In vitro roles of invariant helix-turn-helix motif residue R383 in {{sigma}}54 ({{sigma}}N)

doi:10.1093/nar/29.5.1163

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Nucleic Acids Research, 2001, Vol. 29, No. 5 1163-1174
© 2001 Oxford University Press

In vitro roles of invariant helix–turn–helix motif residue R383 in ${sigma}$ ⁵⁴ ( ${sigma}$ ^N)

Siva R. Wigneshweraraj, Akira Ishihama¹ and Martin Buck^*

Department of Biology, Imperial College of Science, Technology and Medicine, Sir Alexander Fleming Building, Imperial College Road, London SW7 2AZ, UK and ¹Department of Molecular Genetics, National Institute of Genetics, Mishima, Shizuoka 411, Japan

Received October 24, 2000; Revised and Accepted December 13, 2000.

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In vitro DNA-binding and transcription properties of ${sigma}$ ⁵⁴ proteinswith the invariant Arg383 in the putative helix–turn–helixmotif of the DNA-binding domain substituted by lysine or alanineare described. We show that R383 contributes to maintainingstable holoenzyme–promoter complexes in which limitedDNA opening downstream of the –12 GC element has occurred.Unlike wild-type ${sigma}$ ⁵⁴, holoenzymes assembled with the R383A orR383K mutants could not form activator-independent, heparin-stablecomplexes on heteroduplex Sinorhizobium meliloti nifH DNA mismatchednext to the GC. Using longer sequences of heteroduplex DNA,heparin-stable complexes formed with the R383K and, to a lesserextent, R383A mutant holoenzymes, but only when the activatorand a hydrolysable nucleotide was added and the DNA was openedto include the –1 site. Although R383 appears inessentialfor polymerase isomerisation, it makes a significant contributionto maintaining the holoenzyme in a stable complex when meltingis initiating next to the GC element. Strikingly, Cys383-tetheredFeBABE footprinting of promoter DNA strongly suggests that R383is not proximal to promoter DNA in the closed complex. Thisindicates that R383 is not part of the regulatory centre inthe ${sigma}$ ⁵⁴ holoenzyme, which includes the –12 promoter regionelements. R383 contributes to several properties, includingcore RNA polymerase binding and to the in vivo stability of ${sigma}$ ⁵⁴.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The promoter specificity of bacterial RNA polymerases (RNAP)is determined by the ${sigma}$ subunit present in the holoenzyme (E ${sigma}$ ).Two classes of ${sigma}$ factors, ${sigma}$ ⁷⁰ and ${sigma}$ ⁵⁴ ( ${sigma}$ ^N), have been identified.In marked contrast to the ${sigma}$ ⁷⁰ factor, ${sigma}$ ⁵⁴ associates with coreRNAP to form a holoenzyme that binds to promoter DNA forminga closed complex that rarely spontaneously isomerises to theopen complex. Conversion of the ${sigma}$ ⁵⁴ holoenzyme closed complexto a transcription-competent open complex is dependent upon ${gamma}$ –ß bond hydrolysis of nucleoside triphosphatesby activator proteins that bind DNA elements with enhancer-likeproperties. Activation is mediated by direct activator–closedcomplex interactions (1–6).

Promoter-specific DNA-binding activity of ${sigma}$ ⁵⁴ is central toformation of the E ${sigma}$ ⁵⁴–promoter complex. DNA binding by ${sigma}$ ⁵⁴ appears complex and the interaction between ${sigma}$ ⁵⁴ and DNA ismodulated by core RNAP (7,8). The promoter sequence recognisedby E ${sigma}$ ⁵⁴ is generally characterised by the presence of GG andGC doublets 24 and 12 bp, respectively, upstream of the transcriptioninitiation point (9). The specific DNA-binding determinantsof ${sigma}$ ⁵⁴ are located in the C-terminal Region III (residues 329–477in Klebsiella pneumoniae). Included are a putative helix–turn–helix(HTH) motif (residues 367–386) and a patch (residues 329–346)that UV cross-links to DNA, each located C-terminal to the coreRNAP-binding domain (residues 120–215) (10–15).

The N-terminal Region I has important regulatory roles in E ${sigma}$ ⁵⁴function, including effects on DNA binding (8,16,17). RegionI sequences also bind to core RNAP, an interaction suggestedto control properties of the holoenzyme important for activatorresponsiveness, but dispensable for core RNAP binding per se(7,10,13,18,19). The solvent accessibility of sequences withinthe DNA-binding domain of ${sigma}$ ⁵⁴ is changed in the holoenzyme whenRegion I is deleted, suggesting that Region I contributes tophysical properties of the holoenzyme, some of which involvesequences that are closely associated with the DNA-binding functionof ${sigma}$ ⁵⁴ (7). Holoenzymes formed with mutant or deleted RegionI ${sigma}$ ⁵⁴ function in activator-independent transcription, in whichthe promoter-bound E ${sigma}$ ⁵⁴ isomerises and produces transcripts viaan unstable open promoter complex (17,20,21–24). Mutantor deleted Region I ${sigma}$ ⁵⁴ proteins display changes in DNA-bindingactivity associated with recognition of the local DNA meltingthat occurs next to the consensus GC element upon closed complexformation (8,25,26). Proper recognition of this local DNA meltingdownstream to the GC is a hallmark for regulated transcriptioninitiation by E ${sigma}$ ⁵⁴ (8,10,15,26). The GC promoter region of ${sigma}$ ⁵⁴-dependentpromoters in known to be a key DNA element contributing to thenetwork of interactions that keep the polymerase in the closedcomplex and limit DNA opening prior to activation (8,22,27).Region I, the ${sigma}$ ⁵⁴ UV cross-linking patch and the –12 promoterregion form a centre in the holoenzyme that contains proteinand DNA determinants for activator responsiveness and DNA melting(15,17,22,27,28).

Region III residues 367–386 of ${sigma}$ ⁵⁴ are proposed to forma HTH DNA-binding structure. R383 in the recognition helix issuggested to interact with bases in the –12 promoter element,in particular with the consensus G of the GC promoter doublet(14). Substitution of R383 with any other amino acid exceptlysine and, to a lesser extent, histidine was suggested to resultin an inactive protein, implying that the nature of the chargeon this residue is important for ${sigma}$ ⁵⁴ function (14). The suppressionof –12 promoter-down mutations in the K.pneumoniae glnAp2promoter by R383K in vivo is considered as evidence for a rolefor R383 in recognition of the –12 promoter region. Anextension of these conclusions was that the promoter interactionwas direct, based largely on the idea that the suggested bi-helicalstructure would make specific contacts to promoter DNA and thatthe apparent suppression data might not be explained by indirecteffects (14).

Here we have explored the functionality of purified ${sigma}$ ⁵⁴ proteinsaltered at position 383 to determine if R383 is part of theregulatory centre in the ${sigma}$ ⁵⁴ holoenzyme. Results indicate thatR383 is not a part of the centre and that R383 may not establisha direct contact to DNA. Rather it seems that residue 346 ispart of the centre and is close to the GC promoter region. However,it is clear that R383 contributes to DNA binding and discriminationbetween bases at the G of the GC. It is also required for ${sigma}$ ⁵⁴stability in vivo. We show that R383 contributes to maintainingstable promoter complexes in which limited one base DNA openingdownstream of the –12 GC element has occurred. AlthoughR383 appears inessential for polymerase isomerisation, it appearsto make a significant contribution to maintaining the holoenzymein a stable complex when melting is initiating next to the GCelement.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Site-directed mutagenesis
Plasmids pSRW-R383K and pSRW-R383A expressing K.pneumoniae ${sigma}$ ⁵⁴as an N-terminal His₆-tagged protein with alanine or lysinesubstitution, respectively, at residue R383 were created usingthe Quickchange mutagenesis kit (Stratagene) as previously described(18). Briefly, pET28::rpoN (pMTH ${sigma}$ ^N) plasmid DNA (29) was usedas template with a large molar excess of complementary mutagenicprimers. Following mutagenesis PCR, DNA was transformed intoEscherichia coli strain XL2B and mutant clones were identifiedby sequencing. The BamHI–HindIII fragment carrying partof the C-terminal Region III of ${sigma}$ ⁵⁴ and harbouring the R383 mutationswas cloned into pMT1/306 (29). A cysteine-free ${sigma}$ ⁵⁴ [pSRW-Cys(–)]was created by changing the native cysteines at positions 198and 346 by site-directed mutagenesis using pMTH ${sigma}$ ^N as template.pSRW-Cys(–) was used to introduce a cysteine at positionR383 to generate pSRW-R383C (18).

