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Journal of Bacteriology, November 2006, p. 7354-7363, Vol. 188, No. 21
0021-9193/06/$08.00+0     doi:10.1128/JB.00637-06
Copyright © 2006, American Society for Microbiology. All Rights Reserved.

Switched or Not?: the Structure of Unphosphorylated CheY Bound to the N Terminus of FliM

Department of Chemistry and Biochemistry, University of California at Santa Barbara, Santa Barbara, California 93106

Received 4 May 2006/ Accepted 26 July 2006

	ABSTRACT

Top Abstract Introduction Dynamic excursions to the... Intermediate chey conformations. Materials and Methods Results Discussion References

 
Phosphorylation of Escherichia coli CheY increases its affinity for its target, FliM, 20-fold. The interaction between BeF₃^–-CheY, a phosphorylated CheY (CheYP) analog, and the FliM sequence that it binds has been described previously in molecular detail. Although the conformation that unphosphorylated CheY adopts in complex with FliM was unknown, some evidence suggested that it is similar to that of CheYP. To resolve the issue, we have solved the crystallographic structure of unphosphorylated, magnesium(II)-bound CheY in complex with a synthetic peptide corresponding to the target region of FliM (the 16 N-terminal residues of FliM [FliM₁₆]). While the peptide conformation and binding site are similar to those of the BeF₃^–-CheY-FliM₁₆ complex, the inactive CheY conformation is largely retained in the unphosphorylated Mg²⁺-CheY-FliM₁₆ complex. Communication between the target binding site and the phosphorylation site, observed previously in biochemical experiments, is enabled by a network of conserved side chain interactions that partially mimic those observed in BeF₃^–-activated CheY. This structure makes clear the active role that the ß4-4 loop plays in the Tyr⁸⁷-Tyr¹⁰⁶ coupling mechanism that enables allosteric communication between the phosphorylation site and the target binding surface. Additionally, this structure provides a high-resolution view of an intermediate conformation of a response regulator protein, which had been generally assumed to be two state.

	INTRODUCTION

Top Abstract Introduction Dynamic excursions to the... Intermediate chey conformations. Materials and Methods Results Discussion References

 
Two-component systems, composed of an autohistidine kinase and a phosphorylatable response regulator, are widely used in bacterial signal transduction. In Escherichia coli, the response regulator CheY controls the sense of rotation of the flagellar motor by switching between two stable states (CheY and phosphorylated CheY [CheYP]), enabling bacterial chemotaxis. CheYP interacts strongly with the flagellar motor switch protein FliM to effect a change in the motor rotational bias from counterclockwise to clockwise. Unphosphorylated CheY also interacts with FliM, though with substantially reduced affinity. Because residues on the FliM binding surface of unphosphorylated CheY (e.g., Tyr¹⁰⁶) would sterically block FliM from binding, the structural basis of the moderate affinity of unphosphorylated CheY for FliM remains unclear.

The structures of unphosphorylated, Mg²⁺-free CheY (apoCheY) (28) and CheY bound to the BeF₃^– phosphoryl analog (19) provide evidence that a network of conserved residues enables allosteric communication between the phosphorylation site (Asp⁵⁷) and the target binding site. Like phosphorylation, activation by the BeF₃^– phosphoryl analog requires a bound Mg²⁺ ion and causes a coordinated rearrangement of Tyr¹⁰⁶ and Thr⁸⁷ toward the active site, resulting in the burial of the Tyr¹⁰⁶ side chain and formation of an H bond between the Thr⁸⁷ hydroxyl and the phosphoryl group, termed Y-T coupling (19). Another rearrangement that characterizes the activation process is the reorientation of Lys¹⁰⁹ (which forms a salt bridge with Asp⁵⁷ in unphosphorylated CheY) to form a salt bridge with Asp¹² and one of the fluorine atoms of BeF₃^–, while Mg²⁺ binding alone also induces the Lys¹⁰⁹-Asp¹² salt bridge (4). The backbone conformation of CheY also changes in response to BeF₃^– activation, most notably at the ß4-4 and ß5-5 loops on the 4-ß5-5 surface (19), where FliM binds (20).

	Dynamic excursions to the active state.

Top Abstract Introduction Dynamic excursions to the... Intermediate chey conformations. Materials and Methods Results Discussion References

 
There exists a growing body of evidence that the unphosphorylated state of response regulators exists in dynamic equilibrium between inactive (unphosphorylated-like) and active (phosphorylated-like) conformations. Perturbations such as phosphorylation or mutation might then shift this equilibrium to favor the active conformation, giving rise to the notion of equilibrium shift activation (Fig. 1B). Here we imagine that the inactive conformation is favored in the absence of a ligand. The ligand binds more tightly to the active conformation and drives the equilibrium to favor the active conformation. Since the active and inactive conformations preexist, the idea that a bound ligand is not required to flip the conformational switch is fundamental to the equilibrium shift model. This is in contrast to the induced-fit model, where ligand binding and switching are concomitant (Fig. 1A). In this case the active conformation cannot be formed until the ligand is bound. It should be noted that although the original formulation of the Y-T coupling model includes no elements of equilibrium shift, the two models (Y-T coupling and equilibrium shift) are not mutually exclusive, as the equilibrating species could be coupled by the Y-T mechanism.

View larger version (13K): [in this window] [in a new window]   FIG. 1. Two views of activation: In the induced-fit model (A), ligand (M) binding results directly in conformational change, while in the equilibrium shift model (B), ligand binding serves to stabilize the active conformation, which preexists in a small fraction of the population prior to phosphorylation. Squares, inactive conformation; circles, active conformation.

	Intermediate CheY conformations.

Top Abstract Introduction Dynamic excursions to the... Intermediate chey conformations. Materials and Methods Results Discussion References

 
In the atomic resolution structure of apoCheY (i.e., CheY in the absence of Mg²⁺, phosphoryl group, or peptide ligand; Protein Data Bank accession no. 1JBE.pdb), there exist two roughly equally populated conformations of the ß4-4 loop and the Tyr¹⁰⁶ side chain (25). The authors of that study suggested that these sets of conformations are correlated and that one is the bona fide inactive conformation, which sterically blocks FliM, while the other, "meta-active" conformation is "responsible for the active properties seen in apoCheY" (25). As the authors point out, this structure does not support the equilibrium shift model, as the meta-active conformation is significantly different from the conformation of BeF₃^–-CheY. A physiological role for such intermediate species was recently demonstrated by the structures of CheY in complex with CheZ residues 200 to 214 (CheZ_C), in which CheZ_C-bound CheY is found in a partially switched conformation (11).

