Control of Photosystem Formation in Rhodobacter sphaeroides

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J Bacteriol, June 1998, p. 2801-2809, Vol. 180, No. 11
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

MINIREVIEW
Control of Photosystem Formation in Rhodobacter sphaeroides

Jill Zeilstra-Ryalls, Mark Gomelsky, Jesus M. Eraso, Alexei Yeliseev, James O'Gara, and Samuel Kaplan^*

Department of Microbiology and Molecular Genetics, University of Texas Health Sciences Center-Houston, Houston, Texas

	INTRODUCTION

Top Introduction References

Rhodobacter sphaeroides has the capacity to grow by aerobic and anaerobic respiration and photosynthetically in the lightunder anaerobic conditions, as well as fermentatively. It canfix atmospheric nitrogen and carbon dioxide. It resembles othergram-negative members of the class Proteobacteria when growingaerobically, but a reduction in oxygen tension induces an intracellulardifferentiation of the inner membrane, leading to the formationof the intracytoplasmic membrane system (ICM). The ICM housesthe integral membrane pigment-protein complexes constituting thephotosystem (PS), comprised of the reaction center (RC) and twolight-harvesting (LH) complexes. For an early review of ICM biosynthesis,see reference 44. The LH complexes are designated B800-850 (LHII)and B875 (LHI), based on their respective absorption maxima. Theratio of LHI to RC is fixed at approximately 15:1, whereas theratio of LHII to the LHI-RC unit is variable, changing in a mannerinverse to the incident light intensity. These three pigment-proteincomplexes are the spectral complexes (SC) of the R. sphaeroidesPS. Detailed structural information about these complexes in severalspecies of Rhodobacter is emerging (72).

The LH complexes capture light energy and direct that energy to the RC, where conversion of the excitation energy takes placeand is intrinsically coupled with a cyclic flow of electrons,ultimately to the periplasmically localized cytochrome c₂, whichserves to rereduce the RC to allow a new cycle of electron flow(for further details, see references 42, 44, and 72).

Bacteriochlorophyll (Bchl) absorbs most of the light energy within the SCs and is critical to the assembly and final structureof the SCs (44, 84, 87). The carotenoids (Crt) have a minorrole in absorbing light energy (15), but they function to protectthe complexes against photo-oxidative damage, dissipate excessradiant energy, and help to maintain the structure and relativeabundance of each SC (35, 50, 53).

A reduction in oxygen tension is both necessary and sufficient to induce synthesis of the ICM (reviewed in references 42and 44), which is gratuitously produced under anaerobic darkgrowth conditions, in the presence of an alternate electron acceptorsuch as dimethyl sulfoxide (DMSO). Oxygen tension is the majorenvironmental stimulus controlling PS induction, with variationsin light intensity determining the cellular level of the ICM andthe abundance of the different SCs. PS formation is tightly regulated,with checkpoints at all levels of information flow, from transcriptionalthrough posttranslational. In the following sections, we willdescribe what we currently know about the regulatory processescontrolling the formation and abundance of SCs in R. sphaeroides.We will present a working model for the regulation of PS formationin R. sphaeroides 2.4.1 which is based on the critical role ofcellular redox carriers. For clarity, we will, throughout thisreview, define aerobic growth as that which occurs under highlyoxygenic conditions, under which there are no detectable SCs presentin wild-type membranes.

	TRANSCRIPTIONAL REGULATION OF PS GENE EXPRESSION

Transcriptional regulation of PS genes, from an initial low background level, involves the coordinate action of several signaltransduction pathways which result in the induction of PS geneexpression following oxygen removal. Some of these pathways arespecific to PS genes and others are more global, while still othersare commonly recognized to be involved in cellular adaptationto anaerobiosis. Different PS genes are not all controlled bythe same regulatory pathways, although these may overlap. We firstdescribe those factors which appear to play a major role in sensing,signal generation, and transduction, as well as DNA binding. Thereafter,we describe other factors which have less pronounced effects and/orless obvious roles in PS gene transcription; these are believedto participate in fine tuning of transcriptional control. Finally,we described posttranscriptional processes essential to SC formationand abundance.

Sensors, signal generators, and transducers. (i) The Cco/Rdx redox signal-generating system. The identification of CcoNOQP cytochrome c oxidase and RdxBH (redox) as components (Fig. 1) of a signal-generating pathwaystemmed from the observation that inactivation of the ccoNOQPoperon resulted in PS gene expression (93, 94) under aerobicconditions. The ccoNOQP operon encodes the cbb₃-type cytochromec oxidase of R. sphaeroides 2.4.1. Of the three respiratory oxidasespresent in R. sphaeroides, the cbb₃ type is believed to have thehighest affinity for oxygen and is the primary oxidase presentunder microaerobic conditions (26, 27, 37). Immediatelydownstream of the ccoNOQP operon is the rdxBHIS operon (70,94). These operons are located at 443 kbp on chromosomeI (94). (The locations of genes that map outside the PS genecluster and are pertinent to this discussion are in boldface throughoutthe text.) The rdxB gene is a homolog of the rdxA gene, whichmaps to chromosome II (69). Both RdxB and RdxA are predictedto coordinate two [4Fe-4S] clusters (69), and these, togetherwith other clusters of cysteine residues, may be involved in redoxprocesses. They are both likely to be membrane bound, as has beenshown for RdxA (69).

