Instituto de Microbiología Bioquímica, Consejo Superior de Investigaciones Científicas/Universidad de Salamanca and Departamento de Microbiología y Genética, Universidad de Salamanca. 37007 Salamanca, Spain
Correspondence
César Roncero
crm{at}usal.es
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ABSTRACT |
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INTRODUCTION |
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Cytokinesis in S. cerevisiae is properly achieved when three independent but concerted processes occur at the neck region, leading to septum formation (Cabib et al., 1996; Bi, 2001
). First, and very early in the cycle, a chitin ring is formed at the base of the emerging bud (Cabib et al., 2001
). Second, the contractile actomyosin ring guides centripetal invagination of the plasma membrane (Lippincott & Li, 1998
) and, concomitantly, chitin synthase II (CSII) activity (Roh et al., 2002
) synthesizes the chitin disc known as the primary septum (PS) (Molano et al., 1980
). Finally, cell wall material is added from the mother and daughter cells and laid out over the PS, thus creating the secondary septum (SS), whose composition is not precisely known. Once the septum has been formed, cell separation is promoted by the action of hydrolytic enzymes from the daughter side of the cell (Baladron et al., 2002
; Colman-Lerner et al., 2001
), producing an asymmetric distribution of cell wall material that leaves most, if not all, chitin in the mother cell (Cabib et al., 1996
). To a certain extent, the structure of the bud scars reflects the story of the events leading to septum formation. The efficient completion of all these processes requires the involvement of the septin filament ring (for a review, see Longtine & Bi, 2003
).
The chitin ring surrounds the three-layered structure formed by the PS and SS, conferring strength to the neck region. Recently, it has been shown that the chitin ring cooperates with the septin ring in maintaining neck integrity (Schmidt et al., 2003). This ring is assumed to contain most of the cellular chitin, which constitutes the base of bud scars (Molano et al., 1980
). This chitin ring is synthesized by the action of chitin synthase III (CSIII) activity, which is subjected to complex regulation (Roncero, 2002
). The catalytic subunit of CSIII is Chs3p, a protein whose levels do not change significantly during the cell cycle and whose intracellular trafficking is essential in the control of the activity. At different stages, anterograde transport of Chs3p depends on the Chs7p, Chs6p and Chs5p proteins, although endocytic recycling also appears to participate in CSIII regulation (for a review, see Roncero, 2002
). Other key elements in CSIII regulation are Chs4p (Trilla et al., 1997
) and Shc1p (Sanz et al., 2002
), although the function of the latter is restricted to the sporulation process. The involvement of Chs4p in Chs3p trafficking is not well established. In contrast, it has been well documented that Chs4p acts as an activator of CSIII through an unknown mechanism (Choi et al., 1994
; Trilla et al., 1997
; Ono et al., 2000
). In addition, Chs4p plays an essential role in the correct positioning of CSIII at the neck site (DeMarini et al., 1997
). Chs4p interacts physically with Chs3p (DeMarini et al., 1997
; Ono et al., 2000
) and at the same time with Bni4p, a protein whose function is unknown but which appears to form part of the septum synthesis machinery (DeMarini et al., 1997
; Kozubowski et al., 2003
). The physical interaction between Chs4p and Chs3p would explain why these two proteins also depend on each other for correct localization.
PS formation requires CSII activity, whose catalytic subunit is encoded by CHS2, and Myo1p, the only type II myosin in S. cerevisiae, which is required for the function of the contractile ring. Both processes have been shown to be interdependent (Schmidt et al., 2002). In the absence of the actomyosin ring (
myo1 null mutants), cytokinesis is still accomplished, albeit less efficiently (Bi, 2001
; Tolliday et al., 2003
). In
chs2 mutants, the actin and Myo1p rings are formed but are unable to contract (Bi, 2001
). In both cases cytokinesis is achieved through the formation of very thick, aberrant septa (Shaw et al., 1991
; Schmidt et al., 2002
; Tolliday et al., 2003
). These remedial septa require a functional CSIII activity, but not the chitin ring (Cabib & Schmidt, 2003
).
