Department of Developmental Biology and Neurosciences, Graduate School of Life Sciences, Tohoku University, Aoba, Sendai 980-8578, Japan
* Author for correspondence (e-mail: ymaeda{at}mail.tains.tohoku.ac.jp)
Accepted 30 January 2004
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Summary |
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Key words: Mitochondrial DNA, Rho-depleted cells, Growth, Differentiation, Pattern formation, Phototaxis, Dictyostelium
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Introduction |
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D. discoideum Ax-2 cells grow axenically as free-living cells and multiply by mitotic fission with a doubling time of about 7.5 hours, pinocytosing external nutrients. The differentiation phase is induced by nutritional deprivation, and starving cells gather together forming streams in response to pulsatile emissions of cAMP from the aggregation center (Konijin et al., 1967; Bonner, 1970
). The cell aggregate assumes a hemispherical structure (mound). Subsequently, a tip arises at the apex of the mound, elongates and forms a migrating slug. At the slug stage, there is clear zonal differentiation along the long axis, with anterior prestalk cells (pst) and posterior prespore cells (psp). In differentiating prespore cells, there arise unique vacuoles called prespore-specific vacuoles (PSVs) (Maeda and Takeuchi, 1969
; Hohl and Hamamoto, 1969
). The PSV has been shown to be constructed from a mitochondrion with the help of the Golgi complex (Matsuyama and Maeda, 1998
). During culmination, the prestalk cells of a slug differentiate into stalk cells, while the prespore cells differentiate into spores. The proportion of the two cell types (the number-ratio of pst/psp in the slug or stalk cells/spores in the fruiting body) is usually constant, with a 2.5-fold tolerance range (Rafols et al., 2000
). The growth and differentiation phases in this organism are temporally separated from each other and easily controlled by nutritional conditions. In addition, the developmental system is relatively simple compared with that in other organisms. Moreover, a particular checkpoint (referred to as a PS-point) from growth to differentiation phase has been precisely specified in the mid-late G2 phase of the cell cycle (Maeda et al., 1989
). This is the point from which cells initiate differentiation when placed under conditions of nutritional deprivation. Thus, Dictyostelium development offers us a particularly useful system for elucidating the cellular and molecular mechanisms of the growth/differentiation transition (GDT), pattern formation in cell masses and a variety of other problems of current interest in developmental biology.
As previously presented, the dia3 gene, which encodes a mitochondrial protein cluster including ribosomal protein S4 (RPS4), is expressed specifically during the GDT of Ax-2 cells: its overexpression enhances the progress of cell differentiation, while its partial inativation by means of homologous recombination greatly impairs differentiation and morphogenesis after starvation (Inazu et al., 1999). In differentiating prespore cells, the mitochondrion exerts a remarkable structural transformation to form a sort of vacuole (M-vacuole), in which PSV, a cell-type-specific organelle (Maeda and Takeuchi, 1969
; Hohl and Hamamoto, 1969
), is constructed with the help of the Golgi complex (Matsuyama and Maeda, 1998
). Mitochondrial cyanide (CN)-resistant respiration has been shown to be tightly involved in cell-type proportioning (e.g. the ratio of prestalk/prespore cells in a slug or stalk cells/spores in a sorocarp): application of specific inhibitors of CN-resistant respiration to starved Dictyostelium cells induces the formation of unique cell masses, in which almost all of the cells differentiate into prestalk cells and then stalk cells, thus being completely devoid of prespore and spore differentiation (Matsuyama and Maeda, 1995
). The large subunit (mt-lrRNA) of Dictyostelium mitochondrial rRNA is also essential for phototaxis and thermotaxis of the migrating slug (Wilczynska et al., 1997
). Taken together, these data offer indications of the dynamic involvements of mitochondria and mitochondrial DNA in a variety of processes during Dictyostelium development.