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FIG. 1. Most of the PS genes are arranged in a cluster on chromosome I of R. sphaeroides 2.4.1 (83). This region of approximately 60 kb begins with the pufKBALMX operon and extends, in a clockwise direction, to the pucBAC operon, which is 18 kb downstream of puhA. The pufB and -A genes encode structural polypeptides of the LHI SC, the pufL and -M genes encode two of the three structural proteins of the RC, and the two structural polypeptides of the LHII SC are encoded by pucB and -A, respectively (reviewed in reference 44). The Q gene, located upstream of the puf operon, together with the pufK and pucC genes, are not part of the PS, nor is orf1696. The pufX gene product is required for PS competence (4); it facilitates light-driven cyclic electron transfer (23). Between pufKBALMX and puhA, the latter of which codes for the largest structural polypeptide of the RC, are genes encoding enzymes catalyzing the biosynthesis of Crt and Bchl (1-3, 8, 9, 17, 52) and some genes that have a regulatory role in PS gene expression. Between puhA and the pucBAC operon is the cycA gene (19, 97), encoding the obligatory cytochrome c₂ protein. In the related bacterium R. capsulatus, a similar arrangement of a portion of these genes extending from puf to puh (25), called the photosynthesis gene cluster, is present, and the DNA sequence of the entire R. capsulatus photosynthesis gene cluster has been determined (14). The PS gene cluster is defined as the region from 0 to 3,000 kbp on chromosome I of R. sphaeroides 2.4.1. In the text are presented the locations, in boldface, of those genes that map outside this cluster and are pertinent to the discussion presented here. For a detailed description of the above model of PS gene regulation, see the text. ALA, 5-Aminolevulinic acid.

Mutations in either ccoNOQP or the rdxB gene generate mutants which, under aerobic growth conditions, produce SCs, as wellas high levels of expression of pucBAC and pufKBALMX. Uncouplingof PS gene expression from the presence of oxygen in Rdx and Ccomutant strains involves the activation of the two-component PrrBAregulatory system (71). Thus, a pathway involving cbb₃ throughits interaction with oxygen serves as an oxygen "sensor" to generatean "inhibitory signal" through RdxB to, presumably, PrrB (seebelow), which results in a lack of PrrA activation. This inhibitorysignal may be through the membrane portion of PrrB. However, nophysical interaction between cbb₃ and PrrB has been demonstrated.This is analogous to the Arc system of Escherichia coli (40).The fact that the levels of SCs and PS gene expression in cbb₃and RdxB mutant strains are also substantially increased relativeto those of the wild type, even under anaerobic conditions, stronglyaffirms the likely functioning of these redox carriers under suchconditions. Under these same conditions, the activation of PSgene expression in these mutant strains is dependent upon thePrr system. FnrL (see below) is indirectly involved in modulatingthe activity of PrrA by regulating the level of ccoN gene expressionin response to oxygen levels (~10-fold increase following a high-to-lowO₂ transition; 66) and, presumably, rdxB as well.

(ii) The redox-responsive two-component Prr system. Prr (photosynthetic response regulator) is a signal transduction system (Fig. 1) involved in the activation of PS gene expression(20-22). The prrA gene product functions as a response regulator,and the prrB gene product functions as a sensor histidine kinase/phosphatase.A third gene, prrC, located upstream of prrA, encodes a membrane-associatedprotein. This genetic region is located outside of the regionof PS genes, 1149 kbp, on chromosome I of R. sphaeroides2.4.1. The prrCA genes form a transcriptional unit, although prrAhas its own promoter and prrB is divergently transcribed fromprrCA. Prr is similar to the R. capsulatus regBA-and-senC system,which is also involved in regulation of PS gene expression (64,79), as well as the Rhizobium meliloti actRS system, which isinvolved in acid tolerance (86). PrrBA regulates transcriptionof puhA, cycA, and the puc and puf operons, as well as some ofthe genes involved in Bchl and Crt synthesis and/or accumulation.The expression of genes involved in CO₂ and N₂ fixation is alsoaffected by the Prr system (41). Inactivation of prrA causesa photosynthesis-negative phenotype, as the result of a nearlytotal shutdown of PS gene expression. Mutants defective in prrBare photosynthesis negative when grown at low-to-medium lightintensities but grow photosynthetically at high light intensities,albeit with severely reduced levels of SCs. PrrC inactivationalso leads to a small reduction in SC formation, but cells remainphotosynthetically competent.

