Characterization of the Autocleavage Process of the Escherichia coli HtrA Protein: Implications for its Physiological Role

The Escherichia coli HtrA protein is a periplasmic protease/chaperonethat is upregulated under stress conditions. The protease andchaperone activities of HtrA eliminate or refold damaged andunfolded proteins in the bacterial periplasm that are generatedupon stress conditions. In the absence of substrates, HtrA oligomerizesinto a hexameric cage, but binding of misfolded proteins transformsthe hexamers into bigger 12-mer and 24-mer cages that encapsulatethe substrates for degradation or refolding. HtrA also undergoespartial degradation as a consequence of self-cleavage of themature protein, producing short-HtrA protein (s-HtrA). The aimof this study was to examine the physiological role of thisself-cleavage process. We found that the only requirement forself-cleavage of HtrA into s-HtrA in vitro was the hydrolysisof protein substrates. In fact, peptides resulting from thehydrolysis of the protein substrates were sufficient to induceautocleavage. However, the continuous presence of full-lengthsubstrate delayed the process. In addition, we observed thatthe hexameric cage structure is required for autocleavage andthat s-HtrA accumulates only late in the degradation reaction.These results suggest that self-cleavage occurs when HtrA reassemblesback into the resting hexameric structure and peptides resultingfrom substrate hydrolysis are allosterically stimulating theHtrA proteolytic activity. Our data support a model in whichthe physiological role of the self-cleavage process is to eliminatethe excess of HtrA once the stress conditions cease.

INTRODUCTION

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INTRODUCTION

The cell envelope of gram-negative bacteria mediates the communicationof the cell with the environment, and it is responsible formany vital functions, including nutrient uptake and interactionwith other bacteria and host cells. These activities are performedby a large collection of proteins that make the periplasm acellular compartment with an even higher protein concentrationthan the cytoplasm (2). Bacteria are frequently exposed to multiplestresses such as heat shock, osmotic stress, and pH changesand are regularly challenged by the host immune system. Thus,the maintenance of periplasmic proteins in a fully functionalstate is a challenging task undertaken by the protein qualitycontrol system (5). It is generally accepted that under stressconditions misfolded proteins, protein fragments, and mislocalizedmembrane proteins appear, activating a stress response throughthree different signal transduction pathways ( ${sigma}$ ^E, Cpx, and Bae)(21, 22). Activation of this stress response in the periplasmtriggers the upregulation of molecular chaperones, peptidases,proteases, and other enzymes with a role in eliminating or refoldingdamaged periplasmic proteins.

The Escherichia coli HtrA protein (also called DegP or proteaseDo) is a periplasmic protein (4) that is upregulated under stressconditions such as heat shock (14, 15). HtrA functions as achaperone and a protease in a temperature-dependent fashion(24). Recent studies have also shown that HtrA substrates targetedfor degradation or refolding are recognized differently, suggestingthat the mechanisms through which HtrA recognizes the substratemay play a role in the protease-chaperone switch (8).

HtrA contains an N-terminal protease domain, followed by thePDZ1 and PDZ2 domains. In the absence of substrates, HtrA oligomerizesinto a hexameric cage (12) that represents the resting stateof the protein (10, 13). Upon binding to protein substrates,HtrA transforms into bigger cages formed by 12 or 24 monomersthat encapsulate substrates for degradation or refolding (9,13).

HtrA is a 474-residue protein whose first 26 amino acids areremoved at the N terminus most likely by a signal peptidaserendering the mature 48-kDa protein (14, 15). This form of theprotein will hereon be referred to as full-length HtrA. However,it has been described (11, 23) that mature HtrA undergoes partialdegradation both in vivo and in vitro as a consequence of self-cleavageoccurring after Cys⁶⁹ and Gln⁸² of the mature protein. Theseforms of the protein have been named short-HtrA (s-HtrA) (23).

A similar phenomenon of autocleavage has been observed in othermembers of the HtrA family such as the human homologs HtrA1(7) and HtrA2 proteins (6). The autocleavage process is notspecific for proteases of the HtrA family. Several prokaryoticproteins involved in regulation of gene expression, such asthe SOS response proteins LexA (16-18) and UmuD (3), are inactivatedthrough a self-cleaving mechanism. Conversely, many mammalianproteases are produced as longer inactive precursors and dependon an intramolecular cleavage event to become active. This isthe case for some gastric proteases such as pepsin and chymosinor the lysosome cathepsins D and E (1).

Although autocleavage as a mechanism of activation or inactivationof certain proteases is well documented, the physiological roleand the events triggering the self-cleavage of HtrA are poorlyunderstood. In this study, we observed that the hexameric cagestructure is required to observe autocleavage of HtrA. In addition,we analyzed the conditions that led to self-cleavage of HtrAand we found that the only requirement to observe accumulationof the s-HtrA form in vitro was the hydrolysis of protein substrates.In fact, peptides resulting from the degradation of proteinsubstrates were sufficient to induce autocleavage. Therefore,considering the current functional model for HtrA (9, 13), ourdata suggest that the physiological role of the HtrA autocleavageis to eliminate the excess of HtrA protein expressed under stressconditions when the enzymatic activities of the protein areno longer needed.

