Lon-mediated proteolysis of the Escherichia coli UmuD mutagenesis protein: in vitro degradation and identification of residues required for proteolysis

doi:10.1101/gad.12.24.3889

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Vol. 12, No. 24, pp. 3889-3899, December 15, 1998

RESEARCH PAPER
Lon-mediated proteolysis of the Escherichia coli UmuD mutagenesis protein: in vitro degradation and identification of residues required for proteolysis

Martín Gonzalez, Ekaterina G. Frank, Arthur S. Levine, and Roger Woodgate¹

Section on DNA Replication, Repair, and Mutagenesis, National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, Maryland 20892-2725 USA

Abstract

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

Most SOS mutagenesis in Escherichia coli is dependent on the UmuD and UmuC proteins. Perhaps as a consequence, the activityof these proteins is exquisitely regulated. The intracellularlevel of UmuD and UmuC is normally quite low but increases dramaticallyin lon strains, suggesting that both proteins are substrates of theLon protease. We report here that the highly purified UmuD proteinis specifically degraded in vitro by Lon in an ATP-dependent manner.To identify the regions of UmuD necessary for Lon-mediated proteolysis,we performed `alanine-stretch' mutagenesis on umuD and followedthe stability of the mutant protein in vivo. Such an approachallowed us to localize the site(s) within UmuD responsible forLon-mediated proteolysis. The primary signal is located betweenresidues 15 and 18 (FPLF), with an auxiliary site between residues26 and 29 (FPSP), of the amino terminus of UmuD. Transfer of theamino terminus of UmuD (residues 1-40) to an otherwise stableprotein imparts Lon-mediated proteolysis, thereby indicating thatthe amino terminus of UmuD is sufficient for Lon recognition andthe ensuing degradation of theprotein.

[Key Words: UmuD'; ATP-dependent protease; SOS mutagenesis; degradation signal]

	Introduction

Top Abstract Introduction Results Discussion Materials and methods References

Exposure of Escherichia coli to DNA-damaging agents, whether they be natural or man-made, invokes the induction of a numberof unlinked genes required for DNA repair, cell division, anddamage tolerance. This inducible pathway is often referred toas the SOS response (for review, see Friedberg et al. 1995; Kochand Woodgate 1998). One of the hallmarks of the SOS response isthat it is graded in such a way that error-free pathways of DNArepair are induced early (so that DNA fidelity remains high),whereas pathways that may ensure survival under more severe conditions(but are error-prone) are induced much later (Sommer et al. 1998).Key participants in the latter pathway, which is often calledSOS mutagenesis, are the UmuD' and UmuC proteins (Woodgate andLevine 1996; Smith and Walker 1998). Together with RecA and Ssbproteins, the Umu proteins allow DNA polymerase III holoenzymeto traverse otherwise replication-blocking lesions (Rajagopalanet al. 1992; Reuven et al. 1998; Tang et al. 1998), but with aconcomitant reduction in replication fidelity. As a consequence,it is believed that the regulatory mechanisms that determine theexpression and levels of these proteins have evolved so that UmuD'and UmuC are used only as a last resort (Woodgate and Levine 1996).

To achieve such regulation, the cell utilizes transcriptional control (the umu operon is one of the most tightly regulatedin the SOS regulon), together with a variety of post-translationalmechanisms to keep the activity of the Umu proteins to a minimum.The pivotal step in controlling the activity of the Umu proteinsis the RecA-mediated cleavage of UmuD. This cleavage reactionis primarily intermolecular in nature (McDonald et al. 1998a)and results in the removal of the 24 amino-terminal residues fromUmuD to generate UmuD' (Burchhardt et al. 1988; Shinagawa et al.1988). Not only does cleavage activate UmuD' for its mutagenesisfunctions (Nohmi et al. 1988), it also converts UmuD from a substratethat is sensitive to the Lon protease to one that is relativelyinsensitive to Lon (Frank et al. 1996a). The increased stabilityof UmuD' is problematic in that it is likely to result in an increasein aberrant mutagenesis. The cell generally avoids such problems,however, by targeting UmuD' for degradation by the ClpXP protease(Frank et al. 1996a). Both UmuD and UmuD' form homodimers (Burckhardtet al. 1988; Woodgate et al. 1989; Battista et al. 1990); butunder conditions of limited cleavage (as might be expected incells exposed to mild DNA damage), UmuD' preferentially interactswith the more abundant UmuD protein to form a UmuD/D' heterodimerand this complex directs ClpXP degradation of UmuD' (Frank etal. 1996a). All three dimer species of UmuD and UmuD' (the individualhomodimers and the heterodimer) are capable of interacting withUmuC but with varying affinities (Woodgate et al. 1989; Franket al. 1996a,b; Jonczyk and Nowicka 1996). The UmuC protein, inthe absence of interacting partners, is also highly labile andhas also been shown to be a substrate of the Lon protease in vivo(Frank et al. 1996a).

It is evident that the extent of SOS mutagenesis is contingent on the proper protein-protein interactions and the resultingstability of these complexes. The regulated proteolysis of theUmu proteins therefore provides a critical mechanism by whichthe cell maintains the correct levels of the Umu proteins, bothduring and after exposure to DNA damage (Gonzalez et al. 1998;Sommer et al. 1998). The question remains as to what featuresthese proteins possess that specifically target them for degradation.There are numerous reports implicating the carboxyl terminus inprotease recognition. For example, mutants of the P22 Arc repressoror the $lambda$ cI repressor were found to be unstable, and this instabilityis dependent on the carboxy-terminal 5 amino acids (Bowie andSauer 1989; Parsell et al. 1990; Keiler et al. 1995). These 5amino acids are nonpolar residues, and any change in them to apolar or charged carboxyl terminus make the protein stable (Parsellet al. 1990; Keiler et al. 1995). Similarly, recent work has demonstratedthat addition of a nonpolar 11-amino-acid carboxy-terminal sequence,encoded by E. coli ssrA, to peptides results in their rapid degradation(Tu et al. 1995; Keiler et al. 1996). The carboxyl terminus ofthe Mu transposase, MuA, is known to have a role in ClpX recognitionand disassembly of the transposase-DNA complex as well as in itsdegradation by ClpXP (Levchenko et al. 1995; Levchenko et al.1997). In contrast to the nonpolar nature necessary for recognitionof the SsrA-tagged fusions, the MuA carboxyl terminus is positivelycharged (Levchenko et al. 1995, 1997).

