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Journal of Bacteriology, August 2007, p. 5472-5481, Vol. 189, No. 15
0021-9193/07/$08.00+0     doi:10.1128/JB.00529-07
Copyright © 2007, American Society for Microbiology. All Rights Reserved.

CsrA Inhibits Translation Initiation of Escherichia coli hfq by Binding to a Single Site Overlapping the Shine-Dalgarno Sequence

Carol S. Baker,¹ Lél A. Eöry,^1,2, Helen Yakhnin,¹ Jeffrey Mercante,³ Tony Romeo,³ and Paul Babitzke^1*

Department of Biochemistry and Molecular Biology, The Pennsylvania State University, University Park, Pennsylvania 16802,¹ School of Biochemistry and Microbiology, University of Leeds, Leeds, United Kingdom,² Department of Microbiology and Immunology, Emory University School of Medicine, Atlanta, Georgia 30322³

Received 6 April 2007/ Accepted 18 May 2007

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Csr (carbon storage regulation) of Escherichia coli is a global regulatory system that consists of CsrA, a homodimeric RNA binding protein, two noncoding small RNAs (sRNAs; CsrB and CsrC) that function as CsrA antagonists by sequestering this protein, and CsrD, a specificity factor that targets CsrB and CsrC for degradation by RNase E. CsrA inhibits translation initiation of glgC, cstA, and pgaA by binding to their leader transcripts and preventing ribosome binding. Translation inhibition is thought to contribute to the observed mRNA destabilization. Each of the previously known target transcripts contains multiple CsrA binding sites. A position-specific weight matrix search program was developed using known CsrA binding sites in mRNA. This search tool identified a potential CsrA binding site that overlaps the Shine-Dalgarno sequence of hfq, a gene that encodes an RNA chaperone that mediates sRNA-mRNA interactions. This putative CsrA binding site matched the SELEX-derived binding site consensus sequence in 8 out of 12 positions. Results from gel mobility shift and footprint assays demonstrated that CsrA binds specifically to this site in the hfq leader transcript. Toeprint and cell-free translation results indicated that bound CsrA inhibits Hfq synthesis by competitively blocking ribosome binding. Disruption of csrA caused elevated expression of an hfq'-'lacZ translational fusion, while overexpression of csrA inhibited expression of this fusion. We also found that hfq mRNA is stabilized upon entry into stationary-phase growth by a CsrA-independent mechanism. The interaction of CsrA with hfq mRNA is the first example of a CsrA-regulated gene that contains only one CsrA binding site.

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Bacteria have evolved several regulatory strategies that ensure their survival in response to changes in their growth environment. The Csr (carbon storage regulation) and homologous Rsm (repressor of secondary metabolites) global regulatory systems of several eubacterial species control numerous genes and processes posttranscriptionally. Csr systems consist of at least one RNA binding protein that either activates or represses expression of target mRNAs, as well as one or more small noncoding regulatory RNAs (sRNAs) that contain multiple CsrA binding sites. The sRNAs function as antagonists of the RNA binding protein(s) via protein sequestration (reviewed in references 1 and 26). The Csr system of Escherichia coli is involved in the repression of several stationary-phase processes and the activation of some exponential-phase functions. Four major components of Csr in this organism include the homodimeric RNA binding protein CsrA, two sRNA antagonists of CsrA (CsrB and CsrC), and CsrD, a protein that specifically targets both sRNAs for degradation by RNase E (18, 35, 45). CsrA represses gluconeogenesis, glycogen metabolism, peptide transport, and biofilm formation (11, 16, 27, 28, 42, 48), while it activates glycolysis, acetate metabolism, and flagellum biosynthesis (28, 43, 44). CsrB and CsrC sequester CsrA and prevent its interaction with mRNA targets. Multiple imperfect repeat sequences in these regulatory RNAs function as CsrA binding sites, such that each sRNA is capable of sequestering several CsrA dimers (14, 18, 45).

CsrA negatively regulates expression of the glycogen biosynthetic gene glgC by binding to four sites in the untranslated leader of the glgCAP operon transcript, one of which overlaps the glgC Shine-Dalgarno (SD) sequence (reference 2 and unpublished results). CsrA binding to the glgCAP leader transcript inhibits GlgC synthesis by blocking ribosome binding. Presumably, CsrA-mediated inhibition of glgC translation is responsible for the accelerated rate of glgCAP mRNA decay (19). CsrA also represses translation of cstA, a carbon starvation-induced gene thought to be involved in peptide transport (11, 31), as well as the first gene in the pgaABCD operon, a cluster of genes that are required for the synthesis of the polysaccharide adhesin poly-ß-1,6-N-acetyl-D-glucosamine (PGA), which participates in biofilm formation (42). CsrA binds to four sites in the cstA transcript and to six sites in the pga operon leader transcript. In each case, one of the CsrA binding sites overlaps the cognate SD sequence. Translational repression of these genes proceeds by a mechanism that is similar to the mechanism identified for glgC (11, 42). Considerable sequence variation exists among the known E. coli CsrA binding sites; however, GGA is a highly conserved sequence element which is often present in the loop of short RNA hairpins. Systematic evolution of ligands by exponential enrichment (SELEX) was used to isolate high-affinity CsrA ligands (10). The high-affinity RNA ligands contained a single CsrA binding site with a consensus sequence of RUACARGGAUGU, with the underlined residues being 100% conserved. In each case the GGA motif was present in the loop of a short predicted hairpin (10).

