Analysis of the puc Operon Promoter from Rhodobacter capsulatus

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Nickens, D. G.
	Articles by Bauer, C. E.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Nickens, D. G.
	Articles by Bauer, C. E.

Previous Article | Next Article

Journal of Bacteriology, August 1998, p. 4270-4277, Vol. 180, No. 16
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Analysis of the puc Operon Promoter from Rhodobacter capsulatus

David G. Nickens and Carl E. Bauer^*

Department of Biology, Indiana University, Bloomington, Indiana 47405

Received 8 April 1998/Accepted 9 June 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Expression of the Rhodobacter capsulatus puc operon, which codes for structural polypeptides of the light-harvesting-II peripheralantenna complex, is highly regulated in response to alterationsin oxygen tension and light intensity. To obtain an understandingof the puc promoter region we report the high-resolution 5' mappingof the puc mRNA transcriptional start site and DNA sequence analysisof the puc upstream regulatory sequence (pucURS). A $sigma$ ⁷⁰-type promoter sequence was identified (pucP1) which has a highdegree of sequence similarity with carotenoid and bacteriochlorophyllbiosynthesis promoters. Inspection of the DNA sequence also indicatedthe presence of two CrtJ and four integration host factor (IHF)binding sites. Transcriptional fusions of the pucURS fused tolacZ also confirmed that puc promoter activity is regulated bythe transcriptional regulators IHF, CrtJ, and RegA. Gel retardationanalysis using cell extracts indicates that mutations in IHF andRegA disrupt protein binding to DNA fragments containing the pucURS.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The Rhodobacter capsulatus photosynthetic apparatus is composed of three membrane-spanning photopigment protein complexesknown as the reaction center and the B875 light-harvesting-I (LH-I)and B800-850 light-harvesting-II (LH-II) antenna complexes (15,56). The light-harvesting complexes are responsible for absorptionof most of the light energy that irradiates the cells. The absorbedenergy is subsequently passed to the reaction center, which donatesan electron from bacteriochlorophyll to ubiquinone. Structuralstudies indicate that the reaction center is surrounded by a pigmentedring composed of 16 LH-I $alpha$ and $beta$ polypeptide pairs (18). Thereaction center-LH-I core complex is, in turn, associated witha variable number of LH-II rings composed of nine $alpha$ and $beta$ polypeptidepairs (28, 31, 56).

The $alpha$ and $beta$ structural proteins of the LH-II antenna complex are encoded by the pucBA gene pair that has been found in allphotosynthetic purple nonsulfur bacteria that have been examined(56). Organization of this gene pair on the chromosome, thesize of the intergenic region between the pucB and pucA genes,the proteins they encode, and their regulation are highly conservedamong purple nonsulfur bacteria (2, 4, 10, 19, 24,36, 56). The R. capsulatus puc operon contains three additionalopen reading frames, pucC, pucD, and pucE (43, 45). PucC isthought to be involved in assembly of the LH-II ring (23, 57),but the roles of PucD and PucE have not yet been established (23,45).

Northern blot analysis has demonstrated the presence of several puc transcripts including a 2.4-kb segment coding for pucBACDE,a 1.0-kb segment composed of a mixture of pucC and pucDE transcriptsthat are thought to be generated as processing products from thelarger pucBACDE transcript, and a 0.55-kb pucBA segment (5,23, 44). A predicted secondary structure is located in thepucA-pucC intercistronic region, and it has been suggested thatthe short pucBA transcript may be generated by differential decayof the larger pucBACDE transcript (24, 44, 57). This presumablyoccurs in a manner analogous to the well-characterized mRNA processingevents that generate a stable pufBA mRNA segment that codes forthe LH-I structural polypeptides (6, 20, 21, 23, 54,55).

Given the numerous studies that have been undertaken on the regulation of puc expression, it is surprising that there is relativelylittle information regarding the R. capsulatus puc promoter. Todate, neither high-resolution mRNA mapping or detailed promoterdeletion studies have been undertaken on the R. capsulatus pucpromoter. In contrast, detailed studies on the puc promoter fromRhodobacter sphaeroides have indicated that oxygen and light controlof promoter activity involve a complex set of cis-acting regulatorysites, some of which are located at extended distances (up to629 bases) from the start of transcription (25-27). Clearly, comparablestudies on the R. capsulatus puc promoter are warranted, and indeednecessary, now that several transcription factors responsiblefor controlling puc expression in response to oxygen have beenidentified and isolated from this species (4, 32, 35, 41).

As a prelude to performing DNA binding studies of transcription factors to the puc promoter region, we need to have a goodunderstanding of the location of transcription initiation as wellas of the functional length of the puc promoter region. Consequently,this study describes the high-resolution mapping of the startsite of puc expression coupled with detailed in vitro and in vivomapping of the puc promoter. Our results indicate that the R.capsulatus puc operon has a single transcriptional start sitelocated 116 bp upstream from the initiation codon of pucB andthat the putative puc promoter exhibits a $sigma$ ⁷⁰-type sequence motif that is similar to that of the carotenoid(crt) and bacteriochlorophyll (bch) promoters (1, 3, 30,50). Functional length of the puc promoter region was also analyzedby both deletion analysis and gel mobility shift analysis usingcrude extracts derived from various regulatory mutants that areknown to affect puc expression.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Bacterial strains and cultures. All bacterial strains used in this study are listed in Table 1. R. capsulatus strains were routinely grown at 34°C in peptone-yeastextract (PY) broth or agar medium (52), whereas Escherichiacoli strains were routinely grown at 37°C in Luria broth (LB)or agar medium (38). For maintenance of plasmids, spectinomycinor kanamycin was added to media at a concentration of 10 µg/mlfor R. capsulatus. For E. coli, spectinomycin, kanamycin, andrifampin were used at a concentration of 100 µg/ml, whereas ampicillinwas used at a concentration of 200 µg/ml.

View this table:
[in this window]
[in a new window]

TABLE 1. Bacterial strains used in this study

Growth of R. capsulatus under aerobic-dark conditions was achieved by growing 20-ml cultures in 250-ml Erlenmeyer flasks withshaking (300 rpm). Anaerobic photosynthetic conditions were achievedby growing cultures in completely filled 17-ml-capacity screw-captubes under high (7,000 lx)- or low-light conditions (200 lx)with banks of incandescent lumiline (Sylvania 30W) lamps. To preventoxygen depletion in aerobic cultures or self-shading in photosyntheticcultures, R. capsulatus cells were harvested at a cell densityof ca. 1.5 × 10⁸, which corresponds to 50 Klett-Summerson photometer units whenfitted with a no. 66 filter.

DNA manipulations and promoter probe analysis. Descriptions of plasmids used in this study are listed in Table 2. Standard recombinant DNA techniques were performed withE. coli DH5 $alpha$ as a host (38). Restriction enzymes and T4 DNAligase were purchased from New England BioLabs, Inc. The promoterprobe vector pZM400 was used to make transcriptional fusions ofthe puc upstream regulatory sequence (pucURS) to a promoterlesslacZ gene (30). Details are given in Table 2.

View this table:
[in this window]
[in a new window]

TABLE 2. Plasmids and phage used in this study

Plasmids pDN14 and pDN15 each have internal BstEII sites that were not compatible with the BstEII site needed for cloningin plasmids pDC400 and pZM400 (30). Thus, conversion adapters(5' GTACCGAAGGGGTTCGC and 5' GTCACGCGAACCCCTTCG) were used tomutate the internal BstEII sites in pDN14 and pDN15 to compatibleBstEII sites according to the method of Stover et al. (42).pDN16 and pDN18 were constructed by cloning a BstEII-SphI DNAfragment from pDN14 and pDN15 into pDC400. For these constructionsthe presence of an internal SphI site was circumvented by RecA-mediatedprotection (29) by using RecA (Promega Corp.) and nonhydrolyzable[ $gamma$ -S]ATP (Sigma Corp.) in conjunction with the SphI-RecA protectionoligonucleotide (CGCCGATCTCGACCGGCATGCCCTCGGCGGCCTCGC).

