Email updates

Keep up to date with the latest news and content from BMC Microbiology and BioMed Central.

Open Access Research article

A ring-like nucleoid is not necessary for radioresistance in the Deinococcaceae

Julie M Zimmerman and John R Battista*

Author Affiliations

Department of Biological Sciences, Louisiana State University and A&M College, Baton Rouge, Louisiana 70803, USA

For all author emails, please log on.

BMC Microbiology 2005, 5:17  doi:10.1186/1471-2180-5-17

The electronic version of this article is the complete one and can be found online at: http://www.biomedcentral.com/1471-2180/5/17


Received:12 November 2004
Accepted:31 March 2005
Published:31 March 2005

© 2005 Zimmerman and Battista; licensee BioMed Central Ltd.

This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

Abstract

Background

Transmission electron microscopy images of Deinococcus radiodurans R1 suggest that the nucleoid of this species exists as a "ring-like" body, and have led to speculation that this structure contributes to the radioresistance of the species. Since extreme radioresistance is characteristic of six other species of Deinococcus, we have attempted to correlate nucleoid morphology and radioresistance by determining whether the genomic DNA of each of these species exhibit similar structures.

Results

The nucleoid morphologies of seven recognized species of Deinococcus, the radioresistant bacterium Rubrobacter radiotolerans, and the more radiosensitive deinococcal relative Thermus aquaticus were evaluated using epifluorescence and deconvolution techniques. Although the nucleoids of Deinococcus murrayi, Deinococcus proteolyticus, Deinococcus radiophilus, and Deinococcus grandis have structures similar to D. radiodurans, the majority of nucleoids found in Deinococcus radiopugnans and Deinococcus geothermalis lack any specific organization. The nucleoid of R. radiotolerans consists of multiple highly condensed spheres of DNA scattered throughout the cell. The genomic DNA of Thermus aquaticus is uniformly distributed throughout the cell.

Conclusion

There is no obvious relationship between the shape of a species' nucleoid and extreme radioresistance. However, the genomes of all extremely radioresistance species examined are highly condensed relative to more radiosensitive species. Whether DNA in this tightly packed configuration contributes to the radioresistance of these bacteria remains unknown, but this common structural feature appears to limit diffusion of fragments generated post-irradiation even in cells incapable of repairing strand breaks.

Background

The Deinococcaceae are a small family within the domain Bacteria that are distinguished by their ability to tolerate DNA double strand breaks [1,2]. There are eleven validly described species and seven of these tolerate what for most microorganisms is a sterilizing dose of ionizing radiation, exhibiting detectable survival after exposure to 10 kGy (1,000,000 Rad) γ radiation [3]. The ionizing radiation resistance of the four remaining species, Deinococcus indicus [4], Deinococcus frigens, Deinococcus saxicola, and Deinococcus marmoris [5] has not been reported. Ionizing radiation generates an array of DNA damage in the target cell, including many types of base damage, single, and double strand breaks [6]. Of these types of damage, DNA double strand breaks (DSBs) are considered the greatest threat to cell viability, and an excessive number of DSBs are expected to be lethal. E. coli, for example, cannot survive introduction of greater than one or two DSBs into its genome [7]. In contrast, D. radiodurans survives doses of ionizing radiation that generate greater than 100 DSBs per genome without mutation or loss of viability [8-10]. It is the ability to endure and accurately repair these lesions that set the deinococci apart from other species.

The reasons for the deinococci's radioresistance are poorly understood. Genetic and biochemical evidence obtained from D. radiodurans, the best studied of these species, argues that recovery requires RecA-mediated homologous recombination [9,11,12]. D. radiodurans is multi-genomic, and depending on the growth phase, cells contain from 4 to 10 copies of their genome depending on growth conditions [13,14]. It is believed that this increased DNA content is protective in that it serves as a reservoir of genetic information that can be used during recombinational repair. In addition, it has been suggested that there may be a pre-existing alignment of homologous sequences between copies of the genome and that this alignment accounts for the remarkable speed and fidelity of DNA double strand break repair in this species [15]. However, the existence of such an alignment has not been established.

Levin-Zaidman et al. [16] have reported that the genome of D. radiodurans assumes a tightly packed ring-like structure that may represent an alternative mechanism for protecting D. radiodurans from DSBs. These authors suggest this structure contributes to D. radiodurans radioresistance by preventing fragments formed by DSBs from diffusing apart during repair. Having the capacity to maintain the linear continuity of its genome in the face of the extensive fragmentation resulting from high dose ionizing radiation would provide obvious advantages to D. radiodurans. Assuming that DNA repair proteins can function within the proposed structure, gene order is preserved and the gaps generated by damage and subsequent DNA degradation could be bridged by homologous recombination with redundant genetic information available in the genome copies. Such an arrangement does not require a pre-existing alignment between sequences, but if homologous genetic information is aligned prior to irradiation, the time needed to effect repairs should be reduced.

