FlbT Couples Flagellum Assembly to Gene Expression in Caulobacter crescentus

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Journal of Bacteriology, October 1999, p. 6160-6170, Vol. 181, No. 19
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

FlbT Couples Flagellum Assembly to Gene Expression in Caulobacter crescentus

Erin K. Mangan,¹^, Jaleh Malakooti,² Anthony Caballero,² Paul Anderson,¹ Bert Ely,² and James W. Gober¹^,^*

Department of Chemistry and Biochemistry and Molecular Biology Institute, University of California $---$ Los Angeles, Los Angeles, California 90095-1569,¹ and Department of Biological Sciences, University of South Carolina, Columbia, South Carolina 29208²

Received 27 April 1999/Accepted 22 July 1999

	ABSTRACT

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The biogenesis of the polar flagellum of Caulobacter crescentus is regulated by the cell cycle as well as by a trans-actingregulatory hierarchy that functions to couple flagellum assemblyto gene expression. The assembly of early flagellar structures(MS ring, switch, and flagellum-specific secretory system) isrequired for the transcription of class III genes, which encodethe remainder of the basal body and the external hook structure.Similarly, the assembly of class III gene-encoded structures isrequired for the expression of the class IV flagellins, whichare incorporated into the flagellar filament. Here, we demonstratethat mutations in flbT, a flagellar gene of unknown function,can restore flagellin protein synthesis and the expression offljK::lacZ (25-kDa flagellin) protein fusions in class III flagellarmutants. These results suggest that FlbT functions to negativelyregulate flagellin expression in the absence of flagellum assembly.Deletion analysis shows that sequences within the 5' untranslatedregion of the fljK transcript are sufficient for FlbT regulation.To determine the mechanism of FlbT-mediated regulation, we assayedthe stability of fljK mRNA. The half-life (t_1/2) of fljK mRNAin wild-type cells was approximately 11 min and was reduced toless than 1.5 min in a flgE (hook) mutant. A flgE flbT doublemutant exhibited an mRNA t_1/2 of greater than 30 min. This suggeststhat the primary effect of FlbT regulation is an increased turnoverof flagellin mRNA. The increased t_1/2 of fljK mRNA in a flbT mutanthas consequences for the temporal expression of fljK. In contrastto the case for wild-type cells, fljK::lacZ protein fusions inthe mutant are expressed almost continuously throughout the C.crescentus cell cycle, suggesting that coupling of flagellin geneexpression to assembly has a critical influence on regulatingcell cycleexpression.

	INTRODUCTION

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Cells of the gram-negative, aquatic bacterium Caulobacter crescentus possess an intrinsic asymmetry, which upon division resultsin the formation of two distinct daughter cells: a motile swarmercell and a sessile stalked cell (reviewed in references 10,26, and 80). These cell types differ in their programs ofgene expression and DNA replication. For example, in the stalkedcell, replication of chromosomal DNA initiates immediately followingcell division, whereas this process is silenced for a definedperiod in the newly formed swarmer cell. Following this periodof repression, the swarmer cell differentiates into a stalkedcell. This differentiation event is accompanied by the degradationof flagellar components, stalk growth, the transcription of genesencoding DNA replication proteins, and the initiation of DNA replication(10, 26, 80).

Differentiation into a stalked cell type also initiates a cascade of events that culminate in the assembly of a single polarflagellum at the pole opposite the stalk. Flagellar biogenesisin C. crescentus requires the coordinated expression of approximately50 genes (17, 20, 39) and is regulated by a complex interplayof both cell cycle and flagellar assembly events. The initiationof DNA replication is required for expression of early class IIflagellar genes (13, 75), which encode the MS ring (37,58), the flagellar switch (58, 83), and a flagellum-specificsecretory apparatus (29, 64, 68, 75, 84), as well asthe trans-acting factors encoded by flbE (78) and flbD (7,8, 54, 59, 63, 79, 81) (Fig. 1). Class II promotersare transcribed relatively early in the cell cycle and containconserved cis-acting sequences located between 35 and 10 bp upstreamof the transcription start site (29, 58, 68, 75, 84).The transcription of these early flagellar operons is regulatedby the global response regulator CtrA, which has been shown tobind to these conserved sequence elements and to activate thetranscription of class II flagellar promoters at a specific timein the C. crescentus cell cycle (15, 50, 62).

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FIG. 1. The C. crescentus flagellar regulatory hierarchy (reviewed in references 10, 26, and 80). A schematic of the flagellar regulatory hierarchy is shown. The hypothetical structures are depicted in the order in which they are assembled. Below each intermediate structure is indicated the class of flagellar genes that encode it. Flagellar assembly is coupled to gene expression at two distinct levels of the regulatory hierarchy. A cell cycle cue activates the response regulator CtrA, which in turn activates the transcription of the class II subset of flagellar genes. These genes encode regulatory proteins such as FlbD and FlbE, as well as the MS ring, the flagellar switch, and components of the flagellum-specific class III secretory apparatus. The expression and activation of FlbD and FlbE are required for the transcription of class III genes, which encode components of the basal body and hook structure. In addition, in the absence of assembly of the MS ring-switch secretory complex, the transcription of class III genes is negatively regulated by the bfa gene product. The proper assembly of class III genes is, in turn, necessary for the expression of the class IV genes, which encode flagellins. In this report, we describe how FlbT negatively regulates the expression of flagellin in the absence of assembly of the basal body-hook complex. OM, outer membrane; IM, inner membrane.

