Identification of an Actinobacillus pleuropneumoniae Consensus Promoter Structure

doi:10.1128/JB.183.6.1983-1989.2001

This Article

	Abstract
	Full Text (PDF)
	A correction has been published
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Doree, S. M.
	Articles by Mulks, M. H.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Doree, S. M.
	Articles by Mulks, M. H.

Previous Article | Next Article

Journal of Bacteriology, March 2001, p. 1983-1989, Vol. 183, No. 6
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.6.1983-1989.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Identification of an Actinobacillus pleuropneumoniae Consensus Promoter Structure

Scott M. Doree and Martha H. Mulks^*

Department of Microbiology, Michigan State University, East Lansing, Michigan 48824-1101

Received 15 November 2000/Accepted 20 December 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Actinobacillus pleuropneumoniae promoter-containing clones were isolated from a genomic DNA library constructed in our lVETpromoter trap vector pTF86. The promoter-containing clones wereidentified by their ability to drive expression of the promoterlessluxAB genes of Vibrio harveyi. The degree of expression was quantifiable,and only high-expression or "hot" promoters were used for thisstudy. Nine clones were sequenced, and their transcriptional startsites were determined by primer extension. The sequences upstreamof the start site were aligned, and a consensus promoter structurefor A. pleuropneumoniae was identified. The consensus promotersequence for A. pleuropneumoniae was found to be TATAAT and TTG/AAA,centered approximately 10 and 35 bp upstream of the transcriptionalstart site, respectively. A comparison of the A. pleuropneumoniaeconsensus with other prokaryotic consensus promoters showed thatthe A. pleuropneumoniae consensus promoter is similar to thatfound in other eubacteria in terms of sequence, with an identical $-$ 10 element and a similar but truncated $-$ 35 element. However,the A. pleuropneumoniae consensus promoter is unique in the spacingbetween the $-$ 10 and $-$ 35 elements. The promoter spacing was analyzedby site-directed mutagenesis, which demonstrated that optimalspacing for an A. pleuropneumoniae promoter is shorter than thespacing identified for Escherichia coli and Bacillus subtilispromoters.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Actinobacillus pleuropneumoniae is the causative agent of an acute necrotizing hemorrhagic pleuropneumonia in swine (13,19, 22). Unfortunately, there is not an abundance of knowledgeabout what gene products play an important role in A. pleuropneumoniaedisease. Our laboratory has developed an in vivo expression technology(IVET) system to identify gene products that have a role in thepathogenesis of swine pleuropneumonia (6). This IVET systemhas been used to identify gene promoters that are specificallyinduced duringinfection.

This IVET approach is based on the complementation of a defined attenuated riboflavin-requiring auxotroph (Rib) by a promoter trap vector that contains promoterless copiesof the genes necessary to complement the genetic lesion in riboflavinsynthesis. If the fragment of A. pleuropneumoniae genomic DNAligated into the vector contains a functional promoter, the ribgenes are expressed and the auxotroph is able to survive and causedisease in experimentally infected pigs. The goal of our IVETstudies is to recover clones from infected pigs, to characterizethe promoters that are selected, and to determine what gene(s)lies downstream of each promoter to identify its role in A. pleuropneumoniaepathogenesis. A part of this work is to characterize these invivo-expressed promoters and compare their structure to that ofhousekeeping gene promoters. However, the housekeeping or sigma-70promoter structure in A. pleuropneumoniae isunknown.

The sigma-70 promoters in Escherichia coli are characterized by two nucleotide sequences that are centered at positions $-$ 35and $-$ 10 relative to the transcriptional start site. The acceptedconsensus sequences are TTGACA and TATAAT for the $-$ 35 and $-$ 10regions, respectively. These sequences are separated by 17 ± 1nucleotides (10, 11, 16). There is a similar structure forother well-studied organisms such as Bacillus subtilis (12),but the research on promoter structures in pathogens such as A.pleuropneumoniae islimited.

Only a few attempts have been made to identify promoter elements in A. pleuropneumoniae, and none of the sigma factors havebeen identified or characterized (5, 9, 14). The resultsfrom these experiments show no clear similarity to E. coli promotersor to promoters from other eubacteria. This raises the questionas to the structure of a sigma-70-like promoter in A. pleuropneumoniaeand how it compares with other eubacterial promoters. Since severalgenes encoding antibiotic resistance markers that are readilyexpressed in E. coli are not expressed in A. pleuropneumoniae(25), it is likely that the A. pleuropneumoniae consensus promoterdoes differ in some way from that found in E. coli.

The goal of this study was to identify and characterize promoter sequences active in A. pleuropneumoniae under standard laboratorygrowth conditions. We identified DNA fragments with promoter activityby their ability to express promoterless lux genes and identifiedtheir transcriptional start sites by primer extension analysis.We have compared the DNA sequences of these active promoters andpropose a consensus promoter sequence for A. pleuropneumoniae.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains, media, and growth conditions. The A. pleuropneumoniae strains used in this study were AP100, a virulent serotype 1 strain (ATCC 27088), and AP233, a riboflavin-requiringderivative of AP100 (7). A. pleuropneumoniae strains were culturedat 35°C in a waterbath with shaking at 150 rpm in brain heartinfusion (BHI; Difco Laboratories, Detroit, Mich.) containingNAD (10 µg/ml; Sigma Chemical Company, St. Louis, Mo.). Riboflavin(Sigma) was added to a final concentration of 200 µg/ml when necessary.E. coli XL1-blue MRF (Stratagene, La Jolla, Calif.), used forplasmid construction and analysis, was cultured in Luria-Bertani(LB) medium. Ampicillin was added to 100 µg/ml for plasmid selectionin E. coli and to 50 µg/ml for selection in A. pleuropneumoniae.

Promoter trap vector pTF86. The promoter trap vector pTF86 was developed as an IVET vector (6). The vector contains a T4 terminator, a unique BamHIcloning site, promoterless luciferase genes (luxAB) genes fromVibrio harveyi, and promoterless riboflavin genes (ribBAH) fromB. subtilis in shuttle vector pGZRS19 (25). This plasmid iscapable of replicating in both A. pleuropneumoniae and E. coli.The copy number of pTF86 was shown to be 8 to 10 copies per cellin A. pleuropneumoniae (6). We have not measured the copy numberof pTF86 in E. coli, but qualitative analysis indicates that thecopy number is substantially higher than in A. pleuropneumoniae.