In an attempt to gain insight into whether the structures reported by Levin-Zaidman et al contribute to ionizing radiation resistance, we have combined epifluorescence and deconvolution microscopy to describe the structure of the nucleoid of the seven species of the Deinococcaceae known to be ionizing radiation resistant. We assume that if ring-like structures are required for extreme radioresistance, all deinococci will contain a similarly organized nucleoid. In addition, we have examined the nucleoid structure of a related but less radioresistant species, Thermus aquaticus, and a phylogenetically distinct, but more radioresistant [17] species Rubrobacter radiotolerans seeking to correlate variations in nucleoid morphology with radioresistance. We find little evidence to support the assertion that a specific nucleoid structure is required for bacterial ionizing radiation resistance, but note that the genomic DNA of the most radioresistant species examined is more condensed relative to more radiosensitive species, suggesting that this generic feature is passively facilitating repair processes.

Results

The nucleoid of Deinococcus radiodurans R1

Sequential digital images were collected at 100 nm increments from stationary phase cultures of D. radiodurans R1. Cells were stained with the membrane dye FM4-64 and the DNA specific dye DAPI (4', 6-diamidino-2-phenylindole), and the images obtained using each dye were merged to form the sequence of images depicted in Fig. 1. In agreement with previous descriptions of this species' nucleoid, the genomic DNA of R1 exhibits a clear organized pattern [16,18,19], distinct from that observed in E. coli (Fig. 2) where the DAPI-stained DNA appears uniformly distributed throughout each cell. The DNA of R1 has a distinctive ring-like structure in each cell of this tetrad, suggesting that the genome of this species is spooled around a sphere or cylinder that excludes the dye. Given the size and organization of this structure we assume that the proposed core is primarily proteinaceous, but don't exclude the possibility that other macromolecules, including DNA that is inaccessible to the dye, may be present in the core. Based on the images in Fig. 1, we believe that the DAPI-stained DNA exists as an equatorial band (or possibly a tight spiral) over the surface of this core. In each of the cells the band is tilted relative to the focal plane. For example, in the lower half of the tetrad, the bands are tilted slightly away from the viewer; toward the upper left in the cell on the left and toward the upper right in the cell on the right. Consistent with this interpretation, we find that the dye does not form a closed ring in every optical section and that the patterns vary from cell to cell. In many cells the DNA first appears in a crescent shape in one area of the cell. This crescent changes in sequential sections (Fig. 1), ultimately disappearing and giving way to a crescent shaped structure that mirrors where the dye first appeared. This pattern of changes is most simply explained by assuming that the DNA is on the surface of a larger structure capable of tilting about a central axis. When tilted, the ring of dye will cross the focal plane at an angle and produce a falcate shape.

thumbnailFigure 1. Optical sections of a tetrad of D. radiodurans R1. The series is in order from left to right of images within a row and from top to bottom of rows within the figure. Images are taken at 100 nm intervals. The DNA (blue) is stained with DAPI and the lipid membrane (red) is stained with FM-4-64.

thumbnailFigure 2. An epifluorescence image of E. coli K12 strain AB1157.

The nucleoid of most, but not all, species of Deinococcus is similar to that of D. radiodurans R1

D. radiophilus and D. proteolyticus have a nucleoid reminiscent of that described for D. radiodurans (Fig. 1). In cross section, the DAPI accumulates in a halo surrounding a circular core that excludes the dye. However, the organization of the DNA in these species differs subtly relative to D. radiodurans; the DNA appears to completely surround the structure at the core of the nucleoid. This point is best illustrated in Fig. 3, which depicts 20 sequential sections (moving from upper left to the lower right panel) through the DAPI-stained nucleoids in a pair of D. proteolyticus cells. (The stained membrane is not included in this image.) The first image corresponds to a focal plane at the top of the nucleoid and with each successive image; it becomes clear that the DNA forms a shell that follows the contour of an internal sphere that has not been stained. The nucleoid morphology of D. radiophilus was found to be identical to that of D. proteolyticus (data not shown).

thumbnailFigure 3. Optical sections of nucleoids in a pair of D. proteolyticus cells. The series is in order from left to right of the images within a row and from top to bottom of the rows within the figure. Images are taken at 100 nm intervals.

