The PDZ Domain of the SpoIVB Serine Peptidase Facilitates Multiple Functions

doi:10.1128/JB.183.14.4364-4373.2001

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Journal of Bacteriology, July 2001, p. 4364-4373, Vol. 183, No. 14
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.14.4364-4373.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

The PDZ Domain of the SpoIVB Serine Peptidase Facilitates Multiple Functions

Ngo T. Hoa,¹ James A. Brannigan,² and Simon M. Cutting¹^,^*

School of Biological Sciences, Royal Holloway University of London, Egham, Surrey TW20 0EX,¹ and Department of Chemistry, University of York, York Y010 5DD,² United Kingdom

Received 20 February 2001/Accepted 25 April 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

During spore formation in Bacillus subtilis, the SpoIVB protein is a critical component of the $sigma$ ^K regulatory checkpoint. SpoIVB has been shown to be a serine peptidasethat is synthesized in the spore chamber and which self-cleaves,releasing active forms. These forms can signal proteolytic processingof the transcription factor $sigma$ ^K in the outer mother cell chamber of the sporulating cell. Thisforms the basis of the $sigma$ ^K checkpoint and ensures accurate $sigma$ ^K-controlled gene expression. SpoIVB has also been shown to activatea second distinct process, termed the second function, which isessential for the formation of heat-resistant spores. In additionto the serine peptidase domain, SpoIVB contains a PDZ domain.We have altered a number of conserved residues in the PDZ domainby site-directed mutagenesis and assayed the sporulation phenotypeand signaling properties of mutant SpoIVB proteins. Our work hasrevealed that the SpoIVB PDZ domain could be used for up to fourdistinct processes, (i) targeting of itself for trans proteolysis,(ii) binding to the protease inhibitor BofC, (iii) signaling ofpro- $sigma$ ^K processing, and (iv) signaling of the second function ofSpoIVB.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

PDZ domains are relatively small ( $approx$ 100 amino acids) domains involved in protein-protein interactions (21, 23). Many ofthese interactions occur at the interface of the plasma membrane,enabling the recruitment and formation of larger complexes (24).PDZ domains have been shown to allow high selectivity in the targetingof proteins and can bind to short COOH-terminal peptide motifs.There are two main classes of binding site, h-X-V-COO (where h is a hydrophobic amino acid) and S/T-X-V-COO, based on the sequences of these motifs (1, 23, 24, 32,34, 35). In addition, PDZ domains have been shown to be ableto bind to internal motifs, as well as to other PDZ domains (14).Some PDZ proteins contain more than one domain; for example, theDrosophila InaD scaffolding protein carries five discrete PDZdomains (36). These multivalent PDZ domain proteins enable aseries of distinct protein-protein interactions which can be usedto build a protein complex in steps. PDZ domains can be carriedas discrete modules within a multidomain protein, and pertinentexamples of these modular PDZ proteins for this work are two familiesof bacterial serine peptidases, the Prc (also called Tsp) family(15) and the HtrA (also called DegP) family (22). In theseproteases, the PDZ domain enables substrate recognition, whichis thought to occur at the C terminus of the target. The crystalstructures of four PDZ domains, in complex with their cognatepeptide ligands, have provided invaluable insight into how thesedomains interact with their targets (7, 8, 14). The PDZdomains consist of a compact arrangement of six $beta$ strands andtwo $alpha$ helices (Fig. 1C). Peptides bind in a groove between $beta$ Band $alpha$ 2 in an antiparallel manner to $beta$ B that extends the $beta$ -sheetstructure. The peptide bound in this orientation places the carboxylgroup of the C-terminal residue in a position to interact witha loop between $beta$ A and $beta$ B. This loop has the consensus sequenceh-G-h (where h is a hydrophobic residue) and forms a "carboxylate-bindingpocket." Remarkably, recognition of such a short, degenerate motif,coupled with the presence of a free carboxyl group, is sufficientto confer high selectivity of binding, and artificial PDZ constructshave been demonstrated to bind new targets and efficiently transportthem to a defined subcellular location (32).

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FIG. 1. The SpoIVB PDZ domain. (A) Schematic diagram showing the position of the PDZ domain of SpoIVB (residues 102 to 187). The arrow indicates the site of the first self-cleavage reaction in the SpoIVB polypeptide. Also shown are the propeptide sequence, the region containing the serine peptidase domain, and a region thought to be involved in SpoIVB's putative second function (shaded box). (B) Structure-based sequence alignment of the putative PDZ domain in B. subtilis SpoIVB (accession no. P17896; residues 102 to 187; Sp4B, center) with four PDZ domains of known structure (above the Sp4B sequence) and four SpoIVB homologues (below the Sp4B sequence). Amino acid identity and similarity between the groups are indicated (h, hydrophobic; s, small; $-$ , negative charge; +, positive charge). A consensus secondary structure ( $alpha$ 1 and $alpha$ 2, $alpha$ helices; $beta$ A to -F, $beta$ strands) is given above the PDZ sequences. Note that all gaps and insertions required for maximal primary sequence alignment are placed outside of these structural elements. Residues known to contact ligands based on the structures of PDZ-peptide complexes are underlined. The positions of mutations in B. subtilis SpoIVB are indicated by arrows. These correspond to three positions that are conserved between the two groups (G114, D149, and N155) and three which are conserved within the SpoIVB group (G126, G144, and R185). Of the 286 PDZ domains identified by the Simple Modular Architecture Research Tool (33), Gly114 is conserved in 266 sequences, Gly126 is conserved in 114, Gly144 is conserved in 156, Asp149 is conserved in 269, Asn155 is conserved in 209, and Arg185 is conserved in 37. Preliminary sequence data were obtained from The Institute for Genomic Research (www.tigr.org), the B. stearothermophilus Genome Sequencing Project at the University of Oklahoma (www.genome.ou.edu), and Genome Therapeutics Corp. (www.cric.com). Pdz1, brain postsynaptic density protein 95 (residues 312 to 397); Pdz2, rabbit $alpha$ -syntrophin (residues 80 to 164); Pdz3, neuronal nitric oxide synthase (residues 15 to 101); Pdz4, hCASK (residues 482 to 574). Bant, B. anthracis; Bste, B. stearothermophilus; Bhal, B. halodurans (BAB06494); Cace, Clostridium acetobutylicum. (C) Stereoscopic representation of the SpoIVB PDZ domain structure. A homology model of the B. subtilis SpoIVB PDZ domain was constructed based on the crystal structures of PDZ 1 to 4 (Protein Data Bank codes 1be9, 1qav, 1qau, and 1kwa; [7, 8, 14]) by using the program Modeller (29). The peptide-binding groove is between $beta$ B and $alpha$ 2, and the carboxylate-binding loop is between $beta$ A and $beta$ B. The positions of glycine residues 114, 144, and 126 are shown as yellow balls. The side chains of residues Asp149, Asn155, and Arg185 are drawn as ball-and-stick images and colored with carbon atoms in grey, nitrogen atoms in blue, and oxygen atoms in red. The image was drawn with Molscript (16).

