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Common and Variable Contributions of Fis Residues to High-Affinity Binding at Different DNA Sequences
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     Department of Biological Sciences, University at Albany, 1400 Washington Avenue, Albany, New York 12222,Department of Chemistry, College of Staten Island and Macromolecular Assemblies Institute of the City, University of New York, Staten Island, New York 10314,Department of Chemistry and Chemical Biology, Rensselaer Polytechnic Institute, 110 Eighth Street, Troy, New York 12180

    ABSTRACT

    Fis is a nucleoid-associated protein that interacts with poorly related DNA sequences with a high degree of specificity. A difference of more than 3 orders of magnitude in apparent Kd values was observed between specific (Kd, 1 to 4 nM) and nonspecific (Kd, 4 μM) DNA binding. To examine the contributions of Fis residues to the high-affinity binding at different DNA sequences, 13 alanine substitutions were generated in or near the Fis helix-turn-helix DNA binding motif, and the resulting proteins were purified. In vitro binding assays at three different Fis sites (fis P II, hin distal, and attR) revealed that R85, T87, R89, K90, and K91 played major roles in high-affinity DNA binding and that R85, T87, and K90 were consistently vital for binding to all three sites. Other residues made variable contributions to binding, depending on the binding site. N84 was required only for binding to the attR Fis site, and the role of R89 was dramatically altered by the attR DNA flanking sequence. The effects of Fis mutations on fis P II or hin distal site binding in vitro generally correlated with their abilities to mediate fis P repression or DNA inversion in vivo, demonstrating that the in vitro DNA-binding effects are relevant in vivo. The results suggest that while Fis is able to recognize a minimal common set of DNA sequence determinants at different binding sites, it is also equipped with a number of residues that contribute to the binding strength, some of which play variable roles.

    INTRODUCTION

    Fis (factor for inversion stimulation) is the most abundant nucleoid-associated protein during the logarithmic growth phase in rapidly growing Escherichia coli cells (3, 6). However, during mid- to late-logarithmic growth, the intracellular levels of Fis decrease over 500-fold and become nearly imperceptible during the stationary phase. The impact of Fis on cell physiology is widespread. As a nucleoid-associated protein, it is able to interact with a large number of DNA sites to alter DNA topology (66, 67). Numerous genes are subject to positive or negative regulation by Fis directly or indirectly (6, 10, 19, 22, 30, 49, 56, 61, 73-75). In the case of the promoters rrnB P1 and proP P2, Fis binding to sites centered at positions –71 and –41, respectively, directly stimulates transcription by contacting the C-terminal domain of the RNA polymerase subunit (-CTD) (9, 43). In the case of the fis promoter (fis P), Fis binding to sites I and II, centered at positions +25 and –44, respectively, negatively autoregulates the fis operon by hindering RNA polymerase binding (6, 50, 58). As its name suggests, Fis also stimulates site-specific DNA inversion involving the Hin, Gin, and Cin family of recombinases (24, 32, 35). During Hin-mediated DNA inversion, Fis binds to two high-affinity DNA sites (hin-proximal and -distal sites) in a 60-bp recombinational enhancer region and interacts with two DNA-bound Hin recombinases to form a nucleoprotein complex intermediate required for efficient DNA strand cleavage and inversion (25, 33). Bacteriophage DNA excision from the E. coli chromosome is also stimulated by Fis by a mechanistically different process involving a high-affinity Fis binding site within attR (5, 51, 53, 71). In this case, Fis appears to play an architectural role by contributing to a higher-order nucleoprotein complex that facilitates DNA cleavage and excision (40). Thus, Fis participates in a variety of mechanistically different cellular functions in different nucleoprotein contexts.

    A fundamental property of Fis is its ability to bind and bend DNA. However, it is not yet known how Fis attains the specificity with the wide array of DNA-binding sequences that has been reported for this protein. Comparisons of a number of DNA sequences that are specifically bound by Fis have led to proposals for several consensus sequences (16, 17, 26, 28). However, these consensus sequences are somewhat degenerate, which permits substantial sequence variation. Previously, random mutagenesis showed that residues in the C-terminal helix-turn-helix (HTH) DNA binding motif were required for DNA binding because mutations in these residues reduced or abolished this function (38, 53). However, because many of the mutations resulted in changes that could potentially alter the local protein structure or interfere with DNA binding, the precise contributions of the mutated residues to DNA binding were unclear. Although crystal structures have been solved for Fis and for a number of Fis variants (12, 39, 63, 77, 78), a Fis-DNA cocrystal structure remains to be resolved. Several useful docking models have been proposed to explain the specific interactions between Fis and DNA (16, 55, 65, 72), but these models have been based on partial knowledge of residues mediating DNA binding and of the DNA sequence contributing to the binding affinity.

    In this work we present a more definitive characterization of the contribution of Fis residues to the binding affinity at different Fis binding sites. To this end, we created alanine substitutions at 13 locations in or near the HTH region and purified each of the mutant proteins. We determined the effects of these substitutions on the protein stability, the binding affinities to three different DNA sites in vitro, and the ability of Fis to function in vivo. These experiments gave both expected and unexpected results, which together showed that some Fis residues are crucial in achieving high-affinity binding to multiple DNA sequences, while others make variable contributions to DNA binding.