The nucleoid of rod-shaped D. grandis is distinctive, but shares similarity to that of D. radiodurans. The DNA in most cells is highly condensed, localized to a specific area of the cell (Fig 4). The sequential sections obtained from D. grandis suggest that the DNA surrounds an unstained core. A number of cells (~7%) exhibit additional condensed spots of DAPI stain, as illustrated in the cell on the right in Fig 4. The significance of these "spots" is not known at present.

thumbnailFigure 4. Optical sections of a pair of D. grandis cells. The series is in order from left to right of the images within a row and from top to bottom of the rows within the figure. Images are taken at 100 nm intervals.

In D. murrayi, the ring of DAPI-stained DNA is remarkably uniform (Fig. 5), varying little between cells. As with D. radiodurans, the center of the ring is not stained, but the number of sections containing DNA is more variable, ranging between 20 and 30. This suggests that the nucleoid of D. murrayi may be more cylindrical than that of D. radiodurans with the DNA forming a sleeve around the core. Consistent with this interpretation, most of the cells display a ring of DAPI in every optical section.

thumbnailFigure 5. Optical sections of a pair of D. murrayi tetrads. The series is in order from left to right of the images within a row and from top to bottom of the rows within the figure. Images are taken at 100 nm intervals.

In contrast to the other species discussed thus far, only 2% of D. radiopugnans and 10% of D. geothermalis cells exhibit a structurally well-defined nucleoid (Figs. 6 and 7). In the majority of these cells, the DNA is condensed in that it is not uniformly spread throughout the cell as was observed with E. coli (Fig 2), but it does not seem to be associated with an intracellular structure. Instead the DNA appears to be distributed chaotically through the cytosol. The absence of a consistent pattern in DAPI staining within most of the cells suggests that the DNA in these species does not adopt a fixed shape.

thumbnailFigure 6. Optical sections of a pair of D. radiopugnans cells. The series is in order from left to right of the images within a row and from top to bottom of the rows within the figure. Images are taken at 100 nm intervals.

thumbnailFigure 7. Optical sections of a D. geothermalis tetrad. The series is in order from left to right of the images within a row and from top to bottom of the rows within the figure. Images are taken at 100 nm intervals.

The nucleoid of Thermus aquaticus

The genera Thermus and Deinococcus are part of the same phylum within the domain Bacteria [3]. Because of this relationship, we sought 1) to establish if Thermus species also exhibit increased tolerance to ionizing radiation, and 2) to determine if the nucleoid of this genus bore any resemblance to that of the deinococci. We assessed the ionizing radiation resistance of Thermus aquaticus YT-1, the type species for its genus, and compared it to D. radiodurans R1. As indicated in Fig. 8, YT-1 does not display extraordinary resistance relative to R1, but this strain is better able to survive γ radiation than the E. coli AB1157 control. After 1 kGy exposure, approximately 20% of the YT-1 population remained viable, whereas only 0.2% of the AB1157 culture survived.

thumbnailFigure 8. Representative survival curves for cultures of Thermus aquaticus YT-1, E. coli AB1157, and Deinococcus radiodurans R1. Values are the means +/- standard deviations of three independent experiments. n = 9.

Images of YT-1 (Fig. 9) failed to show evidence of sub-cellular organization or condensation similar to that observed in the deinococcal species. The pattern obtained with DAPI most closely resembles that observed in E. coli (Fig. 2).

thumbnailFigure 9. An epifluorescence image of Thermus aquaticus.

The nucleoid of Rubrobacter radiotolerans

Rubrobacter radiotolerans is an extremely ionizing radiation resistant bacterium that is, based on 16S rDNA-based phylogeny, unrelated to the Deinococcaceae [17]. This species is a member of a lineage within the Actinobacteria. The nucleoid of this species is quite different from that observed in the deinococci (Fig. 10). The DNA appears to form highly compact structures without a well-defined shape. Most cells contain two or three of these structures, and it is unclear whether each dye spot represents a unit length of genomic DNA. Based on differences in size and intensity, the spots do not appear to contain equivalent amounts of DNA, but these differences may be spurious. We suspect that the cell envelope of R. radiotolerans is less permeable to DAPI than that of the other species examined in this study. Attempts to stain the DNA of the closely related R. xylanophilus [17] were unsuccessful; the dye being unable to penetrate the cell. Differing quantities of dye entering individual R. radiotolerans cells may account for the differences in dye intensity observed.

thumbnailFigure 10. Optical sections of a Rubrobacter radiotolerans cell. The series is in order from left to right of the images within a row and from top to bottom of the rows within the figure. Images are taken at 100 nm intervals.

