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ENVIRONMENTAL STRESS AND ADAPTATION TO STRESS

Characterization of Single and Double Inactivation Strains Reveals New Physiological Roles for Group 2 Factors in the Cyanobacterium Synechocystis sp. PCC 6803^1,[W]

Plant Physiology and Molecular Biology, Department of Biology, University of Turku, FI–20014 Turku, Finland (M.P., L.G., I.T., V.R., E.T., T.T.); and Department of Biochemistry and Pharmacy, Åbo Academi University, FI–20520 Turku, Finland (T.S.)

	ABSTRACT

TOP ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

 
Cyanobacteria are eubacteria that perform oxygenic photosynthesis like plants. The initiation of transcription, mediated by the RNA polymerase holoenzyme, is the main determinant of gene regulation in eubacteria. The factor of the RNA polymerase holoenzyme is responsible for the recognition of a promoter sequence. In the cyanobacterium Synechocystis sp. PCC 6803, the primary factor, SigA, is essential for cell viability. The SigB, SigC, SigD, and SigE factors show significant sequence similarity with the SigA factor but are nonessential. In this study, we have used homology modeling to construct a three-dimensional model of Synechocystis RNA polymerase holoenzyme and all group 1 and 2 factors. According to the models, the overall three-dimensional structures of group 1 and 2 factors are similar, the SigB and SigD factors being the most similar ones. In addition, we have constructed a complete set of group 2 factor double inactivation strains, sigBC, sigBD, sigBE, sigCD, sigCE, and sigDE. All double mutants grow well under standard conditions, but differences are observed in stress conditions. The transition from lag phase to exponential growth is slow in the sigBD strain, and all strains lacking the SigD factor were found to be sensitive to bright light. Furthermore, all group 2 factors were found to be involved in acclimation to salt- or sorbitol-induced osmotic stresses.

In eubacteria, the main determinant of gene regulation is the initiation of transcription mediated by the RNA polymerase holoenzyme. The eubacterial RNA polymerase holoenzyme is composed of a core enzyme (with the subunit composition ₂, β, β', ) and a factor. The core enzyme of the RNA polymerase exhibits the RNA polymerase activity, while the factor is responsible for the recognition of promoter sequences. Most bacteria synthesize several factors that compete for the same RNA polymerase core (Maeda et al., 2000), and it is believed that replacement of the factor with another factor is a major switch for changing the global transcription pattern in eubacteria.

Nine genes encode factors in Synechocystis (Kaneko et al., 1996). The sigA gene encodes the principal (group 1) factor that is essential for cell viability. The sigB, sigC, sigD, and sigE genes encode group 2 factors (primary-like factors) that show extensive amino acid similarity with the SigA factor but are not essential for cell viability under optimal growth conditions (Imamura et al., 2003; Tuominen et al., 2003). Recent results have shown that group 2 factors are important under suboptimal conditions (Osanai et al., 2005; Singh et al., 2006; Tuominen et al., 2006, 2008; Summerfield and Sherman 2007). A complicated regulatory network between the group 1 and group 2 factors has been suggested to function in Synechocystis (Lemeille et al., 2005). The sigF, sigG, sigH, and sigI genes encode alternative factors that vary more considerably in amino acid sequence that those of group 1 and 2 factors.

The structure of the bacterial RNA polymerase holoenzyme from the thermophilic bacteria Thermus thermophilus (Vassylyev et al., 2002, 2005) and Thermus aquaticus (Murakami et al., 2002a, 2002b) has been determined by x-ray crystallography. In this study, we took advantage of the high sequence identity between bacterial RNA polymerases and used the crystal structure of the RNA polymerase of T. thermophilus to construct a three-dimensional model of the RNA polymerase holoenzyme with SigA factor in Synechocystis. In addition, we constructed three-dimensional models of all group 2 factors of Synechocystis. Based on the models, the overall three-dimensional structures of group 1 and 2 factors resemble each other; the SigB and SigD factors being the most similar ones. In addition to homolog models, we have constructed a complete set of double inactivation strains of group 2 factors, including sigBC, sigBD, sigBE, sigCD, sigCE, and sigDE. We show that although all double mutants grow well under standard conditions, the transfer from lag phase to exponential growth is slow in the sigBD strain. All strains lacking the SigD factor were found to be sensitive to bright light. Furthermore, all group 2 factors were found to be involved in acclimation to osmotic stress.

