Biochemical and Genetic Evidence for Participation of DevR in a Phosphorelay Signal Transduction Pathway Essential for Heterocyst Maturation in Nostoc punctiforme ATCC 29133

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Journal of Bacteriology, July 1999, p. 4430-4434, Vol. 181, No. 14
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Biochemical and Genetic Evidence for Participation of DevR in a Phosphorelay Signal Transduction Pathway Essential for Heterocyst Maturation in Nostoc punctiforme ATCC 29133

Kari D. Hagen and John C. Meeks^*

Section of Microbiology, Division of Biological Sciences, University of California, Davis, California 95616

Received 23 February 1999/Accepted 11 May 1999

	ABSTRACT

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In a test of the hypothesis that DevR is a response regulator protein that functions in a phosphorelay signal transductionsystem involved in heterocyst development in Nostoc punctiformeATCC 29133, purified affinity-tagged DevR was shown to be phosphorylatedin vitro by the noncognate sensor kinase EnvZ. Site-directed mutagenesiswas used to generate N. punctiforme mutants with single aminoacid substitutions at the putative phosphorylation site of DevR.These mutants exhibited a Fox phenotype like the original devR insertion mutant UCD 311, consistentwith a phosphotransferase role forDevR.

	TEXT

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When limited for combined nitrogen, certain filamentous cyanobacteria, including Nostoc punctiforme ATCC 29133, respond byinitiating a developmental program that results in the productionof terminally differentiated nitrogen-fixing cells known as heterocysts.These specialized cells occur as 3 to 10% of the total cell populationand are typically found singly at regular intervals along thefilaments. Mature heterocysts differ from the vegetative cellsfrom which they arise in several ways that reflect their rolein providing a micro-oxic environment for the oxygen-sensitiveenzyme nitrogenase (30): they lack the oxygen-producing reactionsof photosystem II, they have a high rate of respiratory oxygenuptake, and they have a unique envelope consisting of an innerglycolipid layer and an outer polysaccharide layer that is locatedoutside the cell wall. This envelope is thought to impede thediffusion of oxygen into the cell while allowing the entry ofsufficient dinitrogen for nitrogen fixation (28, 30).

Several genes that are involved in the differentiation of heterocysts have been identified and cloned. The proteins encodedby these genes include some that are required for the initiationof heterocyst differentiation, such as NtcA, a global nitrogen-regulatoryprotein (13, 29), and HetR, an autoregulated serine-type proteasethat accumulates in cells destined to become heterocysts and whosesynthesis is enhanced within 3 h after deprivation for combinednitrogen (2, 4, 31). Genes that are essential in the laterstages of heterocyst development have also been identified. Thesegenes include those that are required for the formation of a mature,functional heterocyst envelope, such as devBCA (12), hglK (1),and hglE (5), which are involved in the production and assemblyof the glycolipid layer, and hepK (11) and hepA (17), whichare required for the synthesis of envelope polysaccharide (32).

Two-component signal transduction systems play an essential role in the regulation of complex developmental programs in manyeubacteria; in filamentous cyanobacteria, three genes with similarityto members of two-component regulatory systems are known to influenceheterocyst development. We previously identified a gene in N.punctiforme 29133, designated devR, that is required for heterocystmaturation (6). Strain UCD 311, a devR insertion mutant, synthesizesheterocyst glycolipids but makes a defective heterocyst envelopesuch that nitrogen fixation occurs only in the absence of oxygen(Fox). The 135-amino-acid protein encoded by devR is similar to thewell-characterized response regulators CheY (25), Spo0F (16),and DivK (21), which lack C-terminal effector domains. DevRdiffers structurally from other response regulators (27) inhaving 7 additional amino acids in the highly conserved $gamma$ -turnloop region adjacent to the site of phosphorylation (Fig. 1).

