Multiple In Vivo Roles for the -12-Region Elements of Sigma 54 Promoters

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Journal of Bacteriology, November 1998, p. 5626-5631, Vol. 180, No. 21
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Multiple In Vivo Roles for the $-$ 12-Region Elements of Sigma 54 Promoters

Lei Wang and Jay D. Gralla^*

Department of Chemistry and Biochemistry and Molecular Biology Institute, University of California, Los Angeles, Los Angeles, California 90095-1569

Received 26 May 1998/Accepted 26 August 1998

	ABSTRACT

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Alignment of sigma 54-dependent promoters indicates conservation of two sequence elements. Six nucleotides in the downstream $-$ 12 element were mutated individually to each nonconsensus nucleotide.mRNA levels were measured in vivo for each promoter under stronglyactivating conditions. The results showed that the consensus sequencewas not the strongest promoter. Instead, the $-$ 12 consensus elementconsists of two subregions that behave differently when mutated.Single changes in the upstream TTT consensus subregion can leadto increases in transcription, whereas single changes in the downstreamGC(A/T) can lead to decreases in transcription. Selected doublemutations with changes in both subregions were constructed andstudied in vivo. No double mutation increased promoter strength,and some decreased it. Mutant promoters were also assayed undernonactivating conditions in vivo. No mRNA was detected in 23 ofthe 24 promoters tested. However, one double mutant showed substantiallevels of transcript, indicating that the $-$ 12 sequence was capableof specifying basal transcription under nonactivating conditions.Overall, the results show that the $-$ 12 region has multiple rolesin transcription in vivo, including modulating both basal andinduced RNA levels.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Sigma 54 is an alternative sigma factor that binds the common bacterial core RNA polymerase and converts it into an enhancer-dependentenzyme (15, 16, 35). It targets promoters with recognitionelements centered near positions $-$ 24 and $-$ 12 (19, 20). Whensigma 54 holoenzyme initially binds to such promoters, it failsto melt the DNA and thus remains in an inactive state (2, 21,22, 26). Activation occurs when a modified activator proteinbinds the remote enhancer and loops to the bound polymerase, causingit to melt the DNA (3, 8, 22, 25, 29). Transcriptionthen proceeds from this open complex.

DNA binding by sigma 54 polymerase is complex. Sigma 54 alone has a low affinity for most promoters but can bind to the Rhizobiummeliloti nifH promoter in the absence of core RNA polymerase (2).Core polymerase association increases the DNA-binding affinity,allowing occupancy on other promoters (5). The main DNA-bindingdeterminants are in the C-terminal portion of sigma 54 (27,37). However, several other parts of the protein make importantcontributions to DNA recognition (7). Candidate subregionsof sigma involved in DNA binding have been identified (6, 11,13, 30). These regions of sigma have not been assigned definitivelyto the recognition of particular elements within the promoter.

Recognition of the promoter $-$ 24 element appears to be dominant for DNA binding. That is, there are no examples where sigma54 mutant complexes form but do not protect the $-$ 24 region ina footprinting experiment (14, 37). By contrast numerous mutationsexist, both in sigma and in DNA, that allow binding to occur butinterfere specifically with protection of the $-$ 12 element. Thesebound complexes that are defective in $-$ 12-element recognitionare typically of lower affinity (33). Despite the occupancyof the promoter by the holoenzyme, such complexes often are defectivein function, implying that $-$ 12 interactions have functions inaddition to binding to DNA.

Other lines of evidence confirm that the $-$ 12 region has multiple effects in sigma 54-dependent transcription. Changes in thisregion are known to be associated with changes in transcriptionlevel (1, 4, 17, 28). The sequence at $-$ 12 can determinehow sensitive the promoter is in vivo to a particular activator(4, 23). In vitro transcription studies showed that certain $-$ 12 sequences tend to promote leaky "bypass" expression in theabsence of an activator (34). Consistent with these multiplepotential roles of the $-$ 12 region is the fact that several separatedparts of the sigma 54 polypeptide appear to cooperate to recognizethe $-$ 12 region (7, 27). Despite the apparent multifunctionalrole of the $-$ 12 region there have not been systematic studiesof the effects of changing $-$ 12 region sequences.