PrrA is thought to be cytoplasmically located. The carboxy-terminal end of PrrA lacks similarities with other DNA-bindingproteins. Nonetheless, PrrA acts either by binding DNA directly(45) or by interacting with another protein(s) that binds DNA.When prrA is present in multicopy in aerobically growing wild-typeor PrrB cells, such cells aberrantly produce spectral complexes and haveincreased puc expression despite the inhibitory signal emanatingfrom cbb₃ (22). This further suggests that other phosphodonorsare active in activating PrrA (20, 30, 71) and that PrrBmay possess an intrinsic phosphatase activity (20). Thus, thecellular levels of PrrA must be carefully regulated (22). Additionally,there is some evidence to suggest that different PS genes requiredifferent levels of active PrrA for their activation (20).

In R. capsulatus, a truncated form of the PrrB homolog RegB lacking the membrane-associated domain phosphorylates the PrrAhomolog RegA in vitro (39). A point mutation involving a Leu-to-Prochange at position 78 of the PrrB protein (PRRB78) confers anoxygen-insensitive phenotype on the cell (21); i.e., PS geneexpression is "full on" under both aerobic and anaerobic conditions.This region of the protein is believed to be located in a nonmembranouscytoplasmic loop far removed from the active histidine.

The role of PrrC, SenC in R. capsulatus (11), in PS gene expression is much more subtle than that of PrrA or PrrB. PrrCshares amino acid sequence similarity with the yeast ScoI andScoII proteins (10) believed to be involved in the assemblyof mitochondrial cytochrome c oxidase subunits. PrrC appears tobe membrane localized, based on prrC'-'phoA fusion analyses (21),with the carboxy-terminal region of the protein located in theperiplasmic space.

(iii) AppA. The appA (activation of photopigment and puc expression) gene resides at approximately 1285 kbp clockwise on chromosomeI; i.e., approximately 1.2 Mb from the PS gene cluster (28).Deletion of appA results in greatly diminished SC formation, whichcorrelates with decreased expression of the corresponding PS genes(28) (Fig. 1). Low levels of SC result in a prolonged lag inthe growth of an AppA null mutant when it is shifted from aerobicto anaerobic light conditions, and this is followed by reducedphotosynthetic growth rates (31). However, anaerobic dark growthis normal (31).

AppA consists of 450 amino acids and shows no homology with proteins of known function. Following overexpression of severaltruncated forms of the protein, specific ligand binding has beenobserved. The approximately 120-residue amino-terminal domainhas been shown to bind flavin. The approximately 70-residue carboxy-terminaldomain contains an unusual cysteine-rich motif which is capableof binding iron or, more likely, an Fe:S center. The central regionof AppA appears to bind a heme. Removal of either the amino- orcarboxy-terminal portion of AppA result in only slight impairmentof AppA function, as judged by complementation of an AppA nullmutant (32).

The activity associated with AppA is currently unknown. However, AppA affects PS gene expression independently of both thePrr and FnrL systems (31). Existing data strongly suggest thatAppA antagonizes PpsR repressor activity (31) (see below). Whetherthe role of AppA is limited to PpsR alone has yet to be elucidated.

DNA-binding factors. (i) Anaerobiosis activator/repressor FnrL. The fnrL gene encodes the R. sphaeroides 2.4.1 homolog of Fnr (Fig. 1), the E. coli anaerobic regulatory protein. It is locatedat approximately 443 kbp on chromosome I, in close proximityto the ccoNOQP and rdxBHIS operons of R. sphaeroides 2.4.1 (94).FnrL mutant strains are unable to grow anaerobically, either photosyntheticallyor in the dark using DMSO as an electron acceptor, and such mutantshave no detectable SCs under conditions of ICM induction (94).

FnrL has 11 of 22 amino acid identities with E. coli Fnr within the region corresponding to the helix-turn-helix DNA-bindingdomain. Residues that are thought to form direct amino acid-basecontacts (54) are identical between the two. Therefore, we suggestthat the recognition sequence for binding by FnrL resembles theFNR (fumarate nitrate regulator) consensus sequence, TTGAT-N₄-ATCAA.Sequences similar or identical to this consensus sequence havebeen identified upstream of several genes involved in tetrapyrroleand Bch1 biosynthesis, including hemA (68), hemZ (94), hemF(recently renamed hemN) (18) and bchE (28, 95), as wellas the puc operon (56). Under conditions of reduced oxygen tension,FnrL activates expression of hemA (94) and the puc operon (95).These results provide good evidence that the target sequence forregulation by FnrL is the FNR consensus sequence.