    MATERIALS AND METHODS

    Chemicals, enzymes, and growth media. Chemicals were purchased from Sigma-Aldrich, Fisher Scientific, Life Technologies Inc. (Gibco BRL), Pharmacia, or VWR Scientific. Enzymes were obtained from New England BioLabs, Inc., Promega Corp., or Roche Molecular Biochemicals. Radioisotopes were obtained from Amersham Biosciences. Oligonucleotides were generated with a Perkin-Elmer automated DNA synthesizer operated in the Department of Biological Sciences, State University of New York at Albany. Bacterial culture media were obtained from Difco Laboratories. Cultures were grown at 37°C in Luria-Bertani (LB) medium or were plated on LB agar or NZCYM medium as required (64). To select for drug resistance, 100 μg of ampicillin per ml, 50 μg of kanamycin per ml, and 75 μg of spectinomycin per ml were added to the growth medium as appropriate for each strain.

    Bacterial strains and plasmids. Strains used in this work are listed in Table 1. fis P repression activity was assayed in vivo using the lysogenic strain RO1046. To construct this strain, the fis promoter region from position –83 to position +5 (relative to the primary transcription start site) was fused to lacZ in plasmid pLF413, transformed into JM101, and recombined in RS45 as described previously (70). The recombinant phage was purified and used to lysogenize RJ1561 in order to make RO1046. The excision assay was performed with strain RJ1765, which is a thermosensitive lysogen of phage. The Hin-mediated DNA inversion assay was performed with E. coli strain RJ2539, which carries the hin invertible DNA segment from Salmonella enterica serovar Typhimurium fused to lacZ on the chromosome in the "OFF" orientation. Induction of fis from pET11c was performed in RO820, which is a DE3 lysogen (Novagen from EMD Biosciences) made in RJ1561.

    The plasmids used in this work are listed in Table 2. Fis mutants were engineered as described below and were used to replace the wild-type (WT) fis gene in pRJ807 in order to make plasmid pRJ950 (53), as well as plasmids pLF209, pLF252, pLF254, pLF256, pLF257, pLF259, pLF271, pLF307, pLF308, pLF352, pLF386, and pLF387. The various fis genes cloned in pRJ807-based plasmids were amplified by PCR and cloned into the T7 promoter-based pET11c expression vector (15) between the NdeI and BamHI sites to make pLF317, pLF318, pLF320, pLF321, pLF322, pLF326, pLF327, pLF328, pLF329, pLF330, pLF354, pLF355, pLF407, and pLF408. Three 23-bp DNA fragments containing 15-bp sequences for specific Fis binding sites were obtained by annealing complementary oligonucleotides and were cloned in the XbaI and SacI sites of pCY4 to create pLF234, pLF235, and pLF236. pRJ903 contains the attR Fis site immediately flanked on each side by 5 bp of natural sequence cloned into the BglII and SacI sites of pCY7 (53). Using pRJ1028 as the template, the fis P region from position –83 to position +5 was amplified by PCR and cloned in the SmaI site of pRJ800 to make pLF309 or in the EcoRI and SmaI sites of plasmid pRS415 (70) to make pLF413.

    Site-directed mutagenesis. Site-directed mutagenesis was performed using a two-step PCR megaprimer technique, as described previously (6). The first step consisted of a PCR performed with an oligonucleotide (5'-CGGAATTCATGTTCGAACAACGCG-3'; EcoRI site underlined) that annealed to the beginning of the fis gene, a downstream primer that annealed to fis and contained the desired fis mutation, and pRJ807 as the template. The resulting PCR product was used as a megaprimer in a second PCR along with another primer annealing downstream of fis (5'-CCCAAGCTTGCGGCACTGGAGATCG; HindIII site underlined) to generate the full-length fis gene plus an additional 390 bp of downstream sequence. The PCR products were purified, digested with EcoRI and HindIII, and cloned into the same sites in pRJ807 to replace the wild-type fis gene with a mutated variant. Each cloned fis gene was verified by DNA sequencing using Sequenase 2.0 and dideoxy nucleotides, as described by the supplier (USB Corp.).

    Purification of Fis mutant proteins. RO820 strains carrying the wild-type or mutant fis genes on pET11c-based plasmids were grown in LB medium at 37°C until the optical density at 600 nm was between 0.6 and 0.7, and then they were induced with 0.6 mM isopropyl--D-thiogalactopyranoside (IPTG) for 2 h at 37°C. Fis purification was performed by using a previously described procedure (53), which essentially involved phosphocellulose liquid chromatography of the crude cell lysate, ammonium sulfate precipitation, and precipitation by dialysis against low-salt buffer. For purification of Fis mutants R76A, R85A, R89A, K91A, K93A, K94A, and N98A, the NaCl concentration used to load the proteins on the cellulose phosphate column was decreased from 0.3 M (the concentration used for the wild-type Fis) to 0.2 or 0.1 M as needed to ensure column retention. K90A was not retained even at 0.1 M NaCl and was instead collected in the flowthrough. A subsequent Sephadex G-100 size exclusion chromatography column removed the bulk of the remaining contaminants from K90A Fis. The final preparation was dialyzed against storage buffer (500 mM NaCl, 20 mM Tris-HCl [pH 7.5], 0.1 mM EDTA, 50% glycerol) and stored at –20°C.

    Protein concentrations were determined using the Bio-Rad protein assay dye reagent (Bio-Rad Laboratories) with bovine serum albumin as the standard. Fis purity was determined by electrophoresis in 15% sodium dodecyl sulfate (SDS)-polyacrylamide-bisacrylamide (29:1) gels that were stained with SYPRO Red (Molecular Probes, Inc.). Gels were analyzed using a STORM 860 PhosphorImager set to the red fluorescence mode with a photomultiplier voltage of 850, and the relative intensities of bands within each lane were quantified using the ImageQuant software (Molecular Dynamics, Inc., Sunnyvale, CA). The Fis purity was factored into determination of the Fis concentration in each preparation.

