Localization of Fission Yeast Type II Myosin, Myo2, to the Cytokinetic Actin Ring Is Regulated by Phosphorylation of a C-Terminal Coiled-Coil Domain and Requires a Functional Septation Initiation Network

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Vol. 12, Issue 12, 4044-4053, December 2001

Localization of Fission Yeast Type II Myosin, Myo2, to the Cytokinetic Actin Ring Is Regulated by Phosphorylation of a C-Terminal Coiled-Coil Domain and Requires a Functional Septation Initiation Network

Daniel P. Mulvihill, Caroline Barretto,^* and Jeremy S. Hyams

Department of Biology, University College London, London WC1E 6BT, United Kingdom

Submitted December 7, 2000; Revised July 5, 2001; Accepted September 19, 2001
Monitoring Editor: Paul T. Matsudaira

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Myo2 truncations fused to green fluorescent protein (GFP) defined a C-terminal domain essential for the localization of Myo2to the cytokinetic actin ring (CAR). The localization domain containedtwo predicted phosphorylation sites. Mutation of serine 1518 toalanine (S¹⁵¹⁸A) abolished Myo2 localization, whereas Myo2 with a glutamic acidat this position (S¹⁵¹⁸E) localized to the CAR. GFP-Myo2 formed rings in the septationinitiation kinase (SIN) mutant cdc7-24 at 25°C but not at 36°C.GFP-Myo2S¹⁵¹⁸E rings persisted at 36°C in cdc7-24 but not in another SIN kinasemutant, sid2-250. To further examine the relationship betweenMyo2 and the SIN pathway, the chromosomal copy of myo2⁺ was fused to GFP (strain myo2-gc). Myo2 ring formation was abolishedin the double mutants myo2-gc cdc7.24 and myo2-gc sid2-250 atthe restrictive temperature. In contrast, activation of the SINpathway in the double mutant myo2-gc cdc16-116 resulted in theformation of Myo2 rings which subsequently collapsed at 36°C.We conclude that the SIN pathway that controls septation in fissionyeast also regulates Myo2 ring formation and contraction. Cdc7and Sid2 are involved in ring formation, in the case of Cdc7 byphosphorylation of a single serine residue in the Myo2 tail. Otherkinases and/or phosphatases may control ringcontraction.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The critical events for the successful execution of cytokinesis are the recruitment of the proteins that form the contractilering to the incipient cleavage site and the timing of ring contractionsuch that the newly segregated sister chromatids are equally partitionedinto two daughter cells, each of which contains an allocationof the parental cell cytoplasm and organelles. In cells possessinga cell wall, such as the fission yeast, Schizosaccharomyces pombe,the timing and positioning of the contractile machinery on theinside of the cell membrane must be additionally coordinated withthe formation of a new cell wall structure, the septum, on theoutside of the cell. The analysis of S. pombe mutants defectivein septum timing and placement have provided important clues asto the nature of these control mechanisms (Le Goff et al., 1999).Fission yeast cells divide by means of a contractile actin ring(CAR) that both positions the cytokinetic septum and determinesits structural and functional integrity (Marks and Hyams, 1985).The CAR contains two type II myosins encoded by the genes myo2+(Kitayama et al., 1997; May et al., 1997) and myp2+/myo3+ (Bezanillaet al., 1997; Motegi et al., 1997). Myo2 is an essential componentof the CAR (Kitayama et al., 1997; May et al., 1997). Cytokinesiscan proceed in the absence of Myp2 but less efficiently than whenit is present (Bezanilla et al., 1997, Motegi et al., 1997, 2000;Mulvihill et al., 2000). Bezanilla et al. (2000) have claimedMyo2 assembles into the CAR in advance of Myp2, whereas Motegiet al. (2000) conclude that the two myosins arrive at the divisionsite coincidentally. Myo2 dimerizes like other myosin IIs butMyp2 appears to be monomeric (Bezanilla and Pollard, 2000). Thetwo type 2 myosins are associated with the same light chains,Cdc4 (McCollum et al., 1995; Naqvi et al., 1999; Motegi et al.,2000) and Rlc1 (Le Goff et al., 2000; Naqvi et al., 2000).