The expression of class III flagellar genes, which encode the rods and rings of the basal body and hook, follows the assemblyof class II gene products (11, 12, 28, 30, 40, 46,51-53). Class III gene expression is regulated by two distinctcellular events: the progression to a specific stage in the celldivision cycle and the assembly of class II gene products intothe nascent flagellar structure. The transcription of class IIIflagellar promoters requires the general transcription factors $sigma$ ⁵⁴-containing RNA polymerase (3, 9) and integration host factor(27, 28, 46), as well as the flagellar transcription factorFlbD (64). FlbD is a member of the response regulator familyof bacterial two-component regulatory systems (64) and bindsto a conserved enhancer element called ftr which is located approximately100 bp from the transcription start site (7, 8, 52-54, 79,81). Cell cycle expression of class III promoters is accomplishedthrough the temporal phosphorylation of FlbD (8, 79). Theproduct of the flbE gene is also required for the temporal expressionof class III genes and has been shown to be required for FlbDactivity (78). Activation of class III gene expression requireslocalization of FlbE to the mid-cell site in the predivisionalcell (78). Therefore, FlbE is thought to couple an early celldivision event to the activation of class III geneexpression.

The assembly of class II gene products is also required for the expression of class III genes (Fig. 1). For example, a mutationin any one of the class II flagellar genes results in a lack oftranscription of class III genes (11, 45, 56, 59, 82).A mutation, in bfa (for bypass of flagellar assembly), that permitsexpression of class III genes in the absence of an assembled flagellarstructure has been isolated (45). Strains containing a mutationin bfa also exhibit an alteration in the cell cycle timing ofclass III gene transcription, indicating that bfa, and presumablyflagellar assembly, has an influence in regulating temporal expression(45). It is hypothesized that bfa encodes a repressor of classIII gene expression whose activity or availability is regulatedby the assembly of an early flagellar structure. This would beanalogous to the anti-sigma factor FlgM, which inhibits $sigma$ ²⁸ activity in response to a flagellar assembly defect in Salmonellatyphimurium (24, 25, 34, 60). The bfa gene has not yetbeen isolated, and therefore it is not known whether Bfa inhibitsFlbE and/or FlbD activity or whether it binds to class III promotersand represses transcriptiondirectly.

The incorporation of flagellin monomers into the filament follows the assembly of the hook structure (Fig. 1). C. crescentuspossesses six different flagellin genes that map in two clustersat distinct chromosomal locations. The $alpha$ cluster contains genesencoding 27-kDa (fljL), 25-kDa (fljK), and 29-kDa (fljJ) flagellins(21-23, 49). The genetically unlinked $beta$ cluster contains threegenes, fljMNO, each encoding a 25-kDa flagellin (18). The transcriptionalregulation of fljL and fljK has been examined in some detail (49).Like class III flagellar promoters, fljL and fljK require $sigma$ ⁵⁴-containing RNA polymerase (3, 9, 49, 51) and integrationhost factor (27). In addition, these promoters each containFlbD binding sites (7, 8, 49, 79). fljL transcriptionrequires the assembly of class II gene products (2, 45) andtherefore is regulated by bfa. Interestingly, although fljK transcriptionrequires the same trans-acting factors as fljL expression, itis not regulated by bfa (i.e., the promoter is transcribed inclass II flagellar mutants) (2, 79).

Experiments using bfa mutants have revealed another level of this trans-acting regulatory hierarchy (45). bfa mutant strains,which were able to transcribe the 27-kDa flagellin gene, fljL,in the absence of flagellar assembly, synthesized no detectableflagellin protein (45). It has also been shown that althoughflagellin promoters are transcribed in strains with mutationsin class III genes, flagellin protein and flagellin-lacZ proteinfusions are not expressed (2). Furthermore, in the case ofthe 25-kDa flagellin (fljK product), this effect requires the5' untranslated region of the mRNA (2). From these experiments,it has been inferred that the assembly of class III flagellargene products is required for the expression of flagellin, whichcomprises the final assembled structure of the flagellar filament(2). In contrast to the coupling of class III gene expressionto the assembly of class II flagellar structures, which is regulatedthrough the inhibition of transcription, the coupling of the assemblyof class III flagellar structures to flagellin synthesis is regulatedat the posttranscriptionallevel.

In this study, we investigated the mechanism of posttranscriptional regulation of fljK expression. We show that mRNA sequencesthat are 5' to the translation start codon are sufficient to exertregulation and that fljK mRNA has a dramatically shorter half-lifein the absence of flagellar assembly. Mutations in flbT, a well-characterized(16, 68-71) but previously unclassified flagellar gene, can reversethis effect, indicating that the flbT gene product may act asa negative regulator of fljK gene expression in the absence offlagellar assembly. Strains containing mutations in flbT havean altered cell cycle pattern of fljK expression, suggesting thatposttranscriptional repression and the progression of flagellarassembly have a critical role in influencing temporal expressionof C. crescentus flagellingenes.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, and growth conditions. The bacterial strains and plasmids used in these experiments are listed in Table 1. C. crescentus NA1000, a motile, synchronizablestrain, was used as the wild-type strain. AE8006 is a mutant strainwith a Tn5-VB32 (6) insertion in flgE (11). A flbT flgE doublemutant strain (JG551) was created by transducing flgE806::Tn5-VB32into SC276 (flbT650) by using phage $phi$ CR30 (19). C. crescentuscells were grown with shaking at 31°C in either PYE medium (61)or minimal M2-glucose medium (38). Escherichia coli strainswere grown in Luria-Bertani medium at 37°C (48). To generatea wild-type fljK::lacZ translational fusion, a 505-bp PstI-EcoRIfragment spanning the entire fljK promoter region to codon 23within the gene was fused to the eighth codon of lacZ in pJBZ282(45). The fljK::lacZ fusions in pJBZ282 were introduced intoC. crescentus by conjugation, using E. coli S17-1 containing thehelper plasmid pLVC9 (74). A fljK-lacZ transcription fusion(79) contained this same sequence cloned upstream of a promoterlesslacZ in pRK290 (14) (placZ/290) (28). To construct a templatefor site-directed mutagenesis, the 505-bp PstI-EcoRI fragmentwas subcloned first into Bluescript KS (Stratagene) and then intoM13-BM21 (Boehringer Mannheim Biochemicals) as a 524-bp BamHI-HindIIIfragment.

