Evidence that the Extracytoplasmic Function Sigma Factor sigma E Is Required for Normal Cell Wall Structure in Streptomyces coelicolor A3(2)

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Journal of Bacteriology, January 1999, p. 204-211, Vol. 181, No. 1
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Evidence that the Extracytoplasmic Function Sigma Factor $sigma$ ^E Is Required for Normal Cell Wall Structure in Streptomyces coelicolor A3(2)

Mark S. B. Paget,¹^,²^,^* Leony Chamberlin,¹ Abdelmadjid Atrih,³ Simon J. Foster,³ and Mark J. Buttner¹^,²

John Innes Centre, Colney, Norwich NR4 7UH,¹ School of Biological Sciences, University of East Anglia, Norwich NR4 7TJ,² and Department of Molecular Biology and Biotechnology, University of Sheffield, Sheffield S10 2TN,³ United Kingdom

Received 28 August 1998/Accepted 20 October 1998

	ABSTRACT

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The sigE gene of Streptomyces coelicolor A3(2) encodes an RNA polymerase sigma factor belonging to the extracytoplasmic function(ECF) subfamily. Constructed sigE deletion and disruption mutantswere more sensitive than the parent to muramidases such as henegg white lysozyme and to the CwlA amidase from Bacillus subtilis.This correlated with an altered muropeptide profile, as determinedby reverse-phase high-performance liquid chromatography analysisof lytic digests of purified peptidoglycan. The sigE mutants requiredhigh levels of magnesium for normal growth and sporulation, overproducingthe antibiotic actinorhodin and forming crenellated colonies inits absence. Together, these data suggest that sigE is requiredfor normal cell wall structure. The role of $sigma$ ^E was further investigated by analyzing the expression of hrdD,which is partially sigE dependent. The hrdD gene, which encodesthe $sigma$ ^HrdD subunit of RNA polymerase, is transcribed from two promoters,hrdDp₁ and hrdDp₂, both similar to promoters recognized by otherECF sigma factors. The activities of hrdDp₁ and hrdDp₂ were reduced20- and 3-fold, respectively, in sigE mutants, although only hrdDp₁was recognized by E $sigma$ ^E in vitro. Growth on media deficient in magnesium caused the inductionof both hrdD promoters in a sigE-dependentmanner.

	INTRODUCTION

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The $sigma$ ^E subunit of Streptomyces coelicolor RNA polymerase was originally identified by its ability to direct transcription invitro from dagAp₂, one of four promoters of the dagA gene, whichencodes an extracellular agarase (8, 9). Cloning of the $sigma$ ^E gene (sigE) led to the discovery of a distinct subfamily of sigmafactors, named the extracytoplasmic function (ECF) subfamily,which are structurally distinct from other members of the $sigma$ ⁷⁰ family (39). ECF sigma factors have now been described in awide range of gram-positive and gram-negative bacteria and, wherestudied, have been shown to be involved in regulating a varietyof functions, typically concerned with the extracytoplasmic environment(44). Well-studied examples include $sigma$ ^E of Escherichia coli, required for transcription of genes involvedin the turnover and correct folding of periplasmic proteins (13,54, 56); $sigma$ ^FecI, which responds to extracellular iron(III) dicitrate and directsthe transcription of genes required for its uptake in E. coli(2); $sigma$ ^CarQ, required for carotenoid biosynthesis in Myxococcus xanthus (22);and $sigma$ ^AlgU, which regulates the production of extracellular alginate inPseudomonas aeruginosa (16, 24).

Members of the ECF subfamily have a number of common features which distinguish them from other members of the $sigma$ ⁷⁰ family. First, of the four conserved regions in $sigma$ ⁷⁰-related sigma factors (38, 39), region 3 and much of region1 are usually absent, resulting in the typically small size ofECF sigma factors (usually 20 to 30 kDa). Second, promoters regulatedby ECF sigma factors are strikingly similar, especially in the $-$ 35 region, where a GAAC motif is conserved (39, 44). Third,their activity is often regulated by specific anti-sigma factorsencoded by downstream genes. Examples are RseA in the case ofE. coli $sigma$ ^E (14, 45) and CarR in the case of $sigma$ ^CarQ (22).

One of the most striking aspects of ECF sigma factors is that relatively few have been identified by traditional genetic means,although very large numbers of ECF sigma factor genes are nowbeing uncovered in a variety of bacteria through genome sequencing.For example, in Bacillus subtilis there are seven ECF sigma factorgenes (37), none of which was discovered genetically. This seemsto imply either that they are functionally redundant or that theycontrol the expression of genes not relevant to normal laboratoryculture conditions. Recently, it was shown that there is indeedsome redundancy among the ECF sigma factors of B. subtilis. AsigX mutant of B. subtilis has slightly increased sensitivityto heat and oxidative stress but has no other obvious phenotype(30). $sigma$ ^X contributes to the transcription from at least seven promoters,four of which are also recognized by one or more different ECFsigma factors in vivo (29). The other three promoters are completelydependent on $sigma$ ^X in vivo, but a second, $sigma$ ^X-independent promoter also contributes to the expression of therespective genes. Therefore, each of the seven known members ofthe $sigma$ ^X regulon is transcribed by more than one RNA polymerase holoenzyme,meaning that disruption of sigX will not abolish the expressionof any of these genes. This may explain, at least in part, thesubtlety of the sigX mutant phenotype (29).