A bioinformatics approach was used to search the E. coli genomic database for genes containing potential CsrA binding sites. A potential CsrA binding site was identified that overlaps the hfq SD sequence, suggesting that CsrA might regulate translation initiation of this gene. E. coli Hfq is a toroid-shaped homohexamer that was discovered as a protein required for in vitro transcription of bacteriophage Qß RNA (12, 29). Hfq is present in a wide range of bacterial species, and its role in global control of gene expression is readily apparent, as it impacts numerous physiological processes, such as virulence, bacteriocin production, and nitrogen fixation (40). Numerous studies have established that Hfq functions as an RNA chaperone in promoting sRNA-mRNA base-pairing (reviewed in references 13 and 34). For example, it is well established that Hfq activates translation of S, the stationary-phase sigma factor, by promoting base-pairing of two sRNAs to the rpoS leader transcript. Base-pairing of either sRNA disrupts an inhibitory RNA structure in the rpoS leader such that translation is stimulated (13, 23, 34).

We confirmed that CsrA binds to the site in hfq identified in silico. As this CsrA binding site overlaps the hfq SD sequence, bound CsrA inhibits translation initiation of hfq by blocking ribosome binding. The interaction of CsrA with the hfq transcript described here is unique, as this is the first example of a CsrA-regulated mRNA that contains only a single CsrA binding site. Because Hfq mediates many intermolecular sRNA-mRNA interactions in the cell, these findings imply that CsrA has a substantially greater influence on global regulatory networks than previously recognized.

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Bacterial strains and plasmids. Plasmid pCSB52 contains the wild-type hfq leader and the first 55 nucleotides (nt) of the hfq coding region (+1 to +124 relative to the start of P3_hfq promoter transcription) (37) cloned into the pTZ18U polylinker (United States Biochemical Corp.). pCSB60 contains an hfq'-'lacZ translational fusion consisting of the P3_hfq promoter and leader region as well as the first 18 codons of hfq (–66 to +124 relative to the start of P3_hfq transcription), cloned in frame with the lacZ gene of pMLB1034 (32). Three nucleotide substitutions in the hfq leader just upstream of the SD sequence and within the CsrA binding site (A51T:T52G:A53C) were introduced into pCSB60 using the QuikChange II protocol (Stratagene), resulting in plasmid pCSB62. E. coli strains used for ß-galactosidase assays were constructed to create single-copy chromosomal gene insertions of hfq'-'lacZ translational fusions into the att site using the InCh protocol as described previously (5). Strains PLB785 and PLB786 contain the hfq'-'lacZ fusion from pCSB60 integrated into the chromosome of strains CF7789 (MG1655 lacI-Z [MluI]) and TR1-5CF7789 (CF7789 csrA::kan), respectively. Strains PLB923 and PLB924 contain the hfq'-'lacZ fusion from pCSB62 integrated into the chromosomes of CF7789 and TR1-5CF7789, respectively. Plasmid pCRA16 (36) contains csrA cloned into pBR322 (4). Strain PLB786 was transformed with pBR322 and pCRA16 to generate strains PLB789 and PLB793, respectively. Plasmid pYH109 was generated by replacing the Bacillus subtilis trp operon sequence in pYH28 (30) with a PCR fragment containing the hfq leader and amino-terminal coding sequence (+1 to +179 relative to P3_hfq transcription), resulting in an hfq'-'gfp translational fusion (37th hfq codon fused in frame with gfp). The E. coli smpB gene was cloned into the pET28A⁺ polylinker (Novagen) to create pETB. Unless otherwise indicated, all strains were grown at 37°C in Lennox LB medium. When appropriate, growth media were supplemented with antibiotics to the following concentrations: ampicillin, 100 µg/ml; kanamycin, 50 µg/ml; tetracycline, 20 µg/ml.

Gel mobility shift assay. Quantitative gel mobility shift assays followed a previously published procedure (46). E. coli CsrA-H6 protein was purified as described previously (10). RNA was synthesized in vitro using the MEGAscript kit (Ambion) and linearized pCSB52 as template. Gel-purified RNA was 5'-end labeled with [-³²P]ATP as described previously (46). RNA suspended in Tris-EDTA (TE) buffer was renatured by heating to 80°C followed by slow cooling to room temperature. Binding reaction mixtures (10 µl) contained 10 mM Tris-HCl, pH 7.5, 10 mM MgCl₂, 100 mM KCl, 32.5 ng of yeast RNA, 7.5% glycerol, 20 mM dithiothreitol (DTT), 4 U of RNase inhibitor (Promega), 0.5 nM hfq leader RNA, purified CsrA-H6 (various concentrations), and 0.1 mg/ml xylene cyanol. Competition assay mixtures also contained unlabeled RNA competitor. Reaction mixtures were incubated for 30 min at 37°C to allow CsrA-RNA complex formation. Samples were then fractionated on native 8% polyacrylamide gels. Radioactive bands were visualized with a phosphorimager. Free and bound RNA species were quantified using ImageQuant (Molecular Dynamics), and the apparent equilibrium binding constant (K_d) of the CsrA-hfq RNA interaction was calculated as described previously (46).