The mitochondrial genome (mtDNA) of D. discoideum consists of 55,564 bp of nucleotides that encode two rRNAs, ten subunits of the NADH dehydrogenase complex (NAD 1, 2, 3, 4, 4L, 5, 6, 7, 9 and 11), apocytochrome b (cyt b), three subunits of the cytochrome oxidase (COX1/2 and 3), four subunits of the ATP synthase complex (APT1, 6, 8 and 9), 15 ribosomal proteins and five other open reading frames (ORFs), excluding intronic ORFs (essential peptides of enzymes for oxidative phosphorylation, three rRNAs and 18 tRNAs) (Gray et al., 1998; Ogawa et al., 2000
). Mitochondria and mtDNA are believed to be closely associated with cell growth, because mitochondria are organelles that produce chemical energy in the form of ATP (Kotsifas et al., 2003; Zhu et al., 1997
). Ethidium bromide (EtBr) is known to be a potent inhibitor of mtDNA replication and transcription in mammalian cultured cells (Nass, 1970
; Leibowitz, 1971
; Zylber et al., 1969
) and avian cultured cells (Desjardins et al., 1985
; Desjardins et al., 1989
), but it does not substantially affect the synthesis of nuclear DNA (Radask et al., 1971; Nass, 1972
; Leblond-Larouche et al., 1979
). In cultures of Dictyostelium Ax-3 cells, EtBr actually inhibits any new synthesis of mtDNA (Firtel and Bonner, 1972
; Kobilinsky and Beattie, 1977
), and growth of Ax-3 cells stops after one or two generations in the presence of 10 µg/ml EtBr (Stuchell et al., 1973
). The creation of cells completely lacking mtDNA, termed
0 or rho0 cells, by repeated cell division in the presence of EtBr, has been achieved in both mammalian and avian cell cultures. In this study, in order to elucidate possible involvements of mtDNA in Dictyostelium development, we aimed to prepare
0 cells from D. discoideum Ax-2 cells, by means of their exposure to EtBr in axenic growth medium. In Dictyostelium cells, it proved to be difficult to create complete
0 cells, presumably because of the prerequisite of mtDNA for cell growth. However, we succeeded in preparing
0-like cells with about 1/4 of mtDNA compared with that of Ax-2 cells. In the remainder of this article we refer to these cells as
or rho-depleted cells. Fascinating phenotypes of these
cells are described, and possible roles of mtDNA in Dictyostelium development are discussed, with special emphasis on cell differentiation and pattern formation.
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Materials and Methods |
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Preparation of cells
Exponentially growing cells (2-5x106 cells/ml) were transferred to fresh PS medium containing various concentrations of ethidium bromide (EtBr) at a density of 2-5x105 cells/ml, followed by shake culture at 22°C in the dark. For this, culture flasks were covered with aluminum foil. Under this culture condition, cells with a reduced amount of mtDNA were found to arise after about two times of cell division in PS medium containing 30 µg/ml of EtBr, as presented later.
Developmental conditions
To allow cells to differentiate, exponentially growing cells were harvested, washed twice in Bonner's salt solution (BSS; 0.6 g NaCl, 0.75 g KCl, 0.3 g CaCl2, 1000 ml distilled deionized water) (Bonner, 1947) as starvation medium, and incubated either on agar at a density of 5x106 cells/cm2 or in a 24-well plate (Falcon, #3047) under submerged conditions at a density of 5x105 cells/cm2 (1 ml cell suspension/well) at 22°C. To obtain migrating slugs, starved cells were suspended in BSS at a density of about 2.5x107 cells/ml and aliquots (2 ml) of the cell suspension were plated on 1.5% agar in 9 cm glass dishes and incubated at 22°C for 18-48 hours. Slugs that had migrated out of the original streaks were used for subsequent histochemical staining of ß-gal activity and immunocytochemical detection of PSVs. In another experiments, starving cells were plated at a density of about 1.5x106 cells/cm2 on white Millipore filters (HAWP; Nihon Millipore) placed on 1.5% non-nutrient agar in 9 cm glass dishes and incubated at 22°C for 18-48 hours.
