Transcriptional Analysis and Mutation of a dnaA-Like Gene in Synechocystis sp. Strain PCC 6803

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Journal of Bacteriology, September 1998, p. 4946-4949, Vol. 180, No. 18
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Transcriptional Analysis and Mutation of a dnaA-Like Gene in Synechocystis sp. Strain PCC 6803

Stefan Richter,¹^, Martin Hagemann,² and Walter Messer¹^,^*

Max-Planck-Institut für molekulare Genetik, D-14195 Berlin,¹ and Fachbereich Biologie, Universität Rostock, D-18051 Rostock,² Germany

Received 14 May 1998/Accepted 17 July 1998

	ABSTRACT

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Transcription of the dnaA gene of the cyanobacterium Synechocystis sp. strain PCC 6803 is light dependent and yields a monocistronicmRNA, as determined by Northern analysis. Surprisingly, mutantswith inactivated dnaA were viable. In batch cultures under standardconditions, the mutants grew like the wild type and did not showan aberrant phenotype. We conclude that, unlike the situationin other bacteria, dnaA of Synechocystis sp. cannot have an essentialfunction, such as initiation of DNA replication.

	TEXT

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Cyanobacteria are photosynthetic microorganisms with a light-dependent cell cycle. Cell division and initiation of DNA replicationare blocked when an exponentially growing culture is transferredto the dark (2, 3, 11). Culture growth starts immediatelyupon a return to light. Molecular mechanisms that activate orrepress the cell cycle under light or dark conditions are unknown.

In Escherichia coli, under a variety of growth conditions, DNA replication and cell division are coordinated. The initiationof DNA replication occurs simultaneously at all chromosomal origins,oriC, and the initiation frequency is correlated with the growthrate. One protein, DnaA, initializes chromosomal replication byspecific binding to conserved nonamer sequences, DnaA boxes, whichare organized as a cluster at oriC. Subsequently, DnaA promoteslocal DNA unwinding at oriC and organizes assembly of the replisome(for a review, see reference 12). DnaA is thought to be involvedin the timing of replication initiation (6), is subject toan autoregulation mechanism (12), and operates in concert withother proteins that may modulate the initiation frequency (7).

The dnaA gene is highly conserved among eubacteria and was found to be present in cyanobacteria as well (15, 16), e.g.,the identity between the deduced DnaA amino acid sequences ofE. coli and the cyanobacterium Synechocystis sp. strain PCC 6803is 38.8%. It is assumed that DnaA functions as an initiator proteinin all eubacteria (21). The assumption is supported for cyanobacteriaby demonstration of specific binding of two cyanobacterial DnaAproteins to isolated oriC fragments from E. coli and Bacillussubtilis in an in vitro binding assay (15). Functional analysisof the dnaA gene of a cyanobacterium, Synechocystis sp., mightbe helpful to elucidate the light-dependent regulation of replicationinitiation in cyanobacteria. However, a potential target sequenceof DnaA, a DnaA box cluster with properties of a chromosomal origin,has not been isolated from Synechocystis sp. and is not evidentfrom the complete nucleotide sequence (8).

In this study, examination of dnaA mRNA levels in light- and dark-incubated cells of Synechocystis sp. demonstrates light-dependenttranscription of the gene. However, analysis of dnaA mutants revealedthat the gene is not essential for growth under standard conditions.

Synechocystis sp. strain PCC 6803 was used in all experiments and cultured on agar plates or in batch cultures as describedpreviously (5). E. coli TG1 (17) was used for routine DNAmanipulations and cultured in Luria broth at 37°C. The plasmidsused in this work are listed in Table 1.

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TABLE 1. Plasmids used in this study

Transcription of dnaA and the adjacent genes in Synechocystis sp. cells cultured under light and dark conditions. The dnaA gene and the adjacent reading frames have the same transcriptional orientation (16). Upstream of dnaA, there isan open reading frame, orf134, with an unknown function. The psbDCoperon, which encodes photosystem II reaction center proteinsD2 and CP43, lies downstream of dnaA. Transcription of dnaA wasstudied under light and dark conditions and compared with thetranscription of adjacent genes.

