The relA/spoT-Homologous Gene in Streptomyces coelicolor Encodes Both Ribosome-Dependent (p)ppGppSynthesizing and -Degrading Activities

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Journal of Bacteriology, August 1998, p. 4123-4132, Vol. 180, No. 16
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

The relA/spoT-Homologous Gene in Streptomyces coelicolor Encodes Both Ribosome-Dependent (p)ppGppSynthesizing and -Degrading Activities

Oscar H. Martínez-Costa, Miguel A. Fernández-Moreno, and Francisco Malpartida^*

Centro Nacional de Biotecnología, Consejo Superior de Investigaciones Científicas, Campus Universidad Autónoma de Madrid, Cantoblanco, 28049-Madrid, Spain

Received 27 April 1998/Accepted 15 June 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Streptomyces coelicolor (p)ppGpp synthetase (Rel protein) belongs to the RelA and SpoT (RelA/SpoT) family, which is involvedin (p)ppGpp metabolism and the stringent response. The potentialfunctions of the rel gene have been examined. S. coelicolor Relhas been shown to be ribosome associated, and its activity invitro is ribosome dependent. Analysis in vivo of the active recombinantprotein in well-defined Escherichia coli relA and relA/spoT mutantsprovides evidence that S. coelicolor Rel, like native E. coliRelA, is functionally ribosome associated, resulting in ribosome-dependent(p)ppGpp accumulation upon amino acid deprivation. Expressionof an S. coelicolor C-terminally deleted Rel, comprised of onlythe first 489 amino acids, catalyzes a ribosome-independent (p)ppGppformation, in the same manner as the E. coli truncated RelA protein(1 to 455 amino acids). An E. coli relA spoT double deletion mutanttransformed with S. coelicolor rel gene suppresses the phenotypeassociated with (p)ppGpp deficiency. However, in such a strain,a rel-mediated (p)ppGpp response apparently occurs after glucosedepletion, but only in the absence of amino acids. Analysis ofppGpp decay in E. coli expressing the S. coelicolor rel gene suggeststhat it also encodes a (p)ppGpp-degrading activity. By deletionanalysis, the catalytic domains of S. coelicolor Rel for (p)ppGppsynthesis and degradation have been located within its N terminus(amino acids 267 to 453 and 93 to 397, respectively). In addition,E. coli relA in an S. coelicolor rel deletion mutant restoresactinorhodine production and shows a nearly normal morphologicaldifferentiation, as does the wild-type rel gene, which is in agreementwith the proposed role of (p)ppGpp nucleotides in antibiotic biosynthesis.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Actinomycetes are very well-known for their ability to produce several secondary metabolites with important biological properties(10). In general, antibiotic formation in Streptomyces is developmentallyregulated, with production in liquid cultures being associatedwith the stationary phase, while in agar-grown cultures it iscoupled to morphological differentiation (11, 14, 19). Whilethe global regulatory mechanisms of antibiotic production arestill poorly understood, a role for growth rate or growth cessationin triggering synthesis of secondary metabolites has been suggested(10, 12).

Attempts at elucidating some of the steps in the mechanism(s) controlling antibiotic production by Streptomyces coelicolorhave been conducted in several laboratories. Many putative regulatorygenes have been isolated and characterized. Such a gene, whosededuced product shows strong similarities to proteins of the RelAand SpoT (RelA/SpoT) family (implicated in ppGpp metabolism),has recently been cloned from S. coelicolor (7, 8, 30).Deletion of this gene gave an actinorhodine-nonproducing phenotype(7, 30), suggesting a role for ppGpp in antibiotic production.This gene, originally called ORF1, will be referred to as rel,while relA and spoT will be exclusively used for E. coli.

In members of the family Enterobacteriaceae, the highly phosphorylated guanine nucleotides [(p)ppGpp] are pleiotropic effectorsinvolved in the adaptation of bacterial cells to nutritional andenvironmental changes. The transient (p)ppGpp accumulation uponnutrient depletion is characterized by several features: reductionin stable RNA accumulation, stimulation of certain amino acidoperons, and induction of specific stationary-phase gene expression(for reviews, see reference 6). In Escherichia coli, (p)ppGppformation depends on two coordinated pathways, which are catalyzedby two gene products: RelA (34) [(p)ppGpp synthetase I] andSpoT (50) [ppGpp 3' pyrophosphohydrolase, or (p)ppGpp synthetaseII]. Under amino acid deprivation, when codon-specific unchargedtRNA is bound to the ribosomal acceptor site, a relA-dependent(p)ppGpp-synthesizing activity occurs, allowing the cell to adaptto the reduced amino acid availability. Biochemical studies ofthe RelA protein reveal that it is a ribosome-associated enzyme,whose activity involves the pyrophosphoryl transfer from ATP toGTP (or GDP). During carbon source starvation, the (p)ppGpp accumulationseems to be largely dependent on the spoT gene product (18,35, 59) (despite the possible partial contribution of RelA,due to the transient amino acid limitation that follows carbonsource deprivation [9]). Recent in vivo functional studiesof several spoT deletions support the notion that the proteinis a bifunctional enzyme with (p)ppGpp-synthesizing and -degradingactivities, although SpoT 3' pyrophosphate transferase activityhas not been demonstrated in vitro (17). E. coli RelA/SpoT sequencecomparison has revealed that both proteins are closely related(36). The similarities might well be a consequence of a geneduplication, following which relA has evolved to a (p)ppGpp-synthesizingactivity, while spoT has become more specialized for (p)ppGppdegradation (36).