Toeprint assay. Toeprint assays were performed by modifying published procedures (2, 15). hfq leader transcripts used in this analysis were synthesized using the MEGAscript kit and linearized pCSB52 as template. Gel-purified hfq leader RNA (500 nM) in TE was renatured and hybridized to a 5'-end-labeled DNA oligonucleotide (500 nM) in TE that was complementary to the 3' end of the transcript. Hybridization was accomplished by heating the mixture to 80°C followed by slow cooling to room temperature. Toeprint assay mixtures contained various concentrations of CsrA-H6 and/or 260 nM 30S ribosomal subunits and 5 µM tRNA^fMet. E. coli ribosomes were purified as described previously (25). Purified 30S ribosomal subunits were obtained by denaturing 70S ribosomes, followed by purification through a sucrose gradient. 30S subunit fractions were pooled and stored at –80°C in 10 mM Tris-HCl, pH 7.5, 60 mM NH₄OAc, 6 mM 2-mercaptoethanol, 10 mM MgCl₂, and 10% glycerol. Previously frozen 30S ribosomal subunits were thawed, activated by incubation at 37°C for 15 min, and kept on ice until addition to toeprint reaction mixtures. Toeprint reaction mixtures (20 µl) contained 2 µl of the hybridization mixture, 375 µM each deoxynucleoside triphosphate, and 10 mM DTT in toeprint buffer (10 mM Tris-HCl, pH 7.4, 10 mM MgCl₂, 60 mM NH₄OAc, 6 mM 2-mercaptoethanol). Mixtures containing CsrA were incubated for 30 min at 37°C to allow CsrA-mRNA complex formation. 30S ribosomal subunit toeprint reactions were performed by incubating RNA, 30S ribosomal subunits, and tRNA^fMet in toeprint buffer as described previously (15). Following the addition of 3 U of avian myeloblastoma virus reverse transcriptase (Roche), the reaction mixture was further incubated for 15 min at 37°C. Reactions were terminated by the addition of 12 µl of stop solution (70 mM EDTA, 85% formamide, 0.1x Tris-borate-EDTA, 0.025% xylene cyanol, and 0.025% bromophenol blue). Samples were heated at 95°C for 5 min prior to fractionation through standard 6% polyacrylamide sequencing gels. Sequencing reactions were performed using pCSB52 as the template and the same end-labeled DNA oligonucleotide as a primer. Radioactive bands were visualized with a phosphorimager.

RNA footprint assay. Preparation of 5'-end-labeled hfq leader transcripts was as described for the gel shift analysis. Titrations of RNase T₁ (Roche) and RNase T₂ (Sigma) were performed to identify the amount of enzyme in which 90% of the transcripts were full length to minimize multiple cleavages in any one transcript. Binding reaction mixtures (10 µl) containing various concentrations of CsrA-H6 and 50 nM hfq RNA were otherwise identical to those described for the gel shift assay. After the initial binding of CsrA-H6, either RNase T₁ (0.025 U) or RNase T₂ (0.03 U) was added to the reaction mixtures, and incubation was continued for 15 min at 37°C. Reactions were terminated by the addition of 10 µl of gel loading buffer II (Ambion) and kept on ice. Partial alkaline hydrolysis and RNase T₁ digestion ladders of each transcript were prepared as described previously (3). Samples were fractionated through standard 6% polyacrylamide sequencing gels. Radioactive bands were visualized with a phosphorimager.

ß-Galactosidase assays. Bacterial cultures growing in liquid medium at 37°C were monitored using a Klett-Summerson colorimeter (no. 52 green filter). Culture samples (4 ml) were harvested at various times, washed once with 10 mM Tris-HCl, pH 7.5, and frozen as cell pellets at –20°C. Cell extracts were prepared by suspending frozen cell pellets in 0.5 ml of BugBuster protein extraction reagent (Novagen), followed by incubation at 37°C in an air shaker. After 30 min, 0.3 ml of Z buffer (24) containing 0.2 mg/ml lysozyme was added to each sample, and incubation was continued for 30 min at 37°C in an air shaker. Cell debris was removed by centrifugation at 4°C. ß-Galactosidase assays were performed using the cell extracts (2, 24). Protein concentrations were determined by the Bio-Rad protein assay with bovine serum albumin as a standard.

mRNA abundance and mRNA half-life assays. Bacterial cultures were mixed with 2 volumes of RNAprotect bacterial reagent (QIAGEN) and incubated at room temperature for 5 min. Cells were then harvested, and total RNA was prepared using the Masterpure RNA purification kit (Epicenter) and treated with DNase I according to the manufacturer's recommendations. RNA was quantified by measuring the absorbance at 260 and 280 nm.

To measure hfq transcript levels, strains MG1655 (wild type) and TR1-5MG1655 (csrA::kan) were grown at 37°C in Lennox LB medium to exponential phase (optical density at 600 nm of 0.4) or to early stationary phase (optical density at 600 nm of 4.0). Total RNA was purified, and the steady-state level of hfq mRNA was determined by real-time quantitative reverse transcription-PCR (RT-qRT-PCR) using the primer pair hfq-Fw (5'-AAGCACGCGATTTCTACTGTTG-3') and hfq-Rv (5'-CCACCGGCGTTGTTACTGT-3') and the probe Hfq-6FAM-BHQ1 (5'-CCCGTCTCGCCCGGTTTCTCA-3'), which was 5'-end labeled with 6-carboxyfluorescein (6FAM) and 3'-end labeled with Black Hole Quencher 1 (BHQ1). RT-qRT-PCR was performed using the iScript one-step RT-PCR kit for probes (Bio-Rad) with a Bio-Rad iCycler IQ real-time system. The conditions used for RT-PCR were as follows: 50°C for 10 min, 95°C for 5 min, and 40 cycles of 95°C for 15 s and 65°C for 30 s. Unless otherwise noted, all primers and probes were used at a final concentration of 200 nM. Real-time measurements were taken during the 65°C step. Reactions were performed in triplicate in two independent experiments, each time with 100 ng of template RNA. A set of reactions lacking reverse transcriptase was performed for each RNA sample as a control for DNA contamination. For normalization of hfq RNA levels, RT-qRT-PCRs were performed with each sample for 16S rRNA quantitation using the primer pair 16S-Fw (5'-CGTGTTGTGAAATGTTGGGTTAA-3') and 16S-Rv (5'-CCGCTGGCAACAAAGGATA-3') and the probe 16S-6FAM-BHQ1 (5'-TCCCGCAACGAGCGCAACC-3'). The reaction conditions for RT-qRT-PCR of 16S rRNA were identical to hfq except that 1 ng of RNA template was used for each reaction. The 2^–CT method was used to calculate relative hfq RNA levels, which allowed for the use of a 16S rRNA control (20).

