The resulting
plasmids (pNR3Km and pNR4Km, respectively) were
then digested with NcoI, which produced 2.2-kb DNA fragments
spanning the entire mutant nahR sequence and part of the
-Km fragment. The equivalent NcoI segment
pCNB4lacZ was then replaced by each of these NcoI
segments, thus replacing the wild type nahR sequence by the
mutant variants and reconstructing
-Km interposon. These
manipulations originated transposon delivery plasmids
pCNB43lacZ and pCNB44lacZ that carry hybrid
mini-transposons containing nahR3/Psal-lacZ and
nahR4/Psal-lacZ reporter elements, respectively. Once
inserted into the chromosome of E. coli CC118 (Table
I), the accumulation of
-galactosidase by cells
exposed to aromatic inducers was carried out as described above.
In order to determine which specific portions of the salicylate molecule were engaged in activation of NahR, we examined the degree of structural permissiveness of the regulator toward structural variants of the natural inducer. To this end, we assembled the entire segment of the NAH7 plasmid that spans the wild type nahR gene and adjacent regions in a mini-Tn5 transposon vector (Fig. 1), thereby faithfully reconstructing in E. coli all the regulatory elements that participate in the activation of the Psal promoter in Pseudomonas. In this construct, nahR is expressed under its own promoter and transcribed divergently from the Psal promoter, followed by a promoterless lacZ reporter gene (Fig. 1). This element was then placed into the chromosome of E. coli, and the resulting strain (E. coli RSL9) was challenged with a variety of aromatic compounds as described under "Materials and Methods." Reproduction of the system in E. coli prevented any metabolism of the aromatic compounds leading to other intermediates than those added to the culture and ensured their transport to the cell cytoplasm through a broad specificity facilitated diffusion system (20).
The results of measuring accumulation of -galactosidase under the
different inducers is summarized in Table II. One
important conclusion of this experiment is that the presence of a
carboxyl group in the effector is an absolute requirement for NahR
activation. As shown in Table II, salicylamide (compound B),
2-hydroxy-acetophenone (compound C), and salicyl alcohol (compound D)
caused no accumulation of the reporter product. On the contrary,
substitutions of the 2-hydroxyl group of salicylate were more
tolerated, as indicated by the
-galactosidase activity produced
after the addition of anthranilic acid (compound F),
o-acetyl-salicylic acid (compound G), or to a lesser extent
o-methoxy-benzoic acid (compound H). However, benzoate
(compound E) or 2-chloro-benzoate (compound I) did not give rise to any
significant induction of the reporter system. Chloro and methyl
substituents in positions C-3, C-4, and C-5 of the aromatic ring of
salicylate appeared also to be tolerated (Table II). Introduction of
hydroxyl or methoxyl groups in sites C-4 or C-5 of salicylate decreased
the induction ability of the compounds that were, however, still able
to activate NahR to significant levels. Finally, although with reduced
activity, di- or tri-chloro salicylate derivatives (compounds M and N)
could induce also the reporter system.
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In summary, it seems that specific contacts between substituents of the aromatic ring and the protein engage exclusively positions C-1 and C-2 of the salicylate, the minimal apparent requirements being the presence of a carboxyl group in C-1 and the presence of a small functional group with available electrons in C-2. NahR appeared to accept a wide variety of salicylate structural analogs as effectors, thus reflecting the permissiveness of the protein domain(s) that interacts with the aromatic molecules. The decrease and even lack of activity observed when bulkier groups are entered in other positions may reflect a steric hindrance related to the size of the "effector pocket" in the regulator and not to the disruption of specific protein-inducer interactions.