Septins are involved in diverse processes, mainly acting as scaffolds for multiple proteins (Longtine & Bi, 2003). Very recently, it has been shown that septins participate in the recruitment to the septum of the actomyosin contractile machinery as well as of CSII activity, both directly involved in PS synthesis (Lippincott & Li, 1998
; Bi, 2001
; Schmidt et al., 2002
). In addition, the localization of Chs3p and Chs4p at the septum also depends on septins (DeMarini et al., 1997
). However, this interaction is not direct, but occurs through Bni4p, which in turn also interacts physically with the septin ring (DeMarini et al., 1997
). Preliminary evidence has suggested that Bni4p is required for correct chitin synthesis (DeMarini et al., 1997
; Kozubowski et al., 2003
).
Additional evidence concerning the involvement of Bni4p in chitin synthesis arises from a global study of synthetic interactions that has been published recently (Tong et al., 2004). This work clearly shows that Bni4p and Chs3p participate in the same cellular process, cell wall synthesis, but also that both proteins must exert additional and independent functions.
Our work in the search for Calcofluor White (CFW)-resistant mutants (for a review, see Roncero, 2002) has led to the identification of a CFW-resistant bni4 mutant, a result typically related to defects in chitin synthesis. Thus, in this report we reappraise the role of Bni4p by analysing the role of this protein not only in chitin synthesis but also in the construction of the yeast division septum.
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METHODS |
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CFW resistance was assayed in SC solid media, supplemented with different CFW (Blankophor BBH; Bayer) concentrations (1251000 µg ml1) as described previously (Sanz et al., 2002).
Yeast strains construction.
The null mutants generated in this work were obtained by the gene replacement technique as described by Rothstein (1983).
For the disruption of BNI4, two DNA fragments flanking the BNI4 ORF were amplified by PCR from chromosomal DNA. The oligonucleotides used to amplify the 450 bp BNI4-N fragment were as follows: BNI4-N1 (XhoI) 5'-ACTCGAGCAACCGTACCATTAAGTG-3' and BNI4-N2 (HindIII) 5'-AAAGCTTGAAATACTATCCGAC-3'. To amplify the 350 bp BNI4-C fragment, the oligonucleotides used were: BNI4-C1 (HindIII) 5'-AAAGCTTGGCTCAAATGATCAAATTGG-3' and BNI4-C2 (SalI) 5'-AGTCGACAGGTATTCAATGCTCTGG-3'. Both PCR products were cloned separately into pGEM-T vectors (Promega). In a second step, the BNI4-C fragment was cut with HindIII/SalI and ligated into pGEM-BNI4-N previously digested with the same enzymes, obtaining pGEM-BNI4-N-C. Finally, a 1·2 kb HindIIIHindIII fragment containing the URA3 marker was inserted into the HindIII site remaining between the BNI4-N and -C fragments, thus creating pGEM-bni4 : : URA3. Digestion of this plasmid with XhoI/SalI released the 2·0 kb fragment containing the bni4 : : URA3 deletion cassette, which was transformed into different yeast strains by the lithium acetate method. URA3 prototrophs were selected and correct gene replacement was confirmed by PCR analysis.
Disruption of MYO1 and CHS2 in the W303 strain was performed using the same strategy. The myo1 : : HIS5 deletion cassette was kindly provided by Dr Rodríguez-Medina (Universidad de Puerto Rico). The chs2 : : LEU2 cassette was constructed by inserting the LEU2 marker into a SalI restriction site created between two fragments of 800 and 400 bp, corresponding to flanking zones, upstream and downstream, respectively, from the CHS2 ORF inserted in a pKS vector that was kindly provided by Dr Valdivieso (Universidad de Salamanca, Spain). Subsequent digestion with BstUI released the 3·0 kb fragment containing the chs2 : : LEU2 cassette.