MATERIALS AND METHODS

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MATERIALS AND METHODS

Plasmids and mutagenesis. The pET21b-HtrA plasmid and the ${Delta}$ PDZ2 HtrA mutant were obtainedas described previously (10). The C57A+C69G HtrA mutant wasobtained from the pET21b-HtrA plasmid using the QuikChange site-directedmutagenesis method (Stratagene).

Protein expression and purification. Wild-type and HtrA mutants were expressed as C-terminal His-taggedproteins. The method to express and purify the proteins witha HiTrap metal chelating column (GE Healthcare Life Sciences)was performed as described previously (10).

When a protein preparation containing mostly full-length HtrAwas required, E. coli BL21(DE3) cells with the expression vectorcontaining wild-type or mutant HtrA were induced for 30 minat 37°C with 1 mM IPTG (isopropyl-β-D-thiogalactopyranoside).However, to obtain a protein preparation with higher proportionof s-HtrA form, cells were induced for 3 h at 37°C with1 mM IPTG in LB medium containing 5 mM dithiothreitol (DTT)freshly added at the moment of induction.

Size exclusion chromatography. Gel filtration chromatography experiments were performed ona Superdex 200 10/300 GL column (GE Healthcare Life Sciences).The column was equilibrated in 50 mM HEPES (pH 7.3)-100 mM NaClat 4°C. Protein samples (100 µl) at a concentrationbetween 0.5 and 3.5 mg/ml were injected to the column. A gelfiltration calibration kit (HMW; GE Healthcare Life Sciences)was used for column calibration.

Protease activity assays. Protease activity assays in Fig. 1 were assembled as 250-µlreaction mixtures containing HtrA at 1.3 µM and substrateat 13 µM in 50 mM HEPES (pH 7.3). As substrates, we usedmalate dehydrogenase (MDH) from porcine heart (Roche and Sigma),bovine milk β-casein (Sigma), and egg white lysozyme (Bioshop).Reactions were incubated at 37°C for the β-casein andlysozyme assays and at 43°C for the MDH experiments. DTTwas added to the lysozyme reactions up to a final concentrationof 2 mM. At the indicated times, 10-µl samples were takenand mixed with 2x concentrated sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) loading buffer, resolved by SDS-PAGE,and stained with Coomassie brilliant blue (GE Healthcare LifeSciences). The remaining β-casein hydrolysis assays performedfollowed the same procedure as the one in Fig. 1. However, reactionmixtures contained HtrA at 4.1 µM and β-casein at66 µM.

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FIG. 1. HtrA autocleavage in the presence of substrate. Proteolytic reactions were assembled in a total volume of 250 µl containing 1.3 µM HtrA and 13 µM concentrations of substrate. The substrates tested were lysozyme (top panel), β-casein (middle panel), and MDH (bottom panel) (lanes labeled "HtrA + Substrate"). A control reaction was performed for each degradation assay consisting of HtrA protein incubated in the absence of substrate (lanes labeled "HtrA"). Reactions were incubated and, at the indicated time points, samples were obtained, and the products of the reaction resolved by SDS-PAGE and stained by Coomassie brilliant blue. Arrows indicate the bands for the corresponding substrate, full-length HtrA and s-HtrA protein in each gel.

To obtain the accumulation profiles of s-HtrA protein for C57A+C69GHtrA mutant, the hydrolysis reactions were performed by mixingβ-casein (66 µM) with HtrA or the C57A+C69G HtrAmutant (4.1 µM) in a reaction volume of 250 µl (50mM HEPES [pH 7.3]). Where indicated, DTT was added to a finalconcentration of 2 mM. At the indicated times, 10-µl sampleswere resolved by SDS-PAGE and stained with Coomassie brilliantblue. The proteolysis reaction for the C57A+C69G HtrA mutantin each condition (i.e., the presence or absence of DTT) wasrun in the same gel together with the analogous reaction performedwith the wild type to account for differences in staining betweengels. Gels were scanned in a flatbed scanner, and the totalintensity of the bands representing s-HtrA protein was measuredand subtracted from the intensity of the band at time zero minby using ImageQuant TL software. These intensities were usedto plot the accumulation profiles. Each proteolysis reactionwas repeated three times, and an average and standard deviationwas calculated.

To generate and purify β-casein peptides, 250-µlreaction mixtures were assembled in 50 mM HEPES (pH 7.3) containinga concentration of 4.1 µM HtrA and 66 µM β-casein.In the case where the peptides were generated by trypsin, thereaction contained 4.1 µM trypsin and 132 µM β-casein.The buffer conditions were the same, but MgCl₂ was added upto a final concentration of 5 mM. Reaction mixtures were incubatedat 37°C for 40 min and then boiled for 10 min and immediatelychilled at 4°C to terminate the reaction and to precipitateHtrA and trypsin. Subsequently, reactions were spun down at12,000 rpm in a benchtop centrifuge at 4°C, and the supernatantcontaining the β-casein peptides was topped up to 250 µlwith 50 mM HEPES (pH 7.3) buffer containing HtrA. The finalconcentration of HtrA in the mixture was 4.1 µM. The reactionwas then incubated at 37°C for 4 h. At the indicated times,20-µl samples were taken, mixed with 2x concentrated SDS-PAGEloading buffer, and 12.5 µl was resolved by SDS-PAGE (12%).Gels were stained with Coomassie brilliant blue.

