Role of Alternative sigma  Factor AlgU in Encystment of Azotobacter vinelandii

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J Bacteriol, May 1998, p. 2766-2769, Vol. 180, No. 10
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Role of Alternative $sigma$ Factor AlgU in Encystment of Azotobacter vinelandii

Soledad Moreno, Rebeca Nájera, Josefina Guzmán, Gloria Soberón-Chávez, and Guadalupe Espín^*

Departamento de Microbiología Molecular, Instituto de Biotecnología, Universidad Nacional Autónoma de México, Cuernavaca, Morelos 62250, México

Received 23 October 1997/Accepted 5 March 1998

	ABSTRACT

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Alginate is essential for encystment in Azotobacter vinelandii. Transcription of the algD gene, which codes for GDP-mannosedehydrogenase, a key enzyme in the alginate biosynthetic pathway,is initiated at two promoters, one of which, p2, has $sigma$ ^E consensus sequences. AlgU is the A. vinelandii alternative $sigma$ ^E factor. In this study, we constructed an algU mutant (SMU88)which, as expected, is impaired in alginate production, encystment,and transcription of the algD gene from the p2 promoter. PlasmidpJMSAT1, carrying the A. vinelandii algU gene, restored alginateproduction and encystment to SMU88 and to strain UW136, a naturallyoccurring algU mutant. Plasmid pSMU865, carrying the A. vinelandiimucABCD genes coding for negative regulators of AlgU activityand previously shown to diminish alginate production in the wild-typestrain, ATCC 9046, was shown here to impair encystment and transcriptionof the algD gene from the p2 algU-dependent promoter. Since nonencystingstrain ATCC 9046/pSMU865 produced more alginate than some encystingstrains, such as UW136/pJMSAT1, we propose an AlgU role in encystment,independent of the structural role that alginate plays in maturecysts.

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Encystment in Azotobacter vinelandii has been studied at the morphological and biochemical levels (9, 10, 22, 27).This differentiation process is induced by growth on n-butanolas the sole carbon source (12); mature cysts develop in 3 to5 days and are characterized by a central body surrounded by anintine and a thick, laminated exine. Alginate is essential forencystment since it is a component of intine and exine layers(1, 3). The alginate biosynthetic pathways of A. vinelandiiand Pseudomonas aeruginosa are very similar (21). The moleculargenetics of alginate biosynthesis have been widely studied inP. aeruginosa (for reviews, see references 5 and 17), wherethe genes encoding the alginate biosynthetic enzymes are organizedin an operon starting with algD (4), encoding a GDP-mannosedehydrogenase, which converts GDP-mannose to GDP-mannuronic acid,the substrate for alginate polymerization. The algU mucABCD clustercontrols alginate production. AlgU (also known as AlgT) is a $sigma$ ^E homolog (8); it is required for transcription of algD andits own gene, algU (15, 25). The mucA and mucB genes codefor negative regulators of AlgU activity; MucA interacts withAlgU as an anti-sigma factor, inhibiting its activity (6, 24,25, 28).

The A. vinelandii alginate biosynthetic gene cluster is organized in at least three operons, one of which includes the algDgene (3, 13, 18). In the highly mucoid strain A. vinelandiiATCC 9046, algD is transcribed from two promoters: a putativeAlgU dependent promoter, p2, and a promoter (p1) showing consensussequences for the vegetative sigma factor $sigma$ ^D (3). We identified and sequenced the algU and mucABCD genesof A. vinelandii and presented evidence showing that they controlalginate biosynthesis in a manner similar to that of the P. aeruginosahomologs (16).

An A. vinelandii strain unable to produce alginate due to a mutation in the algD gene is unable to encyst (3). The naturallyoccurring A. vinelandii strain UW136 does not produce alginate,due to a mutation in the algU gene, which codes for the AlgU sigmafactor (16), and is also unable to encyst (20). The questionof whether algU mutations affect encystment exclusively via itseffect on alginate biosynthesis or whether AlgU activity is alsorequired for expression of other genes involved in cyst formationwas raised. In the present work we present evidence suggestingthat AlgU is involved in the formation of mature cysts, independentlyof its role in alginate production.

