Journal of Bacteriology, January 2003, p . 693-697, Vol . 185, No . 2

Polar Targeting of DivIVA in Bacillus subtilis Is Not Directly Dependent on FtsZ or PBP 2B

Leendert W . Hamoen and Jeffery Errington^*

Sir William Dunn School of Pathology, University of Oxford, Oxford OX1 3RE, United Kingdom

Received 29 July 2002/ Accepted 28 October 2002

During cell division, DivIVA is recruited to the newly formed Z ring, and after septation is completed and the Z ring dissolves, DivIVA remains attached to the newly formed cell poles (5) . FtsZ is an essential protein, but in a B . subtilis mutant in which the concentration of FtsZ can be regulated, depletion of FtsZ prevents accumulation of DivIVA at the potential division site, as no Z rings are formed (12) . Under these conditions, DivIVA remains present at the cell poles . On the basis of this experiment, it was postulated that FtsZ is involved in recruiting DivIVA to the newly formed septum and therefore is required for polar positioning of DivIVA . In such a scenario, DivIVA is retained at the poles by a mechanism independent of the presence or absence of FtsZ . However, since DivIVA was already present at the poles, this experiment did not prove that FtsZ itself is essential for the polar positioning of DivIVA . It remains possible that a certain factor associated with the polar regions of the cell is the determinant for the localization of DivIVA and that this factor depends on the formation of a polar region, a process that normally depends on cell division and therefore on the presence of FtsZ . To address this issue, we needed a system in which the presence of a cell pole is not directly linked to the preceding formation of a Z ring . In B . subtilis, such a situation is found in the germinating spore . Spores are very compact structures developed to survive extremely inhospitable environmental conditions . The chromosome is compressed into a ring-like structure, and no replication or Z ring or other cytokinesis apparatus is likely to be present in the dormant spore (16) . When spores germinate, they start to swell and burst out of their rigid spore coats . They then elongate to normal-sized cells before cell division starts . Since outgrowing spores divide like normal vegetatively growing cells, DivIVA (and the MinC/MinD protein couple) should be present at the cellular extremities from an early stage . However, there is no Z ring present at the poles of germinating spores to which DivIVA can attach . Thus, the normal division of outgrowing spores suggests that FtsZ is not essential for the polar positioning of DivIVA . We set out to investigate this supposition by monitoring the localization of a DivIVA-green fluorescent protein (GFP) fusion during germination of spores from a wild-type B . subtilis strain and a strain in which FtsZ can be depleted .

Localization of DivIVA in outgrowing spores. Before we could start with fluorescence microscopy studies of germinating B . subtilis spores, we had to overcome an important obstacle, namely, the strong autofluorescence of the spore coat . The spore coat tends to snap in half and stay attached to the poles of the outgrowing spore, as a consequence of which the fluorescence of pole-localized GFP fusion proteins is masked . We tried several extraction procedures to reduce the autofluorescence of the spore coat but with no success . However, treatment of spores with sodium dodecyl sulfate (SDS) under strong reducing conditions, a procedure normally used to extract certain spore coat proteins, appeared to be useful (19) . After such extraction, outgrowing spores detached much more easily from the enveloping spore coat . Unfortunately, such extraction decreases the efficiency of germination . We discovered that the addition of the detergent Tween 20 to the growth medium substantially stimulated germination and countered the adverse effects of SDS extraction . With these adjustments, the complete procedure for spore isolation, extraction, and germination was as follows . Schaeffer's sporulation medium (8) was inoculated with B . subtilis strain 1803 (containing a divIVA-gfp reporter fusion under the transcriptional control of the divIVA promoter) (Table 1) . This strain was used in previous studies to examine the localization of DivIVA (17) . Spores were collected by centrifugation and washed in TES buffer (10 mM Tris-HCl [pH 8], 1 mM EDTA, 1 M NaCl) . The pellet was resuspended in water and incubated with lysozyme (0.1 mg/ml) for 1 h at 37°C . After this, DNase (20 µg/ml), RNase (20 µg/ml), and SDS (0.5%) were added and incubation was continued for another hour . Next, spores were washed once with TES buffer and three times with 0.01% Tween 20 and stored at -80°C . Washed spores were extracted in a solution of 10 mM Tris-HCl, 0.5% SDS, 10 mM dithiothreitol, and 100 mM NaCl for 1 h at 37°C . After this extraction, the spores were washed six times with 0.01% Tween 20 . Spores were diluted in germination medium to an optical density at 600 nm (OD₆₀₀) of 1 . The germination medium consisted of S medium (chosen for its low-fluorescence background signal) supplemented with the germinant alanine (10 mM) (8) and Tween 20 (0.002%) (12) . To increase the germination efficiency, spores were heat shocked for 30 min at 70°C (19) . After heat shock, the spore mixture was incubated at 30°C under continuous shaking . At different time intervals, samples were taken for fluorescence microscopy examination . Outgrowing spores were viewed on agarose slides, and images were obtained as described by Marston and Errington (11) . Figure 1 shows a compilation of the different stages of outgrowing spores as observed by fluorescence microscopy . DivIVA-GFP appears as fluorescent dots concentrated at the cell poles . During growth of the cell, more DivIVA-GFP spots emerge at the periphery of the cell, and when cytokinesis starts, DivIVA-GFP concentrates at the site of division . The localized concentrations of DivIVA-GFP are presumably a consequence of oligomerization of DivIVA (13) . Thomaides et al . (17) have reported that DivIVA is not targeted to the asymmetric sporulation septum . Since DivIVA-GFP is observed at both cell poles of germinating spores, the possibility that small amounts of old DivIVA molecules, remaining from the prespore, serve as polar attachment sites for newly synthesized DivIVA is unlikely .