In contrast to R. sphaeroides, an FnrL mutant strain of R. capsulatus which has been shown to contain an fnrL homolog is unaffectedin its ability to grow photosynthetically with many of the genesdescribed above, lacking upstream FNR-binding sequences (92).However, like R. sphaeroides FnrL mutant strains, an FnrL mutantof R. capsulatus is incapable of anaerobic growth in the darkwith DMSO (92). For both R. sphaeroides and R. capsulatus, theDMSO-inducible cytochrome c (encoded by dorC) and DMSO reductase,encoded by dorA (65), are not induced in the mutant strains(93). It appears that the role of FnrL in dor operon (65)expression is mediated through the FnrL-dependent regulation ofdorS. DorS, which encodes a redox-responsive sensor histidinekinase, regulates its cognate transducer, the product of the dorRgene (65).

Based on the presence of upstream FNR consensus sequences (94), the ccoNOQP operon, the rdxBHIS operon, and the ctaD andctaABC genes (24, 36) encoding subunits of the aa₃ cytochromeoxidase are likely to be regulated, in whole or part, by FnrLin R. sphaeroides (94). Thus, FnrL could, by affecting the abundanceof these redox carriers, control the flow of electrons throughthe respective terminal oxidases and the Rdx redox center. Thishas been shown to be true for the ccoN gene. In addition to directlyeffecting puc operon transcription due to the presence of an upstreamFNR-binding sequence (95), FnrL could also indirectly affectpuc operon transcription (95, 96) through its regulation ofccoNOQP and, thus, the signal reaching Prr (71).

(ii) PpsR. The upstream regions of many bch and crt genes and operons, as well as the puc operon from both R. sphaeroides and R. capsulatus,contain the same dyad symmetry motif (Fig. 1), TGT-N₁₂-ACA (52,56, 61). The localization of this motif downstream of, oroverlapping with, putative $sigma$ ⁷⁰-type promoters of PS genes and studies of the cis regulatoryelements of the puc operon (56, 59) suggest that this sequencecan function as a repressor-binding site. This repressor-encodinggene, designated ppsR (photopigment suppression) in R. sphaeroides(73; Fig. 1), was identified because of its ability to suppressphotopigment production in wild-type cells when provided in extracopy. Inactivation of ppsR results in constitutive expressionof both the photopigment genes and puc, which triggers productionof SCs, even under aerobic conditions, thus making such mutantsgenetically unstable under these conditions (31, 74).

ppsR is localized within the region of PS genes, at approximately 26 kbp on chromosome I. PpsR contains a putativehelix-turn-helix motif at the carboxy terminus which resemblesthose found in several known DNA-binding transcription factors(74). The ability of PpsR to act as a repressor has been demonstratedgenetically in E. coli (74) and in Paracoccus denitrificans(29). Point mutations in the putative DNA-binding region resultin decreased repression (31, 56, 59). It has been shownthat the PpsR protein overexpressed in E. coli and P. denitrificansspecifically retards DNA fragments containing the sequence TGT-N₁₂-ACA(32). The PpsR homolog from R. capsulatus, designated CrtJ,has been purified recently and shown to bind to this motif asa dimer (75). Cooperative binding of CrtJ to two binding motifspositioned in the regulatory regions of several putative CrtJ/PpsRtarget genes, has also been indicated, which correlates well withearlier genetic studies (29).

R. sphaeroides ppsR gene expression is largely independent of growth conditions, and PpsR repressor activity does not responddirectly to oxygen deprivation. Therefore, other cellular factorsare required to communicate to PpsR the state of oxygen availabilityand changes in growth conditions (31, 32). Further, PpsR functionsas a repressor not only under aerobic but also under anaerobicphotosynthetic conditions, where it regulates LHII SC abundance,depending on light intensity (31). Because it is unlikely thatPpsR senses both oxygen and light directly, we believe that PpsRmust respond to an integral signal generated by changes in eitherof these environmental stimuli, e.g., either redox poise or aredox carrier. This view is complemented by the in vitro analysisof the R. capsulatus repressor protein, whose DNA-binding capacityhas been shown to depend on redox-active agents (75).

The nature and regulation of the redox sensitivity of PpsR remain largely unknown (Fig. 1). Disruption of the ppsR gene inan AppA null mutant background completely overcomes the impairment(s)imposed by the appA null mutation. Furthermore, a large numberof suppressors of the appA null mutation, showing improved photosyntheticgrowth, contain point mutations in ppsR, and partial suppressionof the appA null mutation can be achieved by titration of PpsRin vivo (31, 32). AppA significantly decreases PpsR-mediatedrepression when these genes are simultaneously expressed in P.denitrificans (31). Therefore, we believe that AppA serves toregulate PpsR repressor activity by communicating a redox signalto PpsR which is ultimately derived from oxygen- and/or light-generatedredox responses. The signal could affect either the redox stateof PpsR or its dimerization or both. The overall role of PpsRin both oxygen and light control of SC formation, as well as itsspecificity toward PS genes, makes it a major player in PS generegulation.