To more thoroughly map the regions of conformational space accessible to CheY in the absence of phosphorylation, we have solved the X-ray crystal structure of unphosphorylated Mg²⁺-bound CheY in complex with a 16-mer peptide corresponding to FliM₁₆ to 2.4-Å resolution. Analysis of the structure indicates that unphosphorylated CheY accommodates bound FliM₁₆ without switching to the canonical active conformation yet shares several features of the active conformation, perhaps most notably the complete burial of Tyr¹⁰⁶. Combined with the observations that a functionally important region (the ß4-4 loop) is stabilized by an interaction network that is unique to this complex, while another region (the 1 helix) remains in a distinctly inactive conformation, these results indicate that the energy landscape between the inactive and active conformations of CheY is more complex than previously thought.

Finally, this structure provides a molecular view of how allostery in CheY works in reverse, whereby the binding of FliM is coupled to conformational changes in the active site that affect phosphorylation (24). Whereas neither the Y-T coupling nor the equilibrium shift model of activation is completely consistent with the details of the CheY-FliM₁₆ complex, we discuss an alternate allosteric activation model that recognizes a role for the ß4-4 loop in signal propagation.

	MATERIALS AND METHODS

Top Abstract Introduction Dynamic excursions to the... Intermediate chey conformations. Materials and Methods Results Discussion References

 
Protein purification, crystallization, and data collection. E. coli CheY was overexpressed and purified using a previously described protocol (13). The FliM peptide (MGDSILSQAEIDALLN) was purchased from Macromolecular Resources (Fort Collins, CO) at 90% purity. The Mg²⁺-CheY-FliM complex crystallized in space group P2₁. To form the complex, a solution of 0.5 mM CheY and 10 mM Tris (pH 7.0) was slowly saturated with solid FliM peptide (10 mM). Diffraction quality crystals were grown by mixing 3 µl of this solution with 3 µl of well solution containing 30% polyethylene glycol 6000, 50 mM MES (morpholineethanesulfonic acid), and 50 mM MgCl₂, at pH 6.0 Crystals were grown in about 8 weeks at 4°C using the hanging-drop method. A single crystal was mounted in a 1-mm silanized glass capillary tube containing a reservoir of well solution to allow for room temperature data collection. Data collection took place at 24°C on an R-AXIS II (Molecular Structure Corporation) with CuK radiation. A total of 149 nonoverlapping degrees of data were collected, with a 1.0° oscillation range and an exposure time of 10 min. Because we did not find suitable cryoconditions, data were collected on two sections of the same crystal to minimize the effects of radiation damage. In the first orientation, 103° were kept. In the second orientation, 46° were kept, giving a total of 149°. Data were processed to 2.4 Å in space group P2₁ with MOSFLM (21) and scaled using SCALA (7).

Structure determination. Initial phases were determined by molecular replacement using the program EPMR (17) and Protein Data Bank entry 3CHY.pdb (28), with Tyr¹⁰⁶ modeled as alanine, as the search model. As suggested by the Matthews coefficient, EPMR found a solution with two CheY molecules in the asymmetric unit (R value of 0.36 using data to 3.0 Å). Electron density generated following anisotropic B-factor and bulk solvent correction (used throughout refinement) clearly showed the bound peptide and the buried orientation of the Tyr¹⁰⁶ side chain for both CheY molecules. Residues 5 to 12 of the two FliM₁₆ peptides as well as the Tyr¹⁰⁶ side chains were modeled into _A-weighted 2|F_o| – |f_c| and |F_o| – |f_c| maps. This model was refined against the complete range of data (40.7 to 2.40 Å) with multiple rounds of conjugate gradient least-squares minimization, torsion angle simulated annealing, and isotropic individual B-factor refinement using the program CNS (5) with noncrystallographic symmetry (NCS) restraints imposed on the two CheY molecules. Interspersed with rounds of refinement, manual adjustments to the model were performed using the program O (15), guided by _A-weighted 2|F_o| – |f_c|, |F_o| – |f_c|, and 2|F_o| – |f_c| composite omit maps. During the later stages of refinement, residues 13 to 16 and 2 to 4 of the peptides, two magnesium(II) ions (one per CheY), and 144 water molecules were modeled. Neither NCS restraints nor simulated annealing was used in the later refinement cycles. Residues 14, 27, and 88 to 90 of CheY chain A and residues 14, 17, 88 to 90, and 100 of CheY chain B are modeled as two conformations. The R and R_free values for the final model are 0.18 and 0.24, respectively. In Ramachandran space, 88.5% of residues are in the favored region, 9.5% are in the allowed region, 1.2% are in the generously allowed region, and 0.8% are in the disallowed region, due to the CheY Asn⁶² -turn (28). Data collection and refinement statistics are given in Table 1.

	RESULTS

Top Abstract Introduction Dynamic excursions to the... Intermediate chey conformations. Materials and Methods Results Discussion References

 
The refined structure contains two unphosphorylated Mg²⁺-bound CheY-FliM₁₆ complexes per asymmetric unit (Protein Data Bank accession no. 2B1J.pdb), which will hereafter be referred to simply as CheY-FliM₁₆. Electron density corresponding to residues 2 through 16 of the bound peptides (chains C and D, bound to CheY chains A and B, respectively) is unambiguous, though it is weak at the termini (Fig. 2). Met¹ of FliM₁₆ could not be located unambiguously, presumably due to disorder, and was not modeled. Met¹ of CheY is cleaved during bacterial overexpression and so was not modeled. Several features of the CheY-FliM₁₆ complex are reminiscent of the BeF₃^–-CheY-FliM₁₆ complex: the Tyr¹⁰⁶ side chain is exclusively buried, the Ile⁹⁵ C 1-methyl group is oriented toward the phenyl ring of Tyr¹⁰⁶, Lys¹⁰⁹ and Asp¹² side chains form a salt bridge, and Asn⁵⁹ is oriented toward the ß4-4 loop. Similarly, Thr⁸⁷ is sequestered toward the active site, and the ß4-4 and ß5-5 loops have undergone conformational changes relative to apoCheY that are similar in direction to, yet smaller in magnitude than, those changes observed in the BeF₃^–-CheY-FliM complex (Fig. 3 and 4).