For these reasons, we have investigated the effects of changing each residue in the $-$ 12 region to each other residue. Theeffects of the changes were assayed by measuring mRNA levels invivo. The results showed that the consensus $-$ 12 sequence was onlyintermediate in promoter strength. The data also showed that the $-$ 12 region consists of two subelements, each of which could havean independent role in transcriptional control.

	MATERIALS AND METHODS

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Plasmid construction and site-directed mutagenesis. The plasmid pBR-M12 was constructed by replacing the tetracycline gene of pBR322 with the M12 promoter fragment from pFC50-M12(9). Plasmid pBR322 was cut with EcoRI and AvaI (New EnglandBiolabs) to separate the 1,008-bp tetracycline gene region fromthe main body. The large fragment of pBR322 was purified by agarosegel electrophoresis, and the AvaI site was made blunt by usingKlenow enzyme (New England Biolabs). Plasmid pFC50-M12 was digestedwith EcoRI and EheI (New England Biolabs) to release a 1,236-bpfragment containing the functional glnH promoter region, initialcoding sequences, and the previously inserted T7 early terminator.The purified fragment was ligated with the pBR322 main-body fragmentto create plasmid pBR-M12. The M12 mutant promoter was createdpreviously by point mutation of T to G at $-$ 14 in the glnHp₂ promoter(9).

The QuikChange site-directed mutagenesis kit (Stratagene) was used to introduce single mutations in the $-$ 12 consensus sequenceof the M12 promoter in Epicurian Coli XL1-Blue supercompetentcells. The presence of mutations was confirmed by sequencing.

Cell growth and RNA analysis. pBR-M12 and its derivatives were transformed into a PcnB strain (with the pcnB gene deleted) to maintain low copy numbers.Cells were grown overnight in Luria broth (LB) medium and thendiluted 1:20 into 3 ml of either LB or G-gln (500 ml of G-glnmedium contains W salts [5.25 g of K₂HPO₄, 2.25 g of KH₂PO₄, 0.215ml of 1 M MgSO₄], 0.4% glucose, 1.0 ml of thiamine [10.0 mg/ml],and 1 g of L-glutamine) containing 100 µg of ampicillin/ml. Whenthe cells reached an optical density at 600 nm of 0.4 to 0.6,they were collected and RNA was extracted with the RNeasy kit(Qiagen) and eluted in a total volume of 30 µl. Sample volumeswere adjusted slightly to use the same number of cells in separateexperiments.

Samples (12 µl) were taken for mRNA analysis. Primer extension with reverse transcriptase (RT) (Promega) was done with the³²P-labeled oligonucleotide primer GCCAGGGTCAGTGCAGCCA, complementaryto the glnH transcript. The 86-nucleotide radioactive cDNA wassized on a 6% urea polyacrylamide gel with sequencing markersand corresponded to expectations based on in vitro transcription(34). Amounts were quantified with a PhosphorImager (MolecularDynamics).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Derivation of the consensus and construction of mutant promoters. To update the consensus sequence for sigma 54 promoters, we aligned the sequences for 16 confirmed promoters from Escherichiacoli, Salmonella typhimurium, and Klebsiella pneumoniae (4,10, 12) (Fig. 1). The lower portion of the figure shows thosenucleotides that are conserved in at least half of the promoters.The analysis confirms that recognition is likely to involve twosequence-conserved blocks. These are CTGGCACA, from $-$ 21 to $-$ 28(the $-$ 24 region), and ATTTGC(A/T)T, from $-$ 11 to $-$ 18 (the $-$ 12 region).(The numbering system used here is based on glnHp₂ and differsfrom that used for some individual promoters due to minor variationsin the location of the transcription start site.) We note thatthe centers of these two blocks are separated by 10 bp, suggestingthat they are centered on the same face of the DNA helix.