Strain constructions. Mobilization of plasmids from E. coli DH5 $alpha$ to R. capsulatus was accomplished by triparental mating with E. coli HB101 harboringthe helper plasmid pRK2013, which conjugates plasmids containingan RK2 origin of replication (14, 30). Donor and helper strainswere grown with antibiotic selection overnight, centrifuged, resuspendedin fresh LB with a 1:10 dilution, and incubated for 2 h beforemating, while recipient strains were grown overnight in PY medium.Spot matings were performed on the surface of plates of slightlydry RCV medium (49) for 2 h of incubation followed by soft agaroverlay containing appropriate antibiotics. After a 48-h incubation,transconjugants were purified by repeated streaking on RCV mediumsupplemented with 10 µg of spectinomycin/ml.

Strain IR4 (himA) (46) was made resistant to 100-µg/ml rifampin by gene transfer agent (GTA)-mediated transduction as previouslypublished (51). GTA was obtained from the rif10 GTA-overproducingstrain, CB1127 (52). The rifampin-resistant derivative of IR4was used throughout this study for reporter plasmid expressionstudies as well as for gel mobility shift analysis.

$beta$ -Galactosidase assays. Cell extracts were prepared and assayed for $beta$ -galactosidase activity as described by Young et al. (52). Protein concentrationswere determined by Bradford assay (9). Final results are reportedas the amount of o-nitrophenyl- $beta$ -galactoside (ONPG) hydrolyzedper minute per milligram of total protein. Reported $beta$ -galactosidasevalues all had standard deviations of $<=$ 6.2%.

Dideoxynucleic acid sequencing. puc operon subclones in M13mp18 and M13mp19 were used to generate single-stranded DNA (ssDNA) templates in both orientationswhich were used for DNA sequence analysis (38) (Table 2). PlasmidpRPSLHIIKAN was digested with ClaI and then blunt ended with DNApolymerase I Klenow fragment, followed by digestion with EcoRI,releasing a 2-kb EcoRI-ClaI fragment that includes the pucURS(53). The EcoRI-ClaI fragment was subcloned into the EcoRI-AccIsites of the M13 phage vectors. DNA sequence was obtained by usingthe Sanger dideoxynucleotide chain termination method with modifiedT7 DNA polymerase (Sequenase; U.S. Biochemical Corp.) in combinationwith the nucleotide analog 7-deaza-guanidine added to reactionmixes. DNA sequence data were analyzed and assembled using programsfrom the GCG Sequence Analysis Package of the University of WisconsinGenetics Computer Group. All oligonucleotides used for DNA sequencingare shown in Fig. 1.

View larger version (63K):
[in this window]
[in a new window]

FIG. 1. Primers used to analyze the puc promoter region. Arrows located above the strand indicate primers identical to the strand shown, whereas primers located below the strand are complementary. Dotted lines indicate nonhomologous sequences added for cloning with the following scheme: PCR1, GCGGTAACC; PCR2, GCGCATGC; PCR3, GCTACGTA; PCR4, GCGGGCC; PCR5, GCGCATG; PCR6, GCGGTAACC; PCR7, GCGCATGC; PCR8, GCGCA. Sequence numbers indicate location relative to the start of the pucB gene, which is numbered +1. Primers Puc1, Puc2, Puc3, and Puc4 were used for sequence, Northern blot, and primer extension analyses. Primer Puc5 was used for sequence and primer extension analyses, and Puc6 was used for sequence analysis. Primers Puc7, PucRev1, PucRev2, PucRev3, PucRev4, PucRev5, PucRev6, and PucRev7 were used for sequence and Northern blot analyses. Primers PCR1, PCR2, PCR3, PCR4, PCR5, PCR6, PCR7, and PCR8 were used as PCR primers.

Northern blot mRNA transcript analysis. Total RNA was isolated from R. capsulatus cells grown photosynthetically in 500-ml tissue culture flasks completely filledwith PY medium by the guanidinium thiocyanate method of Chomczynskiand Sacchi (12). Northern blot analyses were performed by sizeseparating 30 µg of RNA on a 1.5% agarose gel containing 8.4%(vol/vol) formaldehyde. RNA was then blotted onto a nylon membrane(Nytran) by capillary transfer in 20× SSC buffer (1× SSC is 0.15M NaCl plus 0.015 M sodium citrate) (38) and then UV cross-linkedto the filter by exposure to 120 J of UV irradiation. Filterswere hybridized for 16 h with the ³²P-labeled Puc1 oligonucleotide (Fig. 1) in a hybridization solutioncomposed of 0.5 M NaH₂PO₄ (pH 7.2), 1 mM EDTA, 6.8% (wt/vol) sodiumdodecyl sulfate (SDS), 10 mg of bovine serum albumin/ml, and 100µg of sheared salmon sperm DNA/ml at 52°C (38). Following hybridization,filters were washed in 2× SSC-0.1% SDS at 52°C and exposed toX-ray film with an intensifying screen at $-$ 80°C. Lengths of pucmRNA fragments were estimated by ethidium bromide staining ofBrome mosaic virus RNA ladders of 3.2, 2.9, 2.1, and 0.8 kb insize (obtained as a gift from Cheng Kao).

Primer extension analysis. Primer extension was performed as described in reference 13 with slight modifications. ³²P-end-labelled Puc1 oligonucleotide was hybridized with 125 µgof total RNA by heating for 10 min at 80°C and slowly coolingto 52°C. Samples were precipitated, resuspended in reverse transcriptasereaction buffer with 5 U of avian myeloblastosis virus-reversetranscriptase (Boehringer Mannheim), and incubated at 42°C for2 h. After transcription the samples were precipitated and resuspendedin standard denaturing gel electrophoresis buffer containing 10mM NaOH, heated to 75°C for 2 min, and separated on urea denaturing6% polyacrylamide gels. Dideoxynucleotide sequencing ladders wereprepared with the ³²P-end-labelled Puc1 oligonucleotide, using the sequencing reactionsas described above. Sequencing gels were dried and exposed tofilm with an intensifying screen at $-$ 80°C.

Gel mobility shift assays. Crude cell extracts were prepared as described by Ma et al. except that cells were lysed by sonication (30). Probes forgel mobility shift assays were prepared by PCR amplification withplasmid pRPSLH2KAN digested with EcoRI as a template (53) using5'-³²P-end-labelled oligonucleotide primers. Probe I was amplifiedwith the Puc4-PucRev3 oligonucleotide pair (Fig. 1), which amplifiesa 242-bp fragment that includes the distal pucURS. Probe II wasamplified with the PCR2-PucRev4 oligonucleotide pair (Fig. 1),which amplifies a 285-bp fragment that includes the proximal pucURS.Probe III was amplified with the Puc1-PucRev2 oligonucleotidepair (Fig. 1), which amplifies a 146-bp fragment that includesthe pucP1 promoter and 68 bp upstream of the transcriptional startsite. Cell extracts were diluted with the buffer used to preparethe extracts to a final concentration of 15 µg of protein/20 µlof reaction mix. A total of 1 µl of labelled DNA probe (2 to 4fmol, ca. 5,000 cpm) and 2 µl (1 µg/µl) of poly(dI-dC) nonspecificcompetitor DNA at a 500-fold weight excess relative to the probewere added. Reaction mixtures were then incubated at 28°C for30 min, loaded onto 4% polyacrylamide gels composed of 50 mM Tris-HCl(pH 8.3)-380 mM glycine-2 mM EDTA, and electrophoresed at 115V for 2.5 h. Gels were dried and exposed to film with an intensifyingscreen at $-$ 80°C. Retention factors (R_f) were calculated for shiftedprobes according to the following formula: distance traveled bythe shifted probe/distance traveled by the free probe.