View larger version (74K): [in this window] [in a new window]   FIG. 2. Electron density and structural model corresponding to FliM16 (chain C, green) bound to unphosphorylated Mg2+-CheY (chain A, tan). The displayed electron density is a|Fo| – |fc|-simulated annealing omit map generated with chain C omitted in the program CNS. In order to display the weak density at the peptide termini, the map has been contoured at 3.6 around the entire peptide (cyan, fine mesh, residues 2 to 16) and at 2.4 around the peptide termini (purple, coarse mesh, residues 2 to 5, 15, and 16).

View larger version (26K): [in this window] [in a new window]   FIG. 3. Displacements of the C atoms of several CheY conformations following a least-squares overlay with inactive CheY (3CHY) are shown for all residues (A) and residues in and around the ß4-4 loop (B). The CheY conformation in the CheY-FliM16 complex (heavy line, Protein Data Bank accession no. 2B1J) is intermediate between that of apoCheY (lower line) and the BeF3–-CheY-FliM16 complex (light upper line, Protein Data Bank accession no. 1F4V). The mean displacements of chains A and B of the CheY-FliM16 complex are shown. Displacements associated with the meta-active apoCheY substructure are also shown (dashed black line, Protein Data Bank accession no. 1JBE).

View larger version (80K): [in this window] [in a new window]   FIG. 4. The superimposed structures of the CheY-FliM16 complex (chain A is in dark blue and chain B is in light blue; Protein Data Bank accession no. 2B1J), apoCheY (red; Protein Data Bank accession no. 3CHY.pdb), and the BeF3–-CheY-FliM16 complex (green; Protein Data Bank accession no. 1F4V) are shown for the -4 loop, Thr87, and Tyr106 (A), the ß4-4 loop and Asn59 (B), and the ß5-5 loop and the 1 helix (C). In panel B, the hydrogen bond formed between Gly89 and Asn59 (dashed line; chain B, subconformation b) is similar to the association between these residues in the BeF3–-CheY-FliM16 complex. In panel C, the 1 helix of the CheY-FliM16 complex, which remains in the inactive conformation (see Fig. 3), is omitted for clarity. (D) A previously unobserved conformation of Glu89 in the ß4-4 loop of the CheY-FliM16 complex (chain A) is stabilized by hydrogen bonds with Asn94 and Tyr106 (dashed lines). All structures were superimposed onto inactive CheY (3CHY).

The two CheY molecules in the asymmetric unit are NCS related yet are not identical; chain B has more "active character" than does chain A, as shown in Fig. 4. However, because the differences are small (<1 Å), occur primarily in loop regions, and may arise from different constraints placed on the two complexes within the crystal, they will not discussed in detail here.

Details of the CheY-FliM₁₆ interface. In complex with Mg²⁺-CheY, the conformation of FliM₁₆ is similar to that observed previously in the BeF₃^–-CheY-FliM₁₆ (20) and CheY**-FliM₁₆ (8) complexes; residues 2 through 7 are in an extended conformation, and residues 8 to 14 form two helical turns. Additionally, the amount of surface area that is buried in the CheY-FliM₁₆ interface is similar for the three complexes (1,075 Ų for unphosphorylated CheY-FliM₁₆, 1,110 Ų for BeF₃^–-CheY-FliM₁₆, and 991 Ų for CheY**-FliM₁₆). For residues 6 to 12, details of the interactions that stabilize the conformation of FliM₁₆ and anchor it to CheY are very similar to those described previously (8, 20) and will not be described in detail here. In contrast, the termini (residues 2 to 5 and 13 to 16) of FliM₁₆ in complex with Mg²⁺-CheY differ from those in the previously determined BeF₃^–-CheY-FliM₁₆ and CheY**-FliM₁₆ structures. The ß-sheet-like interaction between residue 4 of FliM and residue 90 of CheY is not formed in one of the NCS-related complexes (chains B and D), and in the other complex (chains A and C) it takes place at a substantially farther distance (3.3 Å, versus 2.6 Å for BeF₃^–-CheY-FliM₁₆). Additionally, the salt bridge between Asp³ of FliM₁₆ and Lys⁹¹ of CheY is not formed in the unphosphorylated Mg²⁺-CheY-FliM₁₆ complex. At the C terminus of FliM₁₆, residues 13 to 16 are arranged much less tightly about the helical axis than has been seen in previous structures (i.e., the backbone unwinds somewhat), which displaces the bulk of Asn¹⁶ away from the CheY backbone at Tyr¹⁰⁶, preventing the Asp¹⁶ side chain from contributing to the H bond network that anchors FliM₁₆ to ß-sheet 4 of CheY (see Fig. 4 in reference 8). Additionally, the salt bridge between Lys¹²² N and the FliM₁₆ C-terminal carboxylate is replaced by an H bond between Lys¹²² N and the Asn¹⁶ side chain carbonyl. High B-factors for the C-terminal residues of FliM₁₆ are consistent with the loss of previously observed stabilizing interactions.

The loss of several previously observed intermolecular contacts in the CheY-FliM₁₆ interface is consistent with the reduced affinity of FliM for CheY relative to CheYP. The observed perturbation of contacts between CheY and the N-terminal region of FliM₁₆ appears to result largely from the inability of the ß4-4 loop to adopt a fully active conformation in the CheY-FliM₁₆ complex (Fig. 4A). Clearly this result does not support the equilibrium shift view of activation, which supposes that CheY and CheYP interact identically with FliM.