To date, the biological role of $sigma$ ^E in Streptomyces has been investigated only in the actinomycin producer S. antibioticus.An S. antibioticus sigE null mutant was deficient in actinomycinproduction, although direct targets for $sigma$ ^E have not been identified (34). Here we investigate the biologicalrole of $sigma$ ^E in S. coelicolor. We show that constructed sigE null mutantshave an altered cell wall structure, increased sensitivity tocell wall-lytic enzymes, and a distinct peptidoglycan muropeptideprofile. We also show that sigE mutants require high levels ofmagnesium for normal growth and sporulation, and we identify a $sigma$ ^E-dependent promoter that is induced when cultures are grown underconditions of magnesiumdeficiency.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, and growth conditions. S. coelicolor A3(2) M600 (11) and its derivatives were cultivated on MM, R2, R2YE (28), MS agar (mannitol plus soy flour)(27), SMMS agar (19), and NMMP liquid media (28), essentiallyas described previously (28). Unmethylated DNA for introductioninto S. coelicolor was isolated from E. coli ET12567 (dam dcmhsdS) (40). Plasmids are described in Table 1.

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TABLE 1. Plasmids used in this study

Overproduction of $sigma$ ^E. A 2.05-kb PvuII fragment carrying sigE was cloned into SmaI-cut pIJ2925 (33) such that, in the resulting plasmid, pIJ5950,the HindIII site in the polylinker was upstream of sigE. The 870bp of DNA between the HindIII site and a unique XhoI site 10 bpdownstream of the sigE ATG start codon was replaced with two complementaryoligonucleotides (5'-AGCTTCCATATGGGTGAAGTTC-3' and 5'-TCGAGAACTTCACCCATATGGA-3')that introduced an NdeI site overlapping the ATG start codon andalso replaced the second, third, and fourth codons with synonymouscodons commonly associated with genes expressed at high levelsin E. coli. The cassette replacement was verified by sequencingthe resulting plasmid (pIJ2076), and sigE was excised as a 1.2-kbNdeI-BglII fragment and cloned into the expression vector pET11c(Novagen), which had been cut with NdeI and BamHI, to generatepIJ2078.

pIJ2078 was introduced into E. coli BL21 $lambda$ DE3(pLysS) (59), and sigE expression was induced in exponentially growing cells(optical density at 600 nm, 0.5) by the addition of 1 mM isopropyl- $beta$ -D-thiogalactopyranoside(IPTG). $sigma$ ^E was recovered from inclusion bodies essentially as describedpreviously (48). Inclusion bodies were solubilized with 0.25(wt/vol) Sarkosyl (N-lauroylsarcosine), followed by extensivedialysis to remove Sarkosyl and to allow $sigma$ ^E to refold. $sigma$ ^E was further purified by Mono-Q anion-exchange columnchromatography.

Approximately 10 µg of purified $sigma$ ^E was subjected to sequential Edman degradation in order to determine the sequence of the1st 10 N-terminal residues. The result $---$ GEVLEFEEYV $---$ showed completeagreement with that predicted from the DNA sequence of sigE (39)and showed that the N-terminal N-formylmethionine had been removed,as it is in S. coelicolor (39).

In vitro transcription. Runoff transcription assays were performed with [ $alpha$ -³²P]CTP (600 Ci mmol¹; Dupont-NEN) as described by Buttner et al. (8). Typical reactionmixtures contained 1.25 pmol of E. coli core RNA polymerase (EpicentreTechnologies, Madison, Wis.) and 12.5 pmol of $sigma$ ^E. Transcription from the hrdD promoter region was assayed by usingtwo fragments isolated from pIJ2036: a 490-bp HindIII-NarI fragmentand a 630-bp HindIII-SstI fragment. Transcripts were analyzedon 6% polyacrylamide-7 M urea gels with heat-denatured ³²P-labelled HpaII digests of pBR322 as size standards. S. coelicolorRNA polymerase holoenzyme, purified from YEME-grown cultures,was a gift from T. Fujii and E.Takano.

