Development and Characterization of a Xylose-Dependent System for Expression of Cloned Genes in Bacillus subtilis: Conditional Complementation of a Teichoic Acid Mutant

doi:10.1128/AEM.67.1.403-410.2001

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Applied and Environmental Microbiology, January 2001, p. 403-410, Vol. 67, No. 1
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.1.403-410.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Development and Characterization of a Xylose-Dependent System for Expression of Cloned Genes in Bacillus subtilis: Conditional Complementation of a Teichoic Acid Mutant

Amit P. Bhavsar, Xumei Zhao, and Eric D. Brown^*

Antimicrobial Research Centre, Department of Biochemistry, McMaster University, Hamilton, Ontario, Canada L8N 3Z5

Received 22 May 2000/Accepted 24 September 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

We have developed a xylose-dependent expression system for tight and modulated expression of cloned genes in Bacillus subtilis.The expression system is contained on plasmid pSWEET for integrationat the amyE locus of B. subtilis and incorporates components ofthe well-characterized, divergently transcribed xylose utilizationoperon. The system contains the xylose repressor encoded by xylR,the promoter and 5' portion of xylA containing an optimized catabolite-responsiveelement, and intergenic xyl operator sequences. We have rigorouslycompared this expression system to the isopropyl- $beta$ -D-thiogalactopyranoside-inducedspac system using a thermostable $beta$ -galactosidase reporter (BgaB)and found the xyl promoter-operator to have a greater capacityfor modulated expression, a higher induction/repression ratio(279-fold for the xyl system versus 24-fold with the spac promoter),and lower levels of expression in the absence of an inducer. Wehave used this system to probe an essential function in wall teichoicacid biosynthesis in B. subtilis. Expression of the teichoic acidbiosynthesis gene tagD, encoding glycerol-3-phosphate cytidylyltransferase,from the xylose-based expression system integrated at amyE exhibitedxylose-dependent complementation of the temperature-sensitivemutant tag-12 when grown at the nonpermissive temperature. PlasmidpSWEET thus provides a robust new expression system for conditionalcomplementation in B. subtilis.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Manipulated gene expression in bacteria is of fundamental importance to understanding the effects of expression or depletionof gene products on bacterial physiology. Such investigationsideally require the controlled expression of a cloned gene froma tightly regulated, inducible promoter. This is particularlytrue in studies of indispensable genes in bacteria where targeteddeletions of these genes require expression from complementingcopies of the genes. The dispensability of such genes and thephenotypes associated with their loss are most rigorously examinedthrough conditional expression of the complementing genes. Especiallychallenging in such studies are the need for extremely tight regulationof expression and the tendency for the majority of regulated expressionsystems to "leak" in the absence of aninducer.

The state of the art in controlled expression in Bacillus subtilis is the spac expression system, which is based on the applicationof the lac repressor-operator control system from Escherichiacoli. In B. subtilis, the system uses a constitutive penicillinasepromoter to express the lac repressor. Isopropyl- $beta$ -D-thiogalactopyranoside(IPTG)-dependent expression of the target gene is from a hybridpromoter-operator consisting of the SPO1 bacteriophage promoterand lac operator sequence (35). Despite its broad use for conditionalexpression in B. subtilis, the spac system has been widely recognizedfor its capacity to allow significant expression in the absenceof an inducer. Indeed, only relatively recently has there beena systematic study of expression from the spac promoter, indicatingdemonstrable uninduced expression of lacZ from the spac promoterof the pMUTIN vector system (33).

The xylose operon has emerged as a well-characterized B. subtilis regulatory system with the potential for particularly tighttranscriptional regulation (5, 6, 12, 13, 16-19). Xyloseutilization in B. subtilis requires the production of xylose isomerase(XylA) and xylulose kinase (XylB) and is regulated at the levelof transcription by a xylose-responsive repressor protein encodedby xylR and by catabolite repression. Genes xylR and xylAB aredivergently transcribed from a common intergenic region containingxyl operator sequences which are bound by XylR in the absenceof an inducer. Transcription of the xyl operon is also cataboliterepressed through the cis-acting catabolite-responsive element(CRE) located in the coding sequence of xylA.

Cell wall teichoic acids are a diverse group of phosphate-rich polymers which are covalently linked to peptidoglycan and constitutea substantial portion of the cell wall of gram-positive bacteria.Teichoic acids have been implicated as virulence factors in avariety of gram-positive bacterial infections (14, 22, 30),and growing evidence indicates that teichoic acid biosynthesisis indispensable for the growth of B. subtilis (2, 21, 23).Conditional lethal mutations in the poly(glycerol phosphate) teichoicacid gene cluster (tag) of B. subtilis 168 have been mapped toa number of genes, including tagD (27), encoding glycerol-3-phosphatecytidylyltransferase (25).

In this work, we have taken advantage of a notable depth of knowledge of the xylose utilization operon to develop a xylose-dependentpromoter-operator system for tight and modulated expression ofcloned genes in B. subtilis. As a point of reference, we haverigorously compared this expression system to the IPTG-inducedspac system for efficiency of regulation and modulation of expression.Finally, we have put expression of tagD under control of the xylose-basedexpression system described here and have for the first time showntrans complementation of a teichoic acidmutant.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

General methods. Strains, plasmids, and primers used are listed in Tables 1 and 2. B. subtilis strains were grown in rich (Luria-Bertani[LB]) or minimal [15 mM (NH₄)₂SO₄, 80 mM K₂HPO₄, 44 mM KH₂PO₄,3.4 mM sodium citrate, 1 mM MgSO₄ (pH 7.4)] medium plus arabinose(0.2%). (Arabinose was previously found not to exert a catabolite-repressiveeffect on the xylose operon [18].) The following concentrationsof antibiotics were used for selection: 50 µg of ampicillin perml, 10 µg of chloramphenicol (CHL) per ml, and 1 µg of erythromycinper ml. Unless otherwise stated, glucose was added to 0.2%, xylosewas added to 2%, IPTG was added to 1 mM, and 5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside(X-Gal) was added to 80 µg/ml. Cloning was performed in E. colistrain Novablue (Novagen) according to established methods (29).Transformation of these cells was performed according to the manufacturer'sinstructions. Restriction enzymes were purchased from New EnglandBiolabs (Beverly, Mass.) and used according to the manufacturer'sinstructions. Transformation of B. subtilis organisms was performedaccording to procedures previously described (4); derivativesof pDG364 were targeted to amyE via double recombination as linearDNA, using approximately 1 µg of PstI-digested plasmid. All otherchemicals were purchased from Sigma (Mississauga, Ontario, Canada).