Nucleotide sequence accession number. The sequence shown in Fig. 1 was submitted to the GenBank and EMBL databases under accession no. AF031407.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Sequencing of the pucURS. As a prelude to promoter mapping studies, we performed DNA sequence analysis of a 1,543-bp segment upstream of the pucB translationalstart codon (Fig. 1). Inspection of this sequence (Fig. 2) indicatedthe presence of (i) a potential $sigma$ ⁷⁰ promoter sequence motif spanning positions $-$ 123 to $-$ 152 relativeto the start of pucB, (ii) two palindromes centered at positions $-$ 162 and $-$ 403 that contain a consensus DNA binding sequence (TGT-N₁₂-ACA)for the aerobic repressor CrtJ, and (iii) potential integrationhost factor (IHF) binding sites centered at positions $-$ 182, $-$ 491, $-$ 504, $-$ 517, $-$ 696, and $-$ 683 that exhibit sequence similaritiesto the R. capsulatus IHF consensus sequence (46-48). The resultsbelow address several of these features.

View larger version (45K):
[in this window]
[in a new window]

FIG. 2. Features of the puc upstream regulatory region. (A) The predicted $-$ 35 and $-$ 10 regions of the pucP1 promoter are highlighted by black boxes. The transcriptional start site is identified with a thick, filled arrow. Thin, open arrows show the locations of palindromes associated with CrtJ binding. Unshaded boxes show consensus R. capsulatus IHF binding sites. (B) The pucP1 promoter region and alignments with $sigma$ ⁷⁰-type promoters. The sequence at the top of the panel represents the first 58 nucleotides upstream of the pucP1 transcriptional start site with the $-$ 10 and $-$ 35 regions boxed. Alignments with $sigma$ ⁷⁰-type promoters from purple photosynthetic bacteria as well as the E. coli consensus sequence are shown below. Asterisks indicate bases identical to those of the lacZ UV5 promoter, a cyclic AMP receptor protein-independent promoter from E. coli. Rb. cap., R. capsulatus; Rb. sph., R. sphaeroides; Rs. pal., Rhodopseudomonas palustris.

Northern blot analysis. Northern blot analysis was performed to define regions that may be transcribed with ³²P-labeled oligonucleotide primers designed to hybridize to specificregions upstream of pucB. As shown in Fig. 3A, hybridization withprimer Puc1, which is complementary to a region 46 to 67 nucleotidesupstream of the transcribed pucB start codon, hybridized to a2.4-kb mRNA segment as well as to discrete 1.4-, 1.0-, and 0.5-kbmRNA segments. Longer exposures also indicate the presence oftwo additional weak signals of approximately 3.0 and 3.4 kb insize that hybridize to the Puc1 probe (33). This supports aprevious report that the puc operon contains transcripts of varioussizes that are formed as a result of processing (23). Northernblot analysis with oligonucleotides Puc2, Puc3, and Puc4, whichwere designed to hybridize 288 to 310, 356 to 386, and 618 to637 bp upstream of the pucB gene, respectively (Fig. 1), failedto give rise to a signal (33). This indicates that initiationof puc transcription most likely occurs in the region bracketedby the Puc1 and Puc2 probes (from 46 to 310 bp upstream of pucB).

View larger version (55K):
[in this window]
[in a new window]

FIG. 3. Northern blot and primer extension analyses of the puc operon transcript using 5'-³²P-labeled Puc1 oligonucleotide as a probe. (A) Lane 1 is a control loaded with E. coli RFS859 RNA, while lane 2 contains RNA from R. capsulatus SB1003. Estimated sizes (in kilobases) of puc mRNA fragments are shown on the right. (B) High-resolution end mapping of the 5' terminus of the puc operon by primer extension analysis using 5'-³²P-labeled Puc1 oligonucleotide as a primer. Individual reactions from a DNA sequencing ladder were loaded in the first four lanes. Lane 1 contains the product of a primer extension reaction with total RNA isolated from high-light photosynthetic cells, lane 2 contains the product formed from low-light photosynthetic cells, and lane 3 contains the product from a dark-aerobic-grown culture. The arrow indicates the $-$ 116 base signal proposed as the pucP1 transcriptional start site.

Primer extension analysis. Detection of a stable mRNA 5' end in the region thought to initiate the puc transcript (based on the Northern blot results)was undertaken by performing primer extension analysis using a³²P-labeled Puc1 primer as a probe. As shown in Fig. 3B, a predominantprimer extension product located 116 bp upstream of the startof pucB was obtained with mRNA from photosynthetically grown cellsunder high-light conditions (Fig. 3B, lane 1). Primer extensionwith mRNA obtained from low-light-grown cells had higher amountsof the 116-bp product (lane 2), whereas mRNA obtained from aerobicallygrown cells had a significant reduction in the amount of the primerextension product (lane 3). This correlates well with previousstudies which indicated that transcription of the puc operon islight regulated under anaerobic conditions and repressed underaerobic growth conditions (3, 4, 11, 22, 23, 32,34, 35, 41). Primer extension with oligonucleotides thathybridize >288 bp upstream of pucB (Puc2, Puc3, and Puc4) exhibitedno primer extension signal, which supports the negative Northernblot results obtained with these oligonucleotides (33). We concludedtherefore that puc transcription is predominantly initiated froma cytosine located 116 bp upstream of pucB.

In vivo promoter probe analysis. To determine if the observed primer extension signal represents an actual transcription initiation start site rather thanan artifact of mRNA processing, various regions of the pucURSwere cloned into a promoter probe plasmid that uses lacZ as areporter of transcription activity. As shown in Fig. 4A, $beta$ -galactosidaseactivity was observed with plasmid pDN12S, which contains a 272-bpfragment 49 to 320 bp upstream of the start codon of pucB, andplasmid pDN13S, which contains a segment that overlaps that ofpDN12S as well as an additional 760 bp of upstream DNA sequence(from 49 to 1,080 bp upstream of pucB) (Fig. 4). No activity couldbe detected with plasmids pDN11S, pDN20S, pDN21S, and pDN24S,which contained segments spanning sequences from 173 to 1,341bp upstream of pucB. The in vivo activities observed with thesevectors thus localizes the initiation of puc transcription toa region between 49 and 173 bp upstream of pucB, which correspondswell with the $-$ 116 bp location of the primer extension product.

View larger version (20K):
[in this window]
[in a new window]

FIG. 4. In vivo promoter probe analysis of the puc upstream regulatory region. (A) The organization of the 5.75-kb EcoRI fragment used to clone the puc operon is shown at top (53). Below this is shown the PstI-ClaI fragment used for many subsequent subclones. The bottom of the panel shows DNA-restricted and PCR-generated fragments that were cloned into pZM400 as well as the results of transcriptional assays under photosynthetic growth conditions. +, levels of $beta$ -galactosidase activity significantly above that observed with the control reporter plasmid pZM500, which has no insert DNA; $-$ , $beta$ -galactosidase activity equal to or below that observed with the control plasmid pZM500. (B) Plasmids tested for expression are shown on the x axis, and $beta$ -galactosidase units (micromoles of ONPG hydrolyzed per minute per milligram of protein) are shown on the y axis. Results are shown for extracts prepared from dark-aerobic-grown cells (O₂), photosynthetic high-light-grown cells (HL), and photosynthetic low-light-grown cells (LL).

Regulation of promoter reporter constructs pDN12 and pDN13. Previous studies by Lee and Kaplan indicated that the puc promoter in R. sphaeroides contains regulatory elements that arelocated up to 600 bp upstream of the location of transcriptioninitiation (25, 26). Since pDN12S exhibited $beta$ -galactosidaseactivity with only 57 bp of DNA upstream of the site of transcriptioninitiation, we decided to undertake an analysis of expressionof this construct in comparison with that of plasmid pDN13S, whichcontains 964 bp of DNA upstream of the transcription start site.As shown in Fig. 4B, wild-type cells harboring either plasmidpDN12S or pDN13S exhibited similar patterns of expression underthe tested conditions. However, pDN12S had a slightly lower levelof expression than pDN13S when grown under both photosynthetichigh-light and low-light conditions. There was also a slightlyhigher level of expression of pDN12S than of pDN13S when bothconstructs were grown under aerobic growth conditions. This indicatesthat pDN12S contains many, but not all, of the critical cis-actingsites needed for regulating puc expression.