Among the RelA/SpoT homologs so far studied, the Streptococcus equisimilis Rel protein has been reported to function as SpoTwhen expressed in E. coli, but S. equisimilis disruptants behavesimilarly to relA mutants (32). For the S. equisimilis enzyme,both weak ribosome-independent (p)ppGpp-synthesizing and -degradingactivities have been demonstrated in vitro (32). These experimentalfindings suggest that the S. equisimilis rel gene performs bothrelA and spoT activities; this suggestion has been reinforcedby recent in vivo studies of this bacterium (33) and Bacillussubtilis (58).

We have reported that an S. coelicolor rel-deleted mutant loses its ribosome-associated (p)ppGpp-synthesizing activity (30).A similar rel-deleted mutant of a different S. coelicolor strain(M600) has been reported to be unable to accumulate ppGpp uponamino acid deprivation (7, 8). Taken together, these resultssuggest that S. coelicolor rel might function as E. coli relA.However, sequence comparison of S. coelicolor Rel with other RelA/SpoTproteins has shown higher similarities to E. coli SpoT (8,30), which, unlike E. coli RelA, is directly involved in (p)ppGppdegradation; this opens up a crucial question: does S. coelicolorRel have some functions similar to those of SpoT?

In addition, an unrelated gene (polynucleotide phosphorylase) apparently involved in (p)ppGpp metabolism has recently beenreported in Streptomyces antibioticus; when assayed in vitro,both a ribosome-independent (p)ppGpp synthetase and a polynucleotidephosphorylase activity are found (22).

In this paper, we describe the functional characterization of S. coelicolor Rel, determined by using complementation analysisof well-defined E. coli relA and spoT mutants.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Bacterial strains and plasmids. The bacterial strains used are listed in Table 1. The E. coli vectors and recombinant plasmids used are shown in Table 2.E. coli M13mp19-derivative phage (60) was used for in vitromutagenesis. The Streptomyces plasmids pIJ486 (57), pIJ941 (27),and pSCNB080 (30) were used. The Streptomyces $phi$ C31-derivativephages used were PM1 (29) and KC859 (4). pCNB3033, a Streptomycesintegrative vector, was constructed by cloning the 3.6-kbp NdeI-KpnIfragment from phage KC859, previously made blunt ended by T4 DNApolymerase treatment, into SmaI-digested pIJ2921, yielding plasmidpMF2058; the hygromycin resistance gene from PM1 was finally clonedinto BamHI-PstI-digested pMF2058. Similarly, the Streptomycesintegrative thiostrepton-derived vector pMF2024 was obtained.

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TABLE 1. Bacterial strains used in this study

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TABLE 2. Plasmids used in this study

General techniques. Isolation, cloning, and manipulation were performed as previously described for E. coli (48) and Streptomyces (20). NdeIrestriction sites were generated by using the Sculptor in vitromutagenesis system (Amersham; RPN 1526). Previously, suitablerestriction fragments from either rel or relA were cloned in M13mp19,and mutagenesis was performed according to the manufacturer'srecommendations, with the following synthetic oligonucleotides:P01, 5'-ACTTCTTACCGCAACCATATGTCCTCTCCT-3'; P02, 5'-TGGGCCTCGTCTGGCATATGGACTCCTCGTGCGCGAT-3';and P03, 5'-CCGCCTGGCCCATATGGGCGTGCAGCGC-3'.

Construction of recombinant plasmids. The recombinant plasmids used and their construction are summarized in Table 2. Hybrid plasmids containing the relA and relgenes, including their promoter regions, were constructed by previouslygenerating an NdeI restriction site by in vitro mutagenesis asdescribed above; primers P01 and P02 were used for relA and rel,respectively. From the resulting NdeI-engineered pCNB0118 andpCNB0121 (for the relA and rel genes, respectively), the hybridconstructions were obtained, in which the rel gene is under thecontrol of the relA promoter (pCNB0127) and the relA gene is underthe control of the rel promoter (pCNB0129). To construct pCNB0163,expressing the truncated Rel(93-847) protein, an NdeI restrictionsite was previously generated with primer P03.

To localize the Rel catalytic domains, several recombinant plasmids carrying various deletions of the gene were constructed(Table 2). In some cases, the rel coding fragments were previouslycloned into pET19b, creating suitable restriction sites for furthersubclonings and generating translation start and stop codons.By this procedure, some of the resulting recombinant gene productshave additional amino acids, which are indicated in Table 2.

The rel expression plasmids have been cloned under the control of the relA promoter and possess the original relA ribosome-bindingsite.

Media and growth conditions. E. coli strains were grown on either liquid or solid 2YT medium (48). For in vivo ³²P_i labeling, MOPS (morpholinepropanesulfonic acid) glucose minimalmedium (38) containing 0.2 mM phosphate, 0.4% glucose, aminoacids (50 µg/ml each), and bases (20 µg/ml each) was used. Growthon serine-methionine-glycine (SMG) medium (56) was used to testthe rel-dependent (p)ppGpp response. Growth of E. coli CF1693was also checked on minimal glucose M9 medium (48). Glycogenassays were performed as described elsewhere (17), with glucose-richmedium (0.5% tryptone, 0.5% yeast extract, 2% glucose).