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TABLE 1. List of strains and plasmids

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TABLE 2. List of primers

Plasmid construction. Plasmid pSWEET-tagD was constructed using the following strategy. The xylR gene, the xylA promoter, and the first 58 nucleotidesof the xylA gene (including the CRE site) were amplified as asingle product from B. subtilis W23 chromosomal DNA, using theprimers AB01 and AB02. Primer AB02 incorporated two mutationsin the CRE site, G $right-arrow$ T and A $right-arrow$ T at positions 3 and 10, respectively(18, 34). Gene tagD, from $-$ 24 to stop (including its nativeribosome binding site), was amplified from B. subtilis 168 usingthe primers AB03 and AB04. The above PCR products were digestedwith PacI and ligated together. The ligation product was reamplifiedwith primers AB01 and AB04, digested with BamHI, and ligated intoBamHI-digestedpDG364.

To create pSWEET-bgaB the xylR-xylA fragment was reamplified from pSWEET-tagD with primers AB05 and AB06. The amplified fragmentwas digested with BamHI and BglII and ligated into BamHI-digestedpDG364 to create plasmid pSWEET. Plasmid pKL4 was used as a templatefor amplification of bgaB (31) using primers AB07 and AB08.Primer AB07 incorporated nucleotides $-$ 24 to $-$ 1 of B. subtilistagD so that the ribosome binding sites and their contexts wereidentical in pSWEET-tagD and pSWEET-bgaB. The bgaB PCR productwas digested with PacI and BamHI and ligated into pSWEET digestedwith the sameenzymes.

To facilitate a rigorous comparison of the xylose-based expression system in pSWEET with that of the commonly used spac system,we constructed clones of bgaB and tagD under the control of thespac promoter in pDR67 (15) with ribosome binding sites andcontexts identical to those used with pSWEET (i.e., nucleotides $-$ 24 to $-$ 1 of tagD, as described above). Those plasmids were namedpSPAC-bgaB and pSPAC-tagD, respectively. In addition, we constructeda lacI deletion of pSPAC-bgaB, designated pSPAC-bgaB $Delta$ lacI, inorder to test the importance of lacI to the regulation of thespac promoter. Gene bgaB was amplified from pKL4 using primersAB07 and AB09. To create pSPAC-bgaB, the amplified product wasdigested with SmaI and BglII and ligated to SmaI- and BglII-digestedpDR67. For pSPAC-bgaB $Delta$ lacI, the amplified product was digestedwith SmaI and BamHI and ligated to SmaI- and BamHI-digested pDR67.To place tagD under the control of the spac promoter, tagD wasexcised from pSWEET-tagD with PacI and BamHI and ligated intoPacI- and BamHI-digested pSPAC-bgaB.

$beta$ -Galactosidase activity assay. An assay of thermostable $beta$ -galactosidase has been described previously (31, 32). In brief, cells were grown to an opticaldensity at 600 nm (OD₆₀₀) of 0.5, pelleted, and resuspended inan equivalent volume of buffer B (25 mM potassium phosphate, 50mM KCl, and 1 mM MgSO₄ [pH 6.4]). Sample aliquots ranging from0.1 to 0.5 ml were diluted to 0.8 ml in buffer B and lysed for30 min at 28°C with the addition of 16 µl of lysozyme (10 mg/ml).Lysis was followed by the addition of 40 µl of 10% Triton X-100.Subsequently, a preincubation at 60°C for 15 min was used to inactivateendogenous $beta$ -galactosidase. The assay was initiated with the additionof 0.2 ml of o-nitrophenyl- $beta$ -D-galactopyranoside (ONPG) at a concentrationof 4 mg/ml and quenched by the addition of 0.5 ml of 1 M Na₂CO₃.Absorbance was recorded at 420 nm in a Spectramax Plus spectrophotometer(MolecularDevices).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

We chose to construct a xylose-based expression system by incorporating components of the xylose operon from strain W23 ofB. subtilis. The xylose utilization machinery of this B. subtilisstrain has been the subject of extensive characterization (5,6, 12, 13, 16-19). The xyl expression system developed inthis work includes the xylose repressor encoded by xylR, intergenicxyl operator sequences, the xylA promoter, and the 5' portionof xylA containing an optimized CRE (Fig. 1). The system is containedon plasmid pSWEET, a derivative of pDG364 (3), for ready integrationof the expression system in the B. subtilis chromosome at amyE.

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FIG. 1. Map of plasmid pSWEET-bgaB. (a) Significant features of the xylose-based expression system. Plasmid pSWEET-bgaB is a derivative of pDG364 (3), which allows integration into the B. subtilis chromosome at amyE via double recombination and selection with CHL (10 µg/ml). The plasmid also has an E. coli origin of replication, denoted ori, and an ampicillin resistance cassette (50 µg/ml) for routine cloning steps. On the outside of the plasmid map, restriction sites of interest are highlighted, including two PstI sites for convenient plasmid linearization, a PacI site (eight-base recognition sequence TTAATTAA) upstream of bgaB, and a polylinker downstream of bgaB (HindIII is not unique). (b) Close-up of key elements of the xylose expression system (not to scale). Shown are xylR, encoding the xylose repressor; the xyl intergenic region, including promoters for xylR (P_xylR), xylA (P_xylA), and xyl operator sequences (xylO); translationally truncated xylA (first 58 nucleotides followed by an in-frame TAA), including an optimized CRE in xylA (see Materials and Methods and reference 18); PacI 5' cloning site; ribosome binding site (SD) native to B. subtilis tagD; and gene bgaB, encoding a thermostable $beta$ -galactosidase from B. stearothermophilus.