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FIG. 1. Alignment of 16 available sigma 54-dependent promoters from three related bacteria (1, 10, 12, 19). The consensus nucleotides and their frequency of appearance are indicated below the alignment. The $-$ 24 and $-$ 12 regions that contain these consensus elements are boxed, with the consensus nucleotides shown in boldface.

This is consistent with prior alignments (19) but suggests more extended conservation of sequence. In this study of the $-$ 12 region we chose to modify the central hexanucleotide sequence.This includes bases identified previously as "consensus," withthe addition of a single upstream T that prior studies have implicatedin sigma recognition (2).

The starting plasmid (pFC50-M12) for this work contains a promoter with the hexanucleotide consensus (9). This M12 promoteris a derivative of glnHp₂ in which the T at $-$ 14 has been changedto the consensus G. Nucleotide $-$ 12 in this promoter is an A, whichis slightly better conserved than T at this position in the collectionshown in Fig. 1. The M12 promoter retains the natural upstreambinding sites for activator NtrC (also called NR1) as well asthe intervening IHF binding sites. A segment of the initial glnHcoding region is also retained.

In the experimental scheme for making changes in the consensus sequence, a large set of mutant promoters are studied, eachcarried in by the vector, which is a multicopy plasmid. In orderto minimize potential titration of required transcription factorsby the plasmid, two conditions were used. First, a PcnB host strain was used, which greatly reduces copy numbers (18).Second, the promoter insert of pFC50-M12 was transferred to pBR322to form pBR-M12, which has a lower copy number than the originalpUC-based vector. Two experiments demonstrated that the low copynumber was achieved. First, PcnB cells transformed with pFC50-M12 could not grow when plated on1/10 the amount of ampicillin required to prevent wild-type growth.Second, agarose gel analysis showed a 10-fold reduction in theamount of DNA (pFC50-M12 or pBR-M12) isolated from the PcnB host. Based on these and other experiments we estimate that thereare two or three copies of the plasmid per cell. As this is substantiallyless than the number of sigma 54 regulatory regions on the chromosome,we infer that there will be little perturbation of metabolismby factor titration.

Seventeen changes were introduced by site-directed mutagenesis into the central TTTGCA of the $-$ 12 region of the M12 promotercontained on this vector (Table 1). These included changes toeach nonconsensus nucleotide at each position (position $-$ 12 wasnot changed from the more conserved A to the less conserved T).The goal was to measure the mRNA levels associated with each ofthese 17 promoters and thereby deduce the importance of each nucleotide.

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TABLE 1. In vivo mRNA levels from promoter M12 and its derivatives^a

mRNA production from singly mutated promoters. We first measured mRNA from cells transformed with the consensus glnH-M12 promoter in different media. The purpose was toidentify the media giving the highest and lowest mRNA signals.The transformed cells were diluted from overnight cultures inrich media. The cells were grown to mid-log phase in four mediathat differ in nitrogen availability: LB medium with excess nitrogen,glucose minimal medium supplemented with either arginine (W-Arg)(31) or glutamine (G-Gln) (24), and glycerol minimal mediumsupplemented with glutamate (36). The amount of promoter-specificmRNA was estimated by hybridizing a small DNA primer complementaryto the initial glnH mRNA sequence and copying it with RT. Becausethe cells are expected to require glnH operon function for growthon certain media, the endogenous glnH promoter is present on thechromosome; the RT products include those from this single-copygene. Figure 2 shows the signal obtained on G-Gln medium for nontransformedcells (lane host) and cells transformed with the glnH-M12 fusion(lane M12). The signal from the M12 promoter on the plasmid istaken as the difference between these two signals.

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FIG. 2. Autoradiograph of primer extension products of mRNAs with various promoters in strongly activating G-Gln medium. "Host" refers to nontransformed cells, and the signal is from the endogenous glnH gene.