Determinations of intracellular (p)ppGpp concentrations. Cell labeling was performed as described previously (49). Changes in the intracellular (p)ppGpp pool upon amino acid starvationwere quantitated after DL-serine hydroxamate treatment (1 mg/ml,final concentration) (55); cells were uniformly ³²P_i labeled in MOPS medium with the composition described above,but with serine omitted. The glucose concentration in MOPS mediumwas lowered to 0.04% when glucose starvation was induced, eitherwith or without amino acids, by $alpha$ -methylglucoside addition (2.5%,final concentration). Amino acid (isoleucine) deprivation in MOPSmedium was achieved with valine at 500 µg/ml and relieved by additionof isoleucine (100 µg/ml, final concentration). Acid extractionof nucleotides was done as described previously (2) and resolvedby one-dimensional polyethylenimine thin-layer chromatographydeveloped with 1.5 M KH₂PO₄ (pH 3.4) as described by Cashel (5).Nucleotides were quantified with a Fujix Bas 1000 imaging systemwith TINA 2.08 software (Raytest, Straubenhardt, Germany). Theamounts of (p)ppGpp were expressed as fractions of the total nucleotidepool [GTP plus (p)ppGpp]; correction was done as previously described(30), with acid extracts from either CF1652 or CF1693. In somecases, quantification of (p)ppGpp was also performed by liquidscintillation counting as described previously (30).

Ribosome purification. Ribosomes were prepared essentially as described by Krohn and Wagner (25) with minor modifications: cells were disruptedby sonication, and buffer A consisted of 50 mM Tris acetate (pH8), 15 mM magnesium acetate, 60 mM potassium acetate, 30 mM ammoniumacetate, 1 mM dithiothreitol, 0.2 mM EDTA, and 0.5 mM phenylmethylsulfonylfluoride. High-salt-washed ribosomes were obtained by resuspensionof low-salt-washed ribosomes in buffer A containing 0.7 M ammoniumacetate and centrifuged as previously described (25); the resultingpellet was resuspended in buffer A and used directly as high-salt-washedribosomes, while the supernatant, which constituted the high-saltwash, was dialyzed against buffer A. The crude extract is definedas the supernatant after centrifugation of the disrupted cellsat 25,000 × g for 30 min at 4°C.

Measurement of (p)ppGpp synthetase activity. (p)ppGpp synthetase assays were carried out essentially as described previously (30), except that the incubation time was30 min. To measure this enzyme activity in crude extracts, eitherwith or without 18% methanol, 12-µl aliquots of the reaction mixturewere taken at 0, 5, 10, and 30 min, and reactions were stoppedwith 2 µl of 4 M formic acid. Nucleotides were resolved and quantifiedas described above; the activity was calculated within the linearrange.

Preparation of (p)ppGpp. Preparative scale synthesis of ppGpp and pppGpp was performed essentially as described elsewhere (25), with low-salt-washedribosomes from E. coli CF1652 carrying the relA plasmid (pCNB0115).Labeled 3'-[ $alpha$ -³²P]ppGpp and -pppGpp were prepared according to the method of Syand Lipmann (53) with some modifications: the reaction proceededfor 1 or 2 h at 30°C with [ $alpha$ -³²P]GTP and was stopped by two phenol-chloroform extractions andthen a final chloroform extraction. The aqueous phase was dilutedat least six times with 50 mM triethylammonium acetate (pH 7.7)and applied to a 1-ml DEAE-Biogel column that had been equilibratedwith the same buffer. Stepwise elution was performed as describedpreviously (53), and ppGpp- and pppGpp-containing fractionswere lyophilized to remove excess salt and dissolved in a smallamount of water.

Preparation and assay of (p)ppGpp phosphohydrolase activity. Crude extracts were obtained as described above, except that buffer B (50 mM Tris acetate [pH 8], 1 mM EDTA, 0.3 M KCl, 0.5mM phenylmethylsulfonyl fluoride, 1 mM dithiothreitol, 20% glycerol)was used. Because of high nonspecific nucleotidase activities,1.5 ml of the crude extract was previously fractionated with ammoniumsulfate up to 20%. After centrifugation at 25,000 × g for 20 minat 4°C, the pellet was suspended in 0.5 ml of buffer B and dialyzedagainst buffer B. The insoluble protein aggregates were collectedby centrifugation at 9,000 × g for 30 min at 4°C, dissolved in0.1 ml of buffer B containing 1 M KCl, and stored at $-$ 20°C untiluse. (p)ppGpp-degrading activity was carried out in 30 µl of reactionmixture in buffer B containing 45 µg of protein, 0.2 mM [ $alpha$ -³²P](p)ppGpp (about 1 µCi/µmol), and 10 mM MnCl₂. The final KClconcentration was 0.3 M. Six-microliter aliquots were taken at0, 5, 10, 15, and 20 min (in which the reaction was shown to belinear), and the reaction was stopped with 1 µl of 4 M formicacid. Nucleotides were resolved and quantified as described above.

Miscellaneous methods. Protein was measured as described elsewhere (3) with bovine serum albumin as a standard. Sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) was carried out with the buffersystem described by Laemmli (26) in either a 10 or 15% polyacrylamidegel, and protein bands were visualized by staining with Coomassiebrilliant blue R250.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Expression of S. coelicolor Rel in E. coli. (i) In vitro assay of S. coelicolor (p)ppGpp synthetase. As a first approach to analyze the functional properties of S. coelicolor rel gene, we examined the expression of the S. coelicolorrel gene in the E. coli relA deletion CF1652 strain. To this end,this strain was transformed with plasmid pCNB080, which containsthe S. coelicolor rel gene under the control of its own promoter.However, neither the presence of a recombinant protein by SDS-PAGEanalysis nor (p)ppGpp synthetic activity was detected (data notshown). Clearly, this could be due to a failure to obtain expressionof rel gene. Consequently, a construct was made in which the nativerel gene-initiating UUG codon was changed to AUG, and the codingsequence was cloned under the control of the relA promoter, includingthe original relA ribosome-binding site (pCNB0127). Crude extractfrom CF1652 strain transformed with pCNB0127 showed a solubleprotein in SDS-PAGE, having the expected apparent molecular mass(94 kDa) for the S. coelicolor Rel protein (Fig. 1). The expected84-kDa RelA protein could be detected when strain CF1652 is transformedwith pCNB0115, which harbors the relA gene. By using crude extractsfrom this strain expressing either the rel or relA gene, the (p)ppGppsynthesizing activities were calculated to be 2.8 and 22.5 nmolof (p)ppGpp formed/min/mg, respectively; as with the wild-typeRelA, the S. coelicolor Rel activity was detected in the ribosomalfraction (Fig. 2).