Immunocytochemical detection of prespore-specific vacuoles (PSVs)
Slugs migrating on 1.5% non-nutrient agar were collected by centrifugation and disaggregated by 1% pronase E (Merck, NJ) and 25 mM 2,3-dimercapto-1-propanol (BAL; Wako Chemical, Japan) dissolved in 50 mM Tris-HCl buffer (pH 7.0) for 15 minutes with intermittent pipetting (Takeuchi and Yabuno, 1970). The dissociated cells were washed three times in BSS, pre-fixed in ice-cold 50% methanol and fixed in absolute methanol for 10 minutes on an ice-bath. The fixed cells were dried on cleaned coverslips. They were dipped in PBS (140 mM NaCl, 3 mM KCl, 10 mM Na2HPO4, 2 mM K2HPO4, pH 7.2) for 5 minutes and stained with FITC-conjugated anti-D. mucoroides spore IgG in a moisture chamber for 45 minutes at room temperature, according to the method of Takeuchi (Takeuchi, 1963
). The sample was washed three times in PBS (5 minutes for each) and mounted in PBS containing 20% glycerol. The percentage of cells (prespore cells) with stained PSVs to the total cells examined was determined under a fluorescence microscope.
Histochemical staining of ß-galactosidase activity
Cell masses of the transformants (pEcmAO-gal or pD19-gal cells) were fixed and stained for ß-gal activity according to a modification of the method described previously (Dingermann et al., 1989). Filters on which slugs had been formed were floated on Z-buffer containing 0.1% glutaraldehyde (GA) and 0.1% TritonX-100 (TX-100) for 5 minutes and then submerged in the same solution for 10 minutes. After two washings in Z-buffer, the preparations were incubated at 37°C in the staining solution (5 mM of both K3[Fe(CN)4] and K4[Fe(CN3)]; 1 mM X-gal; in Z buffer) for ß-gal activity. The staining was stopped by washing in Z buffer and the stained slugs were photographed in color under a binocular microscope. To determine the cell types at a single-cell level, slugs were dissociated by pronase-BAL, washed three times in BSS and incubated on cleaned coverslips for 20 minutes at 22°C in a moisture. Cells adhering on the coverslip were fixed by two changes of Z-buffer containing 0.05% GA and 0.1% TX-100, and stained as described above. The cell type (PstAO cells or prespore cells) of dissociated slug cells was determined by counting the ratio of stained/nonstained cells under an optical microscope (Optiphot; Nikon & Co., Tokyo, Japan).
Staining of cells with a DNA-specific dye, DAPI
The vegetatively growing cells were washed twice with BSS by centrifugation at 400 g for 1 minute. Subsequently, ice-cold absolute methanol was poured into the cells suspended in BSS and centrifuged. The cells were resuspended in ice-cold absolute methanol. After centrifugation, the cells were suspended in 0.5 ml of ice-cold absolute methanol and fixed for 10 minutes on ice. Three to four drops of the cell suspension in methanol were put on a cleaned coverslip and dried. Staining of the fixed cells with DAPI was done as described previously (Leeman and Ruch, 1982; Maeda, 1986
). The stained cells were observed under a fluorescence microscope.
Staining of cells with a mitochondrion-selective dye, MitoTracker Orange
The vegetatively growing cells were incubated in PS medium containing 0.5 µM MitoTracker Orange CMTMRos (Molecular Probes) for 30 minutes at room temperature. The stained cells were washed twice with BSS. One drop of the cell suspension was put on a cleaned coverslip and cells were fixed with 3.7% formaldehyde in 20 mM Na/K phosphate buffer (pH 7.2) for 20 minutes. Subsequently, the cells were washed with PBS, basically according to the method of Morita et al. (Morita et al., 2002). The stained cells were observed under a fluorescence microscope.