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TABLE 1. Bacterial strains and plasmids used

Mutagenesis of fljK mRNA. The 505-bp PstI-EcoRI fljK fragment in M13-BM21 (Boehringer Mannheim Biochemicals) was used as a template for site-directedmutagenesis. Single-stranded DNA was isolated from E. coli CJ236,and mutagenesis was performed as described by Kunkel and Roberts(42). Mutants were identified by DNA sequencing (69). To generatepfljK1::lacZ, a HindIII site was created at codon 14. Likewise,pfljK2::lacZ was constructed by creating a HindIII site aftercodon 1 of fljK. pfljK3::lacZ was generated by creating a BglIIsite immediately following the transcription start site and anotherBglII site before the ribosomal binding site in the upstream leader.The resulting mutant was cloned from M13-BM21 into BluescriptKS by using BamHI-HindIII. The upstream leader was then deletedby digesting with BglII and religating. All products of site-directedmutagenesis were subcloned in frame to pJBZ282. Expression ofwild-type and mutant constructs was assayed by $beta$ -galactosidaseactivity (48) with C. crescentus cultures grown to mid-logarithmicphase in PYE medium at 31°C. The reported $beta$ -galactosidase valuesrepresent mean values from assays performed in triplicate on threeseparately growncultures.

Immunoprecipitation of flagellin and $beta$ -galactosidase. C. crescentus cultures were grown in M2-glucose to an optical density at 660 nm of 1.0 to 1.4. An aliquot was removed andpulse-labeled with Tran³⁵S-label (ICN) for 5 min. Labeled protein was immunoprecipitatedwith either a polyclonal antiflagellin antibody (33) or a monoclonalanti- $beta$ -galactosidase antibody (Boehringer MannheimBiochemicals).

mRNA stability assay by primer extension. C. crescentus NA1000, AE8006, SC276, and JG551 cells were grown in M2-glucose medium to an optical density at 600 nm of 1.0to 1.2. To initiate the experiment, rifampin was added to thecultures to a final concentration of 200 µg/ml. Aliquots of cellswere removed at various times following the addition of rifampin,and RNA was isolated from each sample (29). Primer extensionwas performed as described by Ausubel et al. (5) with an oligonucleotideprimer complementary to fljK mRNA coding sequences 53 to 71 nucleotidesfrom the start of translation. The 71-nucleotide extension productswere resolved by electrophoresis in a denaturing 8% acrylamide-ureasequencing gel. The dried gel was exposed to X-ray film and subjectedto phosphorimageranalysis.

Cell cycle expression experiments. C. crescentus cultures were grown in M2-glucose to an optical density at 660 nm of 1.0 to 1.4. Swarmer cells were isolatedby centrifugation through a Ludox gradient (21). Swarmer cellpopulations (greater than 97% pure as assayed by light microscopy)were suspended in fresh M2-glucose medium and allowed to progressthrough the cell cycle. At various times throughout the cell cycle,samples were removed and proteins were pulse-labeled with Tran³⁵S-label (ICN) for 5 min. Labeled protein was immunoprecipitatedwith the monoclonal anti- $beta$ -galactosidase antibody (BoehringerMannheim Biochemicals) (33) and separated by sodium dodecylsulfate-polyacrylamide gel electrophoresis (SDS-PAGE), and thedried gel was subjected tofluorography.

	RESULTS

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Previous experiments have demonstrated that although the C. crescentus 25-kDa flagellin gene (fljK) is transcribed in strainscontaining mutations in class II flagellar genes, flagellin proteinis not synthesized (79). Furthermore, experiments comparingthe expression of flagellin-lacZ transcription fusions and proteinfusions have shown that class III flagellar mutant strains havea marked reduction in $beta$ -galactosidase activity generated fromlacZ protein fusions, whereas transcription is largely unaffected(2). The conclusion from both of these experiments is thatflagellin synthesis is subject to negative posttranscriptionalregulation in strains that exhibit defects in flagellarassembly.

To determine whether the rate of $beta$ -galactosidase synthesis generated by reporter fusions was regulated in the same manneras that of flagellin protein, cellular proteins were pulse-labeledwith Tran³⁵S-label and immunoprecipitation experiments were performed. Wild-typeand hook mutant (SC511) strains were assayed for expression ofeither a fljK::lacZ protein fusion reporter or a fljK-lacZ transcriptionalfusion reporter (Fig. 2). Proteins were immunoprecipitated witha polyclonal antiflagellin antibody or a monoclonal anti- $beta$ -galactosidaseantibody. Flagellin protein was expressed in wild-type cells (Fig.2, lane 1), but was poorly expressed in hook mutant cells (Fig.2, lane 2). Likewise, a fljK::lacZ protein fusion was expressedin wild-type cells (Fig. 2, lane 3) and exhibited a marked decreasein expression in a hook mutant strain (Fig. 2, lane 4). However,a fljK-lacZ transcriptional fusion was expressed in both wild-typecells and a hook mutant background (Fig. 2, lanes 5 and 6). Theseresults suggest that a fljK::lacZ protein fusion is regulatedby a posttranscriptional mechanism in the same manner as wild-typeflagellin protein.

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FIG. 2. Posttranscriptional regulation of the 25-kDa flagellin gene, fljK. Expression of flagellin protein or fljK-lacZ fusions in either wild-type or hook mutant cells was assayed by immunoprecipitation. Cells were grown in M2 medium to mid-log phase, and an aliquot of cells was removed and labeled with Tran³⁵S-label for 5 min. Labeled protein was immunoprecipitated with either antiflagellin (lanes 1 and 2) or anti- $beta$ -galactosidase (lanes 3 to 6) antibody and separated by SDS-PAGE as described in Materials and Methods. Lane 1, NA1000; lane 2, SC511; lane 3, NA1000 containing a fljK::lacZ protein fusion; lane 4, SC511 containing a fljK::lacZ protein fusion; lane 5, NA1000 containing a fljK-lacZ transcription fusion; lane 6, SC511 containing a fljK-lacZ transcription fusion. The apparent molecular masses of the immunoprecipitated proteins are indicated with arrows.