Western blotting. Samples were resolved by SDS-12% PAGE and transferred to anImmobilon-P filter (Millipore) according to manufacturer's protocols.The membrane was then saturated with 5% skim milk in TBS-T buffer(50 mM Tris-HCl [pH 7.4], 150 mM NaCl, 0.1% Tween 20) for 12h at 4°C. The filters were incubated with a 1:12,500 dilutionof the anti-HtrA serum for 1 h at 4°C. They were washedone time for 15 min and three times for 5 min with TBS-T bufferand then incubated with a 1:4,000 dilution of goat anti-rabbitimmunoglobulin G conjugated to peroxidase. Finally, the filterswere washed one time for 15 min and three times for 5 min asdescribed above, plus an additional wash for 5 min in TBS buffer(50 mM Tris-HCl [pH 7.4], 150 mM NaCl). The filter was developedby using enhanced chemiluminescence.

The anti-HtrA serum was prepared by immunization of rabbitswith C-terminal His-tagged HtrA protein that was purified aspreviously described (10).

RESULTS

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RESULTS

Only substrate degradation is required for the autocleavage of HtrA and production of s-HtrA protein in vitro. It was shown previously that both proteolytic activity of HtrAand reducing conditions were essential to observe autocleavageof HtrA and production of s-HtrA protein (23). To initiate ourstudy aimed to unveil the physiological role of the s-HtrA protein,we investigated whether autocleavage of HtrA occurs during degradationof lysozyme, β-casein, and MDH. In the performed assaysthe concentrations of HtrA (1.3 µM) and substrate (13µM) were similar to the ones used by Skorko-Glonek etal. (23). Consistent with that study, we observed autocleavageof HtrA in a lysozyme degradation assay under reducing conditions(Fig. 1, top panel). β-Casein and MDH did not require reducingconditions to be degraded by HtrA (11). However, s-HtrA proteinwas also obtained upon degradation of these substrates (Fig.1, middle and bottom panels). The amount of s-HtrA generatedin these reactions was very similar in the presence or absenceof reducing agents (data not shown). Furthermore, no s-HtrAwas produced in any of the conditions when HtrA was incubatedin the absence of substrate (Fig. 1). The N-terminal sequencesof the two degradation products observed in our proteolysisreactions (data not shown) were consistent with previously publisheddata (23), establishing that the two s-HtrA protein forms ariseas a consequence of cutting occurring after Cys⁶⁹ or after Gln⁸².

Consistent with the study by Skorko-Glonek et al. (23), we observedthat the amount of s-HtrA protein generated in these assayscorrelated with the amount of full-length substrate degradedand the speed of hydrolysis. The amount of s-HtrA protein accumulatedover 4 h of incubation time was most prominent in the β-caseinassay and followed by the experiment using MDH. In these experimentsfull-length substrate was eliminated in $~$ 30 (β-casein) and $~$ 120 (MDH) minutes (Fig. 1, middle and bottom panels), and thes-HtrA protein started to accumulate soon after the full-lengthsubstrate disappeared. Lysozyme hydrolysis progressed slowly,and there was still a significant amount of full-length substrateleft after 4 h. As a result, only very little s-HtrA proteinwas generated even in the presence of reducing agents (Fig.1, top panel).

In the previous experiment, the concentrations of HtrA and substrateswere higher than those used in previous HtrA studies (19) andalso those occurring in vivo. Therefore, these experiments wererepeated at concentrations 10 times lower (HtrA at 0.13 µMand substrate at 1.3 µM). Similarly to the previous experiment,only substrate degradation was needed to observe autocleavegeof HtrA (see Fig. S1 in the supplemental material) and reducingconditions were only essential in cases where they were requiredto unfold the substrate and make it susceptible for degradationby HtrA. The amount of s-HtrA protein generated in the assayalso correlated with the amount of full-length substrate degradedand the speed of hydrolysis. Therefore, we concluded that autocleavageof HtrA occurs in a similar manner in a broad range of HtrAand substrate concentrations.

Cys⁵⁷ and Cys⁶⁹ residues in HtrA do not confer additional stability to the protein against autocleavage and are not essential to maintain the HtrA hexameric cage. It has been previously suggested that reducing stress couldinduce autocleavage of HtrA because these conditions disruptthe disulfide bridge formed by the only two existing cysteineresidues (Cys⁵⁷ and Cys⁶⁹) in the HtrA sequence (23). In ourexperiments, the presence of reducing agents was not a requirementin order to observe autocleavage of HtrA. However, we decidedto test whether Cys⁵⁷ and Cys⁶⁹ residues are essential to maintainthe HtrA hexameric cage or the disulfide bridge formed conferredadditional stability to the protein against autocleavage.