	RESULTS

TOP ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

 

Specific Features of the Synechocystis RNA Polymerase

We constructed the structural models of the Synechocystis RNA polymerase holoenzyme using the crystal structure of the RNA polymerase holoenzyme of T. thermophilus (Artsimovitch et al., 2005; Protein Data Bank [PDB] code 2A6E; chains A–F) as a template. The details of the different subunits of the RNA polymerase of T. thermophilus, including areas that are missing from the template structure, together with the RNA polymerase subunits of Synechocystis, are shown in Supplemental Table S1. The subunit was excluded from the model because its sequence identity (20%) with the template was too low to ensure reliable modeling. The other subunits were 40% to 50% identical (Supplemental Table S1). Ramachandran plots of the models showed that approximately 90% of amino acid residues were in the most favorable regions and less than 1% were in disallowed regions (the corresponding values for the template were 83.9% and 0.1%), indicating good overall reliability for the models.

A specific feature of the cyanobacterial RNA polymerase is that the β' subunit has been split into two different polypeptides (Schneider and Hasekorn, 1988). The subunit of the RNA polymerase in cyanobacteria is homologous with the N-terminal part of the β' subunit of other eubacteria, and the cyanobacterial β' subunit is homologous with the C-terminal part of the β' subunit of other eubacteria. In Synechocystis, the subunit consists of 626 residues (light gray in Fig. 1 ) and the β' subunit consists of 1,317 residues (light blue in Fig. 1). According to the model, the splitting has very little effect on the overall structure of the RNA polymerase of Synechocystis, as the last amino acid residue of the subunit and the first amino acid of the β' subunit are located on the surface of RNA polymerase. Another special feature of the cyanobacterial β' subunit is that it includes a large insertion (Iyer et al., 2004) containing 635 amino acid residues in Synechocystis. The first and last amino acid residues of the insertion are shown in magenta in Figure 1A, but the insertion is not included in the model because of the lack of template for modeling. Although the three-dimensional structure of the cyanobacterial insertion remains to be solved, our model suggests that the insertion can be accommodated in the three-dimensional structure without introducing dramatic changes in the other parts of the RNA polymerase holoenzyme (Fig. 1A).

View larger version (67K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 1. Model of Synechocystis RNA polymerase. A, Homology modeling of the RNA polymerase holoenzyme with the SigA factor was performed using the crystal structure of the RNA polymerase holoenzyme of T. thermophilus (Artsimovitch et al., 2005; PDB code 2A6E; chains A–F) as the template. Views are from the front toward the catalytic center (left) and from the side (right). The core enzyme consists of two subunits (light pink), the β subunit (light brown), the β' subunit (light blue), and the subunit (gray). The first and last residues of the cyanobacterial insertion in the β' subunit are indicated with magenta. In the otherwise yellow factor, the 4.2 region is green, the 2.4 region is blue, and the NCR connecting the conserved regions 1.2 and 2.1 is red. The catalytic magnesium ion is presented as an orange sphere, and two zinc ions are presented as green spheres. B, Models of principal (SigA) and group 2 (SigB–SigE) factors of Synechocystis. The coloring is as in A. C, Sequence alignment of Synechocystis and T. thermophilus factors. Absolutely conserved residues are shown in orange, and conserved regions from 1.2 to 4.2 are indicated with boxes. Residues missing from the structures are shaded gray. The numbering of amino acid residues and the secondary structure assignment, with barrels denoting -helices, are shown above the alignment for the template. The coloring of secondary structures is as in A. The cyanobacterial conserved Trp residue is indicated with a black background.

Single and Double Inactivation Strains of Group 2 Factors in Synechocystis

In order to study the role of each group 2 factor, we constructed single and double inactivation strains. The sigB (strain sigB), sigC (strain sigC), sigD (strain sigD), and sigE (strain sigE) genes were inactivated with a kanamycin (Kn) resistance cassette in Synechocystis. The constructs of all inactivation strains are shown in Supplemental Figure S1. The double inactivation strains were constructed by inactivating the second sig gene with a streptomycin/spectinomycin (Str/Spc) resistance cassette. The sigC gene was inactivated in the sigB strain (resulting in sigBC), the sigD gene was inactivated in the strains sigB (resulting in sigBD) and sigC (resulting in sigCD), and the sigE gene was inactivated in strains sigB (resulting in sigBE), sigC (resulting in sigCE), and sigD (resulting in sigDE). Two lines that were descendants of two independently raised colonies on the first selection plate were originally tested from each inactivation strain. Because the two lines behaved similarly, the results are shown only for one line. Testing of two independent lines minimizes the possibility that the results could be affected by secondary mutations. PCR verification confirmed that the strains were completely segregated (Supplemental Fig. S2).