Immunoblotting
Mutant plasmids pSRW-R383K and pSRW-R383K were transformed intoE.coli strain TH1 ( ${Delta}$ rpoN2518, endA1, thi1, hsdR17, supE44, ${Delta}$ lacU169),which has a deletion of chromosomal rpoN, and grown in LuriaBroth (LB) to an OD₆₀₀ of 1.0. Cells (1 ml) were collectedby centrifugation and resuspended in 100 µl of sterileH₂O. Aliquots of 20 µl of concentrated cells were lysedwith 20 µl of 2x SDS sample buffer, heated at 95°Cand 10 µl used for loading. Proteins were separated ondenaturing 7.5% SDS–PAGE mini-gels and blotted onto PVDFmembranes (0.2 µm pore size for western blotting; Millipore).Anti- ${sigma}$ ⁵⁴ (30) and alkaline phosphatase-conjugated anti-rabbitIgG (Promega) antibodies were used for detection (20).

Protein expression and purification
The R383A and R383K mutant ${sigma}$ ⁵⁴ proteins were overexpressed inE.coli strain BL21 (pLysS). Freshly transformed E.coli BL21(pLysS) cells (overnight growth) were used to inoculate ( $~$ 100–200c.f.u.) 1 l of 2x YT medium and grown at 37°C with 50 µg/mlkanamycin. The cultures were grown to an OD₆₀₀ of between 0.5and 0.7 and then induced with 1 mM IPTG at 25°C for 2 h.This temperature shift protocol increases the level of solubilityof ${sigma}$ ⁵⁴ (29) and improves stability of the R383A mutant, whichotherwise becomes severely proteolysed when overproduced athigher temperatures. The cells were collected by centrifugationand resuspended in cold 25 mM sodium phosphate (pH 7.0), 0.5M NaCl, 5% (v/v) glycerol and 1 mM PMSF and lysed in a Frenchpress. The lysate was centrifuged at 20 000 g for 30 min and>50% of R383K and $~$ 25% of R383A were found in the solublefraction. The N-terminal His-tagged mutant proteins were partiallypurified by Ni affinity chromatography using FPLC and elutedwith an imidazole gradient (29). Since R383K and, to a largerextent, R383A co-purified with a truncated form (implying proteolysisof R383K and R383A in the C-terminal domain), peak fractionsfrom the Ni affinity column were dialysed into TGED buffer (10mM Tris–HCl, pH 8.0, 50 mM NaCl, 0.1 mM EDTA, 1 mM DTTand 5% v/v glycerol) overnight at 4°C for further purification.The truncated fragments in the two protein preparations wereremoved by heparin and finally Mono Q chromatography essentiallyas previously described (13). Elution was achieved with a NaClgradient in both cases. Peak fractions from the Mono Q chromatographywere pooled and dialysed against TGED buffer and stored at –70(long-term storage) or –20°C (short-term storage).Cys383 protein was overexpressed and purified as previouslydescribed (18) using a Ni affinity column.

The activator proteins E.coli PspF ${Delta}$ HTH and K.pneumoniae NtrCwere overexpressed and purified as His₆-tagged fusion proteinsfrom pMJ15 (31) and pDW78 (provided by David Widdick and RayDixon). PspF ${Delta}$ HTH was stored at –70°C in TGED bufferwith 50% (v/v) glycerol and NtrC in TGED buffer with 10% glycerol(50 mM Tris–HCl, pH 8.0, 300 mM NaCl, 20 mM imidazoleand 10% v/v glycerol). Escherichia coli core RNAP was purchasedfrom Epicentre Technologies.

Assay for free sulfhydryl groups (CPM test)
A modified version of the method of Parvari et al. (32) wasused. Briefly, ß-mercaptoethanol standard solutionswere prepared in MOPS buffer (10 mM MOPS pH 8.0, 0.1 mM EDTAand 50 mM NaCl) at concentrations of 100, 50, 20, 10, 5, 1,0.5 and 0.1 µM. Cys383 was exchanged into MOPS bufferby dialysis at 4°C and protein concentration was determinedby Bradford assay. A 15 µl aliquot of 0.4 mM 7-diethylamino-3-[4'-maleimidylphenyl)-4-methylcoumarin(CPM) in dimethylformamide was added to 15 µl of eachstandard and each protein sample. After 1 h incubation at 37°Cthe reaction was stopped by adding 3 ml of 1% (v/v) Triton X-100.The intensity of fluorescence emission was measured on 1 mlsamples, using a Perkin-Elmer 2000 fluorescence spectrophotometer.The excitation wavelength was 390 nm and the emission wavelengthwas 473 nm.

Core RNAP binding assays
These were performed essentially as previously described as10 µl reactions in Tris–NaCl buffer (40 mM Tris–HClpH 8.0, 10% v/v glycerol, 0.1 mM EDTA, 1 mM DTT and 100 mM NaCl)(29). Briefly, E.coli core RNAP (250 nM) and different amountsof mutant ${sigma}$ ⁵⁴ proteins were mixed together and incubated at 30°Cfor 10 min, followed by addition of glycerol–bromophenolblue loading dye. Aliquots of 10 µl of the samples wereloaded onto Bio-Rad native 4.5% polyacrylamide Mini-ProteanII gels and run at 50 V for 2 h at room temperature in Tris–glycinebuffer (25 mM Tris and 200 mM glycine). Complexes were visualisedby Coomassie blue staining of the gels.

Gel mobility shift assays
³²P-end-labelled, fully complementary 88 bp homoduplex or heteroduplexfragments mismatched at positions –12, –12 to –11,–12 to –6, –12 to –1, –5 to –10and –10 to –1 (heteroduplexes 1–6, respectively,consisting of the –60 to +28 S.meliloti nifH promotersequence; Table 2) were formed as described (15) and used asprobes. Escherichia coli glnHp2 promoter fragments were obtainedby PCR using pFC50 (33) and pFC50-m12 as templates with primersFC5 and FC6 (34). The promoter fragments were gel purified andend-labelled with ³²P. A typical ${sigma}$ ⁵⁴ or E ${sigma}$ ⁵⁴ (formed with ${sigma}$ ⁵⁴ ata 2-fold molar excess over core RNAP) binding assay contained16 nM DNA and ${sigma}$ ⁵⁴ or E ${sigma}$ ⁵⁴ (concentrations as indicated in figuresor corresponding legends) in STA buffer (25 mM Tris–acetatepH 8.0, 8 mM magnesium acetate, 10 mM KCl, 1 mM DTT and 3.5%w/v PEG 6000) and incubated for 10 min at 30°C. For activation,4 µM PspF ${Delta}$ HTH activator protein and 4 mM dGTP were used.Briefly, core RNAP, ${sigma}$ ⁵⁴ and DNA were pre-incubated at 30°Cfor 10 min and then nucleotide and activator were added for10 min and, if required, heparin (final concentration 100 µg/ml)for a further 5 min prior to gel loading. Samples were thenloaded onto native 4.5% polyacrylamide gels and run at 60 Vfor 80 min (for the E.coli glnHp2 promoter fragments 60 V for150 min) at room temperature in Tris–glycine buffer. DNA–proteincomplexes were detected and quantified by phosphorimager analysis.