Residues Cys⁵⁷ and Cys⁶⁹ in HtrA are located within the LA loopof the protease domain. The LA loop protrudes from the HtrAmonomer and acts as a molecular spacer between the two trimersforming the HtrA hexameric cage. Two LA loops from oppositemonomers in the hexamer wrap around each other and form thecorner pillars of the cage. Our previous studies found thatresidues 39 to 78 in the LA loop (containing the Cys⁵⁷ and Cys⁶⁹)are essential to maintain the hexameric cage (10). To test specificallywhether these two cysteine residues are essential to maintainthe integrity of the hexamer, we constructed and purified theC57A+C69G HtrA mutant. The purified mutant behaved similarlyto wild-type HtrA on a size exclusion chromatography columnand produced an elution profile consistent with the hexamericform of the protein (Fig. 2A) ruling out any role of Cys⁵⁷ andCys⁶⁹ on maintaining the HtrA hexamer.

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FIG. 2. Characterization of the oligomeric state and stability of the C57A+C69G HtrA mutant. (A) Elution profile of the C57A+C69G HtrA (left) and wild-type HtrA (right) proteins from a Superdex-200 column. The dashed line in the plot on the right-hand side indicates the expected elution volume (Ve) for the hexameric form of the protein (11.5 ml). (B) C57A+C69G HtrA and wild-type HtrA proteins were eluted from a metal chelating column and resolved by SDS-PAGE and stained with Coomassie brilliant blue. Both full-length HtrA and s-HtrA proteins coeluted from this column. Bovine serum albumin (BSA) protein (2 µg) was added to each sample as a loading control. (C) Accumulation profiles of s-HtrA protein for the C57A+C69G HtrA mutant and wild-type HtrA in the presence or absence of DTT. Profiles were obtained by performing proteolysis reactions containing β-casein and HtrA or the C57A+C69G HtrA mutant. Reactions shown on the left were performed either in the absence (left panels) or in the presence (right panels) of DTT. Samples of the reactions at the specified time points were resolved by SDS-PAGE (upper panel). Each proteolysis reaction for the C57A+C69G HtrA mutant was run in the same gel, together with the analogous reaction performed with wild-type HtrA. BSA protein (2 µg) was added to samples as a loading control. Gels were stained by Coomassie brilliant blue and scanned, and the intensity of the bands representing s-HtrA protein (boxed areas, upper panel) was measured and plotted with respect to time (bottom panel). The plots represent the average and standard deviations obtained upon repeating each experiment three times.

Furthermore, two additional observations suggested that thedisulfide bridge formed by these two cysteine residues doesnot confer additional stability to the protein. First, the autocleavageof wild-type HtrA also occurs in vivo during protein expression(23) and both full-length and s-HtrA coelute together from themetal chelating column used in our protein purification strategy.Thus, to minimize the amount of s-HtrA in our protein preparations,the expression time was limited to 30 min (10). Higher proportionsof s-HtrA protein would be anticipated to coelute from the columnwith a preparation of an HtrA mutant with higher autocleavagerates. However, when the C57A+C69G HtrA was eluted under conditionsidentical to those used for the wild type, we did not observeincreased amounts of s-HtrA protein coeluting with full-lengthHtrA (Fig. 2B). Second, the C57A+C69G HtrA mutant degraded β-caseinas efficiently as wild-type HtrA both in the presence and inthe absence of DTT (Fig. 2C, top panel). However, we did notobserve any statistically significant differences between theaccumulation profiles of s-HtrA protein from wild-type HtrAand the Cys mutant for any of the conditions tested (Fig. 2C,bottom panel). A similar experiment performed with MDH as asubstrate did not show any statistically significant differenceseither (data not shown).

Altogether these experiments indicate that the cysteine residuespresent in the HtrA protein (Cys⁵⁷ and Cys⁶⁹) are not essentialto maintain the integrity of the hexameric cage, and they donot stabilize HtrA in a manner that significantly prevents ordelays autocleavage of the protein.

Continuous addition of full-length substrate delays autocleavage of HtrA. To further investigate the conditions leading to the productionof s-HtrA protein, we assembled a proteolysis reaction by mixingHtrA with β-casein. In the tested conditions, full-lengthβ-casein was degraded after 30 min, and smaller peptidesproducts started to accumulate (Fig. 3A). A significant amountof s-HtrA was already present after 2 h, and approximately 90%of the HtrA protein became autocleaved after 7 h of incubation(Fig. 3A). Incubation of the reaction for 24 h produced almosta complete self-degradation of the HtrA protein into the s-HtrAprotein first and subsequent shorter HtrA forms, most of themnot observed in the SDS-PAGE. When fresh β-casein was addedat this point in the reaction mixture, we observed that substratehydrolysis was significantly slowed down, suggesting that thesefragments are proteolytically inactive (Fig. 3B, left panel).In a replica of this experiment, HtrA autocleavage progressedslightly faster during the overnight incubation, and we in factobserved a complete self-degradation of the enzyme, and no HtrAor s-HtrA form was left after 24 h of incubation. In this case,the reaction mixture showed no further degradation of newlyprovided β-casein (Fig. 3B; right panel). These reactionsshow that HtrA degrades the substrate first before the autocleavagebecomes significant, and then it progresses until complete self-degradationand consequent inactivation of HtrA. A control experiment wascarried out simultaneously by incubating HtrA protein alonefor 24 h to ensure that the protein remains stable and activeupon such a long incubation at 37°C. As expected, no s-HtrAprotein was formed in the absence of substrate, and the enzymeremained proteolytically active, as demonstrated by fast degradationof the β-casein after 24 h of incubation of HtrA at 37°C(Fig. 3C).