We have proposed previously that recruitment of Myo2 to the CAR is regulated by the septation initiation network (SIN), leadingto septum formation and cytokinesis (Mulvihill et al., 2000).At the heart of this signal transduction pathway are three proteinkinases, Cdc7, Sid1, and Sid2 (Fankhauser and Simanis, 1994; Sparkset al., 1999; Guertin et al., 2000) and their activating GTPaseSpg1 (Schmidt et al., 1997). The timing of Spg1 activation isdetermined by a two-component GTPase-activating protein consistingof Cdc16 and Byr4 (Furge et al., 1998). All of these components,with the exception of Sid1, have homologs in the budding yeastmitotic exit network (Hoyt, 2000). Mutations in Cdc7, Sid1, Sid2,and Spg1 abolish septation, whereas mutations in Cdc16 and Byr4drive cells into cytokinesis and they become multiseptate (Minetet al., 1979; Fankhauser et al., 1993). A similar phenotype isseen when Cdc7 and Spg1 are overexproduced (Fankhauser and Simanis,1994; Schmidt et al., 1997). The evidence that the SIN pathwayalso regulates Myo2 function includes a strong genetic interactionbetween a myo2 deletion strain and cdc7-24 (May et al., 1997)and the reduced efficiency of septation in myo2 mutants afteroverexpression of Spg1 or Cdc7, or the inactivation of Cdc16 (Mulvihillet al., 2000). This raises the question as to whether the Myo2heavy chain is a substrate for Cdc7 or a downstream kinase, orwhether regulation could work through an associated light chain.Cdc4 function does not appear to be regulated by phosphorylation(although it is a phosphoprotein; McCollum et al., 1999) and bothCdc4 and Rlc1 lack the serine at position 19 whose phosphorylationis associated the activation of myosin II ATPase activity by myosinII regulatory light chain in nonmuscle cells. We have thereforeexamined the role of Myo2 heavy chain phosphorylation in the recruitmentof this myosin to theCAR.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cell Culture and Strains

Cell culture and maintenance were carried out according to Moreno et al. (1991). Experiments were carried out in Edinburghminimal medium 2 (EMM2). Repression of the nmt1 promoter (Maundrell1993) was achieved by the addition of 4 µM thiamine to the growthmedium. To examine the effect of overexpressing the myo2⁺ constructs, cells were grown for 24 h to mid-log phase in EMM2supplemented with thiamine to repress transcription. Cells werethen washed three times in EMM2 lacking thiamine and resuspendedto a suitable cell density (2 × 10⁶ cells/ml), and cultured overnight at 25°C. Phenotypes were examinedafter 22 h of fusion protein expression. The strain myo2-gc wascreated with the use of the method of Bahler et al. (1998b) Geneticcrosses to create double mutants with mutants in the SIN pathwaywere carried as described in Egel et al. (1994). The strains usedin this article are listed in Table 1.

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Table 1. Strains used in this study

Molecular Genetic Manipulations

The amino terminal half (the first 2302 base pairs) of the myo2⁺ gene was isolated from the plasmid pBluemyo2⁺ (May et al., 1997) as an SalI-BamHI fragment and was ligatedinto SalI-BamHI cut pREP41Negfp⁺ (Craven et al. 1998) to give the plasmid pREFP41gfp-myo2⁷⁶⁸. The carboxyl-terminal half (the last 2275 base pairs) of themyo2⁺ gene was isolated from pBluemyo2⁺ as a BamHI-BamHI fragment and was ligated into the BamHI siteof pREP41gfp-myo2^768, to give pREP41gfp-myo2⁺. The C-terminal 3552 base pairs of myo2+ were isolated as anNdeI-SmaI fragment from pREP41gfp-myo2⁺ and ligated into pREP41Negfp⁺ to create p41gfp-myo2^343-1526. A SalI-ScaI fragment containing a truncated form of myo2⁺ was purified from pBluemyo2⁺ and ligated into pREP41Negfp⁺, to create p41gfp-myo2⁸¹⁹. A SalI-Bgl2 fragment was purified from pBluemyo2+, and ligatedinto pREP41gfp⁺, to create p41GFP-myo2¹²²⁸. A SalI-SnaB1 myo2⁺ fragment was eluted from pBluemyo2⁺ and ligated into pREP41gfp⁺ to create p41gfp-myo2¹³³⁶. A Bgl2-BamHI fragment, which contains the sequence encodingthe final 303 amino acids of Myo2 was purified from pBluemyo2⁺ and ligated into pREP41gfp⁺ to create p41gfp-myo2^1228-1526. p41GFP-myo2^1228-1526 was digested with the use of SnaB1 and SmaI, and the subsequentplasmid was religated together to create p41gfp-myo2^1228-1335. A Bgl2-Msc1 fragment was purified from p41gfp-myo2⁺ and ligated into pREP41gfp⁺, which had been cut with NdeI and SmaI to create p41gfp-myo2^1228-1448.