A PDZ domain has been identified in the Bacillus subtilis regulatory protein SpoIVB (Fig. 1) (21). SpoIVB is a multifunctionalprotein which plays a crucial role in the $sigma$ ^K checkpoint by providing the signal that activates proteolyticprocessing of pro- $sigma$ ^K (2, 3). SpoIVB has been shown to be a serine peptidasethat is synthesized in the forespore chamber and is secreted acrossthe inner forespore membrane (IFM), where it somehow activatesthe proteolysis of pro- $sigma$ ^K (37). Pro- $sigma$ ^K is an inactive transcription factor synthesized in the outermother cell chamber of the sporulating cell and is cleaved bya proposed complex of three proteins, SpoIVFA, SpoIVFB, and BofA,which are embedded in the outer forespore membrane (5, 26,27, 40). The SpoIVFB protein has been identified as the zincmetalloprotease which cleaves pro- $sigma$ ^K to its active form, $sigma$ ^K (17, 28). When activated by proteolytic cleavage, $sigma$ ^K directs the final program of gene expression in the mother cellchamber of the sporulating cell. The important feature of thisregulatory checkpoint is that $sigma$ ^K-directed gene expression must wait until the appropriate signalis received from the forespore. Accurate signaling is essentialto maintaining the fidelity of spore formation, since prematuresignaling leads to a marked decrease in spore-forming efficiency(3). How this is achieved is revealed by the extraordinarynumber of regulatory elements in the $sigma$ ^K checkpoint which inhibit premature signaling. Initially, $sigma$ ^F-directed transcription of the spoIVB gene is repressed at stageII (10, 12); it has been shown that should any inadvertentexpression occur then, the BofC protein would inhibit SpoIVB autoproteolysis,most probably by direct protein-protein interaction (11, 38).Premature signaling is also prevented by two inhibitors, SpoIVFAand BofA, which are thought to maintain the SpoIVFB protease inan inactive state (5, 25, 27). The C termini of both ofthese inhibitors protrude into the space between the IFM and outerforespore membrane and could interact with SpoIVB (13).

Potentially, the PDZ domain of SpoIVB could be used for protein-protein interactions to control these events, by activatingand targeting its peptidase function or providing surfaces todirect inhibition by binding to protein partners. In this work,we have used site-directed mutagenesis to analyze the functionof the SpoIVB PDZ domain. The results suggest that the PDZ domainis involved in multiple roles, including autoproteolysis, interactionwith BofC, and signaling of pro- $sigma$ ^Kprocessing.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains. The strains used in this work are listed in Table 1 and were all congenic with prototrophic spo⁺ strain PY79. To construct lysogens of SP $beta$ ::gerE-lacZ, a phagelysate was prepared from strain SC433 and used for transductionof the appropriate recipient strain. For integration of DNA atthe amyE locus, cells were transformed with linearized DNA. Strainconstructions using DNA-mediated transformation are outlined brieflyin Table 1. SC2373 was constructed by transformation of competentcells of SC2221 (spoIVB $Delta$ ::spc bofB8) with linearized pNH1134 (seepDG364-spoIVBDN149 below) plasmid DNA, followed by selection forchloramphenicol resistance (Cm^r; encoded by the pDG364 plasmid).

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TABLE 1. B. subtilis strains used in this study

General methods. The general Bacillus methods used (transduction, transformation, antibiotic selection, etc.) were those described by Cuttingand Vander-Horn (6). Sporulation was induced by the resuspensionmethod (19). Determination of heat and lysozyme resistance andmeasurements of gerE-directed $beta$ -galactosidase synthesis were doneas described previously (19).

Site-specific mutagenesis. Two oligonucleotide primers were used to amplify a 1,429-bp spoIVB product by PCR using chromosomal DNA from B. subtilis strainPY79 as a template. The primers used were P1 (5'-TTATGGATCCCGTGCACATCCATTCGTTC-3'),which annealed to nucleotides $-$ 146 to $-$ 127 from the spoIVB startcodon, and P2 (5'-AACAAGCTTAGTCAGCTTGCTTTTTCTTTTCC-3'),which annealed to the spoIVB stop codon (in bold) and a further18 bases upstream. The PCR product carried either a BamHI (P1)or a HindIII (P2) restriction site (underlined), enabling directcloning into pBluescript II KS(+). The resultant clone, pNH252,was sequenced completely to verify the presence of an unmodifiedspoIVB cistron. Next, mutations were created with mismatch oligonucleotidesby using the method of Kunkel as described by Sambrook et al.(30). In each pBluescript clone, the presence of a single aminoacid change was verified by DNA sequencing. Finally, the spoIVBgenes were subcloned as 1.4-kb HindIII-BamHI fragments into pDG364(6). pDG364 clones were pNH674 (spoIVBGA114), pNH973 (spoIVBGA126),pNH534 (spoIVBGA144), pNH1134 (spoIVBDN149), pNH487 (spoIVBND155),pNH676 (spoIVBGA144/ND155), NH970 (spoIVBRK185), NH977 (spoIVBGQ114),NH979 (spoIVBGQ126), NH981 (spoIVBA144), NH983 (spoIVBNY155),and pNH985 (spoIVBRH185).

pDG364 enables insertion of cloned DNA, in trans, at the amyE locus by double-crossover marker replacement. In each case,we linearized the pDG364 subclones by digestion with XhoI andintroduced them into SC1836 (spoIVB $Delta$ ::spc) cells by DNA-mediatedtransformation, followed by selection for Cm^r (encoded by pDG364). Insertion at the amyE locus was confirmedby testing for an Amy phenotype (failure to digest starch) as described elsewhere (6).Mutant strains had the genotype spoIVB $Delta$ ::spc amyE::spoIVB. Tomake the spoIVBGA144/ND155 double mutant, we first constructedthe spoIVBGA144 allele and then used the resultant mutant plasmidas a template to create a second spoIVBND155mutation.