Mutations in flbT restore flagellin protein synthesis in strains bearing mutations in flagellar structural genes. Previous experiments have demonstrated that mutations in flbT, a gene that lies near the $alpha$ -flagellin gene clusters in C. crescentus,increase the level of flagellin expression (69, 72). Therefore,FlbT is an attractive candidate for a negative regulator of flagellinexpression. To test this idea, the levels of flagellin in strainscontaining a mutation in a flagellar structural gene alone orin combination with a flbT mutation were assayed by immunoblotting(Fig. 3). Compared to wild-type cells, a strain bearing a flbTmutation produced slightly increased levels of the 27-kDa flagellin,encoded by the fljL gene, and the 25-kDa flagellin, encoded byfljK as well as fljMNO of the $beta$ cluster. In addition, as previouslydemonstrated, the mutant flbT strain also produced a variant ofthe 25-kDa flagellin that migrates at an apparent molecular massof 22 kDa (70, 73). The effect of a flbT mutation on flagellinexpression in class II and class III flagellar mutants was alsoexamined. All of the class II and III mutant strains tested producedlittle or no flagellin protein (Fig. 3). If these strains alsocontained a mutation in flbT, 25-kDa flagellin expression wasrestored in all cases. Therefore, in the case of the 25-kDa flagellins,mutations in flbT bypass the requirement for flagellar assembly.In most cases, the mutation in flbT could not restore expressionof the 27-kDa flagellin. Expression was evident in only two strains:a flbT flaN mutant and a flbT flbX mutant. These two strains containmutations in class III flagellar genes, whereas the remainderof the strains tested contain mutations in class II genes. Incontrast to the 25-kDa flagellin gene, fljK, fljL is not transcribedin class II mutants (2, 45) as a consequence of Bfa activity(45) and therefore is not expressed in flbT-class II doublemutant strains.

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FIG. 3. A mutation in flbT restores flagellin expression in flagellar mutants. Proteins from whole-cell extracts from mutant strains were separated by SDS-PAGE and subjected to immunoblotting as described in Materials and Methods. Mutations in a single flagellar gene were introduced into the flbT mutant strain SC276 by generalized transduction. The mobilities of flagellins derived from these strains are compared to that of purified flagellin protein. W.T., wild type.

Interestingly, mutations in flbT were also able to restore flagellin expression in strains containing mutations in genes encodingtrans-acting factors, such as rpoN (encoding the $sigma$ ⁵⁴ subunit of RNA polymerase holoenzyme), flbD (encoding a $sigma$ ⁵⁴ transcriptional activator), and flbE (encoding a trans-actingfactor required for FlbD activity). Previous experiments haveshown that these genes are essential for the expression of fljKand fljL. The simplest interpretation of these results is thatthe flagellin produced in these double mutant strains derivesfrom fljMNO in the $beta$ cluster. Recent evidence indicates that thetranscription of fljMNO is not dependent on rpoN or flbD (18).However, the fact that this cluster does not produce flagellinin the absence of flagellar assembly probably indicates that proteinsynthesis is regulated in a fashion similar to that for fljL andfljK.

Effect of flbT mutations on fljK::lacZ expression. We next tested whether the flbT mutant strain had the same effect on fljK::lacZ reporter expression. To accomplish this, awild-type fljK::lacZ protein fusion (Fig. 4) was introduced intowild-type cells, a flgE mutant (AE8006), a flbT mutant (SC276),and a flgE flbT double mutant (JG551) (Fig. 5A). This fusion generated2,772 U of $beta$ -galactosidase activity in wild-type cells. In contrast,in the flgE mutant, the fljK::lacZ fusion was expressed at levels10% of that in wild-type cells, generating 246 U of $beta$ -galactosidaseactivity (Fig. 5A). This result is consistent with the observationthat fljK expression is subject to negative posttranscriptionalregulation. In a flbT mutant, expression of fljK::lacZ was almosttwice that in wild-type cells (5,955 U). This increase in expressionis similar to that observed when flagellin protein was assayedin cell extracts derived from wild-type and flbT mutants (Fig.3). To determine whether a mutation in flbT could restore fljK::lacZexpression in a class III mutant, we constructed a strain, JG551,that contained both the flgE::Tn5-VB32 mutation and the flbT650mutation and then assayed $beta$ -galactosidase activity. The mutationin flbT completely bypassed the requirement for an assembled hookstructure; the fljK::lacZ fusion in this strain possessed approximately40 times the $beta$ -galactosidase activity of strain AE8006 which containsonly a mutation in flgE (9,253 versus 246 U) (Fig. 5A). This resultindicates that flbT has a critical role in negatively regulatingfljK expression in the absence of flagellar assembly.

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FIG. 4. Schematic diagram of deletion derivatives of fljK::lacZ translation fusions. Site-directed mutagenesis was used to construct different deletions of fljK. The sequence encoding amino acids 1 to 23 was fused in frame to lacZ to create fljK::lacZ. fljK1::lacZ corresponds to a deletion of amino acids 15 to 23 fused in frame to lacZ. The sequence encoding amino acids 2 to 23 was deleted, resulting in an in-frame fusion of the ATG from fljK to lacZ to create fljK2::lacZ. fljK3::lacZ is a deletion of the upstream leader, leaving only the ribosomal binding site intact, fused in frame to lacZ. IHF, integration host factor.