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Table 2. The S.meliloti nifH and E.coli glnHp2 DNA fragments used for the gel mobility shift assays

The S.meliloti nifH and E.coli glnHp2-13T $->$ G (–12) heteroduplex promoter DNA fragments (from –60 to +28) used for the gel mobility shift assays. Shown are sequences from –26 to +3, where the ${sigma}$ ⁵⁴ consensus promoter sequences are in bold and mutant sequences introduced in the top strand to create the mismatch are boxed in black (16,27).

In vitro transcription assays
The template for transcription assays was either the supercoiledplasmid pMKC28 carrying the S.meliloti nifH promoter in pTE103(35,36) or pFC50 containing the E.coli glnHp2 promoter and itsmutant derivatives (33) harbouring –13 GC element mutations(Table 1): –13T $->$ G (pFC50-m12), –13T $->$ C (pFC50-m33)and –13T $->$ A (pFC50-m11) (the nucleotide numbering systemused here is based on E.coli glnHp2 and differs from that usedfor S.meliloti nifH due to minor variations in the locationof the transcription start site; Table 1). The transcriptionassays were performed in STA buffer as previously outlined (35),except that 30 nM E ${sigma}$ ⁵⁴ (30 nM core RNAP:120 nM ${sigma}$ ⁵⁴) and 10 nMDNA was used. For activation, 4 µM PspF ${Delta}$ HTH or 100 nM NtrCwere added with 4 mM ATP (plus 10 mM carbamyl phosphate, usedfor NtrC phosphorylation). The reactions were incubated for20 min to allow open complexes to form. The remaining rNTPs(100 nM), 3 µCi [ ${alpha}$ -³²P]UTP and heparin (100 µg/ml)were added and incubated for a further 20 min at 30°C. Thereactions were stopped with 4 µl of formamide loadingbuffer and 7 µl aliquots were loaded on 6% denaturingsequencing gels. The dried gel was analysed on a phosphorimager.

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Table 1. E ${sigma}$ ${chi}$ ${eta}$ ${varepsilon}$ ${rho}$ ${iota}$ ${chi}$ ${eta}$ ${iota}$ ${alpha}$ ${chi}$ o ${lambda}$ ${iota}$ ${gamma}$ ${lambda}$ ${nu}$ H ${pi}$ 2 and S.meliloti nifH promoter sequences.

DNA cleavage of the S.meliloti nifH promoter DNA
DNA cleavage was conducted essentially as previously described(28). Briefly, closed complexes were formed with 100 nM holoenzyme(ratio 1:2, core RNAP to FeBABE-modified ${sigma}$ ⁵⁴) and incubated at30°C for 10 min. Cleavage was initiated by rapid sequentialaddition of 2 mM sodium ascorbate (pH 7.0) and 1 mM hydrogenperoxide. Reactions were allowed to proceed at 30°C for10 min before quenching with 30 µl of stop buffer (0.1M thiourea and 100 µg/ml sonicated salmon sperm DNA) and80 µl of TE buffer (10 mM Tris–HCl pH 8.0, and 1mM EDTA pH 8.0). The stopped reactions were phenol/chloroformextracted, precipitated with ethanol and electrophoresed on10% denaturing urea–polyacrylamide gels. The cleavagesites were determined using end-labelled fragments of the S.melilotinifH promoter DNA.

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Expression and stability of the R383K and R383A ${sigma}$ ⁵⁴ mutant proteins
We constructed the ${sigma}$ ⁵⁴ mutants R383K and R383A to explore theiractivities in vitro. Denaturing gel analysis of whole cell extractsfrom induced E.coli BL21 (pLysS) cultures revealed proteolysisof the overexpressed R383A protein (Fig. 1A, lane 2). Incontrast, the R383K protein, harbouring the more conservativesubstitution, appeared to be more stable and migrated mainlyas a single band, as did the wild-type protein during denaturinggel electrophoresis (Fig. 1A, lane 4). Overexpression of theR383A protein in different E.coli backgrounds and altering overexpressionconditions (time and temperature) did not improve the stabilityof the R383A protein (data not shown). Since the truncated R383Aco-purified with full-length R383A protein during Ni affinitychromatography, R383A appears to be proteolysed in its C-terminaldomain. These observations indicate that R383 is structurallyimportant, not readily predicted from the suggestion that R383is solvent exposed (14). We therefore constructed the R383Cmutant protein in a cysteine-free ${sigma}$ ⁵⁴ background to measure solventaccessibility (18). The CPM reactivity of R383C in its nativestate showed that R383C is indeed solvent accessible. Furthermore,the R383C protein was more stable upon overexpression and moreactive in transcription in vitro than were R383A and R383K (18;data not shown). We therefore infer that R383 has a structuralrole related to the bulk of the side chain and that 383 is asurface accessible residue.

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Figure 1. Overexpression and in vivo stability of R383K and R383A mutant ${sigma}$ ⁵⁴ proteins. (A) Uninduced whole cell extracts from E.coli BL21 pLysS carrying pSRW-R383A (lane 1) and pSRW-R383K (lane 3). The arrow indicates expression of R383A (lane 2) and R383K (lane 4) in whole cell extracts after 2 h induction. The arrow with asterisk indicates the proteolysed R383A protein (lane 2). The marker (lane M) is BroadRange SDS-7L (Sigma). (B) Whole cell extracts from E.coli strain TH1 carrying pMTH ${sigma}$ (lane 1), pET28b⁺ (lane 2), pSRW-R383A (lane 3) or pSRW-R383K (lane 4) were probed with anti- ${sigma}$ ⁵⁴ antibodies. The arrow indicates ${sigma}$ ⁵⁴. The prestained marker M (lane M) is from BioRad (broad range) and lane S contains a partially purified sample of ${sigma}$ ⁵⁴.

Previous in vivo studies led to the conclusion that R383A isunable to initiate transcription from the E.coli glnAp2 promoter(14). The instability of R383A we observed (Fig. 1A) suggestedthat the apparant inactivity of the R383A protein could be dueto proteolytic cleavage in vivo rather than solely a functionaldefect caused by the mutation. We therefore conducted in vivopromoter activation assays (ß-galactosidase promoterfusion assays) and western blots with the R383A protein. Leakyexpression of rpoN in pET28b+ allows use of the overexpressionplasmid in these assays (20). Consistent with the previous invivo results (14), the R383A mutant did not support activationin vivo (data not shown). Analysis of whole cell extracts containingpSRW-R383A prepared from E.coli TH1 cells under activating conditionswith anti- ${sigma}$ ⁵⁴ polyclonal antibodies failed to detect full-lengthR383A ${sigma}$ ⁵⁴ protein (Fig. 1B, lane 3); wild-type and R383K proteinswere detected (Fig. 1B, lanes 1 and 4). It appears that theactivity of R383A may not be easily judged by in vivo activityassays. We therefore conducted a series of in vitro assays toexplore the activity of the R383A and R383K mutants.

Interaction of R383K and R383A with the E.coli core RNAP
Native gel holoenzyme assembly assays were used to detect complexesforming between core RNAP and ${sigma}$ ⁵⁴ based on the different mobilitiesof core versus holoenzyme. Results showed that R383K has a slightlyreduced affinity for core RNAP (Fig. 2). In contrast, R383Ahad a significantly reduced affinity and, compared to wild-type ${sigma}$ ⁵⁴, forms a holoenzyme with an increased mobility on nativegels. The R383A protein did not produce a characteristic ${sigma}$ ⁵⁴band but was diffuse and slower running (Fig. 2, lane 16), incontrast to the R383K and wild-type proteins (Fig. 2, lanes14 and 15). Previously we showed, using Cys383-tethered FeBABEfootprinting methods, that R383 is not proximal to the coresubunits ß and ß' (18). We conclude thatchanging the invariant R383 to A results in a conformationalchange that may not be localised and which results in significantchanges in core RNAP binding and in formation of holoenzymewith a different conformation. These observations further supporta structural role for R383.