Strains myo1
bni4,
myo1
chs3 and
chs2
chs3 were obtained by crossing isogenic W303 haploid strains containing the single deletions. Diploids were sporulated, tetrads dissected and spores were checked to select the double mutants, which were confirmed by PCR. To create the
chs2
bni4 double mutant, strain CRM787 (chs2 : : LEU2) was transformed with the linear DNA fragment containing the bni4 : : URA3 cassette. Strain cdc10-11 (Cid et al., 1998
) was transformed with the linear DNA fragment containing the bni4 : : URA3 cassette, yielding CRM820 (cdc10-11
bni4), and with the chs3 : : LEU2 cassette, previously created in our laboratory, thus obtaining CRM824 (cdc10-11
chs3). Homologous recombination was always confirmed by PCR.
Plasmid construction.
To construct plasmid pRS315 : : CHS4-GFP (green fluorescent protein), we used site-directed mutagenesis to introduce an in-frame NdeI site just after the ATG start codon of CHS4 (oligonucleotide 5'-GGTGAACTTGCCATATGTTATCC-3'). Then, an NdeINdeI DNA fragment of 729 bp containing the E-GFP (Fernandez-Abalos et al., 1998) coding sequence was cloned into this newly created site. Construction was confirmed by direct sequencing. The CHS4-GFP chimera was also cloned into the pRS314 vector. The Chs4p-GFP protein was confirmed to be fully functional by testing the complementation of the phenotypes associated with the
chs4 deletion strain.
Plasmid pRS314 : : MYO1-GFP was constructed by digesting plasmid pRS315 : : MYO1-GFP (pLP8) (Lippincott & Li, 1998) with SalI/NotI. The 6·7 kb fragment containing MYO1-GFP was treated with Klenow to create blunt-ends and ligated into the SmaI site of pRS314.
Chitin and CSIII determinations.
Chitin was measured enzymically as described previously (Sanz et al., 2002) using chitinase from Serratia marcescens (Sigma) and colorimetric determination of the total N-acetylglucosamine released.
CSIII activity determination was performed as described by Choi & Cabib (1994). The addition of Ni2+ and Co2+ cations to the reaction mixtures allowed specific measurement of CSIII activity in the presence of CSI and CSII activities. Different trypsin concentrations were assayed to determine the best proteolysis activation.
In both cases, the quantitative values are represented as the means of at least three independent experiments.
Preparation of samples for microscopy and image processing.
For vital chitin staining with CFW, early-exponential-phase cells in YEPD liquid medium were supplemented with CFW (50 µg ml1 final concn). After 23 h growth, samples were collected and immediately visualized using the appropriate UV filter (340380 nm excitation and 425 nm emission wavelengths). Alternatively, early-exponential-phase cells were fixed and stained with CFW as described by DeMarini et al. (1997).
Isolation of unbudded (virgin) cells was achieved by centrifugation in a sucrose gradient as described by Schmidt et al. (2003). Cells were then incubated in YEPD medium in the presence of 50 µg CFW ml1 at 28 °C. Every 20 min samples were removed, observed and counted to determine the synthesis of chitin rings.
To estimate cell viability in growing cultures, cells were collected, resuspended in 0·3 % methylene blue and immediately observed under bright-field microscopy. Cells stained blue were recorded as lysed cells.
Localization of Chs4p-GFP was observed directly in exponentially growing cells containing plasmid pRS315 : : CHS4-GFP using a specific GFP filter (GFP blue, 470440 nm excitation and 525550 nm emission wavelengths). Indirect immunofluorescence was used to localize Chs3p-3XHA and Cdc11p intracellularly as described by Garcia-Rodriguez et al. (2000b). Mouse HA.11 anti-HA (BabCo), diluted 1 : 75, and Cdc11(y-415) anti-Cdc11 (Santa Cruz Biotechnology), diluted 1 : 150, were used as primary antibodies. Alexa Fluor 594 anti-mouse and Alexa Fluor 488 anti-rabbit, diluted 1 : 400, were used as secondary antibodies, respectively.