The effect of ionizing radiation on nucleoid morphology

As has been shown previously, when D. radiodurans cells are exposed to high dose γ radiation they exhibit substantial DNA damage [10]. The distinctive pattern formed on a pulsed field gel by the NotI digested genome (data not shown) is initially obliterated by the DNA double strand breaks introduced during a 5 kGy exposure [10,20], but after three hours recovery, the pattern is restored indicating that the majority of the breaks have been repaired. To establish whether the introduction of large numbers of DNA double-strand breaks affect the distribution of DNA within the irradiated cell, we examined nucleoid structure in exponential phase D. radiodurans two hours post-irradiation, comparing the distribution of DAPI stain to that of E. coli AB1157 treated identically (Fig. 11B). The differences in the images obtained are striking. While we are able to detect DAPI-stained material in some E. coli cells, the diffuse distribution, apparent in Fig. 2, is no longer evident; only infrequent spots of DAPI remain. Furthermore, images of E. coli cells captured three hours post-irradiation of 5 kGy show a complete loss of the DAPI-stained material (data not shown). One reason for this may be that the E. coli genome is being progressively degraded following irradiation [21]. In contrast, the nucleoids of D. radiodurans and D. radiopugnans appear intact and retain the ability to be stained (Fig. 11A and 11D). These images provide support for the hypothesis of Levin-Zaidman et al [16,19], which proposes that fragments generated by the double strand breaks may be in some manner held in place and protected from extensive degradation by cellular nucleases.

thumbnailFigure 11. The nucleoid of deinococcal strains and E. coli 2 hrs after exposure to 5000Gy γ radiation. A1 – projection image of D. radiodurans R1 control cells; A2 – projection image of D. radiodurans R1 irradiated cells; B1 – 2D image of E. coli control cells; B2 – 2D image of E. coli irradiated cells; C1 – 2D image of Rec30 control cells; C2 – 2D image of Rec30 irradiated cells; D1 – one optical slice of a series of D. radiopugnans control cells; D2 – one optical slice of a series of D. radiopugnans irradiated cells.

The notion that the release of fragments from the damaged genome of D. radiodurans is limited is also apparent in our analysis of the effects of ionizing radiation on the nucleoid of the recA strain, rec30. The rec30 strain, which lacks the ability to carry out homologous recombination [8,9], is incapable of reassembling its genome following irradiation. However, like R1, the nucleoid of rec30 remains a coherent structure (Fig. 11C) two hours post-irradiation, providing further evidence that fragments generated do not diffuse throughout the cytosol despite the presence of massive numbers of un-repaired DNA double strand breaks.

Discussion

Levin-Zaidman et al [16] have reported that genomic DNA of stationary phase cells of D. radiodurans is ordered as a tightly packed toroid, and it has been argued that this organization is in part responsible for D. radiodurans resistance to ionizing radiation [16,19]. These authors assume that the dense packaging characteristic of toroids restricts the diffusion of DNA fragments generated when cells are exposed to ionizing radiation, preventing a loss of genetic information that is needed for effective recovery from the insult. However, these authors also describe logarithmic phase cultures of D. radiodurans R1, and indicate that the nucleoids of these cells do not always exhibit a toroidal ring-like morphology even though they remain extremely radioresistant [2]. This observation seems to argue against a requirement for involvement of a specific nucleoid structure in ionizing radiation resistance. In addition, Daly et al [18] have demonstrated that growth in different media alters the organization of the nucleoid of D. radiodurans, and that the change does not correspond to changes in radioresistance. This group reports that ring-like nucleoids predominate in cultures growing in defined minimal medium, but that these cultures are more sensitive to ionizing radiation than cultures with fewer ring-like nucleoids growing in a rich medium.

We initiated this study in an attempt to correlate nucleoid structure with radioresistance, reasoning that if the inferences of Levin-Zaidman et al [16] are correct, it will be reflected in morphological differences between radioresistant and radiosensitive species. We have examined species known to be ionizing radiation resistant as well as strains that are more sensitive to γ irradiation, and in agreement with Daly et al [18] find no compelling evidence that specific structures contribute to radioresistance. We base this conclusion on our failure to identify a distinctive repetitive pattern in the DAPI-stained DNA associated with the majority of D. geothermalis and D. radiopugnans cells in stationary phase culture. Cultures of D. geothermalis [22] and D. radiopugnans [23] are as radioresistant as D. radiodurans, but their genomes are more fluid, arguing that a nucleoid need not maintain a well-defined shape to sustain ionizing radiation resistance.