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Figure 2. Binding of ${sigma}$ ⁵⁴ to E.coli core RNAP. Native gel holoenzyme assembly assays were used to detect complexes forming between core RNAP and R383K and R383A, respectively. The formation of holoenzyme (E ${sigma}$ ⁵⁴) was detected as the presence of a faster migrating species when compared with core (E, lane 1) alone. Titrations of core RNAP with ${sigma}$ ⁵⁴ were carried out using 250 nM core RNAP and increasing concentrations of ${sigma}$ ⁵⁴ at ratios of 1:1 (lanes 2, 5 and 10), 1:2 (lanes 3, 6 and 11), 1:4 (lanes 4, 7 and 12) and 1:8 (lanes 8 and 13). Wild-type ${sigma}$ ⁵⁴ shifted nearly all the core into the holoenzyme form at a 1:1 molar ratio of core to ${sigma}$ ⁵⁴ (lane 2); in contrast, R383K shifted all the core to the holoenzyme form at a ratio of 1:2 (lane 6) and R383A at 1:4 (lane 12). Free ${sigma}$ ⁵⁴ (2.5 µM) proteins are also shown: lane 14, wild-type; lane 15, R383K; lane 16, R383A.

DNA-binding activities of the R383K and R383A mutant ${sigma}$ ⁵⁴ proteins and their holoenzymes
The R383K mutant was suggested to show an altered DNA-bindingpreference for the promoter GC element (14). Using a gel mobilityshift assay we compared the DNA-binding activities of the R383A,R383K and wild-type ${sigma}$ ⁵⁴ proteins and their holoenzymes for E.coliglnHp2 (termed Hp2-13T) and a mutant derivative with a T $->$ G substitutionat position –13 (termed Hp2-13T $->$ G) (Fig. 3A and B, respectively).The glnHp2 promoter is very close in sequence to the K.pneumoniaeglnAp2 promoter used in previous in vivo work with R383 mutants(14; Table 1). Previous in vivo and in vitro studies have shownthat the glnHp2 promoter with a G at –13 is a better substratefor ${sigma}$ ⁵⁴ holoenzyme function than one with a T at –13 (33).Binding of ${sigma}$ ⁵⁴ confirmed the promoter with a G at position –13(Hp2-13T $->$ G) as the preferred template, to which ${sigma}$ ⁵⁴ had 7-foldincreased binding (at 250 nM) compared to the Hp2-13T promoter.The R383K mutant bound both promoter sequences similarly, buthad a 7- to 8-fold reduced overall binding (at 1 µM)to the Hp2-13T and Hp2-13T $->$ G templates compared to wild-type ${sigma}$ ⁵⁴ (Fig. 3A). This observation, together with the inabilityof R383A to detectably bind either promoter probe even at higherprotein concentrations (1.5 and 2 µM; Fig. 3A) establishesthat R383 is important for DNA binding by ${sigma}$ ⁵⁴.

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Figure 3. Interactions of R383K and R383A with E.coli glnHp2 and S.meliloti nifH promoter fragments. Gel mobility shift assays were used to detect the binding activities of the ${sigma}$ mutants and their holoenzymes to E.coli glnHp2 promoter fragments. Binding of (A) wild-type ${sigma}$ ⁵⁴ (closed circles), R383K (closed squares) and R383A (closed diamonds) and (B) their holoenzymes to Hp2-13T (closed symbols) and Hp2-13T $->$ G (open symbols). Binding of (C) wild-type ${sigma}$ ⁵⁴ (open circles), R383K (open squares) and R383A (open diamonds) and (D) their holoenzymes [as in (C), but with closed symbols] to the S.meliloti nifH promoter fragment.

By comparing the binding activities of the wild-type, R383Aand R383K holoenzymes for the two promoter probes we determinedthat the wild-type holoenzyme (at 100 nM) had a 4- to 5-foldhigher binding to the Hp2-13T $->$ G than the Hp2-13T promoter sequence(Fig. 3B). The biphasic nature of the graph in Figure 3B (wild-typeholoenzyme binding to Hp2-13T $->$ G) probably reflects the complexbinding mode of ${sigma}$ ⁵⁴ holoenzyme to DNA. Like R383K ${sigma}$ ⁵⁴, the R383Kholoenzyme showed a similar binding preference to both promoterprobes, being unable to distinguish between them (Fig. 3B).Clearly, ${sigma}$ ⁵⁴–core RNAP interactions are significant indetermining promoter binding (compare Fig. 3A and B) and itseems that ${sigma}$ ⁵⁴ dominates the promoter binding preference. Anybinding preferences of the R383A holoenzyme for Hp2-13TandHp2-13T $->$ G could not be determined due to low binding of the R383Aholoenzyme to both probes (data not shown). Overall, our datashow that R383K and its holoenzyme bind the Hp2-13T $->$ G and Hp2-13Ttemplates equally. In contrast, wild-type ${sigma}$ ⁵⁴ and its holoenzymebind to the Hp2-13T $->$ G probe better than to the Hp2-13T probe.R383 is significant for DNA binding by ${sigma}$ ⁵⁴ and is needed forpreferential binding to –13G rather than the –13Tprobe.

To further explore the DNA-binding properties of the mutant ${sigma}$ ⁵⁴ proteins and their holoenzymes we compared the binding activitiesof R383K and R383A to S.meliloti nifH promoter DNA, a higheraffinity binding site used for many ${sigma}$ ⁵⁴ activity measurements(see below). As shown (Fig. 3C), R383K bound less S.melilotinifH probe (3-fold reduced) compared to wild-type ${sigma}$ ⁵⁴. In contrast,the R383A mutant appeared defective for DNA binding. Next, holoenzymebinding to the S.meliloti nifH promoter was assayed using saturatingratios of ${sigma}$ to core RNAP. The wild-type holoenzyme shifted 70%of the S.meliloti nifH promoter probe DNA at 150 nM, whereasmutant holoenzymes shifted 60 (R383K) and 45% (R383A) of theprobe (Fig. 3D). This observation contrasts with the behaviourof the R383A holoenzyme on Hp2-13T $->$ G and suggests that sequencesin the S.meliloti nifH promoter rescue promoter binding by R383Aholoenzyme.

In vitro transcription activity of the R383K and R383A holoenzymes
To begin to examine the consequences of altered DNA bindingby R383K and R383A upon later steps in activation, we next examinedthe ability of the R383K and R383A holoenzymes to support transcriptionin vitro from supercoiled plasmid pFC50, which contains thewild-type E.coli glnHp2 promoter or GC promoter region mutantderivatives of this promoter (Table 1). Changing –13Tto a C (pFC50-m33) or A (pFC50-m11) results in a strong promoter-downphenotype or a largely inactive mutant promoter, respectively(33).

Initially, the response of wild-type and mutant holoenzymesto saturating concentrations of the E.coli activator proteinPspF ${Delta}$ HTH, which functions in solution, was tested. The abilityof the holoenzymes to promote transcription at glnHp2-13T, glnHp2-13T $->$ Gand glnHp2-13T $->$ C was expressed as a percentage of wild-type holoenzymeactivity at the glnHp2-13T $->$ G promoter (Fig. 4A). Assays wereconducted with sub-saturating amounts of holoenzyme to allowquantitative detection of holoenzyme activities (see Materialsand Methods). Experiments were performed at least six timesto enhance reliability. The standard error range for the datashown in Figure 4A and B was ±4%. The results clearlyshow that the R383A holoenzyme is active and able to supporttranscription in vitro (40–50% of wild-type activity onthe glnHp2-13T $->$ G promoter; Fig. 4A). Transcription by R383A isapparently greater than promoter DNA binding by the holoenzyme(Fig. 3B). Formation of stable open complexes that do not rapidlydecay to heparin-sensitive closed complexes could explain this.