Transcriptional regulatory sequences in the xyl operon include tandem overlapping operator sequences downstream of the xylAtranscriptional start site (5) and a CRE located 36 nucleotidesinto the coding sequence of the xylose isomerase gene (xylA) (18).To ensure that the xyl system was maximally subjected to cataboliterepression, we included the first 58 nucleotides of the gene xylAand introduced two mismatches in the CRE site to perfectly matchthe consensus sequence established previously (18, 34). Anin-frame stop codon was placed in the xylA gene following the58th nucleotide, effectively truncating the XylA protein. Downstreamof that translational stop, we constructed pSWEET-bgaB so thatPacI (eight-base recognition sequence TTAATTAA) and one of severalpolylinker enzymes could be used to replace bgaB and its associatedribosome binding site with any sequences ofinterest.

Schrogel and Allmansberger (31) have optimized the use of heat-stable $beta$ -galactosidase, bgaB from B. stearothermophilus,as a reporter gene in B. subtilis, which permits inactivationof endogenous background $beta$ -galactosidase activity. We employedthis reporter system in order to describe the lower limits oftranscriptional control afforded by the xyl system relative tothe spac system. For an unbiased comparison of the xyl and spacexpression systems, we constructed pSPAC-bgaB and pSWEET-bgaBso that their ribosome binding sites and their contexts were identical(see Materials andMethods).

Figure 2a and b demonstrate expression of bgaB from the xyl and spac expression systems (induced with xylose and IPTG, respectively)as indicated by X-Gal hydrolysis in LB agar (EB107 and EB103,respectively). Strain EB104 (spac system without lacI) also showedsignificant X-Gal hydrolysis. Strains EB106 (xyl) and EB105 (spac)were negative-control strains, containing the corresponding expressionsystem but lacking the bgaB gene, and showed no evidence of X-Galhydrolysis. Strains containing both expression systems were platedon X-Gal in the absence of any inducer to assess transcriptionalcontrol (i.e., the leakiness of the expression system). Figure2c shows that the spac system (EB103) produced clearly discerniblelevels of BgaB as revealed by the extent of X-Gal hydrolysis.This cleavage is not due to endogenous $beta$ -galactosidase genes,as demonstrated by the lack of color development in the negative-controlstrain (EB105). The strain lacking lacI (EB104) served to illustratethat while the lac repressor allowed significant transcriptionalcontrol, it did not limit expression beyond the detection of thisassay. In contrast, the xyl expression system (EB107) showed nodiscernible expression in the absence of an inducer and showedno significant deviation from the negative-control strain (EB106).

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FIG. 2. Detection of reporter gene expression by X-Gal hydrolysis on solid media. (a) Strains EB106 (pSWEET) and EB107 (pSWEET-bgaB) were plated on LB-CHL-X-Gal in the presence of 2% xylose. (b) Strains EB103 (pSPAC-bgaB), EB104 (pSPAC-bgaB $Delta$ lacI), and EB105 (pSPAC) were plated on LB-CHL-X-Gal in the presence of 1 mM IPTG. (c) All five strains were plated on LB-CHL-X-Gal in the absence of an inducer. Strains were grown overnight at 37°C and then incubated at 55°C for color development (up to 36 h).

To better characterize the xyl and spac expression systems, B. subtilis strains carrying transcriptional fusions of bgaB toP_xyl and P_spac, respectively, were assayed for $beta$ -galactosidase activity after growth in liquid media. Figure3 shows an example ( $beta$ -galactosidase activities of EB104 underinducing conditions) of our efforts to ensure that the assay waslinear both with time and with the volume of cells. Under theconditions used in this work, o-nitrophenol production remainedlinear for 240 min and was directly dependent on the amount ofsample added to the assay. Having established parameters for alinear response in the assay of thermostable $beta$ -galactosidase,EB103 and EB107 were grown in both rich (LB) and minimal media(plus 0.2% arabinose) in the presence or absence of an inducer.The xyl expression system showed a significantly higher ratioof induction to repression than the spac system (ratios of 279versus 24 in rich media, respectively), which can be attributedto higher levels of expression under inducing conditions (Table3). Our analysis of the spac system indicates a somewhat lowerinduction/repression ratio than that previously recorded (140-fold)for the comparable spac system of pMUTIN1 (33), perhaps dueto differences in the genetic contexts of each system. Overall,the xyl system demonstrated a 16-fold increase in expression relativeto the spac system ( $beta$ -galactosidase units of 12,824 and 814 inrich media for the xyl and spac systems, respectively). Undernoninducing conditions, however, there was no significant differencebetween the xyl and spac expression systems using this assay ( $beta$ -galactosidaseunits of 46 ± 21 [mean ± standard deviation] and 34 ± 20 in richmedium, respectively). Indeed, significant noise in this assay,which was particularly troublesome at the lower limits of detection,may have precluded our detection of otherwise significant differencesbetween these two expression systems.

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FIG. 3. Linearity of heat-stable $beta$ -galactosidase assay. Strain EB104 was grown (LB-CHL with 1 mM IPTG) to mid-log phase (OD₆₀₀ = 0.5) and assayed for BgaB activity (see Materials and Methods) at different sample volumes ( $open circle$ , $down-triangle$ , and

denote 0.1, 0.2 and 0.5 ml of culture, respectively) for up to 4 h. $beta$ -Galactosidase activity was defined as micromoles of o-nitrophenol released after 0, 10, 30, 60, 120, and 240 min. Slopes for 0.1, 0.2, and 0.5 ml of culture were 0.11, 0.20, and 0.47 nmol/min. Errors are standard deviations from three separate experiments.

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TABLE 3. Induction and repression of xyl and spac expression systems^a

The role of the CRE in catabolite repression of the xyl operon and its capacity for optimization through mutation has beenwell documented (13, 16, 18, 34). Furthermore, glucose-specific,XylR-mediated repression has also been reported (18). In Table3, we report about a 250-fold difference in reporter gene expression,comparing growth on minimal medium with xylose (2%) to growthon minimal medium plus glucose (0.2%). This result is consistentwith previous studies of the xyl regulon in which induction/repressionratios as high as 260-fold have been reported (13). We alsoexamined reporter gene expression after growth in minimal mediumwith xylose (0.2%) and one of three sugars (glucose, fructose,or glycerol) at a level of 0.2%. Regardless of the type of sugaradded, we observed about a 100-fold decrease in reporter geneexpression (data not shown). These findings are also consistentwith a previous study in which the CRE sequence used in our studies(G $right-arrow$ T and A $right-arrow$ T at positions 3 and 10, respectively) resulted insimilar levels of catabolite-mediated repression and masked toa large extent the glucose-specific effect seen with wild-typeCREs (18). Kim et al. (17) have described a xylose-inducibleintegration vector using xyl regulatory sequences from Bacillusmegaterium. Induction/repression ratios ranging from 150- to 200-foldwere reported for that system, which lacked the CRE sequence andwas not subject to catabolite repression. Eichenbaum et al. havealso published a comparison study of a plasmid-based B. subtilisxylose expression system with spac, lac, and nisA promoters (9).In that work, the xyl and spac systems demonstrated similar induction/repressionratios in B. subtilis (11- and 16-fold, respectively), thoughfew details were published regarding the construction of thatxylose-based expressionsystem.