Despite this conclusion, we note that among the extremely radioresistant species examined DAPI-stained DNA is condensed relative to what is observed in E. coli and T. aquaticus. The DAPI is localized within the more radioresistant cells, and not spread throughout the cytosol. This aggregation of DNA indicates that a basic tenet of the model of Levin-Zaidman et al [16] may be valid: specifically that the deinococci utilize mechanisms for protecting the fragments generated by strand breaks including a passive process that limits the diffusion of these fragments. This concept is most clearly demonstrated by the behavior of rec30 strain subsequent to irradiation. Despite the fact that this strain is incapable of restituting the majority of the DSBs generated, the rec30 nucleoid retains its shape.

However, it must be noted that under certain conditions E. coli cells can undergo changes in nucleoid morphology similar to those reported for the deinococci. E. coli nucleoids become condensed spheres with cores of unknown composition when protein synthesis is inhibited [24], and when the mukB locus is disrupted the resulting mutant maintains a ring-like nucleoid [25]. Clearly, since E. coli strains are much more sensitive to ionizing radiation relative to D. radiodurans, the presence of a condensed nucleoid alone is not a sufficient explanation for radioresistance. Instead, we assume the combination of a condensed nucleoid structure and unique protein-dependent DNA repair mechanisms is responsible for the radioresistant phenotype displayed by the deinococci.

The physical basis for the condensed nucleoid we observe is unknown. We suspect that this level of spatial organization is in large part mediated by proteins that either link copies of the genome together (assuming that a species contains more than one genome copy), or coordinates genome folding in a manner that generates the shapes we have described. For those species, such as D. radiodurans or D. murrayi, in which the nucleoid forms an obvious structure, we envision a protein lattice that acts as a scaffold that the genome is organized around. We predict these proteins are functionally analogous to the SMC (structural maintenance of chromosomes) proteins described in many eukaryotic and prokaryotic species [26-28]. It seems unlikely that genomic DNA is as condensed as the DNA-Dps assemblies described in some stationary phase bacteria [29,30]. These structures are tightly packed, almost crystalline, and it is difficult to envision how an actively metabolizing cell could function under this circumstance; the DNA needs to remain accessible to proteins that catalyze essential housekeeping functions.

We also predict that the ionic composition of the cytosol of the deinococci examined favors the formation of the structures we observe. The Deinococcaceae exhibit unusually high intracellular levels of Mn+2 [18] and it is possible that accumulating this metal creates an environment that facilitates DNA condensation within this species in vivo through direct or indirect mechanisms. In vitro, the condensation of DNA can be achieved by adding a condensing agent, such as a multivalent cation, to an aqueous solution of DNA. The strong electrostatic interaction of the DNA and these cations neutralizes the repulsion of phosphate groups in the DNA backbone, and it has been shown that approximately 90% of the DNA charge must be neutralized for condensation to occur [31]. Intracellular Mn+2 may also indirectly facilitate nucleoid condensation by, for example, augmenting the function of deinococcal DNA-binding proteins. On the other hand, high Mn+2 content may have no affect on nucleoid morphology since, as described above, E. coli can have a condensed nucleoid even though this species has a much lower level of intracellular Mn+2 [18].

Years of experimental evidence irrefutably argue that DNA repair is essential for D. radiodurans recovery from high dose exposure to ionizing radiation, but this fact does not necessarily lead to the conclusion that efficient DNA repair is sufficient for extreme radioresistance. Although there has been a great deal of speculation concerning subtle differences in the properties of DNA repair proteins isolated from D. radiodurans, there has yet to be a convincing demonstration that this species' DNA repair proteins are "better" relative to homologues found in more radiosensitive species. Given this, it remains a formal possibility that D. radiodurans DNA repair proteins function within a molecular environment that enhances their effectiveness. In other words, it seems likely that there are features of deinococcal physiology that augment DNA repair processes, allowing the conventional complement of DNA repair proteins to more efficiently deal with DNA damage. We believe that the images presented here suggest that the genomic DNA of the deinococci is more condensed relative to other species. We suggest that this aggregation is protective, and that it may significantly contribute to the radioresistance of these species by confining the fragments generated subsequent to irradiation and preserving the linear continuity of the damaged genome.

Conclusion

This work resulted in two key observations. First, all evidence obtained is consistent with the notion that the genomes of radioresistant species are more condensed than radiosensitive species. Second, irradiation does not seem to disturb the pattern of condensation observed in the deinococci, even when we examined that pattern in a recA defective strain incapable of repairing DNA double strand breaks. Therefore, in agreement with Levin-Zaidmen et al [16], we assume that the deinococci have the capacity to passively prevent the diffusion of DNA fragments post-irradiation, and that this ability may contribute to the radioresistance of these species.