Previous studies on the effects of various regulatory mutants on puc expression were undertaken using translational fusions(23, 41). These studies indicated that puc expression is regulatedby several factors including the aerobic repressor CrtJ (8,35), the two-component anaerobic activator circuit RegB-RegA(32, 41), and IHF (27). To directly test the effects ofregulatory mutants on promoter activity we assayed pDN13S expressionin a variety of previously described regulatory mutants. As shownin Fig. 5, strains containing mutations in the response regulatorRegA, in the aerobic repressor CrtJ, and in IHF had effects ontranscription of pDN13S. Specifically, mutations that disruptIHF or RegA had an identical twofold reduction in transcriptionalactivity of pucP1 under aerobic and high-light photosyntheticgrowth conditions (Fig. 5). When grown under photosynthetic low-lightconditions the IHF mutant exhibited a 1.5-fold drop in transcriptionactivity compared to that of SB1003 (the RegA mutant is incapableof growth under low-light conditions and thus could not be usedfor comparison under this growth condition). Disruption of CrtJresulted in a reproducible, slight 1.3-fold elevation in aerobicpromoter activity and had no effect under high-light or low-lightphotosynthetic growth conditions (Fig. 5).

View larger version (18K):
[in this window]
[in a new window]

FIG. 5. Results of $beta$ -galactosidase assays with plasmid pDN13S (pucP1) in wild-type (W.T.) and regulatory mutants of R. capsulatus. Strains tested are shown on the x axis, and $beta$ -galactosidase activities (micromoles of ONPG hydrolyzed per minute per milligram of protein) are shown on the y axis. (A) Results with extracts prepared from high-light-grown cells. (B) Results with extracts prepared from low-light grown cells. (C) Results with extracts prepared from dark-aerobic-grown cells.

Gel mobility shift analysis. We also undertook in vitro gel mobility shift analysis with cell extracts to assay for the presence of transcription factorsthat may bind to the puc promoter region. As shown in Fig. 6,extracts derived from wild-type strain SB1003 retard probe I,which contains the distal upstream regulatory region from 618to 860 bp upstream of pucB, to two different R_f positions of 0.81and 0.84 (with the free probe having an R_f of 1.0) (Fig. 6B, lane2). Probe II, which contains the proximal upstream regulatoryregion from 306 to 591 bp upstream of pucB, shifts to three differentR_f positions of 0.87, 0.74, and 0.43 (Fig. 6B, lane 6). ProbeIII, which contains the pucP1 promoter region from 46 to 192 bpupstream of pucB, exhibits three shifts with R_fs of 0.80, 0.72,and 0.66 (Fig. 6B, lane 10).

View larger version (63K):
[in this window]
[in a new window]

FIG. 6. Gel mobility shift analysis of the pucP1 promoter and upstream regulatory region. (A) Probes used for gel shift analysis. See text for details. (B) Gel mobility shifts are shown immediately below the respective probe that was used for each experiment with no protein (lanes 1, 5, 9) and with cell extracts derived from SB1003 (lanes 2, 6, and 10), IR4 rif10 (IHF) (lanes 3, 7, and 11), and TB1 (RegA) (lanes 4, 8, and 12) cells. Because each of the probes were run on different gels, the R_fs observed with individual probes are independent of each other.

Extracts prepared from cultures of IR4 cells, which contain a point mutation in IHF (46, 47), exhibited shifts similarto that observed with wild-type extracts with probe I (Fig. 6B,lane 3) and a loss of several bands with probes II and III (Fig.6B, lanes 7 and 11, respectively). Extracts obtained from TB1cells, which contain a deletion of regA (7), exhibited no significanteffects on shifts observed with probe I or II. However, with probeIII, a band with 0.66 R_f was lost, the 0.72-R_f band was diminishedin intensity, and a new band was observed with an R_f of 0.75 (Fig.6B, lane 12). Extracts prepared from cultures of MW442 (whichcontain a disruption of $Delta$ LHII [40]) had no significant effecton shifts of any of the probes tested (33).

Purified IHF from R. capsulatus (obtained as a generous gift from B. Toussaint) was used to further localize IHF binding sitesthat were observed with crude extracts (46). Purified IHF at10.8 nM caused two predominant shifts with probe I (R_fs of 0.88and 0.79) (Fig. 7, lane 2), two with probe II (R_fs of 0.90 and0.82) (Fig. 7, lane 5), and one with probe III (R_f of 0.88) (Fig.7, lane 8). When incubated with 21.6 nM IHF, an additional bandwas observed with probe I (Fig. 7, lane 3) and probe III (Fig.7, lane 9). Two additional bands were observed with probe II whenincubated at the highest IHF concentration (Fig. 7, lane 6).

View larger version (69K):
[in this window]
[in a new window]

FIG. 7. Gel mobility shift analysis of the pucP1 promoter and upstream regulatory region with purified R. capsulatus IHF. (A) Probes used for gel shift analysis. (B) Gel shifts shown immediately below the respective probe used for each experiment with no protein (lanes 1, 4, and 7), 10.8 nM IHF (1X) (lanes 2, 5, and 8), and 21.6 nM IHF (2X) (lanes 3, 6, and 9).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Previous low-resolution S1 mapping studies indicated that the puc 5' mRNA terminus was located 110 to 125 bp upstream of thepucB translational start codon (23). This is in good agreementwith the results of our high-resolution in vitro primer extension(Fig. 3B) and in vivo promoter probe analyses (Fig. 4), whichdemonstrate that a single puc operon transcription start siteoccurs 116 bp upstream of the pucB translational start codon.Analysis of the pucP1 promoter region (Fig. 2B) shows that itcontains a $sigma$ ⁷⁰-type promoter consensus (TTGAtc-N₁₇-cATAgT) that has a high degreeof sequence similarity with other proposed or identified promotersfrom R. capsulatus that are involved in carotenoid and bacteriochlorophyllbiosynthesis (1, 30). Further inspection reveals strong similaritiesbetween the pucP1 $-$ 35 and $-$ 10 regions and similar regions in thecyclic AMP receptor protein-independent lacZ UV5 promoter fromE. coli, i.e., 16 of 20 nucleotides identical around the $-$ 35 regionand 11 of 14 nucleotides identical around the $-$ 10 region (seebases highlighted with asterisks in Fig. 2B). A significant differenceis that these regions are spaced 6 nucleotides closer in lacZUV5 than is the case for pucP1 (37).

Previous studies using pucB::lacZ translational fusions gave results consistent with the degree of oxygen and light regulationreported here for the transcriptional vector pDN13S (11, 41).Specifically, we observed that transcription initiated from thepucP1 promoter increases two- to threefold when cultures are grownunder low-light compared to high-light growth conditions, whichcorrelates with the effect of light intensity on synthesis ofthe LH-II complex. These results contradict the results of Zucconiand Beatty (57), who concluded that puc mRNA levels vary inverselywith LH-II protein levels with respect to changes in light intensitybased on mRNA hybridization studies. However, our own primer extension(Fig. 3B) and Northern blot (33) experiments indicate that levelsof puc mRNA are significantly greater under low-light comparedto high-light growth conditions when equal amounts of total RNAwere used. This would indicate that there is no substantial light-mediatedposttranscriptional control of puc expression.

The results of our expression analysis with reporter plasmids in different regulatory mutant backgrounds, coupled with thein vitro gel mobility shift results, provide a low-resolutionview of the complexity of the transcription factors that are responsiblefor controlling puc expression. Mutations in RegA and IHF hadsimilar 2- to 2.5-fold reductions of puc expression under photosyntheticand aerobic-dark growth conditions (Fig. 5). Gel mobility shiftpatterns demonstrated that cell extracts derived from a regA-deletedstrain affect a higher-order structure of proteins bound to aDNA segment (from 45 to 192 bp upstream of pucB) that codes forthe pucP1 promoter region (Fig. 7). Indeed, this is confirmedby recent DNase I nuclease protection experiments with purifiedRegA, which demonstrate that RegA binds to a segment spanningfrom 52 to 80 bp upstream of the start of puc transcription initiation(16).