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Figure 4. In vitro activator-dependent transcription assays on E.coli glnHp2 wild-type and mutant promoter sequences. The sequences of the promoters used for transcription are as shown in Table 1. (A) PspF ${Delta}$ HTH-activated transcription and (B) NtrC-activated transcription on glnHp2-13T $->$ G (pFC50-m12) (black bars), glnHp2-13T (pFC50) (grey bars) and glnHp2-13T $->$ C (pFC50-m33) (white bars). The transcription activities are expressed as a percentage of wild-type activity at the glnHp2-13T $->$ G (pFC50-m12) promoter.

The R383K holoenzyme was 20 ± 4% less efficient in transcriptionthan the wild-type holoenzyme at all the promoters tested (Fig.4A). This result differs from the in vivo assays on K.pneumoniaeglnAp2 (Table 1), which showed that the R383K holoenzyme transcribedbetter from –13T or –13T $->$ C promoters than did wild-type ${sigma}$ ⁵⁴ (14). To explore the potential for suppression in vitro wevaried the assay conditions. We failed to see any significantR383K-specific suppression at the promoter-down mutant (glnHp2-13Tand glnHp2-13T $->$ C) sequences in the presence of nucleotides thatfacilitate formation of initiated complexes prior to heparinchallenge, at higher temperatures (37 instead of 30°C) usedto stimulate transient DNA melting, at different (10–8000nM) PspF ${Delta}$ HTH concentrations or with varying incubation times(5, 10, 20 and 30 min) before and after addition of heparin(data not shown).

The possibility that the suppression of promoter-down K.pneumoniaeglnAp2 mutants by R383K seen in vivo could be either activator-specificor require an enhancer-bound activator was considered. We usedNtrC instead of PspF ${Delta}$ HTH and examined in vitro transcriptionactivity of the wild-type and mutant holoenzymes at the glnHp2promoters. The results showed that when activated by NtrC, theR383K holoenzyme transcribed from the glnHp2-13T and glnHp2-13T $->$ Gpromoters at levels consistent with our observation using glnHp2-13T $->$ Gand PspF ${Delta}$ HTH (compare Fig. 4A and B). In contrast to the PspF ${Delta}$ HTHresults, a much lower activity of R383A holoenzyme at the glnHp2-13T $->$ Gor no detectable activity at the glnHp2-13T and glnHp2-13T $->$ Cpromoters, even at higher holoenzyme and NtrC concentrations(data not shown), was evident. This could be linked to an alteredholoenzyme conformation (Fig. 2) and reduced DNA binding bythe R383A holoenzyme (Fig. 3B).

In conclusion, our in vitro transcription results do not showthe suppression of promoter-down phenotypes of the E.coli glnHp2promoter by R383K holoenzyme reported for in vivo K.pneumoniaeglnAp2 promoter assays (14). The in vitro activities of theR383K and R383A holoenzymes argue that R383, at least in vitro,is not absolutely required for productive transcription initiationby E ${sigma}$ ⁵⁴. It seems that R383 is not needed to allow preferentialinitiation of transcription in which the –13 base is Grather than T (Fig. 4).

Activator-independent transcription activity of the R383K and R383A holoenzymes
Maintaining the transcriptionally silent state of E ${sigma}$ ⁵⁴ in closedcomplexes depends upon the interaction of ${sigma}$ ⁵⁴ with locally distortedpromoter DNA downstream of the consensus –12 GC promoterelement (10,26,27). ${sigma}$ ⁵⁴ proteins defective in recognition ofthe –12 GC promoter element proximal DNA distortion arecapable of increased activator-independent transcription in vitro,so called bypass transcription (8,20,25). We used the in vitrobypass assay to see whether holoenzymes formed with R383K andR383A were active in unregulated transcription from the glnHp2-13T $->$ Gpromoter. We used R336A mutant ${sigma}$ ⁵⁴ as a positive control forthe bypass transcription assay (35) and PspF ${Delta}$ HTH for activator-dependenttranscript formation. As shown, no bypass transcription wasobserved with R383K or R383A (Fig. 5). Additional assays fromglnHp2-13 variants (33) or pMKC28 carrying the S.meliloti nifHpromoter (33) failed to give unregulated transcription withthe R383 mutants (data not shown). The failure to detect bypasstranscription with R383K and R383A suggests tight binding ofthese mutant ${sigma}$ ⁵⁴ proteins to the early melted DNA formed in closedcomplexes, as seen in heteroduplex DNA-binding assays (25,27).Bypass transcription correlates with strong defects in the bindingof ${sigma}$ ⁵⁴ to early melted DNA, a defect that is only weakly evidentwith the R383 mutants (see below). Thus we infer that the R383Aand R383K mutants appear functionally intact in the generationand maintenance of locally melted –12 proximal promoterstructures associated with the closed complex (8,25). Further,chemical footprinting with copper o-phenanthroline of closedcomplexes formed with R383 mutant holoenzymes revealed a localdistortion of promoter DNA 3' adjacent to the GC element, asseen with the wild-type holoenzyme but not in bypass mutants(26,35; data not shown). Overall, R383 is neither directly norindirectly associated with inhibition of unregulated bypasstranscription in vitro. By inference, R383 does not closelyinteract with the elements of the –12 promoter regionthat are involved in maintaining the stable conformation ofthe closed complex and in limiting DNA opening prior to activation.

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Figure 5. In vitro activator-independent transcription assays on the E.coli glnHp2-13T $->$ G (pFC50-m12) promoter. Activator-dependent (lanes 1–3) and activator-independent ‘bypass’ transcription (lanes 5–7) for wild-type ${sigma}$ ⁵⁴, R383K and R383A, respectively, are shown. The R336A mutant ${sigma}$ ⁵⁴ (35) was used as the positive control in both cases (lane 4 for activator-dependent and lane 8 for activator-independent reactions).

Interaction of R383K and R383A mutant proteins and their holoenzymes with heteroduplex S.meliloti nifH promoter DNA probes
In the course of the in vitro transcription experiments we observedthat the R383K and R383A holoenzymes were essentially inactivefor transcription at the S.meliloti nifH promoter even thoughpromoter binding was sufficiently efficient to expect transcripts(Fig. 3D and data not shown, respectively). The transcriptionalinactivity of the mutant proteins at the nifH promoter but notat the glnHp2-13T $->$ G promoter with essentially the same –12region sequences (Table 1) prompted us to further explore theproperties of the R383K and R383A mutant proteins. Sinorhizobiummeliloti nifH (from –11 to –1) is rich in G andC residues, whereas E.coli glnHp2, like the K.pneumoniae glnAp2promoter used in the in vivo assays, is AT-rich in this region,which is melted in open complexes (Table 1). This led us toconsider that the R383K and R383A mutant holoenzymes might bedefective in some aspect of DNA melting or single-stranded DNAbinding at the S.meliloti nifH promoter. We used heteroduplexDNA that mimics the DNA at different stages of open complexformation to test this idea (Table 2). In marked contrast tothe failure to transcribe from the S.meliloti nifH promoter(data not shown), both the R383K and R383A mutant holoenzymesgave heparin-stable, activator- and nucleotide hydrolysis-dependentcomplexes on promoters with a region of heteroduplex from –10to –1 (Table 2, heteroduplex 5) (Fig. 6A). On thisDNA structure the mismatched region includes the non-conservedsequence from –10 to –1 that interacts with ${sigma}$ ⁵⁴ withinthe closed complex (13) or with ${sigma}$ ⁵⁴ holoenzyme in the open promotercomplex (37–39). The ability of the wild-type, R383K andR383A holoenzymes to form activator- and nucleotide hydrolysis-dependent,heparin-stable complexes when bound to promoter DNA where thesequence from –10 to –1 is heteroduplex (Table 2,heteroduplex 5) argues that the R383K and R383A holoenzymesare not per se defective in polymerase isomerisation at thenifH promoter. Also, pre-opening from –10 to –1appears to allow a range of activities with R383K and R383Asimilar to that seen with the glnHp2 promoters in transcriptionassays. As expected from the in vitro activator-dependent transcriptionresults, the wild-type holoenzyme, like the R383K and R383Aholoenzymes, does not form heparin-stable, activator- and nucleotidehydrolysis-independent complexes on heteroduplex 5 (16; datanot shown).