An exponentially growing culture was transferred to the dark, and after 12 h, the cells were incubated under standard conditionswith light. RNA of Synechocystis sp. cells was isolated as describedpreviously (5). RNA samples were separated, and the relativecontent of 16S rRNA (size, 1.5 kb; see Fig. 1A) of each samplewas quantified and used as the internal standard. RNA was transferredfrom gels onto nylon membranes (Hybond-N; Amersham) and hybridizedwith ³²P-labeled antisense transcripts which were synthesized by in vitrotranscription in accordance with the manufacturer's protocols(MAXIscript kit; Ambion). Different DNA templates for in vitrotranscription were generated as PCR fragments of coding regions(Synechocystis sp. genome sequence, http://www.kazusa.or.jp/cyano/cyano.html;full-length dnaA, nucleotide positions 1,351,579 to 1,350,236;5'-end of dnaA, 1,351,579 to 1,351,179; 3'-end of dnaA, 1,350,648to 1,350,236; orf134, 1,352,030 to 1,351,634; partial psbC sequence,1,348,463 to 1,347,474) with an appended T7 phage promoter whichwas introduced by the antisense primers containing a 23-base T7promoter sequence at the 5' end (19). In vitro transcriptioncontrols were checked by electrophoresis. Relative content ofin vitro transcripts was quantified by using ImageQuant software(Molecular Dynamics) and normalized to a standard length of 1kb. Based on the normalized values, one specific factor for eachin vitro antisense transcript was calculated to equalize the slightlydifferent yields observed in control reactions. The specific factorswere used to standardize signals detected by ³²P-labeled antisense transcripts on dot blots or Northern blots.Labeling reactions and hybridizations were done simultaneouslyto allow direct comparisons.

Transcripts of dnaA, orf134, and psbDC were barely detectable after 12 h in the dark. They were strongly induced by lightand reached steady-state levels after 4 h. Changes of transcriptlevels were less than 20% between h 4 and h 12 of the light period(Fig. 1A).

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FIG. 1. Northern analysis of dnaA, orf134, and psbDC from Synechocystis sp. under light and dark conditions. Samples for RNA isolation were collected at the end of a 12-h dark period and at 2-h intervals during a following 12-h light period. (A) RNA is a negative image of total RNA stained with SYBRgreen; sizes of rRNA fragments are indicated (14). dnaA, orf134, and psbC are images of Northern blots with total RNA of the samples that were probed by ³²P-labeled antisense transcripts of dnaA, orf134, and psbC. Arrowheads indicate the locations of full-length transcripts. Images were generated by ImageQuant software. (B) Comparison of the relative mRNA levels from dot blots in which total RNA of a 6-h light sample was hybridized by dnaA, orf134, and psbC antisense transcripts.

The proximity of orf134 and dnaA suggested transcription of a dicistronic mRNA (16). However, only monocistronic transcriptswere detected with either the dnaA-specific or the orf134-specificprobe. The transcript which hybridized with the dnaA probe wasfound to be very unstable (Fig. 1A). The largest transcripts detectedby the probe were estimated to be 1.6 kb, which corresponds tothe predicted size of a monocistronic message. In another experiment,total RNA was probed by using a 5'- and a 3'-end antisense transcriptof dnaA. A ratio of 4:1 was found for the relative signal intensitiesof the 5' probe compared to the 3' probe, suggesting that degradationoccurs mainly from the 3' end (data not shown). In the light-darkexperiment, the orf134 probe hybridized with a 0.4-kb transcriptwhich did not show detectable degradation products and whose levelwas about 100-fold higher than the dnaA transcript level (Fig.1B). The psbC probe detected a 2.5-kb transcript of the psbDCoperon and a smaller monocistronic psbC transcript (Fig. 1B).About 10% of the transcripts detected by the psbC probe were monocistronic.The level of all psbC transcripts is about 1,000-fold higher thanthe dnaA transcript level. The transcriptional structure of psbDCwas described previously (22).