Cell extracts derived from the IHF mutant were also altered in mobility shifts in all three DNA probes tested when comparedto that observed with extracts derived from wild-type cells (Fig.7). This indicates that there may be multiple IHF binding siteslocated from the promoter region to up to several hundred basesupstream of the transcription start site. This conclusion is supportedby our observation that purified R. capsulatus IHF shifted allthree DNA probes encompassing the pucP1 promoter region. Inspectionof the DNA sequence upstream of pucB indicates that there aremultiple copies of a related sequence motif containing ATT (AAATTGC,AGATTCG, CAATTCG, AAATTCC, and AAATTCG) that are present in theDNA segments that exhibited a gel mobility shift with purifiedIHF (Fig. 2). Variants of this sequence are also located upstreamof the R. capsulatus hip and himA genes, which code for subunitsof IHF, as well as in the hupS promoter, which requires IHF fortranscription initiation (46-48). Footprint analysis indicatesthat R. capsulatus IHF protects the variant sequence CCATTGA presentin the hupS promoter (47) as well as in the pucURS (33), whichcontains three repeats of this sequence (AAATTCG-N₆-CAATTCG-N₆-AAATTCC,shown in Fig. 2 at position $-$ 489 to $-$ 521). Our current model isthat IHF binds in the pucURS and stabilizes RegA binding whichsubsequently interacts with RNA polymerase bound at the pucP1promoter.

Sequence analysis also indicated the presence of two putative CrtJ binding sites separated by 222 bp with one site overlappingwith the pucP1 promoter (Fig. 2). Reporter plasmid expressionfrom the crtJ-disrupted strain DB469 exhibited a 1.5-fold increasein transcriptional activity in the presence of oxygen, which isconsistent with previous reports that CrtJ acts as an aerobicrepressor of puc expression (36) (Fig. 6). Recent DNA bindingstudies indicate that CrtJ binds to these two palindromes in acooperative manner, suggesting that the intervening DNA segmentbetween the palindromes is "looped out" (17).

Conclusion. This study provides the first detailed analysis of the R. capsulatus puc operon promoter. In many respects, the results ofour analyses indicate that the puc promoter region exhibits featuresthat are typical of $sigma$ ⁷⁰ type promoters. Ongoing footprint analyses in our laboratoryusing purified transcription factors are beginning to define individualcis-acting sites that are involved in binding various activatorsand repressors that control puc expression in response to alterationsin light intensity and oxygen tension (16, 36). The challengewill be in further defining the complex interactions that mustbe occurring among the transcription factors and RNA polymeraseat the puc promoter.

	ACKNOWLEDGMENTS

We thank members of the Photosynthetic Bacteria Group for stimulating discussions and especially Sylvie Elsen for carefulreading of the manuscript.

This work was supported by National Institutes of Health grants GM53940, GM40941, and GM00618 to C.E.B.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biology, Jordan Hall, Indiana University, Bloomington, IN 47405. Phone:(812) 855-6595. Fax: (812) 855-6705. E-mail: cbauer{at}bio.indiana.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Alberti, M., D. E. Burke, and J. E. Hearst. 1996. Structure and sequence of the photosynthesis gene cluster, p. 1083-1106. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.

2. Ashby, M. K., S. A. Coomber, and C. N. Hunter. 1987. Cloning, nucleotide sequence, and transfer of genes for the B800-850 light-harvesting complex of Rhodobacter sphaeroides. FEBS Lett. 213:245-248.

3. Bauer, C. E. 1995. Regulation of photosynthesis gene expression, p. 1221-1234. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.

4. Bauer, C. E., and T. H. Bird. 1993. Regulatory circuits controlling photosynthesis gene expression. Cell 85:5-8.

5. Beatty, J. T. 1995. Organization of photosynthesis gene transcripts, p. 1209-1219. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.

6. Belasco, J. G., J. T. Beatty, C. W. Adams, A. von Gabin, and S. N. Cohen. 1985. Differential expression of photosynthetic genes in Rhodopseudomonas capsulata results from segmental differences in stability within a polycistronic transcript. Cell 40:71-181[Medline].

7. Bird, T., and C. E. Bauer. Unpublished strain construction.

8. Bollivar, D. W., J. Y. Suzuki, J. T. Beatty, J. M. Dobrowolski, and C. E. Bauer. 1994. Directional mutational analysis of bacteriochlorophyll a biosynthesis in Rhodobacter capsulatus. J. Mol. Biol. 237:622-640[Medline].

9. Bradford, M. M. 1976. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Anal. Biochem. 72:248-254[Medline].

10. Braun, P., and A. Scherz. 1991. Polypeptides and bacteriochlorophyll organization in the light-harvesting complex B850 of Rb. sphaeroides R26.1. Biochemistry 30:5177-5184[Medline].

11. Buggy, J. J., M. W. Sganga, and C. E. Bauer. 1994. Characterization of a light-responding trans-activator responsible for differentially controlling reaction center and light-harvesting-I gene expression in Rhodobacter capsulatus. J. Bacteriol. 176:6936-6943[Abstract/Free Full Text].

12. Chomczynski, P., and N. Sacchi. 1987. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Anal. Biochem. 162:156-159[Medline].

13. Colman, A. 1984. Expression of exogenous DNA in Xenopus oocytes, p. 49-69. In B. D. Hames, and S. J. Higgins (ed.), Transcription and translation: a practical approach. IRL Press, Oxford, United Kingdom.

14. Ditta, G., T. Schmidhauser, E. Yakobsen, P. Lu, X. W. Liang, D. R. Finlay, D. Guiney, and D. R. Helinsky. 1985. Plasmids related to the broad host range vector, pRK290, useful for gene cloning and for monitoring gene expression. Plasmid 13:149-153[Medline].

15. Drews, G., and J. R. Golecki. 1995. Structure, molecular organization, and biosynthesis of membranes of purple bacteria, p. 231-257. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.

16. Du, S., T. H. Bird, and C. E. Bauer. 1998. DNA binding properties of RegA*. A constitutively active anaerobic activator of photosynthesis gene expression in Rhodobacter capsulatus. J. Biol. Chem. 273:18509-18513[Abstract/Free Full Text].

17. Elsen, S., S. N. Ponnampalam, and C. E. Bauer. Unpublished data.

18. Karrasch, S., P. A. Bullough, and R. Ghosh. 1995. The 8.5 Å projection map of the light-harvesting complex I from Rhodospirillum rubrum reveals a ring composed of 16 subunits. EMBO J. 14:631-638[Medline].

19. Kiley, P. J., and S. Kaplan. 1987. Cloning, DNA sequence, and expression of the Rhodobacter sphaeroides light-harvesting B800-850- $alpha$ and B800-850- $beta$ genes. J. Bacteriol. 169:3268-3275[Abstract/Free Full Text].

20. Klug, G. 1993. The role of mRNA degradation in the regulated expression of bacterial photosynthesis genes. Mol. Microbiol. 9:1-7[Medline].

21. Klug, G. 1995. Post-transcriptional control of photosynthesis gene expression, p. 1235-1244. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.

22. Klug, G., N. Kaufman, and G. Drews. 1985. Gene expression of pigment proteins of the bacterial photosynthetic apparatus: transcription and assembly in the membrane of Rhodopseudomonas capsulata. Proc. Natl. Acad. Sci. USA 82:6485-6489[Abstract/Free Full Text].

23. LeBlanc, H. N., and J. T. Beatty. 1993. Rhodobacter capsulatus puc operon: promoter location, transcript sizes and effects of deletions on photosynthetic growth. J. Gen. Microbiol. 139:101-109[Medline].

24. Lee, J. K., P. J. Kiley, and S. Kaplan. 1989. Post-transcriptional control of puc operon expression of B800-850 light-harvesting complex formation in Rhodobacter sphaeroides. J. Bacteriol. 171:3391-3405[Abstract/Free Full Text].

25. Lee, J. K., and S. Kaplan. 1992. cis-acting regulatory elements involved in oxygen and light control of puc operon transcription in Rhodobacter sphaeroides. J. Bacteriol. 174:1146-1157[Abstract/Free Full Text].

