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Department of Physics of Complex Systems, The Weizmann Institute of Science, Rehovot 76100, Israel; and * Department of Molecular Genetics and Biotechnology, The Hebrew University-Hadassah Medical School, Jerusalem 91010, Israel
Correspondence: Address reprint requests to Joel Stavans, Dept. of Physics of Complex Systems, The Weizmann Institute, Rehovot 76100, Israel. Tel.: 972-8-9342615; Fax: 972-8-9344109; E-mail: joel.stavans{at}weizmann.ac.il.
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ABSTRACT |
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 TOP ABSTRACT INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGEMENTSREFERENCES |
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-DNA-H-NS complexes show that these adopt more extended configurations compared to the naked DNA substrates. Crosslinking indicates that H-NS can decorate DNA molecules at one H-NS dimer per 15–20 bp. These results suggest that H-NS polymerizes along DNA, forming a complex of higher bending rigidity. These effects are not observed above 32°C or at high osmolarity, supporting the hypothesis that a direct H-NS-DNA interaction plays a key role in gene silencing. Thus, we propose that H-NS plays a unique structural role, different from that of HU and IHF, and functions as one of the environmental sensors of the cell. |
INTRODUCTION |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGEMENTSREFERENCES |
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; Trun and Marko, 1998). A dozen DNA-binding proteins known as histonelike proteins serve as a dynamic scaffold for nucleoid organization (Drlica and Rouviere-Yaniv, 1987). In Escherichia coli, it was shown that the relative concentration of the various nucleoid-associated proteins changes as the cells enter the stationary phase of growth (Azam et al., 1999). One of the major nucleoid proteins, the histonelike nucleoid structuring protein (H-NS; see Ussery et al., 1994; Williams and Rimsky, 1997), is an abundant protein, present at 
20,000 copies in exponential phase. The H-NS protein is structurally unrelated to histones. It does not exhibit high affinity for specific sequences but binds preferentially to intrinsically curved DNA and A+T-rich sequences (Dame et al., 2001; Rimsky et al., 2001). Cyclization experiments suggest that H-NS can bend DNA upon binding (Spurio et al., 1997). It was claimed that H-NS compacts DNA strongly (Spassky et al., 1984). Recent atomic force microscopy (AFM) observations have suggested a mechanism of lateral compaction based on H-NS-induced bridging of distal DNA segments along the same molecule, in a hairpin configuration (Dame et al., 2000, 2001). In contrast, when H-NS is present at high concentration, electron microscopy suggested that H-NS coats long DNA substrates end-to-end with no appreciable compaction (Tupper et al., 1994). At low concentration, H-NS was shown to affect nucleoid structure by constraining negative supercoils of DNA in vivo and in vitro (Tupper et al., 1994). Thus the precise way by which H-NS participates in shaping nucleoid structure remains uncertain.
In addition to its role in nucleoid architecture, H-NS plays a pleiotropic role in bacterial response to environmental stimuli such as starvation, changes in pH, temperature, and osmolarity (Atlung and Ingmer, 1997; McLeod and Johnson, 2001; Williams and Rimsky, 1997). H-NS was found to affect gene expression in a number of different ways, as the expression of over 5% of the E. coli genes are affected in an hns mutant (Hommais et al., 2001). A remarkable property of H-NS is its ability to act in gene silencing, a mechanism requiring, in contrast to direct repression, a high affinity H-NS binding site located at a distance from the promoter. Silencing by H-NS was recently demonstrated for gene clusters in pathogenicity islands (Bustamante et al., 2001; Falconi et al., 1998; Friedberg et al., 1999). Although the molecular basis for gene silencing is not known, it was suggested that H-NS could polymerize along DNA from the silencer region to the promoter (Caramel and Schnetz, 1998; Rimsky et al., 2001).
To shed more light on H-NS function and on its role in shaping nucleoid structure, we studied the elastic response of single twist-free DNA-H-NS complexes. Single -phage DNA molecules (16.5 µm long) tethering a magnetic bead to glass surface were stretched, in a solution containing H-NS, by an external magnetic field. The setup allows the direct measurement of the end-to-end extension of the nucleoprotein complex as a function of the stretching force. This experimental approach offers a number of advantages. The DNA molecules, attached both to bead and glass substrate by single bonds, are free to fluctuate and swivel, supporting no torsion. Furthermore, the DNA-H-NS complexes are in thermodynamic equilibrium with the protein solution, allowing H-NS to bind and dissociate from DNA unhindered. These features are particularly important for studying weak nonspecific protein-DNA interactions that are difficult to study by most molecular biology techniques.