    Thermal denaturation analysis. Fis protein samples (0.1 mg/ml in 0.1 M NaCl-20 mM NaPO4, pH 7.0) were subjected to various temperatures, at which the circular dichroism signal at 222 nm (far-UV circular dichroism) was collected, and the baseline value at 255 nm was subtracted. The ellipticity was measured as a function of temperature in at least two assays, and the experiments were individually fitted with a model of the heat-induced D22U equilibrium denaturation pathway using Kaleidagraph (Synergy Software) (44). The average midpoint denaturation temperatures (Tm) derived from the fits were used as indicators of relative protein stability.

    Gel electrophoretic mobility shift assays (GEMSA). DNA fragments (42 to 53 bp) carrying a specific Fis binding site were obtained by cleaving plasmids pLF234, pLF235, pLF236, pRJ903, and pJS482 with EcoRI and BamHI and labeling with [-32P]dATP using the end-fill reaction, and they were purified by polyacrylamide gel electrophoresis (64). Various amounts of purified Fis were mixed with approximately 1 fmol 32P-labeled DNA in 20 μl binding buffer (20 mM Tris-HCl [pH 7.5], 10 mM EDTA, 80 mM NaCl), incubated at room temperature for 10 min, and combined with 5 μl of loading buffer (20 mM Tris-HCl [pH 7.5], 10 mM EDTA, 80 mM NaCl, 100 μg/ml sonicated salmon sperm DNA, 7.5% Ficoll, 0.1% bromophenol blue). Samples were then loaded onto an 8% polyacrylamide-bisacrylamide (60:1) gel in TBE buffer (0.089 M Tris-borate [pH 8.3], 2.5 mM EDTA) with a 15-mA conducting current. The relative signal intensities were quantified by phosphorimaging. The percentage of bound DNA was plotted against the Fis concentration, and the concentration required to achieve 50% binding (which was not less than a 40-fold molar excess over the DNA concentration) was considered an experimental approximation of the Kd (apparent Kd). Since a fragment lacking a defined Fis binding site and two of the mutant Fis proteins (R85A and K90A) failed to produce a discrete bound complex, we measured the disappearance of the unbound DNA as a function of the Fis concentration to estimate Kd in these cases. A maximum concentration of 2.2 μM was used for several of the mutant Fis preparations since higher concentrations resulted in potential salt interference. This was not the case for WT Fis, which was purified and stored at much higher concentrations.

    To examine the effects of the flanking sequences on Fis-induced DNA bending at the attR site, pLF235 and pRJ903 were cleaved with BamHI or NheI to place the corresponding Fis binding sites near the end (BamHI) or near the middle (NheI) of a 413-bp (from pLF235) or a 424-bp (from pRJ903) DNA fragment and labeled with 32P as described above.

    fis P repression assay. RO1046 contains a lacZ fusion to the fis promoter region from position –83 to position +5 on the chromosome, which includes a single fis P II centered at position –44. RO1046 carrying pMS421 was transformed with pRJ807-based plasmids containing the wild-type or mutated fis genes and grown in LB medium in the presence of ampicillin and spectinomycin. Saturated cultures were diluted 75-fold in LB medium and grown for 90 min at 37°C, and then -galactosidase assays were performed as described previously (46). In these cells, uninduced Fis levels were sufficient to achieve about 4.5-fold repression of fis P. Repression activity was calculated using the following formula: 100 x (MUfis – MUMut Fis)/(MUfis – MUWT Fis), where MUfis is the -galactosidase activity (700 U) in the absence of Fis (RO1046 transformed with pRJ1122), MUWT Fis is the activity (154 U) in the presence of wild-type Fis (RO1046 transformed with pRJ807), and MUMut Fis is the activity in the presence of the mutant Fis.

    Hin-mediated DNA inversion assay. A lacZ fusion to the hin invertible DNA region was present in the E. coli chromosome of RJ2539 such that the promoter located in the invertible region was transcribed away from lacZ ("OFF" orientation) (29, 53). This strain expressed hin from plasmid pKH66 but lacked a functional fis gene, so that inversion was highly inefficient. In the presence of wild-type Fis expressed from pRJ807, DNA inversion occurred, the invertible region switched to the "ON" orientation, and lacZ was expressed. RJ2539 was transformed with pRJ807 or pRJ807-derived plasmids expressing one of the mutant fis genes and was grown in LB medium containing ampicillin and spectinomycin. Cultures were periodically plated on LB agar and LB agar containing ampicillin and spectinomycin to monitor the growth of total and transformed cells, respectively. Cultures reaching a concentration of about 2 x 109 cells/ml were diluted in the same fresh medium to continue growth. After 52 to 55 generations, samples were withdrawn for -galactosidase assays. Relative inversion activity was calculated using the following formula: 100 x (MUMut Fis – MUfis)/(MUWT Fis – MUfis), where MUWT Fis is the -galactosidase activity in the presence of wild-type Fis (from pRJ807), MUfis is the activity in the absence of Fis, and MUMut Fis is the activity in the presence of the mutant Fis.

    phage DNA excision assay. The pRJ807-based plasmids containing the wild-type or mutated fis genes were transformed into the cI857 lysogenic strain RJ1765. Thermoinduction of cI857 lysogens was performed as described previously (5, 53). Saturated cultures were diluted 30-fold in 6 ml of LB medium containing ampicillin and were grown in a shaking water bath at 32°C to an optical density at 600 nm of 0.6. The cultures were then shifted to 42°C for 30 min with shaking and then to 37°C for 2 h with constant aeration. After addition of 0.5 ml chloroform and vigorous vortexing, samples were centrifuged at 5,000 rpm for 10 min, and the supernatants were immediately titrated to determine the number of PFU per ml. Relative excision activities were obtained using the following formula: 100 x (PFU/mlMut Fis – PFU/mlfis)/(PFU/mlWT Fis – PFU/mlfis), where PFU/mlWT Fis is the number of PFU/ml in the presence of WT Fis (4.35 x 1010 PFU/ml), PFU/mlfis is the number of the PFU/ml in the absence of Fis (1.84 x 108 PFU/ml), and PFU/mlMut Fis is the number of PFU/ml in the presence of a Fis mutant.