26. Lee, J. K., and S. Kaplan. 1995. Transcriptional regulation of puc operon expression in Rhodobacter sphaeroides. Analysis of the cis-acting downstream regulatory sequence. J. Biol. Chem. 270:20453-20458[Abstract/Free Full Text].

27. Lee, J. K., S. Wang, J. M. Eraso, J. Gardner, and S. Kaplan. 1995. Transcriptional regulation of puc operon expression in Rhodobacter sphaeroides. Involvement of an integration host factor-binding sequence. J. Biol. Chem. 268:24491-24497[Abstract/Free Full Text].

28. Lien, S., H. Gest, and A. San Pietro. 1973. Regulation of chlorophyll synthesis in photosynthetic bacteria. Bioenergetics 4:423-434.

29. Lindsley, J. E., and M. M. Cox. 1989. Dissociation pathway for RecA nucleoprotein filaments formed on linear duplex DNA. J. Mol. Biol. 205:695-711[Medline].

30. Ma, D., D. N. Cook, D. A. O'Brien, and J. E. Hearst. 1993. Analysis of the promoter and regulatory sequences of an oxygen-regulated bch operon in Rhodobacter capsulatus by site-directed mutagenesis. J. Bacteriol. 175:2037-2045[Abstract/Free Full Text].

31. McDermott, G., S. M. Prince, A. A. Freer, A. M. Hawthornthwaite-Lawless, M. Z. Papiz, R. J. Cogdell, and N. W. Isaacs. 1995. Crystal structure of an integral membrane light-harvesting complex from photosynthetic bacteria. Nature 374:517-521.

32. Mosley, C. S., J. Y. Suzuki, and C. E. Bauer. 1994. Identification and molecular genetic characterization of a sensor kinase responsible for coordinately regulating light harvesting and reaction center gene expression in response to anaerobiosis. J. Bacteriol. 176:7566-7573[Abstract/Free Full Text].

33. Nickens, D., and C. E. Bauer. Unpublished data.

34. Oberlé, B., H. V. Tichy, and G. Drews. 1990. Regulation of formation of photosynthetic light-harvesting complexes in Rhodobacter capsulatus, p. 77-84. In G. Drews, and E. A. Dawes (ed.), Molecular biology of membrane-bound complexes in phototrophic bacteria. Plenum Press, New York, N.Y.

35. Ponnampalam, S. N., J. J. Buggy, and C. E. Bauer. 1995. Characterization of an aerobic repressor that coordinately regulates bacteriochlorophyll, carotenoid, and light harvesting-II expression in Rhodobacter capsulatus. J. Bacteriol. 177:2990-2997[Abstract/Free Full Text].

36. Prentki, P., and H. M. Krisch. 1984. In vitro insertional mutagenesis with a selectable DNA fragment. Gene 29:303-313[Medline].

37. Reznikoff, W. S., and J. N. Abelson. 1978. The lac promoter, p. 221-243. In J. H. Miller, and W. S. Reznikoff (ed.), The operon. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

38. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

39. Schleif, R. 1972. Fine-structure deletion map of the Escherichia coli L-arabinose operon. Proc. Natl. Acad. Sci. USA 69:3479-3484[Abstract/Free Full Text].

40. Scolnik, P. A., D. Zannoni, and B. L. Marrs. 1980. Spectral and functional comparisons between the carotenoides of the two antenna complexes of Rhodopseudomonas capsulata. Biochim. Biophys. Acta 593:230-240[Medline].

41. Sganga, M. W., and C. E. Bauer. 1992. Regulatory factors controlling photosynthetic reaction center and light harvesting gene expression in Rhodobacter capsulatus. Cell 68:945-954[Medline].

42. Stover, C. K., M. H. Vodkin, and E. V. Oaks. 1987. Use of conversion adapters to clone antigen genes in $lambda$ gt11. Biochemistry 30:5177-5184.

43. Tadros, M. H., A. F. Garcia, G. Drews, N. Gad'on, and M. P. Skatchkov. 1990. Isolation and characterization of a light-harvesting complex II lacking the gamma-polypeptide from Rhodobacter capsulatus. Biochim. Biophys. Acta 1019:245-249.

44. Tichy, H. V., B. Oberlé, H. Stiehle, E. Schilitz, and G. Drews. 1989. Genes downstream from pucA are essential for the formation of the B800-850 complex of Rhodobacter capsulatus. J. Bacteriol. 171:4914-4922[Abstract/Free Full Text].

45. Tichy, H. V., K. U. Albien, N. Gad'on, and G. Drews. 1991. Analysis of the Rhodobacter capsulatus puc operon: the pucC gene plays a central role in the regulation of LHII (B800-850 complex) expression. EMBO J. 10:2949-2956[Medline].

46. Toussaint, B., C. Bosc, P. Richaud, A. Colbeau, and P. M. Vignais. 1991. A mutation in a Rhodobacter capsulatus gene encoding an integration host factor-like protein impairs in vivo hydrogenase expression. Proc. Natl. Acad. Sci. USA 69:3479-3484.

47. Toussaint, B., I. Delic-Attree, R. De Sury d'Aspremont, L. David, M. Vinçon, and P. M. Vignais. 1993. Purification of the integration host factor homolog of Rhodobacter capsulatus: cloning and sequencing of the hip gene, which encodes the $beta$ subunit. J. Bacteriol. 175:6499-6504[Abstract/Free Full Text].

48. Vignais, P. M., B. Toussaint, and A. Colbeau. 1995. Regulation of hydrogenase gene expression, p. 1175-1190. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.

49. Weaver, P. F., J. D. Wall, and H. Gest. 1975. Characterization of Rhodopseudomonas capsulata. Arch. Microbiol. 105:207-216[Medline].

50. Wellington, C. L., and J. T. Beatty. 1989. Promoter mapping and nucleotide sequence of the bchC bacteriochlorophyll biosynthesis gene from Rhodobacter capsulatus. Gene 83:251-261[Medline].

51. Yen, H.-C., and B. Marrs. 1976. Map of genes for carotenoid and bacteriochlorophyll biosynthesis in Rhodopseudomonas capsulata. J. Bacteriol. 126:619-629[Abstract/Free Full Text].

52. Young, D. A., C. E. Bauer, J. C. Williams, and B. L. Marrs. 1989. Genetic evidence for superoperonal organization of genes for photosynthetic pigments and pigment binding proteins in Rhodobacter capsulatus. J. Bacteriol. Gen. Genet. 218:1-12.

53. Youvan, D. C., and S. Ismail. 1985. Light-harvesting II (B800-85 complex) structural genes from Rhodopseudomonas capsulata. Proc. Natl. Acad. Sci. USA 82:58-62[Abstract/Free Full Text].

54. Zhu, Y. S., and J. E. Hearst. 1986. Regulation of expression of genes for light-harvesting antenna proteins LH-I and LH-II; reaction center polypeptides RC-L, RC-M, and RC-H; and enzymes of bacteriochlorophyll and carotenoid biosynthesis in Rhodobacter capsulatus by light and oxygen. Proc. Natl. Acad. Sci. USA 83:7613-7617[Abstract/Free Full Text].

55. Zhu, Y. S., D. N. Cook, F. Leach, G. A. Armstrong, M. Alberti, and J. E. Hearst. 1986. Oxygen-regulated mRNAs for light-harvesting and reaction center complexes and for bacteriochlorophyll and carotenoid biosynthesis in Rhodobacter capsulatus during the shift from anaerobic to aerobic growth. J. Bacteriol. 168:1180-1188[Abstract/Free Full Text].

56. Zuber, H., and R. J. Cogdell. 1995. Structure and organization of purple bacterial antenna complexes, p. 315-348. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.

57. Zucconi, A. P., and J. T. Beatty. 1988. Posttranscriptional regulation by light of the steady-state levels of mature B800-850 light-harvesting complexes in Rhodobacter capsulatus. J. Bacteriol. 170:877-882[Abstract/Free Full Text].