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FIG. 5. Effect of deletions on the expression of fljK::lacZ translation fusions in wild-type and mutant strains. Wild-type and deleted fljK::lacZ translation fusions were introduced into the mutant strains indicated on the x axis. Values on the y axis represent $beta$ -galactosidase activity, in units (48), assayed in triplicate from three different mid-logarithmic-phase cultures. NA1000 is a synchronizable derivative of wild-type C. crescentus CB15. AE8006 contains a Tn5-VB32 insertion in flgE (hook). JG551 contains a Tn5-VB32 insertion in flgE and a flbT650 mutation from strain SC276. SC276 contains the flbT650 allele. (A) Mean $beta$ -galactosidase activity generated from pfljK::lacZ, which contains the entire 5' untranslated region of fljK and the first 23 codons fused in frame to lacZ. The mean $beta$ -galactosidase activities were 2,772 U for NA1000, 246 U for AE8006, 9,253 U for JG551, and 5,955 U for SC276. (B) $beta$ -Galactosidase activity generated from pfljK1::lacZ, which contains the entire 5' untranslated region of fljK and the first 14 codons fused in frame to lacZ. The mean $beta$ -galactosidase activities were 1,328 U for NA1000, 503 U for AE8006, 14,926 U for JG551, and 3,407 U for SC276. (C) $beta$ -Galactosidase activity generated from pfljK2::lacZ, which contains the entire 5' untranslated region of fljK and the first codon fused in frame to lacZ. The mean $beta$ -galactosidase activities were 2,426 U for NA1000, 373 U for AE8006, 12,279 U for JG551, and 9,135 U for SC276. (D) $beta$ -Galactosidase activity (note difference in scale) generated from pfljK3::lacZ, in which the entire 5' untranslated region of fljK except the ribosome binding site was deleted, fused in frame to lacZ. The mean $beta$ -galactosidase activities were 685 U for NA1000, 132 U for AE8006, 479 U for JG551, and 1,791 U for SC276. See Fig. 4 for a schematic representation of these fusions.

Since the nature of the flbT mutation in strain SC276 is unknown, we tested whether strains containing deletions in flbT exhibiteda similar effect. The flgE::Tn5-VB32 mutation was introduced,by transduction, into SC603 and SC604, which have flmGH flbT flaFand flmGH flbT deleted, respectively (44, 72). flmG and flmHencode proteins that are homologous to O-linked acetylglucosaminetransferases and acetyltransferases, respectively, and are regardedto be required for posttranslational modification of flagellins(44). The function of flaF is unknown. Previous experimentshave demonstrated that mutations in flmG, flmH, and flaF resultin a decrease in the level of flagellin produced (72). In strainsSC603 and SC604, the level of $beta$ -galactosidase generated by fljK::lacZwas increased approximately twofold over that in wild-type cells(data not shown). The deletion in flbT in both these strains isapparently able to bypass the requirement for a hook structure.When the flgE::Tn5-VB32 allele was introduced into these strains,the level of $beta$ -galactosidase generated by fljK::lacZ was increasedapproximately 23 times over that assayed in AE8006 (5,800 versus246 U) (data not shown). Since the other genes deleted in bothof these strains are probably involved in the posttranslationalmodification of flagellin (44), the simplest conclusion thatcan be drawn from these results is that the deletion in flbT isresponsible for the restoration of fljK::lacZ expression in theabsence of a hookstructure.

The restoration of fljK expression observed in flbT and flgE flbT mutants could be attributable to an increase in transcriptionand/or translation. To distinguish between these two possibilities,we tested the expression of fljK-lacZ transcription fusions inthe flbT mutant strain SC276. In contrast to the high levels of $beta$ -galactosidase generated by the fljK::lacZ protein fusion, expressionof the fljK-lacZ transcription fusion was dramatically decreasedcompared to that in wild-type cells (135 versus 3,500 U) (datanot shown). This result indicates that FlbT probably functionsas a posttranscriptional repressor. In addition, the decreasein transcription and the increase in translation in SC276 suggestthat transcription of fljK is influenced by the level oftranslation.

In an attempt to define the region of fljK mRNA that is responsible for the posttranscriptional repression in a class IIImutant background, a set of deletions were created and in-framefusions to lacZ were constructed (Fig. 4). Mutants in which aminoacids 15 to 23 (pfljK1::lacZ) or 2 to 23 (pfljK2::lacZ), encodedin the fljK coding region, were deleted (Fig. 4) exhibited a patternof regulation similar to that for the fljK::lacZ fusion, whichencoded all 23 of these amino acids; the fusions were expressedin wild-type cells and had a decreased expression in a hook mutantstrain (Fig. 5B and C). The flbT mutation increased the expressionof both of these fusions and could restore expression in a hookmutant to levels greater than that measured in wild-type cells(Fig. 5B and C). A final deletion mutant was created, in whichthe entire upstream leader sequence except the ribosomal bindingsite had been deleted (pfljK3::lacZ) (Fig. 4). In contrast tofusions with deletions within the coding region, this fusion wasexpressed poorly in wild-type cells (Fig. 5D [note change in scale]).Expression was reduced an additional fivefold in the hook mutantstrain, indicating that this fusion was still subject to posttranscriptionalrepression. Furthermore, introduction of a flbT mutation intothis strain partially restored expression; however, the increasein expression compared to that in the hook mutant was less thanthat observed for fusions containing a wild-type leader sequence.In this case, when the hook mutant strain also contained a flbTmutation (JG551), the expression of fljK3::lacZ was only 3.6 timeshigher than that in the strain containing a single mutation inthe hook. In strains containing a fljK::lacZ fusion possessinga wild-type leader sequence, a flbT mutation increased expressionlevels by 37-fold. These results indicate that the sequences withinthe upstream leader are required for the regulation of expressionof fljK in class III flagellar mutants and, in addition, thatthe likely site of FlbT-mediated regulation lies within this leaderregion.