PhosphorImager analysis was used to determine the amount of promoter M12 transcription in the various media. Transcriptionwas highest on G-Gln medium and lowest (undetectable) on LB, consistentwith expectations based on the availability of nitrogen. In theinitial studies we use the high-activation potential G-Gln medium.

The 17 promoters were individually transformed, and mRNA production was studied as described above. Examples of mRNA assaysfrom six promoters are shown in Fig. 2. As can be seen in theseexamples, some $-$ 12-region changes from the M12 consensus leadto decreases in transcription. Obvious examples are G-14C (i.e.,the G at position 14 changed to a C), C-13T, and A-12G. Each ofthese mRNA signals is less intense than M12 and only slightlyabove the background signal from the endogenous host glnH gene.Other mutant promoters behave differently. Mutation C-13A showslittle change in mRNA level. T-17G shows an increased mRNA levelcompared to that of the M12 consensus promoter.

The mRNA signals were somewhat variable, and for that reason mRNA was assayed from each of the 17 promoters between threeand seven times. Identical numbers of cells were used for eachexperiment, and each experiment included a parallel sample fromthe M12 promoter plasmid. The mRNA signal levels for the variouspromoters were normalized to the M12 levels from the same experiment.The resulting mean (± standard deviation) signals are collectedin Table 1.

The results show that at least four promoter mutations cause increases in transcription: T-17G, T-16G, T-15C, and T-15A. Inaddition, at least three promoter mutations cause decreases intranscription: G-14C, C-13T, and A12-G. It is obvious from thesedata that the consensus sequence is neither the best nor the worstpromoter at directing high mRNA levels. The variation caused bythe introduction of single-point mutations is eight- to ninefold,increased about 2.6-fold by T-15A and decreased 3.3-fold by C-13T.

The effect of changing each consensus nucleotide is shown in Fig. 3. The data indicate that changing the upstream and downstreamparts of the $-$ 12 consensus leads to quite different consequences.When the upstream TTT segment is mutated the resulting promotereither produces more mRNA or is unaffected. When the downstreamGCA segment is mutated the resulting promoter either producesless mRNA or is unaffected. We infer that the $-$ 12 consensus sequenceelement contains two subelements which have the potential to behavedifferently in mRNA production.

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FIG. 3. The effect on mRNA levels of single substitutions at each position in the M12 consensus promoter. Changes that increase transcription are shown above the axis, and those that decrease transcription are shown below the axis; the height of each bar represents the ratio of RNA to that of M12. The solid bars represent statistically significant differences from M12, as indicated in Table 1. The nucleotide change associated with each mutant promoter is indicated below each bar.

Effects of double mutations in which both subelements are mutated. Some of the above-mentioned results are expected based on prior studies, and some are not. The data indicate that the effectsof the T stretch may be particularly complex in that changes couldlessen sigma binding but enhance transcription (1). The deleteriouseffect of mutating the highly conserved $-$ 13C to T is unsurprising.However, the lack of effect of G and A substitutions at this mosthighly conserved position is unexpected. One possible explanationis that these $-$ 13 substitutions show no effect because they aremade in the context of an otherwise consensus promoter. To testthis idea, we made double mutants D1 and D2, in which the C-13Amutation was coupled with substitutions for the highly conservedT at position $-$ 15 (the sequence is shown in Fig. 4A). For thesemutants, and other double mutants discussed below, the mRNA wascompared to that of the M12 promoter. This allowed the comparisonof levels from double and single mutations.

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FIG. 4. Transcription from double mutants in nonactivating and activating media. (A) Sequences of the mutants. The changed nucleotides in each of the double mutants are underlined. (B) Analysis of RNA from double mutants D1 and D2 in activating G-Gln medium. (C) Analysis of RNA from double mutants in nonactivating LB medium. The induced transcripts from the consensus M12 promoter in activating G-Gln medium are shown for comparison. (D) Analysis of RNA in a strain lacking ( $-$ ) or containing (+) sigma 54 (rpoN).