For hfq mRNA half-life studies, strains MG1655 (wild type) and TR1-5MG1655 (csrA::kan) were grown as described above. Cells were harvested at various times following the addition of rifampin (200 µg/ml final concentration), and total RNA was purified as described above using RNAprotect. RT-qRT-PCR was performed as described above for steady-state hfq RNA determinations. The percentage of RNA remaining through the time course was determined by calculating the difference in cycle threshold (C_T) and the subsequent fold difference compared to the 0-min time point after controlling for 16S rRNA levels.

RNA-directed cell-free translation. Cell-free translation reactions followed previously published procedures (9, 47). Transcripts for this analysis were synthesized using the Ambion MEGAscript kit. hfq'-'gfp and smpB transcripts were synthesized using linearized pYH109 and pETB as templates, respectively. bla was transcribed from a 1,020-nt PCR fragment containing a T7 promoter. CsrA-deficient E. coli S-30 extract was prepared from TR1-5 MG1655 (csrA::kan) according to published procedures (47). The S-30 extract was preincubated with RNase-free DNase I for 15 min at 37°C to remove chromosomal DNA and to allow time for E. coli RNases to degrade endogenous mRNA. Reaction mixtures (24 µl) contained 60 mM Tris-HEPES, pH 7.5, 60 mM NH₄Cl, 5 mM to 15 mM MgCl₂ (determined empirically for each transcript), 12 mM KCl, 0.5 mM EGTA, 5 mM DTT, 2 mM ATP, 0.6 mM GTP, 0.08 mM calcium folinate, 4 mg/ml of aprotinin, 4 mg/ml of leupeptin, 4 mg/ml of pepstatin A, 4 µl S-30 extract (12 mg of total protein), 800 U/ml of DNase I, 500 U/ml of RNasin, 10 mM phosphoenolpyruvate, 35 U of pyruvate kinase, 0.4 mg/ml of E. coli tRNA, 0.04 µg/ml of mRNA, 10 µCi [³⁵S]methionine, 0.5 mM of each of the other amino acids, and 0.8 mM spermidine. Reaction mixtures were incubated for 45 min at 37°C and terminated by adding 6 µl of stop buffer (125 mM Tris-HCl, pH 6.8, 5% sodium dodecyl sulfate [SDS], 25% glycerol, 2% 2-mercaptoethanol, and 12.5 mg/ml of bromophenol blue). Samples were heated at 95°C for 5 min prior to fractionation by 14% SDS-polyacrylamide gel electrophoresis (PAGE). Radioactive bands were visualized with a phosphorimager and quantified using ImageQuant.

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Identification of hfq as a potential CsrA-regulated gene. A genome search program was developed to identify potential CsrA binding sites by exploring the properties of known CsrA binding motifs. A total of 14 CsrA binding sites were previously identified in the leader regions of glgC, cstA, and pgaA (references 2, 11, and 42 and unpublished results). These sequences were aligned using ClustalW (7), and a position weight matrix (pwm) was calculated from the alignment using the MATCH tool (17). The pwm was then used as a scoring function to identify potential CsrA binding sites within the E. coli genomic database. The scores were assigned from 0 to 100% according to the minimum and the maximum score calculated from the pwm. The details of the pwm will be published elsewhere. This program predicted the presence of CsrA binding sites in 278 genes with scores of 96.5% or above, including the three genes that were used in generating the pwm (cstA, glgC, and pgaA). A CsrA binding site with a score of 96.8% was identified that overlaps the hfq SD sequence. This predicted sequence also conformed to the SELEX-derived consensus sequence in 8 out of 12 positions (Fig. 1). However, unlike the CsrA binding sites identified by SELEX, secondary structural predictions using MFOLD (49) indicated that the GGA motif within this putative CsrA binding site was not present in the loop of a hairpin. The pwm also identified three potential sites with scores between 81.8 and 83.5%; however, since all three of these sites overlapped the predicted site with a score of 96.8% and none of them contained an appropriately positioned GGA motif, it appeared that hfq contained one likely CsrA binding site. Because all of the known CsrA-controlled genes contained four to six CsrA binding sites, experiments were carried out to determine whether hfq contained a single CsrA binding site and whether CsrA could bind to this site in hfq and regulate its expression.

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FIG. 1. Predicted CsrA binding site overlapping the hfq SD sequence. The SELEX-derived CsrA binding site consensus sequence is shown above the predicted CsrA binding site in hfq mRNA. Vertical lines mark the residues in the predicted site that match those in the consensus. Positions of the hfq SD sequence and translation initiation codon (Met) are shown.

CsrA binds to the predicted site in hfq. hfq transcription is driven by three promoters just upstream of its coding sequence. The hfq transcript originating from the SD sequence-proximal P3 promoter (P3_hfq) contains a 68-nt untranslated leader (37). To characterize the interaction of CsrA with hfq RNA, quantitative gel mobility shift assays were performed with an hfq transcript containing nucleotides +1 to +124 relative to the start of P3_hfq transcription. Since quantitative gel mobility shift assays using native CsrA or C-terminal His-tagged CsrA (CsrA-H6) did not show any significant difference in binding affinities for target transcripts (data not shown), CsrA-H6 was used in all in vitro assays and is referred to as CsrA from here on. CsrA bound to this hfq transcript as a distinct band in native gels between 4 and 512 nM CsrA (Fig. 2A). A complete shift was observed at 128 nM CsrA, and no additional shifted species of higher molecular weights were observed as the concentration of CsrA was increased further, suggesting that CsrA binds to a single site in the hfq leader transcript. A nonlinear least-squares analysis of these data yielded an estimated K_d value of 38 ± 13 nM CsrA (mean ± standard deviation). For comparison, the affinities of CsrA for glgC (four CsrA binding sites), cstA (four CsrA binding sites), and pgaA (six CsrA binding sites) were 39 nM, 40 nM, and 22 nM, respectively (2, 11, 42).