Comparison of Lon substrates yields no identifiable features that might function in substrate recognition. The carboxyl terminusof the Lon substrate, SulA, was demonstrated to be sufficientfor recognition, but not for degradation, of a fusion of $beta$ -galactosidasewith the carboxy-terminal 20 amino acids of SulA (Higashitaniet al. 1997).

In an attempt to identify the signal in UmuD that targets it for degradation by Lon, we have used a dual approach; first,we demonstrate that as predicted from our previous in vivo studies(Frank et al. 1996a), highly purified UmuD protein is a substrateof the Lon protease in vitro; second, we use the in vivo assayto monitor the susceptibility of various mutant UmuD proteinsto proteolysis by Lon. Our results suggest that certain regionswithin the amino-terminal tail of UmuD are necessary and sufficientfor Lon-mediated degradation of UmuD and that these signals canbe transferred to an otherwise stable protein to impart Lon-mediatedproteolysis.

	Results

Top Abstract Introduction Results Discussion Materials and methods References

In vitro degradation of UmuD

Previously, we have demonstrated that the UmuD protein is highly labile in vivo and is stabilized in lon cells (Frank et al. 1996a). To determine whether UmuD stabilityis directly related to the Lon protease, we incubated highly purifiedUmuD and Lon proteins in the presence or absence of exogenousATP (Fig. 1A). To maximize the in vitro activity of Lon (Van Melderenet al. 1996), the reaction also utilized an ATP regeneration system.As demonstrated clearly in Figure 1A, the Lon protease degradedUmuD in the presence of ATP. No detectable degradation productswere observed, indicating that degradation proceeds in a processivemanner (data not shown). In contrast, no degradation was evidentin the absence of ATP. On the basis of these experiments, we calculatethat the in vitro half-life of UmuD is ~30 min (Fig. 1B). Theseresults clearly demonstrate, in concordance with our in vivo observations(Frank et al. 1996a), that UmuD is specifically recognized anddegraded by the Lon protease in vitro.

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Figure 1. In vitro degradation of UmuD by Lon. (A) Highly purified UmuD and Lon proteins were incubated at 37°C in the presence or absence of ATP, as described in Materials and Methods. An aliquot was removed at the indicated time, electrophoresed in 17% SDS-polyacrylamide gels, and visualized after staining with Coomassie brilliant blue. (B) Kinetics of UmuD degradation. These data were generated by quantifying the gels described in A, on a ChemiImager 4000 low-light imaging system.

Specificity of Lon-mediated degradation of UmuD

The Lon protease has long been known for the housekeeping role it has in the removal of abnormal or damaged cellular proteins(for review, see Gottesman 1996). Lon also functions in the selectivedegradation of proteins such as SulA (Huisman and D'Ari 1981;Mizusawa and Gottesman 1983), $lambda$ N (Maurizi 1987), CcdA (Van Melderenet al. 1996), RcsA (Torres-Cabassa and Gottesman 1987; Stout etal. 1991), and UmuC (Frank et al. 1996a). To date, little is knownas to what `signature' identifies a protein as a substrate ofLon. As noted above (Fig. 1), UmuD is degraded by Lon in the presenceof ATP. To determine the extent of Lon specificity, we purifiedan engineered version of the post-translationally processed UmuDprotein, UmuD', and examined the effects of Lon on the stabilityof UmuD'. In vivo, UmuD' appears relatively insensitive to Londegradation (Frank et al. 1996a). We reasoned, therefore, thatassaying the stability of UmuD' would be a rigorous test of thein vitro specificity of the Lon protease. As shown in Figure 2A,the UmuD' protein is relatively stable after a 1-hr incubationin the presence of Lon, thus verifying our previous observationsin vivo (Frank et al. 1996a).

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Figure 2. In vitro specificity of Lon. (A) Highly purified UmuD and UmuD' proteins were individually incubated with ATP in the presence (open bars) or absence (stippled bars) of Lon at 37°C for 1 hr. Reactions were processed, visualized, and quantitated as described in Fig. 1. (B) Limited $alpha$ -chymotrypsin digest of either purified UmuD or UmuD' was performed at 25°C for 20 min with increasing concentrations of $alpha$ -chymotrypsin. The concentrations of $alpha$ -chymotrypsin used were 0 ng (lanes 1,6), 5 ng (lanes 2,7), 50 ng (lanes 3,8), 250 ng (lanes 4,9), and 500 ng (lanes 5,10). Reactions were electrophoresed and visualized as described in Materials and Methods. The positions of intact UmuD and UmuD' are indicated at left.

One possible explanation for these results is that UmuD and UmuD' possess very different tertiary structures (Guzzo et al.1996). To test this hypothesis, we examined the effect of chymotrypsindigestion on both UmuD and UmuD'. Under limiting protease conditions,UmuD was efficiently processed to a species of similar electrophoreticmobility as UmuD' (Fig. 2B). In contrast, however, no significantdegradation of UmuD' was observed. This suggests that the globularstructures of UmuD and UmuD' (Peat et al. 1996a,b; Ferentz etal. 1997) are essentially similar and that the 24-amino-acid aminoterminus of UmuD does not destabilize UmuD by imparting majorstructural changes not evident in UmuD'. On the basis of theseobservations, the amino-terminal 24 amino acids of UmuD appearto be all that is efficiently cleaved by chymotrypsin during the20-min incubation time. Similar results were obtained after trypticdigestion of UmuD (D. Wall and W. Hendrickson, pers. comm.).