We find that at physiological concentrations, H-NS-DNA complexes assume extended configurations that on average are twofold larger than bare DNA. This is in stark contrast to the effects of two other important nucleoid-associated proteins, IHF (Jaffar Ali et al., 2001) and HU (Schnurr et al., unpublished results). In addition, crosslinking experiments indicate that H-NS is associated in very large numbers with DNA. These findings suggest a picture in which massive polymerization of H-NS on DNA, covering extended tracts, increases DNA stiffness. This picture is consistent with H-NS participation in gene silencing as has been recently proposed (Rimsky et al., 2001). Interestingly, we find that in this purified system one can reproduce the temperature and osmolarity response of H-NS in vivo. Thus it appears that H-NS can act directly as a high-resolution temperature and osmolarity sensor in the control of gene expression.
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MATERIALS AND METHODS |
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-phage DNA labeled at the right and left ends with biotin and digoxigenin, Dig (Roche Molecular Biochemicals, Indianapolis, IN), with 2.8 µm M280 magnetic tosyl-activated beads (Dynal, Lake Success, NY) coated with anti-digoxigenin and passivated with 
-casein, respectively. Labeling was achieved by hybridizing and ligating bare -phage DNA (Roche Molecular Biochemicals, Indianapolis, IN) with labeled complementary DNA oligomers. H-NS purification was carried out with minor modifications of existing protocols (Dersch et al., 1993).
Sample cells
Cells for DNA elasticity measurements have already been described in detail (Jaffar Ali et al., 2001). In brief, samples were prepared in capillaries of square cross section (Vitro Dynamics, Rockway, NJ), which were washed first in a NH4:H2O2:H2O solution (1:1:5), rinsed in H2O for 10 min, and dried. The inner surface of each capillary was then made hydrophobic by soaking in Sigmacote (Sigma-Aldrich, St. Louis, MO), and rinsed in both ethanol and H2O. Next, the capillary was coated with BSA-biotin (Sigma-Aldrich) (incubation for 2 h at 37°C), followed by incubation with streptavidin for 2 h at 37°C. DNA-bead constructs in casein buffer (CB: 10 mM Tris-HCl, 200 mM KCl, 5% DMSO, 0.1 mM EDTA, 0.2 mg/ml -casein, pH 8.0) were then introduced and incubated at room temperature, to allow for enough constructs to bind to the lower inner side of the capillary.
Force measurements and optical setup
Samples containing -DNA-tethered magnetic beads were observed by bright-field illumination using a home-built inverted microscope. Extension-force measurements were made by using a magnetic force technique (Jaffar Ali et al., 2001; Strick et al., 1996). In brief, a vertical magnetic force stretching the tethering DNA molecule was applied on a bead by means of a pair of magnets, whose height could be controlled accurately. The vertical force F was obtained from measurements of the bead's Brownian motion transverse to the direction of the force, using the equipartition theorem: F/L = kBT/
X2
. Here, L is the extension of the tether, X2 representing an average over the square of the bead transverse displacements; T is the temperature; and kB is Boltzmann's constant. The extension L was measured by correlating the bead's image with a library of images taken of the same bead-DNA construct, when stretched by a large force (>10 pN) to prevent large fluctuations in the longitudinal z direction. The images in the library were obtained at different foci separated by a known amount over a range of 20 µm. The reproducibility of force-extension curves was checked by making measurements on five different -DNA molecules for each H-NS concentration.
Data processing and analysis
The extension of -DNA molecules was measured by the following procedure: the center of the first bead image in an experimental run and the center of all the bead images in the library were initially determined. The radial intensity profiles of the bead image and those in the library were then calculated. Next, the radial intensity profile of the bead image was correlated with the profiles corresponding to each image in the library. The bead height was determined by performing a parabolic fit around the maximum of the correlation, as a function of the height corresponding to each library image. The height value corresponding to the maximum of the fit was then defined as the bead height. This procedure was repeated for each image in an experimental run after the first, calculating the correlation only with images in the library corresponding to small differences in height relative to the previous image in the experimental run. We estimate the error in our measurements at 1% of the total length, or 150 nm.