flbT regulates fljK mRNA stability. The decreased expression of flagellins and fljK::lacZ protein fusions in class III flagellar mutants may be a consequenceof negative regulation of translation. If this is the case, ablock in translation should result in a shorter half-life of flagellinmRNA, as has been observed for other bacterial mRNAs whose translationis negatively regulated (32, 35, 55, 65). To test thisidea, we assayed the decay of fljK mRNA over time in wild-typecells, and in flgE, flbT, and flgE flbT mutant strains. The cultureswere treated with rifampin to inhibit transcription, and totalRNA was isolated at 3-min intervals and subjected to primer extensionanalysis. In wild-type cells, fljK mRNA had an estimated half-lifeof 11 min (Fig. 6). Previous experiments have demonstrated thatthe steady-state levels of flgK mRNA were reduced in a class IIIflagellar mutant (2). Consistent with this observation, ina strain containing a mutation in flgE, the fljK mRNA had a greatlyreduced half-life of less than 1.5 min. This result suggests thatdecreased flagellin synthesis in class III mutant cells may beattributable to a decrease in the stability of fljK mRNA. fljKmRNA stability was increased to greater-than-wild-type levelsin a flbT mutant background (half-life of greater than 30 min).The same experiment was performed with a flbT flgE double mutant.Like the flbT mutant background alone, a mutation in flbT wassufficient to increase fljK message stability to greater-than-wild-typelevels (half-life of greater than 30 min). We hypothesize thatthe decrease in mRNA half-life observed in flgE mutant strainsis a consequence of inhibition of translation, perhaps mediatedthrough the action of the flbT gene product.

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FIG. 6. Effect of flagellar mutations on fljK::lacZ mRNA stability. C. crescentus NA1000 cells were grown to mid-logarithmic phase in M2 medium. At 0 min, 200 µg of rifampin per ml was added to inhibit transcription. At 3, 6, 9, 12, and 15 min, an aliquot was removed, RNA was isolated from each sample, and primer extension was performed with a ³²P-labeled oligonucleotide that hybridized to the coding sequence of lacZ. The primer extension products were subjected to electrophoresis in a denaturing polyacrylamide gel. (A) C. crescentus NA1000 cells. The mRNA half-life is approximately 11 min. (B) Strain AE8006 (flgE::Tn5-VB32). The mRNA half-life is less than 1.5 min. (C) Strain SC276 (flbT650). The mRNA half-life is greater than 30 min. (D) Strain JG551 (flgE::Tn5-VB32 flbT650). The mRNA half-life is greater than 30 min.

A mutation in flbT alters the temporal pattern of fljK expression. One possible function of FlbT in wild-type cells may be to influence the temporal expression of flagellin genes. For example,FlbT activity may exist to shut off flagellin synthesis followingthe completion of flagellar assembly. To test this hypothesis,the temporal expression of fljK::lacZ was assayed in wild-typeand flbT mutant backgrounds. Cell cycle expression of fljK wasassayed by synchronizing a culture containing an integrated fljK::lacZprotein fusion. The isolated swarmer cells were suspended in freshmedium and allowed to progress through the cell cycle. At varioustimes thereafter, proteins were pulse-labeled with Tran³⁵S-label, and radioactive $beta$ -galactosidase was immunoprecipitatedfrom the cell extracts and subjected to PAGE. In wild-type cells,the fljK::lacZ fusion was expressed under temporal control. Aspreviously shown (49, 79), expression was observed in swarmercells (0 cell division units) and was turned off in stalked cells(0.45 cell division unit) (Fig. 7). Later in the cell cycle, whenthe cells reached the predivisional stage, expression of the fljK::lacZfusion returned and continued until cell division occurred. Ina flbT mutant strain the fljK::lacZ fusion had an altered patternof expression. A full-length, labeled FljK::LacZ fusion was synthesizedat the same period in the cell cycle as observed in wild-typecells. In contrast to the case for wild-type cells, in newly formedstalked cells and early predivisional cells of the flbT mutantstrain, a smaller polypeptide of approximately 20 kDa was synthesized.Since a monoclonal antibody was employed in these experiments,the most likely source of this polypeptide is $beta$ -galactosidase.The best interpretation of this observation is that the fljK::lacZfusion is expressed throughout the C. crescentus cell cycle butthat protein which is expressed in stalked and early predivisionalcells is subject to proteolysis. In this case, proteolysis isdependent on the fusion of fljK to lacZ, since fusions that expressfull-length lacZ at this time of the cell cycle, such as gyrB-or recF-lacZ transcription fusions, do not exhibit proteolysisof $beta$ -galactosidase (67). Therefore, we hypothesize that sincefljK is not transcribed in stalked cells, the extended fljK mRNAstability observed in the flbT mutant is responsible for fljK::lacZexpression in stalked cells.

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FIG. 7. Effect of a flbT mutation on the temporal expression of a fljK::lacZ translation fusion. The temporal expression of $beta$ -galactosidase was assayed with either C. crescentus NA1000 or SC276 cells containing a fljK::lacZ translation reporter fusion. Isolated swarmer cells were suspended in fresh M2 medium and were permitted to progress through the cell cycle. At various times during the cell cycle (0, 30, 60, 90, 120, 150, and 180 min), an aliquot was removed and proteins were labeled with Tran³⁵S-label for 10 min. Labeled protein was immunoprecipitated with a monoclonal anti- $beta$ -galactosidase antibody and subjected to SDS-PAGE as described in Materials and Methods. The gel was dried and exposed to X-ray film. (Top) fljK::lacZ expression in wild-type strain NA1000. The drawing above the fluorogram shows the cell types present at each time point, as determined by light microscopy. Labeled $beta$ -galactosidase is indicated by an arrow. (Bottom) fljK::lacZ expression in a flbT mutant strain, SC276. A low-molecular-mass (approximately 20-kDa) proteolytically generated fragment of $beta$ -galactosidase is also indicated by an arrow.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Flagellar biogenesis in C. crescentus is characterized by cell cycle assembly of a polar flagellar structure. The assemblyof the polar flagellum is a complex process that requires over50 gene products (17) and is regulated both by progression throughthe cell cycle and by the assembly of the structure itself. Inthis report, we have identified flbT as a key player in couplingflagellar assembly to the expression of flagellin. The gene, encodingFlbT, maps to a region that contains a cluster of late-actingflagellar genes (70), including those encoding proteins involvedin the posttranslational modification of flagellin (44) as wellas three flagellin genes, fljL, fljK, and fljJ. Mutations in flbThave been shown to have pleiotropic effects, including impairedmotility, defects in the temporally regulated loss of the flagellumfrom stalked cells, and a marked increase in flagellin proteinsynthesis (70, 73). The last property suggests that flbT mightfunction in the negative regulation of flagellin expression. Thedata presented here indicate that FlbT functions to inhibit flagellinexpression in the absence of an intermediate flagellar structureinto which flagellin monomers can be incorporated. In supportof this view, mutations in flbT restore the expression of thefljK flagellin gene in the absence of a flagellar hook structure(i.e., in a flgE mutant strain). Although the precise nature ofthe flbT mutation in strain SC276 is not known, we have found,using anti-FlbT antibodies, that this strain produces no detectableFlbT protein (4). This suggests that the restoration of flagellinexpression observed in flgE flbT double mutants is a consequenceof a loss of FlbT and is probably not attributable to a gain-of-functionallele. This is supported by the observation that deletions inflbT can also restore fljK::lacZ expression in a flgEmutant.