Identification of the regions in UmuD necessary for Lon degradation

The fact that UmuD, but not UmuD', is a substrate of Lon suggests that the signal conferring Lon-mediated proteolysis is mostlikely located in the very amino terminus of UmuD that is naturallyabsent in UmuD'. To identify these regions, we have taken advantageof the fact that the orthologous Salmonella typhimurium UmuD proteinalso appears to be a substrate of Lon (Gonzalez et al. 1998).Therefore, we hypothesized that the signal for Lon-mediated degradationwould be located within the amino-terminal residues of UmuD thatare identical in the two proteins. Overall, the two UmuD proteinsshare 73% identity, but as seen in Figure 3A, the amino terminiare more diverged with only 54% identical residues in the regionfrom the amino terminus to the RecA-mediated post-translationalcleavage site. To test our hypothesis, we constructed plasmid-encodedmutants of E. coli UmuD in which the wild-type residues (identicalor highly conserved in S. typhimurium UmuD) were substituted with4 alanine residues (Fig. 3B). Transformed lon⁺ cells expressing the individual mutant UmuD proteins were grownto early logarithmic phase at which time chloramphenicol was addedto block further protein synthesis. Samples were taken at subsequenttime intervals and UmuD visualized by standard Western blottingtechniques. Figure 4A shows time course experiments for the individualUmuD `alanine-stretch' mutants. The half-life of wild-type UmuDwas calculated to be ~11 min and was similar to that of the UmuD9-4and UmuD26-4 mutants. In striking contrast, the UmuD15-4 alaninemutant was appreciably stabilized with a half-life of ~38 min.In parallel experiments, UmuD and all the UmuD alanine-stretchmutants were further stabilized (half-life >60 min) in a lon background (data not shown). The marked stabilization of UmuD154indicates, therefore, that amino acids 15-18 (FPLF) of UmuD areimportant for efficient Lon-mediated degradation, but the increasedstability noted in a lon background suggests that other regions of UmuD are also importantfor efficient Lon recognition.

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Figure 3. Proteins used to identify the Lon recognition signal of UmuD. (A) E. coli and S. typhimurium UmuD proteins are both substrates of Lon (Gonzalez et al. 1998

). Their primary amino acid sequences were aligned using the program Geneworks, and areas that are boxed indicate regions that are 100% conserved between the two proteins. Overall, the proteins are 73% identical, but most divergence occurs in the amino- and carboxy-terminal tails. (B) The amino terminus of the UmuD alanine-stretch mutants. Areas boxed indicate the multiple alanine substitutions made within the UmuD amino terminus for each mutant protein. The normal post-translational cleavage site is located between Cys-24 and Gly-25. The positions of the genetically engineered silent restriction sites for NdeI and SacII in the umuD gene are indicated at their approximate position in the corresponding UmuD protein.

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Figure 4. Stability of the UmuD mutants in a lon⁺ strain. Cultures were grown in LB medium at 37°C to logarithmic phase at which time chloramphenicol was added to block protein synthesis. An aliquot was removed at the indicated times thereafter. Whole cell protein extracts from an equivalent number of cells were electrophoresed in 17% SDS-polyacrylamide gels, blotted onto an Immobilon P membrane, probed with anti-UmuD antibody, and quantitated as described in Materials and Methods. (A) Single region (4-alanine stretch) mutants of UmuD. ( $open circle$ ) Wild-type UmuD; ( $triangle$ ) UmuD9-4; (

) UmuD15-4; ( $diamond$ ) UmuD26-4. (B) The double region (4 plus 4 alanine stretch) mutants of UmuD. ( $open circle$ ) Wild-type UmuD; ( $black-triangle$ ) UmuD15/9; ( $black-diamond$ ) UmuD26/9; (

) UmuD26/15. All experiments were performed two to three times with no significant variation in results.

To determine the region of UmuD that might be required for complete stabilization, we created plasmids expressing UmuD mutants,each consisting of four alanine stretches within two regions ofthe amino terminus (see Fig. 3B). The kinetics of degradationof the double alanine-stretch mutant, UmuD15/9 were very similarto that of UmuD15-4 (Fig. 4, cf. A and B), and therefore no additionalrole in Lon-mediated degradation could be assigned to UmuD9-4.Likewise, UmuD26/9 behaved identically to the individual alanine-stretchmutants UmuD9-4 and UmuD26-4, resulting in a half-life of ~12min (Fig. 4B). However, substitution of four alanine amino acidsat residues 26-29 in the relatively stable UmuD15-4 mutant resultedin a dramatic increase in stability. The half-life of UmuD26/15is >1 hr (Fig. 4B), and the decay kinetics for UmuD26/15 in alon⁺ background are similar to those of the wild-type UmuD proteinin a lon background (data notshown).

These data support a model in which the Lon protease recognizes two specific regions within the amino terminus of UmuD, theprimary site being located between residues 15 and 18 and theauxiliary site between residues 26 and 29. Note that the auxiliarysite alone is insufficient to target UmuD degradation (Fig. 4A),explaining why UmuD' (which lacks the primary Lon recognitionsignal but possesses the secondary site) is insensitive to proteolysisby Lon (Fig. 2A; Frank et al. 1996a).