DNA digestion
Reaction mixtures, 20 µl, in buffer (50 mM NaCl, 10 mM Tris-HCl pH 7.9, 10 mM MgCl2, 1 mM DTT) containing 0.5 µg of -DNA was incubated with the restriction enzyme Sau3A (New England Biolabs, Beverly, MA) in the absence or presence of H-NS at a concentration of 1 µM for 30 min. The DNA fragments were separated on 1% agarose gel and visualized with ethidium bromide.
Density gradient centrifugation of H-NS-DNA complexes
These experiments were carried out as described previously (Jaffar Ali et al., 2001) with the following modifications: formaldehyde and sarcosyl were omitted during the run. Centrifugation was carried out at 32,000 rpm for 64 h.
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RESULTS |
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twofold increase in end-to-end extension. This increase is not a result of an H-NS-induced change in the contour length of DNA as in the case of RecA (Hegner et al., 1999; Leger et al., 1998; Shivashankar et al., 1999). No hysteresis was observed upon repeated extension-retraction cycles. After elasticity measurements were completed, flushing with buffer without H-NS led to the recovery of the elastic behavior of naked DNA. Furthermore, addition of poly(dI-dC), a nonspecific competitor, eliminates all H-NS effects (data not shown). These results suggest that H-NS can bind to DNA with low specificity.
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-DNA, we measured the shift in buoyant density of the H-NS-DNA complexes. Radioactively labeled -DNA was incubated with H-NS, crosslinked with formaldehyde to prevent dissociation, and resolved by equilibrium density centrifugation in CsCl gradients. Without H-NS, the radioactively labeled DNA appears as a sharp band overlapping with marker unlabeled -DNA (Fig. 2 A). In contrast, nucleoprotein complexes formed in the presence of H-NS (Fig. 2 B) appear in a wide distribution of densities, indicating the predominance of complexes with a large number of H-NS molecules. We estimate the number of H-NS dimers per -DNA to be 2500–3200, equivalent to one H-NS dimer per every 15–20 bp. To obtain an indication whether H-NS is uniformly distributed along the DNA, the DNA was subjected to cleavage by the restriction enzyme Sau3A that recognizes 116 GATC sites along -DNA. The results show that in the absence of H-NS, discrete bands are easily discerned in the range 1–3 kbp. The addition of H-NS greatly inhibits digestion by the enzyme and most of the discrete bands disappear (Fig. 3) (the same pattern was seen under low UV exposure).
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; Bustamante et al., 1994), with an associated effective persistence length lp. This quantity is an unknown function of the (small-scale) persistence lengths of naked DNA tracts, tracts fully covered by H-NS, their number and spatial distribution. We show fits to the elasticity data using the worm-like chain model in Fig. 1. We determined from the fits values of lp characterizing complexes at different H-NS concentrations. The persistence length increases, as a function of H-NS concentration, reaching a value of 130 nm at the highest concentration measured, nearly threefold that of naked DNA (Fig. 4). In comparison, this ratio lies between 4 and 15 for RecA-DNA filaments (Hegner et al., 1999; Leger et al., 1998; Shivashankar et al., 1999).
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0.5 µM. Replacement of KCl by NaCl resulted in the same behavior shown in Fig. 2 A (data not shown), demonstrating that H-NS responds to both ions. Since our DNA substrates support no torsion, the attenuation of H-NS effects we observe at high osmolarity is not a result of changes in the supercoiling level of the substrate, but to H-NS-DNA interactions directly. These results are consistent with the inhibitory effect of H-NS observed on transcription of the proV gene at 50 mM KCl, the relief of inhibition at 200 mM KCl (Ueguchi and Mizuno, 1993), and with gel retardation and fluorescence analysis of H-NS-DNA complexes (Tippner and Wagner, 1995). The effects of temperature on H-NS-DNA complex formation was investigated by elasticity measurements in the range 23°C to 37°C at low osmolarity (Fig. 5). Remarkably, lp decreases monotonically with increasing temperature. A change of 5–7°C is sufficient to abolish most H-NS function. At 37°C, the full force-extension curves of naked DNA and DNA in the presence of a 2 µM solution of H-NS coincide within experimental error (inset, Fig. 5). Thus H-NS does not exert any effects on DNA conformation at high temperatures. Consistent with these data, H-NS was found to be ineffective in protecting DNA from digestion with Sau3A at 37°C (Fig. 3, compare lanes 4 and 5). Taken together, our experimental system appears to display similar signal response to that observed in vivo.