(iii) Spb. The hvrA gene of R. capsulatus, located immediately downstream of the response regulator regA, is involved in regulation ofRC and LHI SC gene expression (12). The hvrA gene encodes asmall, 104-residue DNA-binding factor. Analogous to hvrA, a homologfrom R. sphaeroides, termed spb, is positioned immediately downstreamof prrA (77). Both Spb (Sphaeroides puf-binding protein) andHvrA bind upstream of the puhA gene and the puf operon under variousconditions (49, 80). The amino-terminal regions of Spb andHvrA bear similarity to the HU-like proteins from E. coli andbacteriophages (49, 77). These proteins often have multipletargets and therefore are involved in transcriptional regulationof a variety of processes. Conforming with this idea are recentobservations that HvrA is also involved in the ammonium regulationof nitrogen fixation in R. capsulatus (62). Thus, these proteinsmay be involved in PS gene expression by facilitating the bindingof other transcription factors, e.g., PrrA, RNA polymerase, etc.,and their role in light regulation may be a reflection of theirabundance as a function of light intensity. It was also foundthat the amino terminus of Spb has some homology to the leucinezipper motif of the eukaryotic transcription factor c-JUN. Thismotif is proposed to play a role in protein dimerization (80).Because it is difficult to describe a more specific role for thesefactors, they have not been included in Fig. 1.

(iv) IHF. The integration host factor (IHF) of E. coli is a global regulatory protein which acts by binding DNA targets and bendingthe DNA so that looping occurs. This brings together noncontiguousregions of the DNA, which interact through DNA-binding regulatoryproteins (88). The genes for the two subunits of the R. sphaeroidesIHF heterodimer have been cloned (78). Interestingly, the himAgene is located at approximately position 1760 kbp on chromosomeI, while the himD (hip) gene is located at approximately 830kbp on chromosome II. In vitro studies have shown that IHFof E. coli binds to the regulatory region of the puc operon (58).Additionally, mutations that alter the consensus IHF-binding sitein this region abolish binding in vitro and negatively affectpuc expression in vivo.

Modulators of PS gene transcription. The tspO gene (formerly crtK, or orf160 in R. capsulatus), located within the crt gene cluster on chromosome I, encodes a17-kDa protein (tryptophan-rich sensory protein) which is characterizedby an unusually high content of aromatic amino acids, especiallyL-tryptophan. TspO (Fig. 1) has been localized to the outer membraneof R. sphaeroides 2.4.1 (90) and is present at severalfold higherlevels in photosynthetic than in aerobically grown cells. Resultsof cross-linking studies suggest that TspO may form a homodimerwithin the bacterial membrane (91).

A TspO mutant has higher levels of Crt and Bchl than do wild-type cells when strains are grown aerobically or semiaerobically.The effect of TspO on pigment production occurs at the level oftranscription of those same crt and bch biosynthetic genes whichconstitute the PpsR regulon (90). TspO also negatively affectsthe expression of the puc operon under both aerobic and photosyntheticconditions but has no effect on the expression of the puf operon.The available evidence implicates TspO as a both oxygen- and light-responsivemodulator of PS gene expression with the same spectrum of regulatorytargets as the PpsR repressor (29, 90). How a signal is transmittedfrom outer membrane-localized TspO to the cell interior is unknown.However, the quantitative effect of TspO upon PS gene expressionis not as strong as that of PpsR, which suggests that there mustbe other elements or factors interposed between TspO and the PpsRregulon.

Useful information about the physiological activity of TspO may be drawn from studies on its mammalian homolog (91), the18-kDa outer membrane component (pk18) of the mitochondrial peripheralbenzodiazepine receptor (MBR). Although the precise biologicalrole of MBR is not yet understood, this receptor was shown tobe involved in the regulation of steroidogenesis, heme biosynthesis,mitochondrial respiratory control, and other metabolic activities(51). The rat pk18 gene, when expressed in R. sphaeroides inthe TspO background, functionally substituted for the bacterial homolog,negatively affecting the expression of crtI and puc. Additionally,when the pk18 gene was expressed in R. sphaeroides, it retainedits quantitative binding properties towards a variety of MBR ligands.These results suggest that TspO is both evolutionarily and functionallyrelated to the mammalian MBR and indicate the possibility thatin both bacterial and mammalian cells, these proteins are involvedin similar metabolic activities (91).

How TspO might "sense" and "transmit" an oxygen- or light-generated signal remains a mystery, although no ligand has beenfound to be associated with TspO. Very recent results suggestthat TspO may be involved in regulating the entry of specificsmall molecules through the outer membrane in response to oxygenand light. Mutants with single changes of the five conserved tryptophanshave either lost or retain partial TspO activity.