We also constructed two isogenic control strains, NH578 (spoIVB $Delta$ ::spc amyE::spoIVB⁺) and NH577 (spoIVB $Delta$ ::spc amyE::pDG364). NH578 was created byintegrating a pDG364 subclone, pNH470, carrying the full-length,1,429-bp, wild-type spoIVB gene into the amyE locus, and NH577was created by integrating the unmodified pDG364 plasmid intothe chromosome by a double-crossover recombinational event atamyE.

Preparation of extracts for Western blotting. Samples (1 ml) were taken from sporulating cultures, and cells were harvested by centrifugation and frozen in liquid N₂. Tobreak the cells, pellets were suspended in 50 µl of TS buffer(25 mM Tris-HCl, pH 7.4; 0.1 M NaCl) containing lysozyme (0.2µg/ml) and incubated for 10 min on ice. A 50-µl volume of 2× sodiumdodecyl sulfate (SDS)-polyacrylamide gel electrophoresis (PAGE)loading dye was then added, and the samples were sonicated for10 s before gel loading (approximately 20 µl of sample perwell).

Western analysis. Immunoblotting of sporulating extracts with polyclonal antiserum to pro- $sigma$ ^K or SpoIVB was done as described previously (13, 37).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Site-specific mutagenesis of the PDZ domain. We used the alignment of bacterial PDZ domains, including SpoIVB, created by Pallen and Ponting (21) to identify key residueswithin the SpoIVB PDZ domain for site-directed mutagenesis (Fig.1B). These residues span the entire PDZ domain and represent three(Gly114, Asp149, and Asn155) which are conserved in almost allPDZ domains and Gly126, Gly144, and Arg185, which are conservedwithin SpoIVB homologues. Two types of amino acid alteration weremade as shown in Table 2, i.e., semiconservative (GA114, GA126,GA144, DN149, ND155, and RK185) and nonconservative (GQ114, GQ126,GQ144, NY155, and RH185) changes. In addition, we constructeda double mutant carrying two changes, GA144 and ND155, that werefer to here as spoIVBGA144/ND155.

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TABLE 2. Mutations in the SpoIVB PDZ domain

As described in Materials and Methods, the mutated spoIVB alleles were introduced at the amyE locus in cells carrying a spoIVB $Delta$ ::spcinsertion-and-deletion mutation. By using appropriate spoIVB andspoIVB⁺ congenic controls, we examined spore-forming efficiency duringsporulation (Table 2). Only one mutation, spoIVBDN149, substantiallyimpaired the formation of heat-resistant and lysozyme-resistantspores. For the other alleles, which had no effect on spore formation,we examined the capacity of spores to germinate correctly sinceimpaired activation of the $sigma$ ^K checkpoint has been shown, in some circumstances, to lead tothe production of germination-defective spores. We found that,in each case (with the exception of spoIVBDN149), spores germinatednormally.

Since the spoIVBDN149 allele caused a direct impairment of signaling, we determined whether it is dominant or recessive. Weintegrated the spoIVBDN149 gene at the amyE locus of spo⁺ (strain PY79) cells. In trans at the amyE locus, we found thatspoIVBDN149 is recessive, with the merodiploid producing essentially(99%) the same amount of heat-resistant spores (data not shown)as a control spo⁺ strain (NH578 spoIVB $Delta$ ::spc amyE::spoIVB⁺).

We also examined whether the spoIVBDN149 mutation is involved in both of SpoIVB's sporulation-specific functions, i.e., signalingin the $sigma$ ^K checkpoint and the development of heat resistance through a $sigma$ ^K-independent process (20). This can be established by engineeringspoIVBDN149 cells to express active $sigma$ ^K constitutively and determine whether heat-resistant spores develop.If so, then the spoIVBDN149 mutation only affects signaling ofpro- $sigma$ ^K processing. Accordingly, we constructed a strain (SC2373 amyE::spoIVBDN149spoIVB $Delta$ ::spc bofB8) carrying both the bofB8 and spoIVBDN149 alleles.In these cells, the bofB8 suppressor mutation renders the pro- $sigma$ ^K processing enzyme, SpoIVFB, constitutively active. We found thatin SC2373 cells, spore formation was blocked at stage IV-V withthe production of phase grey spores. Phenotypically, then, sporeformation had advanced, which is attributed to the premature synthesisand assembly of spore coat proteins onto the forespore, leadingto the production of phase grey spores and referred to as theBof phenotype, in contrast to a SpoIVB null phenotype, where stablephase grey spores are not produced (3). However, heat-resistant,phase bright spores were not formed at 37°C (Table 3). Failureto restore spore formation demonstrated that the spoIVBDN149 mutationdisrupts both functions. As described below, the DN149 alleleis temperature sensitive, so we also examined the phenotype ofSC2373 at 30°C (Table 3). We found that at this permissive temperature,signaling in the $sigma$ ^K checkpoint was restored in SC2373 cells, which was confirmedby the presence of phase grey stage IV-V spores and normal gerE-lacZexpression. However, 10 times fewer spores were produced thanin cells carrying only the spoIVBDN149 allele. This phenomenonhas been observed before and is due to premature signaling ofpro- $sigma$ ^K processing, which results in a 10-fold reduction in spore-formingefficiency (3).