All microscopic techniques were performed with a Leica RX150 photomicroscope, using an epifluorescence system with a 100 W Hg lamp. Phase-contrast, bright-field and CFW fluorescence images were obtained with a Leica DC 100 digital camera. For GFP and immunofluorescence, a Sensys (Photometrics) digital camera and Leica QFISH V2.3a software were used. Digital photographs were processed using the Adobe Photoshop 5.0 software package.
Electron microscopy.
Transmission electron microscopy (TEM) was performed essentially as described by Wang et al. (2002). Briefly, S. cerevisiae cultures were grown to an OD600 of 0·51·0. Then, 12·5 OD600 units of cells were collected by centrifugation, washed and fixed in 2 % potassium permanganate for 1 h at room temperature. Excess potassium permanganate was removed by exhaustive washing and stained cells were finally dehydrated by incubation in increasing concentrations of ethanol. Samples were processed in the embedding medium (Spurr Resin Embedding Kit; TAAB) by successive 2 h incubations in 1 : 1 and 1 : 3 ethanol/embedding medium mixtures and, finally, in fresh embedding medium. Cells were concentrated in 500 µl resin and were allowed to polymerize overnight at 60 °C. Ultrathin sections were obtained using an LKB Ultratome III microtome and samples were visualized under a Zeiss EM900 transmission electron microscope.
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RESULTS |
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The bni4 null mutant (see Methods for details of construction) was resistant to low CFW concentrations. However, growth at high CFW concentrations (1 mg ml1) was significantly diminished with respect to that of the
chs4 mutant or other
chs mutants deficient in chitin synthesis (not shown). Accordingly,
bni4 cells appeared to contain chitin, as determined by CFW staining (Fig. 1
a, b). CFW staining of fixed cells revealed a rather uniform chitin distribution across the mother cell surface (Fig. 1b
), in agreement with previous reports (DeMarini et al., 1997
). However, vital staining with CFW (Fig. 1a
) (see Methods for details) allowed clearer discrimination between wild-type (wt) and
bni4 cells. In wt cells most chitin was accumulated at the septum between the mother and daughter cells, while in
bni4 cells a significant number of buds showed a defined staining pattern, indicating that chitin synthesis was occurring actively in the daughter cells. In addition, chitin deposition at the neck appeared altered in the
bni4 mutant.
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Further observation of the vitally stained cells suggested that chitin deposition at the neck in the bni4 mutant occurred mostly at the mother-side of the neck (Fig. 2
a), contrary to what was observed in the wt cells, where chitin appeared to be deposited symmetrically at both sides of the neck. TEM of these cells confirmed these results since CFW treatment of wt cells produced an increased deposition of cell wall material symmetrically to the neck, in agreement with a previous report (Roncero & Duran, 1985
) (Fig. 2b
). In
bni4 cells, cell wall deposition after CFW was only increased at the mother-side (Fig. 2b
).
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Despite the described defects in chitin deposition, chitin synthesis was not quantitatively reduced in the bni4 mutant; instead, we observed a modest but significant increase in chitin levels compared with the control (Table 2
). CSIII activity was fairly similar to that of the control strain and it did not display the zymogenic character observed in the
chs4 mutant (Table 2
and Trilla et al., 1997
). No additive effects on chitin synthesis or CSIII activity were observed in the double
chs4
bni4 mutant (Table 2
). These results indicate that the presence of Bni4p is not required for the synthesis of fully functional CSIII activity as other CHS products are.
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Since our results partially differed from previous reports, we investigated Chs4p localization under our experimental conditions using a fully functional CHS4-GFP chimera that was introduced into different strains in a centromeric plasmid (see Methods). In wt cells, Chs4p accumulated at the presumptive budding site and at the neck in small-budded cells. Further progression of the cycle expanded the localization of Chs4p and, occasionally, two rings were visible at both sides of the neck (Fig. 3a). Conspicuously, in medium-budded cells the population of cells showing Chs4p-GFP localization was reduced compared to other cell cycle stages (data not shown). A similar pattern of localization has been observed for Chs3p (Santos & Snyder, 1997
; and data not shown).