First we measured the growth rates of all single and double inactivation strains under standard growth conditions (32°C, continuous light of 40 µmol photons m^–2 s^–1, ambient CO₂ concentration). A₇₃₀ was set to 0.1, and the growth of a 50-mL cell culture in a 250-mL Erlenmeyer flask was followed for 14 d. All inactivation strains grew autotrophically with the same growth rate as the control strain (Fig. 2A ). In our standard conditions, growth was exponential only at the very beginning of the growth experiment; thereafter, the growth was linear for a few days. Finally, growth of the cells slowed down, and by the 14th d the cells were hardly growing (Fig. 2A). As some researchers routinely grow Synechocystis cells under CO₂-enriched atmosphere, we tested the growth of all inactivation strains under otherwise similar conditions as our standard conditions but supplemented the air of the growth chamber with 3% CO₂. All strains grew faster under high-CO₂ conditions than under ambient CO₂ conditions, the doubling time being 8 h at high CO₂ and 14 h at air level CO₂ during the 1st d, but no differences were detected between the control and inactivation strains (Fig. 2B). The growth rate became slower throughout the whole experiment, both in 3% CO₂ and in ambient CO₂.

View larger version (18K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 2. Growth of single and double inactivation strains of group 2 factors of Synechocystis. The A730 of the cell culture was set to 0.1, and the cells were grown in BG-11 medium under the continuous illumination of 40 µmol photons m–2 s–1 at 32°C under air levels of CO2 (A) or under 3% CO2 (B). Each growth curve represents the mean of five independent experiments, and the error bars denote SE.

View larger version (28K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 3. Light-saturated rates of photosynthesis (A) and PSII electron transport (B) in the factor inactivation strains. The rate of in vivo photosynthetic oxygen evolution was measured with an oxygen electrode in BG-11 medium supplemented with 10 mM NaHCO3 under saturating light (500 µmol photons m–2 s–1) at 32°C. The light-saturated rate of PSII electron transport was measured similarly as photosynthesis, except that 0.7 mM 2,6-dichlorobenzoquinone was used as an artificial electron acceptor. The measurements were repeated three times using independent liquid cultures each time. The error bars denote SE.

All Strains with an Inactivated sigD Gene Grow Slowly under Bright Light, and the Transition from Lag to Exponential Phase Is Slow in the sigBD Strain

To follow the growth of the inactivation strains under different light conditions, dilute Synechocystis cultures (A₇₃₀ was 0.1, corresponding to 3.6 x 10⁶ cells mL^–1) were spotted on BG-11 plates and the plates were grown under constant irradiance of 20, 40, or 80 µmol photons m^–2 s^–1 at 32°C. Under low light (20 µmol photons m^–2 s^–1), the growth of the sigBD strain was delayed, and also the sigBC strain grew slightly more slowly than the control strain or the other inactivation strains (Fig. 4A ).

View larger version (57K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 4. Growth of the inactivation strains under different light intensities. A, The A730 of each strain was set to 0.1, and 5 µL of each cell culture was spotted on BG-11 plates. The plates were grown under continuous illumination of 20 (low light), 40 (growth light), or 80 (high light) µmol photons m–2 s–1 at 32°C for 7 d (growth and high light) or 8 d (low light). The data shown are representative of three independent experiments showing similar results. B, The A730 of the control (CS) and sigBD strains was set to 10, 1, 0.1, or 0.01, and 5 µL of each dilution was spotted on BG-11 plates or cells were streaked directly from an old plate. The data shown are representative of three independent experiments showing similar results. C, Growth of the control and sigBD strains in liquid culture. The A730 of the cell culture was set to 0.01 (closed symbols) or 0.001 (open symbols), and the cells were grown in BG-11 medium under continuous illumination of 40 µmol photons m–2 s–1 at 32°C for 4 d. Each growth curve represents the mean of three independent experiments, and the error bars denote SE.

The dependence of the growth of the sigBD strain on cell density suggests that cell-to-cell communication might be important for growth. We tested the possibility that cells of the control and sigBD strains secrete different chemical signals to the growth medium. The A₇₃₀ was set to 0.001 and the control and sigBD strains were grown for 3 d. Thereafter, the cells were removed from the growth medium and new dilute batch cultures were started so that cells of the control strain grew in used sigBD strain-BG-11 medium and the new sigBD culture was started in used control strain medium. We compared the growth of control and sigBD strains in these and in fresh BG-11 media; at the beginning of the experiment, the A₇₃₀ was set to 0.001. The sigBD strain always grew more slowly than the control strain, despite the used growth medium (data not shown), indicating that a secreted chemical signal is unlikely to explain the slow growth of the sigBD strain in dilute culture or that the chemical signal is short-lived.