The results show that in the context of a nonconsensus promoter the C-13A change has a strong effect and leads to significantreductions in transcription (Fig. 4B). This is true for both mutantsD1 and D2, which have approximately two-thirds the RNA level ofthe M12 consensus promoter. The reduction due to the $-$ 13 changeis even stronger than that illustrated here, as it is made inthe context of nonconsensus promoters that have mRNA levels higherthan that of the consensus M12 promoter. That is, the single $-$ 13position substitution leads to a three- to fourfold lowering ofmRNA levels in the context of the nonconsensus promoters T-15Cand T-15A (Table 1). Thus, the $-$ 13 nucleotide is clearly important,as expected from its conservation. Apparently, its importancecan be masked in the context of an otherwise consensus promoter.The complex relationship between the two halves of the sequencefrom $-$ 17 to $-$ 12 will be discussed further below.

Previously, we raised the possibility that these $-$ 12-region sequences may play an additional role beyond specifying the levelof RNA made during activating conditions. In vitro-transcriptionexperiments showed that a nonconsensus promoter could be leakierthan a consensus promoter; that is, in the absence of an activatorthe nonconsensus promoter produced more RNA, albeit at ratherlow levels (34). To see if this could be true in vivo, we measuredRNA levels from all the promoters by using LB medium, where theconsensus promoter produced no detectable RNA (Fig. 4, lanes M12).No single-point mutations led to detectable RNA under these conditions,indicating that none of the sequences give leaky transcription(data not shown).

We extended these experiments to learn if double mutations could lead to leaky transcription in vivo. Four additional doublemutations were made, each including a substitution at position $-$ 15 and an additional change in the downstream half of the promoterelement (Fig. 4A). Each of these promoters was used to drive mRNAproduction on nonactivating LB medium. The results with the sixdouble mutations are shown in Fig. 4.

The results show that one double mutation (Fig. 4C, lane D3) leads to production of mRNA under nonactivating conditions. Toconfirm that this mRNA is sigma 54 dependent, we transformed D3and the M12 control into strain ymc109, which lacks sigma 54.Figure 4D shows that the D3 signal is not produced in this strainin LB medium, in contrast to the result obtained in the straincontaining sigma 54 and as expected for a sigma 54-dependent transcript.

Quantitation of D3 mRNA in LB medium shows that the level is fairly substantial, as it is about 1/10 of the amount of RNAmade by the consensus M12 promoter under fully activated conditions(Fig. 4C, G-Gln). This D3 promoter, as well as the promoters D4,D5, and D6, produces mRNA amounts on fully activated G-Gln mediumthat do not differ dramatically from that of M12 (data not shown).Thus, promoter D3 is still inducible but the ratio is only about10-fold, as the basal level is high. Because mRNA from M12 isnot detectable under nonactivating conditions (Fig. 4C and D),we cannot quantify the normal induction ratio; our best estimateis that it should be at least 100-fold, but this is very uncertain.In any case, the D3 double mutation creates a promoter with ahigh basal level and a roughly normal induced level. This demonstratesa new in vivo role for the $-$ 12-region promoter element: it cancontrol the level of basal expression independently of the levelof induced expression.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

These results imply that the $-$ 12 regions of sigma 54 promoters have multiple and complex roles in transcription. In the initialset of experiments each nucleotide in a central consensus sequencewas changed to each possible nonconsensus nucleotide. mRNA productionin vivo from each of the singly substituted promoters was thenmeasured. The results showed that the consensus promoter sequencedid not direct the highest level of transcription.

This result raises the question of why promoter $-$ 12 elements resemble TTTGC(A/T) more than any other sequence. Of the 16 naturalpromoters surveyed, 3 matched this consensus exactly, 7 had asingle mismatch, and 6 had a double mismatch. Each of these promotersneeds to bind sigma 54 polymerase, and the $-$ 12 sequence playsan important secondary role in this binding (see the introduction).We speculate that the various promoters retain significant resemblanceto the consensus so that they will have a sufficient number ofrecognition determinants to achieve this binding. If so, the consensuspromoter would represent the tightest binder of sigma (2).This, however, need not correlate with the highest level of transcription.That is, as long as sigma can become fully bound, other sequenceswould influence how much RNA would be produced by the bound sigma54 holoenzyme.