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From the above results it may be concluded that there is a perfect relationship between Chs4p localization and chitin deposition, strongly supporting the notion that the delocalized deposition of chitin observed in bni4 cells must be mainly due to the altered localization of Chs4p.
The absence of Bni4p alters SS structure
Septum formation at the bud neck is a crucial step in cell division in yeast. This structure is reinforced by the early synthesis of the chitin ring that constitutes the base of the bud scars. Observation of recent bud scars under TEM showed the chitin ring as a translucent zone at both sides of the scar (Fig. 4a; see also Cid et al., 1995
). The chitin ring delimited a darker zone that was clearly different from the surrounding cell wall. This cell wall portion could be interpreted as the SS, whose exact composition remains uncertain. The most external part of the bud scar was the PS, made of chitin synthesized by CSII (see Fig. 4a
for details).
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In conclusion, Bni4p is required for the correct synthesis of the chitin ring, but it is also required for the deposition and/or assembly of the SS material. Whether this phenotype is directly or indirectly related to the absence of Bni4p remains to be elucidated (see Discussion for further comments).
Relationship between Bni4p and PS synthesis
All the data gained so far for bni4 cells pointed to a direct involvement of Bni4p in the construction of the chitin ring, but not in the chitin synthesis process, which is not affected. Thus, this mutant provided an excellent tool to genetically discriminate between both situations: the absence of chitin synthesis (
chs3) and the absence of chitin ring assembly (
bni4). Therefore, we investigated the relationship between the assembly of the chitin ring and the formation of the PS by constructing a set of
bni4 and
chs3 double mutants combined with isogenic PS-deficient strains (
myo1 and
chs2). After tetrad dissection (n=44) the number of
myo1
bni4 colonies obtained was only 20 % of that expected. Rescue of double mutants increased to the expected levels when the diploid dissected contained the MYO1 gene in a plasmid (data not shown). In addition, we were unable to cure (frequency<0·8 %) the MYO1-containing plasmid in the double mutants obtained. The simultaneous loss of Bni4p and Myo1p apparently compromised cell growth. Surprisingly, double
myo1
chs3 mutants were obtained with the same frequency as the single
myo1, suggesting no additional cell growth defects in this double mutant. The differences were confirmed by comparative growth analysis between the different mutants.
myo1
bni4 cells grew poorly, clumpy and had aberrant morphologies, and they showed high levels of lysis after methylene-blue staining (Fig. 5
a). In contrast,
chs3
myo1 cells grew essentially as the single
myo1 mutant and showed very reduced levels of lysis. The differences were independent of the growth medium (Fig. 5a
).
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CFW staining shows that the myo1 and
chs2 single mutants synthesized the thick and symmetric remedial septa characterized by the accumulation of chitin (Fig. 5b
). As expected, the
chs3 single mutant only formed the PS. The accumulation of chitin in the
myo1
bni4 mutant indicated that the formation of the septum was the additive result of the single mutations: chitin deposition at the neck appeared abnormal and chitin synthesis also occurred at the growing bud. However,
chs2
bni4 cells were very similar in appearance to the single
chs2 mutant, with the synthesis of a symmetric remedial septum (Fig. 5b
). Apparently, the absence of Myo1p and Chs2p produces different defects in septum assembly that are only apparent in the absence of Bni4p.
myo1
chs3 cells synthesized only the chitin corresponding to PS, but the absence of the contractile ring prevented the correct synthesis of the PS. However, the abnormal accumulation of chitin (Fig. 5b
) produced by CSII provided a functional septum, which would explain the fairly normal growth of this double mutant. Comparison of growth, morphology and septum assembly between the
myo1
bni4 and
myo1
chs3 mutants suggests that Bni4p could play additional roles in septum formation other than directing the assembly of the chitin ring.