In the spot test experiments, the clearest phenotypes were seen under high-light conditions. Strains with an inactivated sigD gene (sigD, sigCD, and sigDE) hardly grew at all at 80 µmol photons m^–2 s^–1, and the double inactivation strain sigBD died (Fig. 4A). These results indicate that the SigD factor is extremely important for acclimation to bright light and further underline the redundancy of the functions of the SigB and SigD factors. The results also show that the antibiotic resistance cassette used to inactivate the gene does not interfere with the results, as the sigD gene was inactivated with a Kn cassette in strains sigD and sigDE and with a Str/Spc cassette in strains sigBD and sigCD (Supplemental Fig. S1).

All Group 2 Factors Are Involved in Osmotic Acclimation of Synechocystis

Our earlier experiments indicated activation of the sigB gene by a short osmotic shock (Tuominen et al., 2003). We studied the expression of the sigB gene in more detail by following the amount of sigB transcripts under salt- and sorbitol-induced osmotic stress in the control strain. Addition of 0.7 M NaCl induced an 8-fold increase in the amount of sigB transcripts within 10 min, and after a 1-h treatment, the amount of sigB transcripts was still twice as high as that measured under the standard growth conditions (Fig. 5 ). Thereafter, the amount of sigB transcripts decreased below the amount measured under the standard growth conditions, and only traces of sigB transcripts were detected after 24 h of salt treatment (Fig. 5). Sorbitol-induced osmotic stress, in turn, caused more permanent up-regulation of sigB transcripts, and three times as high levels of sigB transcripts, compared with the amount measured under standard growth conditions, were measured even after 24 h of sorbitol-induced osmotic stress (Fig. 5). In addition to the SigB factor, the SigD factor also has been suggested to be involved in signal transduction of short high-salt and high-sorbitol shock treatments (Shoumskaya et al., 2005). To get a more comprehensive picture of the importance of the different factors under osmotic stress, we grew cells of all inactivation strains for 5 d in BG-11 medium supplemented with either 0.7 M NaCl or 0.5 M sorbitol. These concentrations of salt and sorbitol were chosen because they slowed down the growth of the control strain by approximately 30% in our test experiments.

View larger version (31K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 5. Accumulation of sigB mRNA in the control strain under osmotic stress. The growth medium was supplemented with 0.7 M NaCl or 0.5 M sorbitol, as indicated, and samples were withdrawn before the addition (0) and after 10 min and 1, 6, and 24 h of incubation. Thereafter, total RNA was isolated and the amount of sigB mRNA was detected with the northern-blot technique. The data shown are representative of three independent northern-blot experiments showing similar results.

View larger version (19K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 6. Growth of single (A) and double (B) inactivation strains under high-salt stress. The A730 of the cell culture was set to 0.1, and the cells were grown in BG-11 medium supplemented with 0.7 M NaCl under continuous illumination of 40 µmol photons m–2 s–1 at 32°C. Each growth curve represents the mean of three independent experiments, and the error bars denote SE.

View larger version (20K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 7. Growth of single (A) and double (B) inactivation strains under high-sorbitol stress. The A730 of the cell culture was set to 0.1, and the cells were grown in BG-11 medium supplemented with 0.5 M sorbitol under continuous illumination of 40 µmol photons m–2 s–1 at 32°C. Each growth curve represents the mean of at least five independent experiments, and the error bars denote SE.

	DISCUSSION

TOP ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

View this table: [in this window] [in a new window]   Table I. Growth of group 2 factor inactivation strains under different environmental conditions Growth is compared with the growth of the control strain under the same conditions. +++, Similar growth as in the control strain; ++(+), slightly slower growth; ++, slower growth; +, only very slow growth; +/–, slow growth for a short time; –, no growth; ND, not determined.

We show in this study that the SigB factor is rapidly up-regulated by osmotic stress induced by salt and by sorbitol and that cells do not grow without SigB under these conditions. On the other hand, similar rapid transient up-regulation of the sigB gene occurs at mild heat stress at 43°C, but the sigB strain grows almost as well as the control strain (Tuominen et al., 2006). These results indicate that there is no simple direct correlation between the increase in sigB transcripts and the importance of the SigB factor under a particular stress condition.