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FIG. 1. SDS-PAGE of crude extracts from E. coli CF1652. Lanes: 1, plasmid harboring the rel gene (40 µg); 2, plasmid carrying the relA gene (52 µg); 3, with no plasmid (46 µg). The overproduced recombinant S. coelicolor Rel and E. coli RelA of 94 and 84 kDa, respectively, are indicated by arrowheads. The positions and molecular masses of marker proteins are indicated on the right of the gel. The smaller bands observed in either lane 1 or 2 correspond to $beta$ -lactamase and chloramphenicol acetyltransferase, respectively.

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FIG. 2. Synthesis of polyphosphorylated guanine nucleotides by purified ribosomes. Reaction conditions were as specified in Materials and Methods, with low-salt-washed ribosomes from E. coli CF1652 with no plasmid (lane 1); plasmid harboring the E. coli relA gene (pCNB0115), either with or without methanol lanes 2 and 4, respectively); plasmid carrying the S. coelicolor rel gene (pCNB0127), either with or without methanol (lanes 3 and 5, respectively); and without ribosomes added (lane 6). Final protein concentrations were 0.90 (lane 1), 1.05 (lanes 3 and 5), and 0.95 (lanes 2 and 4) mg/ml.

Whether or not this ribosome-associated (p)ppGpp synthetase is also ribosome dependent in vitro was also investigated. Thus,supernatants of high-salt-washed ribosomes from either S. coelicolorJ1501 (carrying additional copies of rel in pSCNB080) or E. coliJM101 (carrying additional copies of relA in pGG21) were obtainedas described in Materials and Methods. No (p)ppGpp formation occurredwith either preparation. Nevertheless, when either supernatantwas analyzed for its (p)ppGpp-synthesizing activity in the presenceof high-salt-washed ribosomes from either S. coelicolor 18J orE. coli CF1652 [which are completely devoid of ribosome-associated(p)ppGpp formation] or 18% methanol, the (p)ppGpp synthesis wasdetected (Table 3). Thus, in both cases, the enzymatic activityappeared to be ribosome dependent. The resulting activities ofS. coelicolor Rel were almost identical, irrespective of the sourceof ribosomes, suggesting that its interactions with E. coli ribosomesmight well be similar to that of RelA.

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TABLE 3. Relative synthesis of (p)ppGpp by supernatants of high-salt-washed ribosomes derived from either S. coelicolor J1501/pSCNB080 or E. coli JM101/pGG21^a

Since the S. coelicolor Rel protein is ribosome associated and its activity is ribosome dependent in vitro, it was of interestto assess if the Rel activity is also functionally ribosome dependent.As a result, we undertook in vivo functional studies.

(ii) In vivo functional analysis of the rel gene in E. coli. Because E. coli CF1652 lacks a functional relA gene and, consequently, has no ribosome-dependent (p)ppGpp formation, thisstrain shows a relaxed response and is unable to grow on SMG medium.To explore if the S. coelicolor rel gene is able to complementthe relaxed phenotype of E. coli CF1652, this strain was transformedwith several plasmids: pCNB080, pCNB0115, pCNB0127, pCNB0128,and pCNB0129 (Table 2). As shown in Fig. 3, pCNB0127 transformantsbehave like those containing pCNB0115 and pCNB0129 (carrying therelA gene), while no growth of either pCNB080 or pCNB0128 (a rel-lacZfusion) transformants was observed. Because pCNB0127 transformantsgrew on SMG medium, a functional rel-dependent (p)ppGpp responsemay be acting.

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FIG. 3. Growth of E. coli CF1652 transformants on SMG medium. The constructs used to transform E. coli CF1652 are shown on the left-hand side, and growth analysis is shown on the right. CF1652 transformants were grown in 2YT medium with the selective antibiotics until the A₄₆₀ was 0.6 to 0.8, washed twice with minimal glucose M9 medium, spread on SMG agar plates, and incubated for 16 h at 37°C. pSU21, control plasmid. Sc, S. coelicolor; Ec, E. coli.

In vivo synthesis of (p)ppGpp by the S. coelicolor rel gene product was estimated after amino acid starvation in responseto the addition of DL-serine hydroxamate. (p)ppGpp accumulatedin E. coli CF1652 carrying pCNB0127 (Fig. 4A), as is observedfor the native relA gene; the maximal production is detected 20min after the addition of serine hydroxamate, which representsan eightfold increase over the basal levels. Upon chloramphenicoladdition, the (p)ppGpp levels dropped within a few minutes (Fig.4A). This result might be expected, since chloramphenicol is knownto be an inhibitor of the ribosome-dependent (p)ppGpp formation(46), and the (p)ppGpp might be rapidly degraded by the (p)ppGppaseactivity of the intact SpoT protein from CF1652. The basal (p)ppGpplevels in CF1652 transformed with pCNB0127 were the same as thosein JM101 (35 and 21 pmol/A₄₆₀ units, respectively) and were 20-foldless than that for CF1652 carrying pCNB0115 (662 pmol/A₄₆₀ units)(Fig. 4B). Notably, the (p)ppGpp levels in strain CF1652 transformedwith the rel gene after 20 min of amino acid deprivation were2- and 10-fold lower than those observed in the presence of eithersingle or multiple copies of the relA gene (268 versus 495 and2,580 pmol/A₄₆₀ units, respectively) (Fig. 4B).