Materials and methods

Growth conditions

Deinococcus radiodurans R1 (ATCC 13939), Deinococcus radiophilus (ATCC 27603), Deinococcus proteolyticus (ATCC 35074), Deinococcus radiopugnans (ATCC 19172), and Deinococcus grandis (ATCC 43672) were grown in TGY broth at 30°C as described elsewhere [3]. Deinococcus geothermalis (DSM 11300) and Deinococcus murrayi (DSM 11303) were grown in TGY broth at 50°C [17]. Rubrobacter radiotolerans (ATCC 51242) was grown at 30°C in a medium consisting of 1% tryptone, 0.5% yeast extract, 0.5% malt extract, 0.5% casamino acids, 0.2% meat extract, 0.2% glucose, 0.005% Tween 80, and 0.1% magnesium sulfate. Thermus aquaticus YT-1 (ATCC 25104) was grown at 70°C in Castenholz TYE medium (ATCC medium 723). E. coli AB1157 cultures were grown at 37°C in LB medium (1% tryptone, 0.5% yeast extract, and 1% NaCl).

Unless otherwise indicated, all cultures were grown to stationary phase prior to microscopic examination. Cultures were harvested with the following densities as measured by OD600: D. radiodurans, 1.2–1.8; D. radiophilus 1.8–2.2; D. proteolyticus 2.0; D. radiopugnans 1.3–2.0; D. grandis 1.7; D. geothermalis 1.8; D. murrayi 1.3; R. radiotolerans 1.9; T. aquaticus 1.1. These values correspond to cultures with densities between 3 × 108 and 1.3 × 109 CFU/ml.

Microscopy

Cultured cells were stained with N-(3-triethylammoniumpropyl)-4-(6-(4(diethylamino) phenyl)hexatrienyl)pyridinium dibromide, (FM 4–64), and 4',6-Diamidino-2-phenylindole dihydrochloride, (DAPI), for the visualization of the lipid membrane and DNA, respectively. Ratios of the amounts of stationary phase culture cells to fluorescent dyes were a 3:1:1 ratio of culture cells to 0.0625 μg/μL of FM 4–64 solution to 3 μg/mL DAPI solution. The cells were then mounted on slides coated with 0.5% agarose.

Figures 1, 3, 4, 5, 6, 7, and 10 were created by capturing two-dimensional images at a series of points along the z-axis that were set at 100 nm apart. The N2.1 filter cube from Leica Microsystems was used for FM 4–64 detection, which includes a 580 nm longpass dichroic mirror, a 515–560 nm bandpass excitation filter, and a 590 nm long pass emission filter. The A4 filter cube from Leica Microsystems was used for DAPI detection, which includes a 400 nm longpass dichroic mirror, a 360-40 nm bandpass excitation filter, and a 470-40 nm bandpass emission filter. The optical series was deconvolved with Slidebook 4.0 from Intelligent Imaging Innovations, Inc., (Denver, CO), using constrained iterative deconvolution and was then imported into Adobe Photoshop 7.0 as separate two-dimensional images. The two-dimensional images were then arranged in order as depicted.

The projection image in Fig. 11A was achieved with the Slidebook 4.0 software by compiling the stack of two-dimensional images into a single two-dimensional image.

All images were captured using a Leica DMRXA2 microscope and a Sensicam QE camera from The Cooke Corporation, (Auburn Hills, MI). The brightness and contrast of all images were enhanced using Adobe Photoshop 7.0.

Ionizing radiation exposure

Cultures (grown in the appropriate medium) of D. radiodurans (OD600 0.12–0.19), D. radiopugnans (OD600 1.5–1.8), rec30 (OD600 1.4) and E. coli (OD600 0.23) were irradiated to a dose of 5000 Grays using a Model 484R 60Co irradiator (J. L. Sheppard & Associates, San Fernando, CA). Controls were kept at room temperature during irradiation exposure of experimental samples. All samples were incubated at the appropriate conditions immediately after irradiation. All of the cells were harvested after 2 hours of incubation and prepared for microscopy as described above.

Survival curves

Cultures were irradiated using the irradiator described above, and survival established by serial dilution of irradiated cultures and plating on appropriate growth medium. Three independent trials were conducted for each species examined with three replicates per trial. Sigma Plot software was used to create the survival curve.