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FIG. 3. Full-length substrate delays autocleavage of HtrA. (A) A proteolysis reaction containing β-casein substrate (66 µM) and HtrA (4.1 µM) was incubated at 37°C for 7 h, and at the indicated times samples of the reaction were obtained and loaded on an SDS-PAGE gel and stained by Coomassie brilliant blue. The asterisk indicates when fresh β-casein was added in the reaction. (B) The previous reaction was kept up to 24 h at 37°C. Then, fresh β-casein was added (asterisk) and incubated for one additional hour. The left panel shows an SDS-PAGE gel resolving the indicated time points of this reaction. The SDS-PAGE results on the right replicate the experiment shown in the left panel, where autocleavage of HtrA progressed slightly faster during the overnight incubation and degraded all of the HtrA in the reaction. (C) HtrA protein (4.1 µM) was preincubated at 37°C for 24 h before the substrate β-casein (66 µM) was added (asterisk). Then, at the indicated times samples were extracted and resolved by SDS-PAGE. Gels were stained by Coomassie brilliant blue. (D) This proteolysis reaction was assembled as in panel A and then kept up to 24 h as in panel B. Asterisks indicate the time points when fresh β-casein was added during the reaction. The indicated time point samples were obtained from the reaction, resolved by SDS-PAGE, and stained with Coomassie brilliant blue. Where indicated an identical amount of BSA protein (2 µg) was added to each sample as a loading control.

To confirm that the presence of full-length substrate delaysautocleavage of HtrA, we performed an additional proteolysisreaction. In this case, fresh β-casein was added at thebeginning of the reaction and after every 60 min of incubationup to 6 h. Interestingly, very small amounts of s-HtrA proteinaccumulated in the SDS-PAGE even after 7 h of incubation, suggestingthat constant presence of full-length β-casein or longdegradation peptides inhibit autocleavage of the HtrA protein(Fig. 3D).

Peptides generated during proteolytic degradation of the substrate are sufficient to stimulate HtrA autocleavage. The previous experiments showed that significant amounts ofs-HtrA protein did not accumulate until all of the full-lengthβ-casein and large degradation products were proteolyzedinto small peptides. Thus, we wanted to test whether the smallpeptides generated during the proteolytic reaction are sufficientto stimulate HtrA autocleavage. A proteolysis reaction usingβ-casein as a substrate was assembled and incubated at37°C. As previously shown, most of the substrate becameproteolyzed after 30 min of reaction and most of the HtrA wasself-cleaved after 4 h (Fig. 4A). The reaction was kept up to24 h at the incubation conditions, and then fresh HtrA was addedto the reaction. Under these conditions the newly added HtrAunderwent autocleavage right from the beginning of the reactionand, similarly, most of the HtrA was autocleaved in 4 h (Fig.4A).

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FIG. 4. Degradation peptides products stimulate HtrA autocleavage. (A) A proteolytic reaction containing β-casein (66 µM) in the presence of HtrA (4.1 µM) was incubated for 4 h at 37°C. Samples were obtained at the indicated times, resolved by SDS-PAGE, and stained with Coomassie brilliant blue. After the reaction was kept at 37°C for 24 h, fresh HtrA (4.1 µM) was added, and the incubation was continued for four additional hours. Samples were taken at the indicated times to monitor the accumulation of s-HtrA protein. BSA protein (2 µg) was added to each sample as a loading control. (B) β-Casein peptides produced by HtrA hydrolysis were incubated with HtrA (4.1 µM) for 4 h at 37°C. At the indicated time points, samples were obtained and resolved by SDS-PAGE (left). The samples at time zero and 240 min were also processed for Western blotting with a rabbit anti-HtrA serum (right). The "+" sign indicates the 25-kDa self-cleavage form of HtrA recognized by the anti-HtrA serum. (C) β-Casein peptides produced by trypsin hydrolysis were mixed with HtrA (4.1 µM) in an autocleavage reaction for 4 h at 37°C. Time points of the reaction were obtained and resolved by SDS-PAGE. The asterisk indicates small peptides produced from HtrA and s-HtrA proteins by a residual amount of trypsin incorporated in the autocleavage reaction along with the β-casein peptides.

In order to confirm that the peptides generated during substratehydrolysis are sufficient to stimulate HtrA autocleavage, wedegraded β-casein substrate in the presence of either HtrAor trypsin for 40 min. Then, the reaction mixtures were boiledfor 10 min to terminate the reaction and precipitate HtrA andtrypsin. The precipitated proteins were spun down, and the supernatantscontaining the peptides were incubated with HtrA (4.1 µM)in two different autocleavage reactions for 4 h at 37°C.Consistent with the results presented in Fig. 4A, the freshlyadded HtrA underwent autocleavage and produced s-HtrA form inthe presence of β-casein peptides starting at very earlytimes of the reaction (Fig. 4B and C).