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FIG. 4. Changes in (p)ppGpp levels upon amino acid deprivation. (A) Relative (p)ppGpp accumulation of strain CF1652 containing the S. coelicolor rel plasmid pCNB0127 after serine hydroxamate addition ( $open circle$ ). Chloramphenicol (at a final concentration of 100 µg/ml and indicated with arrow [Cm]) was added to culture after 20 min ( $bullet$ ). (B) Amounts of (p)ppGpp upon serine hydroxamate treatment of E. coli JM101 (single-copy E. coli relA) (columns 1 and 4) and E. coli CF1652 transformed with either pCNB0127 (S. coelicolor rel) (columns 2 and 5) or pCNB0115 (multicopy E. coli relA) (columns 3 and 6). Results for cultures prior to the addition of serine hydroxamate and after 20 min are shown by columns 1 to 3 and 4 to 6, respectively. At each incubation period, samples of 5 µl of acid extracts were analyzed for their (p)ppGpp content.

Taking these results together, we inferred that the S. coelicolor Rel protein behaves like E. coli RelA. In order to investigateadditional functions of the S. coelicolor Rel protein, we exploredits properties in the well-defined E. coli CF1693 relA spoT doublemutant.

Functional analysis of S. coelicolor Rel in an E. coli $Delta$ relA $Delta$ spoT background. (i) The S. coelicolor rel gene suppresses the phenotypic defects of the E. coli relA spoT double mutant. The wild-type relA gene is lethal in E. coli CF1693 because of the resultant high intracellular (p)ppGpp concentration, whichpresumably arises from the failure of (p)ppGpp degradation normallycatalyzed by SpoT (17, 59). Because S. coelicolor Rel appearsto function in the same manner as E. coli RelA, it was of interestto examine whether the rel gene could be introduced into the CF1693strain. Viable transformants were obtained when the rel gene onplasmid pCNB0127 was introduced in this strain. Nevertheless,the transformants have a severely slow growth rate; well-definedcolonies formed only after 36 to 48 h on 2YT plates at 30°C.

S. coelicolor rel was cloned in a low-copy-number plasmid under the relA promoter (pCNB0165) for further analysis of strainCF1693 because it grows slowly when it harbors pCNB0127. The abilityof the rel gene to reverse several features associated with theppGpp-deficiency phenotype of CF1693 was explored. Growth on minimalmedium of CF1693 transformed with pCNB0165 plasmid was detected,but not with the vector as a control, indicating that the aminoacid requirements of this strain (59) are suppressed by theS. coelicolor rel gene. Because glycogen synthesis is believedto be strongly dependent on (p)ppGpp (47), indirect evidenceof (p)ppGpp synthesis by the S. coelicolor rel product could beobtained by evaluating the accumulation of glycogen in CF1693and its derivative when grown on glucose-rich medium. CF1693 failsto accumulate glycogen and, consequently, strains yellow withiodine vapors, while pCNB0165 transformants showed an intensebrown stain (data not shown). Additionally, when CF1693 carryingeither pVLT31 (control plasmid) or pCNB0165 was grown in 2YT medium,their respective doubling times were 66 and 114 min, respectively.This difference is expected if the levels of (p)ppGpp are elevatedbecause of S. coelicolor (p)ppGpp synthetase activity. Interestingly,when pCNB0165 transformants of CF1693 were plated on solid 2YTmedium, the colonies exhibited a morphology different from thoseof this strain containing the vector plasmid. While the latterdisplayed fuzzy edges and tended to lyse upon prolonged incubationin the stationary phase, those harboring the S. coelicolor relgene were characterized by a translucent appearance and remainedviable for several days. The cell morphology of the CF1693 strainunder the light microscope has been reported as being more elongatedthan that of the wild type (59). This phenotype was observedeither during exponential growth in liquid 2YT medium or duringboth exponential and stationary phases in M9 medium containingall amino acids, while an apparently normal cellular morphologywas restored by transformation with pCNB0165 (data not shown).These results suggest that the rel gene can partially complementsome deficiencies of the relA spoT double deletion mutation.

(ii) Characterization of the rel gene in E. coli relA spoT double mutant. In order to investigate if Rel protein has some functional features similar to those of SpoT, we analyzed the response ofCF1693 transformed with pCNB0165 to (p)ppGpp upon carbon sourcedeprivation. It is well known that upon glucose starvation, (p)ppGppproduction is largely dependent on SpoT when amino acids are presentin the medium (17). After the addition of $alpha$ -methylglucoside,the ppGpp pool (only this compound was detected) in CF1693 transformantsincreased only in the absence of added amino acids (Fig. 5), suggestingthat glucose depletion leads first to amino acid starvation, andthis subsequently causes activation of ribosome-dependent S. coelicolorrel activity.

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FIG. 5. Accumulation of ppGpp upon glucose starvation of E. coli CF1693 containing the S. coelicolor rel plasmid pCNB0165. Relative ppGpp levels are shown at various times after $alpha$ -methylglucoside treatment. (

) MOPS minimal medium containing all amino acids. (

) MOPS minimal medium with no amino acids. Samples of 20 µl (delivered in 5-µl intervals) of the acid extracts were analyzed for the estimations of amounts of (p)ppGpp. Basal ppGpp levels were either 38.5 or 28.1 pmol/A₄₆₀ units with and without amino acids, respectively.