Site-directed mutagenesis was carried out with the use of the site-directed mutagenesis kit from Stratagene (La Jolla, CA)with pREP41Negfp-myo2⁺ as a template and the primers listed in Table 2. The resultantplasmids were sequenced to confirm that only the predicted mutagenesishad taken place.

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Table 2. Oligonucleotides used in this study

Localization

For GFP autofluorescence microscopy cells were fixed in 3.7% formalin for 10 min, washed once in phosphate-buffered salinecontaining 0.1% Triton X-100, and twice in phosphate-bufferedsaline. Cells were mounted onto slides and DNA stained with theuse of 4,6-diamidino-2-phenylindole as described in Moreno etal. (1991). Images obtained with Zeiss Axiophot microscope fittedwith a 1.4 numerical aperture 64× objective were captured withthe use of OpenLab computer software (Improvision, Coventry, UnitedKingdom).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The ability of a series of GFP-tagged truncations of myo2⁺ to localize to the CAR was examined by fluorescence microscopy.Empty vector and full-length, N-terminally GFP-tagged Myo2 (GFP-Myo2)served as negative and positive controls, respectively (Figure1, ai-aiv and bi-biv). The GFP-Myo2 construct was fully functionalbased on 1) its localization to the CAR (Figure 1, bi) and subsequentcontraction and 2) its ability to rescue the mutants myo2-E1 andmyo2 $Delta$ (our unpublished data). The leaky nature of the thiamine-repressiblenmt41 promoter allowed us to compare each construct at low (+thiamine)and high ( $-$ thiamine) levels of expression. At low levels of expression,two of the constructs, GFP-Myo2^343-1526 (lacking the region of the head containing the ATP-binding site)and GFP-Myo2^1228-1526 (encoding the carboxyl terminal half of the tail), located tothe CAR at comparable efficiency to the full-length protein (Figure1, bi, ci, and di). At higher levels of expression, both constructswere toxic and GFP-Myo2 accumulated as aggregates at the cellequator, typical of Myo2 overexpression (Figure 1, ciii and diii;cf., the full-length protein in biii). The construct GFP-Myo2^1228-1448 (the carboxyl-terminal half tail lacking the final 77 amino acids)failed to localize to the CAR (our unpublished data). In fact,no construct lacking this region localized to the CAR (GFP-Myo2^1-768; Figure 1, ei; GFP-Myo2^1-819, Figure 1 fi; GFP-Myo2^1-1228, Figure 1 gi; GFP-Myo2^1-1335, our unpublished data). At higher levels of expression, constructslacking the tail, e.g., GFP-Myo2^1-768 (Figure 1, eiii), GFP-Myo2^1-819 (Figure 1, fiii) or just the C-terminal 77 amino acids, GFP-Myo2^1-1228 (Figure 1, giii) and GFP-Myo2^1-1335 (our unpublished data), localized to actin structures at thecell tips as well as the equator. Thus, the carboxyl-terminalregion of the Myo2 tail not only determines the localization ofMyo2 to the CAR at cytokinesis but also prevents Myo2 from interactingindiscriminately with actin at other points of the cell cycle.We therefore refer to this region as the localization domain (LD).However, expression of the LD alone, either in the presence orabsence of thiamine, did not result in the appearance of GFP rings,neither was its overexpression toxic (our unpublished data). Thus,the LD is essential but not sufficient for the localization theMyo2 to the CAR. These results are summarized in Figure 2. Becausethe contribution of the second fission yeast myosin II gene, myp2⁺, to cytokinesis remains to be precisely defined, we expressedall of the above-mentioned constructs in myp2 $Delta$ (Mulvihill et al.,2000) in both the presence and absence of thiamine. In no casedid we detect a change in Myo2 localization.