We noticed that an additional protein band of $~$ 25 kDa accumulatedat later times of incubation in the proteolytic reaction (Fig.4A, "+" sign, and 4B, left panel). To determine whether thisprotein was an additional self-cleavage product of HtrA, weanalyzed the products of the reaction by Western blotting. Samplesof the autocleavage reaction containing HtrA and β-caseinpeptides produced by HtrA were resolved by SDS-PAGE and processedfor Western blot with a rabbit anti-HtrA serum (Fig. 4B, rightpanel). The 25-kDa band reacted with the anti-HtrA serum, suggestingthat this reaction product is also a self-cleavage form of HtrA.This finding is consistent with our previous experiment (Fig.3B), suggesting that the self-cleavage process of HtrA doesnot stop with the generation of the described $~$ 43-kDa s-HtrAforms. Rather, subsequent self-cleavage events hydrolyzed HtrAuntil complete degradation of the enzyme.

We also observed that a small amount of trypsin remained inthe supernatant after the β-casein hydrolysis reactionwas spun down. However, this amount of trypsin did not contributeto the amount of s-HtrA form generated in the autocleavage reaction.Trypsin is a highly specific enzyme that cleaves peptide bondson the carboxyl side of residues Arg and Lys (20). HtrA containsmore than 30 potential cleaving sites for trypsin, and it isquickly degraded by this protease into small peptides, noneof them corresponding to the length of the s-HtrA forms. Someof these small peptides were observed on the SDS-PAGE (Fig.4C, asterisk).

Similarly to the experiments where we looked at the productionof s-HtrA form in the presence of several substrates at high(Fig. 1) and low (see Fig. S1 in the supplemental material)concentrations, we wanted to test whether peptides also stimulateHtrA autocleavage in a broad range of concentrations. Therefore,we repeated the autocleavage of HtrA by β-casein peptidesbut at significantly lower concentrations (HtrA at 0.13 µM).As expected, HtrA also underwent autocleavage and produced s-HtrAprotein in the presence of β-casein peptides (see Fig.S2 in the supplemental material).

For the experiments performed at both high and low concentrations,we carried out control experiments similar to the ones shownin Fig. 1 and Fig. S1 in the supplemental material1, where HtrAalone was incubated at 37°C for 4 h. s-HtrA protein wasnot produced in any of the tested conditions.

Therefore, we concluded that peptides generated during the proteolyticreaction are sufficient to stimulate HtrA autocleavage in vitro,and this process occurs in a similar manner in a broad rangeof HtrA and peptide concentrations.

The hexameric cage structure is required for the autocleavage of HtrA. We reported that the hexameric structure of HtrA is not essentialfor proteolytic activity since trimeric mutants of the proteinare able to hydrolyze substrates similarly to wild-type HtrA(10). Therefore, the question then arose as to whether the HtrAhexameric cage is required for the autocleavage of HtrA.

To answer this question, we tested the ability of a previouslycharacterized ${Delta}$ PDZ2 HtrA mutant (10) to produce s-HtrA protein.This HtrA construct is able to bind protein substrates and hasproteolytic activity similar to wild-type HtrA; however, anenclosed cavity no longer exists in this mutant since the HtrAhexamer has been separated into two trimers (10). A proteolysisreaction was assembled with this mutant (Fig. 5A) by mixingthe mutant protein (4.1 µM) with β-casein (66 µM)and incubating the reaction up to 24 h at 37°C. A proteolysisreaction was carried out in parallel containing wild-type HtrAand β-casein (Fig. 5B). We found that while the controlreaction containing wild-type HtrA produced s-HtrA protein inlarge amounts (Fig. 5B), the reaction containing the ${Delta}$ PDZ2 HtrAmutant did not produce any s-HtrA, even after 24 h of incubation(Fig. 5A), suggesting that the hexameric cage is required forthe autocleavage of HtrA.

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FIG. 5. A trimeric HtrA mutant does not undergo autocleavage. (A) SDS-PAGE resolving samples obtained at the indicated time points from a β-casein proteolysis reaction performed with the ${Delta}$ PDZ2 HtrA mutant. (B) Control reaction containing HtrA and β-casein showing production of s-HtrA protein at the same time points as for the results shown in panel A.

The s-HtrA form has a decreased proteolytic activity. A previous study indicated that upon HtrA autocleavage, thehexameric cage undergoes irreversible dissociation into monomers(23). These results suggested that the autocleavage processcompromises the oligomeric structure of the protein. In ourstudy, we sought to determine whether the autocleavage of HtrAalso compromises the HtrA proteolytic activity.