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FIG. 1. Comparison of DevR to CheY and to other response regulators. (A) Alignment of amino acid residues near the site of phosphorylation (aspartate-53 of DevR; arrow). Numbering of residues of DevR is shown. DevR, N. punctiforme; DivK, Caulobacter crescentus; Spo0F, Bacillus subtilis; NtrC, E. coli; CheY, Salmonella typhimurium; OmpR, E. coli. (B) Ribbon diagrams of CheY (residues 2 to 129) and DevR (residues 1 to 119). The $gamma$ turn of CheY and additional amino acids in DevR are indicated, as is the site of phosphorylation in each protein. The PILEUP program of the Wisconsin Genetics Computer Group (10) was used to generate sequence alignments. Models of CheY and DevR were prepared with SWISS-MODEL and Swiss-PdbViewer (14).

The other two genes involved in heterocyst differentiation that are similar to members of two-component regulatory systemswere identified in Anabaena sp. strain PCC 7120. One of these,patA, is a response regulator analog required for the positioningof heterocysts within the filaments (22). When patA is inactivated,heterocysts are found mainly at the ends of the filaments, ratherthan being intercalary. The other gene, hepK, mentioned aboveis similar to those encoding histidine kinases (32). Inactivationof hepK in Anabaena strain PCC 7120 results in a Fox phenotype (11), as does the inactivation of devR in the N.punctiforme mutant strain UCD311.

In this study, we have used biochemical and genetic approaches to further characterize DevR from N. punctiforme 29133. Weshow that DevR is phosphorylated in vitro and provide additionalevidence for the role of this protein as a response regulatorin a phosphorelay system that controls heterocystmaturation.

Sequence analysis of the chromosomal region containing devR. The sequence of 3.7 kb of DNA adjacent to devR was analyzed to identify genes encoding proteins that might interact with DevR.Three additional open reading frames (designated gyrA, tprN, andregN) were identified; however, none was found to be homologousto genes encoding histidine kinases, response regulators, or otherproteins known to interact with components of signal transductionpathways.

In vitro phosphorylation of DevR and stability of DevR-P. His-tagged versions of DevR were prepared with the pET system of Novagen. His-DevR was made by PCR with primers 5'-ATGAAAACTGTTTTAATTGTCGAAGAC-3'(upstream) and 5'-CGCGAAGCTTTTATGATTGGCCGTCTGTGG-3' (downstream)and pSCR166 as the template (Table 1). The downstream primercontained a HindIII site to facilitate directional cloning ofthe fragment into the expression vector. After digestion withHindIII, the 420-bp fragment containing devR was ligated intothe Ecl136II and HindIII sites of pET-28a(+) to generate pSCR342.Primer-mediated PCR mutagenesis (15) was used to generate asequence encoding His-DevR $Delta$ 7, which has a 7-amino-acid deletionin the $gamma$ -turn loop region (residues 57 to 63 of DevR [Fig. 1]).Codon 56 was changed from CTG to TTA to introduce a DraI sitewhich was used for screening purposes. Left and right overlappingproducts, each containing the desired deletion, were first generatedin separate reactions with pSCR166 as the template. The insideprimers used were 5'-GATTCCATCAACAGATTTTAAAGAAACATCCAT TAAAATCAGGTC-3'(left) and 5'-CTGATT TTAATGGATGT TTCT TTAAAATCTGT TGATGGAATC-3'(right), while the outside primers were those used to generatethe 420-bp devR fragment above. The left and right PCR productsserved together as the template in a final reaction with onlythe outside primers. This amplification yielded a 399-bp fragment,reflecting the 21-bp deletion. It was digested with HindIII andcloned into pET-28a(+) as described above to generate pSCR343.Each fusion protein was expressed in Escherichia coli BL21(DE3)and purified by affinity chromatography according to the manufacturer'sinstructions.