Construction of sigE mutants of S. coelicolor A3(2). A PCR-based approach was used to generate an internal in-frame deletion in sigE. By using pIJ5950 as a template, DNA downstreamfrom sigE was amplified with a primer complementary to the C-terminalregion of sigE which incorporated an XhoI site at the 5' end (MP1;5'-CGCTCGAGCGTGAGGAGCGG-3') and a primer complementary to a sequencejust downstream from the Asp718 site (KB5; 5'-GCCGGTACCCCCGGTCC-3')(see Fig. 1). The resulting 150-bp product was digested with XhoIand Asp718, then inserted into XhoI-Asp718-digested pMT3000 (50)and checked by DNA sequencing. The XhoI-Asp718 fragment was reisolatedfrom pMT3000 and inserted into pIJ5950, replacing the sigE-containingXhoI-Asp718 fragment. The resulting plasmid, pIJ5951, contains $Delta$ sigE flanked by 0.85 kb of DNA upstream and 0.7 kb downstream. $Delta$ sigE was isolated as a BamHI-BglII fragment and inserted intoBamHI-digested pDH5 to give pIJ5952. pIJ5952 was passaged throughthe nonmethylating E. coli strain ET12567, then used to transformS. coelicolor M600, with selection for thiostrepton resistance(Thio^r). A representative transformant was subcultured on nonselectivemedia for one round of sporulation, and the resulting spores wereplated out to allow identification of Thio^s colonies. Thio^s colonies were screened for the presence or absence of the sigEgene by Southern hybridization of digested chromosomal DNA. Arepresentative Thio^s isolate in which sigE had been deleted was designatedJ2130.

A disruption mutation was made in sigE by inserting a hygromycin resistance cassette (hyg) into the internal NcoI site. The1.7-kb hyg cassette (63) was blunt ended and cloned into pIJ5950which had been digested with NcoI and filled in, to give pIJ5954.The sigE::hyg mutant allele was isolated as a BglII fragment andcloned into pSET151. The resulting plasmid, pIJ5955, was usedto transform S. coelicolor M600, with selection for hygromycinresistance (Hyg^r). All transformants were also Thio^r, indicating a single crossover event. sigE::hyg mutants wereidentified by screening for Hyg^r Thio^s colonies after a round of nonselective growth, and their structureswere confirmed by Southern hybridization. A representative sigE::hygmutant of M600 was designatedJ2141.

Conjugation. pSET152 and its derivatives were introduced by transformation into ET12567 containing the RK2 derivative pUZ8002 (62). pUZ8002can supply transfer functions to oriT-carrying plasmids, suchas pSET152, but is not efficiently transferred itself becauseof a mutation in its own oriT. However, a low level of self-transferallowed pUZ8002 to be introduced into ET12567. Conjugations betweenE. coli (pUZ8002) and S. coelicolor were carried out essentiallyas described previously (34).

RNA isolation. RNA was isolated from liquid-grown mycelium as described elsewhere (28). However, rather than exhaustive phenol-chloroformextraction and DNase treatment, RNA was purified from contaminatingDNA and protein by CsCl gradient centrifugation following an initialphenol-chloroform extraction, as described previously (26).RNA was isolated from solid media by scraping mycelium and sporesfrom cellophane-covered plates and extracting as described aboveexcept that, after the addition of phenol-chloroform, the mixturewas heated at 65°C for 10 min prior to vortexmixing.

S1 nuclease transcription mapping. The hrdD promoter region was mapped by using a probe generated by PCR from pIJ2036 with a 5'-end-labelled oligonucleotideprimer internal to hrdD (HD1; 5'-TTCAGCGGGTGGTCCGGTGGAC-3') andthe reverse sequencing primer. HD1 (30 pmol) was labelled with[ $gamma$ -³²P]ATP (3,000 Ci mmol¹; Dupont-NEN) (57). The end-labelled PCR product was purifiedfrom an agarose gel by using a gel extraction kit (Qiagen). ThedagA promoter region was mapped by using a 560-bp SmaI-AvaII fragmentisolated from pIJ2027, labelled uniquely at the 5' end of theAvaII site, as described elsewhere (8). The protected DNA fragmentswere quantified with a phosphorimager (FujixBAS1000).

Lysozyme sensitivity test. Sensitivity to lysozyme was tested by spotting 5 µl of lysozyme in 10 mM Tris-HCl (pH 8) at various concentrations on confluentlawns of spores on agar (2 × 10⁶ spores per plate). Other cell wall-lytic enzymes tested wereCellosyl (a gift from R. Marquardt, Hoechst AG, Frankfurt, Germany),mutanolysin (Sigma), or CwlA amidase (20).

Isolation and analysis of peptidoglycan. Peptidoglycan was prepared by a modification of the method of Atrih et al. (3). Fifty milliliters of mid- to late-exponentialcultures in NMMP plus glucose were centrifuged for 2 min at 5,000× g. The mycelium was resuspended in 10 ml of extraction buffer(50 mM Tris-HCl, 2 mM EDTA, 10 mM dithiothreitol [pH 7]), heatedin a boiling-water bath for 20 min to inactivate autolysins, andthen transferred to ice. The mycelium was disrupted by using aFrench press, and then 10% sodium dodecyl sulfate was added toa final concentration of 4%, followed by incubation at 37°C for40 min. Crude walls were collected at room temperature by centrifugationat 11,000 × g for 20 min, then washed four times with warm water.The pellet was resuspended in 6 ml of Tris-HCl (pH 7) and treatedwith pronase (0.5 mg/ml; Sigma) at 60°C for 90 min. Cell wallswere collected as before, resuspended in 5 ml of extraction buffercontaining 4% sodium dodecyl sulfate, and boiled for 16 min. Purifiedwalls were collected and washed four times with water as above,then resuspended in MilliQ water and stored at $-$ 20°C.