It is well documented that the SigB factor is involved in the up-regulation of heat shock genes, especially the hspA gene, at high temperatures (Imamura et al., 2003; Singh et al., 2006; Tuominen et al., 2006). Many heat shock proteins, particularly HspA, are important chaperones in acclimation to osmotic stress (Asadulghani et al., 2004). We compared the expression of the hspA gene in the control and sigB strains in osmotic stresses. In salt stress, the amount of hspA mRNA remained lower in sigB than in the control strain (Supplemental Fig. S3), but the expression kinetics was similar in both strains. However, when osmotic stress was induced with sorbitol, the induction of the hspA gene was slower in the sigB strain than in the control strain, but after 1 h the amount of hspA mRNA in sigB exceeded that in the control strain (Supplemental Fig. S3). Interestingly, an hspA inactivation strain has been found to tolerate well mild (0.5 M NaCl) salt-induced osmotic stress (Asadulghani et al., 2004), and we have noticed that the sigB strain grows well in BG-11 medium supplemented with 0.5 M NaCl (data not shown). These results indicate that inactivation of the sigB gene affects the expression of the hspA gene not only in heat stress but also in salt- and sorbitol-induced stresses.

In this study, we show that the SigC factor is involved in acclimation to salt stress and also to a lesser extent to sorbitol stress. Previously, SigC of Synechocystis and SigE, its closest homolog in Synechococcus sp. PCC 7002, were assigned roles in stationary phase-related gene expression and growth (Gruber and Bryant, 1998; Asayama et al., 2004; Imamura et al., 2006) and in Synechocystis also in acclimation to heat stress (Tuominen et al., 2008). We did not see differences in growth rate between the control and sigC strains during the studied 14 d in standard conditions (Fig. 2), but Asayama et al. (2004) noticed a slight delay of growth in a sigC inactivation strain after 3 weeks. A unique feature of the SigC factor is that the sigC gene is not specifically up-regulated at high temperature (Tuominen et al., 2008) or under osmotic stress (Tuominen et al., 2003, Shoumskaya et al., 2005) or stationary phase (Asayama et al., 2004), yet SigC factor is required for acclimation to those conditions. These results suggest that the sigC gene might be regulated posttranscriptionally. One possible explanation is that the RNA polymerase core has an increased tendency to recruit the SigC factor under these stress conditions. In Escherichia coli, the small signaling molecule ppGpp (for guanosine 5'-diphosphate 3'-diphosphate) directly binds to the RNA polymerase core (Artsimovitch et al., 2004), and active transcription from promoters that depend on ^S, the only group 2 factor in E. coli, requires ppGpp (Kvint et al., 2000). A similar system might explain why SigC is important in conditions in which the sigC gene is not up-regulated.

All strains with inactivated sigD gene were unable to grow under high light. DNA microarray analysis has shown that the expression of the sigD gene increases in response to high light in Synechocystis (Hihara et al., 2001; Huang et al., 2002). Furthermore, Imamura et al. (2003) reported an increase in the amount of SigD protein after high-light treatment. In another cyanobacterium, Synechococcus elongatus PCC 7942, one of the five group 2 factors, RpoD3, was recognized as a high-light-responsive factor (Seki et al., 2007). The amino acid sequences of the RpoD3 factor of Synechococcus elongatus PCC 7942 and the SigD factor of Synechocystis suggest that these factors are closely related (Seki et al., 2007).

Enhancement of the expression of the sigD gene has been detected in both sorbitol- and salt-induced stresses (Shoumskaya et al., 2005). However, inactivation of the sigD gene only slightly slowed down the growth of Synechocystis under high-salt or high-sorbitol conditions (Figs. 6 and 7), and our earlier experiments did not show induction of sigD under salt stress (Tuominen et al., 2003). Shoumskaya et al. (2005) used more bright light in their experiments than we used in our experiments; thus, the amount of light during osmotic stress might explain the differences in the results. Interestingly, the SigD factor was suggested to be part of a signaling cascade in which signals are transduced by His kinase (Hik) 33 and the cognate response regulator (Rre) 31 during osmotic acclimation (Marin et al., 2003; Shoumskaya et al., 2005). We noticed that genes (all 10 genes under salt stress and 11 of 12 genes under sorbitol stress) belonging to the Hik33-Rre31 cascade were among those genes that were up-regulated under UV light and high-light stress conditions (Huang et al., 2002). Furthermore, almost all of these same genes were less induced in the Hik33 strain than in the wild-type strain under oxidative stress caused by hydrogen peroxide treatment (Kanesaki et al., 2007). Because UV light and high-intensity visible light, as well as treatment with high salt, can induce the production of reactive oxygen species, it is possible that the SigD factor is required for acclimation to conditions that enhance the production of reactive oxygen species. We tested the effect of mild oxidative stress by growing the sigD and control strains in the presence of 0.1 µM methyl viologen. Methyl viologen accepts an electron from PSI and reduces oxygen to O₂^–, which is converted to hydrogen peroxide by superoxide dismutase. Synechocystis can grow in the presence of 0.5 µM methyl viologen in moderate light (Tichy and Vermaas, 1999). Figure 8 shows that the sigD strain grew slightly more slowly than the control strain. This finding supports our idea that the SigD factor is involved in acclimation to oxidative stress.