To analyze if S. coelicolor Rel had some (p)ppGpp-degrading activity, we measured the decay of ppGpp following direct reversalof stringency conditions. Thus, isoleucine was added to valine-inhibitedcultures of strain CF1693 transformed with either pCNB0165 orpCNB0166, expressing the wild-type Rel and the truncated Rel(93-847),respectively. The results are shown in Fig. 6. Basal ppGpp levelsof CF1693 transformed with pCNB0166 appeared to be 1.5-fold higherthan those with pCNB0165, which might well correlate with itseven lower growth rate (doubling time of 122 min in 2YT medium).Upon amino acid starvation, ppGpp accumulation occurred in thepresence of both full-length Rel and truncated Rel; interestingly,after addition of isoleucine, ppGpp disappears in both strainswithin a few minutes. From the equation k = ln2/half-life, theirfirst-order decay constants were estimated, which were 0.11/minand 0.25/min for native Rel and Rel(93-847), respectively. Thesevalues approximate those observed for E. coli SpoT and S. equisimilisRel (16, 17, 32) and are shorter than the ppGpp half-lifefor the spoT-deleted mutant used here, which has been reportedto be at least 30 min (17). Thus, either the full-length Relor the N-terminally deleted Rel is involved in the ppGpp degradation.Furthermore, in vitro (p)ppGpp hydrolysis was also detected infractionated cell extracts from CF1693 transformed with eitherpCNB0165 or pCNB0166, but not from the strain containing the controlplasmid; their respective activities were calculated to be 3.2and 3.9 nmol/min/mg. ppGpp and pppGpp were similarly degradedto GDP and GTP, respectively, and this activity required Mn²⁺ ions, which could not be substituted for by Mg²⁺.

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FIG. 6. Reversal of a valine-imposed stringent response by isoleucine addition in E. coli CF1693 harboring S. coelicolor rel plasmids. (A and B) ppGpp accumulation upon amino acid (isoleucine) deprivation by valine addition of strain CF1693 transformed with either pCNB0165 (expressing native Rel) ( $open circle$ ) or pCNB0166 [expressing Rel(93-847)] (

), respectively. After 20 min, a valine-induced stringent response was reversed by isoleucine addition, and ppGpp decay was analyzed for either the pCNB0165 ( $bullet$ ) or pCNB0166 (

) strain. (C) Rate of ppGpp decay in either strain. The amounts of ppGpp shown are relative to the time of isoleucine addition.

E. coli relA restores actinorhodine production in an S. coelicolor rel mutant. The S. coelicolor rel-deleted strain 18J does not produce actinorhodine, but its synthesis is restored by the presence intrans of the rel gene (30). Because the Rel protein appearsto share several of the properties of E. coli RelA, it was ofinterest to test if the relA gene was able to restore actinorhodineproduction in the streptomycete mutant.

Attempts to clone the relA gene in S. coelicolor 18J under the control of the rel promoter were unsuccessful. Neither in ahigh- nor a low-copy-number plasmid nor in an integrative vectorwas it possible to obtain a recombinant strain carrying the relAgene, whereas transformants carrying the rel gene were easilyisolated. The inability to obtain recombinants even with an integrativevector (pCNB0173) could well be the result of the lethal accumulationof (p)ppGpp as a consequence of the synthetic activity of theRelA, which might be higher than that of the Rel protein. Therefore,an inducible promoter was chosen for complementation analysisin order to avoid the possible deleterious effects of the relAgene being expressed in S. coelicolor under the control of therel promoter. Thus, the relA gene was cloned under the controlof the tipA promoter (37), with the Streptomyces integrativeplasmid pIJ8600 (52) used as the vector. Several transformantsof S. coelicolor 18J were obtained with this construction. Plasmidintegration into the chromosome was confirmed by Southern analysisof their respective total DNAs. Interestingly, when grown on R5solid medium, even without thiostrepton induction, both actinorhodineproduction and a nearly normal morphological differentiation wereobserved in the 18J mutant strain carrying the E. coli relA gene,while no phenotypic changes were detected in this strain harboringthe integrated vector as a control. Thus, the relA-dependent activityappears to be sufficient to restore actinorhodine production inthe heterologous host, as does the wild-type rel gene.

Localization of the catalytic domains of Rel protein. From the previous results, it can be deduced that the Rel protein, like RelA, has a ribosome-dependent (p)ppGpp-synthesizingactivity, which is activated upon amino acid deprivation. Nevertheless,unlike RelA, the Rel protein is also capable of degrading (p)ppGpp,a function it shares with SpoT. Additionally, the Rel proteinhas been shown to contain a sequence that matches the consensuspattern of a putative ATP-GTP binding motif (amino acids 458 to465) (30), a particular feature which is not present in anyother known protein involved in (p)ppGpp metabolism. In orderto define the functional domains of the Rel protein, expressionanalyses of truncated recombinant Rel proteins (including an internal25-amino-acid in-frame deletion of the Rel protein, by which theputative ATP-GTP binding motif has been removed) were undertakenwith either E. coli CF1652 or CF1693.

(i) (p)ppGpp-synthesizing domain. To localize more precisely the protein region involved in (p)ppGpp-synthesizing activity, several constructs were generatedwith various Rel deletions (Table 2 and Fig. 7). The resultingplasmids were tested with the E. coli relA mutant strain (CF1652)for their ability to induce (p)ppGpp synthesis in vivo. The viabilityand growth rate of CF1693 (the relA spoT strain) when transformedwith the recombinant plasmids might be used as an additional indicationof (p)ppGpp synthesis. By SDS-PAGE analysis, all recombinant proteinswere expressed at a similar level to that detected in Fig. 1 forthe full-length Rel protein, except for the truncated proteinsRel(359-489), Rel(230-422), and Rel(267-453), which were almostundetectable (data not shown). The results are summarized in Fig.7.