Authors' contributions

JRB and JMZ conceived and designed the experiments. JMZ performed all of the experimental studies. JRB and JMZ wrote the paper.

Acknowledgements

The authors gratefully acknowledge Margaret C. Henk and David H. Burk of the Socolofsky Microscopy Center within the Department of Biological Sciences at LSU for their assistance and helpful discussions. This work was supported by the U.S. Department of Energy grant DEFG0201ER63151 awarded to J.R.B.

References

  1. Battista JR: Against all odds: the survival strategies of Deinococcus radiodurans.

    Annu Rev Microbiol 1997, 51:203-224. PubMed Abstract | Publisher Full Text OpenURL

  2. Battista JR, Earl AM, Park MJ: Why is Deinococcus radiodurans so resistant to ionizing radiation?

    Trends Microbiol 1999, 7(9):362-365. PubMed Abstract | Publisher Full Text OpenURL

  3. Battista JR, Rainey FA: Phylum BIV. "Deinococcus-Thermus" Family 1. Deinococcaceae Brooks and Murray 1981, 356,vp emend. Rainey, Nobre, Schumann, Stackebrandt and da Costa 1997, 513. In Bergey's Manual of Systematic Bacteriology. Volume 1. 2nd edition. Edited by Boone DR, Castenholz RW. New York , Springer; 2001::395-414. [Garrity George M (Series Editor): The Archaea and the Deeply Branching and Phototrophic Bacteria] OpenURL

  4. Suresh K, Reddy GS, Sengupta S, Shivaji S: Deinococcus indicus sp. nov., an arsenic-resistant bacterium from an aquifer in West Bengal, India.

    Int J Syst Evol Microbiol 2004, 54(Pt 2):457-461. PubMed Abstract | Publisher Full Text OpenURL

  5. Hirsch P, Gallikowski CA, Siebert J, Peissl K, Kroppenstedt R, Schumann P, Stackebrandt E, Anderson R: Deinococcus frigens sp. nov., Deinococcus saxicola sp. nov., and Deinococcus marmoris sp. nov., low temperature and draught-tolerating, UV-resistant bacteria from continental Antarctica.

    Syst Appl Microbiol 2004, 27(6):636-645. PubMed Abstract | Publisher Full Text OpenURL

  6. Ward JF: Molecular mechanisms of radiation-induced damage to nucleic acids.

    Adv Rad Biol 1975, 5:181-239. OpenURL

  7. Krasin F, Hutchinson F: Repair of DNA double-strand breaks in Escherichia coli, which requires recA function and the presence of a duplicate genome.

    J Mol Biol 1977, 116:81-98. PubMed Abstract | Publisher Full Text OpenURL

  8. Daly MJ, Minton KW: Interchromosomal recombination in the extremely radioresistant bacterium Deinococcus radiodurans.

    J Bacteriol 1995, 177(19):5495-5505. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  9. Daly MJ, Minton KW: An alternative pathway of recombination of chromosomal fragments precedes recA-dependent recombination in the radioresistant bacterium Deinococcus radiodurans.

    J Bacteriol 1996, 178(15):4461-4471. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  10. Grimsley JK, Masters CI, Clark EP, Minton KW: Analysis by pulsed-field gel electrophoresis of DNA double-strand breakage and repair in Deinococcus radiodurans and a radiosensitive mutant.

    Int J Radiat Biol 1991, 60(4):613-626. PubMed Abstract | Publisher Full Text OpenURL

  11. Daly MJ, Ouyang L, Fuchs P, Minton KW: In vivo damage and recA-dependent repair of plasmid and chromosomal DNA in the radiation-resistant bacterium Deinococcus radiodurans.

    J Bacteriol 1994, 176(12):3508-3517. PubMed Abstract | PubMed Central Full Text OpenURL

  12. Moseley BE, Copland HJ: Isolation and properties of a recombination-deficient mutant of Micrococcus radiodurans.

    J Bacteriol 1975, 121(2):422-428. PubMed Abstract | PubMed Central Full Text OpenURL

  13. Hansen MT: Multiplicity of genome equivalents in the radiation-resistant bacterium Micrococcus radiodurans.

    J Bacteriol 1978, 134(1):71-75. PubMed Abstract | PubMed Central Full Text OpenURL

  14. Harsojo, Kitayama S, Matsuyama A: Genome multiplicity and radiation resistance in Micrococcus radiodurans.

    J Biochem (Tokyo) 1981, 90(3):877-880. PubMed Abstract OpenURL

  15. Minton KW, Daly MJ: A model for repair of radiation-induced DNA double-strand breaks in the extreme radiophile Deinococcus radiodurans.