This view is supported by experiments showing that the upstream and downstream halves of a consensus $-$ 12-region promoter havethe potential to function differently. When the upstream TTT stretchwas mutated a number of changes led to increases in transcription.Interestingly, such an effect was observed previously, althoughit seemed to depend on the nature of the activator-promoter combination(1). This was never observed in the downstream GCA stretch;the sequence behaved more according to expectation in that changesto nonconsensus nucleotides often led to decreases in transcription.It is known that a change to create the consensus TTT sequencecan increase the affinity of sigma for DNA (2). One possibleexplanation for these properties of the TTT sequence is that thesequence can help to attract sigma but the binding could be tootight for optimal function (32) in the context of a fully consensuspromoter.

When mutations in the upstream and downstream halves of the $-$ 12 region were combined, a variety of effects were observed.None of the doubly mutated promoters showed mRNA levels that exceededconsensus levels, even though the single T-stretch mutations onwhich they were based had this property. Some of the double mutationsled to significantly lower RNA levels. In view of the above considerations,it may be that some minimal match to the consensus is needed tofully bind the sigma 54 holoenzyme and some double mutations failin this regard. In vitro studies are under way to test these ideas.

Study of the double mutations also revealed a striking effect of the $-$ 12 region on the regulation of induction. All of theabove studies applied to the functioning of the promoters on G-Glnmedium, which is the most strongly activating medium of thosesurveyed. When the very rich medium LB was used no mRNA was detected,as expected on such nitrogen-rich medium. One double mutant, however,failed to fully restrict RNA synthesis under these conditionsof full nitrogen availability. In this case the repressive effectswere sufficiently defective to give rise to approximately 10%of the fully induced level of RNA. This occurs despite the factthat the medium is sufficiently repressing to keep NtrC so inactivethat it fails to direct any transcription of the consensus promoter.The result demonstrates an additional role for certain $-$ 12-regionsequences: keeping transcription levels low during conditionsof nitrogen availability.

Such leaky transcription has been observed in vitro under specialized conditions and with protocols designed to optimize transcriptionin the absence of activator activity (34). We proposed in thosestudies that tight interactions between the $-$ 12 region of DNAand the N terminus of sigma 54 might be responsible for keepingbasal transcription levels low. The present results support thatview, although it would require the construction of many moremultiply mutated promoters to begin to define the sequences involved.

Thus, the diversity of sequences associated with the $-$ 12 regions of natural promoters can be seen as physiologically appropriatein terms of diverse roles for this element. Promoter $-$ 12 elementsshould exist that support the highest level of activated transcriptionfor genes that require such high levels. The data suggest thatsuch promoters may not match the consensus in the upstream T stretch.Other promoters may diverge further from the consensus in somecases to provide a basal level of transcription for genes thatneed low-level expression even under conditions of nitrogen sufficiency.The existing $-$ 12 sequences may be viewed as providing a balancebetween the need for RNA upon activation and the need to restrictit under nonactivating conditions. Further studies will be requiredto learn how the $-$ 12-region sequences influence this balance ofcompeting requirements.

	ACKNOWLEDGMENTS

This work was supported by NIH grant GM35754.

We thank Robert P. Gunsalus and Paul McNicholas for help with the PcnB strain and the Gralla research group for their advice.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Chemistry & Biochemistry and Molecular Biology Institute, Universityof California, Los Angeles, P.O. Box 951569, Los Angeles, CA 90095-1569.Phone: (310) 825-1620. Fax: (310) 267-2302. E-mail: gralla{at}ewald.mbi.ucla.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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30. Taylor, M., R. Butler, S. Chambers, M. Casimiro, F. Badii, and M. Merrick. 1996. The RpoN-box motif of the RNA polymerase sigma factor sigma N plays a role in promoter recognition. Mol. Microbiol. 22:1045-1054[Medline].