Construction of an A. pleuropneumoniae promoter library. Chromosomal DNA of AP100 was prepared and partially digested with Sau3A. Fragments ranging from 0.4 to 1.0 kb in size werepurified from an agarose gel and ligated into the alkaline phosphatase-treatedBamHI site of pTF86 (6). The ligation mixture was electroporatedinto AP233 as previously described (6). Single colonies wereselected and subcultured onto BHI plates containing riboflavin(200 µg/ml), ampicillin (50 µg/ml), and NAD (10 µg/ml).

Screening of the promoter library. Qualitative screening of transformants for expression of the luxAB genes in vitro was performed on a Hamamatsu C1966 photonicmicroscope system. Colonies on agar plates were exposed to 50µl of N-decyl aldehyde (Sigma) distributed evenly on a glass petridish lid. The plate was then analyzed using the standard settingsfor high Lux expression colonies. The camera aperture was setat 11, the intensity setting on the keyboard was set at 8, thebit select was set at 0 to 3, and the offset was set at +1. Coloniesthat exhibited a high degree of Lux expression compared with knownstandard A. pleuropneumoniae Lux expression controls were selectedfor furtheranalysis.

Quantitative analysis of Lux expression was performed using a Turner model 20e luminometer. The substrate, N-decyl aldehyde,was made by dissolving 20 mg of Essentially Fatty Acid Free BSA(Sigma) per ml in 1 ml of H₂O with 10 µl of N-decyl aldehyde perml. The substrate mixture was sonicated in a waterbath at roomtemperature for 20 min. To analyze each clone, 20 µl of a mid-log-phaseculture was added to 20 µl of substrate in a polypropylene luminometercuvette (Turner Designs, Sunnyvale, Calif.) and mixed for 10 s.The mixture was then analyzed with the following settings: fullintegral, autoranging mode with a predelay of 0 s, delay of 10s, and integration time of 30 s. Luminometer readings were normalizedto relative light units per optical density unit at 520 nm (RLU/OD₅₂₀).

RNA isolation. RNA isolation was performed as described by Xiong et al. (27) with modifications. Briefly, A. pleuropneumoniae cells containingthe hot promoter plasmids were grown in 5 ml of BHI medium supplementedwith NAD, riboflavin, and ampicillin as described above. The cellswere grown to an optical density at 520 nm of 0.8 at 37°C. Then1.5 ml of the culture was transferred to a cold microcentrifugetube, and 2 µl of chloramphenicol (20 mg/ml) was added. Cellswere pelleted by centrifugation for 30 s at 13,000 × g. The cellpellet was resuspended in 200 µl of STET buffer (18). and 200µl of phenol-chloroform by vortexing for 30 s. Samples were placedat 100°C for 1 min. All of the subsequent steps were performedin a cold room at 4°C. The samples were centrifuged for 3 minat 13,000 × g. The aqueous phase was removed, extracted with anequal volume of chloroform, and centrifuged again for 3 min at13,000 × g. The aqueous phase was precipitated by adding 100 µlof 7.5 M ammonium acetate and 600 µl of 100% ethanol. After incubationat $-$ 80°C for 15 min, RNA was pelleted by centrifugation for 10min at 13,000 × g. The pellet was washed with absolute ethanol,resuspended in 20 µl of diethyl pyrocarbonate (DEPC)-treated H₂Owith RNase inhibitor (Promega, Madison, Wis.), and stored at $-$ 80°Cuntil reverse transcription reactions wereperformed.

RNA isolation from AP233 was also performed to isolate total cellular RNA from an isolate not containing a plasmid. AP233was cultured in 20 ml of BHI supplemented with NAD and allowedto grow to an optical density of 0.8 at 520 nm. The cells weretransferred to a cold centrifuge tube, and 20 µl of chloramphenicol(20 mg/ml) was added. Cells were pelleted by centrifugation for2 min at 6,000 × g. The cell pellet was resuspended in 2.5 mlof STET buffer by vortexing, and 2.5 ml of phenol-chloroform wasadded. The sample was placed at 100°C for 1 min and then centrifugedfor 5 min at 10,000 × g at 4°C. The aqueous phase was removed,extracted with an equal volume of chloroform, and centrifugedagain for 5 min at 10,000 × g. The aqueous phase was precipitatedby adding 1.25 ml of 7.5 M ammonium acetate and 7.5 ml of 100%ethanol. After incubation at $-$ 80°C for 30 min, the RNA was pelletedby centrifugation for 20 min at 10,000 × g. The pellet was washedwith absolute ethanol, resuspended in 100 µl of DEPC-treated H₂Owith RNase inhibitor, and stored at $-$ 80°C.

Primer extension. Primer extension analysis was performed using RNA isolated as above that was not more than 1 day old. The primers were 5'-endlabeled using [ $gamma$ -³²P]ATP and T4 polynucleotide kinase (Gibco-BRL, Rockville, Md.)(20) and purified using Centri-step spin columns (Boehringer-Mannheim).Following end labeling and purification, 1 to 2 µl of labeledprimer was incubated with 10 µl of RNA at 85°C for denaturation.The mixture was centrifuged for 10 s at 13,000 × g and allowedto cool to room temperature for 1 h to allow the primer to annealto the mRNA. Then 4 µl of avian myeloblastosis virus (AMV) reversetranscriptase buffer, 2 µl of DEPC-treated H₂O, 1 µl of 1.25 mMdeoxynucleoside triphosphate mix, and 1 µl of AMV reverse transcriptase(Boehringer Mannheim Biochemicals, Indianapolis, Ind.) were added,and the mixture was incubated for 1 h at 42°C. The reaction wasstopped by adding 4 µl of STOP solution, provided in Sequenase2.0 kits (U.S. Biochemical, Cleveland,Ohio).