Having determined the extremes of expression, we wanted to assess the ability of each system to modulate expression in responseto an inducer. Strains EB107 and EB103 were grown in various concentrationsof inducers (xylose and IPTG, respectively) in rich liquid media,and expression levels were assessed using the $beta$ -galactosidaseassay (Fig. 4). The xylose-induced expression system showed aparticular capacity for modulation, as $beta$ -galactosidase activityvaried from 30 units to about 11,000 units over an inducer concentrationrange of 3.5 log units (0.0002 to 0.63% xylose). In contrast,the spac system was modulated over an inducer concentration rangeof only 1.5 log units (0.003 to 0.1 mM IPTG).

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FIG. 4. Modulation of the xyl and spac expression systems. Saturated cultures of EB107 (pSWEET-bgaB) and EB103 (pSPAC-bgaB) were inoculated (1/100) into fresh LB-CHL media supplemented with increasing concentrations of inducer, i.e., 0.00002 to 6.3% xylose ( $open circle$ ) and 100 nM to 1 mM IPTG (

). Cultures were grown to mid-log phase and assayed for BgaB activity (see Materials and Methods). $beta$ -Galactosidase units are picomoles of o-nitrophenol released per minute per milliliter of culture at an OD₆₀₀ of 0.5. Errors are standard deviations from at least three separate experiments.

As a test case for the capacity of the xyl expression system to provide conditional complementation of essential functions,we attempted to complement a temperature-sensitive mutant (tag-12)previously attributed to B. subtilis tagD (23), which encodesglycerol-3-phosphate cytidylyltransferase. Again, for comparativepurposes, tagD was cloned into both pSWEET and pSPAC in orderto create EB123 and EB127, which expressed wild-type tagD in thetemperature-sensitive background under xyl and spac control, respectively.We assessed the ability of each system to complement the temperature-sensitivemutant at the nonpermissive temperature. As a control, we includedthe parental tag-12 temperature-sensitive strain (EB4) and theisogenic tag⁺ strain (EB6) in these experiments. As expected, EB6 grew wellat both the permissive (30°C) and nonpermissive (47°C) temperatures,while EB4 showed almost no growth at the nonpermissive temperature(Fig. 5a and b). Both EB123 and EB127 were able to complementthe mutant at the nonpermissive temperature in the presence oftheir respective inducers (Fig. 5c and d). In the absence of addedinducer, the spac expression system (EB127) showed substantialgrowth at the nonpermissive temperature, while the xyl system(EB123) showed only very slight growth relative to the controlEB4 (Fig. 5b). Interestingly, we have consistently noted thatin the absence of inducer and with a heavy inoculum, a mixed populationof large and small colonies is evident with strains EB123 andEB127 (e.g., Fig. 5b). These large colonies subsequently demonstratea temperature-insensitive and inducer-independent growth phenotypeand may have arisen from recombination of the temperature-sensitivecopy of tagD at the tag locus with the wild-type copy of tagDresident at amyE.

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FIG. 5. Xylose-dependent complementation of a temperature-sensitive mutant in teichoic acid biosynthesis. Strains were plated on LB agar in the presence or absence of an inducer and incubated at 30°C (permissive temperature) or 47°C (nonpermissive temperature). Strains EB4 (tag-12), EB6 (tag⁺), EB123 (tag-12 pSWEET-tagD), and EB127 (tag-12 pSPAC-tagD) were plated at 30°C (a), plated at 47°C (b), supplemented with 1 mM IPTG at 47°C (c), and supplemented with 2% xylose at 47°C (d). Strains shown in panels b through d were plated as indicated in panel a.

To further assess the ability of the xyl system to conditionally complement the tag-12 mutant, a growth curve was examinedusing strain EB123 (expression of tagD under xyl control in thetag-12 background) grown in the presence and absence of the inducerxylose (0.2%) (Fig. 6). Again, the parental strains EB4 and EB6were included as controls. The cultures were initially grown atthe permissive temperature (30°C) for 300 min and were then shiftedto the nonpermissive temperature (47°C) and monitored for up to25 h. The tag-12 mutant (EB4) showed a lytic phenotype upon temperatureshift, as indicated by the steady decrease in OD after 660 min.In the absence of xylose, strain EB123 duplicated the growth andlysis exhibited by EB4. In the presence of the inducer, EB123showed slightly better growth than EB6, likely due to the presenceof a rich carbon source (xylose). Nevertheless, we are certainthat this complementation was due to the expression of tagD andnot the presence of xylose, since, when grown at the nonpermissivetemperature and in the presence of xylose, EB4 showed only veryslight growth (Fig. 5d). We also tested EB127 (expression of tagDunder spac control in the tag-12 background) in an analogous experimentand found that the strain exhibited a growth curve which was indistinguishablefrom that seen for EB123 (data not shown).