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TABLE 1. Bacterial strains and plasmids

Cross talk between purified histidine kinases and response regulators from different two-component regulatory systems canoccur in vitro (18, 23); therefore, we used EnvZ, a histidinekinase involved in osmoregulation in E. coli, to demonstrate thatDevR can be phosphorylated (Fig. 2). The purified proteins usedin the phosphorylation reactions are shown in Fig. 2A. A standardphosphorylation reaction mixture contained 50 mM Tris-Cl (pH 8.0),50 mM KCl, 10 mM MgCl₂, 1 mM dithiothreitol, 0.1 mM EDTA, and0.1 µM [ $gamma$ -³²P]ATP (6,000 Ci mmol¹; Du Pont NEN). Maltose binding protein (MBP)-EnvZ was added toa final concentration of 1.0 µM, and the mixture was allowed toincubate for 5 min at room temperature. OmpR (20 µM) or His-DevR(35 µM) was then added. Aliquots (7.5 µl) were withdrawn intoan equal volume of double-strength sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) sample buffer at various intervalsafter addition of the response regulator. All samples were kepton ice and were not heated prior to electrophoresis on 15% acrylamidedenaturing protein gels. His-DevR was phosphorylated in the presenceof MBP-EnvZ and [ $gamma$ -³²P]ATP (Fig. 2B, lanes 3 to 7) but not in the presence of [ $gamma$ -³²P]ATP alone (lane 8). As has been noted previously for phosphotransferbetween nonpartner proteins (18, 23), phosphotransfer fromEnvZ to DevR occurred more slowly and less efficiently than didthe transfer of phosphate from EnvZ to its cognate response regulatorOmpR (lane 2).

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FIG. 2. Phosphorylation of His-DevR and OmpR by MBP-EnvZ. (A) Coomassie blue-stained SDS-PAGE gel (15% acrylamide) of purified proteins used in phosphorylation assays. Lane 1, MBP-EnvZ; lane 2, OmpR; lane 3, His-DevR. (B) Autoradiogram of SDS-PAGE gel showing phosphorylation of His-DevR. MBP-EnvZ was autophosphorylated when incubated in the presence of [ $gamma$ -³²P]ATP for 5 min (lane 1) or 60 min (lane 9). After a 5-min incubation of MBP-EnvZ with [ $gamma$ -³²P]ATP (lanes 2 to 7), OmpR or His-DevR was added. Samples were removed 5 min (OmpR; lane 2) or 1, 5, 15, 30, or 60 min (His-DevR; lanes 3 to 7, respectively) after the addition of the response regulator. In lane 8, His-DevR and [ $gamma$ -³²P]ATP were incubated for 60 min in the absence of MBP-EnvZ.

To assess the stability of phosphorylated DevR, the phosphorylation reaction described above was allowed to proceed for 60min after the addition of His-DevR. Excess unlabeled ATP (5 mM)was added to render the assay insensitive to subsequent EnvZ kinaseactivity, and small aliquots were again removed and electrophoresed.Quantitation of radiolabeled bands was performed with a StormPhosphorImager with ImageQuant software (Molecular Dynamics).Once phosphorylated, DevR-P appeared to be relatively stable;the amount of DevR-³²P decreased exponentially with time with an apparent first-orderrate constant of 0.004 to 0.005 min¹, corresponding to a half-life of 2 to 3 h at roomtemperature.

The fact that an MBP-DevR that we originally purified could not be phosphorylated by MBP-EnvZ implies that the contributionof the affinity tag to the conformation of the fusion proteinis critical to its activity. We also considered that the extensionof the $gamma$ -turn loop in DevR (Fig. 1) might hinder its phosphorylationby heterologous histidine kinases and contribute to the specificityof the cognate histidine kinase. However, MBP-EnvZ failed to phosphorylateHis-DevR $Delta$ 7 (data not shown) while phosphorylating His-DevR, implyingthat this region is essential to the conformation of the receiverdomain. It remains possible that this loop is involved in recognitionof the other substrates with which DevR-Pinteracts.