DNA sequencing. For sequencing the promoter fragments, 5 ml of E. coli XL1-Blue MRF containing the appropriate promoter fragment plasmid wasgrown for 16 h in LB medium supplemented with ampicillin (100µg/ml). Plasmid DNA was prepared using Qiagen spin columns (QiagenInc., Chatsworth, Calif.) and eluted in 100 µl of water. Plasmidswere sequenced with the same primer that was used for reversetranscription by the dideoxy chain termination method using theSequenase 2.0 kit (U.S. Biochemical) and [³⁵S]dATP (Amersham Corp, Arlington Heights, Ill.). The productsof the sequencing reactions and the reverse transcription reactionwere separated on an 8.0% polyacrylamide gel containing 8 M ureato analyze the mRNA 5' ends of each promoter fragment clone. Thegels were exposed to film for 24 h, and the mRNA 5' ends weredetermined.

DNA and protein sequence analysis. Nucleotide and amino acid sequences were compared with sequences in the GenBank and EMBL databases using the FASTA and BLASTprograms (1). Alignments of the promoter regions were donewith MultiAlin version 5.4.1 (3) and the Genetics ComputerGroup (GCG) suite of programs (8).

Construction of promoter deletion mutant. A deletion mutant (SD2 $Delta$ P) was constructed from clone SD2 using a PCR strategy that utilized long-range PCR with primers thatcontained internal NotI sites. Two primers were designed to primeaway from the promoter region. A long-range PCR kit (BoehringerMannheim) was used to amplify the entire plasmid from the specificprimers. The products were then digested with NotI (Boehringer-Mannheim)and ligated overnight at 4°C using T4 DNA ligase (Boehringer-Mannheim).The ligation mixture was electroporated into AP233, and individualtransformants were screened for Lux expression as described above.SD2 $Delta$ P was sequenced as describedabove.

Construction of a functional promoter in the deletion mutant SD2 $Delta$ P. Two primers were designed to reconstruct the promoter region in SD2 $Delta$ P. The primers were used to amplify the promoter regionfrom SD2 by PCR. The primers contained internal NotI sites, andfollowing digestion with NotI for 90 min at 37°C, the promoterfragment was ligated into NotI-digested SD2 $Delta$ P. The ligation mixturewas electroporated into AP233, and the transformants (SD2 $Delta$ PR)were screened for Lux expression. SD2 $Delta$ PR was sequenced as describedabove.

Construction of promoter clones from two characterized E. coli promoters. Two pairs of oligonucleotide primers were designed to clone the bla promoter from pUC18 and the promoter from the str operonfrom the E. coli genome. The str promoter has a high degree ofsimilarity with the E. coli consensus promoter sequence (16).These two promoters were amplified by PCR and cloned into theBamHI site inpTF86.

In vitro site-directed mutagenesis of asd promoter clone. Four pairs of oligonucleotide primers were designed that encode four specific mutations in the spacer region of the asd promoterclone. Each primer pair primes in opposite directions away fromthe promoter region on opposite strands of the plasmid. The primerpairs allow amplification of the entire asd plasmid and incorporationof the desired mutations in the spacer region. The primers wereused in a system modified from the QuikChange site-directed mutagenesismethod (Stratagene). The asd promoter plasmid was purified fromE. coli XL1-Blue MRF and used as the template in four PCRs. ThePCR cycling conditions were an initial denaturation at 95°C for30 s, followed by 15 cycles of 95°C for 30 s, 55°C for 1 min,and 68°C for 18 min. The reactions were then cooled to 37°C, and10 U of DpnI was added to each reaction to digest the methylatedtemplate asd plasmid. Following digestion with DpnI, a portionof each reaction was used to transform competent E. coli XL1-BlueMRF. The transformants were screened and sequenced to confirmthe presence of the desired mutation in the spacerregion.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction and screening of an A. pleuropneumoniae promoter library. The promoter trap vector used in this study was developed as an IVET vector (6). This vector, designated pTF86, containsa T4 terminator, a unique BamHI cloning site, promoterless V.harveyi luxAB genes, and promoterless ribBAH genes from B. subtilisin a shuttle vector, pGZRS19 (25), capable of replicating inboth A. pleuropneumoniae and E. coli. When a DNA fragment withan active A. pleuropneumoniae promoter is inserted in the appropriateorientation into the BamHI cloning site, the luxAB genes and theribBAH genes are expressed. This restores to AP233, a riboflavin-requiringderivative of virulent A. pleuropneumoniae serotype 1 (ATCC 27088),the ability to grow in the absence of riboflavin, but more importantlyfor this study, these clones have Lux activity. A library of potentialpromoter clones was constructed in pTF86 and transformed intoAP233, and clones were screened qualitatively for Lux activityby photonic camera (Fig. 1). Clones with a high degree of Luxexpression, such as the asd and TF7 clones shown in Fig. 1, werechosen for further study. Inserts from each of these hot promoterclones were sequenced, using a primer complementary to the 5'end of the luxA coding region as well as additional internal primersas needed. The nucleotide and predicted amino acid sequences ofthese inserts were used to search the GenBank and EMBL databases,and putative identification of the genes encoded was made basedon homology data (Fig. 2).

View larger version (52K):
[in this window]
[in a new window]

FIG. 1. Qualitative screen of an A. pleuropneumoniae promoter library. (A) Photograph of duplicate colonies on an agarose plate. (B) Photograph of luminescence using a photonic camera. The asd clone and the TF7 clone have a high degree of lux expression. The iviA clone, which was recovered from an IVET experiment, is an example of a clone with low lux expression (6). The vector pTF86, containing no insert, is also shown.