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FIG. 6. Growth profile of the B. subtilis tag-12 mutant and conditional complementation with tagD under xylose control. Overnight cultures (LB) of EB4 (tag-12), EB6 (tag⁺), and EB123 (tag-12 pSWEET-tagD) were inoculated (1/100) into fresh medium (LB) and grown for 25 h, with periodic monitoring of growth by OD₆₀₀. Growth curves for EB4 and EB6 are represented by the symbols $open circle$ and

, respectively. EB123 was grown in the presence ( $black-down-triangle$ ) and absence ( $down-triangle$ ) of 0.2% xylose. Growth was at 30°C (permissive temperature for tag-12) until mid-log phase, when cultures were shifted to 47°C (restrictive temperature for tag-12) at 300 min (denoted by the arrow).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We have undertaken the development and characterization of a system for efficient expression in B. subtilis in order to characterizeputatively indispensable functions in teichoic acid biosynthesis.To that end, we have taken advantage of an extensive body of workon the xylose utilization operon of B. subtilis W23, which hasdescribed in detail the machinery for xylose induction and cataboliterepression in that system (5, 6, 12, 13, 16, 18,19). Accordingly, we chose to construct a xylose-based expressionsystem by incorporating components of the xylose operon from strainW23. The expression system contains the xylose repressor encodedby xylR, intergenic xyl operator sequences, the xylA promoter,and the 5' portion of xylA containing an optimized CRE. Thesecomponents are present on plasmid pSWEET, a derivative of pDG364(3), for integration into the B. subtilis chromosome at amyE.

We have made significant contributions to the improvement of xylose-based systems (9, 17) with the inclusion of xyl sequencesimportant in catabolite repression (CREs) and with an extensivecharacterization of the expression system constructed. The xylexpression system developed was effective in achieving very lowlevels of induction in the absence of an inducer, was capableof a wide range of induction levels, and had the capacity formodulated expression over a broad scale of inducer concentrations.We have carefully compared the performance of the xyl expressionsystem to that of the widely used spac system as a point of referenceand found it to be superior to spac in each of thesecharacteristics.

The tight control of expression afforded by the xyl expression system is an attractive feature in the study of null mutations,where strongly regulated expression of a complementing copy ofthe gene of interest can lead to an unambiguous interpretationof phenotype. Indeed, this expression system has particular utilityin the study of null mutations in essential genes. In the studiesdetailed here, the temperature-sensitive mutant tag-12 showedlittle or no growth at the restrictive temperature. Significantgrowth was seen, however, at the nonpermissive temperature forthe tag-12 mutant with spac-tagD at amyE in the absence of IPTG,whereas only very slight growth was evident with the xyl-tagDcomplementation system in the absence of xylose. Were this a tagDnull mutant, complementation experiments with the spac expressionsystem might incorrectly indicate that a phenotype of impairedgrowth, not lethality, is associated with a tagDknockout.

The particular capacity for modulation of gene expression with the xyl system is arguably a very attractive feature for thedeliberate expression of cloned genes in B. subtilis. While thespac system modulated expression over a narrow range of inducerconcentrations (1.5 log units), the xyl system controlled expressionover a >3.5-log span of xylose concentrations. When combined withthe large induction/repression ratio characteristic of the xylsystem, this broad response to inducer concentration should facilitateexploration of the effects of expression level of a cloned geneon phenotype. Indeed, protein expression levels can be importantto phenotypic analyses in bacteria for a wide variety of reasons,including an exquisite sensitivity, in some cases, to proteinstoichiometry, such as that observed for the E. coli proteinsFtsZ and FtsA (7, 8).

Despite the apparent superiority of the xyl promoter-operator system over that of spac, both systems showed considerable capacityfor control of expression in B. subtilis. Together, these twosystems may be particularly useful in instances where more thanone induction system may be warranted. Plasmid pMUTIN, for example,provides the means for facile inactivation of a target gene whileplacing downstream genes under the control of the spac promoterto test for polar effects (33). Complementation of the inactivatedgene by placing a copy under spac transcriptional control wouldnot provide the means to distinguish the effects of transcriptionof downstream genes from those of complementation. Use of pSWEETfor this purpose would facilitate an unequivocal analysis of anyphenotype(s) associated with the null mutant by placing the targetgene in trans under the control of the xylosepromoter.

The tag genes are responsible for the synthesis of poly(glycerol phosphate), the predominant cell wall-linked polyanionicpolymer of B. subtilis strain 168. A considerable body of workindicates an essential role in this strain for poly(glycerol phosphate)synthesis (2, 23, 24, 26, 27). Paradoxically, two otherwall polymers, poly(glucose N-acetylgalactosamine phosphate) andteichuronic acid, are also produced and are capable of at leastpartially substituting for the predominant polymer (10, 11).In fact, certain strains of B. subtilis have been reported tocompletely replace wall teichoic acid with phosphate-free teichuronicacid under phosphate-limiting conditions (20). Therefore, whileteichoic acid biosynthesis may have great potential as a therapeuticdrug target in gram-positive bacterial physiology, a clear understandingof the putatively essential role for this polymer, even in themodel organism B. subtilis 168, has remainedelusive.

An essential role for tagD, encoding glycerol-3-phosphate cytidylyltransferase (25), was indicated by the localization oftwo thermosensitive mutations, tag-11 and tag-12, to tagD (23).In addition, glycerol-3-phosphate cytidylyltransferase activityin extracts of the tag-11 mutant was shown to be thermolabileand significantly reduced relative to that of wild-type extracts(27). In the work reported here, we noted a pronounced growthdefect in the tag-12 mutant, such that this strain showed littleor no growth at the restrictive temperature and demonstrated asignificant drop in OD soon after a temperature shift from 30to 47°C. The decrease in cell density upon shifting to the nonpermissivetemperature is remarkable in its similarity to the lytic responsenormally reserved for defects in peptidoglycan biosynthesis andis consistent with previous studies detailing gross morphologicalchanges associated with teichoic acid mutants (1, 28). Usingthe xyl expression system developed here, we have demonstrated,for the first time, trans complementation of a teichoic acid biosynthesismutant. Rescue of the tag-12 mutant at the restrictive temperaturewith tagD under xyl control was xylose dependent, unequivocallyindicating a role for tagD in this growth defect. This work setsthe stage for further analysis of teichoic acid biosynthesis genesin B. subtilis through the construction of null mutants thereinand conditional complementation usingpSWEET.

	ACKNOWLEDGMENTS

We thank Dimitri Karamata for tag and tag-12 B. subtilis strains, Oliver Schrogel for pKL4, Petra Levin for pDR67, and ChristopherMurphy for fruitful discussions. We also thank Justin Nodwell,Gerry Wright, and Janet Wood for offering comments on themanuscript.

This work was supported by an operating grant and scholarship from the Medical Research Council of Canada to E.D.B. and bya postgraduate fellowship to A.P.B. from the Natural Sciencesand Engineering Research Council ofCanada.