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FIG. 2. Gel mobility shift analysis of the CsrA-hfq RNA interaction. 5'-end-labeled hfq RNA was incubated with the concentration of CsrA shown at the bottom of each lane. Gel shift assays were performed in the absence (A) or presence (B) of various unlabeled competitor RNAs. The concentration of each competitor RNA is shown at the bottom of each lane in panel B. The positions of bound (B) and free (F) hfq RNA are shown at the left of each gel. (A) Determination of the equilibrium binding constant of the CsrA-hfq RNA interaction. The simple binding curve for these data is shown at the right. (B) Competition assay for the CsrA-hfq RNA interaction to establish binding specificity. Lanes corresponding to competition with specific (hfq and SELEX) and nonspecific (trpL) RNAs are indicated.

The specificity of the CsrA-hfq RNA interaction was investigated by performing competition experiments with specific (hfq leader and a SELEX-derived ligand) and nonspecific (Bacillus subtilis trp leader) unlabeled RNA competitors (Fig. 2B). Unlabeled hfq and SELEX transcripts were effective competitors, whereas the B. subtilis trp leader RNA (trpL) did not compete with the CsrA-hfq RNA interaction. These results establish that CsrA binds specifically to hfq RNA.

CsrA-hfq RNA footprint experiments were conducted to identify the position of bound CsrA in the hfq transcript. Single-strand-specific RNases were used as probes for these studies. As the concentration of CsrA was increased from 0 to 2 µM, protection of several nucleotides from RNase T₁ (G specific) and RNase T₂ (A preference) cleavage was observed (Fig. 3A). CsrA protected G49, G57, and G58 from RNase T₁ cleavage, as well as residues A51 through A61 from RNase T₂ cleavage. Importantly, the entire sequence overlapping the hfq SD sequence identified in silico was protected from RNase cleavage. The composite footprint indicates that CsrA protects one RNA segment extending from G49 through A61 (Fig. 3B). Previous RNA structure mapping identified two stable RNA hairpins in the hfq transcript (h1 and h2) (41). The presence of these hairpins was confirmed; residues corresponding to h1 and h2 were protected from RNase cleavage in the absence of bound CsrA (Fig. 3). Bound CsrA also resulted in increased RNase T₂ cleavage of C20 and C42. These two residues are located within the 5' side bulge of h1 and just downstream of h1, respectively. CsrA-dependent protection was also observed for residues A76 (RNase T₂), G77 (RNase T₁), and G78 (RNase T₁). These residues are present within the stem of a predicted RNA hairpin containing a GNRA tetraloop (G, –4.0 kcal/mol) (22, 49). Thus, it appears that bound CsrA stabilizes this structure (Fig. 3).

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FIG. 3. CsrA-hfq RNA footprint analysis. (A) hfq RNA was treated with RNase T1 or RNase T2 in the absence or presence of CsrA. The concentration of CsrA used is indicated at the top of each lane. Partial alkaline hydrolysis (OH) and RNase T1 digestion (T1) ladders, as well as control (C) lanes in the absence of RNase treatment, are shown. The RNase T1 ladder was generated under denaturing conditions so that every G residue in the transcript could be visualized. Residues in which RNase cleavage was reduced (–) or enhanced (+) in the presence of CsrA are marked. The positions of the CsrA footprint (FP), the hfq SD sequence, and the translation initiation codon (AUG) are shown. Two RNA segments corresponding to RNA secondary structures (h1 and h2) that were previously identified are shown (41). Numbering at the left of each gel is from the start of hfq transcription. (B) Summary of the hfq footprint results (from panel A) and toeprint results (from Fig. 4, below). The composite CsrA footprint shows the residues in which cleavage was reduced (–) or enhanced (+) by the presence of bound CsrA. Residues corresponding to the CsrA-dependent and 30S ribosomal subunit (Rib) toeprints are marked with arrowheads. An additional 30S ribosomal subunit-dependent toeprint is marked (*). The positions of the hfq SD sequence and translation initiation codon (Met) are indicated. Inverted horizontal arrows identify the residues corresponding to h1, h2, and a short RNA hairpin containing a GNRA tetraloop. Vertical arrows identify a triple nucleotide substitution introduced into the CsrA binding site. Numbering is from the start of hfq transcription.

Bound CsrA inhibits translation initiation of hfq. Primer extension inhibition (toeprint) experiments were performed to determine whether CsrA was capable of competing with 30S ribosomal subunits for binding to the hfq transcript. The presence of bound CsrA or 30S ribosomal subunits should stop primer extension by reverse transcriptase, resulting in a toeprint band near the 3' boundary of the bound macromolecule. Stable secondary structures are also capable of inhibiting extension by reverse transcriptase, resulting in a toeprint band near the 3' end of the RNA hairpin. The toeprint results are presented in Fig. 4 and summarized in Fig. 3B. The presence of CsrA resulted in toeprints at positions A43, A82, and A91. The toeprint at A91 provides additional evidence for the hairpin containing the GNRA tetraloop, as this structure ends at A89 (Fig. 3B). The toeprint at A43 likely corresponds to the base of h1, as this RNA hairpin ends at G39. The origin of the A82 toeprint is unclear, as it is not near the 3' end of a stable hairpin and is 21 nt downstream from the 3' end of the CsrA footprint (Fig. 3 and 4). Since a toeprint corresponding to the 3' boundary of bound CsrA was not observed, it appears that reverse transcriptase is effective at displacing CsrA when bound to a single site.