Cell walls were treated with aqueous hydrofluoric acid to remove the accessory polymers, then digested with Cellosyl and reducedwith sodium borohydride (at a final concentration of 2 mg/ml)as previously described (3). The muropeptide profile was investigatedby applying Cellosyl-digested peptidoglycan to a TSK SWXL2000gel filtration column (7.8 mm by 30 cm; Anachem, Luton, UnitedKingdom). The muropeptides were eluted with 40 mM sodium phosphate(pH 6.5) at a flow rate of 0.3 ml min¹, and the eluted compounds were detected by the absorbance at202 nm (A₂₀₂). Muropeptide separations carried out at a highertemperature (45°C versus the standard 40°C) or over a longer gradient(180 min versus the standard 160 min) resulted in similar profiles.Amino acid analysis was performed by the Pico Tag method (3).The cross-linking index was determined as described elsewhere(42).

	RESULTS

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sigE mutants are sensitive to cell wall-hydrolytic enzymes. To investigate the biological role of sigE in S. coelicolor, two mutant alleles were constructed in vitro: one with an in-frameinternal deletion mutation and one with a hygromycin resistancegene (hyg) insertion mutation (Fig. 1). These mutant alleles wereused to replace the wild-type allele in M600, a plasmid-free derivativeof the wild-type strain, creating J2130 ( $Delta$ sigE) and J2141 (sigE::hyg).The former mutation should be nonpolar on potential downstreamgenes, whereas the hyg insertion mutation might affect the expressionof any genes cotranscribed with sigE.

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FIG. 1. Restriction map of the S. coelicolor 2.05-kb PvuII insert containing sigE in pIJ5950. The sigE open reading frame is represented by an open arrow; the position of the hyg insertion mutation (A) and the extent and sequence of the $Delta$ sigE in-frame deletion mutation (B) are shown.

Compared to M600, the sigE mutants grew well and sporulated with equal vigor on MM, R2, R2YE, and SMMS media. They producednormal levels of the pigmented antibiotics actinorhodin and undecylprodigiosinand of the calcium-dependent lipopeptide antibiotic CDA. The sigEmutants were also unaffected in their resistance to heat, theirability to produce siderophores, and their resistance to oxidizingagents $---$ phenotypes controlled by ECF sigma factors in other bacteria(44).

However, the sigE mutants were up to 50 times more sensitive to egg white lysozyme (Fig. 2), an enzyme which hydrolyzes the $beta$ 1-4 linkage between adjacent N-acetylmuramic acid and N-acetylglucosamineunits in the glycan backbone of peptidoglycan. In our standardassay, lysozyme was spotted onto freshly plated confluent lawnsof spores and zones of clearing were noted after 48 h. Under theseconditions, lysozyme sensitivity probably arises soon after germinationbecause Streptomyces spores are lysozyme resistant, whereas germlingsare especially sensitive (55). Indeed, identical results wereobtained by spotting lysozyme on newly germinated spores. Vegetativemycelia from sigE mutants were also more sensitive to lysozymethan that from the wild type, as judged by spotting lysozyme on12-h-old confluent plates. To rule out the possibility that lysozymesensitivity was caused by polar effects on possible downstreamgenes, sigE was reintroduced into the mutants by using the vectorpSET152, which integrates site-specifically at the phage $phi$ C31attB site (5). A derivative of pSET152 carrying a 2.05-kb PvuIIfragment containing sigE restored lysozyme resistance to J2130and J2141, whereas pSET152 carrying the $Delta$ sigE mutation in thesame fragment did not (data not shown).

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FIG. 2. Lysozyme sensitivity of M600 (sigE⁺) (A) compared to that of J2130 ( $Delta$ sigE) (B). Spores of each strain were plated on Difco nutrient agar to give confluent lawns and then a twofold dilution series of egg white lysozyme (from 1 mg ml¹, as indicated) was spotted onto the plates immediately after plating. Zones of clearing, seen here as dark circles, were photographed after 2 days of incubation at 30°C.

In other organisms, resistance to lysozyme has been attributed to O acetylation of peptidoglycan at the C-6 hydroxyl moietyof muramyl residues (18). However, the sigE mutants were alsomuch more sensitive than their parent to Cellosyl and mutanolysin,muramidases which are insensitive to this type of O acetylation,suggesting that the C-6 position is unaltered inacetylation.

To see if the sigE mutants were also susceptible to cell wall-lytic enzymes that cut other linkages in the peptidoglycan,we tested their sensitivity to the CwlA amidase from B. subtilis(20), which cleaves the peptide side chain from the glycan backbone.By the plate assay, the sigE mutants were found to be at least50-fold more sensitive than the wild type to the CwlA amidase(data not shown). Sensitivity to more than one type of cell wall-hydrolyticenzyme suggested that the mutants have an altered cell wall structure,which allowed hydrolytic enzymes increased access to thepeptidoglycan.