Other elements in PS gene expression. Several additional factors have been observed to effect PS gene expression, but their precise role is presently unknown. Theppa (photopigment activation) gene (also known as ppsS and orf192)is positioned immediately upstream of ppsR (29). A role forPpa in controlling PpsR repressor activity has been proposed butnot yet tested (74). Thus, we have not included Ppa in Fig.1. A locus at 2110 kbp on chromosome I, identified by virtueof its effect on expression of the puc operon (76), has beennamed mgpS (modulator of genes for photosynthesis) and containsan open reading frame of ~2.8 kb. The N-terminal portion of mpgSshares similarity with a number of RNA helicase proteins whichare involved in RNA modifications (76), suggesting that mpgSmay have an additional role in posttranscriptional regulationof PS gene expression. The rpgS1 gene (regulator for photosystemgenes; 77) a histonelike protein located approximately 500bp clockwise from prrA, encodes a protein with similarityto the functionally unidentified orf5 gene from R. capsulatus(13). The rpgS1 gene is predicted to encode a protein of 187amino acids which contains a putative helix-turn-helix motif locatedat its amino-terminal end (77).

Regulation of PS gene expression at the message level. As is evident from the previous sections, transcriptional regulation of PS gene expression plays a crucial role in PS formationin R. sphaeroides 2.4.1. However, it has been observed that mRNAscorresponding to the structural polypeptides of the SCs are producedin excess, relative to the actual levels of the complexes presentunder a variety of growth conditions (34, 55, 67, 81).This provides evidence of posttranscriptional regulation. Suchcomplexity of regulation is not surprising, given the fact thatPS development requires coordination of a variety of diverse processes,involving protein and pigment biosynthetic pathways, SC assembly,and adaptation between alternative cellular steady states.

In the related organism R. capsulatus, PS genes are organized into superoperons (reviewed in references 5, 6, and 48).It is thought that there are multiple transcription initiationsat several start sites within the superoperons which result indifferences in message levels for genes and operons within thesuperoperons. However, degradation of larger transcripts is alsoconsidered to contribute to the disproportionate representationof gene messages in the cell (reviewed in reference 48). Somedata also suggest the possibility that degradation of large transcriptsis regulated by oxygen tension (46, 47).

While certain large transcripts indicative of a similar superoperon organization have been detected in R. sphaeroides (63),their physiological role, if any, is not known. In the case ofthe puc and puf operons of R. sphaeroides, multiple transcriptswith differing half-lives are also detected. The longer puc andpuf transcripts have been shown to be products of transcriptionalreadthrough of terminatorlike sequences within those operons (55,57).

The first gene of the R. sphaeroides puf operon is the pufK gene, encoding a 20-amino-acid-residue polypeptide. It has beendemonstrated that pufK is translated and that its expression iselevated severalfold under high-light PS conditions, comparedto that in aerobically grown cells (33). An interesting featureof the pufK gene is the high occurrence of rare codons, with 9of the 20 codons of pufK among those rarely used by R. sphaeroides2.4.1. Studies suggest that translation through these rarely usedcodons serves to "gate" the entry of ribosomes to the immediatedownstream pufBA cistrons (Fig. 1) and, as such, can affect thecellular abundance of the $alpha$ and $beta$ polypeptides of the LHI complex(33).

	THE ROLE OF BCHL AND CRT

Bchl and Crt are major nonprotein structural components of the SCs whose synthesis is regulated in response to oxygen availabilityand/or light intensity (Fig. 1). The availability of Bchl hasbeen shown to be of critical importance and the limiting componentfor the formation and stability of the RC and the LH SCs (87).The puf-encoded RC-M and RC-L polypeptides, as well as the puhA-encodedRC-H protein, are detected at low levels under aerobic growthconditions but are rapidly degraded due to the absence of Bchl,both in R. sphaeroides and in R. capsulatus (16, 84, 85,87).

Unlike Bchl, Crt are not essential components of the RC or the B875 complex, and mutants defective in Crt biosynthesis genesare photosynthetically competent. In contrast, the formation ofthe LHII complex requires colored Crt (intermediate products ofthe Crt biosynthetic pathway downstream of neurosporene), andit has been proposed that this requirement may be at the levelof assembly (53). The type of Crt accumulated is also importantin determining the relative stoichiometry between the two LH complexes.Spheroidenone (SO), the end product of the Crt biosynthetic pathway,is predominantly associated with the RC and LHI complexes, whereasspheroidene (SE), the penultimate product of the Crt pathway,is more abundant in the LHII complex (38, 89). The relativeamounts of these two major Crt pigments are regulated in responseto oxygen tension and/or light intensity, apparently through thelocalized cellular redox state (Fig. 1), which affects the CrtA-catalyzedconversion of SE to SO (89).