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Figure 6. Binding of R383K and R383A to homo- and heteroduplex promoter DNA probes. (A) Activator- and nucleotide-dependent, heparin-resistant open complex formation on the S.meliloti nifH heteroduplex –10 to –1 (heteroduplex 5, Table 2) by wild-type ${sigma}$ ⁵⁴ (lane 1), R383K (lane 2) and R383A (lane 3) holoenzymes (100 nM). Black arrows indicate the position of the E ${sigma}$ ⁵⁴–DNA complex; white arrows the position of core RNAP complex. Reactions without (lanes 1–3) and with (lanes 4–6) heparin (100 µg/ml) challenge for 5 min prior to loading are shown. (B) Activator-dependent, heparin-resistant E ${sigma}$ ⁵⁴–DNA complex formation on heteroduplexes (heteroduplexes 1–6, Table 2). Percent DNA shifted with the wild-type ${sigma}$ ⁵⁴ (black bars), R383K (grey bars) and R383A (white bars) holoenzymes are shown. (C) Stability of wild-type and mutant E ${sigma}$ ⁵⁴–DNA complexes on S.meliloti nifH heteroduplex –12 to –1 (heteroduplex 4) under non-activating and activating conditions in the presence and absence of heparin (100 µg/ml), respectively (lanes as indicated on figure). The slower running band in the lanes containing E ${sigma}$ ⁵⁴ is a heparin-unstable complex of E ${sigma}$ ⁵⁴ with DNA (15,35,40). (D) DNA-binding activities of R383K (grey bars) and R383A (white bars) to homo- and heteroduplex DNA (see Table 2) expressed as a fraction of wild-type ${sigma}$ ⁵⁴ (black bars) binding. (E) As (D) but for holoenzymes. (F) Activator- and nucleotide hydrolysis-independent, heparin-stable E ${sigma}$ ⁵⁴–DNA complex formation on E.coli glnHp2-13T $->$ G(–12) (see Table 2). Reactions without (lanes 1–3) and with (lanes 4–6) heparin challenge are shown. Lanes 1 and 4, wild-type ${sigma}$ ⁵⁴; lanes 2 and 5, R383K; lanes 3 and 6, R383A.

Heteroduplex with early melted sequences. Next we examined whetherthe R383A and R383K mutants were defective in interacting withDNA structures representing the early stages of DNA melting.We used heteroduplex promoter DNA fragments unpaired at –12(Table 2, heteroduplex 1) and at –12/–11 (Table2, heteroduplex 2) to mimic the structure believed to be involvedin initial DNA opening (25,27). These heteroduplexes allow thewild-type holoenzyme to form complexes that survive a heparinchallenge independently of activator and nucleotide hydrolysis(25). As shown (Fig. 6B), we were unable to form heparin-stablecomplexes with the R383K and R383A holoenzymes on either ofthe heteroduplexes, even under activating conditions. This defectcorrelates with the inability of the R383 mutants to transcribefrom the nifH promoter. However, when using heteroduplex promoterDNA where the sequences from –12 to –6 (Table 2,heteroduplex 3) and –12 to –1 (Table 2, heteroduplex4) were unpaired, the R383K and R383A holoenzymes survived theheparin challenge, but only with activator and nucleotide hydrolysis(compare Fig. 6B and C). In contrast, the wild-type holoenzymeformed heparin-stable complexes on heteroduplex 4 in the absenceof activator and nucleotide, as predicted from the results withheteroduplexes 1 and 2, opened at –12 (Table 2, heteroduplex1) and from –12 to –11 (Table 2, heteroduplex 2)(16,25,27,40). Although non-native structures near –12have the property of allowing the wild-type holoenzyme to formheparin-stable complexes independently of activation, the R383Kand R383A holoenzymes formed heparin-stable and activator- andnucleotide hydrolysis-dependent complexes with promoter probescontaining –12 proximal melts (Table 2, heteroduplexes1 and 2) only when these heteroduplexes included further regionsof heteroduplex proximal to the start site (Table 2, heteroduplexes3 and 4). These results show that R383 specifies an interactionin the closed complex associated with stable complex formationby the holoenzyme when the –12 proximal sequences aremelted. Other interactions required to acquire heparin-stablecomplex formation involving late melted sequences appear intactin the R383K and R383A mutants.

DNA-binding activities on heteroduplexes. Next, we measuredthe DNA-binding activities of the mutant proteins (Fig. 6D)and their holoenzymes (Fig. 6E) on S.meliloti nifH heteroduplexDNA with –12 promoter element proximal melts (Table 2,heteroduplexes 1 and 2), start site proximal melts (Table 2,heteroduplexes 3 and 4) and on heteroduplexes with mismatchesbetween –10 and –1 (Table 2, heteroduplex 5) and–5 to –1 (Table 2, heteroduplex 6). Results areshown relative to binding of wild-type ${sigma}$ ⁵⁴ and its holoenzymeto S.meliloti nifH homoduplex DNA. It is evident that R383Kand, especially, its holoenzyme bound more (2- to 3-fold) ofthe heteroduplex DNA probes which contain start site proximalmelts, whilst wild-type ${sigma}$ ⁵⁴ and its holoenzyme prefer heteroduplexDNA with –12 proximal melts. Since certain Region I mutantsof ${sigma}$ ⁵⁴ have defects in binding to early melted DNA structures(8,25,27), the DNA-binding properties of R383 mutants (Fig.6) may reflect indirect effects upon the function of RegionI (28).

The results (Fig. 6) clearly imply a role for R383 in interactionswithin the closed complexes in which limited DNA opening nextto the –12 element has occurred. To further explore thisidea we used the E.coli glnHp2-13T $->$ G promoter mismatched at position–11 (i.e. glnHp2-13T $->$ G equivalent to heteroduplex 1; Table2). R383K had 80% of wild-type transcription activity on thispromoter in vitro. As shown (Fig. 6F), whilst the wild-typeholoenzyme was able to form activator- and nucleotide hydrolysis-independent,heparin-stable complexes on the glnHp2 heteroduplex, the R383Kholoenzyme did not. Activation enabled the R383K and, to a lesserextent, R383A holoenzymes to form some heparin-stable complexes(<10% DNA shifted) on this heteroduplex (data not shown).The ease of opening of the glnHp2 AT-rich sequence (from –11to –1) may explain why the activator allows acquisitionof heparin stability, and also why a longer segment of heteroduplexis needed at nifH. Therefore, binding assays with two different ${sigma}$ ⁵⁴-dependent promoters are consistent with the view that R383has a role in interactions within the initial closed complexesin which limited DNA opening next to the –12 element hasoccurred. Unless DNA opening occurs easily, the defects associatedwith R383 dominate and few open complexes form.