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Figure 1. Localization of GFP-Myo2 truncations. Wild-type cells were transformed with plasmids that contained DNA encoding GFP (a), N-terminally GFP-tagged full-length Myo2 (b), and GFP-tagged Myo2 truncations (c-g). The truncations are shown in cartoon form down the left-hand side of the figure. (i) GFP fluorescence. (ii) 4,6-Diamidino-2-phenylindole/Calcofluor staining under repressed conditions (+ thiamine). (iii and iv) As in i and ii but under derepressed conditions (18 h in medium lacking thiamine). GFP alone showed diffuse cytoplasmic fluorescence (ai and aiii). Full-length GFP-Myo2 localized to the CAR in repressed conditions (bi) and accumulated as aggregates at the cell equator when the construct was overexpressed (biii). Similar results were obtained in constructs Myo2^343-1526 and Myo2^1228-1526 containing the C-terminal half of the tail (amino acids 1228-1526) (c and d). In contrast, GFP-Myo2 truncation fusions lacking this C-terminal domain (Myo2^1-768, Myo2^1-819, and Myo2^1-1228) showed no discrete localization in repression conditions (ei, fi, and gi). When overexpressed, these fusions localized indiscriminately to actin structures (eii, fii, and gii). Bar, 10 µm.

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Figure 2. Diagram summarizing which constructs localized to the CAR and which did not. Myo2^1-1526 represents the full-length Myo2 protein. The ATP and actin binding domains are shown as shaded boxes and the two IQ motifs (May et al., 1997

) as vertical lines. The tail domain consists of segments of predicted coiled coil (black boxes) interrupted by proline residues. The final 298 amino acids of the Myo2 protein are required and sufficient for the recruitment of Myo2 to the CAR. Removing the final 77 amino acids abolished Myo2 localization to the CAR.

Because Myo2 is known to be a phosphoprotein (McCollum et al., 1999), an obvious way in which the localization domain mightregulate Myo2 recruitment to the CAR is by phosphorylation. TheMyo2^1448-1526 (LD) sequence was therefore examined for potential phosphorylationconsensus sites with the use of the NetPhos 2.0 Protein PhosphorylationPrediction Server (http://www.cbs.dtu.dk/services/NetPhos/). Twopeptides were found that had a high probability (>0.98) of beingconsensus sites for known serine-threonine protein kinases (serinesat residues 1505 and 1518; Figure 3A). To investigate whetherphosphorylation of these sites was required for the protein localization,the serine residues were individually replaced with alanines bysite-directed mutagenesis of the plasmid pREP41Ngfp-myo2⁺. Mutation of serine 1505 (Myo2S¹⁵⁰⁵A) resulted in the formation of less intense GFP-Myo2 rings (Figure3B, b, arrows) and spots of GFP fluorescence throughout the cell.In contrast, replacing the serine at residue 1518 with alanine(Myo2S¹⁵¹⁸A) abolished GFP-Myo2 ring formation, either in the presence orabsence of thiamine (Figure 3B, c). This mutation also abolishedthe typical Myo2 overexpression phenotype (May et al., 1997; Bezanillaand Pollard, 2000). To examine whether changing serine 1518 toa negatively charged residue such as glutamic acid that wouldmimic phosphorylation at this position, the pREP41gfp-myo2⁺ plasmid was again mutated, and the resultant plasmid, pREP41gfp-myo2S¹⁵¹⁸E, introduced into yeast cells. Myo2S¹⁵¹⁸E was incorporated into the CAR, which contracted with wild-typeefficiency (Figure 3B, d and C). Overproduction of this mutantwas less toxic than the wild-type protein.

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Figure 3. Charge state of two potentially phosphorylated amino acids is intimately associated the recruitment of Myo2 to the actin ring. Mutation of two serines at residues 1505 and 1518 (A) to alanine either inhibits (in the case of S¹⁵⁰⁵A [Bb]) or abolishes (S¹⁵¹⁸A [Bc]) the recruitment of Myo2 to the actin ring. S¹⁵⁰⁵A rings form but lack the structural integrity of the wild-type protein (B, b, arrows). Mutating serine 1518 to glutamic acid (S¹⁵¹⁸E) had no significant effect on Myo2 localization nor on the dynamics of CAR contraction (Bd). Quantification of ring formation in the different constructs is shown in C. Bar, 10 µm.