The ß4-4 loop. The ß4-4 loop (Thr⁸⁷ to Lys⁹¹) following Thr⁸⁷ is found in a conformation that approximates that of BeF₃^–-CheY, though to different degrees for the two NCS-related complexes. Whereas BeF₃^– activation results in a 3.5-Å shift at the Glu⁸⁹ C relative to apoCheY, in chain A of the CheY-FliM₁₆ complex this position is displaced from its inactive position by 1 Å, while in chain B the shift is larger (2 Å) though still less than that observed for the BeF₃^–-CheY-FliM₁₆-complex (Fig. 4A). Additionally, residues 88 to 90 are modeled as two equally populated conformations in both CheY-FliM₁₆ complexes, largely to accommodate two conformations of the Glu⁸⁹ side chain. Therefore, it appears that this loop has a significant degree of conformational freedom in the CheY-FliM₁₆ complex. Besides being in a position intermediate to the that of apoCheY and BeF₃^–-CheY, it should be noted that the four loop subconformations we observe (two per CheY) are each distinct from that of meta-active CheY, where the largest displacement (relative to the 1.7-Å apoCheY structure, which did not model static disorder in the ß4-4 loop) are at Ala⁹⁰ (Fig. 3B). Incidentally, two of the subconformations of the ß4-4 loop that we observe (present in chain A and chain B) are stabilized by H bonds between the Glu⁸⁹ carboxylate side chain and the Asn⁹⁴ side chain amide and Tyr¹⁰⁶ side chain hydroxyl, giving the Glu⁸⁹ side chain the previously unobserved ability to make van der Waal contact with Thr⁸⁷ (Fig. 4D).

The 1 helix remains unswitched. The 1 helix of unphosphorylated Mg²⁺-CheY in complex with FliM₁₆ does not undergo conformational change relative to apoCheY (Fig. 3). Conversely, backbone atoms in the 1 helix experience some of the largest displacements (>2 Å) when active (e.g., BeF₃^–-CheY, BeF₃^–-CheY-FliM₁₆, or CheY**-FliM₁₆) and inactive (e.g., apoCheY, Mg²⁺-CheY, or CheY** alone) CheY structures are compared (Fig. 3; see also Fig. 1 in reference 8). In contrast to the case for wild-type CheY, FliM₁₆ binding (in the absence of Mg²⁺ or a phosphoryl analog) is sufficient to flip the conformational switch in this region of CheY**.

Thr⁸⁷ is partially switched and disordered. Due to its role in phosphorylation/dephosphorylation chemistry, position 87 (or its equivalent) is highly conserved as a small hydroxyl-containing residue (Ser or Thr) in the response regulator protein superfamily. One feature of the CheY-FliM₁₆ complex that is particularly confounding is the intermediate position and weak electron density of the Thr⁸⁷ side chain, since this residue is well ordered in other CheY structures. The disorder at this position is evidenced by high side chain B-factors, which are not observed for the Thr⁸⁷ side chain in other CheY structures or for buried residues generally. Because static disorder in this region prompted us to model two conformations of the ß4-4 loop (Fig. 4A), at several points during refinement dual conformations of Thr⁸⁷ (backbone and side chain) were modeled and subjected to rounds of refinement. However, because these efforts led to increased R_free values and no apparent improvement in the quality of the Thr⁸⁷ side chain electron density, they were abandoned in favor of a single Thr⁸⁷ conformation. We imagine that, similar to the ß4-4 loop, Thr⁸⁷ in the CheY-FliM₁₆ complex has significant conformational freedom, though we cannot rule out the possibility that it takes on two closely spaced static conformations in different unit cells of the crystal (static disorder) which are not resolved. As discussed further in Discussion, the Y-T coupling model would have predicted Thr⁸⁷ to be forced to occupy the active conformation due to the complete burial of Tyr¹⁰⁶ in complex with FliM₁₆, though this is clearly not the case (Fig. 4A).

	DISCUSSION

Top Abstract Introduction Dynamic excursions to the... Intermediate chey conformations. Materials and Methods Results Discussion References

 
Conformational coupling in unphosphorylated CheY. Information flow between the phosphorylation site and the target binding site has been shown to be bidirectional for CheY and other response regulator proteins (1, 24). The notion that ligands can affect CheY autophosphorylation kinetics by inducing conformational changes at the active site, termed conformational coupling, was hypothesized previously to explain the ability of FliM₁₆ to accelerate CheY autophosphorylation by nearly 30-fold (24). The "two-way street" notion of allostery assumes that allosteric communication in both directions (phosphorylation site to the target binding site and vice versa) happens by a flip of the same conformational switch, yet in complex with FliM₁₆, unphosphorylated CheY remains in a substantially inactive conformation (11).

In addition to supporting or refuting allosteric models, this structure provides insight as to the relationship between structure and function (binding, catalysis, etc.) in CheY. In the structure of BeF₃^–-CheY, the Thr⁸⁷ hydroxyl and Ala⁸⁸ backbone amide coordinate the BeF₃^– fluorine atoms that are thought to be analogous to the aspartyl-phosphate phosphoryl oxygens (19). In complex with FliM₁₆, Thr⁸⁷ and Ala⁸⁸ of unphosphorylated CheY are displaced toward the phosphoryl binding site relative to apoCheY (Fig. 4A) and Mg²⁺-CheY, despite the absence of BeF₃^–. However, in the CheY-FliM₁₆ complex, the Thr⁸⁷ side chain does not move so far as to overlay with Thr⁸⁷ of the BeF₃^–-CheY complex but instead is in a position intermediate to those of unphosphorylated CheY and BeF₃^–-CheY (Fig. 4A). This repositioning of Thr⁸⁷ and Ala⁸⁸ in the direction of the phosphoryl-binding site may account for the increased rate of CheY autophosphorylation in the presence of FliM₁₆. This structure-function relationship is also supported by structural and biochemical studies of the CheY-CheA^P2 complex, which has both a decreased autophosphorylation rate (24) and a significantly increased distance between the Thr⁸⁷ side chain and the phosphorylation site (22) relative to CheY alone,. Similarly, when this hydroxyl is made unavailable to the active site by mutation of the Thr⁸⁷ side chain to a non-Ser amino acid, the CheY autophosphorylation rate also decreases dramatically (2). In summary, (i) Thr⁸⁷ can take on a spectrum of conformations intermediate to the fully active and fully inactive conformations, (ii) allosteric ligands can affect the Thr⁸⁷ position, and (iii) the proximity of the Thr⁸⁷ hydroxyl to the active site correlates positively with the autophosphorylation rate. These data provide evidence in support of the conformational coupling hypothesis and highlight a role for Thr⁸⁷ in this process.