Functional activity of the UmuD alanine-stretch mutants

One possible explanation for our finding that certain mutant UmuD proteins are rendered insensitive to Lon is that we havegrossly altered the conformation of the UmuD protein and, as aconsequence, made it less susceptible to Lon proteolysis. A criticalstep in the mutational process is the RecA-mediated self-cleavageof mutagenically active UmuD to mutagenically active UmuD' (Burckhardtet al. 1988; Nohmi et al. 1988; Shinagawa et al. 1988). UmuD'then associates with UmuC, RecA, and DNA polymerase III to promoteerror-prone trans-lesion DNA synthesis (Rajagopalan et al. 1992;Reuven et al. 1998; Tang et al. 1998). A simple, but indirect,assay of the conformational structure of the various UmuD mutantsis, therefore, an ability to promote damage-inducible SOS mutagenesisin vivo. Presumably strains that are mutable express a UmuD proteinthat can undergo cleavage as well as the subsequent protein-proteininteractions necessary for trans-lesion DNA synthesis. Such analysisrevealed, however, that the majority of the UmuD alanine-stretchmutants do not promote significant levels of SOS mutagenesis (Fig.5A). The lone exception is UmuD9-4, which displays a slightlygreater mutation frequency than wild-type UmuD.

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Figure 5. Functional activity of the UmuD alanine-stretch mutants. (A) The ability of the alanine-stretch mutants to function in SOS mutagenesis was assayed using strain RW126 harboring the low-copy-number UmuC-expressing plasmid pRW274 and a compatible plasmid expressing each of the individual UmuD alanine mutants. Strain RW126 carries an ocher mutation in hisG [hisG4(Oc)] that renders it auxotrophic for histidine. In the presence of functional Umu proteins it can, however, revert to His⁺. The number of His⁺ revertants per plate after exposure to MMS represents the mean number from a minimum of three cultures. (B) Western blot analysis of the RecA-mediated self cleavage reaction in vivo. The ability of the alanine-stretch mutants to undergo post-translational cleavage was assayed in the lexA51(Def) recA730 strain RW244. This strain constitutively expresses all LexA-regulated proteins (including the Umu proteins) and promotes constitutive cleavage of UmuD in the absence of exogenous DNA damage. The positions of UmuD and UmuD' are indicated by arrows at left. (C) The ability of the UmuD alanine mutants to act as an enzyme in the intermolecular UmuD cleavage reaction. The UmuDK97A protein cannot undergo intramolecular cleavage because it carries a mutation at the active site of UmuD. It can, however, serve as a substrate in the intermolecular cleavage reaction if a UmuD enzyme is provided in trans (in our case, the various alanine-stretch mutants). Cleavage of the UmuDK97A protein was monitored in strain RW244 in the absence or presence of the individual UmuD alanine mutants and visualized by Western blot analysis as described in Materials and Methods. The positions of UmuD and UmuD' are indicated by arrows at left.

Such findings prompted us to directly assay the ability of the mutant UmuD protein to be processed to UmuD' (Fig. 5B). Ina recA730 background, wild-type UmuD is converted to UmuD' with>90% efficiency (Fig. 5B; Shinagawa et al. 1988; Woodgate andEnnis 1991). In concordance with the in vivo mutagenesis assay,UmuD9-4 was converted to UmuD' with efficiency similar to thatof the wild-type protein. Interestingly, despite its inabilityto promote mutagenesis, ~50% of UmuD26/9 was converted to UmuD',indicating that the mutant protein probably retains the same overallstructure as the wild-type UmuD protein. Given that the resultantUmuD' protein (UmuD'26-4) remains functionally inactive for mutagenesis(Fig. 5A), it would argue that residues 26-29 are important forthe subsequent activity of UmuD'. These residues are absolutelyconserved in all of the bona fide UmuD(D') homologs identifiedto date (Woodgate and Levine 1996).

We have recently demonstrated that UmuD cleavage predominantly occurs via an intermolecular reaction in vivo (McDonald etal. 1998a). That is, one monomer of UmuD (or UmuD') can act asan enzyme to facilitate the cleavage of another substrate UmuDmonomer (McDonald et al. 1998a). Given the fact that the alanine-stretchmutants are in close proximity to (or actually span) the cleavagesite, we hypothesized that such changes might simply alter theability of the protein to act as a substrate molecule. However,if the mutant protein retains the same overall globular structureof the wild-type protein, it should still be capable of actingas an enzyme in the intermolecular cleavage reaction (McDonaldet al. 1998a). To test this hypothesis, the mutant plasmids werecotransformed with pKSD10 (a compatible low-copy-number plasmidexpressing UmuDK97A) into a recA730 strain. The UmuDK97A proteinexpressed by pKSD10 is unable to undergo intramolecular self-cleavagebecause it has a mutation at the catalytic active site but isable to undergo intermolecular cleavage as a substrate moleculeif a UmuD enzyme is provided in trans (McDonald et al. 1998a).As shown in Figure 5C, all of the alanine-stretch mutants (15-4,26-4, 15/9, and 26/15) are able to act as enzymes in the intermolecularcleavagereaction.

The assays described above not only allow us to conclude that the globular bodies of the mutant 15-4, 26-4, 15/9, and 26/15UmuD proteins are similar to that of the wild-type protein, theyalso reveal the multiple types of interactions that are mediatedby the amino terminus of UmuD (seeDiscussion).