Identification of hepK in N. punctiforme 29133 and construction of a hepK mutant strain. Since mutations in hepK of Anabaena strain PCC 7120 (11) yield a Fox phenotype, similar to that of devR in N. punctiforme (6),it is possible that HepK is the cognate sensor histidine kinasefor DevR. Using the hepK gene from Anabaena strain PCC 7120 asa probe, we identified the N. punctiforme hepK gene in a cosmidlibrary of N. punctiforme 29133 genomic DNA (9). The alignednucleotide sequences of the two genes are 75% similar, while thetranslated amino acid sequences are 83% similar (77% identical).An insertion mutation was introduced into N. punctiforme 29133hepK by ligation of an $Omega$ -npt antibiotic resistance cassette conferringNm^r and Km^r (8) into a unique Eco47III site within the gene. A 5.2-kbEcoRV fragment containing the interrupted gene was cloned intothe Ecl136II site of the sacB-containing vector pRL271 (2)to generate pSCR179, and gene replacement was performed as describedpreviously (9). The N. punctiforme 29133 hepK mutant, strainUCD 460, also exhibited a Fox phenotype. Insoluble inclusion bodies formed when LacZ-HepK andHis-HepK fusion proteins were overexpressed in various E. colistrains. Although a soluble protein was produced when HepK lackingN-terminal membrane-spanning regions was fused to MBP, neitherthis protein nor the insoluble proteins described above were competentin autophosphorylation in our experiments (data not shown); thus,the potential for phosphotransfer from HepK to DevR could notbeassessed.

Characterization of N. punctiforme strains with mutations in devR. Single amino acid substitutions at the site of phosphorylation have been successfully employed to generate response regulatorproteins with altered functions. For certain response regulators(e.g., CheY), amino acid substitutions at the site of phosphorylationconsistently result in loss of function (3). For others, suchas NtrC (19) and OmpR (20), conversion of the amino acid residueat the site of phosphorylation from aspartate to asparagine (NtrC)or from aspartate to glutamine (OmpR) resulted in an inactiveprotein, but conversion of the same residue to glutamate resultedin a protein that was constitutively active in the absence ofphosphorylation. It is likely that the conformational change createdby the insertion of the larger, negatively charged glutamate residuemimics the change that normally occurs with phosphorylation, whilethe conversion of the carboxyl group of aspartate to an aminogroup simply prevents phosphorylation without inducing a conformationalchange.

We used a similar strategy to examine the role of phosphorylated DevR in N. punctiforme. PCR mutagenesis and gene replacementwere used to generate two N. punctiforme 29133 strains with differentmutations in the single chromosomal copy of devR. For each strain,the mutations resulted in a single amino acid substitution ataspartate-53, the putative phosphorylation site of DevR. SequentialPCRs were performed to introduce the necessary base changes atthe aspartate (D)-53 codon of devR and to generate a unique downstreamBglII site that was useful for screening purposes but did notalter the amino acid sequence of DevR. To construct strain UCD425, codon 53 of devR was changed from GAT to CAA (D to glutamine[Q]), while codon 59 was changed from AGT to TCT (BglII site).By using pSCR166 as the template with the primers 5'-CCTGCACTAACCTGACTAAGGCATCGT-3'(left outside), 5'-TGGTAAACAGATCTGGACAGAGAAACTTGCATT-3' (leftinside), 5'-TTAATGCAAGTTTCTCTGTCCAGATCTGTTTAC-3' (right inside),and 5'-TTATGATTGGCCGTCTGTGGGTAGAAG-3' (right outside), left andright overlapping PCR products were generated. These were usedas template in a final reaction with the two outside primers,which yielded a single 1,034-bp product that contained the desiredmutations in devR. Identical steps were taken to generate a similar1,034-bp PCR product that was used in the construction of strainUCD 436, in which codon 53 was changed from GAT to GAA (D to glutamate[E]) and the BglII site was again introduced. The outside primersused to construct strain UCD 436 were those used in the constructionof UCD 425, but the left and right inside primers were changedto 5' - TGG TAAACAGATC TGGACAGAGAAACTTCCAT T - 3' and 5'-TTAATGGAAGTTTCTCTGTCCAGATCTGTTTAC-3',respectively.