Bni4p is required for PS assembly when septin function is compromised
Using the same rationale as before, we wished to explore the possibility of a relationship between the synthesis of the chitin ring and the assembly of septins. To accomplish this, we constructed the double mutants cdc10-11 bni4 and cdc10-11
chs3 (see Methods for details). Growth of these double mutants at different temperatures was not significantly different from that observed for the cdc10-11 single mutant (data not shown). However, the morphologies of both double mutants cells were significantly altered, even at 25 °C, a permissive temperature for the cdc10-11 mutation (Fig. 6
). Characterization of the septin ring assembly in this mutant by immunofluorescence with the anti-Cdc11p antibody or by fluorescence microscopy with the Cdc3p-GFP construction (Schmidt et al., 2003
) indicated that the original single mutant had a significant defect in septin assembly at 25 °C as determined by the reduced number of cells showing the septin ring as well as the reduced amount of septins assembled (data not shown). This result suggests that this mutation probably leads to a loss of function. No additional effects on septin assembly were observed in the corresponding double mutants as compared to the single cdc10-11 mutant (data not shown). Incubation of all these mutants at the non-permissive temperature (3237 °C) stopped growth and the mutants displayed the characteristic phenotypes associated with the complete loss of the septin ring.
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These results indicate that both the chitin and septin rings cooperate together in the assembly of the actomyosin ring and hence in the formation of the PS. Additionally, Bni4p probably plays additional roles in the assembly of this structure apart from its involvement in chitin ring assembly.
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DISCUSSION |
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In previous studies, CFW staining of fixed cells indicated that chitin was distributed diffusely in bni4 cells (see Fig. 1b
; DeMarini et al., 1997
; Kozubowski et al., 2003
). However, the vital CFW staining used in the present study shows that although chitin distribution is altered, it is not uniformly distributed in the mutant cells, but mislocalized (compare images in Fig. 1a and b
), thus indicating that S. cerevisiae cells can partially direct chitin deposition in the absence of Bni4p. The differences observed between both CFW staining methods suggest that vital staining highlights the site of active chitin synthesis, allowing a better interpretation of what is happening in the cell. Alternatively, the use of synchronous cultures provides a more precise way of knowing how chitin deposition occurs during the cell cycle. In wt cells, the deposition of chitin at the neck occurs very early on, and this chitin is assumed to constitute the chitin ring structure. Also, it has been proposed that additional accumulation of chitin at the neck takes place late in the cycle (Cabib & Schmidt, 2003
), which would account for the accumulation of chitin in large-budded cells. However, neither CFW staining (Fig. 1
) nor TEM (Fig. 2
) allows easy discrimination between both rounds of synthesis.
The early accumulation of chitin in bni4 cells must be altered since no chitin ring was observed during the early stages of budding (Fig. 1c
). Additionally, the bud surface showed chitin synthesis, which is seldom observed in the wt. An explanation for this could be that chitin synthesis occurs normally, but that the chitin ring is not properly assembled, indicating a direct role for Bni4p in chitin ring assembly. Nevertheless, chitin deposition at the neck was still observed in large-budded cells, suggesting that this deposition would be independent of Bni4p. Fluorescence and TEM clearly revealed that such deposition occurred specifically at the mother-side of the neck in
bni4 cells. Moreover, Fig. 1(d)
shows that this deposition is produced late during the cell cycle. These results indicate that this chitin accumulation is originated once the mother and daughter cells have become physically separated by the PS and is therefore probably related to construction of the SS.
In conclusion, the results discussed so far indicate that Bni4p has a direct role in the assembly of the chitin ring, but not in the late deposition of chitin that presumably corresponds to the formation of the SS. Thus, indirectly, through the bni4 mutant, we have obtained an easy way to experimentally separate the two rounds of chitin synthesis.
The localization of Chs4p in the different strains matches the sites of chitin deposition precisely, proving that proper Chs4p localization also depends on Bni4p. This dependence is only apparent during the initial stages of the cell cycle, since the localization of Chs4p during cytokinesis is not altered in bni4, confirming an earlier report (Kozubowski et al., 2003
). Interestingly, it has been proposed, and later confirmed, that Chs4p disappears from the neck region during the medial part of the cell cycle (Kozubowski et al., 2003
). This result is in clear accordance with the pattern of chitin deposition observed by us, thus explaining the two temporally separated rounds of chitin deposition. In this scenario it is not surprising that chitin deposition only depends on Bni4p during part of the cell cycle.
