Activation of Escherichia coli leuV Transcription by FIS

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Journal of Bacteriology, June 1999, p. 3864-3868, Vol. 181, No. 12
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Activation of Escherichia coli leuV Transcription by FIS

Wilma Ross,¹ Julia Salomon,¹ Walter M. Holmes,² and Richard L. Gourse¹^,^*

Department of Bacteriology, University of Wisconsin, Madison, Wisconsin 53706,¹ and Department of Microbiology and The Massey Cancer Center, Medical College of Virginia, Virginia Commonwealth University, Richmond, Virginia 23298²

Received 10 February 1999/Accepted 16 April 1999

	ABSTRACT

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The transcription factor FIS has been implicated in the regulation of several stable RNA promoters, including that for themajor tRNA^Leu species in Escherichia coli, tRNA₁^Leu. However, no evidence for direct involvement of FIS in tRNA₁^Leu expression has been reported. We show here that FIS binds toa site upstream of the leuV promoter (centered at $-$ 71) and thatit directly stimulates leuV transcription in vitro. A mutationin the FIS binding site reduces transcription from a leuV promoterin strains containing FIS but has no effect on transcription instrains lacking FIS, indicating that FIS contributes to leuV expressionin vivo. We also find that RNA polymerase forms an unusual heparin-sensitivecomplex with the leuV promoter, having a downstream protectionboundary of ~ $-$ 7, and that the first two nucleotides of the transcript,GTP and UTP, are required for formation of a heparin-stable complexthat extends downstream of the transcription start site. Thesestudies have implications for the regulation of leuVtranscription.

	TEXT

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The leuV operon encodes three of the four genes for tRNA₁^Leu, one of the most abundant Escherichia coli tRNA species (12, 21).The promoter for leuV is strong, with activity similar to thatof the rRNA promoter rrnB P1 (6, 7); like many other rRNAand tRNA promoters, it is regulated in response to growth rateand amino acid starvation (6, 37). The leuV promoter hasseveral features similar to those of rRNA promoters, includingnear-consensus $-$ 10 and $-$ 35 hexamers spaced at the nonconsensusdistance of 16 bp, a G+C-rich sequence (the discriminator region)between the $-$ 10 element and the transcription start site, andan upstream sequence that contributes to promoter activity (Fig.1). However, the effect of upstream sequence at leuV is smallerthan that at rrnB P1 (~10- to 40-fold versus ~300-fold) (6,7, 34), and the mechanism(s) responsible for its effectshas not been fully characterized.

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FIG. 1. Sequence of the leuV promoter region. Positions protected by FIS in DNase I footprints and positions of enhanced DNase I cleavage within the FIS site (carets) are indicated. Enhanced DNase I cleavage at $-$ 38 and $-$ 48 in the presence of RNAP is indicated by vertical arrows. The 2-bp substitution mutant T $-$ 71G T $-$ 72G reduces FIS binding (Fig. 2). Boundaries of protection by RNAP in the absence (thin underline, $-$ 47 to $-$ 7) or the presence (thick underline, $-$ 47 to +20) of the initiating nucleotides GTP and UTP are indicated. Similarity of the FIS site to a consensus derived from information in references 15 and 20 [Gnn(c/t)(A/g)(a/t)(a/t)(T/A)(t/a)(t/a)(T/c)(g/a)nnC] is indicated by lines between the top and bottom strands. Dots between strands in the FIS site indicate poorly conserved positions in different FIS sites.

The leuV upstream sequence has two components, and their contributions to promoter strength are similar (6, 7). Theregion just upstream of the $-$ 35 hexamer ( $-$ 39 to $-$ 47) is likelyto increase transcription by interacting with the C-terminal domainof the $alpha$ subunit of RNA polymerase (RNAP), since it is quite similarto the promoter-proximal region of the UP element consensus (13)and since in vitro transcription of leuV in the absence of proteinsother than RNAP is reduced by an RNAP $alpha$ -subunit mutation thatabolishes UP element recognition ( $alpha$ $Delta$ 235) (35). The second region,between $-$ 47 and $-$ 107, affects transcription by a previously uncharacterizedmechanism. It was originally suggested that a T tract in thisregion (at $-$ 69 to $-$ 73) influences leuV promoter activity throughits effects on DNA bending (7). However, a 2-bp substitutionwithin this T tract (T $-$ 71G T $-$ 72G) abolished the upstream effecton transcription without affecting the anomalous electrophoreticmobility (bending) of the promoter fragment (7).