View larger version (28K):
[in this window]
[in a new window]

FIG. 2. Alignment of 12 promoter regions from A. pleuropneumoniae. The promoter regions marked with an asterisk were identified in previous studies. The $-$ 10 and $-$ 35 regions are shown in bold, and the consensus sequence is shown at the bottom. The experimentally found transcriptional start sites are underlined and capitalized. Dashes indicate gaps to align the promoter regions. The distance between each transcriptional start site and the start codon and the sequence of the RBS for each of the clones is shown. The relative strength of each promoter clone is given as Lux activity in RLU/OD₅₂₀. These measurements were performed on three different days and are averages of 15 measurements. The standard deviation was calculated, and the error for each measurement is given. The database homology is given for the promoter clones. The homologies are all based on comparison with H. influenzae. Clone SD7 is homologous to HI0017, which is a hypothetical open reading frame in H. influenzae. Clone SD2 is homologous to lcfA, a long-chain fatty acid coenzyme A ligase; TF8 is homologous to kdtA, a 2-keto-3-deoxyoctolosonic acid transferase involved in lipopolysaccharide biosynthesis; SD20 is homologous to top3, a DNA topoisomerase; SD9 is homologous to xerB, an aminopeptidase; and TF7 is homologous to dnaB, a DNA helicase. The percent identity and the amino acid (aa) overlap are also given. Clone SD10 has a short open reading frame (18 codons), and no homologous protein was found. N/A, data not available; ND, not done. GenBank accession numbers: SD2, AF275726; SD7, AF275727; SD9, AF275728; SD10, AF275729; SD20, AF275730; TF7, AF275731; and TF8, AF275732.

Quantitative Lux assays were performed to determine the relative strength of each promoter (Fig. 2). The weakest promoterselected for this study was that in clone TF7, with a relativestrength of 592 RLU/OD₅₂₀; this promoter controls expression ofa protein that is similar to DNA helicase from Haemophilus influenzae.In contrast, in vivo induced (ivi) promoters were defined as having<200 RLU/OD₅₂₀ in vitro (6).

Identification of mRNA 5' ends or putative transcriptional start sites. To identify the approximate distance of each mRNA 5' end from the luxAB genes, a primer was designed that is complementaryto the 5' end of the luxA gene. A reverse transcription reactionwas performed on all of the promoter clones using this primer.The products were run next to a [ $gamma$ -³²P]ATP-labeled 100-bp ladder on an 8.0% polyacrylamide gel. Thisstep allowed us to design primers that were close enough to eachtranscriptional start site to obtain results with single-base-pairaccuracy. Following sequence analysis of each clone, primers weredesigned complementary to the coding strand for each clone andwithin 100 bp of the mRNA 5' end. Primer extension experimentswere completed, and the cDNA product from each of the reversetranscription reactions was run next to a sequencing ladder thatused the same primer as the reverse transcription reaction. Figure2 shows the DNA sequences of the regions upstream from the putativetranscriptional start sites found in primer extension experiments.Examples of the autoradiographs of the primer extension gels areshown in Fig. 4 and 5.

Identification of a consensus promoter sequence. In Fig. 2, the promoters from the nine promoter clones analyzed in this study are aligned with three promoters identifiedin previous research (5, 9, 15). The alignment was performedby using MultiAlin version 5.4.1 and the GCG suite of programs(3, 8). The consensus sequence determined from this alignmentconsists of nucleotides that occur in more than 50% of the clonesat any position. The two regions identified in Fig. 2 are the $-$ 10 and $-$ 35 regions. The $-$ 10 region is positioned 5 to 12 bp upstreamof the transcription start site. The consensus sequence of thisregion is TATAAT. The spacing between the $-$ 10 and $-$ 35 region rangedbetween 13 and 16 bp. The consensus sequence of the $-$ 35 regionwas TTRAA, where R can be either G or A. The A. pleuropneumoniaeconsensus promoter sequence was compared with consensus housekeepingpromoters for E. coli (11), B. subtilis (12), Streptomycessp. (21), Campylobacter jejuni (26), Corynebacterium glutamicum(20), Caulobacter crescentus (17), and Mycobacterium paratuberculosis(2) (Table 1).

View this table:
[in this window]
[in a new window]

TABLE 1. Comparison of A. pleuropneumoniae consensus promoter sequence with other prokaryotic promoters^a

Analysis of RBS and transcriptional start site of A. pleuropneumoniae promoters. The initiating nucleotide in 11 of the 12 promoter clones was predicted to be A or T. The ribosome-binding site (RBS) foreach of the promoter clones is identified in Fig. 2. Using 16SrRNA sequences the predicted RBS for A. pleuropneumoniae is AGGAGG(4). The promoter clones identified in this study have a consensusRBS ofAGGAGG.

Construction of promoter deletion clone to verify loss of promoter function. A promoter mutant was constructed to verify that the deletion of a putative promoter would cause loss of Lux expression andthe lack of a cDNA product in a reverse transcription experiment.Clone SD2 was chosen because it has relatively high Lux expressionand there were convenient sites to design primers inside the promoterfragment. The primers that were designed are shown schematicallyin Fig. 3. The primers were designed to delete a 114-bp fragmentthat included the putative transcriptional start site, the $-$ 10region, the $-$ 35 region, and some upstream and downstream sequence.The deletion does not remove the binding site for the primer usedin the primer extension mapping experiments. Long-range PCR wasperformed, and 20 transformants (SD2 $Delta$ P1 to SD2 $Delta$ P20) were chosenfor further analysis. Of the 20 transformants that were chosenfor Lux screening, all had no Lux expression when visualized withthe photonic camera. A photonic camera image of AP233 clones containingthe deleted promoter and the wild-type promoter is shown in Fig.3 as well as the quantitative Lux expression data. One of theSD2 $Delta$ P clones was sequenced to confirm that the promoter regionwas indeed deleted and the remainder of the genomic DNA fragmentwas still intact. Primer extension analysis of SD2 (lane 1) aswell as SD2 $Delta$ P (lane 2) is shown in Fig. 4. The sequencing ladderwas prepared from the same primer that was used for the reversetranscription of both SD2 and SD2 $Delta$ P. The loss of the cDNA productin lane 2 is further evidence that the region deleted containedthe sequences necessary for the initiation of transcription inA. pleuropneumoniae.

View larger version (12K):
[in this window]
[in a new window]

FIG. 3. Construction of a promoter deletion mutant from clone SD2. Map of the insert structure of the wild-type SD2 clone and SD2 $Delta$ P. The $-$ 35 and $-$ 10 regions are noted as well as the transcriptional start site (Tx). Sequence analysis of the mutant showed that a total of 114 bp had been deleted, ranging from 82 bp upstream of the transcriptional start site to 32 bp downstream of the start site. The deletion did not delete the primer-binding site for the reverse transcription primer (MM116). (A) Photograph of the colony growth of each clone. (B) Photonic camera image.