Isolation of NahR Mutants with Altered Effector SpecificityOnce the structural requirements of NahR effectors were determined, we set out to probe the location of the protein segments involved in interactions with the aromatic compounds. We assumed that changes in the amino acid residues involved in effector recognition may result in NahR variants that can be activated by otherwise nonproductive inducers. On this basis, we designed a genetic strategy to identify NahR mutants that could respond to compounds found to be unable to act as effectors of wild type NahR (Fig. 2). In particular, we pursued the isolation of mutants responsive to benzoate, because we reasoned that NahR variants lacking the interactions with the quite permissive yet important position C-2 should appear at a reasonable frequency. To this end, we constructed an E. coli strain (named E. coli SAL1) bearing a chromosomal Psal::lacZ fusion, which was used as the recipient of plasmids bearing mutagenized nahR sequences. With the protocol described under "Materials and Methods," we first targeted the portion of NahR spanning amino acids 110-277, corresponding to a DNA segment of 0.49 kb (Fig. 2). This region was amplified through error-prone PCR from plasmid pNR. The ligation of the resulting BglII-SphI fragment with pNR digested with the same enzymes was then electroporated in E. coli SAL1 and plated out on LB/Ap/benzoate/X-Gal plates. After incubation, about 1% of the Ap-resistant colonies were intense blue. In order to discard constitutive mutants, these blue colonies bearing plasmids encoding putative NahR mutants were replicated in LB/Ap/X-Gal plates with or without benzoate, and only those clearly regulated by the aromatic compound were kept for further analysis. This was the case with two-thirds of all colonies tested, i.e. only about one-third of all mutants gave a constitutive, effector-independent phenotype, whereas the rest were genuinely responsive to benzoate. In addition, none of the benzoate-responsive mutants lacked their responsiveness to salicylate.
Characterization of Benzoate-responsive NahR VariantsTwenty
of the nahR+ pNR derivatives present in E. coli colonies giving a benzoate-responsive color in X-Gal plates
were subjected to DNA sequencing. This revealed the existence of at
least six independent mutations (in all cases single-base transitions)
in the nahR sequence (Fig. 2) accountable for the distinct
phenotype observed. Mutants NahR3 (R248C) and NahR4 (N169D) bore a
single-amino acid change that made the resulting proteins to respond to
benzoate to the same extent as the wild type responds to salicylate
(Table III). In contrast, mutants NahR5 (M116I), NahR6
(M116T), and NahR8 (M116V) displayed a remarkably high basal level of
activity in the absence of any inducer, whereas they reached a similar
degree of -gal accumulation with either benzoate or salicylate
(Table III). This semiconstitutive phenotype was caused in all three
cases by the exchange of the Met116 residue for neutral
amino acids. Mutants NahR3 and NahR4 will be termed hereafter as
variants type I, whereas mutants NahR5, NahR6, and NahR8 will be named
variants type II. Interestingly, the same amino acid change bore by
NahR5 was found by Huang and Schell (21) in their quest for
salicylate-independent NahR proteins.
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Mutant NahR7 (R132C), albeit similar to type I mutants, showed an intermediate phenotype because its basal activity was about twice that of the wild type and its induction by benzoate was significantly less than its responsiveness to salicylate. However, it gained a remarkable inducibility by other effectors. In fact, further analysis of the ability of various compounds to activate mutant NahR variants revealed that mutants type I and NahR7 (which bear single amino acid changes) had generally broadened their effector profile while maintaining a tight regulation. For instance, as indicated in Table III, NahR3 and NahR7 acquired the ability of being activated by salicylamide, and they displayed also an enhanced induction by chloro-derivatives, whereas NahR4 seemed to be more specific in gain of responsiveness to benzoate. Similarly, mutants type II generally broadened their effector profile. However, because these mutants display an up phenotype, it was difficult to distinguish which compounds became authentic inducers because of a gain of function in NahR and which behaved as such because of an unspecific amplification of an otherwise residual responsiveness. At least in the case of salicylamide and 4 chloro-benzoate, it seems that two of the type II mutants acquired a genuine ability to respond to these aromatic compounds that was totally missing in the wild type regulator.