View larger version (7K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 8. Growth of the sigD and control strains under mild oxidative stress. The A730 of the cell culture was set to 0.1, 0.1 µM methyl viologen was added, and the cells were grown under continuous irradiance of 40 µmol photons m–2 s–1 at 32°C under air levels of CO2. Each growth curve represents the mean of three independent experiments, and the error bars denote SE.

The fact that the three-dimensional models of the SigB and SigD factors (Fig. 1) are the most similar among Synechocystis factors, and the finding that only the sigBD strain (not sigB or sigD) shows slow transition from lag phase to exponential growth (Fig. 4), suggest partial redundancy in the functions of these two factors. Furthermore, the sigBD strain is more sensitive to heat stress (Tuominen et al., 2006) and to high light (Fig. 4) than sigB or sigD. However, under osmotic stress, the sigBD strain was not more sensitive than the sigB strain. Of the other double mutants, the sigBsigE strain was shown to grow badly under mixotrophic conditions in a 12-h-light/12-h-dark rhythm, although sigB and sigE strains grew well (Summerfield and Sherman, 2007). Both sigB and sigC strains are sensitive to heat stress (Tuominen et al., 2006, 2008). These two factors regulate completely different sets of genes at high temperature, which makes the double mutant sigBC extremely sensitive to heat stress (Tuominen et al., 2008).

In conclusion, the overall three-dimensional structures of all group 1 and 2 factors in Synechocystis resemble each other, despite the NCD, which lies right next to the –10 promoter region in the three-dimensional structure (Fig. 1A) and thus might play a regulatory role in promoter binding. The overall structural similarity suggests that the different factors may have overlapping functions. The physiological results obtained with the single and double inactivation strains support this suggestion. In particular, functional redundancy of group 2 factors is confirmed by the finding that all possible combinations of group 2 factor double inactivation mutants are viable in Synechocystis. Functional redundancy, found in transition from lag phase to exponential growth, is obvious between the SigB and SigD factors that show significant sequence identity even within the NCD connecting the conserved domains 1.2 and 2.1. However, treatments under different stress conditions also revealed that each group 2 factor is important under a specific set of conditions. The SigD factor is involved in high-light responses in Synechocystis, and all group 2 factors have a role in acclimation to salt- or sorbitol-induced osmotic stress, the SigB factor being the most important one.

	MATERIALS AND METHODS

TOP ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

 

Structural Modeling of Synechocystis RNA Polymerase Holoenzyme

The amino acid sequences of the subunits of RNA polymerase of Synechocystis (Table I) were obtained from CyanoBase (www.kazusa.or.jp/cyanobase) and aligned with the sequences of their respective counterparts from the Thermus thermophilus RNA polymerase structure (Artsimovitch et al., 2005; PDB code 2A6E; chains A–F were used as the structural template) with the program MALIGN (Johnson and Overington, 1993) in the Bodil visualization and modeling package (Lehtonen et al., 2004). The secondary structure predictions for the sequences were made with PredictProtein (Rost and Liu, 2003). As the sequence identities between the subunits of T. thermophilus and Synechocystis RNA polymerases were reasonably high (Supplemental Table S1), alignment was fairly straightforward. The only exceptions were the factors, which were aligned as follows: First, SigA and SigC were aligned with the template, the alignment was fixed, and then SigB, SigD, and SigE were aligned with the previously fixed alignment. Finally, the alignment was modified so that the Synechocystis factors have a conserved Trp at the end of the NCD before region 2.1 (Fig. 1C). Structural modeling was done with MODELLER (ali and Blundell, 1993) using the very thorough variable target function optimization method. Ten models were generated for each of the factors, and those with lowest objective function, as given by MODELLER, were chosen for further investigation. The stereochemical quality of the models was assessed with PROCHECK (Laskowski et al., 1993).