The equilibrium shift allosteric model. The equilibrium shift model of activation predicts the structure of unphosphorylated Mg²⁺-CheY-FliM₁₆ to be essentially identical to that of CheYP. While a comparison of BeF₃^–-CheY with the CheY-FliM₁₆ structure clearly indicates that this is not the case, the degree to which these results refute the equilibrium shift model of activation is a matter of perspective. The CheY-FliM₁₆ structure presented shows that in wild-type CheY the network of conserved residues can achieve an active-like arrangement in the absence of phosphorylation, as predicted by the equilibrium shift model. In contrast, phosphorylation appears to be a prerequisite for complete conformational switching of wild-type CheY, especially in regions remote from the target binding site such as the 1 helix and the ß5-5 loop (Fig. 3A). This indicates that, unlike for CheY**, the equilibrium shift model is not sufficient to describe the allosteric activation process for wild-type CheY.

FliM₁₆ affinity and the two-state assumption. The inability of unphosphorylated CheY to form several stabilizing contacts when bound to FliM₁₆ (relative to BeF₃^–-CheY-FliM₁₆) provides a molecular basis for the reduced FliM affinity of unphosphorylated CheY relative to that of CheYP. While the equilibrium shift model rests on the simple assumption that the folded protein can access only two stable states, its proponents must invoke preequilibrating subpopulations that are difficult or impossible to detect. Further, it ascribes affinity changes that result from phosphorylation to a shift in the inactive-to-active preequilibrium. Instead, our results suggest that the affinity difference has straightforward structural origins involving polar interactions near the peptide termini and that phosphorylation is in fact a prerequisite for the formation of the high-affinity FliM₁₆ interface.

The concurrence of active-like (resembling BeF₃^–-CheY) and inactive-like (resembling apoCheY) features in the same CheY conformation represents a clear though unanticipated departure from the two-state model of CheY activation. In the structures of several Salmonella enterica serovar Typhimurium CheY-CheZ_C peptide complexes (solved in both the presence and absence of BeF₃^–), CheY is found to occupy an intermediate region of activation space (11), offering another example of CheY plasticity and reinforcing the notion that the two-state assumption it is not adequate for describing the spectrum of conformations that are accessible to CheY.

The Y-T coupling allosteric model. The intermediate position of Thr⁸⁷ relative to apoCheY and BeF₃^–-CheY was not anticipated by either the equilibrium shift model or the Y-T coupling model of activation. Because Tyr¹⁰⁶ is buried in the CheY-FliM₁₆ complex, yet the "coupled" Thr⁸⁷ is not in the fully active position (Fig. 4A), the correlation between the conformations of these two residues does not appear to be exclusive and may involve the influence of another region of the protein. An alternate model to Y-T coupling that is consistent with the structure presented here would recognize the participation of the ß4-4 loop, in addition to steric occlusion, to explain the conformational correlation between Tyr¹⁰⁶ and Thr⁸⁷.

The structures of meta-active CheY (25), the CheY-CheZ_C complex (11), and the CheY-FliM₁₆ complex indicate that Tyr¹⁰⁶ can be buried without inducing a fully active conformation of the ß4-4 loop, while the structures of BeF₃^–-CheY (19) and the BeF₃^–-CheY-FliM₁₆ (20), CheY**-FliM₁₆ (8), and BeF₃^–-CheY-CheZ_C (11) complexes suggest that Thr⁸⁷ adopts the fully active conformation only when both the Tyr¹⁰⁶ side chain and ß4-4 loop are in their fully active conformations. Because the Thr⁸⁷ C of the CheY-FliM₁₆ complex is essentially in the active position, yet the C-Cß bond vector is inclined away from the active site as in apoCheY (Fig. 4A and D), it appears that the fully active orientation of the ß4-4 loop is related to a twist in the backbone that makes the Thr⁸⁷ hydroxyl available to the phosphorylation site. In a past study, the pseudodihedral angle defined by the C atoms of residues 87, 88, 89, and 90 was used to quantify the ß4-4 loop activation state (10). For unphosphorylated (FliM₁₆-free) CheY structures, including meta-active CheY, the value of this pseudodihedral angle is in the range of 10° to 30°, while values of 110° characterize the BeF₃^–-CheY and BeF₃^–-CheY-FliM₁₆ structures (Fig. 5A). In the CheY**-FliM₁₆ complex, the only instance where complete switching to the active (BeF₃^–-CheY-like) conformation is achieved in the absence of a phosphoryl analog, the value of the 87:88:89:90 pseudodihedral angle is nearly identical to that of BeF₃^–-CheY (108° and 110°, respectively). Consistent with the intermediate conformations of this loop in the CheY-FliM₁₆ structure (Fig. 4A), the values of the 87:88:89:90 pseudodihedral angle for the four observed subconformations (two per CheY) in the structure presented take on a spectrum of values intermediate to those for the canonical active and inactive conformations (Fig. 5A). The partially activated position of the ß4-4 loop in phosphono-CheY (12) is also evidenced by an intermediate value of the 87:88:89:90 pseudodihedral angle (Fig. 5A).

View larger version (17K): [in this window] [in a new window]   FIG. 5. (A) A spectrum of values are observed for the 87:88:89:90 C pseudodihedral angle in different wild-type CheY structures. The values of this angle for the CheY-FliM16 complex (Protein Data Bank accession no. 2B1J) are intermediate those of apoCheY (Protein Data Bank accession no. 3CHY) and BeF3–-CheY (Protein Data Bank accession no. 1FQW). The remaining structures shown are the high-resolution apoCheY structure (Protein Data Bank accession no. 1JBE, 2 subconformations), phosphono-CheY (Protein Data Bank accession no. 1C4W), and the BeF3–CheY-FliM16 complex (Protein Data Bank accession no. 1F4V). In contrast to wild-type CheY, CheY** exhibits a switch-like response to FliM16-binding (CheY**, Protein Data Bank accession no. 1U8T, chain C; CheY**-FliM16, Protein Data Bank accession no. 1U8T, chain A). (B) There is not a strong correlation between the degree of active character in the ß4-4 loop and the rotamer state of the Tyr106 side chain; the buried conformation of Tyr106 is consistent with the entire spectrum of observed ß4-4 loop conformations. However, the combination of an active ß4-4 loop and the solvent-exposed rotamer of Tyr106 is unoccupied. Structures having two subconformations of either Tyr106 or the ß4-4 loop are represented by two points connected with a dashed line. (C) The degree of active character in the ß4-4 loop (as measured by the 87:88:89:90 C pseudodihedral angle) does correlate well with the phi and psi angles of Val86, which position theThr87 side chain. Data derived from the structures of Mg2+-CheY (Protein Data Bank accession no. 2CHE), as well as the activating mutants CheYD13K (Protein Data Bank accession no. 1EHC), CheY!95V (Protein Data Bank accession no. 1D4Z), and CheYY106W (Protein Data Bank accession no. 5CHY) are additionally shown in panels B, C, and D. To avoid redundancy, the lower-resolution apoCheY structure (Protein Data Bank accession no. 3CHY) is not included in panel B, C, or D, and only the high-resolution apoCheY structure (Protein Data Bank accession no. 1JBE) is shown.