Isolation of genomic DNAs and Southern blot analysis
Genomic DNAs were extracted by the method described by Nellen et al. (Nellen et al., 1987). Genomic Southern hybridization was performed using the Southern method (Southern, 1975
) with a slight modification. Three to four micrograms of genomic DNA were extracted from the same number of EtBr (40 hours)-treated cells and nontreated cells, digested with appropriate restriction endonucleases and electrophoresed in 0.7% agarose gel. Before blotting, the gel was treated with 0.25 mM HCl for 10 minutes, and then with 0.5 mM NaOH and 1.5 mM NaCl for 30 minutes. The size-fractionated genomic DNA fragments were transferred to a nylon membrane and blotted for hybridization to the rps4 cDNA probe or Dd-TRAP1 cDNA probe that had been 32P-labeled using a MegaprimeTM DNA labeling system (Amersham). The membrane was baked for 2 hours at 80°C to immobilize DNA and was stored at 4°C. Prehybridization was carried out at 65°C for 2 hours in a solution containing 5 x Denhardt solution [0.02% Ficoll-400, 0.02% bovine serum albumin (BSA), and 0.02% polyvinylpyrrolidone], 5xSSPE (43.8 g NaCl, 6.9 g NaH2PO4·12H2O and 1.85 g EDTA; pH 7.4) or 5xSSC (43.8 g NaCl and 22.05 g sodium citrate), 0.5% sodium dodecyl sulfate (SDS) and 20-100 µg of denatured salmon sperm DNA per ml. Hybridization was carried out at 65°C for 20 hours in the same solution containing the 32P-labeled cDNA probe by use of the MegaprimeTM DNA labeling system. The membranes were washed twice with a washing solution (1xSSC and 0.1% SDS) at room temperature for 15 minutes and then twice with a solution (0.1xSSC and 0.1% SDS) at 65°C for 5-10 minutes. The membranes were exposed to X-ray films for 2 days at 80°C.
Electron microscopy
The vegetatively growing Ax-2 and cells were fixed in 1% solution of osmium tetraoxide (OsO4) dissolved in BSS for 8 minutes at room temperature as described previously (Abe and Maeda, 1991
). During subsequent dehydration in a graded series of ethanol (50%, 70%, 90%, 95% and 100%), specimens were prestained with uranyl acetate saturated in 50% ethanol for 2 hours at room temperature and were embedded in an epoxy resin, Epok-812 (Oken Shoji, Japan). After polymerization of the resin, ultrathin sections (60-80 nm thick) were cut with a Reichert-Nissei Ultracut S (VIM 535). The sections were stained with lead citrate according to Reynolds (Reynolds, 1963
) and were observed with a Hitachi transmission electron microscope (H-8100).
Assay of phototaxis
For a phototaxis assay, a slight modification of the method of Fisher et al. (Fisher et al., 1981) was applied. Starved Ax-2 cells and EtBr-treated cells were incubated for 24-48 hours on 1.5% non-nutrient agar to allow slug formation. After incubation with a lateral light source at 22°C for 24-48 hours, slugs migrated over the agar surface leaving behind the usual trail of collapsed slime sheath. The plates were inspected and scored for normal or defective phototaxis described previously (Fisher et al., 1981
). Trails of slugs were transferred to PVC discs, stained and digitized as described previously (Fisher et al., 1981
), and then plotted from a common origin.
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Results |
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Creation of cells
To estimate approximately the amount of mtDNA in Ax-2 cells treated with various concentrations of EtBr, cells were stained with DAPI 40 hours after exposure to EtBr to measure mtDNA. As a result, cells exposed to lower (0.1-25 µg/ml) or higher concentrations (40-50 µg/ml) of EtBr were found to have DAPI-stained mitochondria, like those in nontreated cells. In the presence of 30 µg/ml EtBr, however, cells that had divided for about two generations exhibited markedly reduced staining of mitochondria with DAPI in contrast to normal staining of nuclei, thus indicating a selective decrease of mtDNA (Fig. 2C). There were no significant differences in the size of nucleus and the ratio of multinucleate cells to mononucleate cells between 30 µg/ml EtBr-treated and nontreated Ax-2 cells.