    Bioessays 1995, 17(5):457-464. PubMed Abstract | Publisher Full Text OpenURL

  16. Levin-Zaidman S, Englander J, Shimoni E, Sharma AK, Minton KW, Minsky A: Ringlike structure of the Deinococcus radiodurans genome: a key to radioresistance?

    Science 2003, 299(5604):254-256. PubMed Abstract | Publisher Full Text OpenURL

  17. Ferreira AC, Nobre MF, Moore E, Rainey FA, Battista JR, da Costa MS: Characterization and radiation resistance of new isolates of Rubrobacter radiotolerans and Rubrobacter xylanophilus.

    Extremophiles 1999, 3(4):235-238. PubMed Abstract | Publisher Full Text OpenURL

  18. Daly MJ, Gaidamakova EK, Matrosova VY, Vasilenko A, Zhai M, Venkateswaran A, Hess M, Omelchenko MV, Kostandarithes HM, Makarova KS, Wackett LP, Fredrickson JK, Ghosal D: Accumulation of Mn(II) in Deinococcus radiodurans Facilitates Gamma-Radiation Resistance.

    Science 2004. OpenURL

  19. Englander J, Klein E, Brumfeld V, Sharma AK, Doherty AJ, Minsky A: DNA toroids: framework for DNA repair in Deinococcus radiodurans and in germinating bacterial spores.

    J Bacteriol 2004, 186(18):5973-5977. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  20. Mattimore V, Udupa KS, Berne GA, Battista JR: Genetic characterization of forty ionizing radiation-sensitive strains of Deinococcus radiodurans: linkage information from transformation.

    J Bacteriol 1995, 177(18):5232-5237. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  21. Pollard EC, Kraus K: All-or-nothing character of DNA degradation in bacteria after ionizing radiation.

    Biophys J 1973, 13(4):332-339. PubMed Abstract OpenURL

  22. Ferreira AC, Nobre MF, Rainey FA, Silva MT, Wait R, Burghardt J, Chung AP, da Costa MS: Deinococcus geothermalis sp. nov. and Deinococcus murrayi sp. nov., two extremely radiation-resistant and slightly thermophilic species from hot springs.

    Int J Syst Bacteriol 1997, 47(4):939-947. PubMed Abstract OpenURL

  23. Davis NS, Silverman GJ, Mausurosky EB: Radiation resistant, pigmented coccus isolated from Haddock tissue.

    J Bacteriol 1963, 86:294-298. PubMed Abstract | PubMed Central Full Text OpenURL

  24. Bohrmann B, Villiger W, Johansen R, Kellenberger E: Coralline shape of the bacterial nucleoid after cryofixation.

    J Bacteriol 1991, 173(10):3149-3158. PubMed Abstract | PubMed Central Full Text OpenURL

  25. Niki H, Yamaichi Y, Hiraga S: Dynamic organization of chromosomal DNA in Escherichia coli.

    Genes Dev 2000, 14(2):212-223. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  26. Cobbe N, Heck MM: Review: SMCs in the world of chromosome biology- from prokaryotes to higher eukaryotes.

    J Struct Biol 2000, 129(2-3):123-143. PubMed Abstract | Publisher Full Text OpenURL

  27. Jessberger R: SMC proteins at the crossroads of diverse chromosomal processes.

    IUBMB Life 2003, 55(12):643-652. PubMed Abstract OpenURL

  28. Volkov A, Mascarenhas J, Andrei-Selmer C, Ulrich HD, Graumann PL: A prokaryotic condensin/cohesin-like complex can actively compact chromosomes from a single position on the nucleoid and binds to DNA as a ring-like structure.

    Mol Cell Biol 2003, 23(16):5638-5650. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  29. Frenkiel-Krispin D, Levin-Zaidman S, Shimoni E, Wolf SG, Wachtel EJ, Arad T, Finkel SE, Kolter R, Minsky A: Regulated phase transitions of bacterial chromatin: a non-enzymatic pathway for generic DNA protection.

    Embo J 2001, 20(5):1184-1191. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  30. Wolf SG, Frenkiel D, Arad T, Finkel SE, Kolter R, Minsky A: DNA protection by stress-induced biocrystallization.

    Nature 1999, 400(6739):83-85. PubMed Abstract | Publisher Full Text OpenURL

  31. Wilson RW, Bloomfield VA: Counterion-induced condesation of deoxyribonucleic acid. a light-scattering study.

    Biochemistry 1979, 18(11):2192-2196. PubMed Abstract | Publisher Full Text OpenURL