Transfer of the UmuD degradation signal

Our finding that the mutant UmuD proteins appear to retain the same overall structure as the wild-type protein supports ournotion that the region of UmuD identified in our mutational studiesis a bona fide Lon recognition/degradation signal. One obvioustest of this hypothesis is an ability of these sequences to impartinstability on an otherwise stable protein. To test this hypothesis,we constructed a plasmid (pKSD-PRP) expressing a chimeric geneencoding the first 40 amino acids of UmuD fused to a 7-amino-acidlinker joined to the entire Streptoalloteichus hindustanus Bleprotein. The S. hindustanus ble gene encodes a small, stable proteinthat provides resistance to the antibiotics of the phleomycinfamily (Dumas et al. 1994; Gatignol et al. 1988). For convenience,the S. hindustanus ble gene product will be referred to as thephleomycin resistance protein (or PRP). The wild-type PRP is itselfquite stable when assayed in our wild-type background (data notshown). In contrast, the UmuD-PRP fusion is unstable in the lon⁺ background and displays a half-life of ~9 min (Fig. 6). Interestingly,UmuD-PRP demonstrates a marked increase in stability when assayedin a lon strain (half-life of ~38 min), indicating that the UmuD-PRP fusionis degraded in a Lon-dependent fashion (Fig. 6). Furthermore,subsequent experimentation demonstrated that residues 1-29 ofUmuD are sufficient to impart Lon recognition and degradationof the PRP similar to that seen with the 40-amino-acid fusion(data not shown). By comparison, a UmuD-PRP fusion protein containingthe two alanine-stretch mutants located between residues 15 and18 and 26 and 29, was stable, and the decay kinetics of the UmuD26/15-PRPfusion in a lon⁺ background (half-life of ~30 min) were similar to those of thewild-type UmuD-PRP fusion in the lon background (Fig. 6). It is important to note, however, that theUmuD-PRP fusion, as well as the UmuD26/15-PRP fusion, is obviouslydegraded by at least one additional protease other than Lon. Theseresults therefore confirm our hypothesis that residues 15-19 and26-29 of UmuD are recognized by Lon and that these sequences conferLon-mediated instability on an otherwise stable protein.

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Figure 6. The amino-terminal 40 amino acids of UmuD are sufficient to target the PRP for degradation by Lon in vivo. The amino-terminal 40 amino acids of UmuD were fused to the amino terminus of PRP to create a UmuD-PRP fusion protein. Western blot analysis of UmuD-PRP stability was determined in lon⁺ (EC10) and lon (EC18) cells. Stability of the plasmid expressed UmuD26/15-PRP fusion protein was also assessed in the lon⁺ strain (EC10). UmuD26/15-PRP describes a similar fusion construct except that the first 40 amino acids of UmuD contain the UmuD26/15 alanine-stretch mutations described in Figure 3B. Cultures were grown in LB medium at 37°C to logarithmic phase at which time chloramphenicol was added to block protein synthesis. An aliquot was removed at the indicated times thereafter. Whole cell protein extracts from an equivalent number of cells were electrophoresed in 17% SDS-polyacrylamide gels, blotted onto an Immobilon P membrane, and probed with antibodies directed against the amino-terminal 24 amino acids of UmuD. This antibody demonstrated limited cross-reactivity with the 8-alanine-substituted UmuD26/15-PRP, and as a consequence, the UmuD26/15-PRP mutant protein was visualized using anti-PRP antibodies.

	Discussion

Top Abstract Introduction Results Discussion Materials and methods References

Trans-lesion DNA synthesis in E. coli involves numerous protein-protein interactions, all of which are vital for ensuringcontinued survival of the organism when challenged with variousstressful conditions. Many of the protein-protein interactionsfunction in maintaining the proper equilibrium of the Umu proteinsso that SOS mutagenesis occurs only as a last resort. The E. coliLon protease contributes to this process by regulating the levelsof the UmuD and UmuC proteins in vivo (Frank et al. 1996a). Ourstudies demonstrate that the degradation of UmuD is directly relatedto the proteolytic action of Lon and occurs in an ATP-dependentfashion. Furthermore, we have shown that the Lon protease displaysstriking specificity for UmuD in vitro, thereby mirroring ourprevious observations in vivo (Frank et al. 1996a). The relativerate of degradation of UmuD, however, is much more rapid in vivo(Fig. 4) than in vitro (Fig. 1A), but such findings are also characteristicof other Lon substrates such as $lambda$ N (Maurizi 1987), CcdA (Van Melderenet al. 1996), and a SulA fusion protein (Sonezaki et al. 1995).

There is an emerging consensus that the termini of labile proteins, both amino and carboxyl, have a vital role in the targetingof many proteins for rapid degradation. For example, a carboxy-terminaltagging system in E. coli is dedicated to identifying stalledribosomes at the 3' end of a truncated mRNA and tagging the carboxylterminus of the respective truncated protein with a nonpolar 11-amino-acid(AANDENYALAA) peptide (Tu et al. 1995; Keiler et al. 1996). Thiscarboxy-terminal addition, a function of the SsrA RNA, resultsin the rapid degradation of the fusion protein (Keiler et al.1996). Moreover, Gottesman et al. (1998) identified the proteasesresponsible for the degradation of the SsrA-tagged peptides asthe ClpAP and ClpXP proteases. In addition, the membrane-boundHflB protease of E. coli is also known to degrade SsrA-taggedpeptides (Herman et al. 1998). Because HflB is membrane-bound,Herman et al. (1998) postulate that the primary role of HflB isto act upon abnormal membrane proteins. The SsrA tag is composedprimarily of nonpolar amino acids that are normally found buriedwithin the protein. The nonpolar nature of the SsrA tag is thereforelikely to resemble exposed areas of damaged and/or denatured proteinsthat are known to be rapidly degraded by many of the E. coli cytoplasmicproteases, possibly including ClpAP and ClpXP (for review, seeGottesman 1996).