Muropeptide analysis of sigE mutant cell walls indicates an altered composition. In an attempt to detect possible changes in cell wall structure, the muropeptide profiles of a sigE mutant and its congenicparent were determined. Cell walls were isolated from exponentiallygrowing cultures and subjected to enzymatic hydrolysis followedby reverse-phase high-performance liquid chromatography (RP-HPLC).The muropeptide profiles obtained after RP-HPLC for M600 (sigE⁺) and J2130 ( $Delta$ sigE) are shown in Fig. 3A and B, respectively.For each strain, the profiles were reproducible both in peak retentiontime and in the relative amounts of different muropeptides forthree independent cultures. The two strains presented an identicalcomplement of muropeptides but showed differences in the abundancesof certain muropeptides. For example, muropeptides X1 and X3,most likely a monomer and a dimer, respectively, are present inlarger amounts in J2130, while muropeptide X2 is less abundantin J2130. Amino acid analysis revealed, in addition to glucosamineand muramic acid, comparable ratios of glutamic acid, glycine,alanine, and diaminopimelic acid in both strains. These aminoacids have been identified previously in the peptidoglycan ofstreptomycetes (58). One possible explanation for the alteredratio of muropeptides would be a difference in the cross-linkingof the peptidoglycan. To determine whether the sigE mutant wasaffected in peptidoglycan cross-linking and in the distributionof oligomers, muropeptides digested with Cellosyl were separatedby gel permeation HPLC. The cross-linking index, as determinedby the method of Martin and Gmeiner (42), was 47 for M600 and46.4 for J2130, indicating no significant difference between thetwo strains.

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FIG. 3. Analysis of peptidoglycan composition by RP-HPLC. Samples of peptidoglycan isolated from M600 (sigE⁺) (A) or J2130 ( $Delta$ sigE) (B) were digested with Cellosyl and subjected to HPLC analysis, and the A₂₀₂ values of the eluates were monitored. Muropeptides that show particularly different abundances in the two strains are marked (X1 through X3).

sigE mutants conditionally overproduce actinorhodin on media deficient in Mg²⁺. Although the sigE mutants appeared identical to the parent strain on most solid media, they overproduced the blue-pigmentedantibiotic actinorhodin on certain complex media such as L agar(Fig. 4) and MS agar (data not shown). On these media the coloniessporulated very poorly and also had a crenellated appearance,which was not caused by actinorhodin overproduction, because itremained in a constructed sigE act double mutant (data not shown).Again, the overproduction of actinorhodin and the crenellationcould be complemented in trans by integrating a functional copyof sigE into the chromosome at the $phi$ C31 attB site by using pSET152.

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FIG. 4. The $Delta$ sigE mutant, J2130, overproduces the blue-pigmented antibiotic actinorhodin on medium deficient in Mg²⁺. Ten microliters of a spore suspension (10⁸ spores ml¹) was spotted on L agar alone or on L agar plus 1.6 mM MgSO₄. Plates were photographed after 3 days of incubation at 30°C.

The media on which the SigE phenotype was apparent (L agar and MS agar) lack added Mg²⁺, in contrast to the media on which the phenotype was not manifested(SMMS, R2YE, R2, and MM). When MgSO₄ (1.6 mM) was included inthe L-agar plates, the $Delta$ sigE mutant J2130 no longer overproducedactinorhodin (Fig. 4) and the colony surface was no longer crenellated(data not shown). Also, when the concentration of MgSO₄ in SMMSagar was reduced from the usual 5 mM to less than 1 mM, the sigEmutants produced actinorhodin earlier and in greater amounts thanthe parental wild type (data not shown). The suppression effectwas caused by Mg²⁺ and not by the counterion, since it was observed with eitherMgSO₄ or MgCl₂. The addition of Ca²⁺ could also suppress the overproduction of actinorhodin and colonycrenellation in the sigE mutants, although to a slightly lesserextent.

However, Mg²⁺ could not suppress the lysozyme sensitivity phenotype of sigE mutants. The presence of 5 mM Mg²⁺ in SMMS agar increased the resistance to lysozyme of both thesigE mutants and the parent, M600, but the sigE mutants remainedsubstantially more sensitive to lysozyme than M600 in the presenceof high (5 mM) or low (50 µM) concentrations of Mg²⁺.

The hrdDp₁ promoter is $sigma$ ^E dependent. To facilitate in vitro analysis of $sigma$ ^E, the protein was overproduced in E. coli and purified to homogeneity. A sigE overexpressionplasmid, pIJ2078, based on the T7 expression vector pET11c, wasconstructed as described in Materials and Methods. Active $sigma$ ^E was recovered from inclusion bodies by using a minor modificationof the method of Nguyen et al. (48). This involved the purificationof the inclusion bodies, their solubilization with 0.25% (wt/vol)Sarkosyl, extensive dialysis to remove the detergent, and furtherpurification by Mono-Q anion-exchange columnchromatography.