FIS is a 12-kDa DNA binding protein that directly activates transcription from a number of promoters by binding to sites upstreamof the core promoter (e.g., rrnB P1, thrU/tufB, tyrT, proP, andmar [26, 29, 31, 32, 36, 40]). FIS also plays a rolein other cellular processes, including repression of transcription(41), site-specific recombination (15), transposition (39),and DNA replication (14). It was suggested that FIS contributesto tRNA₁^Leu transcription, since at higher growth rates in fis mutant strainsthe concentration of tRNA₁^Leu (as well as of some other tRNAs) is reduced relative to thatof 16S rRNA (30). However, it was not known whether this effectof fis was direct orindirect.

The concentration of FIS in the cell varies dramatically as a function of growth rate and growth phase (2, 3), and theextent of activation by FIS at some promoters varies as a functionof growth rate (1, 11). However, regulation of rrnB P1 withgrowth rate appears to involve a different mechanism that involvessensing of the initiating nucleotide concentration (16). Theextent of activation of rrnB P1 by FIS does not vary substantiallywith growth rate in wild-type strains (1), although FIS isresponsible for growth rate-dependent regulation of rrnB P1 instrains with RNAP mutations that alter the nucleoside triphosphate(NTP)-sensing mechanism (4). Thus, the contribution of FISto promoter activity and regulation can vary, depending on thespecific kinetic properties of a promoter and other regulatorymechanisms that affectit.

In this work, we have identified a FIS binding site in the leuV promoter upstream region and we have examined the effectsof FIS on leuV expression both in vivo and in vitro by using promoterderivatives with mutant or wild-type FIS binding sites. We havealso identified an unusual heparin-sensitive RNAP complex withthe leuV promoter. These studies support the proposal that multiplemechanisms, including activation by FIS and NTP sensing, contributeto the transcription and regulation of leuV.

Identification of a FIS binding site upstream of the leuV promoter. FIS binds to the upstream region in several stable RNA promoters (rrnB P1, tyrT, tufB, and valU [10, 31, 36, 38]),and putative FIS binding sites have been identified upstream ofmany others, including leuV (24, 25, 30). The proposed leuVFIS site contains a one-base mismatch from the consensus (Fig.1) (15). However, the degeneracy of the FIS consensus sequencehas limited its predictive value, and not all consensus sequencesactually bind purified FIS (14, 15). We therefore determinedthe location of FIS binding sites in the leuV promoter regionexperimentally.

In a DNase I footprinting experiment, FIS protected a site in the leuV promoter centered at $-$ 71 (Fig. 1 and 2A). The positionof the site and the apparent K_d, approximately 2 to 4 nM (determinedfrom additional DNase I footprint titrations [not shown]), weresimilar to that of FIS site I in the rrnB P1 promoter (17, 36).Sites of enhanced DNase I cleavage within the leuV site ( $-$ 66, $-$ 67, $-$ 78, and $-$ 79 on the bottom strand; $-$ 64, $-$ 66, and $-$ 76 on thetop strand [Fig. 1 and 2A]) are likely to reflect FIS-inducedDNA distortion or kinking, as noted for other FIS sites (15).At much higher FIS concentrations (~160 nM), there was partialoccupancy of a second site, overlapping the core promoter region(data not shown). Similar weak binding sites for FIS also occurin the rrnB P1 core promoter (34), but no function has beenascribed to these sites.

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FIG. 2. DNase I footprints of FIS bound to wild-type (A) or mutant (B) leuV promoter fragments. BglII-HindIII leuV promoter fragments were obtained from pleuD9 (leuV $-$ 109 to +33 [7]) or pHEB3 (leuV $-$ 109 to +11, T $-$ 71G T $-$ 72G [7]) and were ³²P labeled in the bottom (template) strand at the BglII site, approximately 20 bp upstream from leuV position $-$ 109. Footprinting reactions were carried out at 22°C, essentially as described previously (35), in a solution of 10 mM Tris-Cl (pH 7.9), 10 mM MgCl₂, 150 mM NaCl, 1 mM dithiothreitol, and 100 µg of bovine serum albumin per ml. FIS was present at the concentrations indicated. Sequence markers were prepared by the method of Maxam and Gilbert (27).