To do this, we obtained a protein preparation with a high proportionof s-HtrA, and the proteolytic activity was compared to a proteinpreparation containing mostly full-length HtrA. In order tomaximize the amount of s-HtrA in our protein preparation, weextended the expression time to 3 h, and DTT was added to theLB medium at the moment of induction. These conditions stimulatedthe hydrolysis of substrates that require reducing conditionsfor unfolding and as a consequence HtrA autocleavage. This approachyielded a preparation of HtrA containing 60% of the proteinas s-HtrA (Fig. 6). The obtained protein preparation (4.1 µM)was mixed with β-casein (66 µM) and incubated at37°C for 2 h. This reaction was carried out in parallelwith another β-casein proteolytic reaction containing mostlyfull-length HtrA. Samples obtained at 6 and 12 min showed thatthe proteolytic degradation of β-casein was significantlydelayed in the reaction containing high proportions of s-HtrAprotein, suggesting that the autocleavage process inhibits HtrAproteolytic activity. Nevertheless, most of the β-caseinsubstrate was degraded after 2 h of incubation as a consequenceof the remaining 40% full-length HtrA protein in this preparation(Fig. 6).

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FIG. 6. Proteolytic activity of the autocleaved HtrA protein. A preparation containing mostly full-length HtrA protein (lanes labeled "HtrA") or 60% s-HtrA (lanes labeled "s-HtrA") were incubated with β-casein for 2 h at 37°C. Samples were taken at the indicated time points and resolved by SDS-PAGE.

DISCUSSION

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DISCUSSION

This study addresses a new facet of HtrA regulation: the mechanismto eliminate excess of HtrA from the cell once the stress conditionsare overcome.

E. coli upregulates HtrA expression to quickly eliminate unfoldedand damaged proteins associated with heat shock conditions andother form of stress. Based on our observations, particularly(i) that HtrA autocleavage mostly occurred after full-lengthsubstrate is degraded, (ii) that it is induced by the peptidesproduced during substrate hydrolysis, and (iii) that autocleavageaffects the proteolytic activity of the enzyme, we hypothesizedthat the autocleavage of HtrA is in fact a self-regulatory mechanismaiming to eliminate the excess of HtrA produced under stressconditions once its enzymatic activities are no longer needed.

Our hypothesis integrates well with the current functional modelfor this protease: the hexameric HtrA cage is the resting stateof the protein but upon substrate binding the protein reorganizesinto large 12-mer and 24-mer oligomeric cages encapsulatingthe substrate for degradation. When substrate degradation hasbeen completed HtrA reverts to its hexameric resting state (9,13). Proteolytic activity of HtrA is also allosterically stimulatedby oligopeptides, and this activation is mediated by the bindingof the activating peptide to the PDZ1 domain (19).

In the context of this functional model, our data can be interpretedas follows: while full-length substrate or long degradationpeptides are present, HtrA remains mostly as 12-mer and 24-meroligomeric cages, and limited amounts of s-HtrA form are produced.Our finding that the hexameric cage structure is required forthe autocleavage of HtrA and that the s-HtrA form appeared latein the reaction suggests that the self-cleavage occurs whenHtrA reassembles back into the resting hexameric cage once thedegradation is completed and HtrA is in the presence of stimulatingpeptides resulting from substrate hydrolysis (Fig. 7). Existingstructural data (9, 12, 13) support this hypothesis. The X-raystructure of the larger oligomers of HtrA showed that the LAloop has been extracted from the active site and the L1 andL2 loops are set up as a functional proteolytic site (13). However,in the hexameric form the LA loop protrudes into the activesite of the subunit in the opposite trimer forcing the L1 andL2 loops into a twisted inactive conformation. Upon completionof the degradation, the protease returns to its hexameric form,but peptides resulting from substrate hydrolysis allostericallystimulate HtrA proteolytic activity (19). It is likely, althoughthere is no experimental support yet, that peptides allostericallystimulating HtrA may keep the catalytic L1 and L2 loops in anactive conformation. Consequently, the LA loop may be cleavedbecause it is placed back in close proximity to the catalyticsite that may be now in an active conformation.

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FIG. 7. Schematic model of the autocleavage of HtrA. HtrA reorganizes into large cages that encapsulate the substrate for degradation. Once full-length substrate has been degraded, the HtrA reverts to its hexameric resting state, and peptides generated during substrate hydrolysis allosterically activate HtrA, inducing the self-cleavage process. PDB files 1ky9 and 2zle for the hexameric and 12-mer HtrA cages, respectively, were obtained from the Protein Data Bank and are displayed with the program UCSF Chimera (http://www.cgl.ucsf.edu/chimera).

Consistent with our hypothesis that the autocatalytic processis a regulatory suicide mechanism, we found that cleavage ofthe LA loop during autocleavage decreases HtrA proteolytic activity.A previous study reported (but did not show) (23) that the s-HtrAform remains fully active. Our results implicitly suggest thatthe s-HtrA form is inactive (Fig. 6). However, we were unableto overexpress and purify the s-HtrA forms ( ${Delta}$ 1-69 HtrA and ${Delta}$ 1-82HtrA) since the deletion regions compromise the proper foldingof the protease domain and the trimer formation. Instead, ourpurification method yielded a preparation of HtrA containing60% of the protein as s-HtrA, and therefore, at extended incubationtimes, substrate degradation was always observed due to thestill existing full-length HtrA. Nevertheless, our results provideenough evidence to state that the s-HtrA form has a decreasedproteolytic activity compared to full-length HtrA (Fig. 6).