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TABLE 3. Temperature sensitivity^a of the spoIVBDN149 allele

Effects of PDZ domain mutations on signaling of pro- $sigma$ ^K processing. To examine the effects of PDZ mutations on signaling in the $sigma$ ^K checkpoint, we used two methods: first, expression of a $sigma$ ^K-controlled gene, gerE, and second, proteolytic processing ofpro- $sigma$ ^K during spore formation. In the first approach, cells carryingthe spoIVB PDZ allele at the amyE locus were lysogenized withthe bacteriophage SP $beta$ ::gerE-lacZ. Cells carrying this reportergene were induced to sporulate by the resuspension method, andgerE-directed $beta$ -galactosidase synthesis was measured during sporeformation. Our results are summarized in Table 2, and representativeprofiles of gerE-lacZ expression are given in Fig. 2A to D. Wefound that four of the mutations in the PDZ domain, GA144 (Fig.2A), ND155 (Fig. 2B), RK185 (Fig. 2B), and GQ114 (Fig. 2C), aswell as the double mutation GA144/ND155 (Fig. 2B), produced amodest yet reproducible delay in gerE-lacZ expression. We haverepeated these experiments at least three times and found a delayof 20 to 30 min, together with a partial reduction in the levelof gerE expression. Finally, the spoIVBDN149 allele produced strongimpairment of gerE-lacZ expression (Fig. 2B), which was consistentwith the block in spore formation observed with this mutant. Carefulanalysis of the profile of gerE-lacZ expression suggested thatreduced levels (although higher than that of the spoIVB null mutant)were being produced but gerE-lacZ expression initiated 2 h laterthan in wild-type cells and peaked at 8 to 9 h instead of 6 to7 h (Fig. 2D). We also probed wild-type and mutant sporulatingcultures for active $sigma$ ^K and inactive $sigma$ ^K (pro- $sigma$ ^K) by using a polyclonal antiserum to pro- $sigma$ ^K (Fig. 3A and B). Two PDZ alleles produced a noticeable effecton $sigma$ ^K processing. spoIVBGQ114 produced a marked delay in pro- $sigma$ ^K processing of approximately 20 to 30 min (Fig. 3A), and in aspoIVBDN149 mutant, we could not detect any processing of pro- $sigma$ ^K even at the eighth hour of spore formation (Fig. 3B). Since wehave shown that gerE is expressed, albeit at a later time andat reduced levels, in the spoIVBDN149 mutant, we assume that extremelylow levels of $sigma$ ^K are being produced by proteolysis of pro- $sigma$ ^K but at levels undetectable by immunoblotting. That gerE couldbe transcribed by very low threshold levels of $sigma$ ^K-RNAP has been proposed before for $sigma$ ^K-controlled genes (18) and is consistent with the SpoIVBDN149phenotype.

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FIG. 2. $sigma$ ^K-directed gene expression in spoIVB PDZ mutants. $beta$ -Galactosidase synthesis was measured at the indicated times following the initiation of sporulation in cells carrying an SP $beta$ gerE::lacZ reporter. In each case, congenic strains were used and the relevant alleles (at the amyE locus) are given here (Table 1 contains the complete genotypes). (A) NH578, spoIVB⁺ (

); NH577, spoIVB $Delta$ ::spc ( $open circle$ ); NH685, spoIVBGA114 ( $triangle$ ); NH987, spoIVBGA126 ( $black-triangle$ ); NH587, spoIVBGA144 ( $black-diamond$ ). (B) NH578, spoIVB⁺ (

); NH577, spoIVB $Delta$ ::spc ( $open circle$ ); NH1135, spoIVBDN149 ( $triangle$ ); NH573, spoIVBND155 ( $black-triangle$ ); NH687, spoIVBGA144/ND155 ( $black-diamond$ ); NH990, spoIVBRK185 (

). (C) NH578, spoIVB⁺ (

); NH577, spoIVB $Delta$ ::spc ( $open circle$ ); NH1001, spoIVBGQ114 ( $triangle$ ); NH1003, spoIVBGQ126 ( $black-triangle$ ); NH1005, spoIVBGQ144 (

); NH1007, spoIVBNY155 ( $black-square$ ); NH991, spoIVBRH185 ( $black-diamond$ ). (D) NH578, spoIVB⁺ (

); NH577, spoIVB $Delta$ ::spc ( $open circle$ ); NH1135, spoIVBDN149 (

). Background levels of gerE-directed $beta$ -galactosidase synthesis present in cells containing no reporter have been subtracted.

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FIG. 3. Pro- $sigma$ ^K processing during spore formation. Sporulation was induced in wild-type and mutant cells, and at the indicated times, samples were removed, cell extracts were prepared, and proteins were size fractionated by SDS-12% PAGE and then probed with a polyclonal antiserum to pro- $sigma$ ^K. Panels A and B show 10-min time points taken between 3 h and 4 h 10 min for cells carrying semiconservative (A) or nonconservative (B) changes in the spoIVB PDZ domain. The strains used were NH578 (spoIVB⁺), NH577 (spoIVB $Delta$ ::spc), NH685 (spoIVBGA114), NH987 (spoIVBGA126), NH587 (spoIVBGA144), NH573 (spoIVBND155), NH990 (spoIVBRK185), NH687 (spoIVBGA144/ND155), NH1001 (spoIVBGQ114), NH1003 (spoIVBGQ126), NH1005 (spoIVBGQ144), NH1007 (spoIVBNY155), and NH991 (spoIVBRH185). Panel C shows a similar immunoblot but using 30- or 60-min sampling between 3 and 8.5 h for spoIVB, spoIVB $Delta$ ::spc, and spoIVBDN149 (NH1135) cells. In each panel, the onset of pro- $sigma$ ^K processing is indicated by an arrow.

We constructed additional strains in which the bofC $Delta$ ::neo mutation was introduced into spoIIIG $Delta$ 1 spoIVB $Delta$ ::spc amyE::spoIVBPDZcells. In these cells, low levels of SpoIVB would be synthesizeddue to $sigma$ ^F-controlled gene expression (12). Normally, wild-type SpoIVBcannot signal under these conditions due to the BofC inhibition.However, with BofC absent, we would expect delayed activationof pro- $sigma$ ^K processing and $sigma$ ^K-directed gene expression, as has been shown previously (11,38).