The Northern analysis demonstrates that in Synechocystis sp. cells, transcription of dnaA and adjacent genes is light dependent.Under standard conditions, dnaA mRNA was present, albeit at alow level compared with the other two transcripts. The dnaA transcriptwas completely absent after a 12-h dark period. Furthermore, onlya monocistronic transcript could be detected which seems to bequickly degraded, starting from its 3' end.

Construction and characterization of a dnaA knockout mutant of Synechocystis sp. strain PCC 6803. If DnaA has an essential function in Synechocystis sp., a knockout mutant of the dnaA gene should not be viable. To test thisassumption, we undertook an experiment to replace part of thednaA gene with a kanamycin resistance (Km^r) cassette. Plasmid pSYN411 (Table 1), containing a 3.5-kb fragmentencoding Synechocystis sp. DnaA, was digested by Eco47III andEcoRV to generate blunt ends and to cut out a fragment codingfor an essential part of DnaA (Fig. 2A). The fragment was replacedby ligation of a Km^r cassette isolated from a HincII digest of pUC4K (Table 1). Constructswith both orientations of the Km^r insert, i.e., Km^r encoded on the strand complementary to dnaA (pSYNK $-$ ; Table 1)and Km^r encoded on the same strand as dnaA (pSYNK+; Table 1), were obtained.Transformation into Synechocystis sp. and selection of Km^r clones were carried out as described previously (5). To oursurprise, Km^r clones were easily obtainable. Selected clones were transferredinto medium with kanamycin and cultured for several generationsto complete segregation of wild-type dnaA.

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FIG. 2. Physical map and Southern analysis of a dnaA knockout mutant of Synechocystis sp. (A) Restriction map of the dnaA region and the Km^r cassette (aph gene) insertion site. dnaA is a dark gray box, aph is a light gray box, and orf134 (upstream of dnaA) is a blank box. The fragment which is replaced in the mutant is shown as a blank box with dotted borders. Fragments used as probes in Southern analysis are represented by bars with the same shading. (B) Southern analysis of the dnaA region. Southern blots with cleaved chromosomal DNAs from the wild type and the mutant were hybridized with the following probes: full-length dnaA fragment, internal dnaA fragment and Km^r cassette. Lanes: 1 to 4, wild-type DNA cleaved with HindIII (lane 1), HindIII/EcoRV (lane 2), HindIII/XbaI (lane 3), or XbaI (lane 4); 5 to 8, mutant DNA cleaved with HindIII (lane 5), HindIII/EcoRV (lane 6), HindIII/XbaI (lane 7), or XbaI (lane 8). M, digoxigenin-labeled DNA molecular weight marker III (Boehringer). Fragment (frag.) sizes in kilobases are indicated on the left.

Ten clones, five with each orientation (clones K1 $-$ to K5 $-$ and K1+ to K5+, respectively), were examined by Southern analysis.DNA templates for synthesis of specific probes were generatedby digestion of plasmids pSYN411 (Table 1) and pUC4K (Table 1)with appropriate restriction enzymes, followed by DNA fragmentisolation. Synthesis of digoxigenin-labeled DNA probes, Southerntransfer, and hybridization were performed in accordance withthe manufacturer's instructions (nonradioactive DNA labeling anddetection kit; Boehringer, Mannheim) and standard protocols (17).The result for one clone, K1 $-$ , which was analyzed and comparedwith the wild type, is shown in Fig. 2B. A probe covering thednaA coding region detected only a 5.2-kb band in HindIII-digestedwild-type DNA. The Km^r cassette has an internal HindIII site which resulted in two fragments(2.6 and 3.4 kb) detected by the dnaA probe in the HindIII-digestedmutant DNA (Fig. 2B). Another probe made from the internal dnaAfragment, which was replaced by the Km^r cassette in the pSYNK $-$ and pSYNK+ constructs, did not show anysignal with different digests of mutant DNA (Fig. 2B). The correctchromosomal integration of the Km^r cassette was finally confirmed by the signals detected afterprobing of digested mutant DNA with the labeled Km^r fragment (Fig. 2B). In all of the other mutants tested, we foundreplacement of the internal dnaA fragment by the Km^r cassette as well (data not shown).