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The mitochondrial membrane potential has been shown to be transiently reduced in 0 cells derived from several cell lines, as monitored by the staining of cells with MitoTracker Orange. To find out whether mitochondria in Ax-2 cells treated with 30 µg/ml EtBr for 40 hours had any membrane potential, they were vitally stained with MitoTracker. The result showed that some of mitochondria contained in the EtBr-treated cells exhibited rather stronger staining (Fig. 2D) compared with that in nontreated Ax-2 cells (Fig. 2B), suggesting that in a limited number of mitochondria their membrane potential is increased by EtBr-treatment in Dictyostelium cells.
To confirm that the amount of mtDNA is selectively decreased in response to treatment of Ax-2 cells with 30 µg/ml of EtBr, Southern blot analysis was carried out, using a nuclear DNA-specific probe (Dd-trap1; Dictyostelium homologue of trap1) and a mtDNA-specific probe (mitochondrial rps4). For this, total cellular DNAs were prepared from the same number of EtBr (40 hours)-treated cells and nontreated cells, digested with several restriction enzymes and compared after Southern blottings (Fig. 3). Here it is important to note that mtDNA is selectively reduced in the EtBr-treated cells, which is consistent with the result of DAPI staining shown in Fig. 2. The EtBr treatment seemed to have little effect on the amount of nuclear DNA. From densitometric measurements of the autoradiograms obtained, the amount of mtDNA in the EtBr-treated cells was estimated to be about 1/4 of that in nontreated Ax-2 cells. One can explain well the reduced value of mtDNA in the EtBr-treated cell, provided that the synthesis of mtDNA during two cell-doublings in the presence of 30 µg/ml of EtBr is selectively and completely inhibited by EtBr. From another point of view, it is most likely that a certain amount of mtDNA (presumably more than 1/4 of original mtDNA) may be required to maintain cellular activities including growth. In other words, it might be impossible to create cells that have no mtDNA (0 cells) using Dictyostelium cells. Therefore, the EtBr-treated cells with about 1/4 of mtDNA were used in further experiments, as
cells.
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Ultrastructural features of cells
Electron microscopic observations of cells and vegetatively growing Ax-2 cells revealed some characteristic differences between them. As was expected, the most striking difference was the morphology of the mitochondria; in
cells many of the mitochondria exhibited marked structural transformation to form a sort of vacuole, engulfing the nearby cytoplasm (Fig. 4B,D). We previously reported that somewhat similar mitochondrial transformation occurred in differentiating prespore cells just before PSV formation (Matsuyama and Maeda, 1998
). Nontreated Ax-2 cells contained normal-shaped mitochondria with reticular cisternae and an electron-opaque matrix, as shown in Fig. 4A,C. Incidentally, Kobilinsky and Beattie (Kobilinsky and Beattie, 1977
) have reported the EtBr (10 µg/ml)-induced mitochondrial transformation in D. discoideum Ax-3 cells.
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Decreased mtDNA causes delayed differentiation and abnormal morphogenesis
When Ax-2 cells were harvested at the exponential growth phase, washed and incubated on agar, they formed aggregation streams after 6 hours and mounds after 12 hours of incubation at 22°C (Fig. 5A). Subsequently, a tip was formed at the apex of each mound, which elongated and formed a migrating slug after 16 hours of incubation. This was followed by the formation of a fruiting body at about 26 hours of incubation. By contrast, cells exhibited delayed and somewhat abnormal morphogenesis; large aggregation streams were formed after 16 hours of incubation, followed by their subdivision to smaller cell masses (Fig. 5A). After a prolonged time (about 48 hours) of incubation,
cells formed irregular-shaped slugs, but failed to develop to fruiting bodies (Fig. 5B). Another experiment revealed that Ax-2 cells treated with lower concentrations (15, 20 or 25 µg/ml) of EtBr for 40 hours at the growth phase had almost the same amount of mtDNA as that of nontreated Ax-2 cells, after DAPI staining, and that they exhibited normal development after starvation. Also, when Ax-2 cells were harvested and starved either on 1.5% non-nutrient agar or in BSS, both of which contained 30 µg/ml of EtBr, they showed normal development without any loss of mtDNA.