31. Tintut, Y., and J. D. Gralla. 1995. PCR mutagenesis identifies a polymerase-binding sequence of sigma 54 that includes a sigma 70 homology region. J. Bacteriol. 177:5818-5825[Abstract/Free Full Text].

32. Tintut, Y., J. T. Wang, and J. D. Gralla. 1995. A novel bacterial transcription cycle involving sigma(54). Genes Dev. 9:2305-2313[Abstract/Free Full Text].

33. Wang, J. T., and J. D. Gralla. 1996. The transcription initiation pathway of sigma 54 mutants that bypass the enhancer protein requirement: implications for the mechanism of activation. J. Biol. Chem. 271:32707-32713[Abstract/Free Full Text].

34. Wang, J. T., A. Syed, and J. D. Gralla. 1997. Multiple pathways to bypass the enhancer requirement of sigma 54 RNA polymerase: roles for DNA and protein determinants. Proc. Natl. Acad. Sci. USA 94:9538-9543[Abstract/Free Full Text].

35. Wang, J. T., A. Syed, M. Hsieh, and J. D. Gralla. 1995. Converting Escherichia coli RNA polymerase into an enhancer-responsive enzyme: role of an NH2-terminal leucine patch in sigma 54. Science 270:992-994[Abstract/Free Full Text].

36. Willis, R. C., K. K. Iwata, and C. E. Furlong. 1975. Regulation of glutamine transport in Escherichia coli. J. Bacteriol. 122:1032-1037[Abstract/Free Full Text].

37. Wong, C., Y. Tintut, and J. D. Gralla. 1994. The domain structure of sigma 54 as determined by analysis of a set of deletion mutants. J. Mol. Biol. 236:81-90[Medline].

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Appl. Environ. Microbiol.	Infect. Immun.	Eukaryot. Cell
Mol. Cell. Biol.	J. Virol.	Microbiol. Mol. Biol. Rev.
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31.	Tintut, Y., and J. D. Gralla. 1995. PCR mutagenesis identifies a polymerase-binding sequence of sigma 54 that includes a sigma 70 homology region. J. Bacteriol. 177:5818-5825[Abstract/Free Full Text].
32.	Tintut, Y., J. T. Wang, and J. D. Gralla. 1995. A novel bacterial transcription cycle involving sigma(54). Genes Dev. 9:2305-2313[Abstract/Free Full Text].
33.	Wang, J. T., and J. D. Gralla. 1996. The transcription initiation pathway of sigma 54 mutants that bypass the enhancer protein requirement: implications for the mechanism of activation. J. Biol. Chem. 271:32707-32713[Abstract/Free Full Text].
34.	Wang, J. T., A. Syed, and J. D. Gralla. 1997. Multiple pathways to bypass the enhancer requirement of sigma 54 RNA polymerase: roles for DNA and protein determinants. Proc. Natl. Acad. Sci. USA 94:9538-9543[Abstract/Free Full Text].
35.	Wang, J. T., A. Syed, M. Hsieh, and J. D. Gralla. 1995. Converting Escherichia coli RNA polymerase into an enhancer-responsive enzyme: role of an NH2-terminal leucine patch in sigma 54. Science 270:992-994[Abstract/Free Full Text].
36.	Willis, R. C., K. K. Iwata, and C. E. Furlong. 1975. Regulation of glutamine transport in Escherichia coli. J. Bacteriol. 122:1032-1037[Abstract/Free Full Text].
37.	Wong, C., Y. Tintut, and J. D. Gralla. 1994. The domain structure of sigma 54 as determined by analysis of a set of deletion mutants. J. Mol. Biol. 236:81-90[Medline].

Multiple In Vivo Roles for the 12-Region Elements of Sigma 54 Promoters

Multiple In Vivo Roles for the $-$ 12-Region Elements of Sigma 54 Promoters