 
Localization of DivIVA in the absence of FtsZ or PBP 2B. As indicated in the lower half of the top panel of Fig . 1, DivIVA-GFP appears to be present at the cell poles during the early stages of germination prior to Z-ring formation, suggesting that polar positioning of DivIVA does not depend on the presence of FtsZ . To corroborate this supposition, we isolated spores from B . subtilis strain 3291, which contains an IPTG (isopropyl-ß-D-thiogalactopyranoside)-inducible allele of ftsZ . This strain was constructed by chromosomal transformation, and the genetic characteristics of this strain are described in Table 1 . Spore isolation, extraction, and germination were performed as described above, except that 1 mM IPTG was present in the sporulation medium but absent from the germination medium . No FtsZ could be detected in germinating spores when analyzed by Western blotting using polyclonal anti-FtsZ serum (3) (Fig . 2) . The subsequent germination stages displayed in Fig . 1 indicate that repression of FtsZ does not hamper the outgrowth of the spores, but it did completely block cell division . Again, DivIVA-GFP accumulated strongly at the cell poles, indicating that FtsZ is indeed not essential for polar disposition of DivIVA .

 
In addition to FtsZ, recruitment of DivIVA to the site of division requires other septal division proteins such as DivIB and DivIC (12) . Depletion of PBP 2B, which catalyses the final stages of peptidoglycan synthesis in the septum, also prevents targeting of DivIVA to the site of division (H . B . Thomaides and J . Errington, unpublished data) . The finding that targeting of PBP 2B to the cell division site depends on the formation of the Z ring, and the observation that some PBP 2B remains present at the newly formed cell poles, led Daniel et al . (4) to suggest that PBP 2B might be the immediate target for DivIVA . To test this hypothesis, we introduced an IPTG-inducible allele of pbpB into strain 1803 (creating strain 3294) (Table 1) . Spores were isolated and germinated as described for strain 3291 . Immunodetection using polyclonal anti-PBP 2B serum was used to check the absence of detectable amounts of PBP 2B in germinating spores from the mutant strain (Fig . 2) . The findings presented in the lower-middle panel in Fig . 1 indicate that it is unlikely that PBP 2B is the immediate target for DivIVA, as DivIVA still accumulated at the extremities of outgrowing spores in aseptate filaments containing undetectable levels of PBP 2B . Therefore, polar targeting of DivIVA appears to be not directly dependent on the presence of either FtsZ or PBP 2B; the normal requirement for these proteins probably arises only through their role in formation of the new cell pole .