Construction of Group 2 Factor Inactivation Strains in Synechocystis

The Glc-tolerant strain of Synechocystis (Williams, 1988) was used as a control strain. The sigB (sll0306), sigC (sll0184), sigD (sll2012), and sigE (sll1689) genes were amplified by PCR with primers specific for sigB (5'-ATGGTAACAGTGACAGTTAT-3' and 5'-TAGCTCTTGGCCATCGTTA-3'), sigC (5'-ATGACTAAACCAAGCAACGA-3' and 5'-AATCTAGCAAAATTTCCTGC-3'), sigD (5'-ATGACTGCCAGAACCAGCCC-3' and 5'-GCCTCCCTACAGTTGGATCT-3'), and sigE (5'-ATGAGCGATATGTCTTCCCT-3' and 5'-CTATAACCAACCTTTGAGGC-3'). The PCR products were cloned into the pCR-Blunt II-TOPO vector (Invitrogen). The pCR-Blunt II-TOPO-sigB was digested with KpnI and PstI, and the sigB fragment was ligated into the KpnI and PstI double-digested pUC19. The pUC19-sigB was digested with SmaI, and BamHI polylinker (New England Biolabs) was added. The inactivation plasmid pUC19-sigB-Kn was constructed by ligating the BamHI fragment of pUC4K (Amersham Biosciences), carrying the Kn resistance cassette, into the BamHI site. The pCR-Blunt II-TOPO-sigC was digested with SpeI and EcoRV, and the sigC fragment was ligated into the XbaI and SmaI double-digested pUC19. To construct the inactivation plasmid pUC19-sigC-Kn, the pUC19-sigC was digested with BglII and the BamHI fragment of pUC4K was then ligated into the BglII restriction site. To construct the inactivation plasmid pUC19-sigC-, the BamHI fragment (the fragment that confers resistance for Spc and Str) of pHP45 (Prentki and Krisch, 1984) was ligated into BglII-digested pUC19-sigC. The pCR-Blunt II-TOPO-sigD was digested with SpeI and EcoRV, and the sigD fragment was ligated into the XbaI and SmaI double-digested pUC19. The pUC19-sigD-Kn was constructed by ligating the BamHI fragment of pUC4K into BamHI-digested pUC19-sigD. To construct the inactivation plasmid pUC19-sigD-, the BamHI fragment of pHP45 was ligated into BamHI-digested pUC19-sigD. The pCR-Blunt II-TOPO-sigE was digested with PstI and EcoRI, and the sigE fragment was ligated into the PstI and EcoRI double-digested pUC19. The inactivation plasmids pUC19-sigE-Kn and pUC19-sigE- were constructed by ligating the BamHI fragment of pUC4K and the BamHI fragment of pHP45, respectively, into BamHI-digested pUC19-sigD.

The control strain was transformed with the vector pUC19-sigB-Kn, pUC19-sigC-Kn, pUC19-sigD-Kn, or pUC19-sigE-Kn according to Williams (1988). Transformants were isolated on selective BG-11 agar plates containing Kn (50 µg mL^–1). For double mutants, the sigB and sigC inactivation strains were transformed with pUC19-sigD-; the sigB, sigC, and sigD inactivation strains were transformed with pUC19-sigE-; and the sigB strain was transformed with pUC19-sigC-. Transformants were isolated on BG-11 agar plates containing Kn (25 µg mL^–1), Spc (20 µg mL^–1), and Str (10 µg mL^–1).

The complete replacement of the native gene with the inactivated gene was confirmed by PCR analysis of corresponding genomic DNA. Genomic DNA was isolated (Williams, 1988), and the sigB, sigC, sigD, or sigE gene, depending on the strain, was amplified by PCR using the same primers as in the cloning procedure.

Growth Conditions and Measurements

Synechocystis was grown in BG-11 medium (Rippka et al., 1979) supplemented with 20 mM HEPES-NaOH, pH 7.5, under the continuous photosynthetic photon flux density (PPFD) of 40 µmol m^–2 s^–1 and ambient CO₂ levels at 32°C. Liquid cultures were shaken at 90 rpm. These are referred to as standard growth conditions. For high-CO₂ conditions, air was supplemented with 3% CO₂. The BG-11 agar plates for strains sigB, sigC, sigD, and sigE were supplemented with Kn (50 µg mL^–1), and plates for strains sigBD, sigBC, sigBE, sigCD, sigCE, and sigDE were supplemented with Kn (25 µg mL^–1), Spc (20 µg mL^–1), and Str (10 µg mL^–1). For the experiments, cells were grown without antibiotics in liquid BG-11 medium.