    RESULTS

    Specificity of binding. Numerous DNA footprinting experiments (4, 6, 7, 11, 42, 54, 71, 77) demonstrated that Fis has definite binding preferences for specific DNA sites even when their sequences are weakly related (17, 26, 28). With increasing concentrations, Fis interacts with an increasing number of weaker DNA sites until binding becomes nonspecific (8, 67). However, distinctions between specific Fis-DNA interactions of various strengths and truly nonspecific interactions (i.e., interactions at random sites) have seemed vague. Here we examined the ability of Fis to interact with three known Fis sites (fis P II [6, 50, 58], hin distal [11, 33], and attR [5, 71]) and a nonspecific sequence (Fig. 1). Each of the Fis sites (15 bp) was placed at the center of a 42- to 44-bp DNA fragment and used in gel electrophoretic mobility shift assays with a range of Fis concentrations. The small DNA fragment minimized the potential for concurrent occupancy of alternative "weaker" Fis binding sites, which may be observed with much longer fragments. The results showed that binding to the DNA fragments carrying the fis P II or hin distal Fis sites occurred with equivalent apparent Kd values (Kd app) of about 1.0 nM, while binding to the fragment carrying the attR site occurred with a Kd app of about 4.1 nM. However, binding to the DNA fragment having flanking sequences similar to those of the previous three fragments but with a scrambled central sequence occurred with a Kd app of about 4.5 μM. Other 44-bp DNA fragments carrying no recognizable Fis binding sites have resulted in similarly high Kd app values (Shao and Osuna, unpublished results). Such a large difference in Kd app values, over 3 orders of magnitude (Kd ns/Kd sp), indicates that there is very high binding specificity at the fis P II, hin distal, and attR sites. The fourfold increase in the Fis concentration required for binding the attR site compared to the concentrations required for binding the fis P II and hin distal sites is far from the range observed for nonspecific binding and thus also represents highly specific binding.

    Generation, purification, and stability of Fis mutants. Alanine is an excellent helix former (52) that is not generally expected to cause significant disruptions in local structure or interfere with DNA binding. Thus, 13 residues in or near the HTH DNA binding motif were replaced with alanine, and the resulting mutants were purified (Fig. 2A and B). These residues were chosen on the basis of three criteria: (i) the results of previous random mutagenesis that pinpointed residues potentially involved in DNA binding (38, 53), (ii) examination of the Fis crystal structure (39, 63, 77) for solvent-exposed residues in the HTH region (Fig. 2A), and (iii) consideration of several proposed Fis-DNA docking models (16, 65, 72). On the basis of SDS-polyacrylamide gel electrophoresis, 10 of the proteins (including wild-type Fis) were purified to 95% purity or greater, and four (T75A, R85A, R89A, and K90A) were purified to within 70 to 90% purity (Fig. 2C). The three preparations with the lowest levels of purity (R85A, R89A, and K90A) resulted in poor or undetectable DNA binding to three different Fis sites (as discussed below) so that concerns about potential contributions to DNA binding by contaminants in these preparations were largely mitigated. In addition, when mixed with WT Fis, these preparations did not inhibit DNA binding (not shown).

    Circular dichroism-monitored thermal denaturation of WT Fis showed that the average midpoint temperature of denaturation was 63.5°C (Fig. 3), demonstrating that Fis is relatively stable at high temperatures. Mutations that significantly perturb intra- or intermolecular interactions can result in alterations in protein conformation or stability that can be detected by a change in the Tm. The Tm for Fis mutants Q74A, T75A, R76A, N84A, R85A, T87A, R89A, K90A, K93A, and N98A were within 6.5°C of that of WT Fis, suggesting that these mutations caused minimal disturbance to the local structure and stability. However, the Tm for mutants N73A, K91A, and K94A were about 14 to 16°C lower than that of the WT, suggesting that there were appreciable alterations in the local structure or stability.

    Fis residues required for binding to the fis P II site. Using GEMSA, we compared the mutant proteins to WT Fis in terms of the ability to bind the DNA fragment containing fis P II (Table 3). We found that Q74A, N84A, and N98A had a less-than-twofold effect on the binding affinity compared to WT Fis, suggesting that these residues are largely dispensable for binding this site in vitro. Moderate decreases in relative binding were seen with T75A (8-fold), R76A (10-fold), and K93A (20-fold). Greater effects were observed with N73A (47-fold) and K94A (37-fold). Even greater effects (>200-fold) were observed with R89A and K91A, which were located near the middle of the -D helix. The largest effects (>1,000-fold) were observed with R85A, T87A, and K90A, suggesting that these residues play the most critical roles in DNA binding. Of the five last mutants, only K91A exhibited a significant decrease in thermal stability (Fig. 3), suggesting that the drastic decreases in binding for the other four mutants could not be attributed to significant changes in protein structure or stability.