Immunoblot analysis showed that the flbT mutation could restore flagellin synthesis in all class II and class III flagellarmutant strains tested, suggesting that flbT is a general regulatorthat couples assembly to flagellin gene expression. Surprisingly,a mutation in flbT could also restore flagellin expression inrpoN, flbD, and flbE mutant strains, which are deficient in essentialtrans-acting factors. Recent analysis has revealed that the $beta$ cluster of flagellins, which contains three copies of 25-kDa flagellingenes, is not regulated by rpoN, flbD, or flbE (18), suggestingthat the flagellin present in these mutants derives from thiscluster. Interestingly, although the flagellins in the $beta$ clusterdiffer in their transcriptional regulation, they apparently havea common mechanism of regulation in response to flagellumassembly.

The negative regulation of flagellin expression in class III mutant strains is most likely mediated through a posttranscriptionalmechanism. This conclusion is supported by the observation thatalthough the fljK gene is transcribed in mutants that do not assemblea hook structure, there is little, if any, flagellin protein present.Deletion analysis of the fljK transcript showed that the expressionof fljK was reduced in a hook mutant if the entire coding regionwas absent. Deletion of the 5' untranslated sequences resultedin a marked decrease of fljK expression. Even though expressionwas decreased in a hook mutant, this fusion exhibited a relativelymodest increase in activity in a FlbT-hook double mutant. Basedon these data, we hypothesize that FlbT exerts its primary effectthrough acting on the 5' untranslated leader of the fljK transcript.This is consistent with previous experiments demonstrating thatsequences within the 5' untranslated region of the fljK transcriptwere important for regulation by flagellar assembly (2). Theabsence of hook assembly presumably results in an increased turnoverof fljK mRNA. Furthermore, mutations in flbT apparently decreasethis high rate of mRNA turnover. From the experiments presentedhere, it is impossible to distinguish whether the apparent increasein mRNA turnover in class III mutants is a direct consequenceof message instability in these strains or is brought about byan inhibition of translation, which as a secondary result leadsto unstable mRNA. For example, it has been suggested that in somecases in bacteria, message stability is directly proportionalto the formation of a translational complex (32, 35, 55).In the absence of ribosome binding, RNase E sites are exposed,causing rapid degradation of message (66). We envision two possiblemechanisms whereby the flbT gene product promotes the turnoverof flagellin mRNA in class III flagellar mutants. Previous experiments(47), as well as those reported here, have demonstrated thatfljK mRNA has an unusually long half-life for a bacterial message.One plausible possibility is that a trans-acting factor(s) stabilizesfljK mRNA, and FlbT functions to antagonize its activity. Alternatively,FlbT may act directly to either destabilize fljK mRNA or preventtranslation. Either model is consistent with the observation thatmRNA sequences upstream of the translation initiation codon arerequired for FlbT to exert its maximaleffect.

This mechanism of posttranscriptional repression of flagellin gene expression contrasts with an analogous regulation of flagellingene expression in S. typhimurium. In S. typhimurium, the flagellinand chemotaxis genes are not expressed in mutant strains thathave defects in flagellar assembly (41, 43). These genes aretranscribed by $sigma$ ²⁸-containing RNA polymerase. Negative regulation is accomplishedthrough an anti-sigma factor encoded by flgM (24, 25, 59).In the absence of flagellar assembly, the intracellular levelsof the flgM gene product rise and the protein binds to the $sigma$ ²⁸ subunit of RNA polymerase, inhibiting its activity. Once a functionalhook structure is assembled, FlgM is exported from the cell viathe nascent flagellar structure, thereby relieving repression(34). In C. crescentus, as well, the transcription of classIII genes (e.g., those encoding the basal body rods, outer rings,and hook) is repressed in the absence of the assembly of a flagellarstructure encoded by class II gene products (Fig. 1). A mutationin a single uncharacterized gene, called bfa, can restore transcriptionof class III genes in the absence of flagellarassembly.

The regulation of flagellin gene expression by flbT represents another control point in flagellar biogenesis in C. crescentus,which is absent in enteric bacteria. What is the logic in possessingtwo different mechanisms to regulate flagellar biogenesis in responseto assembly? The transcription of both class III and class IVflagellar genes is positively regulated by the FlbD transcriptionfactor (7, 8, 55, 79, 81). FlbD is a member of thetwo-component response regulators (64) and is phosphorylatedin response to a cell cycle cue (79), possibly an early stagein cell division (78). Once cells have progressed past thiscritical cell cycle step, they are competent to transcribe bothclass III and class IV flagellar genes. We speculate that it isat this stage when FlbT inhibits the expression of the class IVflagellin genes until a hook structure is assembled. With analogyto regulation in enteric bacteria, FlbT repression would thenbe inactivated, and any newly transcribed flagellin mRNA wouldbe expressed. This model would ensure that flagellin is not synthesizeduntil the correct stage in flagellar assembly iscompleted.