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DISCUSSION |
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), H-NS binds at AT-rich regions of high intrinsic curvature along the DNA backbone. These regions may serve as initiation sites for the polymerization of H-NS along the double-stranded tracts. Polymerization of H-NS on DNA has already been suggested by electron microscopy studies (Tupper et al., 1994). Without polymerization it would be impossible to account for the larger end-to-end extension of the nucleoprotein complex observed in our experiments. The overall length of double-stranded DNA covered by H-NS must be large enough to compensate for hairpin formation at curved sites. Furthermore, our measurements suggesting the polymerization of H-NS were obtained from experiments in which the H-NS-DNA complex is minimally perturbed. In contrast, direct methods of visualization such as EM (Tupper et al., 1994) and AFM techniques (Dame et al., 2000, 2001) involve larger perturbations of the H-NS-DNA complexes and are not mutually consistent. The large number of H-NS molecules interacting with DNA helps to explain the increased sedimentation behavior of H-NS-DNA complexes that was a major factor in assuming that H-NS compacts DNA (Spassky et al., 1984).
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; Renzoni et al., 2001; Smyth et al., 2000). It has been previously shown that a coiled-coil motif in proteins induces oligomer dissociation in response to increased osmolarity or temperature, suggesting that this region participates in the response of H-NS to high temperature and osmolarity. We propose that the changes in H-NS structure under these conditions prevents polymerization of H-NS along the DNA.
Our model is consistent with the proposed role of H-NS as a transcriptional silencer (Goransson et al., 1990). Curved sequences far away from a promoter serve as nucleation sites for H-NS polymerization, which extend up to the promoter, thereby inhibiting transcription. This situation may occur naturally in the downward regulating element (DRE) of the proU operon in Salmonella typhimurium. The DRE is 200 bp away from the site of transcription initiation. Sequences involved in H-NS-mediated silencing of the bgl promoter are also 200 bp away from the latter (Caramel and Schnetz, 1998). Only long insertions (
800 bp) between the nucleation site and the promoter disrupt silencing (Fletcher and Csonka, 1995). Thus the extent of polymerization around each nucleation site may be taken to be of the order of 200–500 bp, equivalent to 100–250 polymerization regions along the -DNA substrate. In agreement with this estimate, an analysis of high intrinsic curvature sites along the -DNA molecule which we have performed using the CURVATURE software, revealed 90–200 high curvature loci (Shpigelman et al., 1993).
Our studies and previous investigations provide a new perspective for the role played by H-NS in organizing nucleoid structure and its function. H-NS can nucleate on sites of intrinsic curvature, but can also polymerize along short stretches of DNA, increasing DNA rigidity, and leading to gene silencing. These stretches, located within regulatory regions are probably limited on one hand by nucleation sites from which polymerization is initiated, and on the other by roadblocks generated by DNA binding proteins. Our results demonstrate that H-NS alone does not lead to DNA compaction. In contrast to IHF, Fis, and HU, H-NS contributes more to the increased rigidity of small segments of the chromosome. One can only speculate about the implications this may have in nucleoid organization. A unique property of the bacterial nucleoid is its ability to respond rapidly to external input signals. Interestingly, the structure of the H-NS-DNA complex alone permits the nucleoid to respond, with high sensitivity, to changes in temperature and osmolarity, independent of additional host proteins and changes in DNA supercoiling.
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ACKNOWLEDGEMENTS |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGEMENTSREFERENCES |
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This research was supported by The Israel Science Foundation (grant 489/01-1), and the Minerva Foundation.
Submitted on September 24, 2002; accepted for publication December 4, 2002.
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REFERENCES |
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