Affinity of Group I Mutants for Inducer CompoundsTo gain
some insight in the mechanism by which group I mutants
broadened their effector profile, they were subjected to a series of
experiments to compare the apparent affinities of NahR for four
representative effectors, namely salicylate, benzoate, 3-chloro-benzoate and 3-methyl salicylate. To this end, we employed the
procedure developed by Ramos et al. (20) to estimate
in vivo the apparent
Ks values of effectors
for prokaryotic transcriptional regulators. The procedure depends on
the assumptions that (i) benzoate analogs are transported into E. coli cell through nonlimiting facilitated diffusion and (ii) the
output of the reporter lacZ fusion reflects faithfully the
activity of the regulator. Because these two conditions can be safely
assumed in our system, we set out to examine the induction of a
reporter Psal-lacZ fusion by varying effector
concentrations. In order to decrease the number of variables in the
procedure, we engineered the mutant nahR3 and
nahR4 genes along with the reporter Psal-lacZ
fusion within a mini-Tn5 vector (Fig. 1). These elements,
along with that bearing wild type nahR (19), were introduced
into E. coli CC118 by transposition, giving rise to strains
E. coli RSL9 (wild type nahR), E. coli
R3SL1 (nahR3), and E. coli R4SL1
(nahR4). As shown in Fig. 3, each of the
strains was subjected to induction experiments with concentrations of the aromatic compounds ranging from 10
5 to 1 mM. It is interesting to note that the fully induced cells displayed a responsiveness to each of the aromatic compounds virtually identical to that observed when the reporter system carries the nahR variants in a multicopy plasmid (Table III). This ruled
out that the phenotypes raised by the nahR mutants were
simply due to different expression levels. On the other hand, the shape
of the dose-response curves in Fig. 3 clearly indicated that the mutations did increase the affinity of NahR for specific aromatic compounds. This is particularly true for benzoate: as shown in Fig.
3C, the affinity increased from virtually nil to an apparent Ks
value in the range of 0.5 mM. The operative affinities of NahR3 for 3-chloro-benzoate
and 3-methyl salicylate increased >100-fold and >10-fold,
respectively, as compared with wild type NahR. Interestingly, NahR4
also seemed to remarkably increase its affinity toward salicylate. These results suggested that the mutations carried by NahR variants type I affected amino acid residues involved in inducer binding.
Benzoate-responsive Multiple Mutants Share the Same Key Changes in the NahR Sequence
In an attempt to identify additional residues that could simultaneously be involved in interactions with the aromatic effectors, we repeated the mutagenesis protocol under conditions in which error-prone PCR was expected to enter more than one base change per molecule of amplified DNA (see "Materials and Methods"). Furthermore, we employed primers NRH5 and NRSph, which amplified a longer portion of the NahR sequence (Fig. 2) along with plasmid pUC/NR (Table I). This facilitated the recovery of the mutagenized DNA segment. The procedure yielded 47 benzoate-responsive clones. On the basis of their responsiveness to selected inducers (salicylate, o-acetyl-salicylate, 3-methyl-benzoate, 2,3-chloro-benzoate, 2,6-chloro-benzoate, anthranylate, 5-chloro-salicylate, salicylalcohol, phenol, and salicylamide), they fell equally (23 and 24 clones) within the two types of mutants generated with the single-mutation protocol. As before also, none of the mutants lost its responsiveness to salicylate. Out of the entire collection, we selected 12 clones displaying a phenotype of low basal activity and broadening of their effector profile. All turned out to largely behave as NahR3, NahR4, or NahR7. Six of these were sequenced. The variant nahR138 was altered in five bases, three of them producing no amino acid changes, and the other two causing mutations N125S and N169D. Two other mutants were found to bear changes in two bases, both resulting in amino acid exchanges: nahR105 (R248C, A272T) and nahR141 (M139T,N169D). Finally, two mutants bore three changed residues: nahR135 (Q158R,N169D,E208G) and nahR130 (N156S,V226M,R248C), whereas the remaining one (renamed nahR123) was again, N169D. Therefore, four of the new six variants had the change N169D, already studied in nahR4, whereas the other two, alike nahR3, bore the change R248C. Therefore, the benzoate-responsive effect of the multiple mutants was attributed to the presence of mutations already identified and not because of the other amino acid changes.