	FOOTNOTES

^* Corresponding author. Mailing address: Antimicrobial Research Centre, Department of Biochemistry, McMaster University, 1200Main St. West, Hamilton, Ontario, Canada L8N 3Z5. Phone: (905)525-9140, ext. 22392. Fax: (905) 522-9033. E-mail: ebrown{at}fhs.mcmaster.ca.

Present address: Millennium Predictive Medicine, Inc., Cambridge, MA02139.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Boylan, R. J., N. H. Mendelson, D. Brooks, and F. E. Young. 1972. Regulation of the bacterial cell wall: analysis of a mutant of Bacillus subtilis defective in biosynthesis of teichoic acid. J. Bacteriol. 110:281-290[Abstract/Free Full Text].

2. Briehl, M., H. M. Pooley, and D. Karamata. 1989. Mutants of Bacillus subtilis 168 thermosensitive for growth and wall teichoic acid biosynthesis. J. Gen. Microbiol. 135:1325-1334.

3. Cutting, S. M., and P. B. V. Horn. 1990. Genetic analysis, p. 27-61. In C. R. Harwood, and S. M. Cutting (ed.), Molecular biological methods for Bacillus. John Wiley and Sons, Toronto, Canada.

4. Cutting, S. M., and P. Youngman. 1994. Gene transfer in gram-positive bacteria, p. 348-364. In P. Gerhardt, R. G. E. Murray, W. A. Wood, and N. R. Krieg (ed.), Methods for general and molecular bacteriology. American Society for Microbiology, Washington, D.C.

5. Dahl, M. K., J. Degenkolb, and W. Hillen. 1994. Transcription of the xyl operon is controlled in Bacillus subtilis by tandem overlapping operators spaced by four base-pairs. J. Mol. Biol. 243:413-424[CrossRef][Medline].

6. Dahl, M. K., D. Schmiedel, and W. Hillen. 1995. Glucose and glucose-6-phosphate interaction with Xyl repressor proteins from Bacillus spp. may contribute to regulation of xylose utilization. J. Bacteriol. 177:5467-5472[Abstract/Free Full Text].

7. Dai, K., and J. Lutkenhaus. 1992. The proper ratio of FtsZ to FtsA is required for cell division to occur in Escherichia coli. J. Bacteriol. 174:6145-6151[Abstract/Free Full Text].

8. Dewar, S. J., K. J. Begg, and W. D. Donachie. 1992. Inhibition of cell division initiation by an imbalance in the ratio of FtsA to FtsZ. J. Bacteriol. 174:6314-6316[Abstract/Free Full Text].

9. Eichenbaum, Z., M. J. Federle, D. Marra, W. M. de Vos, O. P. Kuipers, M. Kleerebezem, and J. R. Scott. 1998. Use of the lactococcal nisA promoter to regulate gene expression in gram-positive bacteria: comparison of induction level and promoter strength. Appl. Environ. Microbiol. 64:2763-2769[Abstract/Free Full Text].

10. Ellwood, D. C., and D. W. Tempest. 1972. Influence of culture pH on the content and composition of teichoic acids in the walls of Bacillus subtilis. J. Gen. Microbiol. 73:395-402[Abstract/Free Full Text].

11. Estrela, A. I., H. M. Pooley, H. de Lencastre, and D. Karamata. 1991. Genetic and biochemical characterization of Bacillus subtilis 168 mutants specifically blocked in the synthesis of the teichoic acid poly(3-O-beta-D-glucopyranosyl-N-acetylgalactosamine 1-phosphate): gneA, a new locus, is associated with UDP-N-acetylglucosamine 4-epimerase activity. J. Gen. Microbiol. 137:943-950[Abstract/Free Full Text].

12. Gärtner, D., J. Degenkolb, J. A. Ripperger, R. Allmansberger, and W. Hillen. 1992. Regulation of the Bacillus subtilis W23 xylose utilization operon: interaction of the Xyl repressor with the xyl operator and the inducer xylose. Mol. Gen. Genet. 232:415-422[Medline].

13. Gärtner, D., M. Geissendörfer, and W. Hillen. 1988. Expression of the Bacillus subtilis xyl operon is repressed at the level of transcription and is induced by xylose. J. Bacteriol. 170:3102-3109[Abstract/Free Full Text].

14. Heumann, D., C. Barras, A. Severin, M. P. Glauser, and A. Tomasz. 1994. Gram-positive cell walls stimulate synthesis of tumor necrosis factor alpha and interleukin-6 by human monocytes. Infect. Immun. 62:2715-2721[Abstract/Free Full Text].

15. Ireton, K., D. Z. Rudner, K. J. Siranosian, and A. D. Grossman. 1993. Integration of multiple developmental signals in Bacillus subtilis through the Spo0A transcription factor. Genes Dev. 7:283-294[Abstract/Free Full Text].

16. Jacob, S., R. Allmansberger, D. Gärtner, and W. Hillen. 1991. Catabolite repression of the operon for xylose utilization from Bacillus subtilis W23 is mediated at the level of transcription and depends on a cis site in the xylA reading frame. Mol. Gen. Genet. 229:189-196[CrossRef][Medline].

17. Kim, L., A. Mogk, and W. Schumann. 1996. A xylose-inducible Bacillus subtilis integration vector and its application. Gene 181:71-76[CrossRef][Medline].

18. Kraus, A., C. Hueck, D. Gärtner, and W. Hillen. 1994. Catabolite repression of the Bacillus subtilis xyl operon involves a cis element functional in the context of an unrelated sequence, and glucose exerts additional xylR-dependent repression. J. Bacteriol. 176:1738-1745[Abstract/Free Full Text].

19. Kreuzer, P., D. Gärtner, R. Allmansberger, and W. Hillen. 1989. Identification and sequence analysis of the Bacillus subtilis W23 xylR gene and xyl operator. J. Bacteriol. 171:3840-3845[Abstract/Free Full Text].

20. Lang, W. K., K. Glassey, and A. R. Archibald. 1982. Influence of phosphate supply on teichoic acid and teichuronic acid content of Bacillus subtilis cell walls. J. Bacteriol. 151:367-375[Abstract/Free Full Text].

21. Lazarevic, V., and D. Karamata. 1995. The tagGH operon of Bacillus subtilis 168 encodes a two-component ABC transporter involved in the metabolism of two wall teichoic acids. Mol. Microbiol. 16:345-355[Medline].