Each 1,034-bp PCR product was digested with EcoNI and StyI to obtain a 0.8-kb fragment that was used to replace the correspondingwild-type fragment in pSCR166, forming plasmids pSCR176 (devRD53Q)and pSCR180 (devRD53E). These plasmids were sequenced to confirmthat only the correct base changes had been made. The 3.15-kbXbaI fragments from pSCR176 and pSCR180 were cloned into the XbaIsite of the sacB-positive selection vector pRL278 (2) to generateplasmids pSCR178 and pSCR181, respectively, which were introducedinto N. punctiforme 29133 by conjugation as previously described(9). Cells were plated on medium containing neomycin to selectfor homologous recombination and integration of the plasmid. Nm^r exconjugants were cultured in neomycin-free liquid medium andthen plated on neomycin-free medium plus 5% sucrose to selectfor resolution of the plasmid integrate. Because there was nopositive selection for clones that retained the copy of devR bearingthe mutations, the following screening method was used to distinguishsuch clones from those that retained a wild-type copy of the gene.Large single N. punctiforme colonies (containing approximately6 × 10⁶ cells) were taken from plates, suspended in 0.2 ml of 10 mM Tris-Cl-1mM EDTA-1% Triton X-100 (pH 8.0), and lysed by heating for 2 minat 95°C. The lysis mixture was then extracted twice with 0.2 mlof chloroform. Aliquots (10 µl) of the aqueous phase, which containedgenomic DNA, were used for PCR amplifications with primers designedfor sequencing of the devR region. The resulting 1.85-kb PCR productwas digested with BglII, and the fragments were separated by electrophoresis.The PCR product from colonies carrying only a mutated copy ofdevR was cut once by BglII, generating two fragments of 1.1 and0.75 kb, while the product from colonies with only a wild-typecopy of devR lacked the BglII site and was not digested. All threefragments were detected after BglII digestion of the PCR productfrom Nm^r exconjugants containing both a wild-type and a mutated copy ofdevR.

In strain UCD 425, codon 53 of devR was changed to CAA, encoding glutamine; thus phosphorylation at the active site of themutant protein, DevRD53Q, should no longer be possible. To confirmthis, we generated devRD53Q by PCR, with pSCR176 as the templatewith the same primers used in amplification of wild-type devR.The product was then cloned into pET-28a(+) as described above.Purified His-DevRD53Q was not detectably phosphorylated by MBP-EnvZ(data not shown). Moreover, the phenotype of strain UCD 425 waslike that of the devR insertion mutant strain UCD 311; strainUCD 425 grew normally in the presence of combined nitrogen butbegan to bleach within 24 h after deprivation for combined nitrogenand eventually fragmented into single cells or short (two- tothree-cell) filaments. At 48 h, acetylene reduction rates, measuredas described previously (7), were essentially zero under oxicconditions but were similar to those for strain UCD 311 underanoxic conditions. As with strain UCD 311, light microscopy showedthe accumulation of refractive material at the heterocyst polesand what appeared to be detached outer envelope material at someheterocyst-vegetative cell junctions (Fig. 3). Strain UCD 436,the devRD53E mutant, was morphologically indistinguishable fromstrain UCD 425 and also expressed a Fox phenotype with acetylene reduction rates of zero in air.