A previously constructed 2-bp substitution mutation in the leuV promoter is located within the FIS binding site (pHEB3, T $-$ 71GT $-$ 72G [Fig. 1] [7]). This mutation reduced the affinity forFIS by at least 10-fold (apparent K_d, ~40 to 80 nM [Fig. 2B anddata not shown]).

Multiple FIS binding sites contribute to activation at some other promoters (8, 29, 32, 36). However, at leuV onlyone FIS site was observed within the sequence extending to $-$ 109.Since the sequence upstream of ~ $-$ 76 was previously found not tocontribute to leuV promoter activity (7), it seems unlikelythat FIS sites upstream of $-$ 109 have a major effect on leuVtranscription.

FIS activates transcription from the leuV promoter in vitro. Transcription of the wild-type leuV promoter and of two mutant leuV promoters that lack a functional FIS binding site (T $-$ 71GT $-$ 72G and $Delta$ $-$ 47, a leuV derivative with a deletion of sequencesupstream of $-$ 47) was carried out in vitro in the presence of increasingconcentrations of FIS. FIS stimulated transcription from the wild-typeleuV promoter, with maximal activation (about threefold) observedat approximately 10 nM FIS (Fig. 3). Transcription from the promoterdeleted for the FIS binding site ( $Delta$ $-$ 47) was not affected by FISat any concentration tested, while that of the 2-bp substitutionmutant promoter (T $-$ 71G T $-$ 72G) was stimulated only by much higherconcentrations of FIS (>50 nM) than that required for the wild-typepromoter (Fig. 3), consistent with the differences in affinityfor FIS of the wild-type and mutant promoters observed by DNaseI footprinting (Fig. 2).

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FIG. 3. Effects of FIS on in vitro transcription of wild-type and mutant leuV promoters (wild type, diamonds; T $-$ 71G T $-$ 72G mutant, triangles; FIS site deletion [ $-$ 47 endpoint], circles). Transcription was carried out in the absence of FIS or in the presence of the indicated concentrations of FIS by using supercoiled plasmid templates with leuV promoter fragments inserted into the EcoRI and HindIII sites of pRLG770, upstream of the rrnB T1 terminator (36). Plasmids used were pRLG927 (wild-type leuV $-$ 109 to +33, obtained from pleuD9 [7]), pRLG930 (leuV $-$ 109 to +11, T $-$ 71G T $-$ 72G, obtained from pHEB3 [7]), and pRLG931 (leuV $-$ 47 to +55, obtained from pLC118 [7]). Multiple-round transcription was carried out essentially as described previously (36) except that nucleotide concentrations were 100 µM (for ATP, CTP, and GTP) or 10 µM (for UTP, with [ $alpha$ -³²P]UTP [DuPont, NEN]). Purified FIS was a gift from Reid Johnson (University of California at Los Angeles). leuV transcripts were analyzed on 6.5% acrylamide-7 M urea gels and quantified with a Molecular Dynamics PhosphorImager. The effect of FIS is shown as a ratio of transcript values in the presence and absence of FIS. Results from a representative experiment are shown.

FIS activates transcription from the leuV promoter in vivo. The effect of FIS on leuV transcription in vivo was determined by comparing the activity of the wild-type promoter with thatof the promoter containing the FIS site mutation T $-$ 71G T $-$ 72G.Promoter activities were determined in strains containing single-copychromosomal promoter-lacZ fusions. The FIS site mutation reducedpromoter activity to about 44% of its wild-type activity in astrain containing FIS (Table 1 [see also Table 2]), a resultconsistent with previous observations with similar constructs(7). However, this mutation did not reduce leuV promoter activityin a strain lacking FIS (a fis::kan strain [Table 1]). This resultindicates that the effect of the mutation in the wild-type strainis attributable to loss of FIS binding and activation.

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TABLE 1. Effects of FIS site substitution or deletion mutations on leuV promoter activity in wild-type fis and fis::kan strains

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TABLE 2. Strains and plasmids

Deletion of the entire FIS site ( $Delta$ $-$ 47) had a slightly larger effect on promoter activity than the 2-bp substitution, reducingit to 28% of wild-type activity (Table 1). This suggests eitherthat the 2-bp substitution does not fully eliminate activationby FIS (consistent with the weak affinity of the 2-bp mutant DNAfor FIS [Fig. 2B and 3]), that sequences upstream of $-$ 47 contributeslightly to the leuV UP element, or both. The latter possibilityis consistent with the slight reduction in activity of the $Delta$ $-$ 47promoter (74% of the wild type) in a fis::kan strain (Table 1).