Construction and characterization of an ATCC 9046 algU mutant. To study the role of AlgU in encystment, we constructed an ATCC 9046 derivative carrying an algU::Km null mutation. A PstIDNA fragment of 828 nucleotides corresponding to algU from A.vinelandii ATCC 9046 (Fig. 1) was cloned into plasmid pBluescriptII KS to give pSMU85. A 2-kb SmaI fragment containing a kanamycinresistance gene from plasmid pHP45 $Omega$ -Km (7) was inserted intothe unique EcoRV site present within the 828-bp fragment of pMSU85to create an algU::Km mutation between the codons for amino acidresidues 115 and 116 of AlgU. The resultant plasmid, pSMU88, whichis unable to replicate in A. vinelandii, was introduced into strainATCC 9046 by transformation. One of the kanamycin-resistant transformants,strain SMU88, was chosen for further analysis. The replacementof the intact algU gene with the algU::Km mutation on the chromosomeof the SMU88 mutant was confirmed by Southern blotting (Fig. 1).The algU mutation impaired alginate production and encystment(Table 1). To complement the algU mutation, a 1.6-kb DNA fragmentwith the algU-mucA region from ATCC 9046, obtained by PCR, wascloned into plasmid pCRII, which confers ampicillin resistance(2). The resultant plasmid, pJMSAT1, which is unable to replicatein A. vinelandii, was transformed into algU mutant strain SMU88.A transformant, SMU88::pJMSAT1, carrying plasmid pJMSAT1 integratedinto the chromosome, was selected as a mucoid colony resistantto carbenicillin. Integration of the plasmid was confirmed bySouthern blot analysis (data not shown). Strain SMU88::pJMSAT1was able to encyst (Table 1). We also show that plasmid pDMUM13carrying the P. aeruginosa algU gene (14), previously shownto restore alginate production to strain UW136 (16), also restoredencystment and alginate production to strains SMU88 and UW136(Table 1). Although the amounts of alginate synthesized by strainsSMU88, UW136 complemented with plasmid pDMUM13, and UW136::pJMSAT1were significantly lower than that of ATCC 9046, they were sufficientfor encystment (Table 1).

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FIG. 1. Construction of strain SMU88. (A) Schematic representation of the A. vinelandii algU region and the algU::Km mutation in plasmid pSMU88. Bar, 100 bp. (B) Southern blot hybridization of total genomic DNA digested with PstI endonuclease, with pSMU85 as a probe. Lanes: 1, ATCC 9046; 2, SMU88. Molecular sizes (in kilobases) are indicated on the right.

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TABLE 1. Alginate production and encystment^a

Effects of plasmid pSMU865 and the algU::Km mutation on transcription from the algD p1 and p2 promoters. Plasmid pSMU865, carrying the A. vinelandii mucABCD genes, was previously shown to reduce alginate production in strain ATCC9046 (16). We propose that the effect of pSMU865 on alginateproduction in ATCC 9046 is due to the negative effect of the mucAand mucB gene products on AlgU activity and therefore on transcriptionfrom algDp₂. Thus, transcription of the algD gene in strains ATCC9046/pSMU865 and SMU88 should initiate predominantly from p1,the AlgU-independent promoter. Primer extension experiments wereperformed on RNA isolated from strains SMU88 and ATCC 9046 inthe presence and absence of plasmid pSMU865 and grown in liquidBS medium (11) for 48 h at 30°C. Reactions were performed witha primer extension system (Boehringer), as instructed by the manufacturer.Oligonucleotide primers used were labeled with [ $gamma$ -³²P]dATP (Amersham) at the 5' end by using polynucleotide kinaseand were hybridized to 50 µg of total RNA. After extension withreverse transcriptase, cDNA products were examined by electrophoresisin an 8% polyacrylamide gel. To map transcriptional start points,sequencing reactions were performed on pMSD27 (16) DNA by thedideoxy chain termination method (23) with [ $gamma$ -³²P]dATP and a sequencing kit with the same primers as used forthe primer extension reactions.

As expected, primer extension products corresponding to p1 and p2 transcripts were observed with ATCC 9046 RNA, but only theprimer extension products corresponding to p1 transcripts wereobserved with RNA from strains SMU88 and ATCC 9046/pSMU865, confirmingthat p2 is an AlgU-dependent promoter (Fig. 2).