    We developed a repression assay using a fis P::lacZ fusion that relied on the ability of Fis to bind the fis P II site in vivo (Fig. 4A). A Western blot analysis of three separate cultures (data not shown) indicated that the levels of the Fis mutants were within twofold of the levels of WT Fis when they were expressed from pRJ807-derived plasmids. Only N73A and K94A fell outside this range, with about 10-fold decreases in protein levels compared to WT Fis. We compared the mutant Fis proteins to the WT in terms of their ability to repress fis P and expressed the results as percentages of repression (Fig. 4B). Overall, there seemed to be a good correspondence between the effects of the mutations on binding affinities to fis P II in vitro and fis P II-mediated repression activity in vivo. Indeed, if N73A and K94A were excluded, there was an exponential correlation (R = 0.98) between the two relative activities (Fig. 4C), demonstrating that the in vivo repression assay is sensitive to differences in apparent Kd values observed in vitro within 3 orders of magnitude.

    Fis residues required for binding at hin distal and attR sites. The 15-bp core sequences of the hin distal and attR sites differ from each other at nine positions and from fis P II at 5 and 10 positions, respectively (Fig. 1B). Given the high binding affinity of WT Fis at these sites, we asked whether DNA binding contributions made by the Fis residues examined in this work were similar at the three sites or if they varied substantially. Thus, we performed GEMSA with DNA fragments containing the hin distal or attR 15-bp core sequences and each of the 13 Fis mutants. While the effects of many of the Fis mutants on relative binding to the two sequences were roughly similar to the effects observed at fis P II within about a twofold range, some of the mutants exhibited greater variation (Table 3). Q74A had less than a twofold effect at fis P II and attR compared to WT Fis and about a 3.8-fold effect at the hin distal site; N98A had less than a twofold effect at all three sites. Moderate losses of DNA binding were observed with T75A (6- to 8-fold), R76A (6- to 10-fold), and K93A (9- to 20-fold). Larger and more variable effects were seen with N73A (22- to 65-fold), N84A (1.5- to 38-fold), and K94A (4- to 37-fold). The variable effects of N84A were particularly notable because they seemed to be negligible at the fis P II (Kd app, 1.5 nM) and hin distal (Kd app, 1.9 nM) sites but were substantial at the attR site (Kd app, 157 nM). The most severe effects were generally observed with R85A, T87A, R89A, K90A, and K91A, with R85A, T87A, and K90A consistently requiring concentrations in the range required for nonspecific binding at all three sites. The effect of R89A was more severe at the hin distal site (Kd, >2,200 nM) than at the fis P II site (Kd, 232 nM) or the attR site (Kd, 466 nM), and the effect of K91A was more severe at the hin distal and attR sites (Kd, >2,200 nM) than at the fis P II site (Kd, 247 nM).

    Effects of various flanking sequences. Because the DNA fragments carrying the fis P II, hin distal, and attR Fis sites all contained the same plasmid-derived flanking sequences (Fig. 1B), differences in their binding activities could be attributed to differences in their central 15-bp core sequences. However, it has been observed that flanking sequences can affect the extent of Fis-induced DNA bending angles by as much as 50° and, in some cases, can also alter the binding affinity by as much as threefold (55). We found that WT Fis exhibited a 12-fold increase in binding affinity at the attR Fis site when the core sequence was immediately flanked on each side by 5 bp of naturally occurring sequence followed by a plasmid-derived sequence ( attRnat), in contrast to an exclusively plasmid-derived sequence ( attRpd) (Table 4). GEMSA using circularly permuted DNA fragments greater in length than 400 bp showed that the Fis- attRnat complex caused a greater shift in electrophoretic mobility than the Fis- attRpd complex when the binding sites were near the center of the fragment but not when they where near the ends (Fig. 5). This suggests that the flanking sequences of attRnat are more conducive to a Fis-induced DNA bend than the sequences flanking attRpd.

    A greater DNA bend provoked by the flanking sequence may allow the DNA to wrap around the sides of Fis in order to facilitate additional Fis-DNA contacts in the flanking region. Contacts in the core-binding region might also be altered by conformational changes inherent in the highly bent complex. Thus, we examined the binding of each of the Fis mutants to DNA fragments containing attRpd or attRnat (Table 4). Relatively minor differences in binding affinities were observed between the two sites when R76A, N84A, R85A, T87A, K90A, or K94A was used in these assays. It is worth noting that N84A caused a substantial decrease in DNA binding at attR irrespective of the flanking sequence and that the DNA binding with R85A, T87A, and K90A was severely reduced, suggesting that the roles of these residues were not altered by the flanking sequence. N73A, T75A, and K93A exhibited close to twofold decreases in binding to attRnat compared to attRpd, despite the improved WT Fis binding at attRnat. Several improvements in the binding affinities were observed at attRnat compared to attRpd, the most dramatic of which was with R89A, which resulted in an apparent Kd of about 466 nM at attRpd and in an apparent Kd of about 12 nM at attRnat. Thus, it appears that the conformational change produced by the flanking sequence alters the DNA binding contributions of a subset of the Fis residues.

    Effect of Fis mutations on stimulation of DNA inversion and DNA excision in vivo. To evaluate the in vivo significance of the relative in vitro binding affinities of the various Fis mutants at the hin distal and attR sites, we examined their abilities to promote Hin-mediated DNA inversion and excision in vivo. We adapted a previously developed qualitative Hin-mediated DNA inversion assay (29, 53) (Fig. 6A) to obtain a quantitative -galactosidase-based assay that allowed us to measure the relative effects of the various Fis mutants on this process. The -galactosidase activity in RJ2539 transformed with pRJ807 increased in a growing culture until after about 50 generations, after which nearly maximal -galactosidase activity was observed (Fig. 6B). RJ2539 was then transformed with plasmids expressing each of the Fis mutants, grown for 52 to 56 generations, and analyzed for -galactosidase activity, which was considered a measure of the relative DNA inversion activity (Fig. 6C). In general, the results showed that there was good agreement between the effects on relative DNA inversion activity in vivo and the relative binding affinities to the hin distal site in vitro. With the exception of N73A, Q74A, and K94A Fis, a logarithmic correlation (R = 0.98) could be fitted to these relative effects (Fig. 6D), suggesting that the relative differences in DNA inversion activity could be largely attributed to the effects of Fis binding to the hin distal site (and probably also to the hin proximal site).