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FIG. 7. Phenotypic characterization of the recombinant plasmids expressing truncated S. coelicolor Rel proteins. Recombinant pUC18 derivatives containing the indicated rel deletions are shown. NdeI-engineered restriction sites are indicated by asterisks. Restriction sites from pET19b are shown in nonitalic style. In vivo (p)ppGpp activity was determined as specified in Materials and Methods. The ribosome dependence was estimated by subjecting the recombinant strains to amino acid starvation by the addition of serine hydroxamate; samples taken at 0, 7, 15, and 30 min were analyzed for their (p)ppGpp content. +, (p)ppGpp detected (a) or (p)ppGpp accumulation (b) in response to the addition of serine hydroxamate; $-$ , no (p)ppGpp detected (a) or no change in (p)ppGpp levels (b) upon the addition of serine hydroxamate. t, viable transformants; u, unable to select transformants; n.a., not applicable. Transformants of CF1693 carrying pCNB0127 and pCNB0163 showed a very slow growth rate.

While the in vivo basal (p)ppGpp concentration of CF1652 expressing either the native Rel or the truncated Rel proteins Rel(93-847),Rel(1-489), and Rel(267-453) were very similar (32 to 47 pmol/A₄₆₀units), those observed for the truncated Rel proteins Rel(230-847)and Rel(1-453, 479-847) were 200 and 170 pmol/A₄₆₀ units, respectively.The inability to obtain CF1693 transformants by using some ofthe truncated Rel plasmids (Fig. 7) might be due to the high (p)ppGpplevels because of either the deregulated (p)ppGpp synthesis orthe lack of some (p)ppGppase activity; another possible explanationis that these peptides would be toxic to this particular strain.

In addition, by in vitro measurements, (p)ppGpp-synthesizing activity was detected only when crude extracts from the recombinantstrains were used, in which (p)ppGpp was present in vivo (datanot shown).

From these results, it is suggested that the (p)ppGpp synthesizing domain of S. coelicolor Rel can be allocated between residues267 and 453.

(ii) Ribosome dependence. In order to analyze the ribosome dependence of Rel (p)ppGpp-synthesizing activity, transformants of strain CF1652 with severalrecombinant plasmids were subjected to amino acid deprivationby addition of serine hydroxamate (Fig. 7). As expected, transformantsexpressing the truncated Rel(93-847) protein showed a (p)ppGppresponse similar to that of native Rel. The absence of changesin the (p)ppGpp levels for the truncated Rel(1-489) protein isin agreement with the results for a truncated RelA protein (51)and supports the observed ribosome dependence of rel activity.In vivo analysis of Rel(1-453, 479-847) revealed no incrementaleffect on the (p)ppGpp levels during amino acid starvation; thus,this region of Rel protein, which contains the putative ATP-GTPbinding domain, might be important in the modulation of the ribosome-dependentactivity of the Rel protein. Interestingly, transformants expressingthe truncated Rel(230-847) protein showed no change in (p)ppGppconcentration upon amino acid starvation, suggesting that a portionof the Rel N terminus might well participate with the C-terminalfragment in the ribosome-dependent activity.

(iii) (p)ppGpp-degrading domain. To localize the region of the Rel protein which is involved in (p)ppGpp degradation, we focused our attention on the Rel region,homologous to that of SpoT, known to contain this function (17).Recombinant plasmids (pCNB0819, pCNB0820, and pCNB0821) carryingseveral rel deletions (Table 2) were used to transform CF1693carrying pCNB0165. Plasmid pCNB0165 was used as a source of (p)ppGppsynthesis; the role of the corresponding recombinant proteinson ppGpp degradation was analyzed after reversion of the valine-imposedstringent response by addition of isoleucine. Only with plasmidpCNB0819, expressing Rel(93-397), were we able to detect a higherlevel of ppGpp disappearance (k = 0.19/min), indicating that the(p)ppGpp-degrading activity is contained within this 305-amino-acidfragment. It should be stressed that the recombinant proteinsexpressed by these plasmids were not detected by SDS-PAGE analysis(data not shown).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

We have investigated the potential functions of S. coelicolor Rel, providing evidence that it behaves similarly to E. coliRelA; however, unlike this protein, S. coelicolor Rel is capableof degrading (p)ppGpp, a function it shares with SpoT. Conversely,S. coelicolor Rel might not have a (p)ppGpp-synthesizing functionsimilar to SpoT, as deduced by carbon source starvation analysis.Still, the presence of some (p)ppGpp synthesis in the Streptomycesbackground of a Rel protein like SpoT could be argued and constitutesan interesting feature that remains to be investigated.

Notably, the ppGpp decay rate for the native Rel protein (k = 0.11/min) is lower than the values observed for the E. coliSpoT (16, 17) and S. equisimilis Rel (32) proteins but isstill shorter than the reported ppGpp half-life for the E. colistrain, CF1693, used here (k = <0.02/min) (17). This resultmight reflect either some insensitivity of S. coelicolor Rel tothe reversal of the stringent response or the fact that the (p)ppGpp-degradingactivity is somehow slower, probably because of changes in themodulation of its catalytic properties in the heterologous host.Of interest in this context is the higher ppGpp decay constantobtained for the Rel(93-847) protein (k = 0.25/min), which iswithin the range of those found for other (p)ppGppases.