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FIG. 4. CsrA and 30S ribosomal subunit toeprint analysis of hfq RNA. The concentration of CsrA used in each reaction mixture, as well as the absence (–) or presence (+) of tRNAfMet and 30S ribosomal subunits (30S Rib), is shown at the top of each lane. CsrA was added prior to 30S ribosomal subunits when both were present in the same reaction mixture. Arrows identify CsrA-dependent and 30S ribosomal subunit (Rib) toeprint bands. An additional 30S ribosomal subunit-dependent toeprint is marked (*). Positions of the hfq SD sequence and the translation initiation codon (AUG) are shown. The RNA segment corresponding to h1 is also shown. Sequencing lanes to reveal G, U, A, or C residues are marked. Numbering is from the start of hfq transcription.

Toeprint assays were also performed to identify the positions of bound 30S ribosomal subunits. A prominent tRNA^fMet-dependent 30S ribosomal subunit toeprint band was observed 15 nt down from the A of the AUG initiation codon, which is the same distance from the translation initiation codon as was previously observed for several mRNAs (2, 11, 42, 47). The second 30S ribosomal subunit-dependent toeprint at G72 was not expected, and its origin is unknown. Toeprint experiments were also carried out to determine whether bound CsrA could inhibit ribosome binding. Importantly, when CsrA was bound to the hfq transcript prior to the addition of 30S ribosomal subunits and tRNA^fMet, each of the CsrA-dependent toeprint bands was observed, whereas the 30S ribosomal subunit toeprint bands were eliminated (Fig. 3B and 4). Thus, our toeprinting results demonstrate that bound CsrA prevents ribosome binding to the hfq transcript, suggesting that CsrA could be capable of preventing translation initiation and Hfq synthesis.

Since our in vitro binding studies demonstrated that bound CsrA blocks ribosome binding, RNA-directed cell-free translation experiments were conducted to determine whether CsrA inhibits Hfq synthesis (Fig. 5). Our initial attempt to examine the effect of CsrA on Hfq synthesis was problematic, as we observed multiple bands, suggesting that hexameric Hfq was not completely denatured (data not shown). Because we previously found that using gfp translational fusions circumvented similar problems in cell-free translation experiments with B. subtilis S-30 extracts, an hfq'-'gfp translational fusion transcript was tested in the E. coli S-30 extract. In this case, well-behaved Hfq-Gfp fusion polypeptides were produced that migrated as a doublet. Importantly, addition of increasing concentrations of CsrA to the cell-free translation system led to a corresponding decrease in the Hfq-Gfp synthesis (Fig. 5). Similar cell-free translation experiments were carried out using smpB and bla transcripts as negative controls. The smpB transcript contained an SD sequence derived from pET28A⁺, whereas the bla transcript contained its natural SD sequence. Slight CsrA-dependent translation inhibition was observed for the negative controls, although the level of inhibition was far less than for Hfq-Gfp (Fig. 5). These results, in conjunction with the in vitro binding studies, demonstrate that CsrA inhibits translation initiation of hfq by blocking ribosome access to the hfq transcript.

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FIG. 5. Effect of CsrA and Hfq on in vitro translation of hfq'-'gfp mRNA. The E. coli S-30 extract was prepared from a CsrA-deficient strain. (A) Reactions were carried out with the concentration of CsrA indicated at the top of each lane in the absence (–) or presence (+) of hfq'-'gfp or control (smpB or bla) transcripts. Hfq-GFP, SmpB, and Bla translation products were analyzed by SDS-PAGE. (B) Relative levels of Hfq-GFP, SmpB, and Bla polypeptide synthesis as a function of CsrA concentration. All of the bands shown in panel A were used for quantifying the effect of CsrA on protein synthesis. The level of polypeptide synthesis in the absence of CsrA was set to 1.0 for each transcript. (C) Reactions were carried out with the concentration of CsrA and/or Hfq indicated at the top of each lane in the absence (–) or presence (+) of hfq'-'gfp transcripts. Hfq-GFP products were analyzed by SDS-PAGE. The relative level of polypeptide synthesis is shown at the bottom of each lane. The level of polypeptide synthesis in the absence of CsrA and Hfq was set to 100.

As Hfq was previously shown to repress its own translation (41), it was of interest to determine whether CsrA- and Hfq-mediated translation control is additive. Results from cell-free translation experiments confirmed that Hfq represses its own translation (Fig. 5C and data not shown). Moreover, an additive effect of CsrA and Hfq on translation inhibition was observed at protein concentrations of 0.8 µM (Fig. 5C). This latter result was somewhat surprising, as one of the Hfq binding sites overlaps the single CsrA binding site.

CsrA inhibits hfq expression. CsrA-dependent regulation of hfq was examined in vivo using an hfq'-'lacZ translational fusion whose expression was driven by P3_hfq (37). This fusion was integrated into the lambda att site of the E. coli chromosome in single copy, and expression was examined throughout the growth curve in both wild-type and csrA mutant backgrounds. When compared to the wild-type strain, a small but reproducible increase in expression (30%) was observed in the csrA mutant during stationary-phase growth (Fig. 6A). Expression was also examined when cells were grown in LB plus 1% glucose, because we previously found that expression of a cstA'-'lacZ fusion in wild-type and mutant strains differed to a greater extent under this glycolytic growth condition (11). A somewhat higher increase in expression (50%) was observed in the csrA mutant from the late exponential to the stationary phase of growth when cells were grown in LB plus 1% glucose (Fig. 6C). Introduction of csrA on a plasmid complemented the csrA mutant defect, resulting in a twofold reduction of hfq'-'lacZ expression beginning in late exponential phase (Fig. 6B).