Strains were lysogenized with SP $beta$ ::gerE-lacZ, sporulation was induced, and gerE-directed $beta$ -galactosidase synthesis was determined(Fig. 4A to C). In cells carrying a wild-type spoIVB gene at theamyE locus (strain NH1140), gerE expression commenced at 6 h,reaching a maximum at 10 to 11 h, while in cells devoid of anintact spoIVB gene (strain NH1248), no gerE expression was detected.We found essentially no detectable gerE expression in cells carryingthe spoIVBDN149 (Fig. 4C) and spoIVBGQ114 (Fig. 4C) alleles. Instrains carrying the spoIVBGA144 (Fig. 4A), spoIVBRK185 (Fig.4B), spoIVBGQ126 (Fig. 4C), spoIVBNY155 (Fig. 4C), and spoIVBRH185(Fig. 4C) alleles, as well as the double mutation spoIVBGA144/ND155(Fig. 4B), gerE-lacZ expression was clearly delayed and reduced.Both of the experiments outlined above (Fig. 3 and 4) show thatthe PDZ mutations were interfering with signaling of pro- $sigma$ ^K processing.

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FIG. 4. Effects of PDZ mutations on $sigma$ ^K-directed gene expression when spoIVB is expressed prematurely. $beta$ -Galactosidase synthesis was measured at the indicated times following the initiation of sporulation in cells lysogenized with SP $beta$ ::gerE-lacZ. Cells carried both spoIIIG $Delta$ 1 and bofC $Delta$ ::neo, allowing signaling in the $sigma$ ^K checkpoint. In addition, cells carried the following spoIVB alleles at the amyE locus. (A) NH1140, spoIVB⁺ (

); NH1248, spoIVB ( $open circle$ ); NH1250, spoIVBGA114 ( $black-square$ ); NH1252, spoIVBGA126 (

); NH1254, spoIVBGA144 ( $triangle$ ). (B) NH1140, spoIVB⁺ (

); NH1248, spoIVB ( $open circle$ ); NH1256, spoIVBND155 ( $black-square$ ); NH1258, spoIVBGA144/ND155 (

); NH1260, spoIVBRK185 ( $black-triangle$ ); NH1268, spoIVBDN149 ( $triangle$ ). (C) NH1140, spoIVB⁺ (

); NH1248, spoIVB ( $open circle$ ); NH1262, spoIVBGQ114 ( $black-square$ ); NH1264, spoIVBGQ126 (

); NH1266, spoIVBGQ144 ( $triangle$ ); NH1270, spoIVBNY155 ( $black-triangle$ ); NH1272, spoIVBRH185 ( $diamond$ ). Background levels of gerE-directed $beta$ -galactosidase synthesis present in cells containing no reporter have been subtracted.

Temperature-sensitive nature of the spoIVBDN149 allele. When grown on sporulation agar plates at 37°C, spoIVBDN149 mutant cells (NH1135) were Spo and indistinguishable from spoIVB $Delta$ ::spc cells (NH577), producinglow levels of phase grey spores which were not released from themother cell. However, prolonged incubation of these plates atroom temperature revealed a low number of phase bright spores(Spo⁺) which were released from the sporangial cell. This suggestedthat the spoIVBDN149 mutation could be temperature sensitive.To test this, we induced sporulation in spo⁺, spoIVB $Delta$ ::spc, and spoIVBDN149 cells at 30 and 37°C by the resuspensionmethod. Samples were removed at 34 and 24 h from the 30 and 37°Ccultures, respectively, and the numbers of heat-resistant spores(65°C, 45 min) were determined. The different assay times werechosen because spore formation at 30°C is slower at the lowertemperature. As shown in Table 3, we found that at 30°C, approximately3.5% of the culture consisted of heat-resistant spores. Moreover,this was almost 4,000-fold more than were present when sporulationwas induced at 37°C. Since the number of spores was unaffectedin the spoIVB $Delta$ ::spc mutant, these results show that the spoIVBDN149allele is temperaturesensitive.

Genetic evidence that the PDZ domain can interact with BofC. If the PDZ domain is involved in interaction with the BofC inhibitor, then mutations in the PDZ domain may release SpoIVBfrom BofC's inhibitory action. To address this possibility, weconstructed strains carrying the spoIIIG $Delta$ 1 mutation, the wild-typeor mutant spoIVB gene at the amyE locus, and (to monitor $sigma$ ^K activity) the reporter phage SP $beta$ ::gerE-lacZ. These cells wereinduced to sporulate, and gerE-directed $beta$ -galactosidase synthesiswas measured. We found that cells carrying the spoIVBGQ144 alleleat the amyE locus allowed measurable levels of gerE-directed $beta$ -galactosidasesynthesis with expression beginning at 6 h (Fig. 5). With allother mutants, we observed no effect on gerE-lacZ expression (notshown), although, as an example, expression in cells carryingspoIVBGA114 is shown in Fig. 5. As an internal control, we alsomeasured gerE expression in spoIIIG $Delta$ 1 cells carrying the bofCdeletion-and-insertion mutation bofC $Delta$ ::neo. In spoIIIG $Delta$ 1 bofC $Delta$ ::neocells, expression of gerE commenced at 6 h, reaching maximum levelsat 11 h, which was similar to the result obtained with spoIIIG $Delta$ 1amyE::spoIVBGQ144 cells, although the maximum levels of gerE expressionwere higher. Delayed expression of gerE-lacZ in a bofC mutantis thought to occur because of the low levels of SpoIVB producedin this mutant, where spoIVB is transcribed under $sigma$ ^F control and must therefore accumulate to sufficient levels inorder to signal (38). The simplest explanation for these resultsis that the GQ144 allele affects the interaction of SpoIVB withBofC.