As observed previously for other promoters (26, 36), the activity of each of the leuV promoters was greater in fis::kanstrains than in wild-type fis strains (Table 1). This increasemay reflect contributions from at least two factors. First, someof the increase in leuV activity is likely to result from a compensatingeffect of the rRNA feedback system acting on core promoter function,as described previously for the rrnB P1 and tufB promoters (32,36). This feedback effect is thought to result from loss ofactivation of the rrn operons by FIS and may operate through therecently described NTP-sensing mechanism for growth rate regulationof rrn promoters (16). Transcription from growth rate-regulatedrrn P1 promoters lacking FIS sites is increased to a greater extent(approximately four- to fivefold) than transcription from controlpromoters (see below) in fis::kan strains (34b, 36). An effectof the feedback system on the leuV promoter is consistent withpreviously described effects of altered rrn gene dosages on tRNAexpression (19, 22).

In addition, some of the increase in leuV activity in fis::kan strains is likely to derive from a promoter-independent effecton the lacZ reporter system, since all promoter-lacZ fusions thatwe have tested (including non-growth-rate-regulated promoterssuch as lacUV5 and growth rate-defective mutant derivatives ofrrnB P1) show some degree of increase in activity in fis::kanstrains (~1.5- to 2-fold) (34a). Since FIS has many roles inthe cell and fis mutants have pleiotropic effects (14), thisnonspecific effect is notsurprising.

Although transcription of the leuV-lacZ fusion appears to be as active in fis::kan strains as in wild-type strains (Table1), reduced levels of tRNA₁^Leu have been reported (relative to 16S rRNA) in fis mutant strains(30). These observations are consistent with the proposed contributionof a nonspecific increase in promoter-lacZ fusion activity infis::kan strains, together with a feedback derepression of theleuV core promoter activity that may not be as great as the derepressionobserved for rrnB P1. This suggests that the leuV promoter maynot be as responsive to the NTP-sensing mechanism as is rrnB P1(see also references 5 and 33). Alternatively, the apparentdiscrepancy between pleuV-lacZ fusion activity and reduced tRNA₁^Leu levels in fis::kan strains may reflect either an overestimateof tRNA₁^Leu production from the leuV operon (which encodes three tandem tRNA^Leu genes) with the promoter-lacZ fusion or reduced tRNA productionfrom the argT operon, which encodes the fourth tRNA₁^Leugene.

Properties of RNAP-leuV promoter complexes. Since RNAP forms an unstable, heparin-sensitive complex with the rrnB P1 promoter, a feature responsible at least in partfor its regulation by the NTP-sensing mechanism, we also characterizedthe properties of complexes formed between RNAP and the leuV promoterby using DNase I footprinting. RNAP formed a heparin-sensitivecomplex with the leuV promoter in the absence of NTPs (Fig. 4,lanes 4 and 5). The boundaries of this complex are somewhat unusual,extending from $-$ 47 to about $-$ 7, thus not including the transcriptionstart site. At rrnB P1, a closed, heparin-sensitive complex withprotection extending approximately to the transcription startsite ( $-$ 60 to +1) was observed under similar conditions (5,8). These complexes differ from the open, heparin-stable complexesformed at most other promoters in the absence of nucleotides.

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FIG. 4. DNase I footprints of RNAP bound to the wild-type leuV promoter. Complexes were formed with RNAP (10 nM) and the leuV promoter fragment (described in the legend to Fig. 2) in the presence or absence of the initiating nucleotides (500 µM GTP or 500 µM GTP and 50 µM UTP) at 22°C in buffer described in the legend to Fig. 2, except that it contained 30 mM KCl rather than 150 mM NaCl. Where indicated, heparin (10 µg/ml) was added prior to DNase I digestion.