View larger version (63K):
[in this window]
[in a new window]

FIG. 4. Primer extension analysis of clones SD2 (lane 1) and SD2 $Delta$ P (lane 2). The sequencing reactions and the reverse transcription reactions were performed with an identical primer. Lane 1 contains the reverse transcription reaction from the SD2 clone, which contains a wild-type promoter. Lane 2 is the reverse transcription reaction from the SD2 $Delta$ P clone that contains the promoter deletion. The start site is highlighted with an arrow, and the $-$ 10 and $-$ 35 regions are bracketed.

The wild-type promoter fragment from SD2 was cloned back into SD2 $Delta$ P to confirm that the deletion was responsible for the lossof Lux expression. The resulting transformants (SD2 $Delta$ PR) had thesame degree of Lux expression as the wild-type SD2 (1,216 RLU/OD₅₂₀).Sequence analysis showed only 3 bp difference between SD2 andSD2 $Delta$ PR; these were outside the promoter region and were a resultof the cloningstrategy.

Comparison of transcriptional start site identified from plasmid mRNA and from AP233 containing the endogenous copy of asd gene. We compared the mRNA 5' ends that were identified from AP233 containing no plasmids and AP233 containing the asd plasmid.This was done to verify that the transcriptional start sites mappedfrom the plasmid clones were identical to the start sites mappedfrom A. pleuropneumoniae containing only the endogenous copy ofthe gene. The results of the primer extension experiments areshown in Fig. 5. Lane 1 shows the putative transcriptional startsite mapped from total cellular RNA isolated from AP233 containingno plasmids, and lane 2 shows the putative transcriptional startsite identified from the asd promoter clone. The same primer wasused in each reaction, and each putative transcriptional startsite maps to the same position.

View larger version (78K):
[in this window]
[in a new window]

FIG. 5. Comparison of transcriptional start sites mapped from mRNA isolated from AP233 (lane 1) and the asd clone (lane 2). The same primer was used for reverse transcription reactions and sequencing reactions. The reaction in lane 2 was done with 15 µg of total RNA isolated from AP233, and the reaction in lane 1 was completed with 1.5 µg of total RNA isolated from the asd clone. The start site is highlighted with an arrow, and the $-$ 10 and $-$ 35 regions are bracketed.

Quantitative expression of E. coli promoters in E. coli and A. pleuropneumoniae. Two E. coli promoters were cloned in pTF86, and their expression was analyzed by quantitative Lux assays (Table 2). ClonepSDbla contains the $beta$ -lactamase promoter from pUC18, and clonepSDstr contains an E. coli promoter from the str operon that isvery similar to the E. coli consensus promoter. Both promotershave a spacing of 17 bp, and the sequences of their $-$ 10 and $-$ 35elements are shown in Table 2. Both promoters were strongly expressedin E. coli, as predicted, but were only weakly expressed in A.pleuropneumoniae.

View this table:
[in this window]
[in a new window]

TABLE 2. Expression of the asd promoter clone, asd promoter mutants, and E. coli promoters in E. coli and A. pleuropneumoniae^a

In vitro site-directed mutagenesis of asd promoter clone to assess expression differences based on spacer length. Site-directed mutagenesis was performed on the asd promoter clone to alter the spacer length of the clone. Four mutants wereconstructed by inserting or deleting adenosine nucleotides withspacing between the $-$ 10 and $-$ 35 elements ranging from 14 to 18bp. The sequences of each of the promoter mutants as well as thewild-type asd promoter clone and Lux expression for each of theclones in E. coli and A. pleuropneumoniae are shown in Table 2.Note that a spacing of 18 bp in the A. pleuropneumoniae asd promotershould be equivalent to a spacing of 17 bp in an E. coli promoter,due to the different lengths of the $-$ 35 element in these species.In E. coli, expression increased with increased spacing, and thestrongest expression was found in the asd18 promoter. In contrast,in A. pleuropneumoniae expression was strongest at a spacing of16 bp, with high expression at shorter spacings but no significantexpression in the asd18promoter.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this study we identified nine strongly expressed or hot promoters from A. pleuropneumoniae using a promoter trap vector,pTF86. This vector, which encodes the luxAB genes from V. harveyi,allows quantification of Lux expression and therefore the relativestrength of the promoter driving the expression. The nine promoterclones were analyzed by primer extension to determine their transcriptionalstart sites with single-base-pair accuracy. The sequences upstreamof the transcriptional start sites were aligned along with threepreviously identified promoters to determine a consensus promotersequence for A. pleuropneumoniae.

The consensus sequence for the $-$ 10 region is TATAAT, which is identical to that of E. coli and B. subtilis. The $-$ 35 regionwas aligned, and the consensus sequence is TTRAA. The $-$ 35 consensusis identical in the first, second, and fourth positions to thesequences of E. coli and B. subtilis. The spacing between the $-$ 10 region and the transcriptional start site ranges from 5 to10 bp, with an average of 7 bp of separation, which is similarto promoters in other eubacteria. The spacing between the $-$ 10and $-$ 35 sequences in A. pleuropneumoniae ranges between 13 and16 bp. This spacing is shorter than that of the promoters foundin most othereubacteria.

This difference in spacer length was analyzed by constructing mutants of the asd promoter clone to assess the effects of bothinserting and deleting nucleotides in the spacer region. The optimumspacing for the asd promoter in A. pleuropneumoniae was foundto be 16 bp, but a high degree of expression was also seen withspacings of 14 and 15 bp (Table 2). However, a significant lossof Lux expression was seen in the clones with spacer lengths of17 and 18 bp. In comparison, the E. coli clones had their highestLux expression at 17 and 18 bp of spacing between the $-$ 10 and $-$ 35 elements. In addition, both the E. coli str promoter and thebla promoter from pUC18 were strongly expressed in E. coli butonly weakly expressed in A. pleuropneumoniae. It is clear thatthere is a difference in the consensus promoter structure betweenE. coli and A. pleuropneumoniae and that A. pleuropneumoniae promotershave a shorter spacing in the region between the $-$ 10 and $-$ 35 elementsthan do those of E. coli.