The bacterial N-end rule reflects a proteolytic pathway whose specificity is dictated by the amino-terminal amino acid (Tobiaset al. 1991). The pathway was identified by assessing the stabilityof engineered $beta$ -galactosidase fusions, each beginning with a differentamino acid. The protease in E. coli responsible for the degradationof the unstable N-end rule substrates was identified as ClpAP(Tobias et al. 1991). This protease was also shown to be responsiblefor the degradation of a fusion protein consisting of the first40 amino acids of ClpA fused to the amino terminus of $beta$ -galactosidase(Gottesman et al. 1990). When wild-type ClpA stability was assessedin vivo, it was found to be unstable, albeit at a much reduceddegradation rate when compared to the rate of degradation of theClpA- $beta$ -galactosidase fusion (Gottesman et al. 1990). Much likethe SsrA tag described above, the ClpA- $beta$ -galactosidase fusionpresumably places the ClpAP recognition signal in a context allowinggreateraccessibility.

The amino- and carboxy-terminal recognition pathways described above most likely function because terminal recognition signalsprovide easier access for the protease. The UmuD' crystal structurewas determined recently and the amino-terminal region (startingat residue 32) of UmuD' was described as extended and unstructured(Peat et al. 1996a,b). Therefore, if one assumes that UmuD andUmuD' share the same globular structure (Fig 2A; Ferentz et al.1997), the entire amino terminus (residues 1-40) is likely tobe extended and possibly unstructured. The experiments presentedhere suggest that this extended amino terminus of UmuD is essentialfor efficient Lon-mediated degradation. Using alanine-stretchmutagenesis, we have localized the primary Lon recognition signalin UmuD to residues Phe-15, Pro-16, Leu-17, and Phe-18. Multiplealanine substitutions at these residues result in significantstabilization of UmuD, strongly suggesting that this specificregion of the UmuD protein is recognized by the Lon protease.Interestingly, multiple alanine mutations at residues 15-18 inunison with alanine substitutions at residues 26-29 result inalmost complete stabilization of UmuD. In contrast, multiple alaninemutations spanning residues 26-29 had no apparent affect on UmuDdegradation. This suggests that residues 26-29 can function ineither stabilizing the Lon-UmuD interaction at the putative Lonrecognition site (residues 15-18) or in maintaining the accessibilityof the amino terminus for Lon recognition. The 26-4 site is thereforeconsidered an auxiliary site in that it only functions in Lon-mediatedproteolysis in concert with the primarysite.

As noted earlier, the S. typhimurium UmuD protein is also a substrate of Lon (Gonzalez et al. 1998). The auxiliary site (residues26-29) in the S. typhimurium UmuD protein is identical to thatof the E. coli protein. By comparison, the primary site is notidentical but is highly conserved (FPLF_(Ec) $right-arrow$ LPFF_(St)). Moreover,the UmuD homolog RumA, which is found on the incJ plasmid R391as part of the RumAB operon, also has an identical auxiliary siteand a highly conserved primary site (FPLF_(Ec) $right-arrow$ IPLF_(RumA)) (Kulaevaet al. 1995). RumA, however, is not degraded by the Lon protease(M. Gonzalez, unpubl.). A possible explanation for this findingis that the amino acid sequences immediately surrounding the primarysite of RumA are highly charged in comparison to the same regionin the E. coli and S. typhimurium UmuD proteins (Woodgate andLevine 1996). Such findings suggest, therefore, that the majordeterminants leading to Lon-mediated proteolysis are not primaryamino acid sequences per se but, rather, an exposed stretch ofnonpolar amino acid residues and the surrounding protein environment.Site-directed mutagenesis of the primary and auxiliary sites,as well as mutagenesis of the surrounding residues, should furtherelaborate the Lon-UmuD interaction necessary fordegradation.

The amino terminus of UmuD assumes no identifiable secondary structure, and no sequence similarity is evident between UmuDand other known substrates of Lon. Higashitani et al. (1997) identifieda region of similarity between two Lon substrates, the $lambda$ N proteinand the E. coli SulA protein. However, whereas fusion of the carboxy-terminal20 amino acids of SulA to the carboxyl terminus of $beta$ -galactosidasewas sufficient for Lon binding, it was not enough to promote Lon-mediatedproteolysis (Higashitani et al. 1997). In contrast, our resultsdemonstrate that fusion of the amino terminus of UmuD (residues1-40) to an otherwise stable PRP is all that is necessary to targetthe protein for Lon-mediated proteolysis (Fig. 5). Furthermore,mutations in the amino terminus of the UmuD-PRP fusion, identicalto those found in the stable UmuD26/15 mutant, inhibited Lon-mediateddegradation (Fig. 5). The ability to transfer the Lon recognitionsignal of UmuD and thereby provoke Lon-mediated degradation signifiesthat the amino terminus of UmuD not only comprises the informationnecessary for binding but also provides the foundation for degradationof thesubstrate.

Our finding that the two regions of the UmuD amino terminus necessary for Lon-mediated degradation span the UmuD cleavagesite (Cys-24 $right-arrow$ Gly-25) raises the intriguing possibility thatLon recognition and degradation of UmuD is in direct competitionwith the RecA-mediated self-cleavage of UmuD that occurs duringthe SOS response (Fig. 7). Such competition allows exquisite post-translationalregulation of UmuD and provides yet another mechanism by whichUmu-dependent error-prone trans-lesion DNA synthesis is regulated(Woodgate and Levine 1996; Sommer et al. 1998). Clearly, recognitionof protein termini is a common mechanism employed by many proteases.The targeting of the Lon protease to the UmuD amino terminus isone of the critical mechanisms that ensures cell survival in theface of irreparable DNA damage at minimal mutational cost.