The Cco/RdxB putative oxygen-sensing, redox signal-generating pathway has been demonstrated to affect the regulation, throughthe Prr regulon (71), of the type of Crt accumulated under photosyntheticand diazotrophic growth conditions. Presumably, the localizedredox poise generated through these pathways affects CrtA activity(70). Thus, the signal generated by the cbb₃ oxidase-RdxB systemis transferred not only to transcription factors through the Prrpathway (see the section on sensors, signal generators, and transducers)but also to another pathway(s) involved in the control of theconversion of SE to SO under photosynthetic conditions. The recentlydiscovered gene likely to encode the first enzyme in the isoprenoidbiosynthetic pathway (82) and the next downstream gene in thebiosynthetic pathway, mapping to the PS gene cluster, are of majorimportance and are predicted to be highly regulated. These dataprovide further evidence that Cco and RdxB are "functional" asredox carriers under anaerobic, as well as aerobic, growth conditions,perhaps interacting with a light-generated redox intermediate.

Conditions which limit Bchl availability (such as high light illumination or high oxygen tension) are also characterized bylow SE and high SO levels and correspond to limited LHII formation(89). Therefore, the net result is that available Bchl is incorporatedinto the RC and LHI complexes (Fig. 1), which appear to have nopreference for which Crt is used in the assembly process (Fig.1). In this way, changes in environmental conditions (to whichBchl levels and Crt accumulation are evidently sensitive) canbe rapidly reflected by changes in LHII complex formation andthis, in turn, may result in the de facto regulation of RC andLHI complex assembly and ultimate abundance (89).

	ASSEMBLY FACTORS

Genes have been identified whose proposed role in the regulation of PS formation is at the level of SC assembly (Fig. 1).One of these genes is the monocistronic Q gene, located immediatelyupstream of the puf operon of R. sphaeroides, encoding a 187-amino-acidpolypeptide (34). Single amino acid substitutions in the Q geneproduct have dramatic consequences for the formation of SCs, e.g.,loss of LHI complex formation ability for one group of mutants,loss of LHII complex formation ability for another group, andaltered levels of both SCs relative to those in wild-type cellsfor a third group, despite little or no changes in specific mRNAlevels or Bchl and Crt availability. In the absence of the Q geneproduct, the cells are unable to grow under PS conditions. Basedon these studies (34), the Q gene product is proposed to beinvolved in the assembly of the SCs. However, in R. capsulatus,the structure of the Q gene and the function of its product havebeen interpreted differently (7).

orf1696, located immediately upstream of puhA (14) of R. sphaeroides 2.4.1 (Fig. 1), has been shown to be required for LHIcomplex formation (81). The pucC gene product (Fig. 1) is requiredfor LHII complex formation (43, 57, 85). These genes areproposed to encode complex-specific assembly factors (CSAFs).These two factors, together with the product of a third gene,which is called orf428 in R. capsulatus (14) but is not knownto participate in SC formation (8), are similar to each other.This similarity may indicate common interactions with other factors,as part of an overall assembly hierarchy for the SCs. One of theseinteractions may be with the Q gene product (81). Thus, thespecific role of the Q gene product is thought to be through theinsertion of Bchl into the developing SCs (Fig. 1) in a processinvolving interaction(s) with the CSAFs (Fig. 1) (34). The differencein the affinities of the Q polypeptide for the CSAFs would thenaccount for the preferential assembly of the RC complex, followedby the LHI complex, and finally the LHII complex when Bchl isplentiful.

Some of the more conventional chaperone genes have also been identified in R. sphaeroides; e.g., there are two groE operons(60). However, the role (if any) of these and/or other chaperonesin SC formation has not yet been defined.

	OVERALL MODEL FOR THE REGULATION OF SC FORMATION

In the presence of oxygen, the R. sphaeroides cell membrane resembles that of other gram-negative bacteria. Energy for cellularmetabolism is derived from aerobic respiratory chains, terminatingat either one of two cytochrome c oxidases (the low oxygen affinityaa₃ oxidase or the high oxygen affinity cbb₃ oxidase or a bb₃-typequinol oxidase (reviewed in reference 26). There is virtuallyno Bchl or Crt synthesized. There are low but detectable levelsof transcription of the PS genes encoding the apoproteins of theSCs; in the absence of Bchl, these polypeptides turn over rapidly,although they are transported to the cell membrane and assumetheir proper topological orientation within the membrane.

When oxygen tension is reduced, transcription of PS genes is activated in response to three key regulatory systems, namely,the FnrL, Prr, and PpsR systems. We propose that these systemsreflect change in the localized cellular redox poise or a criticalredox intermediate(s) when oxygen tension is lowered. Yeliseevand Kaplan have demonstrated that TspO modulates this response(90). Similarly, the biosynthesis of Bchl and Crt ensues inresponse to these changes and SC formation can now occur.