Further analysis of this set of CheY structures suggests that the conformation of the ß4-4 loop does correlate with the orientation of the Thr⁸⁷ side chain. Because the phosphorylation-dependent reorientation of the Thr⁸⁷ side chain is accomplished largely by changes in the Val⁸⁶ phi and psi angles (–111° and 136°, respectively, in apoCheY and –137° and 100°, respectively, in BeF₃^–-CheY), these values were used as a metric to describe Thr⁸⁷ orientation, providing a quantitative measure of the Thr⁸⁷ activation state. By plotting the 87:88:89:90 pseudodihedral angle versus either the phi (Fig. 5C) or psi (Fig. 5D) angle of Val⁸⁶ for the same family of CheY structures as in Fig. 5B, it is clear that aside from the CheY-FliM₁₆ complex, there exist two well resolved clusters that correspond to the inactive and active forms of CheY. Whereas the BeF₃^–-CheY-FliM₁₆ complex is situated firmly in the active region of pseudodihedral-phi and pseudodihedral-psi space, the CheY-FliM₁₆ complex is found in an intermediate region, between the inactive and active clusters of CheY structures (Fig. 5C and D). This result supports the notion that Thr⁸⁷ and the ß4-4 loop are coupled ("T-loop coupling") and is consistent with the partially switched character of this complex that is evident in structure superpositions (Fig. 3 and 4). When the set of structures in Fig. 5B (except CheY-FliM₁₆) are considered, the Val⁸⁶ phi and psi angles correlate well with the 87:88:89:90 pseudodihedral angle (r values of 0.94 and 0.95, respectively, for a linear fit to Fig. 5C and D). Conversely, for this same set of structures the Val⁸⁶ phi and psi angles are correlated poorly with the chi1 angle of Tyr¹⁰⁶ (r values of 0.58 and 0.53, respectively, for a linear fit) (data not shown).

The T-loop-Y allosteric model. In contrast with the central tenet of the Y-T coupling model, our analysis indicates that the conformation of Thr⁸⁷ and the Tyr¹⁰⁶ rotamer state are not strongly coupled (Fig. 5B), suggesting the existence of a more robust pathway along which the allosteric information can "flow." Strong coupling does exist between the Thr⁸⁷ side chain orientation and the conformation of the ß4-4 loop (Fig. 5C and D), highlighting an alternate pathway along which the phosphorylation signal could potentially be transmitted from the active site to the target binding site. Molecular dynamics simulations offer a similar picture of CheY allostery, wherein Thr⁸⁷ and the phosphorylation signal communicate with Tyr¹⁰⁶ through the ß4-4 loop, rather than by steric occlusion as suggested in the original Y-T coupling model. To supplant the Y-T coupling model, these data support a T-loop model whereby conformational changes at Thr⁸⁷ (e.g., phosphorylation) are strongly coupled to the conformation of the ß4-4 loop. The conformation of the ß4-4 loop is likely to impact target binding directly, as evidenced by the inability of FliM₁₆ to form previously observed contacts with the partially active loop of unphosphorylated CheY. Therefore, in regard to target binding, inducing the active conformation of the ß4-4 loop is an end in itself. However, we imagine that the more important role of this loop in CheY allostery is to facilitate communication between Thr⁸⁷ and Tyr¹⁰⁶.

Analysis of Fig. 5B highlights a potential route for allosteric communication from the ß4-4 loop to the bulky Tyr¹⁰⁶ side chain on the ligand binding surface. Although our analysis has already concluded that the ß4-4 loop and Tyr¹⁰⁶ are not strongly coupled in all cases, the apparent presence of an forbidden combination (Tyr¹⁰⁶ exposed and the loop active [Fig. 5B]) means that the conformation of one appears to restrict, or gate, the conformation of the other, in certain cases. Specifically, an active loop specifies burial of Tyr¹⁰⁶, and solvent exposure of Tyr¹⁰⁶ specifies an inactive loop, while the presence of an inactive loop or a buried Tyr¹⁰⁶ specifies nothing about the partner (Fig. 5B). Note that these relationships are directional; although an active loop specifies burial of Tyr¹⁰⁶, the burial of Tyr¹⁰⁶ does not specify an active loop.

The T-loop-Y model refers simply to an extension of the T-loop model that acknowledges the mutually restrictive relationship that exists between the ß4-4 loop and Tyr¹⁰⁶. According to this model, in apoCheY the default inactive conformation of Thr⁸⁷ is directly coupled to a substantially or fully inactive conformation of the ß4-4 loop. The notion that the inactive conformation(s) of the ß4-4 loop places little or no restriction on the Tyr¹⁰⁶ (though it responds slightly to the conformation of Tyr¹⁰⁶) agrees with the dual conformations of the aromatic ring in apoCheY. Any attempt to force the ring entirely into the buried conformation will be poorly or incompletely transmitted to the active site, since burial of Tyr¹⁰⁶ places few, if any, restrictions on the ß4-4 loop, consistent with the CheY-FliM₁₆ and CheY-CheZ_C (11) complex structures where BeF₃^– is absent. In contrast, forcing Tyr¹⁰⁶ to be entirely exposed, as is the case when CheY is bound to CheA, effectively gates the ß4-4 loop in the fully inactive conformation, consistent with the CheY-CheA^P2 complex structure (22). Similarly, locking Thr⁸⁷ in the active conformation (by phosphorylation) results directly in an activated conformation of the ß4-4 loop, which efficiently gates Tyr¹⁰⁶ to take on only the buried conformation, though it should be noted that in several of the recently published BeF₃^–-CheY-CheZ_C structures (11), the binding of BeF₃^– does not necessarily result in complete switching of Thr⁸⁷ (or, incidentally, of the ß4-4 loop, consistent with our model). One of these structures (Protein Data Bank accession no. 2FMH.pdb) provides particularly compelling support for the T-loop coupling notion, since there exist dual conformations of Thr⁸⁷ and the ß4-4 loop which have corresponding activation states (i.e., active-active and inactive-inactive). In summary, the T-loop-Y model (i) reconciles the complete switching of BeF₃^–-CheY and CheY-CheA^P2 with the incomplete switching of the FliM₁₆- or CheZ_C-bound CheY complexes and (ii) provides a rationale for the conformational heterogeneity of both Tyr¹⁰⁶ in apoCheY and Thr⁸⁷ in theCheY-FliM₁₆ complex.