Taking the results of deletion analysis together, the Rel catalytic region appeared to be contained in a 361-amino-acid fragmentwithin its N terminus (Fig. 8). While 305 amino acids (from 93to 397) are required for (p)ppGpp degradation, the overlappingregion containing residues 267 to 453 is sufficient to yield some(p)ppGpp-synthesizing activity. In addition, a regulatory regionis described at its C terminus, which might be involved in theregulation by ribosome. This regulatory domain might include theputative ATP-GTP binding motif; nevertheless, whether or not thisregion is able to bind ATP or GTP requires further biochemicalstudies. Remarkably, the 187-amino-acid peptide involved in (p)ppGppsynthesis is shorter than the corresponding homologous sequenceof either the C-terminally truncated RelA or the 291-amino-acidSpoT protein, which has been reported to be able to synthesize(p)ppGpp (17, 51). Conversely, the 305-amino-acid peptidethat retains the (p)ppGpp-degrading activity of S. coelicolorRel is larger than the corresponding domain determined for SpoT(17). Attempts to further shorten this fragment failed to obtainfunctional recombinant truncated peptides.

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FIG. 8. Schematic representation of the domain structure of S. coelicolor Rel. The identified domains are drawn to scale. The ATP-GTP binding motif is indicated in black.

It is interesting to note that the truncated Rel(230-847) protein showed a ribosome-independent (p)ppGpp synthesis; thus,there might exist an additional modulatory domain within the Nterminus of the native protein, in addition to that containedat its C terminus, or these regions are both needed for its ribosome-dependentactivity. Alternatively, the (p)ppGpp levels might be regulatedby the (p)ppGpp-degrading activity of S. coelicolor Rel; thisfunction is apparently not present in this truncated Rel protein(31) and, hence, might account for the failure of the ribosome-dependent(p)ppGpp response. This observation is of great interest whentrying to understand the mechanisms of this (p)ppGpp synthetaseregulation and its activation by ribosome.

Unlike native RelA, the in vitro and in vivo (p)ppGpp synthesizing activities of S. coelicolor Rel when expressed in E. coliappeared to be lower. This might be attributed to the presenceof nonfunctional protein. Another possible explanation is thatthe Streptomyces ribosome-associated (p)ppGpp activity might havesome distinct modulation of its catalytic properties. The factthat the in vivo (p)ppGpp levels upon amino acid deprivation inStreptomyces have been reported to be significantly lower thanthose observed in E. coli (45, 54) might be in agreement withthe latter hypothesis. In addition, its closer similarity to SpoTrather than to RelA within its N terminus might reflect the factthat S. coelicolor Rel and SpoT share some common features withinthe proposed (p)ppGpp-synthesizing domain. Such a view is supportedby reports of weak (p)ppGpp synthetase activity of SpoT (17).

Interestingly, relA restores actinorhodine production in the S. coelicolor rel-deleted 18J strain, in the same way as a nativerel gene does. Moreover, relC mutants of Streptomyces have beenrecently characterized (23, 44). These mutants showed a deficiencyin antibiotic production and a defective ribosomal (p)ppGpp synthesis(23, 42-44), which were restored by introducing the rplK (= relC)gene in trans (23, 44). In E. coli, a functional 50S ribosomalprotein, L11, encoded by the relC gene has been shown to be requiredfor the activation of the RelA protein and, consequently, forthe synthesis of (p)ppGpp (6). Although additional work isrequired, these observations provide support for the proposedsignificance of (p)ppGpp in the onset of antibiotic productionin Streptomyces (24, 39-43). It is remarkable that RelA, unlikeS. coelicolor Rel, is apparently completely devoid of (p)ppGppaseactivity (6); a stable S. coelicolor strain, 18J, transformedwith relA indicates that an additional gene for (p)ppGppase activitymay exist in Streptomyces or that the activity might result fromnonspecific (p)ppGpp degradation by other nucleotidases. Thesefeatures are of particular interest and are currently being investigated.

In Streptomyces, a more distantly related isofunctional gene for (p)ppGpp synthesis has been reported (22), providing additionalopportunities for functional specialization and the incorporationof independent regulatory mechanisms associated with specificmetabolic roles. For that reason, definition of the catalyticproperties of S. coelicolor Rel, particularly those responsiblefor regulating its activity, and mutational analysis constitutea useful tool for analyzing Rel's role in Streptomyces (p)ppGppmetabolism. Studies combining these methods are in progress.

	ACKNOWLEDGMENTS

We thank M. Cashel for providing pGG21 plasmid and E. coli relA spoT mutants and gratefully acknowledge his recommendationsfor handling E. coli CF1693. We also thank D. J. MacNeil for thegift of E. coli ET12567, M. Bibb and J. Sun for making availablepIJ8600 before publication, and D. Holmes for critical readingof the manuscript.

This work was supported by grants from the Spanish Comisión Interministerial de Ciencia y Tecnología (95-0101-0P-02-01)and SmithKline Beecham S.A.

	FOOTNOTES

^* Corresponding author. Mailing address: Centro Nacional de Biotecnología, CSIC, Campus Universidad Autónoma de Madrid, Cantoblanco,28049-Madrid, Spain. Phone: 34-91-5854548. Fax: 34-91-5854506.E-mail: fmalpart{at}cnb.uam.es.

Present address: Departamento de Bioquímica, Facultad de Medicina, UAM, and Instituto de Investigaciones Biomédicas, 28049-Madrid,Spain.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
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Gomez-Escribano, J. P., Martin, J. F., Hesketh, A., Bibb, M. J., Liras, P. (2008). Streptomyces clavuligerus relA-null mutants overproduce clavulanic acid and cephamycin C: negative regulation of secondary metabolism by (p)ppGpp. Microbiology 154: 744-755 [Abstract] [Full Text]
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