No sigma factors have been characterized to date in A. pleuropneumoniae. However, it is likely that multiple sigma factorscontrol A. pleuropneumoniae gene expression under different environmentalconditions, as in other eubacteria. The promoter clones in thisstudy were chosen for three reasons. First, each has a high degreeof lux expression when grown on standard laboratory media. Second,the clones identified in the IVET vector (pTF86) are also expressedin vivo. Third, the seven promoter clones (asd, SD2, ribG, TF8,SD20, SD9, and TF7) that were putatively identified have homologousgenes in E. coli that are transcribed by sigma-70 promoters (10).While these facts do not rule out an alternative sigma factor,we expect that these genes are transcribed by a similar housekeepingsigma factor in A. pleuropneumoniae.

To confirm our promoter identification strategy, we compared the mRNA 5' ends that were identified from AP233 containing noplasmids and AP233 containing the asd plasmid. The cDNA productsfrom the reverse transcriptase reactions were identical. Thisresult verified that the putative transcriptional start site thatwe identified using the promoter trap vector was indeed the sameas the promoter used in the A. pleuropneumoniae genome to drivegeneexpression.

To further confirm our promoter identification, we constructed a deletion mutant from the SD2 clone. In this mutant, SD2 $Delta$ P,114 bp were deleted, including the $-$ 35 and $-$ 10 regions and theputative transcriptional start site, but not the primer-bindingsite for the reverse transcriptase reaction or the ATG. The mutantwas sequenced, and the region that was deleted was confirmed.There was no Lux expression in this mutant, and no primer extensionproduct was detected. The promoter region from SD2 was clonedback into the SD2 $Delta$ P mutant, and the resulting clone, SD2 $Delta$ PR, showedLux expression levels that were identical to that of the wild-typeSD2 and an identical primer extension product. Therefore, we concludethat the 114-bp segment contains a true promoter, and we inferthat the mRNA 5' end that we mapped represents a transcriptionalstartsite.

The nine promoters that were identified in this study demonstrated various degrees of promoter strength. However, the strengthof each could not be directly related to how similar the $-$ 10 and $-$ 35 sequences were to the proposed consensus sequence. This variabilityin expression suggests that there are other factors that modulatethe strength of individual promoters. In other eubacteria, thereare many factors that can affect the degree of promoter activity.The UP element and the $-$ 16 and $-$ 45 sequences modulate the activityof individual promoters and can do so with expression differencesof up to 100-fold, depending on the changes that are made (21,24). Additionally, the spacer region between the $-$ 10 and $-$ 35sequences plays a pivotal role in recognition of the promoterand also the promoter strength. In addition to the number of nucleotidesin the spacer region, it has been shown that the sequence of thespacer has an effect on strength (14). We have shown with theasd promoter clone mutant data that by inserting or deleting asingle base pair, we can alter the expression by up to sevenfoldin A. pleuropneumoniae. We theorize that additional factors contributeto modulation of A. pleuropneumoniae geneexpression.

This study has identified a consensus promoter structure for general housekeeping genes in A. pleuropneumoniae. This can beused to identify additional A. pleuropneumoniae promoters andprovides a baseline for future transcriptional studies in A. pleuropneumoniae.In the process of characterizing the promoter structure, we haveshown that A. pleuropneumoniae promoters are different from thoseof E. coli and B. subtilis. The promoters of A. pleuropneumoniaehave a shorter spacing between the $-$ 10 and $-$ 35 elements. A longerspacing of 17 or 18 bp drastically reduced promoter activity.This finding explains why some E. coli promoters do not functionwell in A. pleuropneumoniae and demonstrates that not all eubacterialconsensus promoters are identical to those identified for E. coliand B. subtilis.

	ACKNOWLEDGMENTS

This work was supported by USDA CSREES grant 98-02202.

We thank Robin Shea and Troy Fuller for their contributions to this work. We also thank Lee Kroos for his expert guidanceand critical review of the workpresented.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, Michigan State University, East Lansing, MI 48824-1101.Phone: (517) 355-6515. Fax: (517) 353-8957. E-mail: mulks{at}pilot.msu.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Altschul, S. F., W. Gish, W. Miller, E. W. Myers, and D. J. Lipman. 1990. Basic local alignment search tool. J. Mol. Biol. 215:403-410[CrossRef][Medline].

2. Bannantine, J. P., R. G. Barletta, C. O. Thoen, and R. E. Andrews. 1997. Identification of Mycobacterium paratuberculosis gene expression signals. Microbiology 143:921-928[Abstract/Free Full Text].

3. Corpet, F. 1988. Multiple sequence alignment with hierarchical clustering. Nucleic Acids Res. 16:10881-10890[Abstract/Free Full Text].

4. Dewhirst, F. E., B. J. Paster, I. Olsen, and G. J. Fraser. 1992. Phylogeny of 54 representative strains of species in the family Pasteurellaceae as determined by comparison of 16S rRNA sequences. J. Bacteriol. 174:2002-2013[Abstract/Free Full Text].

5. Frey, J., A. Haldimann, J. Nicolet, A. Boffini, and P. Prentki. 1994. Sequence analysis and transcription of the apxI operon (hemolysin I) from Actinobacillus pleuropneumoniae. Gene 142:97-102[CrossRef][Medline].

6. Fuller, T. E., R. S. Shea, B. J. Thacker, and M. H. Mulks. 1999. Identification of in vivo induced genes in Actinobacillus pleuropneumoniae. Microb. Pathog. 27:311-327[CrossRef][Medline].

7. Fuller, T. E., B. J. Thacker, and M. H. Mulks. 1996. A riboflavin auxotroph of Actinobacillus pleuropneumoniae is attenuated in swine. Infect Immun. 64:4659-4664[Abstract].

8. Genetics Computer Group. 1994. Program manual for the Wisconsin package, 8th ed. Genetics Computer Group, Madison, Wis.

9. Green, J., and M. L. Baldwin. 1997. HlyX, the FNR homologue of Actinobacillus pleuropneumoniae, is a (4Fe-4S)-containing oxygen responsive transcription regulator that anaerobically activates FNR-dependent class 1 promoters via an enhanced AR1 contact. Mol. Microbiol. 24:593-605[CrossRef][Medline].