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FIG. 6. CsrA-dependent regulation of an hfq'-'lacZ translational fusion. Cells were harvested at various times throughout growth and assayed for ß-galactosidase activity. Growth medium was LB (A and B) or LB supplemented with 1% glucose (C). Growth curves for each strain in panels A, B, and C were essentially identical. The time shown is hours of cell growth. These experiments were conducted at least three times with similar results. Results from representative experiments are shown. (A) ß-Galactosidase activity was determined for PLB785 (wild type [WT]) and PLB786 (csrA::kan). Cell growth was measured in strain PLB785. (B) ß-Galactosidase activity was determined for PLB793 (csrA::kan/pCRA16 [WT]) and PLB789 (csrA::kan/pBR322 [csrA]). Cell growth was measured in strain PLB789. (C) ß-Galactosidase activity was determined for PLB785 (WT, WT fusion), PLB786 (csrA::kan [csrA, WT fusion]), PLB923 (WT with mutant hfq'-'lacZ fusion), and PLB924 (csrA::kan [csrA] with mutant hfq'-'lacZ fusion). Cell growth was measured in strain PLB785.

We attempted to examine the influence of a mutant CsrA binding site on hfq expression. Because the critical GGA motif in this binding site is part of the hfq SD sequence, three CsrA binding site residues located just upstream from the hfq SD sequence were altered (A51T:T52G:A53C) (Fig. 3B). Expression from this mutant fusion was reduced 5-fold in both wild-type and csrA mutant strains (Fig. 6C), suggesting that sequence alterations this close to the SD sequence had deleterious effects on translation initiation. Furthermore, it is apparent that these substitutions did not eliminate CsrA-dependent inhibition of hfq expression, suggesting that a more substantial change to the CsrA binding site would be needed to prevent the CsrA-hfq RNA interaction. While the reason for reduced translation of the binding site mutant is not known, RNA secondary structure predictions using MFOLD (49) suggest that RNA structural rearrangements are not the cause.

Previous studies established that the mRNAs of several CsrA-repressed genes were stabilized in csrA mutant strains (1, 26). The steady-state level of hfq mRNA was determined by RT-qRT-PCR in wild-type and csrA mutant strains in the exponential and early stationary phases of growth. The relative abundance of hfq mRNA was 2-fold and 1.7-fold higher in the csrA mutant strain during exponential and early stationary phases of growth, respectively. The increased level of hfq mRNA in the csrA mutant strain could have been caused by increased transcription or a reduction in the mRNA decay rate. Results from mRNA half-life experiments indicated that CsrA does not affect the stability of hfq mRNA, suggesting that CsrA indirectly influences hfq transcription (Fig. 7). While the half-life of hfq mRNA was similar in wild-type and csrA mutant strains, we found that hfq transcripts were dramatically stabilized in the early stationary phase of growth (Fig. 7). Thus, it appears that mRNA stabilization contributes to increased hfq expression in stationary phase by a CsrA-independent mechanism.

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FIG. 7. Effects of growth phase and CsrA on hfq mRNA stability. hfq mRNA half-lives were determined in wild-type (WT) and csrA mutant strains during the exponential and early stationary phases of growth. The relative levels of mRNA remaining at 0, 1, 2, 4, 8, 15, and 32 min after the addition of rifampin were determined by RT-qRT-PCR. The mRNA level corresponding to each 0-min time point was set to 100. The mRNA half-life for each strain and growth phase is shown next to the corresponding symbol. Strains used were MG1655 (wild type) in exponential phase (WT-exp), TR1-MG1655 (csrA::kan) in exponential phase (csrA-exp), MG1655 in early stationary phase (WT-stat), and TR1-MG1655 in early stationary phase (csrA-stat).

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CsrA is a global regulatory RNA binding protein that represses or activates gene expression posttranscriptionally. Bound CsrA inhibits expression of several genes by binding to multiple sites within target transcripts, one of which overlaps the cognate SD sequence, thereby blocking ribosome binding. Inhibition of translation is thought to contribute to the observed accelerated rate of mRNA decay (1, 26). In the case of gene activation, bound CsrA can stabilize target transcripts, although the mechanism of message stabilization is not known (43). Two sRNA antagonists of CsrA, CsrB and CsrC, contain multiple CsrA binding sites and function by sequestering this protein (18, 45). Expression of csrA, csrB, and csrC increases as the culture approaches stationary phase (14, 45). The BarA/UvrY two-component signal transduction system activates transcription of csrB and csrC (36). Although the signal for this activation is not known, BarA signaling appears to be pH dependent (21). Interestingly, CsrA indirectly activates synthesis of both of the sRNAs via the response regulator UvrY, resulting in an autoregulatory circuit for CsrA, CsrB, and CsrC (36, 45). A fourth Csr component, the CsrD protein, was recently shown to be a specificity factor that targets CsrB and CsrC for degradation by RNase E (35). As CsrA acts downstream of transcriptional regulation and generally affects gene expression in the 1.5- to 10-fold range (11, 19, 27, 42, 43), it appears that CsrA functions in a fashion similar to a "governor" on a motor by reducing expression of some genes and increasing expression of others, rather than as an on-off switch.