The state of activation of the putative oxygen-labile [4Fe-4S] center of FnrL as a function of oxygen availability is thoughtto regulate the activity of FnrL. FnrL can act directly to activatespecific PS gene transcriptions, which reflect critical pointsof control, in the tetrapyrrole and Bchl pathways, as well aspuc operon expression. FnrL also affects PS gene expression throughits regulation either positively or negatively of specific redoxchains, e.g., cbb₃ or aa₃.

The Prr two-component regulatory system, in response to an altered signal emanating from the cbb₃/RdxB redox pathway can beginto activate transcription of all or, certainly, most of the PSgenes. Presumably, PrrB is no longer inhibited by this signal,to which it responds by activating PrrA in a mechanism believedto involve PrrB autophosphorylation and subsequent phosphorylationof PrrA. While the means by which PrrA regulates transcriptionof the PS genes is not precisely known, it may involve directDNA binding or the formation of transcriptional complexes involvingother protein factors, the net result being an increased expressionof genes encoding all of the structural components of the SCs.The data also suggest that different levels of activated PrrAmay be required to activate different subsets of PS genes.

In contrast to FnrL and Prr, which have a broad spectrum of gene targets, PpsR appears to repress specifically PS genes; i.e.,most of the bch and crt genes, as well as the puc operon, whichcontain the repressor-binding sequence TGT-N₁₂-ACA. Repressionby PpsR, although relieved under anaerobic conditions, is stillresponsive to light under these conditions, and derepression isbrought about, at least in part, by the action of the flavohemoproteinAppA, which acts either directly or indirectly on PpsR. The factthat PpsR is involved in PS gene control in response to both oxygenand light, perhaps through AppA, suggests that a different sourceof a redox-generated signal is involved in the transmission ofthis effect than in Prr-mediated regulation. However, this remainsto be proven.

TspO modulates the rate of activation of PS gene derepression as oxygen tensions are decreased. Other modulators appear toinclude PrrC, Ppa, HvrA (Spb), and MgpS, as well as IHF. Overall,as the O₂ tension decreases, there develops a cascade of bothorderly and progressive events which serve to reinforce the inductionof PS gene expression. This cascade must also involve subtle interactionsbetween the system of activation and repression of PS gene expression,as oxygen tensions change and as light intensities vary underanaerobic conditions.

The net result of these transcriptional changes is that all of the components leading to SC formation are present at increasedlevels when oxygen tension is reduced, and the assembly processspecific to each can take place. The total amounts of SC formeddepend upon the cellular level of Bchl which, in turn, is determinednot only by the activity of Bchl biosynthetic enzymes but alsoby the available pool of 5-aminolevulinic acid, and therefore,Bchl serves as the ultimate "governor" regulating cellular abundancesof SCs. The Q protein, together with CSAFs, direct the flow ofBchl into the assembling SCs in a hierarchical fashion, with RCassembly first, followed by assembly of the B875 SC, and thenassembly of the B800-850 SC. Usually, the mRNA levels, and thelevels of apoproteins produced, are in excess of cellular needs.The abundance and composition (SE and SO) of the Crt present arealso important for the ratio of LH complexes. Thus, posttranscriptionalregulatory pathways serve to increase the ability of cells torespond rapidly to changes in oxygen availability and light intensity.

Although it has long been known that the amount of SC varies dramatically under anaerobic conditions, depending on the lightintensity, the mechanism(s) of light control of PS formation isless well understood than that of oxygen control. We do know,however, that light regulation is achieved, at least in part,through the same transcriptional regulatory machinery which operatesin response to changes in oxygen tension, e.g., PpsR/AppA (31)and HvrA (Spb) (49). It is also tempting to speculate that cbb₃and RdxB play some role(s), as well, in photosynthetically growingcells. This lends support to the idea that changes in light intensityare first transformed into changes in the cellular redox state.However, the presence of specific light-dependent regulators cannotbe ruled out at present. We currently believe that light controlof PS formation occurs mostly at posttranscriptional levels andinvolves rapid changes in Bchl levels and the cellular levelsof SO and SE. Together with the available assembly factors, theseelements will rapidly determine the abundance and kinds of SCs.

	ACKNOWLEDGMENTS

All of the authors contributed equally to this work.

This work was supported by grant GM15590 from the U.S. Public Health Service.

	ADDENDUM IN PROOF

We have recently observed that the ccoNOQP operon is negatively regulated by the two-component Prr system under aerobic growthconditions.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Molecular Genetics, University of Texas Health SciencesCenter-Houston, 6431 Fannin Street, Houston, TX 77030. Phone:(713) 500-5502. Fax: (713) 500-5499. E-mail: skaplan{at}utmmg.med.uth.tmc.edu.

Present address: Department of Biological Sciences, Oakland University, Rochester, MI 48309.

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MINIREVIEW Control of Photosystem Formation in Rhodobacter sphaeroides

MINIREVIEW
Control of Photosystem Formation in Rhodobacter sphaeroides