10. Harley, C. B., and R. P. Reynolds. 1987. Analysis of E. coli promoter sequences. Nucleic Acids Res. 15:2343-2361[Abstract/Free Full Text].

11. Hawley, D. K., and W. R. McClure. 1983. Compilation and analysis of Escherichia coli promoter DNA sequences. Nucleic Acids Res. 11:2237-2255[Abstract/Free Full Text].

12. Helmann, J. D. 1995. Compilation and analysis of Bacillus subtilis sigma A-dependent promoter sequences: evidence for extended contact between RNA polymerase and upstream promoter DNA. Nucleic Acids Res. 23:2351-2360[Abstract/Free Full Text].

13. Hunneman, W. A. 1986. Incidence, economic effects and control of Haemophilus pleuropneumoniae infection in pigs. Vet. Q. 8:83-87[Medline].

14. Jensen, R. P., and K. Hammer. 1998. The sequence of spacers between the consensus sequences modulates the strength of prokaryotic promoters. Appl. Environ. Microbiol. 64:82-87[Abstract/Free Full Text].

15. Langford, P. R., B. M. Loynds, and J. S. Kroll. 1996. Cloning and molecular characterization of Cu,Zn superoxide dismutase from Actinobacillus pleuropneumoniae. Infect. Immun. 64:5035-5041[Abstract].

16. Lisser, S., and H. Margalit. 1993. Compilation of E. coli mRNA promoter sequences. Nucleic Acids Res. 21:1507-1516[Abstract/Free Full Text].

17. Malakooti, J., S. P. Wang, and B. Ely. 1995. A consensus promoter sequence for Caulobacter crescentus genes involved in biosynthetic and housekeeping functions. J. Bacteriol. 177:4372-4376[Abstract/Free Full Text].

18. Maniatis, T., E. F. Fritsch, and J. Sambrook. 1982. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

19. Nicolet, J. 1992. Actinobacillus pleuropneumoniae, p. 401-408. In A. D. Leman, B. E. Straw, W. L. Mengeling, S. D'Allaire, and D. J. Taylor (ed.), Diseases of swine, 7th ed. Iowa State University Press, Ames, Iowa.

20. Patek, M., B. J. Eikmanns, J. Patek, and H. Sahm. 1996. Promoters from Corynebacterium glutamicum: cloning, molecular analysis and search for a consensus motif. Microbiology 142:1297-1309[Abstract/Free Full Text].

21. Ross, W., S. Aiyar, J. Salomon, and R. L. Gourse. 1998. Escherichia coli promoters with UP elements of different strengths: modular structure of bacterial promoters. J. Bacteriol. 180:5375-5383[Abstract/Free Full Text].

22. Sebunya, T. N. K., and J. R. Saunders. 1983. Haemophilus pleuropneumoniae infection in swine: a review. J. Am. Vet. Med. Assoc. 182:1331-1337[Medline].

23. Strohl, W. 1992. Compilation and analysis of DNA sequences associated with apparent streptomycete promoters. Nucleic Acids Res. 20:961-974[Abstract/Free Full Text].

24. Voskuil, M. I., K. Koepel, and G. H. Chambliss. 1995. The $-$ 16 region, a vital sequence for the utilization of a promoter in Bacillus subtilis and Escherichia coli. Mol. Microbiol. 17:271-279[CrossRef][Medline].

25. West, S. E., M. J. Romero, L. B. Regassa, N. A. Zielinski, and R. A. Welch. 1995. Construction of Actinobacillus pleuropneumoniae-Escherichia coli shuttle vectors: expression of antibiotic resistance genes. Gene 160:81-86[CrossRef][Medline].

26. Wosten, M. M. S. M., M. Boeve, M. G. A. Koot, A. C. van Nuenen, and B. A. M. van der Zeist. 1998. Identification of Campylobacter jejuni promoter sequences. J. Bacteriol. 180:594-599[Abstract/Free Full Text].

27. Xiong, X., N. Cruz, and W. S. Reznikoff. 1991. Downstream deletion analysis of the lac promoter. J. Bacteriol. 173:4570-4577[Abstract/Free Full Text].

This article has been cited by other articles:

Chen, S., Bagdasarian, M., Kaufman, M. G., Bates, A. K., Walker, E. D. (2007). Mutational Analysis of the ompA Promoter from Flavobacterium johnsoniae. J. Bacteriol. 189: 5108-5118 [Abstract] [Full Text]
Blanco, M., Gutierrez-Martin, C. B., Rodriguez-Ferri, E. F., Roberts, M. C., Navas, J. (2006). Distribution of Tetracycline Resistance Genes in Actinobacillus pleuropneumoniae Isolates from Spain. Antimicrob. Agents Chemother. 50: 702-708 [Abstract] [Full Text]
Boekema, B. K. H. L., Van Putten, J. P. M., Stockhofe-Zurwieden, N., Smith, H. E. (2004). Host Cell Contact-Induced Transcription of the Type IV Fimbria Gene Cluster of Actinobacillus pleuropneumoniae. Infect. Immun. 72: 691-700 [Abstract] [Full Text]
Mikael, L. G., Pawelek, P. D., Labrie, J., Sirois, M., Coulton, J. W., Jacques, M. (2002). Molecular cloning and characterization of the ferric hydroxamate uptake (fhu) operon in Actinobacillus pleuropneumoniae. Microbiology 148: 2869-2882 [Abstract] [Full Text]
Shea, R. J., Mulks, M. H. (2002). ohr, Encoding an Organic Hydroperoxide Reductase, Is an In Vivo-Induced Gene in Actinobacillus pleuropneumoniae. Infect. Immun. 70: 794-802 [Abstract] [Full Text]
Schneider, T. D. (2001). Strong minor groove base conservation in sequence logos implies DNA distortion or base flipping during replication and transcription initiation. Nucleic Acids Res 29: 4881-4891 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	A correction has been published
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Doree, S. M.
	Articles by Mulks, M. H.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Doree, S. M.
	Articles by Mulks, M. H.