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FIG. 5. Effects of PDZ mutations on $sigma$ ^K-directed gene expression in the absence of $sigma$ ^G. $beta$ -Galactosidase synthesis was measured at the indicated times following the initiation of sporulation in cells lysogenized with SP $beta$ ::gerE-lacZ. Cells carried a spoIIIG $Delta$ 1 mutation, as well as (i) a wild-type or modified spoIVB gene carried at the amyE locus or (ii) a bofC $Delta$ ::neo insertional mutation, as indicated (Table 1 contains the complete genotypes). PW71, spoIIIG $Delta$ 1 bofC $Delta$ ::neo (

); NH1097, spoIIIG $Delta$ 1 spoIVB⁺ ( $open circle$ ); NH214, spoIIIG $Delta$ 1 spoIVBGQ144 ( $black-triangle$ ); NH1278, spoIIIG $Delta$ 1 spoIVBGA114 ( $triangle$ ). Background levels of gerE-directed $beta$ -galactosidase synthesis present in cells containing no reporter have been subtracted.

Autoproteolysis of SpoIVB in PDZ mutants. The spoIVBDN149 and spoIVBGQ114 mutations produced substantial effects on signaling of pro- $sigma$ ^K processing. One possible explanation for their phenotype is thatin these PDZ mutants, processing of SpoIVB was perturbed, leadingto a consequential effect on signaling. Such an explanation impliesthat the PDZ domain is important for autoproteolysis of SpoIVBinstead of, or in addition to, having a direct role in signalingby protein-protein interaction. To address this possibility, weexamined the proteolysis of SpoIVB in sporulating cells. Figure6 shows Western blots of sporulating cell samples taken from spo⁺ cells (NH578) and cells carrying the spoIVBGQ114 (NH1001) andspoIVBDN149 (NH1135) mutations. In spo⁺ cells, SpoIVB is synthesized as a 50-kDa protein which is subjectto rapid autoproteolysis beginning at about 3 h. Self-cleavageyields intermediate-size products of 46, 45, and 44 kDa, but theseforms are rapidly inactivated by secondary cleavage to yield 42-and 40-kDa products. The 46-, 45-, and 44-kDa species are thoughtto be the active forms of SpoIVB, and these are seen only intermittentlyduring spore formation while the 42- and 40-kDa forms accumulate.Our blots showed that in spoIVBGQ114 cells there appeared lessof the intermediate and presumably active forms of SpoIVB (the46-, 45-, and 44-kDa forms). In addition, the 50-kDa, full-lengthform of SpoIVB appeared to be more stable, unlike in wild-typecells, where the 50-kDa form was gradually processed. While thisis a small difference, it was reproducible and suggests that processingof SpoIVB was impaired or reduced compared with that in wild-typecells. In spoIVBDN149 cells, the 50-kDa form of SpoIVB persistedlonger during the time course we examined, suggesting that SpoIVBwas being processed less efficiently.

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FIG. 6. Autoproteolysis of SpoIVB in PDZ domain mutants. Sporulation was induced in NH578 (wild type [WT]; spo⁺), NH1001 (GQ114; spoIVBGQ114), NH1005 (GQ144; spoIVBGQ144), and NH1135 (DN149; spoIVBDN149) cells, and samples were taken every 10 min. Samples were fractionated by SDS-12% PAGE and examined with a polyclonal antiserum to SpoIVB (2-min enhanced-chemiluminescence exposure time). The full-length, 50-kDa, unprocessed form of SpoIVB is marked, as are 46-, 45-, and 44-kDa intermediate SpoIVB cleavage products and the 42- and 40-kDa cleavage products produced by secondary cleavage.

We have shown GQ144 to be important for PDZ interaction with BofC, so we also examined SpoIVB autoproteolysis in this mutantand found little, if any, effect on SpoIVB cleavage, althoughsome retardation of the cleavage of the intermediate forms ofSpoIVB was apparent. We have also examined all of the other PDZalleles (data not shown) and detected no significant effect onautoproteolysis or on the levels of intermediateforms.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

SpoIVB has been extensively studied primarily because it is the signal which activates pro- $sigma$ ^K processing at the $sigma$ ^K checkpoint (2, 10, 12, 20, 37). This protein has recentlybeen shown to be a serine peptidase (37) and so resembles thePrc and HtrA serine peptidases, which carry both a PDZ and a serinepeptidase domain (15, 22). In work to be published elsewhere(N. T. Hoa, J. A. Brannigan, and S. M. Cutting, unpublished data),we have shown that the catalytic triad for the SpoIVB serine peptidaseis confined to the C terminus and is downstream of the PDZ domain(Fig. 1A).

SpoIVB is synthesized in the forespore and is secreted across the IFM. Since this protein lacks a normal signal sequence,it is probably not released by signal peptide cleavage from themembrane and, instead, releases itself by self-cleavage, whichcan occur in trans. At the time when SpoIVB is synthesized, theBofC protein is made in the forespore and is secreted across theIFM. Unlike SpoIVB, BofC carries a typical secretory signal sequencethat is cleavable by a signal peptidase. BofC has been shown toinhibit autoproteolysis of SpoIVB by stabilizing SpoIVB in aninactive form (38). BofC is only important at stage II of developmentand provides a mechanism by which to ensure that any inadvertenttranscription of the spoIVB gene does not lead to premature signaling.Most probably, BofC would inhibit self-cleavage of SpoIVB by directinteraction and it appears to act stoichiometrically, suggestingthat once the level of SpoIVB molecules exceeds that of BofC,self-cleavage of SpoIVB would commence, leading to signaling (38).When proteolytically active, SpoIVB signals two distinct events.The first is processing of pro- $sigma$ ^K, and the second is an unidentified process, termed the secondfunction, which leads to the formation of heat-resistant spores(20). The second function was illuminated in genetic experimentsin which bypassing of the requirement of SpoIVB for processingof pro- $sigma$ ^K did not restore heat resistance, implying that SpoIVB must, therefore,have two distinct roles. We can assign four processes to SpoIVB,each of which could involve protein-protein interaction: (i) autoproteolysis,(ii) interaction with the BofC protein, (iii) signaling of pro- $sigma$ ^K processing, and (iv) signaling of the second function. Our workhas shown that the PDZ domain could be used in all four of theseputativeinteractions.