There are several aspects of this regulatory model that arestill not fully understood. For instance, the PDZ1 domain inHtrA mediates both substrate recognition and allosteric stimulationby binding to exposed C-terminal residues from the substrateand also short oligopeptides, respectively. Both full-lengthsubstrates and oligopeptides may bind to the same site in thePDZ1 domain; however, only long protein substrates seem to efficientlyinduce reorganization of HtrA into larger oligomeric cages.Further research is required to understand how these two substratestrigger a different response upon binding to HtrA.

In addition, proposing that HtrA has a clearance mechanism thateliminates the enzyme when it is no longer needed implicitlysuggests that HtrA is harmful to the cell in the absence ofadequate levels of substrate. Interestingly, during the courseof our experiments we observed that expression of low levelsof HtrA protein delayed bacterial growth, and expression ofa noncleavable HtrA mutant ( ${Delta}$ PDZ2 HtrA), with a significantlylonger clearance time, delayed bacterial growth even further(data not shown). These observations suggest that bacteria benefitsfrom clearing HtrA when its enzymatic activities are no longerrequired and are an indication of the physiological relevanceof these regulatory mechanism in vivo. However, testing ourhypothesis in vivo is beyond the scope of the present studybut will be the focus of our future work.

We noticed that some of the results presented here differ froma previous study on autocleavage of HtrA (23). Mainly, we foundthat the only requirement for autocleavage of HtrA is degradationof a substrate and, in fact, the peptides generated by HtrAduring substrate degradation are sufficient to induce the self-cleavageof HtrA. The previous study indicates that reducing conditionsmust coexist along with substrate degradation to reduce theCys⁵⁷ and Cys⁶⁹ disulfide bridge in HtrA and induce self-cleavage.Consistent with our own results, the C57A+C69G HtrA mutant didnot show increased instability or a higher degree of self-cleavagecompared to wild-type HtrA under any of the conditions tested.The reason for this discrepancy is unclear to us. There aresome minor differences in the experimental conditions betweenboth studies. In addition, the mutant used to test the influenceof Cys57 and Cys69 in the stability of HtrA against autocleavagein the previous study (23) introduced different mutations onthe cysteine residues (C57S+C69S). Potentially, in this mutantthe oxygens that replace the sulfurs from the thiol groups couldintroduce an electrostatic repulsion between the two side chainsthat may destabilize the protein. Consistently, Skorko-Gloneket al. (23) found that the C57S+C69S mutant produced higheramounts of s-HtrA than did the wild type. Conversely, the C57A+C69GHtrA mutant in our study shortens or deletes the side chainsof the two cysteine residues and probably has a milder effecton the three-dimensional structure of HtrA. In consequence,the C57A+C69G HtrA mutant is ideal for assessing the contributionof the disulfide bond to the stability of HtrA against autocleavage.

A previous publication (23) also reported that purified s-HtrAis stable. This result does not contradict our hypothesis thatthe autocleavage of HtrA is a mechanism aiming to eliminatethe excess of HtrA. In fact, we also observed that in a purifiedHtrA preparation with a high proportion of the autocleaved form(used for experiment in Fig. 6), s-HtrA remained stable uponextended incubations at 37°C in the absence of substrate(data not shown). However, consistent with our hypothesis, ifpeptides resulting from substrate hydrolysis are present, s-HtrAis not stable and undergoes subsequent cleavages (Fig. 3B).

An alternative interpretation for our results is that the autocleavageof HtrA is just a side effect of the allosteric activation mechanismof HtrA. In this scenario, peptides from the hydrolysis reactionactivate HtrA and, as a result, this hyperactive protease degradesitself. This simpler model sees the self-cleavage process asa "defect" of the mechanism of allosteric activation. Accordingto this model, s-HtrA production should be produced in significantamounts as long as peptides resulting from the substrate hydrolysisare present in the reaction. However, our experiment illustratingthat repetitive addition of full-length substrate drasticallydelays the autocleavage process contradicts this hypothesis.As described, we did not observe substantial autocleavage inspite of the presence of abundant peptides resulting from substratehydrolysis. It was only after all of the recurrently added full-lengthsubstrate was hydrolyzed and HtrA reverted to its hexamericform that s-HtrA protein did accumulate significantly, indicatingthat bacteria effectively take advantage of the HtrA "defective"allosteric activation mechanism to eliminate the excess of HtrAin the cell.

ACKNOWLEDGMENTS

We thank Daniela Damjanovic for constructing the C57A+C69G HtrAmutant. We are also grateful to Alba Guarne for insightful commentsand critical reading of the manuscript.

This study was supported by a grant from the Canadian Institutesof Health Research (CIHR). J.O. is a recipient of a CIHR salaryaward and an Early Researcher Award from the Ministry of Researchand Innovation.

FOOTNOTES

* Corresponding author. Mailing address: Department of Biochemistry and Biomedical Sciences, Health Sciences Centre, Room 4H24, McMaster University, 1200 Main Street West, Hamilton, Ontario L8N 3Z5, Canada. Phone: (905) 525-9140, ext. 22703. Fax: (905) 522-9033. E-mail: ortegaj{at}mcmaster.ca

Published ahead of print on 19 December 2008.

Supplemental material for this article may be found at http://jb.asm.org/.

REFERENCES

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