Proximity of residue 383 to promoter DNA
To examine the physical proximity of R383 to promoter DNA weconstructed a ${sigma}$ ⁵⁴ with FeBABE located at 383. A single cysteinesubstitution at 383 was made, the naturally occurring cysteinesof K.pneumoniae ${sigma}$ ⁵⁴ at 198 and 346 having been replaced by alanineto allow 383-specific conjugation of FeBABE. DNA cleavage bytethered FeBABE is achieved through the generation of hydroxylradicals coordinated to the Fe²⁺, which attack the deoxyribose–sugarbackbone of nucleic acids within a radius of 12 Å fromthe FeBABE attachment site (reviewed in 41). Using the S.melilotinifH homoduplex DNA probe the DNA-binding activity of the R383Cmutant was 90% that of the wild-type and Cys-free ${sigma}$ ⁵⁴ activity(data not shown). Upon conjugation with FeBABE (76% efficiency)the DNA-binding activity remained largely unchanged. This suggeststhat even a relatively bulky substituent at 383 is toleratedfor DNA binding, consistent with R383 being dispensable forDNA binding (this paper) and non-essential for transcription(this paper; 18). ${sigma}$ ⁵⁴ containing Cys383-tethered FeBABE failedto produce detectable cutting of several different S.melilotinifH promoter templates (homoduplex and heteroduplexes 2 and5), both in the presence and absence of core RNAP and underactivating conditions that allow open complex formation (seebelow and data not shown). We considered the possibility that ${sigma}$ ⁵⁴ containing Cys383-tethered FeBABE and its holoenzyme mighthave dissociated from the promoter DNA under DNA cleavage conditions.However, binding assays conducted with the Cys383-tethered FeBABEprotein under DNA cleavage conditions showed that 91% of ${sigma}$ ⁵⁴containing Cys383-tethered FeBABE and 48% of holoenzyme containingCys383-tethered FeBABE remained bound to DNA (Fig. 7A). Repeatedexperiments failed to show DNA cutting by ${sigma}$ ⁵⁴ containing Cys383-tetheredFeBABE and its holoenzyme. As one positive control ${sigma}$ ⁵⁴ with FeBABEconjugated to Cys346, at the edge of the DNA cross-linking patchof ${sigma}$ ⁵⁴, produced cutting proximal to the GC element on S.melilotinifH homoduplex promoter DNA (Fig. 7B). The putative HTH motifin ${sigma}$ ⁵⁴ is C-terminal to a patch of amino acids that UV cross-linksto promoter DNA. In this patch FeBABE conjugated to residue336 cut DNA downstream of the conserved GC promoter element(28). As shown in Figure 7B, holoenzyme containing Cys346-tetheredFeBABE strongly cut homoduplex promoter DNA between positions–14 and –7, mostly downstream of the GC element,but this cutting was upstream of that seen with the Cys336-tetheredFeBABE derivative (28). The C-terminal to N-terminal orientationof the cross-linking patch is therefore 5' $->$ 3' with respect tothe template strand of the promoter DNA.

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Figure 7. Sinorhizobium meliloti nifH promoter DNA template strand cleavage by RNAP holoenzyme containing FeBABE-modified ${sigma}$ ⁵⁴ proteins. (A) Cys383-FeBABE ${sigma}$ ⁵⁴ and E ${sigma}$ ⁵⁴ binding to the S.meliloti nifH homoduplex probe under DNA cleavage conditions (lanes as marked on figure). (B) Homoduplex cleavage. Reactions to which hydrogen peroxide and ascorbate were added to initiate DNA cleavage are marked +; control reactions to which no ascorbate and hydrogen peroxide were added are marked –. Lane M contains a mixture of end-labelled S.meliloti nifH promoter DNA fragments as molecular weight markers.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Specific recognition of promoter DNA by ${sigma}$ factors has an essentialrole in locating the RNAP at the correct site for initiation.However, the function of residues in ${sigma}$ ⁵⁴ that contact DNA arelikely to be more complex than just facilitating promoter location.Emerging functions associated with ${sigma}$ ⁵⁴–DNA binding includerecognition of the DNA fork junction created when the DNA startsto melt and keeping the polymerase silent for transcription(8,10,15,35). Protein footprints suggest that the DNA-bindingdomain of ${sigma}$ ⁵⁴ is part of the interface with core RNAP and propertiesof mutants indicate a role in generating polymerase isomerisationand facilitating promoter opening (7,27,35). Our results addressthe functions of invariant residue R383 of ${sigma}$ ⁵⁴, previously implicatedin interactions with the –12 promoter element (14).

Protein stability
R383 is clearly required for protein stability in vivo. Theinstability of R383A may be associated with an unfavourablechange in structure directly increasing its proteolytic sensitivity.Alternatively, the reduced DNA-binding activity of R383A mayindirectly increase proteolysis by changing the intracellularlocation of ${sigma}$ ⁵⁴. The suggestion from in vivo promoter activationassays that R383 is essential for ${sigma}$ ⁵⁴ function may be incorrect,as purified R383A does support transcription from the E.coliglnHp2 promoter in vitro.

Core RNAP binding
That part of ${sigma}$ ⁵⁴ strongly footprinted by the core RNAP is centredon residue 397 and in the absence of Region I ( ${Delta}$ I ${sigma}$ ⁵⁴) much ofthe 325–440 sequence is protected by core RNAP (7). R383Ahad reduced core RNAP binding and formed a holoenzyme with alteredmobility on native gels, suggesting that R383 contributes tocore RNAP binding. Possibly, the core interface of ${sigma}$ ⁵⁴ is alteredin the R383A mutant, potentially in a manner that involves RegionI sequences (7,18,19). Interestingly, Cys383-tethered FeBABEfootprinting of core RNAP failed to show any proximity of residue383 (within at least 12 Å) to the core subunits ßand ß' (18). Thus we suggest that the defects in coreRNAP binding by the R383 mutants are indirect. The R383K mutantwas less disrupted for core binding, consistent with the conservativenature of the mutation.

DNA binding
Gel mobility shift assays showed that R383A was very defectivein DNA binding, R383K less so. R383K did not preferentiallybind E.coli glnHp2-13T promoter DNA. R383K is reported to transcribemore efficiently than wild-type ${sigma}$ ⁵⁴ from a similar promoter sequence(mutant K.pneumoniae glnAp2) (14). Clearly, the increased transcriptionreported may not simply correlate with increased DNA bindingof ${sigma}$ ⁵⁴. R383K might therefore influence other steps to allowincreased transcription in vivo. The R383K holoenzyme did notfootprint the glnAp2-13G $->$ T promoter in vivo, but wild-type ${sigma}$ ⁵⁴did, consistent with the view (developed below) that promoteroccupancy may not be dominant for the increased transcriptionobserved (14). It was striking that the defects in in vitrotranscription at E.coli glnHp2 with the R383K and R383A mutantswere less than the defects in in vitro ${sigma}$ and holoenzyme DNA binding.We interpret this to mean that promoter occupancy is not reducedto a point that severely limits transcription in vitro. It isplausible that tight binding of the holoenzyme to the promoterincreases a transition barrier for open complex formation. TheR383K and R383A mutants may reduce this barrier, compensatingfor reduced promoter occupancy. This favourable effect mightcontribute to the elevated activities observed with R383K invivo and the good level of transcription detected in vitro.It may also partly compensate for the defect in forming stablecomplexes with early melted DNA (discussed below).