Our results have shown that most changes in the PDZ domain produced only slight phenotype changes. In part, this was expecteddue to the size of the PDZ domain. However, we have revealed theimportance of the Asp149 and Gly114 residues in the PDZ domain.These residues correspond to the most highly conserved positionswithin PDZ sequences. Gly114 in the motif h-G-h is important formaintaining the conformation of the carboxylate-binding loop.Interactions with a substrate carboxylate are mediated by backboneamides from the loop, and so the amino acid residue side chainscan vary significantly. Substitutions for glycine in such a structuralrole are acceptable; however, there are energetic penalties, asthe introduced amino acid must take up unfavorable conformationsto preserve the architecture. In the case of the SpoIVB PDZ, weassume that the smaller Ala side chain is more easily accommodatedthan a glutamine. The most drastic effects are produced by mutationof Asp149. It is likely that alterations at this position leadto significant changes in the PDZ structure, and the pleiotropicnature of DN149 mutants suggests that the PDZ domain of SpoIVBis important to all of the functions tested. In some crystal structuresof PDZ domains, Asp149 forms a salt bridge between $beta$ strands Aand D (8). The temperature-sensitive phenotype of a spoIVBDN149mutant (see below) indicates that there may be a similar structuralrole for Asp149 inSpoIVB.

Interestingly, the spoIVBDN149 allele has been isolated previously, in a classical genetic screen for new spoIVB alleles (20).Characterization of this allele, known as spoIVB57, differed somewhatfrom our results described here. Specifically, the spoIVB57 strainwas found to allow very low levels of $sigma$ ^K-directed gene expression and higher levels of heat-resistantphase bright spores (1.2%) at 37°C. In contrast, our work shownhere demonstrated a much lower level of spore formation (<0.0001%)and moderate-to-low levels of gerE-lacZ expression. We have noimmediate explanation for these results, although the spoIVB57mutant was analyzed by inducing spore formation by the exhaustionmethod (using DS medium [19]), whereas here we used the resuspensionmethod. Although it is an unsatisfactory explanation, we now knowthat the spoIVBDN149 allele is temperature sensitive and we cannotbe sure that these two studies were performed under identicalconditions.

Possibly, the most important discovery in this work is that proteolysis of SpoIVB was defective in the spoIVBDN149 and spoIVBGQ114mutants. Self-cleavage of SpoIVB still occurred in these mutantsbut at a reduced rate. This provides strong support for the hypothesisthat the PDZ domain is used for self-cleavage. That there areother families of prokaryotic serine peptidases (e.g., the Prcand HtrA serine peptidases) with PDZ domains makes it likely thatthe PDZ domain has been exploited by bacterial proteases for substraterecognition. We cannot predict how SpoIVB would recognize itselfat this stage, although head-to-tail oligomerization has beenproposed for some PDZ-PDZ interactions (14). Another importantfinding is that the spoIVBDN149 allele is temperature sensitive,which suggests a weaker interaction more easily disrupted at thehigher temperature. Moreover, even at the restrictive temperature,signaling of pro- $sigma$ ^K processing occurred, although this was at levels undetectableby immunoblotting. We can conclude that since, after a pronounceddelay, gerE-lacZ expression reached 50% of the wild-type level,then expression of gerE must be susceptible to a very low thresholdlevel of active $sigma$ ^K, an observation which has been made before, i.e., that some $sigma$ ^K-controlled genes require different levels of $sigma$ ^K for expression (18). This is supported by the GQ114 allele,where the defect in SpoIVB autoproteolysis was less severe thanin the DN149 mutant, producing a delay in pro- $sigma$ ^K processing of 30 min. An important question is whether the defectivesignaling is due to impaired PDZ-mediated interaction of SpoIVBwith one or more components of the pro- $sigma$ ^K processing complex (SpoIVFA, BofA, or SpoIVFB) or whether a simplereduction in active SpoIVB cleavage products is required for signaling.In the first model, the PDZ domain is required specifically fortargeting of SpoIVB to the pro- $sigma$ ^K processing complex in the outer forespore membrane, while inthe second model, the PDZ domain would be required only to enableSpoIVB self-cleavage and the generation of cleavage products whichsignal by a different mechanism. Our work does not provide directevidence that SpoIVB uses its PDZ domain for signaling in the $sigma$ ^K checkpoint or signaling of the second function, although it isattractive to propose this. The simplest way in which a PDZ domainwould achieve this is to interact specifically with C-terminalmotifs. However, we are unable to identify any known PDZ-bindingsequences at the C termini of SpoIVFA, BofA, SpoIVFB, or, indeed,SpoIVB.

A further reason for speculating that the PDZ domain is involved in other interactions (other than self-cleavage) is our geneticevidence that the PDZ domain interacts with BofC. This was revealedby the GQ144 allele, which permitted substantial levels of gerE-lacZexpression under conditions in which the BofC protein inhibitsSpoIVB-mediated signaling. This confirms our previous report,in which we suggested that SpoIVB and BofC interact (38). Again,we have failed to identify any potential PDZ recognition motifwithin BofC, which suggests that the SpoIVB recognition sequencerepresents a new class of motif. Since our work shows interactionof the SpoIVB PDZ domain with BofC, as well as with itself, itseems reasonable to predict that this domain is involved in otherSpoIVB-mediated interactions, such as signaling of pro- $sigma$ ^K processing and the secondfunction.

Our work has revealed that the SpoIVB PDZ domain is involved in at least two, if not more, distinct partner interactions.Unlike other multivalent PDZ-domain proteins, though, SpoIVB appearsto use a single motif to interact with a number of target proteins.Some single PDZ domains mediate a number of interactions, whichsupports the multiple roles proposed for SpoIVB's PDZ domain.For instance, PDZ2 of the 95-kDa postsynaptic density proteincan heterodimerize with neuronal nitric oxide synthase or $alpha$ -syntrophinand interact with the C terminus of the Shaker-type potassiumion channel Kv1.4. Single mutations in PDZ2 can alter the specificityand affinity of one interaction without affecting the other (9).One plausible model is that the level of SpoIVB would dictatewith which protein SpoIVB could interact, and indeed, we haveproposed previously that the level of SpoIVB is important forescaping inhibition by the BofC protein (38).

	ACKNOWLEDGMENTS

We thank Tony Wilkinson and Phil Wakeley for help andadvice.