Bni4p is not necessary for CSIII activity, but does participate in the anchorage of CSIII to the neck during bud emergence. In the absence of Bni4p, the Chs3p/Chs4p interaction occurs normally, but the active CSIII is moved towards the bud surface, probably through polarization mechanisms, until neck closure is achieved. Interestingly, our results also show that the Bni4p/Chs4p interaction partially depends on Chs3p, in agreement with an earlier report (DeMarini et al., 1997). This suggests that the Chs3p/Chs4p interaction precedes its anchoring to the septin ring and would explain why Bni4p is not involved in CSIII regulation. Arrival of Chs4p at the membrane seems to be essentially independent of Chs3p, indicating that Chs4p has its own signals for membrane localization and that the interaction with Chs3p would occur very late during the intracellular protein sorting.
A recent report on synthetic lethality in S. cerevisiae (Tong et al., 2004) has provided indirect confirmation of our results since the synthetic lethality observed for
bni4 and
chs3 mutants was significantly overlapped. Not surprisingly, the importance of chitin synthesis extends beyond the assembly of the chitin ring since the number of synthetic interactions of
chs3 is much higher. In addition,
bni4 shows exclusive lethal interactions, possibly pointing to additional functions of Bni4p (see below).
Bni4 is directly involved in septum architecture
TEM observations indicate that, in comparison with the wt, bni4 cells appear to lack the chitin ring, but the translucent zones observed along the neck (Fig. 4b
) confirm that chitin deposition still occurs at the neck. However, the most significant difference observed was that
bni4 cells conspicuously lacked the darker cell wall zone surrounded by the chitin ring that was easily recognized in the wt (see Fig. 4
, but also Cid et al., 1995
). This zone corresponds to the SS, and so it seems to be clear that
bni4 cells have an altered SS structure. Although this defect could be an indirect effect of the absence of the chitin ring, it is very likely that Bni4p also plays a role in SS formation by targeting other proteins. A feasible candidate could be Crh2p, presumably involved in the formation of transglycosidic linkages (see below) and whose precise localization to the neck at cytokinesis has been shown to depend on Bni4p (Rodriguez-Pena et al., 2002
).
If the only role of Bni4p were the assembly of the chitin ring, then bni4 should behave similarly or even better than
chs3 mutations in combination with other mutations affecting septum assembly. However, the
myo1
chs3 mutant behaved significantly better than the
myo1
bni4 mutant. The former grew almost normally and with a very reduced level of lysis, suggesting that
myo1
bni4 cells would contain additional defects that cannot be attributed to the role of Bni4p on chitin synthesis. The overall function of Bni4p is not completely understood, but it is required for the proper localization of Crh2p at the neck (Rodriguez-Pena et al., 2002
). This protein is probably responsible for part (Rodriguez-Pena et al., 2000
) of the glycosidic linkages between chitin and glucans (Kollar et al., 1995
). Therefore, the absence of such activity in
bni4 mutants would be an attractive hypothesis to account for the different phenotypes observed. Since the discovery of the major in vivo CS activity, CSIII, it has been assumed that such linkages are related to this activity; however, if this were the case, the
myo1
bni4 and
myo1
chs3 mutants should behave similarly, which is not the case. Therefore, our results point to another CS activity, CSII, as being responsible for the synthesis of the chitin serving as the substrate for the transglycosidic linkages that would form part of the PS. In this case, the
myo1
chs3 double mutant would assemble primary septa incorrectly (see Fig. 5b
), but the CSII activity, together with the correctly formed transglycosidic linkages, would allow the synthesis of a functional septum that would support the fairly normal growth of these cells. The participation of other transglycosidases in the construction of the septum remains to be tested.