Previous work showed that the $sigma$ ^E holoenzyme (E $sigma$ ^E) purified from S. coelicolor can direct transcription from the dagAp₂ promoterin vitro (9). An alignment of streptomycete promoters compiledby Bourn and Babb (6) revealed that the hrdDp₁ promoter isidentical to dagAp₂ at 5 of 6 and 4 of 6 bases in the putative $-$ 35 and $-$ 10 regions, respectively (Fig. 5). hrdDp₁ is one of twopromoters that drive expression of the gene encoding $sigma$ ^HrdD, one of three S. coelicolor sigma factors that are very closelyrelated in amino acid sequence and promoter specificity to $sigma$ ^HrdB, the principal, essential sigma factor of this species. However,the function of $sigma$ ^HrdD is unknown; hrdD null mutants are apparently unaffected in growth,morphological development, and antibiotic production (10). Tosee if $sigma$ ^E could direct transcription from hrdDp₁ in vitro, recombinant $sigma$ ^E was added to core RNA polymerase and used to transcribe hrdDp₁-containingtemplates. The two templates used, HindIII-NarI and HindIII-SstI,would be expected to lead to the formation of runoff productsof 316 and 456 nucleotides (nt), respectively. Products of theexpected sizes were obtained in a $sigma$ ^E-dependent manner (Fig. 6). In contrast, no transcription fromhrdDp₂ was detected. In vitro transcription using total RNA polymeraseisolated from YEME-grown cultures of S. coelicolor M145 produceda low level of hrdDp₁ transcripts but abundant transcription fromhrdDp₂ (Fig. 6).

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FIG. 5. The three classes of promoter described in this paper. dagAp₂ and phsAp are recognized by E $sigma$ ^E in vitro, but their activities are unaffected in sigE null mutants; hrdDp₁ is recognized by E $sigma$ ^E in vitro and is highly sigE dependent in vivo; hrdDp₂ is not recognized by E $sigma$ ^E in vitro but is partially sigE dependent in vivo. The putative $-$ 35 and $-$ 10 regions are underlined, and the conserved sequences are shown in boldface. The transcription start points are italicized and boldfaced.

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FIG. 6. In vitro transcription of hrdD. Core RNA polymerase (core), core RNA polymerase plus recombinant $sigma$ ^E (core + $sigma$ ^E), or total RNA polymerase isolated from S. coelicolor M145 (holo) was used in in vitro transcription reactions. Transcription from hrdDp₁ would be expected to lead to the formation of a runoff product of 316 or 456 nt with either a HindIII-NarI or a HindIII-SstI fragment, respectively, used as a template. Transcription from hrdDp₂ would be expected to lead to the formation of a runoff product of 204 nt with the HindIII-SstI template. ETE, end-to-end transcription. The mobilities of the size markers (M) are indicated on the left.

To see if E $sigma$ ^E also transcribed hrdDp₁ in vivo, S1 nuclease mapping of hrdD was performed with RNA isolated from M600 and thesigE mutants J2130 and J2141. For this experiment, RNA was isolatedfrom surface-grown MS agar cultures because growth on this mediumgave a clear mutant phenotype, suggesting that $sigma$ ^E was active in the wild-type strain under these conditions. RNAwas isolated from 36-h cultures; by this time aerial myceliumwas present and a few spores could be seen in both M600 and thesigE mutants. Representative results (Fig. 7A) showed that thelevel of transcription from hrdDp₁ was severely reduced (~20-fold)in J2130 and J2141 compared to that in M600. However, weak promoteractivity could still be detected in RNA samples from both sigEmutants. Taken together with the in vitro data, these data showthat hrdDp₁ is an in vivo target for E $sigma$ ^E but that another form of RNA polymerase holoenzyme also contributesto transcription from hrdDp₁. Interestingly, the level of hrdDp₂activity was also significantly lower (approximately threefold)in RNA isolated from the sigE mutants, suggesting that hrdDp₂also depends partially on sigE. There is considerable similaritybetween hrdDp₁ and hrdDp₂, with 4 of 6 nt in both the proposed $-$ 35 and $-$ 10 promoter recognition sequences being identical (Fig.5), but since E $sigma$ ^E cannot direct transcription from hrdDp₂ in vitro, it is not clearif E $sigma$ ^E recognizes hrdDp₂ in vivo.

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FIG. 7. (A) S1 mapping of the hrdD promoter region using RNA isolated from S. coelicolor M600 (sigE⁺), J2130 ( $Delta$ sigE), and J2141 (sigE::hyg) grown on MS agar. (B) S1 mapping of the hrdD promoter region using RNA isolated from S. coelicolor M600 (sigE⁺) and J2130 ( $Delta$ sigE) grown in NMMP liquid medium with 2 mM (high Mg) or 50 µM (low Mg) MgCl₂. The uniquely 5'-end-labelled probe was prepared as described in Materials and Methods. Protected fragments corresponding to initiation at hrdDp₁ and hrdDp₂ are indicated.