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More striking delay of differentiation was observed in cells starving under submerged conditions. Most
cells showed no sign of cell aggregation and remained as round-shaped single cells even after 12 hours of incubation, while nontreated Ax-2 cells acquired aggregation-competence and began to aggregate at 7 hours of incubation, which was followed by the formation of tight mounds during 12-24 hours of incubation (Fig. 6). By contrast,
cells formed large aggregation streams at 24 hours, which were then subdivided into smaller mounds during another 4 hours of incubation, principally as the case on agar (Fig. 6).
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The genes car1 (for cAMP receptor 1), csA (for contact site A) and rps4 (for mitochondrial ribosomal protein subunit 4) have been shown to be specifically expressed after starvation, coupling with the initiation of cell differentiation. So, we examined expression patterns of these marker genes in EtBr-treated () cells and nontreated Ax-2 cells and compared them. As a result, expression of all of the genes was found to be significantly delayed and reduced in
cells, being consistent with the delay in their development after starvation (Fig. 7).
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cells exhibit almost normal respiration and chemotaxis to folic acid
In spite of greatly reduced mtDNA in cells, measurements of O2 consumption using the O2 electrode revealed the respiration rate of
cells at the growth phase to be almost normal (about 90% of that of nontreated Ax-2) (data not shown). More importantly,
cells were found to exhibit completely normal chemotactic movement towards folic acid, a chemoattractant functioning at the growth phase (Pan et al., 1972
). Therefore, the delay in developmental progression as observed in
cells seemed to be mainly due to the reduced mtDNA, but not to general damage as realized by reduced intracellular ATP levels.
Altered patterning and cell-type proportioning in slugs formed from cells
To examine the effect of reduced mtDNA on cell patterning in slugs, two types of transformants (ecmAO-gal and D19-gal cells) with the vectors bearing a bacterial ß-galactosidase under the promoter of the prestalk-specific gene ecmAO and under the promoter of the prespore-specific gene D19, respectively, were used. The ecmAO gene was expressed in the anterior prestalk cells of migrating slugs and a small number of anterior-like cells (ALC) intermingled in the posterior region (Fig. 8A), as previously reported (Williams et al., 1989). By contrast, the D19 gene was expressed in the posterior prespore cells of migrating slugs (Fig. 8B) (Haberstroh et al., 1991
). When vegetatively growing ecmAO-gal and D19-gal cells were separately treated with 30 µg/ml EtBr for 40 hours and plated on Millipore filters 1.5% agar, they formed relatively normal-shaped slugs after 28 hours of incubation at 22°C (Fig. 8C,D), which was in slight contrast to the irregular-shaped slugs formed on 1.5% agar. A reduced amount of mtDNA in these transformants just after the EtBr-treatment was confirmed by DAPI-staining (Fig. 8C',D'). Moreover, the terminal development of slugs to fruiting bodies was also completely prohibited in these transformants even on Millipore filters, as the case for the slugs derived from
cells.
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Here it is interesting to note that a considerable number of ecmAO-expressing cells (pstAO cells) are scattered in the posterior region (Fig. 8C), and that some D19-expressing cells (prespore cells) are also intermingled with the anterior prestalk cells (Fig. 8D), thus giving an unclear prestalk/prespore pattern along the long axis of slugs.
The number-ratios of pstAO cells and prespore cells to the total number of cells in slugs were determined by histochemical detection of ß-galactosidase activity (Table 1). Interestingly, the results of Table 1 show that the percentage (50.9%) of pstAO cells in slugs (referred to as slugs) formed from
cells is about double of that (24.6%) in slugs (normal slugs) derived from nontreated transformants, whereas the percentage of prespore cells in
slugs is reduced from 75.3% to 47.8%. That is, almost all of cells in
slugs as well as in normal slugs are able to differentiate into either pstAO cells or prespore cells, although the ratio of pstAO cells/prespore cells is markedly increased, coupling with a reduced amount of mtDNA in
slugs.