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FIG. 2. Primer extension analysis of algD transcription in strains SMU88 and ATCC 9046, with and without plasmid pSMU865. (A) DNA sequence of the 5' end of algD. The arrows indicate the start sites of algD transcription, the p1 and p2 promoters are indicated (overbar), and the complementary sequences where oligonucleotides algD1 and algD2 (used for primer extension analysis) were generated are underlined. The algD ATG initiation codon is shown in boldface type. (B and C) Primer extension of the algD gene with oligonucleotide algD1 in strains SMU88 (lane 1) and ATCC 9046 with (lane 2) and without (lane 3) plasmid pSMU865 (B) and with oligonucleotide algD2 in strain SMU88 (C). The algD sequence ladders (GATC) were produced with the oligonucleotides used for primer extension.

In P. aeruginosa, algU mutants are unable to produce alginate, since transcription of the biosynthetic operon starting withalgD, as well as some regulatory genes such as algR, is dependenton the presence of an active AlgU sigma factor (15, 26). Similarly,A. vinelandii algU mutants UW136 and SMU88 are also unable toproduce alginate; in contrast to P. aeruginosa, however, in A.vinelandii transcription of all other known alginate biosyntheticgenes, such as algA and alg8, is not dependent on AlgU (13,18). As shown here, AlgU is absolutely required for transcriptionfrom algDp₂, but algD is still transcribed from algDp₁ in strainATCC 9046. Transcription from algDp₁ was also detected in strainSMU88, with an oligonucleotide corresponding to the nucleotidescoding for amino acids 37 to 44 of AlgD (Fig. 2), indicating thattranscription from p1 extends into the algD structural gene. Thus,the fact that an algU mutation abolished alginate production inthis strain indicates that in A. vinelandii, transcription ofother unidentified regulatory or biosynthetic alginate genes dependson AlgU.

Effect of plasmid pSMU865 on encystment. We studied encystment in strain ATCC 9046/pSMU865, which produces alginate even though its AlgU activity is not sufficientto initiate transcription from algDp₂. Table 1 shows that thisstrain was unable to form desiccation-resistant cysts, despitethe fact that under encysting conditions it produced more alginatethan the encysting strains UW136::pJMSAT1, SMU88/pDMUM13, andUW136/pDMUM13. These data strongly suggest that AlgU plays anadditional role in the expression of genes involved in cyst formation.The observation that an algU mutation, but not plasmid pSMU865,abrogated alginate production in strain ATCC 9046 leads us tohypothesize that in strain ATCC 9046/pSMU865, a low level of AlgUactivity allows some transcription of the unidentified alginategenes mentioned above but not of algD (from p2) and encystmentgenes.

The putative AlgU requirement for transcription of genes involved in encystment may allow the identification and characterizationof such genes.

Ultrastructure analysis of cyst formation. Electron microscopic examination of the cyst structures formed by the mutant strains (Fig. 3) showed that strain SMU88 lacksthe intine and exine layers of mature cysts such as those producedby the wild-type strain, ATCC 9046. SMU88/pDMUM13 cysts were similarto those produced by wild-type strain ATCC 9046, consisting ofthe compacted cell (central body containing poly- $beta$ -hydroxybutyrategranules) surrounded by the intine capsule and the exine outershell. The cyst structures formed by strain ATCC 9046/pSMU865(Fig. 3D) appear to lack the intine layers. An early electronmicroscopy study of the development of A. vinelandii cysts (27)revealed that the exine appears in 36 to 48 h, after which theexine thickens and the intine is formed between the exine andthe central body; thus, at 36 h the intine appears to be nothingbut an empty area. This seems to be the stage at which encystmentdevelopment is blocked in the absence of AlgU activity.

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FIG. 3. Electron micrographs were produced as described previously (19). Thin sections of A. vinelandii cysts formed by strains SMU88 (A), SMU88/pDMUM13 (B), ATCC 9046 (C), and ATCC 9046/pSMU865 (D) are shown. Abbreviations: EX, exine; IN, intine; CB, central body; PHB, poly- $beta$ -hydroxybutyrate. Bars, 0.4 µm.

This study contributes to our understanding of the A. vinelandii differentiation process leading to cyst formation at themolecular level and is the first example of the involvement ofan alternative sigma factor in cellular differentiation of a gram-negativebacterium.