A pwm search tool identified a potential CsrA binding site that overlaps the hfq SD sequence. The finding that this single site was similar to the SELEX-derived binding site consensus (Fig. 1) led us to investigate CsrA-dependent regulation of this gene. hfq is located in the amiB-mutL-miaA-hfq-hflX superoperon, which contains both E³²- and E⁷⁰-specific promoters (37, 38). Transcription of this operon is driven by at least five promoters during exponential growth (P_mutL, P_miaA, P1_hfq, P2_hfq, and P3_hfq). Our studies focused on the 68-nt mRNA leader originating from the SD sequence-proximal promoter, P3_hfq. Our gel shift (Fig. 2) and footprint (Fig. 3) results demonstrate that CsrA binds to the single site identified in silico. Moreover, the toeprint (Fig. 4) and cell-free translation (Fig. 7) results establish that bound CsrA inhibits Hfq synthesis by competitively blocking ribosome binding. While hfq mRNA contains only a single CsrA binding site, the affinity of the CsrA-hfq RNA interaction (K_d, 38 nM) is comparable to the affinity that CsrA has for mRNAs containing four to six binding sites (K_d, 22 to 40 nM). Despite the high affinity for hfq RNA, CsrA-mediated regulation was only 1.5- to 2-fold under our growth conditions (LB and LB plus glucose) (Fig. 5). This level of regulation is comparable to CsrA-dependent regulation of cstA expression in LB; however, regulation of cstA was 5-fold in LB plus glucose (11). Thus, it is possible that growth conditions for optimum CsrA-dependent regulation of hfq were not achieved.

The finding that translational repression did not alter the stability of hfq mRNA constitutes the first example in which CsrA-mediated translational repression did not lead to accelerated mRNA decay (Fig. 6). The observation that CsrA did not influence the stability of hfq mRNA, combined with the finding that the steady-state level of hfq transcripts was elevated in csrA mutant strains, suggests that CsrA has a negative effect on hfq transcription as well as translation. While CsrA caused only a small reduction in expression of the hfq'-'lacZ fusion used in this study, it is important to note that our fusion contained only one of five known hfq promoters, P3_hfq. Since it is reasonable to assume that CsrA is capable of repressing translation initiation of transcripts derived from any of the hfq promoters, it appears likely that CsrA indirectly represses transcription from (at least) one of the other hfq promoters. Thus, the in vivo effect of CsrA on translation, as determined by the hfq'-'lacZ reporter, and the apparent indirect effect of CsrA on hfq mRNA transcription, as determined by RT-qRT-PCR, likely contribute to the overall effect of CsrA on Hfq levels.

All previously characterized CsrA target mRNAs contain four or more CsrA binding sites (references 2, 11, 18, 42, and 45 and unpublished results). As CsrA is not a general repressor of translation, the finding that CsrA is capable of inhibiting translation of an mRNA containing a single CsrA binding site that overlaps its cognate SD sequence raises the question of how CsrA distinguishes one SD sequence from another. RNA secondary structure does not appear to be the only answer, as the majority of the known CsrA binding sites in mRNA targets, including the single binding site in hfq, do not contain their GGA motif in the loop of an RNA hairpin. Thus, additional conserved RNA sequence elements of binding sites must contribute to binding specificity.

Hfq is known to inhibit its own translation by binding to two sites within the hfq leader and initially translated region (41). Site A is located just upstream of the h1 hairpin, while binding site B overlaps its SD sequence (Fig. 3B). Both CsrA and Hfq are effective at inhibiting formation of a translation initiation complex. As Hfq-mediated autoregulation was reported to be about twofold, it is apparent that the level of CsrA-dependent and Hfq-dependent inhibition of hfq translation is similar. Moreover, it appears that CsrA-dependent and Hfq-dependent inhibition of Hfq synthesis is additive despite the fact that the CsrA binding site and Hfq binding site B overlap (Fig. 5C).

Additional studies further establish an interrelationship between CsrA and Hfq. A global analysis of protein-protein interactions in E. coli using Hfq as the "bait" protein identified a stable interaction with CsrA (6). The intracellular levels of Hfq hexamers and CsrA dimers were determined to be approximately 9,000 and 16,000 molecules, respectively (14, 39). The mRNA signal intensity from a transcription profile of cells grown in minimal medium showed that the relative hfq transcript level (11,884) was comparable to that of csrA (7,783) (8). An additional study reported that Hfq stabilized RsmY RNA, a CsrB homolog in Pseudomonas aeruginosa (33). Moreover, that study suggested that RsmA, a CsrA homolog, and Hfq could bind concurrently to RsmY, a known antagonist of RsmA.

Csr and homologous Rsm systems have been identified in a wide variety of bacterial species (1, 26). Depending on the particular organism, this global regulatory system controls a variety of cellular processes and behaviors (e.g., RpoS stress signaling, quorum sensing, biofilm development, motility and chemotaxis, central carbon flux, and pathogenesis). The finding that the Csr circuitry is interconnected with other global regulatory networks suggests that Csr governs cellular behavior and physiology on a scale that is not yet fully understood.

 
We thank Gisela Storz for Hfq, Ken Keiler for pETB, Emine Koc for technical assistance in the preparation of E. coli 30S ribosomal subunits, and Isaac Magaña for computer support.

This work was supported by Public Health Service grant GM59969 from the National Institutes of Health. Lél Eöry was supported in part by a fellowship from the Worldwide University Network.

 
* Corresponding author. Mailing address: Department of Biochemistry and Molecular Biology, The Pennsylvania State University, University Park, PA 16802. Phone: (814) 865-0002. Fax: (814) 863-7024. E-mail: pxb28{at}psu.edu

Published ahead of print on 25 May 2007.

Present address: Institute of Evolutionary Biology, School of Biological Sciences, University of Edinburgh, Edinburgh, United Kingdom.

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Journal of Bacteriology, August 2007, p. 5472-5481, Vol. 189, No. 15
0021-9193/07/$08.00+0     doi:10.1128/JB.00529-07
Copyright © 2007, American Society for Microbiology. All Rights Reserved.

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