In a culturing experiment done under standard conditions, the growth of the wild-type strain was compared with that of someselected mutants. No significant differences between the mutantstrains and the wild type were found. The average growth rates(± the standard deviations) of wild-type Synechocystis sp. anddnaA mutants K1 $-$ (dnaA::aph) and K5+ (dnaA::aph) were 0.0167 ±0.0024, 0.0165 ± 0.0017, and 0.0169 ± 0.0016 h¹, respectively. (Clones K1 $-$ and K5+ show different transcriptionalorientations of the aph gene relative to dnaA. Batch cultureswere incubated under standard conditions. These data were calculatedfrom three independent measurements of optical density at 750nm.) The mutagenesis experiment clearly demonstrates that dnaAis not essential for the viability of Synechocystis sp. cellsunder standard conditions.

Conclusions. Molecular components which are involved in a light-regulated signal pathway that activate or repress the cell cycle in cyanobacteriaare not known. The dnaA-like gene recently found in the cyanobacteriumSynechocystis sp. could be a target of such a signal pathway.

We studied dnaA transcription under light and dark conditions in Synechocystis sp. cells and mutagenized the gene. Transcriptsof dnaA and adjacent genes, orf134 and psbDC, were almost absentafter a 12-h dark period and were strongly induced by light. Similarresults were obtained previously by examination of transcriptlevels of several photosynthetic genes in Synechocystis sp. cellsunder light and dark conditions (13). Here we show that themRNA of a nonphotosynthetic gene, dnaA, behaves like photosynthetictranscripts. orf134 is probably a nonphotosynthetic gene as well,since similar open reading frames were found in the heterotrophicorganisms E. coli (4) and Mycobacterium tuberculosis (GenBankaccession no. Z77163). In another study, the amount of mRNAof the dnaK gene encoding a chaperone was found to be relativelylarge in Synechocystis sp. cells after a 12-h dark period (1).Comparison of this result with our data suggests that mRNA stabilityin Synechocystis sp. cells is transcript specific under darkness.