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FIG. 3. Photomicrographs of N. punctiforme strains taken 48 to 72 h after deprivation for combined nitrogen. (A) N. punctiforme 29133. (B) Strain UCD 311. (C) Strain UCD 436. In contrast to wild-type N. punctiforme 29133, the mutants differentiate heterocysts (indicated with arrows) with large amounts of refractive material at the cell poles. Some heterocysts also appear to have a detached wall layer. Strains UCD 425 (devRD53Q; not shown) and UCD 436 (devRD53E) are morphologically indistinguishable from one another and appear to be phenotypically identical to strain UCD 311, the devR insertion mutant. Bar = 5 µm.

Strain UCD 459 was constructed by introducing devRD53E into wild-type N. punctiforme 29133 on a multicopy plasmid, pSCR187.Overproduction of DevRD53E was confirmed by Western blotting (datanot shown). Strain UCD 459 grew in air in the absence of combinednitrogen and differentiated normal-appearing heterocysts. In contrastwith our previous results with wild-type DevR (6), overproductionof DevRD53E did not result in the atypical production of heterocysts,akinetes, or hormogonia in ammonium-supplementedmedium.

Two different roles are possible for response regulators such as DevR, which lack C-terminal effector domains. Upon phosphorylation,conformational changes that allow the response regulator to interactdirectly with a downstream target and elicit a response couldoccur. Alternatively, the response regulator might act only asa phosphotransferase intermediate in a multicomponent phosphorelay.If DevR-P interacts in a direct manner with its downstream targetand the substitution of glutamate for aspartate-53 mimics theconformational changes that occur with phosphorylation, the devRD53Emutation could result in a DevR-P constitutive phenotype, whichis expected to be similar to that of the wild type. Moreover,overexpression of DevRD53E might result in an aberrant phenotype,such as the atypical akinete production which occurred when wild-typeDevR was overexpressed in N. punctiforme 29133 (6). Neitherof these phenotypes was observed. If, however, the role of DevRis to act as an intermediate in a phosphorelay system, any aminoacid substitution at aspartate-53 (including the substitutionof glutamate for aspartate) that prevents phosphorylation andfurther phosphotransfer would be expected to give rise to theFox phenotype exhibited by the transposon-induced mutant UCD 311.In this case, overexpression of the nonfunctional DevRD53E inwild-type N. punctiforme 29133 would be expected to have littleor no effect. The results we obtained with strains UCD 425, UCD436, and UCD 459 clearly demonstrate that aspartate-53 is requiredfor the normal function of DevR and are consistent with the latterhypothesis that the ability of DevR to act as a phosphotransferaseis essential to its role in heterocystmaturation.

Nucleotide sequence accession numbers. The nucleotide sequences of N. punctiforme hepK and of the complete open reading frames in the devR region are available fromthe National Center for Biotechnology Information under accessionno. L44605 (devR), AF117151 (tprN), AF116873 (regN),and AF114442 (hepK).

	ACKNOWLEDGMENTS

We thank M. Igo (University of California, Davis) for the generous gift of purified MBP-EnvZ and OmpR proteins, and C. P.Wolk (Michigan State University) for kindly providing the Anabaenastrain PCC 7120 hepK gene. We also thank E. L. Campbell and F.Wong for critical reading of themanuscript.

This work was supported by the U.S. National Science Foundation (grant IBN 95-14787).

	FOOTNOTES

^* Corresponding author. Mailing address: Section of Microbiology, Division of Biological Sciences, University of California,Davis, CA 95616. Phone: (530) 752-3346. Fax: (530) 752-9014. E-mail:jcmeeks{at}ucdavis.edu.

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31. Zhou, R., X. Wei, N. Jiang, H. Li, Y. Dong, K. L. Hsi, and J. Zhao. 1998. Evidence that HetR protein is an unusual serine-type protease. Proc. Natl. Acad. Sci. USA 95:4959-4963[Abstract/Free Full Text].

32. Zhu, J., R. Kong, and C. P. Wolk. 1998. Regulation of hepA of Anabaena sp. strain PCC 7120 by elements 5' from the gene and by hepK. J. Bacteriol. 180:4233-4242[Abstract/Free Full Text].

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