    Fis binding to a single site within attR (Fig. 7A) results in cooperative interactions with excisionase (Xis) bound at the X1 site (40) and works together with Xis, integration host factor (IHF), and integrase (Int) to stimulate excision of phage DNA from the chromosome (5, 37). Thermal induction of phage excision from the chromosome has been shown to generate a >200-fold increase in the resulting phage titer in the presence of Fis compared to the titer in its absence (5, 53), an effect that is abolished when the attR Fis site is mutated. Thus, we used the phage titer assay as an indicator of relative DNA excision frequencies stimulated by WT or mutant Fis.

    Thermoinduction of lysogenic strain RJ1765 resulted in about a 240-fold increase in the phage titer in the presence of WT Fis. When the same cells were transformed with the various pRJ807-related plasmids expressing our Fis mutants, a wide range of relative excision activities were observed (Fig. 7B). In this case, no overall correlation between the relative excision activities and relative attR site binding affinities could be clearly delineated (Fig. 7C). This may have been due in part to the cooperative interactions between Fis and Xis, which may have compensated for some of the DNA binding defects in Fis. Nonetheless, the effects of many of the Fis mutants on excision were compatible with their relative binding affinities to attR. For instance, the poor excision activities of N84A, R85A, T87A, and K90A were anticipated from their relatively poor DNA binding activities in vitro. T75A and K91A exhibited decreasing excision activities, which roughly mirrored their relative effects on attR binding. Because N73A and K94A were poorly expressed in vivo compared to the remainder of the Fis proteins, we cannot unequivocally interpret their seemingly poor abilities to stimulate excision. R89A resulted in phage titers that were higher than those of the WT. This effect may have been facilitated to a large degree by the substantial increase in R89A binding affinity to attR that was observed in the context of the naturally occurring flanking sequence (Table 4). R76A and K93A resulted in wild type-levels of excision activity despite the measurable reductions in DNA binding activities in vitro (Kd, 30 nM and 100 nM, respectively), suggesting that the excision reaction in vivo is able to accommodate certain deficiencies in DNA binding observed in vitro. However, Q74A and N98A resulted in significant reductions in excision activity despite their near-WT levels of DNA binding affinity and in vivo expression levels, suggesting that they play important roles in stimulating excision by providing a critical function other than DNA binding.

    DISCUSSION

    Specificity of Fis-DNA binding. Consistent with its role as a nucleoid-associated protein, Fis is able to interact with a wide range of DNA sequences (17). Poorly related sequences can be recognized with a remarkable degree of specificity. As observed in this work, Fis binds several different sites with Kd app values between 3 x 10–10 and 4 x 10–9 M, which are comparable to the values reported for other specific DNA-binding proteins, such as IHF, repressor, 434 repressor, and Fur (18, 41, 48, 76). When the match to the consensus sequence was obliterated, binding occurred with a Kd app of about 4.5 x 10–6 M, and the resulting bound complexes failed to form discrete bands during GEMSA, suggesting that nonspecific weak occupancy of DNA occurred at the high Fis concentrations. In addition, discrete bound complexes were not observed with R85A or K90A, and only a small fraction of bound complexes were observed with T87A even when these proteins were present at micromolar concentrations, suggesting that binding specificity was severely reduced in these mutants. Moreover, the in vivo repression activities were negligible, suggesting that specific recognition of fis P II in vivo was impaired. Hence, a difference in Fis concentration of more than 3 orders of magnitude distinguishes highly specific DNA binding from nonspecific DNA binding.

    We noted that highly specific DNA binding could easily be observed within a 12-fold range of binding affinity, such as that when WT Fis interacts with attRnat or attRpd. Moreover, K91A and R89A, which bind the fis P II site with Kd app values of 247 and 232 nM, respectively, to produce discrete band shifts similar to those of WT Fis, still exhibit more than a 10-fold increase in DNA binding affinity compared to nonspecific binding. K91A and R89A are capable of generating 30 to 50% of the maximum fis P repression activity in vivo (Fig. 4), a function that relies on specific binding to the fis P II site (50, 58). Thus, appreciable DNA selectivity may still occur in a range of DNA binding affinities of more than 2 orders in magnitude (e.g., with Kd app values ranging from 0.33 to 247 nM). This implies that multiple Fis-DNA complexes observed during GEMSA when large DNA fragments are bound with a range of Fis concentrations do not necessarily represent random DNA binding if the affinities are within 1 or 2 orders of magnitude of that for a highly specific Fis binding site.

    Cellular Fis protein levels have been estimated to vary from less than 50 to more than 25,000 dimers per cell during the first 75 min of outgrowth from the stationary phase in rich medium (6). Assuming that the average cell volume is about 1 μm3 (47), Fis concentrations can be estimated to vary from less than 80 nM to more than 40 μM during growth phase transitions. Changes in concentrations can be expected to switch the emphasis for the gamut of Fis-mediated processes from those that rely exclusively on highly specific DNA interactions (e.g., regulation of transcription and site-specific DNA recombination) to processes that rely on nonspecific interactions (e.g., alterations in DNA topology). Between these two extremes the chromosome exhibits a number of specific DNA binding sites with various affinities, which may be effectively occupied when proper intracellular Fis concentrations are generated. This provides an excellent opportunity for cells to control processes that rely on specific Fis binding to sites having relatively low or intermediate strength.