Surprisingly, our mutagenesis analysis revealed that Synechocystis sp. cells are viable without a functional dnaA gene. ThednaA mutants examined grew like the wild type and did not showan aberrant phenotype on agar plates or in batch cultures. InE. coli, the dnaA gene was originally defined by isolation oftemperature-sensitive mutants blocked in the initiation of DNAreplication at 42°C (10). The dnaA gene cannot be knocked outdirectly in this organism. There are two ways to explain our observation;either (i) Synechocystis sp. has at least two modes of replication,a DnaA-dependent one and a DnaA-independent one which is activein the mutant, or (ii) Synechocystis sp., unlike E. coli, hasonly DnaA-independent replication. In E. coli, there are two othermodes of DNA replication that circumvent the DnaA requirementunder certain conditions (for a review, see reference 9). Onemode, inducible stable DNA replication, is induced under circumstancesthat activate an SOS response. The other mode, constitutive stableDNA replication, takes place in mutants of the rnhA gene encodingRNase HI with specificity for RNA in RNA-DNA hybrids. It is conceivablethat Synechocystis sp. also possesses DnaA-independent replicationthat allows some growth under unfavorable conditions and whichwas activated in the dnaA mutants, whereas in the wild type, theDnaA-dependent replication is normally active under optimizedgrowth conditions. One would expect that the growth of such dnaAmutants is impaired under optimized conditions. However, Synechocystissp. dnaA mutants behaved like the wild type, suggesting that thisdnaA-like gene does not have an essential function like initiationof replication. In addition, DnaA amino acid sequences of differentspecies (including Synechocystis sp.) used in a basic local alignmentsearch tool search did not match another open reading frame fromSynechocystis sp. that exhibits the homology pattern typicallyfound for DnaA proteins. Furthermore, there is no indication fora DnaA-dependent oriC in Synechocystis sp. which is characterizedby a DnaA box cluster(s) with adjacent AT-rich regions. A searchof the DNA sequence of the entire Synechocystis genome (8)did not reveal DnaA box clusters. This negative finding is supportedby our unsuccessful attempts to isolate potential oriC fragmentsfrom chromosomal DNA of Synechocystis sp. by using the DNA-bindingdomain of authentic DnaA in an in vitro assay described previously(15, 16a). Thus, Synechocystis sp. is the only eubacteriumknown that carries a nonessential dnaA-like gene. The mechanismof initiation of DNA replication in Synechocystis sp. remainsto be elucidated. However, characterization of Synechocystis sp.DnaA as a specific DNA-binding protein (15) and its light-dependentexpression suggest that this protein could have another functionwhich is important under certain conditions. Statistical analysisof the entire genome of Synechocystis sp. revealed a relativelyhigh frequency of some DnaA boxes; e.g., a total of 36 copiesof the nonamer sequence 5'-TTATCCACA-3', which is characterizedas an efficient DnaA box (18), were found to be present, whereasan average of 13.6 copies of a nonamer would occur on a randomsequence with the same length as the Synechocystis genome. Nonrandomoccurrence of some DnaA boxes suggests the involvement of DnaAin regulatory processes.

	FOOTNOTES

^* Corresponding author. Mailing address: Max-Planck-Institut für molekulare Genetik, Ihnestr. 73, D-14195 Berlin, Germany.Phone: 49-30-8413-1266. Fax: 49-30-8413-1385. E-mail: messer{at}mpimg-berlin-dahlem.mpg.de.

Present address: Department of Molecular Genetics and Cell Biology, University of Chicago, Chicago, IL 60637.

REFERENCES

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Abstract
Text
References

1. Aoki, S., T. Kondo, and M. Ishiura. 1995. Circadian expression of the dnaK gene in the cyanobacterium Synechocystis sp. strain PCC 6803. J. Bacteriol. 177:5606-5611[Abstract/Free Full Text].

2. Armbrust, E. V., J. D. Bowen, R. J. Olson, and S. W. Chisholm. 1989. Effect of light on the cell cycle of a marine Synechococcus strain. Appl. Environ. Microbiol. 55:425-432[Abstract/Free Full Text].

3. Binder, B. J., and S. W. Chisholm. 1990. Relationship between DNA cycle and growth rate in Synechococcus sp. strain PCC 6301. J. Bacteriol. 172:2313-2319[Abstract/Free Full Text].

4. Burland, V., G. Plunkett III, D. L. Daniels, and F. R. Blattner. 1993. DNA sequence and analysis of 136 kilobases of the Escherichia coli genome: organizational symmetry around the origin of replication. Genomics 16:551-561[Medline].

5. Hagemann, M., S. Richter, and S. Mikkat. 1997. The ggtA gene encodes a subunit of the transport system for the osmoprotective compound glucosylglycerol in Synechocystis sp. strain PCC 6803. J. Bacteriol. 179:714-720[Abstract/Free Full Text].

6. Hansen, F. G., B. B. Christensen, and T. Atlung. 1991. The initiator titration model: computer simulation of chromosome and minichromosome control. Res. Microbiol. 142:161-167[Medline].