The A₇₃₀ of liquid cultures was set to 0.1, and the growth of the cells (50 mL of cell culture in a 250-mL Erlenmeyer flask) was monitored under standard growth conditions (PPFD of 40 µmol m^–2 s^–1, 32°C, shaking at 90 rpm) by measuring A₇₃₀ for 14 d. Samples of dense cultures were diluted with BG-11 before the absorbance was measured, so that A₇₃₀ did not exceed 0.4, and the dilutions were taken into account when the final results were calculated. In addition, growth of the control and sigBD strains was followed so that A₇₃₀ was set to 0.01 and 0.001 at the beginning of the growth experiment. Osmotic stress was induced by supplementing BG-11 medium with either 0.7 M NaCl or 0.5 M sorbitol, as indicated. The A₇₃₀ was set to 0.1, and the growth of the cells was monitored under standard growth conditions (PPFD of 40 µmol m^–2 s^–1, 32°C) for 5 d. Oxidative stress was induced by supplementing BG-11 medium with 0.1 µM methyl viologen. The A₇₃₀ was set to 0.1, and the growth of the cells was monitored under standard growth conditions (PPFD of 40 µmol m^–2 s^–1, 32°C) for 2.5 d.

The growth of the inactivation strains was screened on plates under various light conditions. The A₇₃₀ of each strain was set to 0.1, and 5 µL of each cell suspension was spotted onto a BG-11 plate. The plates were then kept under continuous light at the PPFD of 20, 40, or 80 µmol m^–2 s^–1, as indicated, and photographed at the indicated times. The effect of dilution on growth on solid medium was tested in sigBD and control strains. The A₇₃₀ of the cell suspension was first set to 10, 1, 0.1, 0.01, and 0.001, and 5 µL of the cell suspensions was spotted onto BG-11 plates. The plates were kept in the standard growth conditions and photographed after 1 week.

Determination of Photosynthetic and PSII Capacity

In vivo photosynthetic activity of the control and inactivation strains (1 mL of cell suspension containing 10 µg chlorophyll mL^–1) was measured in BG-11 medium supplemented with 10 mM NaHCO₃ under saturating light (500 µmol photons m^–2 s^–1) with a Clark-type oxygen electrode (Hansatech) at 32°C. PSII capacity was measured similarly as photosynthetic capacity, except that 0.7 mM 2,6-dichloro-p-benzoquinone was used as an artificial electron acceptor and 0.7 mM ferricyanide was added to keep the quinone in an oxidized form.

RNA Isolation and Northern Blotting

Total RNA was isolated as described by Tyystjärvi et al. (2001). The RNAs were separated on 1.2% agarose-glyoxal gels and subsequently transferred to Hybond-N⁺ membranes (Amersham Biosciences) according to standard procedures (Sambrook and Russell, 2001). A 7-µg aliquot of total RNA was loaded per lane. Equal loading of the gels was confirmed by methylene blue staining (Sambrook and Russell, 2001). The gene-specific probes were amplified by PCR with primers specific for sigB (5'-TGGTAACAGTGACAGTTAT-3' and 5'-GCTTCAATCATTTTCCGTTT-3') and for hspA/sll1514 (5'-GTCTCTCATTCTTTACAATCC-3' and 5'-TTAGGAAAGCTGAACTTTCAC-3'). The probes were labeled, hybridized, and detected using the DIG High Prime DNA Labeling and Detection Starter Kit II (Roche) according to the instruction manual of the kit.

Supplemental Data

The following materials are available in the online version of this article.

Supplemental Figure S1. The factor inactivation strains of Synechocystis.

Supplemental Figure S2. PCR analysis of inactivation strains.

Supplemental Figure S3. The amount of hspA transcripts in the control and sigB strains under salt or sorbitol stress.

Supplemental Table S1. Similarity of RNA polymerase subunits in Synechocystis and T. thermophilus.

Received May 9, 2008; accepted May 28, 2008; published June 6, 2008.

	FOOTNOTES

 
¹ This work was supported by the Academy of Finland.

The author responsible for distribution of materials integral to the findings presented in this article in accordance with the policy described in the Instructions for Authors (www.plantphysiol.org) is: Taina Tyystjärvi (taityy{at}utu.fi).

^[W] The online version of this article contains Web-only data.

www.plantphysiol.org/cgi/doi/10.1104/pp.108.122713

^* Corresponding author; e-mail taityy{at}utu.fi.

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