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Because the above results strongly suggested the induction of prestalk cells and the selective inhibition of prespore differentiation in slugs, a more quantitative analysis, monitored by the prespore-specific vacuoles (PSVs), was carried out using FITC-conjugated anti-D. mucoroides spore IgG (Table 2). As expected, the ratio of prespore cells with PSVs were found to be decreased from a normal value of 71.9% to 49.5% in
slugs (Table 2), thus confirming the results of Table 1. Prespore cells usually had many strongly stained PSVs in the cytoplasm (Fig. 9A), as reported previously (Takeuchi, 1963
). In
slugs, however, both the number of PSVs in each prespore cell and the strength of fluorescent FITC in each PSV were significantly lower compared with those in normally formed prespore cells (Fig. 9B). This was also confirmed using the electron microscope (Fig. 10).
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Impaired phototaxsis of slugs derived from cells
Wilczynska et al. (Wilczynska et al., 1997) have reported that in many heteroplasmic mitochondrial gene disruptants of Dictyostelium the phototaxis of migrating slugs as well as vegetative growth of cells are greatly impaired, particularly in mitochondrial large rRNA (mt-lrRNA)-deficient mutants. This raised the possibility that slugs derived from
cells might also exhibit impaired phototaxis. This possibility was tested by examining the accuracy of phototactic orientation in
slugs, comparing it with that in normal slugs derived from the parental Ax-2 cells. As was expected the result revealed that the normal slugs migrated almost directly towards the light source, but that the
slugs were highly disoriented (Fig. 11), suggesting the prerequisite of mtDNA for phototaxis. Alternatively, it is also possible that the phototactic defect as observed in
slugs may be a consequence of the incomplete sorting of prestalk and prespore cells in the slug, because only the anterior-most prestalk region of a migrating slug is sensitive to light during normal phototaxis (Poff and Loomis, 1973
).
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Discussion |
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The depletion or elimination of mtDNA with EtBr have been used to examine the genetic function of the mitochondrial genome and to create cells that are defective for ATP synthesis through mitochondrial respiration. Until now, 0 cells devoid of mtDNA have been constructed from yeast (Goldring et al., 1970
), algae (Heilporn and Limbosch, 1971
), avian cell lines (Morais et al., 1988
) and human cultured cells (King and Attardi, 1989
) by means of EtBr-treatment. However, creation of
0 cells is not exactly easy in many cell lines including human cultured cells, presumably because of deficiency in mitochondrial energy generation. Recently, it has been shown in Caenorhabditis elegans that mtDNA amplification is a necessary component of the normal developmental program, and that its blockage by EtBr results in an arrest at the L3 larval stage (Tsang and Lemire, 2002
). In general, a high concentration of EtBr is known to induce cell apoptosis, reducing the mitochondrial membrane potential as monitored by MitoTracker staining. Unexpectely, however, Dictyostelium cells never showed any characteristics of apoptosis even in the presence of relatively high concentrations of EtBr, and the mitochondrial membrane potential seemed to be rather augmented in a limited number of mitochondria in EtBr-induced
cells (Fig. 2). In this connection, similar observations have been reported in a cybrid cell line NARP3-2 by cytoplasmic transfer of mitochondria from fibroblasts of a patient with Leigh's disease into the
0206 osteosarcoma cell line (Tanaka et al., 2002
). Two transfected cells were established; one had a higher percentage of mutant mtDNA (approximately 98%; termed NARP3-1) and the other had a lower percentage of mutant mtDNA (approximately 60%; termed NARP3-2). The transfected NARP3-1 cybrids were similar to the
0206 cells; namely, they had a low mitochondrial membrane potential due to a deficiency of the wild-type mtDNA, but the mitochondrial membrane potential of NARP3-2 cybrids was increased. Therefore, it seems to be possible that in
cells with a reduced mtDNA copy number the mitochondrial membrane potential might be rather increased. In Dictyostelium cells, however, it has been claimed that there is a lot of variation between preparations in the intensity of fluorescent staining with dyes such as MitoTracker Orange (P. R. Fisher, personal communication).