7. Herrick, J., M. Kohiyama, T. Atlung, and F. G. Hansen. 1996. The initiation mess? Mol. Microbiol. 19:659-666[Medline].

8. Kaneko, T., S. Sato, H. Kotani, A. Tanaka, E. Asamizu, Y. Nakamura, N. Miyajima, M. Hirosawa, M. Sugiura, S. Sasamoto, T. Kimura, T. Hosouchi, A. Matsuno, A. Muraki, N. Nakazaki, K. Naruo, S. Okumura, S. Shimpo, C. Takeuchi, T. Wada, A. Watanabe, M. Yamada, M. Yasuda, and S. Tabata. 1996. Sequence analysis of the genome of the unicellular cyanobacterium Synechocystis sp. strain PCC 6803. II. Sequence determination of the entire genome and assignment of potential protein-coding regions. DNA Res. 3:109-136[Abstract].

9. Kogoma, T. 1997. Stable replication: interplay between DNA replication, homologous recombination, and transcription. Microbiol. Mol. Biol. Rev. 61:212-238[Abstract].

10. Kohiyama, M., D. Cousin, A. Ryter, and F. Jacob. 1966. Mutants thermosensibles d'E. coli K-12. Isolement et characterisation rapide. Ann. Inst. Pasteur 110:465-486[Medline].

11. Marino, G. T., and Y. Asato. 1986. Characterization of cell cycle events in the dark in Anacystis nidulans. J. Gen. Microbiol. 132:2123-2127.

12. Messer, W., and C. Weigel. 1996. Initiation of chromosome replication, p. 1579-1601. In F. C. Neidhardt, R. Curtiss III, J. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. S. Reznikoff, M. Riley, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology. American Society for Microbiology, Washington, D.C.

13. Mohamed, A., and C. Jansson. 1989. Influence of light on accumulation of photosynthesis-specific transcripts in the cyanobacterium Synechocystis 6803. Plant Mol. Biol. 13:693-700[Medline].

14. Reddy, K. J., R. Webb, and L. A. Sherman. 1990. Bacterial RNA isolation with one hour centrifugation in a table-top ultracentrifuge. BioTechniques 8:250-251[Medline].

15. Richter, S., W. R. Hess, M. Krause, and W. Messer. 1998. Unique organization of the dnaA region from Prochlorococcus marinus CCMP1375, a marine cyanobacterium. Mol. Gen. Genet. 257:534-541[Medline].

16. Richter, S., and W. Messer. 1995. Genetic structure of the dnaA region of the cyanobacterium Synechocystis sp. strain PCC 6803. J. Bacteriol. 177:4245-4251[Abstract/Free Full Text].

16a. Richter, S., and W. Messer. Unpublished data.

17. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

18. Schaper, S., and W. Messer. 1995. Interaction of the initiator protein DnaA of Escherichia coli with its DNA target. J. Biol. Chem. 270:17622-17626[Abstract/Free Full Text].

19. Stoflet, E. S., D. D. Koeberl, G. Sakar, and S. S. Sommer. 1988. Genomic amplification with transcript sequencing. Science 239:491-494[Abstract/Free Full Text].

20. Vieira, J., and J. Messing. 1982. The pUC plasmids, an M13mp7-derived system for insertion mutagenesis and sequencing with synthetic universal primers. Gene 19:259-268[Medline].

21. Yoshikawa, H., and N. Ogasawara. 1991. Structure and function of DnaA and the DnaA-box in eubacteria: evolutionary relationships of bacterial replication origins. Mol. Microbiol. 5:2589-2597[Medline].