Expression of hrdD is induced in cultures deficient in Mg²⁺ in a $sigma$ ^E-dependent manner. The actinorhodin overproduction and altered colony morphology of the sigE mutants could be suppressed by the addition of Mg²⁺ to the medium. To see if $sigma$ ^E-directed expression of hrdD varied in response to changing Mg²⁺ concentrations, RNA was isolated from NMMP liquid cultures containinghigh (2 mM) or low (50 µM) concentrations of Mg²⁺, and transcription was assessed by S1 nuclease mapping. In thesigE⁺ strain, M600, the levels of hrdDp₁ and hrdDp₂ transcripts increasedapproximately 12- and 4-fold, respectively, in Mg²⁺-deficient medium (Fig. 7B), whereas in J2130 ( $Delta$ sigE) both promoterswere transcribed at low basal levels and were insensitive to Mg²⁺concentrations.

$sigma$ ^E is not essential for dagAp₂ transcription in vivo. $sigma$ ^E was originally identified by its ability to direct transcription from the dagAp₂ promoter in vitro (9). To see if dagAp₂required $sigma$ ^E for activity in vivo, transcript levels were investigated byS1 nuclease mapping. There was no difference between J2130 ( $Delta$ sigE)and its parent, M600, in the level of the dagAp₂ transcript, indicatingthat $sigma$ ^E does not contribute significantly to dagAp₂ transcription invivo, at least under the growth conditions used here (data notshown). To see if $sigma$ ^E was required when the copy number of dagAp₂ was increased, S1nuclease mapping was performed on RNA isolated from J2130 or M600carrying the dagA gene on a multicopy plasmid (pIJ2020). Again,there was no difference in the level of the dagAp₂ transcriptbetween the two strains (data notshown).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The evidence presented here suggests that sigE is required for normal cell wall structure in S. coelicolor. sigE null mutantsare particularly sensitive to cell wall-lytic enzymes, includingmuramidases and amidases, and their peptidoglycan has an alteredmuropeptide composition. Although the $Delta$ sigE mutant showed alterationsin the ratio of certain muropeptides, a wild-type complement ofmuropeptides appeared to be maintained. One possible explanationfor this is a change in the activity of autolysins, enzymes thathydrolyze peptidoglycan and play important roles in cell wallgrowth, cell separation, and differentiation (60). However,because the activities of autolysins can be affected by changesin the cell wall itself (see below), it would be difficult toidentify the root cause of the altered muropeptidecomposition.

Sensitivity to cell wall-lytic enzymes often correlates with increased sensitivity to autolysins and can be attributed toa range of different changes in the cell wall, including O acetylationof the peptidoglycan (18) and modification of the accessorypolymers (see, e.g., references 43 and 61). A change in thedegree of O acetylation of the C-6 hydroxyl moiety of muramylresidues is unlikely to be the cause of increased sensitivityto lysozyme because sigE mutants are also more sensitive to themuramidases Cellosyl and mutanolysin, enzymes which are unaffectedby this type of acetylation. In addition, sigE mutants are alsomore sensitive to the CwlA amidase, which cuts peptidoglycan ata different position (20). Preliminary investigations into possiblechanges in the accessory polymers have not revealed any differencesin the teichoic acid content and composition of sigE mutants (53).The future identification of genes under the control of $sigma$ ^E should help define its precise role in cell wall structure. Helmannand colleagues have used consensus-based computer searches ofthe complete B. subtilis genome sequence to identify promoters,and hence genes, under the control of the ECF sigma factors $sigma$ ^X and $sigma$ ^W (29, 32). The ongoing S. coelicolor genome sequencing project(www.sanger.ac.uk/Projects/S_coelicolor/) should permit the sameapproach to be used in identifying candidate members of the $sigma$ ^Eregulon.

Interestingly, B. subtilis $sigma$ ^X is involved in transcribing a number of genes concerned with cell wall structure, including lytR,a regulator of autolysin expression, and csbB, which encodes aputative membrane-bound glycosyl transferase, possibly involvedin peptidoglycan biosynthesis (29). It is therefore conceivablethat $sigma$ ^E and $sigma$ ^X play related roles in S. coelicolor and B. subtilis,respectively.

sigE mutants required Mg²⁺ or Ca²⁺ for normal growth and sporulation. Divalent cations can stabilize cell walls (17, 36, 41,47) and can protect cells from autolysis as well as from exogenouslytic enzymes (36, 61). Thus, it seems likely that Mg²⁺ stabilizes the defect in the cell walls of sigE mutants, therebysuppressing the phenotype. However, even in the presence of Mg²⁺, the defect in the cell walls of the sigE mutants remains becausethey are still more sensitive to cell wall-lytic enzymes thanthe parental wild-type strain. It is not clear why the sigE mutantsoverproduce the antibiotic actinorhodin on medium with low levelsof Mg²⁺. Antibiotic production can be induced by a number of differentstresses (4), and it is possible that the overproduction ofactinorhodin seen in sigE mutants is an indirect consequence ofstresses induced by the cell wall defect when it is not stabilizedby Mg²⁺.