1.	Altschul, S. F., W. Gish, W. Miller, E. W. Myers, and D. J. Lipman. 1990. Basic local alignment search tool. J. Mol. Biol. 215:403-410[CrossRef][Medline].
2.	Bannantine, J. P., R. G. Barletta, C. O. Thoen, and R. E. Andrews. 1997. Identification of Mycobacterium paratuberculosis gene expression signals. Microbiology 143:921-928[Abstract/Free Full Text].
3.	Corpet, F. 1988. Multiple sequence alignment with hierarchical clustering. Nucleic Acids Res. 16:10881-10890[Abstract/Free Full Text].
4.	Dewhirst, F. E., B. J. Paster, I. Olsen, and G. J. Fraser. 1992. Phylogeny of 54 representative strains of species in the family Pasteurellaceae as determined by comparison of 16S rRNA sequences. J. Bacteriol. 174:2002-2013[Abstract/Free Full Text].
5.	Frey, J., A. Haldimann, J. Nicolet, A. Boffini, and P. Prentki. 1994. Sequence analysis and transcription of the apxI operon (hemolysin I) from Actinobacillus pleuropneumoniae. Gene 142:97-102[CrossRef][Medline].
6.	Fuller, T. E., R. S. Shea, B. J. Thacker, and M. H. Mulks. 1999. Identification of in vivo induced genes in Actinobacillus pleuropneumoniae. Microb. Pathog. 27:311-327[CrossRef][Medline].
7.	Fuller, T. E., B. J. Thacker, and M. H. Mulks. 1996. A riboflavin auxotroph of Actinobacillus pleuropneumoniae is attenuated in swine. Infect Immun. 64:4659-4664[Abstract].
8.	Genetics Computer Group. 1994. Program manual for the Wisconsin package, 8th ed. Genetics Computer Group, Madison, Wis.
9.	Green, J., and M. L. Baldwin. 1997. HlyX, the FNR homologue of Actinobacillus pleuropneumoniae, is a (4Fe-4S)-containing oxygen responsive transcription regulator that anaerobically activates FNR-dependent class 1 promoters via an enhanced AR1 contact. Mol. Microbiol. 24:593-605[CrossRef][Medline].
10.	Harley, C. B., and R. P. Reynolds. 1987. Analysis of E. coli promoter sequences. Nucleic Acids Res. 15:2343-2361[Abstract/Free Full Text].
11.	Hawley, D. K., and W. R. McClure. 1983. Compilation and analysis of Escherichia coli promoter DNA sequences. Nucleic Acids Res. 11:2237-2255[Abstract/Free Full Text].
12.	Helmann, J. D. 1995. Compilation and analysis of Bacillus subtilis sigma A-dependent promoter sequences: evidence for extended contact between RNA polymerase and upstream promoter DNA. Nucleic Acids Res. 23:2351-2360[Abstract/Free Full Text].
13.	Hunneman, W. A. 1986. Incidence, economic effects and control of Haemophilus pleuropneumoniae infection in pigs. Vet. Q. 8:83-87[Medline].
14.	Jensen, R. P., and K. Hammer. 1998. The sequence of spacers between the consensus sequences modulates the strength of prokaryotic promoters. Appl. Environ. Microbiol. 64:82-87[Abstract/Free Full Text].
15.	Langford, P. R., B. M. Loynds, and J. S. Kroll. 1996. Cloning and molecular characterization of Cu,Zn superoxide dismutase from Actinobacillus pleuropneumoniae. Infect. Immun. 64:5035-5041[Abstract].
16.	Lisser, S., and H. Margalit. 1993. Compilation of E. coli mRNA promoter sequences. Nucleic Acids Res. 21:1507-1516[Abstract/Free Full Text].
17.	Malakooti, J., S. P. Wang, and B. Ely. 1995. A consensus promoter sequence for Caulobacter crescentus genes involved in biosynthetic and housekeeping functions. J. Bacteriol. 177:4372-4376[Abstract/Free Full Text].
18.	Maniatis, T., E. F. Fritsch, and J. Sambrook. 1982. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
19.	Nicolet, J. 1992. Actinobacillus pleuropneumoniae, p. 401-408. In A. D. Leman, B. E. Straw, W. L. Mengeling, S. D'Allaire, and D. J. Taylor (ed.), Diseases of swine, 7th ed. Iowa State University Press, Ames, Iowa.
20.	Patek, M., B. J. Eikmanns, J. Patek, and H. Sahm. 1996. Promoters from Corynebacterium glutamicum: cloning, molecular analysis and search for a consensus motif. Microbiology 142:1297-1309[Abstract/Free Full Text].
21.	Ross, W., S. Aiyar, J. Salomon, and R. L. Gourse. 1998. Escherichia coli promoters with UP elements of different strengths: modular structure of bacterial promoters. J. Bacteriol. 180:5375-5383[Abstract/Free Full Text].
22.	Sebunya, T. N. K., and J. R. Saunders. 1983. Haemophilus pleuropneumoniae infection in swine: a review. J. Am. Vet. Med. Assoc. 182:1331-1337[Medline].
23.	Strohl, W. 1992. Compilation and analysis of DNA sequences associated with apparent streptomycete promoters. Nucleic Acids Res. 20:961-974[Abstract/Free Full Text].
24.	Voskuil, M. I., K. Koepel, and G. H. Chambliss. 1995. The $-$ 16 region, a vital sequence for the utilization of a promoter in Bacillus subtilis and Escherichia coli. Mol. Microbiol. 17:271-279[CrossRef][Medline].
25.	West, S. E., M. J. Romero, L. B. Regassa, N. A. Zielinski, and R. A. Welch. 1995. Construction of Actinobacillus pleuropneumoniae-Escherichia coli shuttle vectors: expression of antibiotic resistance genes. Gene 160:81-86[CrossRef][Medline].
26.	Wosten, M. M. S. M., M. Boeve, M. G. A. Koot, A. C. van Nuenen, and B. A. M. van der Zeist. 1998. Identification of Campylobacter jejuni promoter sequences. J. Bacteriol. 180:594-599[Abstract/Free Full Text].
27.	Xiong, X., N. Cruz, and W. S. Reznikoff. 1991. Downstream deletion analysis of the lac promoter. J. Bacteriol. 173:4570-4577[Abstract/Free Full Text].