In conclusion, these observations indicate that, in the absence of the actomyosin ring, CSIII activity is not the key element in constructing a remedial septum, but CSII, which along with Bni4p would cooperate in such a process, plays an essential role in achieving cytokinesis. In the course of our work, appearance of the chs2
chs3 double mutant, which lacks chitin and was originally described as lethal (Shaw et al., 1991
), was rather surprising. This mutant, as well as the
chs2
bni4 double mutant, showed severe growth problems. In this situation, the presence of the actomyosin ring would serve to recruit alternative cell wall material at the neck for supporting deficient cell division. Despite the apparently normal localization of Myo1p-GFP in the
bni4 mutant (data not shown), we cannot rule out a direct role of Bni4p in the function of the contractile actomyosin ring. Such a hypothesis would be in accordance with the synthetic lethality between BNI4 and CYK3 and SEP7, two genes that encode proteins involved in cytokinesis (Tong et al., 2004
).
Growth of the myo1
bni4 and
chs2
bni4 double mutants was severely compromised, but chitin distribution in both mutants was significantly different. The
myo1
bni4 phenotype resulted in the accumulation of
myo1 and
bni4 defects. Consequently, many cells failed to assemble the remedial septum required, thus producing very elongated cells (Fig. 5b
). Surprisingly, the septa appeared enlarged, but rather normal in the
bni4
chs2 double mutant and cell shape was apparently normal. In this mutant the presence of the actomyosin ring was apparently enough for recruiting the machinery that forms the remedial septa. Such recruitment must occur very early on during the cell cycle since virtually no chitin was observed in the bud despite the
bni4 mutation. The differences observed between both double mutants are in contrast with the general belief that
myo1 and
chs2 mutations produce essentially the same phenotype (Schmidt et al., 2002
). Our results support the hypothesis that the functional contribution of Myo1p and Chs2p to the PS assembly would be different, as would be expected from two proteins with completely unrelated biochemical functions.
Bni4p participates in the maintenance of neck integrity
It has been reported that the chitin ring and septins cooperate in the maintenance of neck integrity (Schmidt et al., 2003). During the course of this work we confirmed this by using a genetic strategy involving the characterization of different double mutants. The cdc10-11 mutation, although described as temperature-sensitive (Cid et al., 1998
), proved to be a loss of function since septin assembly is compromised at the permissive temperature; therefore, the synthetic phenotypes observed when combined with
bni4 or
chs3 mutations were apparent even at 25 °C. In terms of growth and PS formation, both double mutants behaved similarly. The cells were elongated as compared to single mutants and they frequently failed to form the chitin disc that physically separates mother and daughter cells; i.e. the PS. This failure was probably due to the fact that the actomyosin ring was not properly assembled, as judged by Myo1p-GFP localization (Fig. 6
). The fact that single mutants did not show these phenotypes strongly supports a model in which the septin and chitin rings would cooperate to ensure the neck integrity required for PS assembly. Apparently, the synthesis of bulk chitin is irrelevant in the process. The phenotypes of the double mutants cannot be attributed to additional defects of Bni4p or Chs3p on assembly of septins since the quantitative analysis of septin distribution indicates that it is very similar to that observed in the single cdc10-11 mutant. However, we cannot rule out a possible interference of the absence of the chitin ring in septin function not detectable by our microscopic analysis. Growth at higher temperatures failed to provide additional clues since septin-deficient phenotypes were dominant, thus masking the role of other proteins. In terms of morphology and neck diameters, both double mutants differed, cdc10-11
bni4 always showing more aberrant phenotypes and a greater enlargement of the neck diameter than cdc10-11
chs3, which again demonstrates that Bni4p exerts additional functions in septum assembly.
In conclusion, our results suggest new alternatives in the assembly of the septum and support genetic strategies that could be very useful in the determination of the function of other proteins involved in the process, including the role of transglycosidic linkages in septum formation.
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ACKNOWLEDGEMENTS |
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Received 21 May 2004;
revised 23 July 2004;
accepted 2 August 2004.
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