$sigma$ ^HrdD is one of three S. coelicolor sigma factors that are very closely related in amino acid sequence and promoter specificityto $sigma$ ^HrdB, the principal, essential sigma factor of this species. However,the function of $sigma$ ^HrdD is unknown; hrdD null mutants are apparently unaffected in growth,morphological development, and antibiotic production (10). Expressionof hrdD was found to be partially dependent on sigE, but sincehrdD mutants do not resemble sigE mutants, the sigE mutant phenotypeis not manifested through hrdD. Expression of hrdD increased incultures grown under conditions of Mg²⁺ deficiency in a sigE-dependent manner. However, it is not clearwhether the cells were responding directly to Mg²⁺ deficiency or to possible changes in the cell wall resultingfrom this deficiency. Magnesium has been shown to affect the expressionof cell wall proteins in Bacillus brevis 47 (1) and to affectlipopolysaccharide composition in Salmonella typhimurium via thePhoP-PhoQ virulence regulatory system (23). However, only inthe case of the PhoP-PhoQ system has Mg²⁺ been shown to act directly as an extracellular signal (21).

In sigE mutants, transcription from hrdDp₁ is severely reduced but not abolished, showing that another RNA polymerase holoenzymealso contributes to hrdDp₁ transcription in vivo. Given that hrdDp₁is clearly similar to cognate promoters of other ECF sigma factors,it is likely that this holoenzyme contains another ECF sigma factor.In addition to $sigma$ ^E, there are at least another five ECF sigma factors encoded bythe S. coelicolor genome (46, 49, 51). Considering thatthere are 10 ECF sigma factors in another actinomycete, Mycobacteriumtuberculosis (not including $sigma$ ^F, which was classified as an ECF sigma factor by Cole et al. [12]but is more similar to the sporulation subfamily [15]), we suspectthat many more ECF sigma factors will be discovered in S. coelicolorby genome sequencing. It will be interesting to establish theextent to which different ECF sigma factors have overlapping promoterspecificity and thus overlapping function. Indeed, there is ampleevidence, from this work and from work with B. subtilis (29,31), that more than one ECF sigma factor can recognize certainpromoters.

Although transcription from both hrdDp₁ and hrdDp₂ was reduced in the sigE mutants, only hrdDp₁ was recognized by E $sigma$ ^E in vitro. This could mean that the dependence of hrdDp₂ on $sigma$ ^E is indirect or that transcription from hrdDp₂ in vivo requiresan accessory factor absent from the in vitro reactions, or thatthe in vitro reaction conditions do not reflect the in vivo conditionsin some other way. It is feasible that $sigma$ ^E can direct transcription from hrdDp₂ in vivo, because the promoteris very similar to hrdDp₁ in both the $-$ 35 and $-$ 10 recognitionsequences (Fig. 5). The residual activity of hrdDp₂ in a sigEnull mutant is due, at least in part, to a newly identified ECFsigma factor, $sigma$ ^R (51). $sigma$ ^R directs transcription from hrdDp₂ in vitro (35), and hrdDp₂depends partially on $sigma$ ^R in vivo (52). The construction of a sigE sigR double mutantwill be needed to establish if yet other holoenzymes are involvedin the transcription of hrdDp₂ invivo.

Although $sigma$ ^E was originally identified by its ability to direct transcription from dagAp₂ in vitro, $sigma$ ^E did not contribute to transcription from dagAp₂ in vivo, at leastunder the conditions used here. Similarly, in a related paperwe showed that while E $sigma$ ^E could direct transcription of the phsA gene of S. antibioticusin vitro, sigE was not required for normal levels of phsA transcriptionin vivo (34). Thus, three classes of promoter have been describedin this paper: dagAp₂ and phsAp are recognized by E $sigma$ ^E in vitro, but their activities are unaffected in sigE null mutants;hrdDp₁ is recognized by E $sigma$ ^E in vitro and is highly sigE dependent in vivo; hrdDp₂ is notrecognized by E $sigma$ ^E in vitro but is partially sigE dependent in vivo. Although allthe promoters are quite similar in both the $-$ 35 and $-$ 10 recognitionregions, there are some clear differences (Fig. 5). Major challengesfor the future will be to establish which nucleotides in thesepromoter regions determine sigma specificity and to establishthe extent to which promoter dependence is affected by the growthconditionsused.

	ACKNOWLEDGMENTS

We thank Keith Chater, David Hopwood, and Tobias Kieser for critical reading of the manuscript and Andrew Philipson, Ian Hancock,and Maureen McCann for unpublished cell wallanalyses.

This work was funded by BBSRC grant GR/J67994 (to M.J.B.), by a Lister Institute research fellowship (to M.J.B.), by a RoyalSociety University Research fellowship (to S.J.F.), by BBSRC grant50/F08202 (to S.J.F.) and by a grant-in-aid to the John InnesCentre from theBBSRC.

	FOOTNOTES

^* Corresponding author. Mailing address: John Innes Centre, Colney, Norwich NR4 7UH, United Kingdom. Phone: (44) 1603 452571.Fax: (44) 1603 456844. E-mail: pagetm{at}bbsrc.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
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Evidence that the Extracytoplasmic Function Sigma Factor E Is Required for Normal Cell Wall Structure in Streptomyces coelicolor A3(2)

Evidence that the Extracytoplasmic Function Sigma Factor $sigma$ ^E Is Required for Normal Cell Wall Structure in Streptomyces coelicolor A3(2)