22. Matsuura, T., Y. Miyake, S. Nakashima, H. Komatsuzawa, Y. Akagawa, and H. Suginaka. 1996. Isolation and characterization of teichoic acid-like substance as an adhesin of Staphylococcus aureus to HeLa cells. Microbiol. Immunol. 40:247-254[Medline].

23. Mauel, C., M. Young, and D. Karamata. 1991. Genes concerned with synthesis of poly(glycerol phosphate), the essential teichoic acid in Bacillus subtilis strain 168, are organized in two divergent transcription units. J. Gen. Microbiol. 137:929-941[Medline].

24. Mauel, C., M. Young, P. Margot, and D. Karamata. 1989. The essential nature of teichoic acids in Bacillus subtilis as revealed by insertional mutagenesis. Mol. Gen. Genet. 215:388-394[CrossRef][Medline].

25. Park, Y. S., T. D. Sweitzer, J. E. Dixon, and C. Kent. 1993. Expression, purification, and characterization of CTP:glycerol-3-phosphate cytidylyltransferase from Bacillus subtilis. J. Biol. Chem. 268:16648-16654[Abstract/Free Full Text].

26. Pooley, H. M., F.-X. Abellan, and D. Karamata. 1992. CDP-glycerol:poly(glycerophosphate) glycerophosphotransferase, which is involved in the synthesis of the major wall teichoic acid in Bacillus subtilis 168, is encoded by tagF (rodC). J. Bacteriol. 174:646-649[Abstract/Free Full Text].

27. Pooley, H. M., F.-X. Abellan, and D. Karamata. 1991. A conditional-lethal mutant of Bacillus subtilis 168 with a thermosensitive glycerol-3-phosphate cytidylyltransferase, an enzyme specific for the synthesis of the major wall teichoic acid. J. Gen. Microbiol. 137:921-928[Abstract/Free Full Text].

28. Prayitno, N. R., and A. R. Archibald. 1997. The effects of growth conditions on cell wall composition and cell morphology in a temperature-sensitive tagB mutant of Bacillus subtilis. World J. Microbiol. Biotechnol. 13:207-217[CrossRef].

29. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

30. Schneider, O., U. Michel, G. Zysk, O. Dubuis, and R. Nau. 1999. Clinical outcome in pneumococcal meningitis correlates with CSF lipoteichoic acid concentrations. Neurology 53:1584-1587[Abstract/Free Full Text].

31. Schrogel, O., and R. Allmansberger. 1997. Optimisation of the BgaB reporter system: determination of transcriptional regulation of stress responsive genes in Bacillus subtilis. FEMS Microbiol. Lett. 153:237-243[Medline].

32. Shimotsu, H., and D. J. Henner. 1986. Construction of a single-copy integration vector and its use in analysis of regulation of the trp operon of Bacillus subtilis. Gene 43:85-94[CrossRef][Medline].

33. Vagner, V., E. Dervyn, and S. D. Ehrlich. 1998. A vector for systematic gene inactivation in Bacillus subtilis. Microbiology 144:3097-3104[Abstract/Free Full Text].

34. Weickert, M. J., and G. H. Chambliss. 1990. Site-directed mutagenesis of a catabolite repression operator sequence in Bacillus subtilis. Proc. Natl. Acad. Sci. USA 87:6238-6242[Abstract/Free Full Text].

35. Yansura, D. G., and D. J. Henner. 1984. Use of the Escherichia coli lac repressor and operator to control gene expression in Bacillus subtilis. Proc. Natl. Acad. Sci. USA 81:439-443[Abstract/Free Full Text].