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Figure 7. Lon degradation vs. RecA processing of the UmuD SOS mutagenesis protein. Competition for UmuD by Lon and RecA provides one mechanism whereby the level of mutagenically active UmuD' protein is kept to a minimum. In the absence of exogenous DNA damage, the equilibrium of the reaction favors Lon degradation and most of the UmuD protein is rapidly degraded before it is converted to UmuD' (Gonzalez et al. 1998

). After DNA damage, when the need for functional Umu proteins increases, the equilibrium begins to shift toward the RecA-mediated cleavage of UmuD to UmuD'. This cleavage reaction most likely occurs as a consequence of RecA altering the conformation of UmuD's amino-terminal tail so as to bring the cleavage site of UmuD into close proximity with the active site (McDonald et al. 1998a

). Initially, most of the UmuD' reassociates with the more abundant UmuD protein to form a UmuD/D' heterodimer that targets UmuD' for proteolysis by ClpXP (Frank et al. 1996a

) (not shown). If cellular damage is severe, more UmuD' is generated than is degraded, and these will associate to form a stable UmuD' homodimer (Frank et al. 1996b

	Materials and methods

Top Abstract Introduction Results Discussion Materials and methods References

Bacterial strains and plasmids

Four E. coli K-12 strains were utilized to investigate Lon-mediated degradation of UmuD in vivo. All four strains carry alexA(Def) mutation (either the mis-sense lexA51(Def) allele orthe Tn5 insertion allele, lexA71(Def)::Tn5), which results inconstitutive expression of LexA-regulated genes (including theumu operon) in the absence of exogenous DNA damage. They alsocarry a deletion of the chromosomal umu operon (either $Delta$ umuDC595::cator $Delta$ umuDC596::ermGT) that allows us to assay the stability ofour various plasmid-encoded umuD mutants in the absence of contaminatingchromosomally encoded UmuD. Strains EC10 [relevant genotype: recA⁺ lexA51(Def) $Delta$ umuDC596::ermGT] and EC18 [recA⁺ lexA51(Def) $Delta$ umuDC596::ermGT lon146::Tn10] (Frank et al. 1996a)were used to characterize the stability of the UmuD alanine-stretchmutants and the UmuD-PRP fusions. RW126 [recA718 srlC300::Tn10lexA71(Def)::Tn5 $Delta$ umuDC595::cat hisG4(Oc)] (Ho et al. 1993), harboringpRW274 (see below), was used to measure damage-induced Umu-dependentmutagenesis. To determine the ability of the various UmuD alanine-stretchmutants to undergo RecA-mediated cleavage to UmuD', we utilizedstrain RW244 [recA730 srlC300::Tn10 lexA51(Def) $Delta$ umuDC595::cat].In a wild-type background, UmuD cleavage is normally damage inducible,but in certain coprotease-proficient recA mutants, like recA730(Shinagawa et al. 1988; Woodgate and Ennis 1991), it is renderedconstitutive.

All of the plasmid constructs described below express their respective protein from the natural LexA-regulated umu operonpromoter-operator. Normally, expression of the Umu proteins isdamage inducible, but as noted above, all of the strains usedin this study carry lexA(Def) mutations, thereby resulting indamage-independent constitutive expression of the various Umuproteins.

Construction of all of the alanine-stretch mutants, except pKSD15/9, was accomplished by digesting the pBR322-derived UmuD-expressingplasmid pJM125 (McDonald et al. 1998b) with NdeI and SacII, andthe resulting ~90 bp fragment containing the 5' end of the umuDgene was replaced with four annealed oligonucleotides (of ~90bp) corresponding to the multiple desired alanine changes (Fig.3B). For the ease of identification, the DNA sequence coding forthe 4 alanine substitutions also created a novel NotI restrictionsite in the umuD gene. pKSD15/9 was created by digesting pKSD15-4with NotI and NdeI, and the ~42 bp fragment was replaced withtwo annealed oligonucleotides (of ~42 bp) that encoded the UmuD15/9mutations. All of the UmuD alanine-stretch mutant plasmids weresequenced (Lark Technologies Inc., Houston, TX) to ensure thatthey did not contain any additional nucleotidechanges.

The UmuD-PRP-expressing plasmid (pKSD-PRP) was constructed by cloning the appropriately modified ~617-bp BclI-NotI fragmentfrom pUT649 (Cayla, Toulouse, France) into the BsaBI-digestedplasmid pJM125 (McDonald et al. 1998b). The resultant plasmidpKSD-PRP is a pBR322-based vector expressing the amino-terminal40 amino acids of UmuD fused to a 7-amino-acid linker followedby the entire PRP. pKSD26/15-PRP, which creates the alanine-stretchmutations in pKSD-PRP identical to those mutations in pKSD26/15,was constructed by ligating a ~790-bp SacII-PvuI fragment frompKSD26/15 into the similarly digested pKSD-PRPvector.

pKSD10 (UmuDK97A) was constructed by cloning the ~1 kb BglII fragment from pRW414 (McDonald et al. 1998a) into the BglII-BamHI-digestedvector pRW362 (Frank et al. 1996b). pRW274 (umuC⁺) was constructed by digesting pRW134 (umuD'C⁺) (Ennis et al. 1995) with NcoI and the site blunt-ended withPol I (Kf) so as to introduce a frameshift mutation in the religatedumuD' gene. Both pKSD10 and pRW274 are derived from the low-copy-numberspectinomycin-resistance plasmid pGB2 (Churchward et al. 1984)and are compatible with the pBR322-derived plasmids describedabove.

Proteins

Purified Lon protease was a gift from Michael Maurizi (National Institutes of Health, Bethesda, MD). UmuD and UmuD' were purifiedas described (Frank et al. 1993). Creatine kinase was purchasedfrom Sigma (St. Louis, MO), and the $alpha$ -chymotrypsin from bovinepancreas was purchased from Boehringer Mannheim (Indianapolis,IN).