Tyr¹⁰⁶ gating. The predicted ability of the inactive ß4-4 loop to discourage the buried orientation of Tyr¹⁰⁶, which was hypothesized on the basis of the meta-active CheY substructure (25) and described using the term "gating" in a more recent study (10), is apparent only as a weak trend in our analysis. Instead, our analysis indicates that restricting the loop in the active conformation very effectively gates the Tyr¹⁰⁶ side chain in the buried orientation and that restricting the Tyr¹⁰⁶ side chain in the solvent-exposed conformation effectively gates the loop to the inactive conformation. While the structural basis of the latter relationship is unclear, the ability of the active loop to gate Tyr¹⁰⁶ is likely due to the hydrogen bond formed between the Tyr¹⁰⁶ side chain hydroxyl and the Glu⁸⁹ backbone carbonyl observed in activated forms of CheY (e.g., BeF₃^–-CheY, BeF₃^–-CheY-FliM₁₆, BeF₃^–-CheY-CheZ_C, and even CheY**-FliM₁₆, where the indole nitrogen on Trp¹⁰⁶ serves as the proton donor). Therefore, these data encourage use of the term gating to acknowledge the more efficient Tyr¹⁰⁶ gating ability of the active, rather than the inactive, loop conformation (Fig. 5B), though the two mechanisms are not mutually exclusive. The T-loop-Y model also recognizes the ability of Tyr¹⁰⁶, when solvent exposed, to gate the ß4-4 loop in the inactive conformation, as is the case when CheY binds to CheA^P2.

Relevance to CheZ_C peptide binding. As mentioned previously, the recently published CheY-CheZ_C complex (11) also agrees well with this formulation of the T-loop-Y model, since the burial of Tyr¹⁰⁶ by bound CheZ is not sufficient to cause switching of Thr⁸⁷ and results in only modest displacement of the ß4-4 loop in the absence of BeF₃^–. Additionally, in all seven of the CheY-CheZ structures (with and without BeF₃^–) and the two substructures, differing degrees of Thr⁸⁷ activation correlate with the ß4-4 loop activation state.

In contrast, the structure-function trend that we observe for Thr⁸⁷ of CheY complexed with FliM₁₆ and CheA^P2 (positive correlation between the Thr⁸⁷ hydroxyl-to-phosphorylation site distance and observed autophosphorylation rate) is not apparent in the CheY-CheZ_C complexes. Instead, in the CheY-CheZ_C structures that lack BeF₃^–, Thr⁸⁷ retains a distinctly inactive conformation despite biochemical studies that shows CheZ_C binding to accelerate CheY phosphorylation kinetics (24). This may indicate that that the mechanism by which events at the peptide ligand binding surface are conformationally coupled to the active site may be subtly different for different ligands.

In conclusion, the crystallographic CheY-FliM₁₆ complex demonstrates that the structural changes associated with CheY phosphorylation are not exclusively coupled and in some regions are capable of adopting conformations intermediate to those of the inactive and active states. Additionally, the partially switched conformation that we observe for the crystalline CheY-FliM₁₆ complex agrees well with the nuclear magnetic resonance peak positions of this complex, which are typically intermediate to those of inactive CheY (apo or Mg²⁺-bound) and active (BeF₃^–-bound) forms of CheY (C. M. Dyer and F. W. Dahlquist, unpublished observations). In light of these results, it is clear that neither the equilibrium shift model, the Y-T coupling model, nor the two-state assumption upon which both models are based is a fully valid descriptor of allostery in CheY. Rather, the T-loop-Y model, which was anticipated on the basis of recent molecular dynamics simulations and acknowledges the active role of the ß4-4 loop in allosteric signaling (10), seems more consistent with the experimental results.

.

	ACKNOWLEDGMENTS

 
We thank John Perona for the use of the R-AXIS II. We also thank Brian Matthews for helpful suggestions regarding the manuscript prior to submission.

This work was funded by NIH grant GM059544 (to F.W.D.).

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Chemistry and Biochemistry, University of California at Santa Barbara, Santa Barbara, CA 93106. Phone: (805) 893-5326. Fax: (805) 893-4120. E-mail: dahlquist{at}chem.ucsb.edu.

	REFERENCES

Top Abstract Introduction Dynamic excursions to the... Intermediate chey conformations. Materials and Methods Results Discussion References

 