The flbT gene product may have an additional regulatory role later in the cell cycle, following cell division. As noted above,flagellin mRNA possesses an unusually long half-life. We havepreviously shown that fljK is transcribed in the swarmer compartmentof the predivisional cell (31, 78, 79). The transcriptionof fljK ceases abruptly upon the completion of cell division;however, the mRNA remains within the progeny swarmer cell andis continually translated (46). Therefore, swarmer compartment-specifictranscription of fljK results in generation of a supply of fljKmRNA for the nascent swarmer progeny cell. This mRNA is translatedinto flagellin protein, which is assembled in the flagellar filament.Thus, the requirement for continued filament growth in the progenyswarmer cells is fulfilled both by the swarmer compartment-specifictranscription of fljK and by the unusual stability of flagellinmRNA. We hypothesize that FlbT plays a critical role in shuttingoff fljK translation in swarmer cells once the demand for newflagellin monomers is satisfied. This idea is supported by theobservation that fljK is synthesized at relatively high levelsin swarmer cells possessing mutant flbT and continues to be translatedafter the swarmer cells have differentiated into stalked cells.Therefore, FlbT, and presumably the assembly of the flagellum,contributes to the temporal expression of fljK. This result issimilar to what occurs in bfa mutant cells, where the cessationof transcription of class III promoters during the cell cycleis significantly delayed (45). This suggests that the functionof these two gene products in wild-type cells is to repress thesynthesis of flagellar genes following the completion of a specificstage of flagellar assembly. Negative regulatory pathways thatcouple flagellar assembly to gene expression in other organisms,such as those present in enteric bacteria, may serve a similarpurpose, perhaps functioning to regulate the number of flagellasynthesized by eachcell.

As noted above, one consequence of a mutation in flbT is the expression of fljK at an inappropriate time in the cell cycle.In this mutant strain, the FljK::LacZ fusion protein is degradedwhen swarmer cells differentiate into stalked cells. This is evidencedby the appearance of a small (approximately 20-kDa) polypeptidethat reacts with the monoclonal anti- $beta$ -galactosidase antibodyemployed in this experiment. Proteolysis of $beta$ -galactosidase isapparently dependent on the presence of FljK amino acid sequenceat the amino terminus. We have shown previously that $beta$ -galactosidaseis not subject to proteolysis at this stage of the cell cycle(66). Therefore, C. crescentus possesses a developmentally regulatedprotease that can degrade intracellular flagellin specificallyin stalked cells. One hallmark of the C. crescentus developmentalprogram is the timed degradation of proteins, often in a cell-type-specificfashion. For example, the transcription factor CtrA (15), theFliF protein (MS ring) (37), and the methyl-accepting chemotaxisreceptor (1) are all degraded specifically in stalked cells.One documented protease which is involved in this process is thehighly conserved ClpXP protease. The ClpXP protease degrades CtrA,an essential response regulator that controls early flagellargene transcription as well as the initiation of DNA replication(36). The ClpXP protease recognizes disordered C-terminal sequences,which possess some degree of conservation, as its substrates.Therefore, ClpXP is probably not involved in the degradation ofFljK::LacZ, since the amino terminus of FljK appears to be thedeterminant for proteolysis. This indicates that C. crescentusprobably possesses at least one additional developmentally regulatedprotease whose activity is restricted to the stalked cell type.In summary, C. crescentus utilizes a diverse array of regulatorymechanisms, such as cell cycle- and cell-type-regulated transcriptionalactivation, flagellar assembly-regulated transcriptional and posttranscriptionalrepression, and cell-type-specific proteolysis, in order to regulateflagellar biogenesis. The simultaneous operation of these pathwaysensures that flagellum synthesis is tightly coupled to the formationof a differentiated daughtercell.

	ACKNOWLEDGMENTS

We are grateful to Charles Boyd, G. Craig Draper, Jenny England, and Rachel Muir for critical reading of themanuscript.

E.K.M. was supported by Public Health Service predoctoral fellowship GM07104. This work was supported by Public Health Servicegrants GM48417 to J.W.G. and GM50547 to B.E. from the NationalInstitutes ofHealth.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Chemistry and Biochemistry and Molecular Biology Institute, Universityof California $---$ Los Angeles, Los Angeles, CA 90095-1569. Phone:(310) 206-9449. Fax: (310) 206-5213. E-mail: gober{at}chem.ucla.edu.

Present address: University of Alabama at Birmingham, Department of Medicine, Division of Clinical Immunology and Rheumatology,Birmingham, AL 35294-0006.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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54. Mullin, D. A., S. M. Van Way, C. A. Blankenship, and A. H. Mullin. 1994. FlbD has a DNA-binding activity near its carboxy terminus that recognizes ftr sequences involved in positive and negative regulation of flagellar gene transcription in Caulobacter crescentus. J. Bacteriol. 176:5971-5981[Abstract/Free Full Text].

55. Nagai, H., Y. Harumi, and Y. Takashi. 1991. Interplay of two cis-acting mRNA regions in translational control of $sigma$ ³² synthesis during the heat shock response of Escherichia coli. Proc. Natl. Acad. Sci. USA 88:10515-10519[Abstract/Free Full Text].

56. Newton, A., N. Ohta, G. Ramakrishnan, D. Mullin, and G. Raymond. 1989. Genetic switching in the flagellar gene hierarchy of Caulobacter requires negative as well as positive regulation of transcription. Proc. Natl. Acad. Sci. USA 86:6651-6655[Abstract/Free Full Text].

57. Ohta, N., E. Swanson, B. Ely, and A. Newton. 1984. Physical mapping and complementation analysis of transposon Tn5 mutations in Caulobacter crescentus: organization of transcriptional units in the hook gene cluster. J. Bacteriol. 158:897-904[Abstract/Free Full Text].

58. Ohta, N., L.-S. Chen, E. Swenson, and A. Newton. 1985. Transcriptional regulation of a periodically controlled flagellar gene operon in Caulobacter crescentus. J. M

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