In vitro protein degradation

Purified UmuD (12.5 µM) was incubated with Lon (0.5 µM) in buffer containing 50 mM Tris-HCl (pH 8.0), 10 mM MgCl₂, 1 mM DTT,50 mM creatine phosphate, and 80 µg/ml creatine kinase. In thereactions containing ATP the concentration of ATP was 4 mM. Thereaction mixture was incubated at 37°C and a 25-µl aliquot wasremoved at the specified times and added to 4× SDS sample buffer(Sambrook et al. 1989). Samples were subsequently visualized by17% SDS-PAGE, stained with Coomassie Blue R-250. Identical reactionconditions (UmuD or UmuD' at 12.5 µM ± Lon 0.5 µM were employedwhen assaying Lon specificity except that only a 1 hr time pointwasassayed.

Limited $alpha$ -chymotrypsin digests (10 µl) contained 65 µM protein substrate (either UmuD or UmuD') and increasing concentrationsof $alpha$ -chymotrypsin (0, 5, 50, 250, and 500 ng final concentration)in a buffer containing 20 mM Tris-HCl (pH 7.5), 50 mM NaCl, 1mM DTT, and 0.1 mM EDTA. The reactions were incubated at 25°Cfor 20 min and visualized by a 17% SDS-polyacrylamide gel stainedwith Coomassieblue.

Measurement of UmuD mutant stability

The stability of the UmuD alanine-stretch mutants, as well as UmuD fusions, was assayed as described previously (Frank etal. 1996b). Briefly, cells were grown in Luria-Bertani mediumat 37°C until they reached early exponential phase. At time zero,100 µg/ml chloramphenicol was added to the medium to block proteinsynthesis and a 1.5-ml aliquot was removed at the indicated times.Cells were harvested by centrifugation and the resulting cellpellet resuspended in 4× SDS sample buffer. Aliquots representingequal cell numbers were electrophoresed on 17% SDS-polyacrylamidegels. Proteins were transferred to an Immobilon P membrane (Millipore)and subsequently probed with polyclonal antibodies raised againstUmuD/UmuD' (Frank et al. 1996b). Visualization of the UmuD-PRPprotein was performed using polyclonal antibodies to the extreme24-amino-acid N-terminus of UmuD raised in rabbits by CovanceLaboratories (Vienna, VA). Because of limited cross-reactivityof the UmuD antibodies with UmuD26/15-PRP, UmuD26/15-PRP was visualizedusing polyclonal anti-PRP antibodies (Cayla, Toulouse, France).The transferred proteins were visualized on Kodak Bio-MaxMR filmusing the Western light chemiluminescent assay (Tropix, Bedford,MA). Quantitation was performed on a ChemiImager 4000, low-lightimaging system (Alpha Innotech Corporation, San Leandro, CA).All experiments were performed two to three times with no significantvariation inresults.

Ability of UmuD mutants to undergo RecA-mediated intermolecular cleavage

RecA-mediated cleavage of various UmuD alanine-stretch mutants was followed in strain RW244 essentially as described above.However, because this assay only determines the steady-state levelof the UmuD (or UmuD') protein, no chloramphenicol was added tothe reaction and only one time point was taken at timezero.

The ability of the various alanine-stretch mutants to act as an enzyme and promote intermolecular UmuD cleavage was assayedin strain RW244/pKSD10 (UmuDK97A). UmuDK97A has a mutation atthe active site of UmuD that inactivates its ability to functionas an enzyme in the intermolecular cleavage reaction. It does,however, still posses a functional cleavage site so that it canserve as a substrate if an active UmuD (or UmuD') enzyme is providedin trans (McDonald et al. 1998a).

Ability of the UmuD mutants to promote damage-inducible mutagenesis

The ability of the various plasmid-encoded UmuD mutants to function in SOS mutagenesis was assayed in strain RW126/pRW274.This strain carries a chromosomal deletion of the entire umu operon,but cellular mutagenesis can be restored in trans by introducingcompatible plasmids expressing UmuC (pRW274) and UmuD (UmuD').Briefly, bacterial cultures were grown overnight in LB mediumcontaining the appropriate antibiotics. A 1.0-ml aliquot was centrifugedand resuspended in an equal volume of SM buffer (Sambrook et al.1989). The ability of particular plasmid bearing strains to promoteUmu-dependent SOS mutator activity was judged by plating a 100-µlaliquot on Davis and Mingioli minimal agar plates containing atrace amount of histidine (1 µg/ml) (Ho et al. 1993). A smallsterile disk was placed in the center of the plate, and 5 µl ofa 1:5 dilution of methylmethane sulfonate (MMS) (Sigma, St Louis,MO) in dimethylsulfoxide (Sigma, St Louis, MO) was added to thedisk. MMS-induced His⁺ mutants were scored after 4 days of incubation at 37°C. The resultsrepresent the average number of His⁺ colonies from at least three cultures from each strain, withsix plates perculture.

	Acknowledgments

M.G. dedicates this paper to the memory of Roy Scott. We thank Michael Maurizi for the generous gift of purified Lon proteinand helpful advice. We also thank the members of the laboratoryfor helpful comments and discussion throughout the course of thiswork and Agnès Tissier for designing Figure 7. This work wasperformed while the M.G. held an National Institutes of Health/NationalResearch Council Section on DNA Replication, Repair, and MutagenesisResearchAssociateship.

The publication costs of this article were defrayed in part by payment of page charges. This article must therefore be herebymarked `advertisement' in accordance with 18 USC section 1734solely to indicate thisfact.

	Footnotes

Received September 18, 1998; revised version accepted October 29, 1998.

¹ Correspondingauthor.

E-MAIL woodgate{at}helix.nih.gov; FAX (301) 594-1135.

References

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Abstract
Introduction
Results
Discussion
Materials and methods
References

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RESEARCH PAPER Lon-mediated proteolysis of the Escherichia coli UmuD mutagenesis protein: in vitro degradation and identification of residues required for proteolysis

RESEARCH PAPER
Lon-mediated proteolysis of the Escherichia coli UmuD mutagenesis protein: in vitro degradation and identification of residues required for proteolysis