    Effect of alanine substitutions on protein stability. While most alanine substitutions had small or negligible effects on the thermal stability, the decreases in the Tm of about 14 to 16°C observed for N73A, K91A, and K94A suggest that these mutations appreciably altered the structure or stability of the protein. There is substantial evidence that there are strong preferences for certain N-cap residues located prior to the first residue in an helix, which help stabilize the helix by forming hydrogen bonds between their side chains and accessible backbone amines of N-terminal residues in an helix (14, 60, 69). Asparagine has been recognized as the most favorable N-cap residue, while alanine is a relatively poor one (14). Indeed, in the Fis crystal structure (39, 63, 77), the carbonyl oxygen in the side chain of N73 forms a hydrogen bond with the backbone amine of R76 in the -C helix, suggesting that N73 is an -C helix N-cap residue. This obscures interpretation of our finding that N73A results in 47- and 65-fold reductions in binding at the fis P II and hin distal sites, respectively, as these effects may be attributed in part or in whole to its -C helix stabilizing role. Our observation that N73A results in a more severe reduction in binding to attRnat than to attRpd may indicate an additional role for N73 in contacting the DNA backbone in the flanking region, particularly when its sequence is more conducive to DNA bending.

    The crystal structure shows that the side chains of K91 and K94 in the -D helix form intramolecular salt bridges with E59 and E52 in the -B helix, respectively. Thus, replacement of K91 or K94 with alanine should disrupt these putative salt bridges, which should decrease the Tm. Despite the similar effects of N73A, K91A, and K94A on protein stability, K91A resulted in a much greater loss of DNA binding affinity than N73A or K94A (Table 3), suggesting that K91 may also participate directly in DNA binding. In a growing number of DNA binding proteins, it has been observed that salt bridges formed near the DNA binding surface can become disrupted during DNA binding so that the cationic side chain can be free to interact with DNA (23, 57, 62). A similar process may occur with K91 in Fis. However, it is also possible that structural alterations caused by K91A affect the DNA binding capability of the neighboring K90 residue.

    Since the in vivo levels of N73A and K94A were considerably lower than those of the other mutant and WT Fis proteins, it was not surprising that their relative in vivo activities were lower than expected based on their relative DNA binding affinities. We previously observed that the P61A mutation, which decreases the stability of the C-terminal region, results in increased susceptibility to proteolytic cleavage (27). Thus, it is possible that structural disturbances caused by N73A and K94A in the C-terminal region also render Fis more susceptible to proteolytic attack in vivo.

    Fis residues required for DNA binding. A qualitative summary of the effects of Fis mutations on the relative binding affinities to the various Fis binding sites analyzed is shown in Table 5. In general, the -D helix residues R85, T87, R89, K90, and K91 were the most critical residues in achieving highly specific DNA binding. Of these, R85, T87, and K90 were consistently vital for highly specific binding at all sites examined, suggesting that they may have obligatory roles in achieving binding specificity at all Fis sites. A previously proposed docking model placed a hydrogen bond between the R85 side chain and the O6 position of the first G base (G1) in the 15-bp core sequence of the hin distal site and another hydrogen bond between the K90 side chain and N7 of the G base at position 12 (16, 55). This is in good agreement with the findings that (i) loss of R85 or K90 consistently abolished specific DNA binding, (ii) despite the poorly related sequences at Fis binding sites, G1 is the most highly conserved base and a purine (either of which provides the suggested N7 contact for K90) is conserved at position 12, and (iii) other solved protein-DNA structures involving HTH DNA binding proteins, such as lac repressor, Cro repressor, and CAP, have side chains at analogous positions in their recognition helices, forming hydrogen bonds with specific bases via the major groove (2, 36, 68). A threonine in the third position of the recognition helix in the lac repressor makes a phosphate contact in the operator region (36). T87 is in an analogous position in Fis and may thus play a similar role.

    Glutamine at the beginning of the HTH region is often found to contact a phosphate on the DNA backbone in other protein-DNA complexes (1, 2, 34), and asparagine at the carboxy-terminal end of Fis appears to come near the DNA backbone in docking models (16, 65, 72). Thus, it was somewhat surprising that Q74A and N98A had minimal effects on the binding affinities at all three sites, suggesting that these residues are not essential for DNA binding. The remainder of the residues examined (N73, T75, R76, N84, K93, and K94) contributed to various degrees to the binding affinity, depending on the residue and the Fis binding site (Table 5). These residues may contribute to the overall binding energy via DNA backbone interactions. The side chains of N73, T75, R76, and K93 extend toward the flanking DNA region or the boundary of the core region in docking models (16, 65, 72) and may be required for stabilizing a Fis-mediated DNA bend through contacts with the outer region of a Fis binding site (Fig. 8A and B).

    Variable contributions of N84, R89, and K91. The effects of N84A, R89A, and K91A differed considerably when different Fis binding sites were used (Table 5). These effects were also seen in vivo since N84A resembled WT Fis in the ability to repress fis P (Fig. 4) and stimulate Hin-mediated DNA inversion (Fig. 6) but was completely unable to stimulate DNA excision (Fig. 7). This is a remarkable finding because it suggests that Fis relies on a different subset of residues for contacting the attR site than for contacting the fis P II or hin distal sites. We noticed that the central sequence of the attR site forms an A6 tract that is not formed in the other Fis sites. This sequence, which has been shown in crystals to adopt a nonbent structure (13, 20, 21), may alter the local structure in the attR core region in order to both enable and require N84 contacts with the DNA backbone or a base. This exemplifies the agility of Fis in adjusting to different DNA sequences and structures to achieve high binding specificity.