A heparin-stable leuV promoter-RNAP complex, in which protection extended downstream to ~+20, was formed in the presence ofthe initiating nucleotides GTP and UTP but not with GTP alone(Fig. 4, lanes 6 to 9). These results are similar to those obtainedwith rrnB P1, where the initiating nucleotides ATP and CTP, generatinga 5-mer slipped transcript (9, 18), were required for a heparin-stablecomplex. At leuV, the presence of GTP and UTP would be predictedto result in formation of a template-directed 5-mertranscript.

The proximal UP element region of the leuV promoter (~ $-$ 40 to $-$ 47) was protected by RNAP in both the heparin-sensitive ( $-$ 47to $-$ 7) and heparin-stable ( $-$ 47 to +20) complexes, although theregion upstream of $-$ 47 was not protected. This protection patternis consistent with stimulation of transcription by the sequencebetween $-$ 39 and $-$ 47 (7). Sites of enhanced DNase I cleavageoccurred at positions $-$ 38 and $-$ 48 (Fig. 1 and 4), suggesting thatRNAP may bend or distort the DNA at these sites. Similar enhancedcleavage was observed at position $-$ 38 in the rrnB P1 promoter(35).

Implications of these findings for the regulation of leuV promoter activity. The results presented here are consistent with the model that multiple mechanisms, including activation by FIS and an NTPconcentration-sensing mechanism, may contribute to regulationof leuV transcription. We find that leuV transcription is directlyactivated by FIS and that, like rrn P1 promoters, it respondsto a feedback regulation signal generated by mutation of the fisgene. However, the response of the leuV promoter to the feedbacksignal may not be as great as that observed for rrnB P1, sincetRNA₁^Leu levels are somewhat reduced in fis::kan strains (30). Consistentwith this hypothesis, RNAP mutations that alter the NTP-sensingmechanism at rrnB P1 also affect leuV transcription but to a lesserdegree than rrnB P1 (5). Other findings are also consistentwith the possibility that the NTP-sensing mechanism describedfor rrnB P1 affects leuV transcription. These include the formationof unusual heparin-sensitive complexes of the leuV promoter withRNAP (Fig. 4), the moderate level of growth rate-dependent regulationof leuV promoter derivatives lacking a FIS site (6, 33),and the dependence of leuV transcription in vitro on the concentrationof the initiating nucleotides GTP and CTP (some transcripts wereobserved to initiate with CTP [33]). Thus, leuV transcriptionmost likely reflects multiple regulatory inputs (33).

	ACKNOWLEDGMENTS

This work was supported by grant GM37408 from the National Institutes of Health to R.L.G. and by grant GM50747 to W.M.H.

We thank Yanira O'Neill-Morales and Mike Bartlett for construction of leuV promoter-lacZfusions.

	FOOTNOTES

^* Corresponding author. Mailing address: Dept. of Bacteriology, University of Wisconsin, 1550 Linden Dr., Madison, WI 53706.Phone: (608) 262-9813. Fax: (608) 262-9865. E-mail: rgourse{at}bact.wisc.edu.

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Zhi, H., Wang, X., Cabrera, J. E., Johnson, R. C., Jin, D. J. (2003). Fis Stabilizes the Interaction between RNA Polymerase and the Ribosomal Promoter rrnB P1, Leading to Transcriptional Activation. J. Biol. Chem. 278: 47340-47349 [Abstract] [Full Text]
Hirvonen, C. A., Ross, W., Wozniak, C. E., Marasco, E., Anthony, J. R., Aiyar, S. E., Newburn, V. H., Gourse, R. L. (2001). Contributions of UP Elements and the Transcription Factor FIS to Expression from the Seven rrn P1 Promoters in Escherichia coli. J. Bacteriol. 183: 6305-6314 [Abstract] [Full Text]
Bartlett, M. S., Gaal, T., Ross, W., Gourse, R. L. (2000). Regulation of rRNA Transcription Is Remarkably Robust: FIS Compensates for Altered Nucleoside Triphosphate Sensing by Mutant RNA Polymerases at Escherichia coli rrn P1 Promoters. J. Bacteriol. 182: 1969-1977 [Abstract] [Full Text]
Pokholok, D. K., Redlak, M., Turnbough, C. L. Jr., Dylla, S., Holmes, W. M. (1999). Multiple Mechanisms Are Used for Growth Rate and Stringent Control of leuV Transcriptional Initiation in Escherichia coli. J. Bacteriol. 181: 5771-5782 [Abstract] [Full Text]

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