A number of NahR mutants had been isolated in the past that could not activate the Psal/Pnah promoters because of their inability to bind DNA (1, 9). Not surprisingly, some of these were found to cluster within the the N-terminal portion of the protein bearing an helix-turn-helix motif (residues 23-45). However, other nondominant mutants unable to bind DNA were mapped closer to the C terminus (residues 239-291), thus suggesting that DNA binding required some multimerization through a different protein domain (1). In addition, a variety of noninducible NahR mutants were found within the region 126-206 that were still competent for DNA binding (9). This central region overlaps also with mutations that led to a constitutive, effector-independent behavior (mapping between residues 99-253; Ref. 21). These data, however, said little on whether salicylate interacts directly with the protein and, if so, which parts of the regulator are involved in such an interaction. In this work, we show that mutations that clearly alter the effector profile of NahR and affect its affinity for aromatic inducers map recurrently at distict sites of the regulator (Fig. 2). This provides an strong genetic evidence that these sites are engaged in effector binding during the earlier steps of the process leading to transcriptional activation of the Psal and Pnah promoters.
NahR mutants type I and the very related variant NahR7 appear to be genuinely affected in residues that participate in inducer recognition, because they show an altered effector specificity without any other detectable phenotypic change. Mutants NahR4 and NahR7 are particularly meaningful in this respect. As shown in Table III and Fig. 3, NahR4 appeared to gain the ability to respond to benzoate in a fashion that seemed to affect only the OH substituent at position C-2 of salicylate. On the contrary, NahR7 gained a remarkable ability of induction by salicylamide, suggesting that the protein residue(s) interacting with the otherwise essential carboxyl group of salicylate have also undergone some change. Mutant NahR3 seems, on the other hand, to increase its general reponsiveness to virtually all salicylate analogs examined, which may reflect a flexibilization of the effector pocket in NahR but not so much the change of a residue directly involved in effector recognition. Finally, mutants type II pinpoint the pivotal role of amino acid 116 in both effector recognition and NahR activation. That the mutations in this residue lock the protein in an intermediate activation step is indicated by the degree of inducer-independent activity observed. But that the 116 residue may also participate in interactions with the carboxyl group of salicylate is suggested by the observation (Table III) that the changes M116I and M116V make the proteins respond to salicylamide, whereas M116T does not. A number of amino acid residues critical for effector binding are therefore placed in a protein segment not larger than 60 amino acids, spanning positions 116 and 169. However, the contribution of more distant locations (i.e. 248) cannot be ruled out. These conclusions generally fit those found in the OccR protein of Agrobacterium tumefaciens, another archetypical LTTR, in which mutations within the central portion of OccR (F113L and G148D) increased the affinity of the protein for its natural effector, octopine (8). Ours is, however, the first case reported of single mutations within an LTTR that alter the effector profile of a protein of this type.
It would be highly speculative to draw structural or mechanistic
conclusions from the data presented in this work. However, the
remarkable similarity (approximately 50%) between two segments present
in NahR and NodD proteins (residues 140-200 and 207-266; Ref. 3)
allows some considerations. These two regions, which include NahR
variants N169D and R248C, span a potential -turn-
motif in NodD
that might be a ligand-binding crevice (1, 22). In fact, segments
109-171 and 189-216 of NodD resemble a consensus steroid-binding
domain, thus suggesting an involvement in effector binding (22).
Furthermore, residue 248 of NahR, which is mutated in variant
nahR3, is located within a region conserved in many LTTRs
that could be involved in multimerization (1). Perhaps the protein
segment around 248 links effector binding to a multimer conformation
shift that leads to activation, as has been suggested for CysB
(23).
The ease for obtaining variants with novel effector specificities makes NahR a system of choice for the generation of proteins responsive to predetermined aromatic molecules, a task of considerable interest for biotechnological applications (19, 24-27). In fact, the proneness of NahR to mutate to forms with a broader effector specificity might not be alien to the fact that LTTRs are frequently found as regulators of bacterial operons for biodegradation of xenobiotic compounds (28), the assembly of which requires a very fast protein evolution (29). This is true also for the NodD proteins of rhizobia, another well known case of LTTR, which are necessary for specific interactions with plants (5). NodD proteins must interact with similar DNA targets (the so-called nod boxes) in response to an array of flavonoid derivatives present in the plant exudates. The sequences available from various NodD proteins indicate that the ability to recognize novel flavonoids resides in the divergence of the amino acid sequences of the central protein domains (4, 30). This substantiates the notion that changes within a few amino acid residues in LTTRs give rise to repertoires of regulators responsive to chemical signals that become instrumental for transcriptional control of many different genes or operons along evolution (29).
We are indebted to M. Schell for various materials used in this study.