This article has been cited by other articles:

Elsen, S., Swem, L. R., Swem, D. L., Bauer, C. E. (2004). RegB/RegA, a Highly Conserved Redox-Responding Global Two-Component Regulatory System. Microbiol. Mol. Biol. Rev. 68: 263-279 [Abstract] [Full Text]
Steunou, A.-S., Ouchane, S., Reiss-Husson, F., Astier, C. (2004). Involvement of the C-Terminal Extension of the {alpha} Polypeptide and of the PucC Protein in LH2 Complex Biosynthesis in Rubrivivax gelatinosus. J. Bacteriol. 186: 3143-3152 [Abstract] [Full Text]
Dong, C., Elsen, S., Swem, L. R., Bauer, C. E. (2002). AerR, a Second Aerobic Repressor of Photosynthesis Gene Expression in Rhodobacter capsulatus. J. Bacteriol. 184: 2805-2814 [Abstract] [Full Text]
Lang, A. S., Beatty, J. T. (2000). Genetic analysis of a bacterial genetic exchange element: The gene transfer agent of Rhodobacter capsulatus. Proc. Natl. Acad. Sci. USA 97: 859-864 [Abstract] [Full Text]
LeBlanc, H., Lang, A. S., Beatty, J. T. (1999). Transcript Cleavage, Attenuation, and an Internal Promoter in the Rhodobacter capsulatus puc Operon. J. Bacteriol. 181: 4955-4960 [Abstract] [Full Text]
Ponnampalam, S. N., Elsen, S., Bauer, C. E. (1998). Aerobic Repression of the Rhodobacter capsulatus bchC Promoter Involves Cooperative Interactions between CrtJ Bound to Neighboring Palindromes. J. Biol. Chem. 273: 30757-30761 [Abstract] [Full Text]
Elsen, S., Ponnampalam, S. N., Bauer, C. E. (1998). CrtJ Bound to Distant Binding Sites Interacts Cooperatively to Aerobically Repress Photopigment Biosynthesis and Light Harvesting II Gene Expression in Rhodobacter capsulatus. J. Biol. Chem. 273: 30762-30769 [Abstract] [Full Text]
Fujita, Y., Bauer, C. E. (2000). Reconstitution of Light-independent Protochlorophyllide Reductase from Purified Bchl and BchN-BchB Subunits. IN VITRO CONFIRMATION OF NITROGENASE-LIKE FEATURES OF A BACTERIOCHLOROPHYLL BIOSYNTHESIS ENZYME. J. Biol. Chem. 275: 23583-23588 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Nickens, D. G.
	Articles by Bauer, C. E.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Nickens, D. G.
	Articles by Bauer, C. E.

Appl. Environ. Microbiol.	Infect. Immun.	Eukaryot. Cell
Mol. Cell. Biol.	J. Virol.	Microbiol. Mol. Biol. Rev.
	ALL ASM JOURNALS