Localization of DivIVA in the absence of the cytoskeletal element Mbl or MreB. Several mechanisms can be envisioned as explanations of how DivIVA accumulates at the cell poles . Passive diffusion combined with a polar capture mechanism is one possibility . Alternatively, DivIVA might migrate to the cell poles by an active mechanism, much like that operating in eukaryotes in which the cytoskeleton guides proteins to their proper locations in the cell . With the recent discovery of two new cytoskeletal elements in B . subtilis, Mbl and MreB, the possibility that an active mechanism is involved became more likely (9) . Mbl forms a double-helix structure along the periphery of the cell, and the helical filaments run through almost the entire length of the cell . MreB forms helical filaments that encircle the cell at midcell . Mbl and MreB are similar in primary structure, and both show some homology with the actin superfamily (2, 9, 18) . It is assumed that these two proteins form an actin-like cytoskeletal structure which determines the shape of the bacterium, since absence of one of the two results in a strong deformation in cell shape . Both proteins are conserved in rod-shaped bacteria, but they are missing in the cocci . How these cytoskeletal components control cell shape is unknown . By analogy with the function of actin in yeast, Jones et al . (9) postulated that the Mbl and MreB helical filaments control the spatial distribution of the cell-wall-synthesizing machinery . Potentially, these cytoskeletal elements might also control polar positioning of DivIVA .

By means of chromosomal transformation, we constructed an mbl-knockout mutant containing a divIVA-gfp reporter fusion (strain 3293) (Table 1) . The absence of Mbl from this strain was checked by Western blotting using polyclonal anti-Mbl serum (Fig . 2) (9) . Strain 3293 is still able to sporulate (1), and spores were isolated and treated as described above . The results depicted in Fig . 1 indicate that spores from an mbl-knockout mutant germinate normally, and accumulation of DivIVA-GFP at the cell poles was not affected by the mutation . The characteristic cell deformation linked to an mbl mutation was not very evident in the germination medium we used . A proportion of cells started to show a bulging appearance (e.g., rightmost image in the bottom panel of Fig . 1) only after cell division had taken place . This distortion of cell shape did not appear to influence DivIVA-GFP localization . A comparable result was found when B . subtilis cells were depleted of MreB . Since MreB is an essential protein, we had to resort to the use of a B . subtilis strain containing mreB under transcriptional control of the repressible P_xyl promoter (strain 3292) (Table 1) . However, Western blotting analysis using polyclonal anti-MreB serum indicated that repression of the P_xyl promoter was insufficient during the early stages of germination (Fig . 2) . Therefore, the dependence of polar DivIVA positioning on the presence of MreB could not be studied in outgrowing spores, and we employed an MreB-depletion protocol essentially as described by Jones et al . (9) . B . subtilis strain 3292 was grown overnight on a nutrient agar plate containing 1% xylose . A colony from this plate was used to inoculate Spizizen's minimal medium without xylose (8) . To ensure that cells went through several rounds of cell division in the absence of MreB, the culture was diluted another 100-fold after reaching an OD₆₀₀ of about 0.5 . When the diluted culture reached an OD₆₀₀ of about 1, cells were collected for Western blotting and fluorescence microscopy analyses . No MreB was detectable by immunodetection (Fig . 2), and many cells showed a deformed morphology, as shown in Fig . 3 . Despite the absence of normal concentrations of MreB, DivIVA-GFP accumulated at the division septa and cell poles even when the poles were deformed . Thus, polar as well as septal positioning of DivIVA does not seem to depend on the presence of MreB or Mbl .

 
In conclusion, we have shown that the formation of septa is not an essential step in the polar positioning of DivIVA . It is therefore unlikely that the positioning process can be simply subdivided into two steps, namely, binding of DivIVA to a component of the cell division septum followed by a mechanism that retains DivIVA at the newly formed poles . Our new results favor a mechanism in which DivIVA is directly recruited to the (newly formed) cell poles . Edwards et al . (6) showed that polar targeting of DivIVA is in fact a rather promiscuous process and that it can be observed in E . coli and even in the fission yeast Schizosaccharomyces pombe . The mechanism behind the apparent general affinity of DivIVA for cell poles remains unclear; at least, the cytoskeletal proteins MreB and Mbl appear not to be involved .

This research was supported by an EMBO long-term fellowship awarded to L . Hamoen and a grant from the U.K . Biotechnology and Biological Science Research Council .

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