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1.	Boylan, R. J., N. H. Mendelson, D. Brooks, and F. E. Young. 1972. Regulation of the bacterial cell wall: analysis of a mutant of Bacillus subtilis defective in biosynthesis of teichoic acid. J. Bacteriol. 110:281-290[Abstract/Free Full Text].
2.	Briehl, M., H. M. Pooley, and D. Karamata. 1989. Mutants of Bacillus subtilis 168 thermosensitive for growth and wall teichoic acid biosynthesis. J. Gen. Microbiol. 135:1325-1334.
3.	Cutting, S. M., and P. B. V. Horn. 1990. Genetic analysis, p. 27-61. In C. R. Harwood, and S. M. Cutting (ed.), Molecular biological methods for Bacillus. John Wiley and Sons, Toronto, Canada.
4.	Cutting, S. M., and P. Youngman. 1994. Gene transfer in gram-positive bacteria, p. 348-364. In P. Gerhardt, R. G. E. Murray, W. A. Wood, and N. R. Krieg (ed.), Methods for general and molecular bacteriology. American Society for Microbiology, Washington, D.C.
5.	Dahl, M. K., J. Degenkolb, and W. Hillen. 1994. Transcription of the xyl operon is controlled in Bacillus subtilis by tandem overlapping operators spaced by four base-pairs. J. Mol. Biol. 243:413-424[CrossRef][Medline].
6.	Dahl, M. K., D. Schmiedel, and W. Hillen. 1995. Glucose and glucose-6-phosphate interaction with Xyl repressor proteins from Bacillus spp. may contribute to regulation of xylose utilization. J. Bacteriol. 177:5467-5472[Abstract/Free Full Text].
7.	Dai, K., and J. Lutkenhaus. 1992. The proper ratio of FtsZ to FtsA is required for cell division to occur in Escherichia coli. J. Bacteriol. 174:6145-6151[Abstract/Free Full Text].
8.	Dewar, S. J., K. J. Begg, and W. D. Donachie. 1992. Inhibition of cell division initiation by an imbalance in the ratio of FtsA to FtsZ. J. Bacteriol. 174:6314-6316[Abstract/Free Full Text].
9.	Eichenbaum, Z., M. J. Federle, D. Marra, W. M. de Vos, O. P. Kuipers, M. Kleerebezem, and J. R. Scott. 1998. Use of the lactococcal nisA promoter to regulate gene expression in gram-positive bacteria: comparison of induction level and promoter strength. Appl. Environ. Microbiol. 64:2763-2769[Abstract/Free Full Text].
10.	Ellwood, D. C., and D. W. Tempest. 1972. Influence of culture pH on the content and composition of teichoic acids in the walls of Bacillus subtilis. J. Gen. Microbiol. 73:395-402[Abstract/Free Full Text].
11.	Estrela, A. I., H. M. Pooley, H. de Lencastre, and D. Karamata. 1991. Genetic and biochemical characterization of Bacillus subtilis 168 mutants specifically blocked in the synthesis of the teichoic acid poly(3-O-beta-D-glucopyranosyl-N-acetylgalactosamine 1-phosphate): gneA, a new locus, is associated with UDP-N-acetylglucosamine 4-epimerase activity. J. Gen. Microbiol. 137:943-950[Abstract/Free Full Text].
12.	Gärtner, D., J. Degenkolb, J. A. Ripperger, R. Allmansberger, and W. Hillen. 1992. Regulation of the Bacillus subtilis W23 xylose utilization operon: interaction of the Xyl repressor with the xyl operator and the inducer xylose. Mol. Gen. Genet. 232:415-422[Medline].
13.	Gärtner, D., M. Geissendörfer, and W. Hillen. 1988. Expression of the Bacillus subtilis xyl operon is repressed at the level of transcription and is induced by xylose. J. Bacteriol. 170:3102-3109[Abstract/Free Full Text].
14.	Heumann, D., C. Barras, A. Severin, M. P. Glauser, and A. Tomasz. 1994. Gram-positive cell walls stimulate synthesis of tumor necrosis factor alpha and interleukin-6 by human monocytes. Infect. Immun. 62:2715-2721[Abstract/Free Full Text].
15.	Ireton, K., D. Z. Rudner, K. J. Siranosian, and A. D. Grossman. 1993. Integration of multiple developmental signals in Bacillus subtilis through the Spo0A transcription factor. Genes Dev. 7:283-294[Abstract/Free Full Text].
16.	Jacob, S., R. Allmansberger, D. Gärtner, and W. Hillen. 1991. Catabolite repression of the operon for xylose utilization from Bacillus subtilis W23 is mediated at the level of transcription and depends on a cis site in the xylA reading frame. Mol. Gen. Genet. 229:189-196[CrossRef][Medline].
17.	Kim, L., A. Mogk, and W. Schumann. 1996. A xylose-inducible Bacillus subtilis integration vector and its application. Gene 181:71-76[CrossRef][Medline].
18.	Kraus, A., C. Hueck, D. Gärtner, and W. Hillen. 1994. Catabolite repression of the Bacillus subtilis xyl operon involves a cis element functional in the context of an unrelated sequence, and glucose exerts additional xylR-dependent repression. J. Bacteriol. 176:1738-1745[Abstract/Free Full Text].
19.	Kreuzer, P., D. Gärtner, R. Allmansberger, and W. Hillen. 1989. Identification and sequence analysis of the Bacillus subtilis W23 xylR gene and xyl operator. J. Bacteriol. 171:3840-3845[Abstract/Free Full Text].
20.	Lang, W. K., K. Glassey, and A. R. Archibald. 1982. Influence of phosphate supply on teichoic acid and teichuronic acid content of Bacillus subtilis cell walls. J. Bacteriol. 151:367-375[Abstract/Free Full Text].
21.	Lazarevic, V., and D. Karamata. 1995. The tagGH operon of Bacillus subtilis 168 encodes a two-component ABC transporter involved in the metabolism of two wall teichoic acids. Mol. Microbiol. 16:345-355[Medline].
22.	Matsuura, T., Y. Miyake, S. Nakashima, H. Komatsuzawa, Y. Akagawa, and H. Suginaka. 1996. Isolation and characterization of teichoic acid-like substance as an adhesin of Staphylococcus aureus to HeLa cells. Microbiol. Immunol. 40:247-254[Medline].
23.	Mauel, C., M. Young, and D. Karamata. 1991. Genes concerned with synthesis of poly(glycerol phosphate), the essential teichoic acid in Bacillus subtilis strain 168, are organized in two divergent transcription units. J. Gen. Microbiol. 137:929-941[Medline].
24.	Mauel, C., M. Young, P. Margot, and D. Karamata. 1989. The essential nature of teichoic acids in Bacillus subtilis as revealed by insertional mutagenesis. Mol. Gen. Genet. 215:388-394[CrossRef][Medline].
25.	Park, Y. S., T. D. Sweitzer, J. E. Dixon, and C. Kent. 1993. Expression, purification, and characterization of CTP:glycerol-3-phosphate cytidylyltransferase from Bacillus subtilis. J. Biol. Chem. 268:16648-16654[Abstract/Free Full Text].
26.	Pooley, H. M., F.-X. Abellan, and D. Karamata. 1992. CDP-glycerol:poly(glycerophosphate) glycerophosphotransferase, which is involved in the synthesis of the major wall teichoic acid in Bacillus subtilis 168, is encoded by tagF (rodC). J. Bacteriol. 174:646-649[Abstract/Free Full Text].
27.	Pooley, H. M., F.-X. Abellan, and D. Karamata. 1991. A conditional-lethal mutant of Bacillus subtilis 168 with a thermosensitive glycerol-3-phosphate cytidylyltransferase, an enzyme specific for the synthesis of the major wall teichoic acid. J. Gen. Microbiol. 137:921-928[Abstract/Free Full Text].
28.	Prayitno, N. R., and A. R. Archibald. 1997. The effects of growth conditions on cell wall composition and cell morphology in a temperature-sensitive tagB mutant of Bacillus subtilis. World J. Microbiol. Biotechnol. 13:207-217[CrossRef].
29.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
30.	Schneider, O., U. Michel, G. Zysk, O. Dubuis, and R. Nau. 1999. Clinical outcome in pneumococcal meningitis correlates with CSF lipoteichoic acid concentrations. Neurology 53:1584-1587[Abstract/Free Full Text].
31.	Schrogel, O., and R. Allmansberger. 1997. Optimisation of the BgaB reporter system: determination of transcriptional regulation of stress responsive genes in Bacillus subtilis. FEMS Microbiol. Lett. 153:237-243[Medline].
32.	Shimotsu, H., and D. J. Henner. 1986. Construction of a single-copy integration vector and its use in analysis of regulation of the trp operon of Bacillus subtilis. Gene 43:85-94[CrossRef][Medline].
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