1.	Alberti, M., D. E. Burke, and J. E. Hearst. 1996. Structure and sequence of the photosynthesis gene cluster, p. 1083-1106. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.
2.	Ashby, M. K., S. A. Coomber, and C. N. Hunter. 1987. Cloning, nucleotide sequence, and transfer of genes for the B800-850 light-harvesting complex of Rhodobacter sphaeroides. FEBS Lett. 213:245-248.
3.	Bauer, C. E. 1995. Regulation of photosynthesis gene expression, p. 1221-1234. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.
4.	Bauer, C. E., and T. H. Bird. 1993. Regulatory circuits controlling photosynthesis gene expression. Cell 85:5-8.
5.	Beatty, J. T. 1995. Organization of photosynthesis gene transcripts, p. 1209-1219. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.
6.	Belasco, J. G., J. T. Beatty, C. W. Adams, A. von Gabin, and S. N. Cohen. 1985. Differential expression of photosynthetic genes in Rhodopseudomonas capsulata results from segmental differences in stability within a polycistronic transcript. Cell 40:71-181[Medline].
7.	Bird, T., and C. E. Bauer. Unpublished strain construction.
8.	Bollivar, D. W., J. Y. Suzuki, J. T. Beatty, J. M. Dobrowolski, and C. E. Bauer. 1994. Directional mutational analysis of bacteriochlorophyll a biosynthesis in Rhodobacter capsulatus. J. Mol. Biol. 237:622-640[Medline].
9.	Bradford, M. M. 1976. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Anal. Biochem. 72:248-254[Medline].
10.	Braun, P., and A. Scherz. 1991. Polypeptides and bacteriochlorophyll organization in the light-harvesting complex B850 of Rb. sphaeroides R26.1. Biochemistry 30:5177-5184[Medline].
11.	Buggy, J. J., M. W. Sganga, and C. E. Bauer. 1994. Characterization of a light-responding trans-activator responsible for differentially controlling reaction center and light-harvesting-I gene expression in Rhodobacter capsulatus. J. Bacteriol. 176:6936-6943[Abstract/Free Full Text].
12.	Chomczynski, P., and N. Sacchi. 1987. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Anal. Biochem. 162:156-159[Medline].
13.	Colman, A. 1984. Expression of exogenous DNA in Xenopus oocytes, p. 49-69. In B. D. Hames, and S. J. Higgins (ed.), Transcription and translation: a practical approach. IRL Press, Oxford, United Kingdom.
14.	Ditta, G., T. Schmidhauser, E. Yakobsen, P. Lu, X. W. Liang, D. R. Finlay, D. Guiney, and D. R. Helinsky. 1985. Plasmids related to the broad host range vector, pRK290, useful for gene cloning and for monitoring gene expression. Plasmid 13:149-153[Medline].
15.	Drews, G., and J. R. Golecki. 1995. Structure, molecular organization, and biosynthesis of membranes of purple bacteria, p. 231-257. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.
16.	Du, S., T. H. Bird, and C. E. Bauer. 1998. DNA binding properties of RegA. A constitutively active anaerobic activator of photosynthesis gene expression in Rhodobacter capsulatus. J. Biol. Chem. 273*:18509-18513[Abstract/Free Full Text].
17.	Elsen, S., S. N. Ponnampalam, and C. E. Bauer. Unpublished data.
18.	Karrasch, S., P. A. Bullough, and R. Ghosh. 1995. The 8.5 Å projection map of the light-harvesting complex I from Rhodospirillum rubrum reveals a ring composed of 16 subunits. EMBO J. 14:631-638[Medline].
19.	Kiley, P. J., and S. Kaplan. 1987. Cloning, DNA sequence, and expression of the Rhodobacter sphaeroides light-harvesting B800-850- $alpha$ and B800-850- $beta$ genes. J. Bacteriol. 169:3268-3275[Abstract/Free Full Text].
20.	Klug, G. 1993. The role of mRNA degradation in the regulated expression of bacterial photosynthesis genes. Mol. Microbiol. 9:1-7[Medline].
21.	Klug, G. 1995. Post-transcriptional control of photosynthesis gene expression, p. 1235-1244. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.
22.	Klug, G., N. Kaufman, and G. Drews. 1985. Gene expression of pigment proteins of the bacterial photosynthetic apparatus: transcription and assembly in the membrane of Rhodopseudomonas capsulata. Proc. Natl. Acad. Sci. USA 82:6485-6489[Abstract/Free Full Text].
23.	LeBlanc, H. N., and J. T. Beatty. 1993. Rhodobacter capsulatus puc operon: promoter location, transcript sizes and effects of deletions on photosynthetic growth. J. Gen. Microbiol. 139:101-109[Medline].
24.	Lee, J. K., P. J. Kiley, and S. Kaplan. 1989. Post-transcriptional control of puc operon expression of B800-850 light-harvesting complex formation in Rhodobacter sphaeroides. J. Bacteriol. 171:3391-3405[Abstract/Free Full Text].
25.	Lee, J. K., and S. Kaplan. 1992. cis-acting regulatory elements involved in oxygen and light control of puc operon transcription in Rhodobacter sphaeroides. J. Bacteriol. 174:1146-1157[Abstract/Free Full Text].
26.	Lee, J. K., and S. Kaplan. 1995. Transcriptional regulation of puc operon expression in Rhodobacter sphaeroides. Analysis of the cis-acting downstream regulatory sequence. J. Biol. Chem. 270:20453-20458[Abstract/Free Full Text].
27.	Lee, J. K., S. Wang, J. M. Eraso, J. Gardner, and S. Kaplan. 1995. Transcriptional regulation of puc operon expression in Rhodobacter sphaeroides. Involvement of an integration host factor-binding sequence. J. Biol. Chem. 268:24491-24497[Abstract/Free Full Text].
28.	Lien, S., H. Gest, and A. San Pietro. 1973. Regulation of chlorophyll synthesis in photosynthetic bacteria. Bioenergetics 4:423-434.
29.	Lindsley, J. E., and M. M. Cox. 1989. Dissociation pathway for RecA nucleoprotein filaments formed on linear duplex DNA. J. Mol. Biol. 205:695-711[Medline].
30.	Ma, D., D. N. Cook, D. A. O'Brien, and J. E. Hearst. 1993. Analysis of the promoter and regulatory sequences of an oxygen-regulated bch operon in Rhodobacter capsulatus by site-directed mutagenesis. J. Bacteriol. 175:2037-2045[Abstract/Free Full Text].
31.	McDermott, G., S. M. Prince, A. A. Freer, A. M. Hawthornthwaite-Lawless, M. Z. Papiz, R. J. Cogdell, and N. W. Isaacs. 1995. Crystal structure of an integral membrane light-harvesting complex from photosynthetic bacteria. Nature 374:517-521.
32.	Mosley, C. S., J. Y. Suzuki, and C. E. Bauer. 1994. Identification and molecular genetic characterization of a sensor kinase responsible for coordinately regulating light harvesting and reaction center gene expression in response to anaerobiosis. J. Bacteriol. 176:7566-7573[Abstract/Free Full Text].
33.	Nickens, D., and C. E. Bauer. Unpublished data.
34.	Oberlé, B., H. V. Tichy, and G. Drews. 1990. Regulation of formation of photosynthetic light-harvesting complexes in Rhodobacter capsulatus, p. 77-84. In G. Drews, and E. A. Dawes (ed.), Molecular biology of membrane-bound complexes in phototrophic bacteria. Plenum Press, New York, N.Y.
35.	Ponnampalam, S. N., J. J. Buggy, and C. E. Bauer. 1995. Characterization of an aerobic repressor that coordinately regulates bacteriochlorophyll, carotenoid, and light harvesting-II expression in Rhodobacter capsulatus. J. Bacteriol. 177:2990-2997[Abstract/Free Full Text].
36.	Prentki, P., and H. M. Krisch. 1984. In vitro insertional mutagenesis with a selectable DNA fragment. Gene 29:303-313[Medline].
37.	Reznikoff, W. S., and J. N. Abelson. 1978. The lac promoter, p. 221-243. In J. H. Miller, and W. S. Reznikoff (ed.), The operon. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
38.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
39.	Schleif, R. 1972. Fine-structure deletion map of the Escherichia coli L-arabinose operon. Proc. Natl. Acad. Sci. USA 69:3479-3484[Abstract/Free Full Text].
40.	Scolnik, P. A., D. Zannoni, and B. L. Marrs. 1980. Spectral and functional comparisons between the carotenoides of the two antenna complexes of Rhodopseudomonas capsulata. Biochim. Biophys. Acta 593:230-240[Medline].
41.	Sganga, M. W., and C. E. Bauer. 1992. Regulatory factors controlling photosynthetic reaction center and light harvesting gene expression in Rhodobacter capsulatus. Cell 68:945-954[Medline].
42.	Stover, C. K., M. H. Vodkin, and E. V. Oaks. 1987. Use of conversion adapters to clone antigen genes in $lambda$ gt11. Biochemistry 30:5177-5184.
43.	Tadros, M. H., A. F. Garcia, G. Drews, N. Gad'on, and M. P. Skatchkov. 1990. Isolation and characterization of a light-harvesting complex II lacking the gamma-polypeptide from Rhodobacter capsulatus. Biochim. Biophys. Acta 1019:245-249.
44.	Tichy, H. V., B. Oberlé, H. Stiehle, E. Schilitz, and G. Drews. 1989. Genes downstream from pucA are essential for the formation of the B800-850 complex of Rhodobacter capsulatus. J. Bacteriol. 171:4914-4922[Abstract/Free Full Text].
45.	Tichy, H. V., K. U. Albien, N. Gad'on, and G. Drews. 1991. Analysis of the Rhodobacter capsulatus puc operon: the pucC gene plays a central role in the regulation of LHII (B800-850 complex) expression. EMBO J. 10:2949-2956[Medline].
46.	Toussaint, B., C. Bosc, P. Richaud, A. Colbeau, and P. M. Vignais. 1991. A mutation in a Rhodobacter capsulatus gene encoding an integration host factor-like protein impairs in vivo hydrogenase expression. Proc. Natl. Acad. Sci. USA 69:3479-3484.
47.	Toussaint, B., I. Delic-Attree, R. De Sury d'Aspremont, L. David, M. Vinçon, and P. M. Vignais. 1993. Purification of the integration host factor homolog of Rhodobacter capsulatus: cloning and sequencing of the hip gene, which encodes the $beta$ subunit. J. Bacteriol. 175:6499-6504[Abstract/Free Full Text].
48.	Vignais, P. M., B. Toussaint, and A. Colbeau. 1995. Regulation of hydrogenase gene expression, p. 1175-1190. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.
49.	Weaver, P. F., J. D. Wall, and H. Gest. 1975. Characterization of Rhodopseudomonas capsulata. Arch. Microbiol. 105:207-216[Medline].
50.	Wellington, C. L., and J. T. Beatty. 1989. Promoter mapping and nucleotide sequence of the bchC bacteriochlorophyll biosynthesis gene from Rhodobacter capsulatus. Gene 83:251-261[Medline].
51.	Yen, H.-C., and B. Marrs. 1976. Map of genes for carotenoid and bacteriochlorophyll biosynthesis in Rhodopseudomonas capsulata. J. Bacteriol. 126:619-629[Abstract/Free Full Text].
52.	Young, D. A., C. E. Bauer, J. C. Williams, and B. L. Marrs. 1989. Genetic evidence for superoperonal organization of genes for photosynthetic pigments and pigment binding proteins in Rhodobacter capsulatus. J. Bacteriol. Gen. Genet. 218:1-12.
53.	Youvan, D. C., and S. Ismail. 1985. Light-harvesting II (B800-85 complex) structural genes from Rhodopseudomonas capsulata. Proc. Natl. Acad. Sci. USA 82:58-62[Abstract/Free Full Text].
54.	Zhu, Y. S., and J. E. Hearst. 1986. Regulation of expression of genes for light-harvesting antenna proteins LH-I and LH-II; reaction center polypeptides RC-L, RC-M, and RC-H; and enzymes of bacteriochlorophyll and carotenoid biosynthesis in Rhodobacter capsulatus by light and oxygen. Proc. Natl. Acad. Sci. USA 83:7613-7617[Abstract/Free Full Text].
55.	Zhu, Y. S., D. N. Cook, F. Leach, G. A. Armstrong, M. Alberti, and J. E. Hearst. 1986. Oxygen-regulated mRNAs for light-harvesting and reaction center complexes and for bacteriochlorophyll and carotenoid biosynthesis in Rhodobacter capsulatus during the shift from anaerobic to aerobic growth. J. Bacteriol. 168:1180-1188[Abstract/Free Full Text].
56.	Zuber, H., and R. J. Cogdell. 1995. Structure and organization of purple bacterial antenna complexes, p. 315-348. In R. E. Blankenship, M. T. Madigan, and C. E. Bauer (ed.), Anoxygenic photosynthetic bacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.
57.	Zucconi, A. P., and J. T. Beatty. 1988. Posttranscriptional regulation by light of the steady-state levels of mature B800-850 light-harvesting complexes in Rhodobacter capsulatus. J. Bacteriol. 170:877-882[Abstract/Free Full Text].