This work was supported by a grant from the Biotechnology and Biological Sciences Research Council (BBSRC) to S.M.C. J.A.B.is supported by the BBSRC-funded Structural Biology Centre atYork.

	FOOTNOTES

^* Corresponding author. Mailing address: School of Biological Sciences, Royal Holloway University of London, Egham, Surrey TW200EX, United Kingdom. Phone: 01784-443760. Fax: 01784-434326. E-mail:s.cutting{at}rhul.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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7. Daniels, D. L., A. R. Cohen, J. M. Anderson, and A. T. Brunger. 1998. Crystal structure of the hCASK PDZ domain reveals the structural basis of class II PDZ domain target recognition. Nat. Struct. Biol. 5:317-325[CrossRef][Medline].

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9. Gee, S. H., S. Quenneville, C. R. Lombardo, and J. Chabot. 2000. Single-amino acid substitutions alter the specificity and affinity of PDZ domains for their ligands. Biochemistry 39:14638-14646[CrossRef][Medline].

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1.	Beebe, K. D., J. Shin, J. Peng, C. Chaudhury, J. Khera, and D. Pei. 2000. Substrate recognition through a PDZ domain in tail-specific protease. Biochemistry 39:3149-3155[CrossRef][Medline].
2.	Cutting, S., A. Driks, R. Schmidt, B. Kunkel, and R. Losick. 1991. Forespore-specific transcription of a gene in the signal transduction pathway that governs pro- $sigma$ ^K processing in Bacillus subtilis. Genes Dev. 5:456-466[Abstract/Free Full Text].
3.	Cutting, S., V. Oke, A. Driks, R. Losick, S. Lu, and L. Kroos. 1990. A forespore checkpoint for mother cell gene expression during development in B. subtilis. Cell 62:239-250[CrossRef][Medline].
4.	Cutting, S., S. Panzer, and R. Losick. 1989. Regulatory studies on the promoter for a gene governing synthesis and assembly of the spore coat in Bacillus subtilis. J. Mol. Biol. 207:393-404[CrossRef][Medline].
5.	Cutting, S., S. Roels, and R. Losick. 1991. Sporulation operon spoIVF and the characterization of mutations that uncouple mother-cell from forespore gene expression in Bacillus subtilis. J. Mol. Biol. 221:1237-1256[Medline].
6.	Cutting, S. M., and P. B. Vander-Horn. 1990. Genetic analysis, p. 27-74. In C. R. Harwood, and S. M. Cutting (ed.), Molecular biological methods for Bacillus. John Wiley & Sons, Ltd., Chichester, England.
7.	Daniels, D. L., A. R. Cohen, J. M. Anderson, and A. T. Brunger. 1998. Crystal structure of the hCASK PDZ domain reveals the structural basis of class II PDZ domain target recognition. Nat. Struct. Biol. 5:317-325[CrossRef][Medline].
8.	Doyle, D. A., A. Lee, J. Lewis, E. Kim, M. Sheng, and R. MacKinnon. 1996. Crystal structures of a complexed and peptide-free membrane protein-binding domain: molecular basis of peptide recognition by PDZ. Cell 85:1067-1076[CrossRef][Medline].
9.	Gee, S. H., S. Quenneville, C. R. Lombardo, and J. Chabot. 2000. Single-amino acid substitutions alter the specificity and affinity of PDZ domains for their ligands. Biochemistry 39:14638-14646[CrossRef][Medline].
10.	Gomez, M., S. Cutting, and P. Stragier. 1995. Transcription of spoIVB is the only role of $sigma$ ^G that is essential for pro- $sigma$ ^K processing during spore formation in Bacillus subtilis. J. Bacteriol. 177:4825-4827[Abstract/Free Full Text].
11.	Gomez, M., and S. M. Cutting. 1997. bofC encodes a putative forespore regulator of the Bacillus subtilis $sigma$ ^K checkpoint. Microbiology 143:157-170[Abstract/Free Full Text].
12.	Gomez, M., and S. M. Cutting. 1996. Expression of the Bacillus subtilis spoIVB gene is under dual $sigma$ ^F/ $sigma$ ^G control. Microbiology 142:3453-3457[Abstract/Free Full Text].
13.	Green, D. H., and S. M. Cutting. 2000. Membrane topology of the Bacillus subtilis pro- $sigma$ ^K processing complex. J. Bacteriol. 182:278-285[Abstract/Free Full Text].
14.	Hillier, B. J., K. S. Christopherson, K. E. Prehoda, D. S. Bredt, and W. A. Lim. 1999. Unexpected modes of PDZ domain scaffolding revealed by structure of nNOS-syntrophin complex. Science 284:812-815[Abstract/Free Full Text].
15.	Keiler, K. C., P. R. Waller, and R. T. Sauer. 1996. Role of a peptide tagging system in degradation of proteins synthesised from damaged messenger RNA. Science 271:990-993[Abstract].
16.	Kraulis, P. J. 1991. Molscript: a program to produce both detailed and schematic plots of protein structure. J. Appl. Crystallogr. 24:946-950[CrossRef].
17.	Lewis, A. P., and P. J. Thomas. 1999. A novel clan of zinc-metalloproteases with possible intramembrane cleavage properties. Protein Sci. 8:439-442[Medline].
18.	Lu, S., and L. Kroos. 1994. Overproducing the Bacillus subtilis mother cell sigma factor precursor, pro- $sigma$ ^K, uncouples $sigma$ ^K-dependent gene expression from dependence on intercompartmental communication. J. Bacteriol. 176:3936-3943[Abstract/Free Full Text].
19.	Nicholson, W. L., and P. Setlow. 1990. Sporulation, germination and outgrowth, p. 391-450. In C. R. Harwood, and S. M. Cutting (ed.), Molecular biological methods for Bacillus. John Wiley & Sons, Ltd., Chichester, United Kingdom.
20.	Oke, V., M. Shchepetov, and S. Cutting. 1997. SpoIVB has two distinct functions during spore formation in Bacillus subtilis. Mol. Microbiol. 23:223-230[CrossRef][Medline].
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