As presented in this study, starved cells exhibited greatly delayed differentiation and abnormal morphogenesis: they still remained as nonaggregated single cells even after a prolonged time of incubation, and failed to form fruiting bodies. Importantly, this developmental phenotype is similar to that of the transformant in which about a half of mitochondrial rps4 gene was disrupted by means of homologous recombination (Inazu et al., 1999
). The failure of
slugs to exert normal phototaxis is also consistent with the finding that disruption of the mt-lrRNA in a subpopulation of mitochondria impaires photosensory signal transduction at the slug stage (Wilczynska et al., 1997
).
In differentiating prespore cells, mitochondria exhibit a drastic structural transformation to form a sort of vacuole (M-vacuole), in which PSVs are constructed with the help of the Golgi complex (Maeda, 1971; Matsuyama and Maeda, 1998
). Interestingly, during the formation of
cells mitochondria exhibit a marked morphological change and form unique vacuoles similar to the M-vacuole (see Fig. 4.) As shown in Table 2 and Fig. 8, however, formation of PSVs was rather suppressed in slugs (
slugs) formed from
cells. This seems to indicate that a reduced amount of mtDNA may be closely related to the induction of M-vacuole by mitochondria, but not to PSV maturation.
Interestingly, cell patterning and cell-type proportioning were found to be greatly altered in slugs:
slug cells exhibited enhanced prestalk differentiation, whereas prespore differentiation was markedly suppressed. Somewhat similar phenomena are observed when starved Ax-2 cells were treated with nocodazole or calyculin A to prevent cell division at the early mound stage (Araki and Maeda, 1998
). It has been shown that the cell division and subsequent nuclear DNA replication are resumed only in the cells just before prespore differentiation around the early mound stage (Zimmermann and Weijer, 1993
; Araki and Maeda, 1998
). Moreover, Shaulsky and Loomis (Shaulsky and Loomis, 1995
) have claimed that mtDNA replication is resumed only in the cells destined to differentiate into prespore cells during late aggregation, and that it is a primary step in the developmental program leading to prespore differentiation. In this connection, our preliminary experiments using developing
cells have shown that cell division and mitochondrial DNA synthesis scarcely occur around the early mound stage in Ax-2 cells treated with 30 µg/ml of EtBr for 40 hours at the vegetative growth phase. This seems to indicate that the cell-cycle progression including nuclear and/or mitochondrial DNA replication is essential for prespore differentiation, whereas a reduced amount of mtDNA, as realized in
slugs, is favorable to prestalk differentiation. In
slugs derived from ecmAO-gal and D19-gal transformants the boundary between the anterior prestalk and posterior prespore regions became unclear. This might be mainly because of imperfect prespore differentiation, resulting in incomplete sorting between the two cell types. Mitochondrial cyanide (CN)-resistant respiration has been shown to be tightly involved in cell-type proportioning (e.g. the ratio of prestalk/prespore cells in a slug or stalk cells/spores in a fruiting body): application of specific inhibitors of CN-resistant respiration to starved Dictyostelium cells induces the formation of unique cell masses, in which almost all of the cells differentiate into prestalk cells and then stalk cells, thus being completely devoid of prespore and spore differentiation (Matsuyama and Maeda, 1995
). Thus, it is important to note that the inhibition of CN-resistant respiration and the enforced reduction of mtDNA have a somewhat similar effect on cell-type proportioning in that both of them preferentially prevent prespore differentiation.
In Dictyostelium cells, it is most likely that at least 1/4 of the mtDNA might be required for maintenance of cell growth, because Ax-2 cells ( cells) treated with 30 µg/ml EtBr stopped dividing after two doublings in growth medium. If that is the case, it is impossible to create complete mtDNA-less cells (
0 cells). In spite of such a situation, however, further efforts will be needed to create
0 cells that completely lack mtDNA using a suitable method. For this, we are now attempting to prepare
0 cells by transforming Ax-2 cells with the EcoRI or SmaI gene fused to a mitochondrial targeting signal sequence, whose expression is under control of the tetracycline on/off system. More importantly, the establishment of an appropriate experimental system by which one can disrupt or overexpress specifically a certain mitochondrial gene will be promising to elucidate precisely the function of each mitochondrial gene.
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Acknowledgments |
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References |
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