	ACKNOWLEDGMENTS

This work was supported by grant IN212096 from DGAPA UNAM.

We thank L. Servin, F. Bastarrachea, and S. Silver for reviewing the manuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Departamento de Microbiología Molecular, Instituto de Biotecnología, UniversidadNacional Autónoma de México, Apdo. postal 510-3, Cuernavaca,Morelos 62250, México. Phone: (52) (73) 291644. Fax: (52) (73)172388. E-mail: espin{at}ibt.unam.mx.

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1.	Brivonese, A. C., and I. W. Sutherland. 1989. Polymer production by a mucoid strain of Azotobacter vinelandii in batch culture. Appl. Microbiol. Biotechnol. 30:97-102.
2.	Brosius, J. 1989. Superpolylinkers in cloning and expression vectors. DNA 8:759-777[Medline].
3.	Campos, M.-E., J. M. Martínez-Salazar, L. Lloret, S. Moreno, C. Núñez, G. Espín, and G. Soberón-Chávez. 1996. Characterization of the gene coding for GDP-mannose dehydrogenase (algD) from Azotobacter vinelandii. J. Bacteriol. 178:1793-1799[Abstract/Free Full Text].
4.	Chitnis, C. E., and D. E. Ohman. 1993. Genetic analysis of the alginate biosynthetic gene cluster of Pseudomonas aeruginosa shows evidence of an operonic structure. Mol. Microbiol. 8:583-590[Medline].
5.	Deretic, V., D. W. Martin, M. J. Schurr, M. H. Mudd, N. S. Hibler, R. Curcic, and J. C. Boucher. 1993. Regulation of mucoidy in Pseudomonas aeruginosa. Bio/Technology 11:1133-1136[Medline].
6.	Deretic, V., M. J. Schurr, J. C. Boucher, and D. W. Martin. 1994. Conversion of Pseudomonas aeruginosa to mucoidy in cystic fibrosis: environmental stress and regulation of bacterial virulence by alternative sigma factors. J. Bacteriol. 176:2773-2780[Free Full Text].
7.	Fellay, R., J. Frey, and H. Krisch. 1987. Interposon mutagenesis of soil and water bacteria: a family of DNA fragments designed for in vitro insertional mutagenesis of Gram-negative bacteria. Gene 52:147-154[Medline].
8.	Hershberger, C. D., R. W. Ye, M. R. Parsek, Z. D. Xie, and A. M. Chakrabarty. 1995. The algT (algU) gene of Pseudomonas aeruginosa, a key regulator involved in alginate biosynthesis, encodes an alternative $sigma$ factor ( $sigma$ ^E). Proc. Natl. Acad. Sci. USA 92:7941-7945[Abstract/Free Full Text].
9.	Hitchins, V. M., and H. L. Sadoff. 1970. Morphogenesis of cysts in Azotobacter vinelandii. J. Bacteriol. 104:492-498[Abstract/Free Full Text].
10.	Hitchins, V. M., and H. L. Sadoff. 1973. Sequential metabolic events during encystment of Azotobacter vinelandii. J. Bacteriol. 113:1273-1279[Abstract/Free Full Text].
11.	Kennedy, C., R. Gamal, R. Hummphrey, J. Ramos, K. Brigle, and D. Dean. 1986. The nifH, nifM and nifN genes of Azotobacter vinelandii: characterization by Tn5 mutagenesis and isolation from pLARF1 gene banks. Mol. Gen. Genet. 205:318-325.
12.	Lin, L. P., and H. L. Sadoff. 1968. Encystment and polymer production by Azotobacter vinelandii in the presence of $beta$ -hydroxybutyrate. J. Bacteriol. 98:1335-1341.
13.	Lloret, L., R. Barreto, R. León, S. Moreno, J. Martínez-Salazar, G. Espín, and G. Soberón-Chávez. 1996. Genetic analysis of the transcriptional arrangement of Azotobacter vinelandii alginate biosynthetic genes: identification of two independent promoters. Mol. Microbiol. 21:449-457[Medline].
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Role of Alternative Factor AlgU in Encystment of Azotobacter vinelandii

Role of Alternative $sigma$ Factor AlgU in Encystment of Azotobacter vinelandii