Interactions with heteroduplex DNA
Results from transcription assays with heteroduplexes suggestedthat slow opening of the DNA at the S.meliloti nifH promotermight mean that the closed complex or an activator-dependentisomerised holoenzyme formed with R383K dissociates prior tofull strand opening. In contrast, more frequent opening of theE.coli glnHp2 promoter or stable opening as in heteroduplexesmay explain why these templates support stable open complexformation with R383K. Even so, these complexes decay more rapidlythan those formed with wild-type ${sigma}$ ⁵⁴ (data not shown), suggestingthat R383 contributes to DNA binding within the open complex.However, R383 is not essential for transcription, at least invitro. Our ability to recover activator-dependent stable complexformation using pre-melted S.meliloti nifH DNA templates withheteroduplex –10 to –1 sequences suggests that themutant holoenzymes are limited at some promoters in steps leadingto full DNA melting. Compared to DNA templates with start siteproximal melts, DNA templates with melted sequences proximalto the –12 promoter element were poor DNA-binding sitesfor the R383K and R383A mutants. The failure of the R383A andR383K mutants to bind well or make stable complexes on the heteroduplexpromoter fragments with –12 proximal melts suggests thatthe R383 mutant proteins are directly or indirectly defectivefor interaction with such structures. With the mutant proteinsthe activator did not allow the use of heteroduplex promoterswith –12 proximal melts for efficient stable complex formationon either the S.meliloti nifH or E.coli glnHp2 promoters, butin the context of the S.meliloti nifH promoter the activatorallowed formation of stable complexes on promoter sequenceswhich were further opened to include the –1 residue. Overall,the results suggest that DNA melting from –10 to –1stabilises the promoter complexes that form with the R383K andR383A mutant holoenzymes and that the initial melting at –12is unfavourable for stable E ${sigma}$ ⁵⁴–DNA binding when R383 isaltered to A or K. Rapid melting at the AT-rich E.coli glnHp2may allow stable complexes to form, but slow melting at theGC-rich S.meliloti nifH may result in reduced stable complexformation.

Bypass transcription
Interaction of ${sigma}$ ⁵⁴ with the –12 GC promoter element appearsimportant in maintaining the transcriptionally silent stateof the holoenzyme. Mutations that change the sequences adjacentto the GC or substitution of certain amino acids in ${sigma}$ ⁵⁴ thatinteract with it allow transcription independent of activator(8,20,22,24,42). The ${sigma}$ ⁵⁴ DNA-binding domain mutant R336A givesstrong bypass transcription (35). R383K and R383A did not, despitesupporting levels of activated transcription and binding to–10 to –1 heteroduplex DNA (heteroduplex 5), whichsuggested that bypass activity might be readily detected. IfR383 interacts with the –12 GC promoter sequence, it wouldappear not to be an interaction contributing to maintainingthe silent state of the holoenzyme prior to activation, in contrastto the properties of the R336A and Region I mutants (20,24,35).

DNA proximities
Residue 383 was suggested to be within a HTH motif, expectedto establish direct contacts with DNA and thought to interactwith the –12 region of the promoter (14). Although ourdata show that substitutions at 383 influence DNA binding, otherdata suggest that a simple direct interaction of R383 with DNAmay not occur. Cleavage of the promoter DNA by Cys383-tetheredFeBABE was not evident. Closed complex promoter DNA cleavageby the FeBABE derivative of ${sigma}$ ⁵⁴ in the UV cross-linking patch(Cys336-tethered FeBABE) is centred around position –9(±1) (28), while DNA cutting by the Cys346-tethered FeBABEderivative is centred further upstream at position –11(±1) (Fig. 7). Given that the UV cross-linking patchis ${alpha}$ -helical in structure, the FeBABE cleavage data suggest thatthe UV cross-linking patch (N-terminal to the HTH motif) alignswith or is inclined towards the promoter DNA template strandin closed complexes. The lack of any discernible cleavage bythe Cys383-tethered FeBABE derivative suggests that either residue383 is not involved in a direct DNA contact or that some structuralconsequences of making substitutions at 383 do not allow detectionusing the FeBABE methodology. However, R383C was active fortranscription in vitro, more so than R383A (18).

Summary
Overall, our data are consistent with a requirement for R383to distinguish between T or G at –13 and overall reducedDNA binding when it is substituted by K or A (14). It is possiblethat some of the overall loss in DNA-binding activity has abasis in an altered protein structure rather than simple lossof a DNA-interacting side chain, a view supported by the invivo instability of R383A. Although instability is unexpectedon substitution of a surface exposed residue in an ${alpha}$ -helix byalanine, there are suggestions from secondary structure predictionsthat R383 may exist within a non-helical structure (http://jura.ebi.ac.uk:8888).The data presented in Figures 1–5 suggest that the interpretationplaced on the in vivo activation data may need reconsiderationand suggest that R383 has a previously unexpected role in thestability of ${sigma}$ ⁵⁴.

In the absence of additional structural or proximity data,any suggestion that the HTH motif lies within a fold that localisessufficiently near the –12 region to contact DNA is speculative.A colinear arrangement, N-terminal to C-terminal (beginningat the –24 promoter element and ending at the start siteproximal sequences), of the UV cross-linking patch, the HTHmotif and the RpoN box is possible, but unproven. Further, theclear involvement of the ${sigma}$ ⁵⁴ Region I sequences in promoter bindinghas shown that determinants outside the DNA-binding domain makecritical contributions to the DNA binding function of ${sigma}$ ⁵⁴ (8,20,25,28).

Specialisation of function across the ${sigma}$ ⁵⁴ DNA-binding domainis evident. Residues F402, F403, F354 and F355 appear to beassociated with interactions needed for efficient polymeraseisomerisation (40,43), R383 with forming stable initially meltedDNA complexes and R336 with maintaining the inhibited silentstate of the polymerase (10,35). We note functional similaritiesbetween the putative ${alpha}$ -helix, in which C346 and R336 in ${sigma}$ ⁵⁴ lie,and helix 14 of E.coli ${sigma}$ ⁷⁰. Both helices interact with promotersequences that include recognition sequences (15,44). They alsocontain determinants for binding locally single-stranded DNAstructures from which melting originates and spreads (8,26,28,45).These and other considerations lead to the view that a seriesof linked interactions that involve ${sigma}$ ⁵⁴–DNA interactionand ${sigma}$ ⁵⁴–core interfaces are required to change in orderto allow the polymerase to progress to the open complex. Itseems that the putative HTH motif of ${sigma}$ ⁵⁴ contributes as a structuralelement rather than as a major direct DNA-contacting surface.Nevertheless, several conformational changes in ${sigma}$ ⁵⁴ are probablynecessary for open complex formation. Transient contacts between ${sigma}$ ⁵⁴ and core RNAP or between ${sigma}$ ⁵⁴ and promoter DNA may have escapedour analysis of Cys383-tethered FeBABE proximities to DNA. Currentdata suggest that the centre formed by Region I, the UV cross-linkingpatch of ${sigma}$ ⁵⁴ and the –12 promoter region does not includethe HTH motif as an element in proximity (15,18,28).

ACKNOWLEDGEMENTS

We thank Nobuyuki Fujita for help with early stages of thiswork, Wendy Cannon for oligonucleotides and members of the MBlaboratory for comments on the manuscript. This work was supportedby a Biotechnology and Biological Sciences Research Council(BBSRC) project grant to M.B. and by a post-graduate studentshipfrom the LEA, Karlsruhe, Germany, to S.R.W.

FOOTNOTES

^* To whom correspondence should be addressed. Tel: +44 20 75945442; Fax: +44 20 7594 5419; Email: m.buck{at}ic.ac.uk

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Salmonella enterica

${sigma}$

⁵⁴

J. Bacteriol

182

[Abstract/Free Full Text]

2 Lee,J.H. and Hoover,T.R., (1995) Protein cross-linking studies suggest that Rhizobium meliloti C-4-dicarboxylic acid transport protein-D, a ${sigma}$ ⁵⁴-dependent transcriptional activator, interacts with ${sigma}$ ⁵⁴-subunit and the ß-subunit of the RNA-polymerase. Proc. Natl Acad. Sci. USA, 92, 9702–9706.[Abstract/Free Full Text]

3 Rippe,K., Guthold,M., von Hippel,P.H. and Bustamante,C. (1997) Transcriptional activation via DNA-looping: visualization of intermediates in the activation pathway of E. coli RNA polymerase and ${sigma}$ ⁵⁴ holoenzyme by scanning force microscopy. J. Mol. Biol., 270, 125–138.[ISI]

Nucleic Acids Research

In vitro roles of invariant helix–turn–helix motif residue R383 in 54 (N)

In vitro roles of invariant helix–turn–helix motif residue R383 in ${sigma}$ ⁵⁴ ( ${sigma}$ ^N)