1. Ames, S. K., N. Frankeema, and L. J. Kenney. 1999. C-terminal DNA binding stimulates N-terminal phosphorylation of the outer membrane protein regulator OmpR from Escherichia coli. Proc. Natl. Acad. Sci. USA 96:11792-11797.[Abstract/Free Full Text]
2. Appleby, J., and R. Bourret. 1998. Proposed signal transduction role for conserved CheY residue Thr87, a member of the response regulator active-site quintet. J. Bacteriol. 180:3563-3569.[Abstract/Free Full Text]
3. Barak, R., and M. Eisenbach. 1992. Correlation between phosphorylation of the chemotaxis protein CheY and its activity at the flagellar motor. Biochemistry 31:1821-1826.[CrossRef][Medline]
4. Bellsolell, L., J. Prieto, L. Serrano, and M. Coll. 1994. Magnesium binding to the bacterial chemotaxis protein CheY results in large conformational changes involving its functional surface. J. Mol. Biol. 238:489-495.[CrossRef][Medline]
5. Brunger, A. T., P. D. Adams, G. M. Clore, W. L. DeLano, P. Gros, R. W. Grosse-Kunstleve, J.-S. Jiang, J. Kuszewski, N. Nilges, N. S. Pannu, R. J. Read, L. M. Rice, T. Simonson, and G. L. Warren. 1998. Crystallography and NMR systems (CNS): a new software system for macromolecular structure determination. Acta Crystallogr. D 54:905-921.[CrossRef][Medline]
6. Clegg, D. O., and D. E. J. Koshland. 1984. The role of a signaling protein in bacterial sensing: behavioral effects of increased gene expression. Proc. Natl. Acad. Sci. USA 81:5056-5060.[Abstract/Free Full Text]
7. Collaborative Computational Project. 1994. The CCP4 suite: programs for protein crystallography. Acta Crystallogr. D 50:760-763.[CrossRef][Medline]
8. Dyer, C. M., M. L. Quillin, A. Campos, J. Lu, E. M. Westbrook, P. Matsumura, B. W. Matthews, and F. W. Dahlquist. 2004. Structure of the constitutively active double mutant CheY^D13KY106W alone and in complex with a FliM peptide. J. Mol. Biol. 342:1325-1335.[CrossRef][Medline]
9. Feher, V. A., and J. Cavanagh. 1999. Millisecond-timescale motions contribute to the function of the bacterial response regulator protein Spo0F. Nature 400:289-293.[CrossRef][Medline]
10. Formaneck, M., L. Ma, and Q. Cui. 2006. Reconciling the "old" and "new" views of protein allostery: a molecular simulation study of chemotaxis Y protein (CheY). Proteins 63:846-867.[CrossRef][Medline]
11. Guhaniyogi, J., V. L. Robinson, and A. M. Stock. 2006. Crystal structures of beryllium fluoride-free and beryllium bound-bound CheY in complex with the conserved C-terminal peptide of CheZ reveal dual binding modes specific to CheY conformation. J. Mol. Biol. 359:624-645.[CrossRef][Medline]
12. Halkides, C. J., M. M. McEvoy, E. Casper, P. Matsumura, K. Volz, and F. W. Dahlquist. 2000. The 1.9 Å resolution crystal structure of phosphono-CheY, an analogue of the active form of the response regulator, CheY. Biochemistry 39:5280-5286.[CrossRef][Medline]
13. Hess, J. F., R. B. Bourret, and M. I. Simon. 1991. Phosphorylation assays for proteins of the two-component regulatory system controlling chemotaxis in Escherichia coli. Methods Enzymol. 200:188-204.[Medline]
14. Jiang, M., R. B. Bourret, M. I. Simon, and K. Volz. 1997. Uncoupled phosphorylation and activation in bacterial chemotaxis. The 2.3 A structure of an aspartate to lysine mutant at position 13 of CheY. J. Biol. Chem. 272:11850-11855.[Abstract/Free Full Text]
15. Jones, T. A., J.-Y. Zou, S. W. Cowan, and M. Kjeldgaard. 1991. Improved methods for building protein models in electron density maps and the location of errors in these models. Acta Crystallogr. A 47:110-119.
16. Kabsch, W. 1976. A solution for the best rotation to relate two sets of vectors. Acta Crystallogr. A 32:922-923.[CrossRef]
17. Kissinger, C. R., D. K. Gehlhaar, and D. B. Fogel. 1999. Rapid automated molecular replacement by evolutionary search. Acta Crystallogr. D 55:484-491.[CrossRef][Medline]
18. Lakowski, R. A., M. W. Macarthur, D. S. Moss, and J. M. Thornton. 1993. PROCHECK: a program to check the stereochemical quality of protein structures. J. Appl. Crystallogr. 26:283-291.[CrossRef]
19. Lee, S.-Y., H. S. Cho, J. G. Pelton, D. Yan, E. A. Berry, and D. E. Wemmer. 2001. Crystal structure of activated CheY. J. Biol. Chem. 276:16425-16431.[Abstract/Free Full Text]
20. Lee, S.-Y., H. S. Cho, J. G. Pelton, D. Yan, R. K. Henderson, D. S. King, L.-s. Huang, S. Kustu, E. A. Berry, and D. E. Wemmer. 2001. Crystal structure of an activated response regulator bound to its target. Nat. Struct. Biol. 8:52-56.[CrossRef][Medline]
21. Leslie, A. G. W. 1992. Recent changes to the MOSFLM package for processing film and image plate data. Joint CCP4 + ESF-EAMCB newsletter on protein crystallography, no. 26. Daresbury Laboratories, Warrington, United Kingdom.
22. McEvoy, M., A. C. Hausrath, G. B. Randolph, S. J. Remington, and F. W. Dahlquist. 1998. Two binding modes reveal flexibility in kinase/response regulator interactions in the bacterial chemotaxis pathway. Proc. Natl. Acad. Sci. USA 95:7333-7338.[Abstract/Free Full Text]
23. Moy, F. J., D. F. Lowry, P. Matsumura, F. W. Dahlquist, J. E. Krywko, and P. J. Domaille. 1994. Assignments, secondary structure, global fold, and dynamics of chemotaxis Y protein using three- and four-dimensional heteronuclear (¹³C,¹⁵N) NMR spectroscopy. Biochemistry 33:10731-10742.[CrossRef][Medline]
24. Schuster, M., R. E. Silversmith, and R. B. Bourret. 2001. Conformational coupling in the chemotaxis response regulator CheY. Proc. Natl. Acad. Sci. USA 98:6003-6008.[Abstract/Free Full Text]
25. Simonovic, M., and K. Volz. 2001. A distinct meta-active conformation in the 1.1-Å resolution structure of wild-type apo CheY. J. Biol. Chem. 276:28637-28640.[Abstract/Free Full Text]
26. Stock, A., E. Martinez-Hackert, B. Rasmussen, A. West, J. Stock, D. Ringe, and G. Petsko. 1993. Structure of the Mg(2+) bound form of CheY and mechanism of phosphoryl transfer in bacterial chemotaxis. Biochemistry 32:13375-13380.[CrossRef][Medline]
27. Volkman, B. F., D. Lipson, D. E. Wemmer, and D. Kern. 2001. Two-state allosteric behavior in a single-domain signaling protein. Science 291:2429-2433.[Abstract/Free Full Text]
28. Volz, K., and P. Matsumura. 1991. Crystal structure of Escherichia coli refined at 1.7-Å resolution. J. Biol. Chem. 266:15511-15519.[Abstract/Free Full Text]

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