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1.	Aoki, S., T. Kondo, and M. Ishiura. 1995. Circadian expression of the dnaK gene in the cyanobacterium Synechocystis sp. strain PCC 6803. J. Bacteriol. 177:5606-5611[Abstract/Free Full Text].
2.	Armbrust, E. V., J. D. Bowen, R. J. Olson, and S. W. Chisholm. 1989. Effect of light on the cell cycle of a marine Synechococcus strain. Appl. Environ. Microbiol. 55:425-432[Abstract/Free Full Text].
3.	Binder, B. J., and S. W. Chisholm. 1990. Relationship between DNA cycle and growth rate in Synechococcus sp. strain PCC 6301. J. Bacteriol. 172:2313-2319[Abstract/Free Full Text].
4.	Burland, V., G. Plunkett III, D. L. Daniels, and F. R. Blattner. 1993. DNA sequence and analysis of 136 kilobases of the Escherichia coli genome: organizational symmetry around the origin of replication. Genomics 16:551-561[Medline].
5.	Hagemann, M., S. Richter, and S. Mikkat. 1997. The ggtA gene encodes a subunit of the transport system for the osmoprotective compound glucosylglycerol in Synechocystis sp. strain PCC 6803. J. Bacteriol. 179:714-720[Abstract/Free Full Text].
6.	Hansen, F. G., B. B. Christensen, and T. Atlung. 1991. The initiator titration model: computer simulation of chromosome and minichromosome control. Res. Microbiol. 142:161-167[Medline].
7.	Herrick, J., M. Kohiyama, T. Atlung, and F. G. Hansen. 1996. The initiation mess? Mol. Microbiol. 19:659-666[Medline].
8.	Kaneko, T., S. Sato, H. Kotani, A. Tanaka, E. Asamizu, Y. Nakamura, N. Miyajima, M. Hirosawa, M. Sugiura, S. Sasamoto, T. Kimura, T. Hosouchi, A. Matsuno, A. Muraki, N. Nakazaki, K. Naruo, S. Okumura, S. Shimpo, C. Takeuchi, T. Wada, A. Watanabe, M. Yamada, M. Yasuda, and S. Tabata. 1996. Sequence analysis of the genome of the unicellular cyanobacterium Synechocystis sp. strain PCC 6803. II. Sequence determination of the entire genome and assignment of potential protein-coding regions. DNA Res. 3:109-136[Abstract].
9.	Kogoma, T. 1997. Stable replication: interplay between DNA replication, homologous recombination, and transcription. Microbiol. Mol. Biol. Rev. 61:212-238[Abstract].
10.	Kohiyama, M., D. Cousin, A. Ryter, and F. Jacob. 1966. Mutants thermosensibles d'E. coli K-12. Isolement et characterisation rapide. Ann. Inst. Pasteur 110:465-486[Medline].
11.	Marino, G. T., and Y. Asato. 1986. Characterization of cell cycle events in the dark in Anacystis nidulans. J. Gen. Microbiol. 132:2123-2127.
12.	Messer, W., and C. Weigel. 1996. Initiation of chromosome replication, p. 1579-1601. In F. C. Neidhardt, R. Curtiss III, J. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. S. Reznikoff, M. Riley, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology. American Society for Microbiology, Washington, D.C.
13.	Mohamed, A., and C. Jansson. 1989. Influence of light on accumulation of photosynthesis-specific transcripts in the cyanobacterium Synechocystis 6803. Plant Mol. Biol. 13:693-700[Medline].
14.	Reddy, K. J., R. Webb, and L. A. Sherman. 1990. Bacterial RNA isolation with one hour centrifugation in a table-top ultracentrifuge. BioTechniques 8:250-251[Medline].
15.	Richter, S., W. R. Hess, M. Krause, and W. Messer. 1998. Unique organization of the dnaA region from Prochlorococcus marinus CCMP1375, a marine cyanobacterium. Mol. Gen. Genet. 257:534-541[Medline].
16.	Richter, S., and W. Messer. 1995. Genetic structure of the dnaA region of the cyanobacterium Synechocystis sp. strain PCC 6803. J. Bacteriol. 177:4245-4251[Abstract/Free Full Text].
16a.	Richter, S., and W. Messer. Unpublished data.
17.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
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