    R89A was unable to bind to the hin distal or attRpd site but was able to bind weakly to the fis P II site and very efficiently to the attRnat site (Table 5). The relative effects of R89A in vivo were compatible with its DNA binding behavior: poor stimulation of DNA inversion (Fig. 6), moderate fis P repression (Fig. 4), and excellent stimulation of excision (Fig. 7). The latter effect suggests that interactions with attRnat more closely resemble interactions at the attR site in vivo than interactions with attRpd.

    Fis-induced DNA bending was enhanced at attRnat, where R89 was not essential, compared to attRpd, where R89 was essential. Docking models of the hin distal site place the R89 side chain near the boundary between the 15-bp core and the flanking sequence (16, 65, 72). It is possible that contacts between R89 and the core-flanking boundary are more critical when the flanking DNA is less prone to bending than when it is more easily bent. Flexible flanking DNA may come in contact with the sides of Fis to help stabilize the bound complex, even in the absence of R89. However, when the flanking DNA is less prone to bending, interactions with the flanking sequence are less likely and the complex relies strongly on R89-DNA contacts. Thus, while a role for R89 may not be imperative at all Fis binding sites, it may help salvage binding to numerous sites flanked by sequences not amenable to bending. In this sense, R89 may be seen to play an important role in broadening the scope of DNA sequences to which Fis may bind specifically.

    Contributions by the 15-bp core site and the flanking DNA sequences. The most important interactions are those between Fis and the 15-bp core region because sequence replacement in this region had the most severe effects on binding. The flanking sequence can also affect the binding affinity by as much as 12-fold and can affect the extent of Fis-induced DNA bending. A previous study showed that there was a 2.5-fold reduction in Fis binding to the attR site when its normal flanking sequence was replaced with that of the hin distal site (55). The attR flanking sequence resulted in increased Fis-induced DNA bending at both the attR and hin distal sites compared to that at the hin distal flanking sequence, but it did not increase the binding affinity at the hin distal site. Thus, the effects of the flanking sequence on the binding affinity seemed to be more pronounced when the interaction with the core sequence was weaker. We have noticed a similar tendency with other Fis core binding sequences (Shao and Osuna, unpublished results).

    In the CAP-DNA structure, two sharp DNA bends are produced by 40° kinks between TG-CA base pairs on each half-site, and the central region has an additional 8° bend that affects the DNA contact by a lysine residue (68). In the case of Fis, we envision a model in which the bound complex is able to achieve considerable stability when the core sequence confers optimal Fis interactions, even if interactions with the flanking region are inefficient (Fig. 8A). When a flexible flanking region facilitates a greater DNA bend, additional backbone interactions are possible in this region (Fig. 8B). The large conformational change can include smaller alterations in the structure of the central binding region that may suffice to alter certain interactions between Fis and the core-binding region. Putative weakening of contacts with the core region may be compensated for by additional contacts in the flanking region with minimal change in the binding affinity. In cases in which interactions with the core region are initially deficient, a flexible flanking region may result in a net increase in the binding affinity. A prediction from this model is that some residues should be essential only under conditions of limited DNA bending, which is what we observed with R89. On the other hand, N73, T75, and K93 stepped up their contributions to the binding affinity under conditions that facilitated DNA bending, an effect that should also be expected.

    Roles of Q74 and N98 in vivo. Q74A and N98A bound the fis P II, hin distal, and attR sites with affinities comparable to those of WT Fis. The fis P repression assay confirmed these observations. However, Q74A was considerably less efficient in terms of the ability to stimulate Hin-mediated DNA inversion (50% of wild-type levels) or excision (40% of wild-type levels). N98A showed normal stimulation of DNA inversion but was completely unable to stimulate excision (Fig. 6C and 7B). These results suggest that Q74 and N98 have an important function in vivo other than DNA binding during stimulation of excision or DNA inversion (in the case of Q74).

    Q74 has been implicated in protein-protein interactions between Fis and the -CTD of RNA polymerase at proP P2 and rrnB P1 (9, 43). Thus, it is plausible that Q74 may participate in contacting other proteins as well, such as the Hin recombinase during DNA inversion or Xis during DNA excision. Interestingly, N98 is located next to Q74 in the crystal structure (Fig. 8C). Therefore, N98 is similarly poised to participate in putative intermolecular interactions during DNA excision. Xis is an attractive candidate because it has been shown to bind cooperatively with Fis in the attR region (40, 71). Other possibilities that cannot be excluded at present include a role for one or both of these residues in achieving a sufficient degree of DNA bending required in these processes and a role in DNA binding required in the context of the chromosomal DNA, which can be altered by DNA supercoiling or DNA looping.

    Concluding remarks. The fact that most of the recognized sequences can be described by a degenerate consensus sequence implies that there is a minimally defined set of sequences that are recognized by Fis. This is mirrored by a minimally defined set of Fis residues (R85, T87, and K90) that are consistently critical in DNA recognition. The stability of the bound complex ultimately relies on the establishment of numerous additional DNA contacts. If, as imagined, the majority of these contacts are with the DNA backbone, then variations in binding affinity are highly influenced by the structure or flexibility of the core and flanking sequences. However, within limits, Fis is able to handle variations in DNA sequence or structure. The combinatorial effects of all these factors should contribute substantially to the variability of sequences recognized by Fis.

    ACKNOWLEDGMENTS

    We are grateful to Sara Boswell and Liye Zhang for assisting with thermal denaturation experiments. We also thank Meranda D. Bradley for helpful suggestions.

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