We suggested previously that the incorporation of Myo2 into the CAR was under the regulation of the SIN pathway that controlsseptum formation in fission yeast (Mulvihill et al., 2000). Toinvestigate this further we expressed GFP-Myo2 in the mutantscdc7-24 and cdc7-A20. At 25°C GFP-Myo2 was incorporated into theCAR. When the culture was transferred to 36°C, to fluorescentMyo2 rings disappeared within 3 h (Figure 4, A and B) but returnedwithin 2 h when cells were restored to 25°C (our unpublished data).Thus, Cdc7 function is required to maintain the integrity of theCAR. We repeated this experiment with Myo2S¹⁵¹⁸E. In this case, Myo2 rings persisted at 36°C although they didnot contract (Figure 4D). These data point to serine 1518 beinga target, either directly or indirectly, of Cdc7. To resolve thispoint, we expressed Myo2S¹⁵¹⁸E in another SIN kinase mutant, sid2-250. As in cdc7-24, bothGFP-Myo2 and Myo2S¹⁵¹⁸E formed rings at 25°C; neither, however, persisted at the restrictivetemperature (Figure 4C).

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Figure 4. GFP-Myo2 localization to the medial ring is abolished in cdc7 and sid2 mutants at the restrictive temperature. (A) cdc7-24 cells bearing the plasmid pREPgfp-myo2⁺ were grown to log phase at 25°C and shifted to 36°C. Samples were taken hourly, fixed, and the proportion of cells with Myo2 rings ( $open circle$ ), two nuclei ( $triangle$ ), and more than two nuclei ( $black-diamond$ ) was examined. Note the decline of Myo2 rings in parallel with the expression of the cdc7 phenotype. Strains bearing mutations in either cdc7 or sid2 were transformed with plasmids bearing either gfp-myo2⁺ or gfp-myo2S¹⁵¹⁸E, grown in the presence of thiamine at the permissive temperature to early-log phase then cultured for 3 h at the restrictive temperature. Cells were fixed to allow GFP-Myo2 and DNA localization to be examined. In both cdc7-A20 (B) and sid2-250 (C), the wild-type GFP-Myo2 (S1518) was unable to form rings. In the case of cells expressing GFP-Myo2S¹⁵¹⁸E, rings persisted in cdc7-A20, but not sid2-250. Note that the S¹⁵¹⁸E rings did not contract. Bars, 10 µm.

To further investigate the relationship of Myo2 to the SIN pathway we created the strain myo2-gc in which the chromosomalcopy of myo2⁺ was fused to the gene encoding GFP to produce a C-terminallytagged Myo2 under the control of its own promoter. myo2-gc hadwild-type morphology and showed normal growth characteristic atall temperatures tested. We created double mutants with myo2-gcand mutants in all of the known components in the SIN pathwayand some of the genetic interactions are summarized in Figure5. myo2-gc showed synthetic lethality with cdc7.24 at the semipermissivetemperature (29°C; Figure 6a). The interaction with sid2-250 wasstronger and myo2-gc sid2-250 showed poor growth even at the permissivetemperature (Figure 6b). Despite repeated attempts, we were unableto create the double mutant myo2-gc sid1-25. We next examinedMyo2 ring formation in myo2-gc cdc7-24 and myo2-gc sid2-250. Inboth cases, rings reversibly disappeared at the restrictive temperature,as they had when Myo2 was expressed from a multicopy plasmid.In some cells a dot of fluorescence was observed at the cell tips(Figure 6, c and d). Because the SIN pathway appears to be essentialfor CAR formation we examined the effect of uncontrolled SIN onMyo2 incorporation into the CAR. The temperature-sensitive mutantcdc16-116 undergoes multiple rounds of septation at the restrictivetemperature. The double mutant myo2-gc cdc16-116 showed syntheticlethality at 31°C (Figure 7A). When these cells were raised tothe nonpermissive temperature for 3 h, Myo2 rings collapsed (Figure7, B-E) and 80% of cells accumulated a single bright dot at thecell equator (Figure 7, C and E). Whereas control cdc16-116 cellsin a myo2⁺ background formed multiple septa (Figure 7D, inset), myo2-gccdc16-116 cells rarely formed more than a single, often distortedseptum (Figure 7D).

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Figure 5. Summary of the genetic interactions between mutations in genes encoding components of the SIN pathway and myo2-gc. A strain in which the 3' terminus of the chromosomal copy of the myo2⁺ gene was fused to gfp⁺ had similar growth kinetics to wild type at all temperatures and in all media examined. Strains bearing the myo2-gc allele in combination with mutants in genes for components of the SIN pathway reduced the permissive temperature for growth in the case of spg1, cdc16, cdc7, and sid2 but not in the case of cdc11 and sid4.

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Figure 6. Functional Cdc7 and Sid2 are required to recruit Myo2-GFP to the actin ring. myo2-gc cdc7-24 (A) and myo2-gc sid2-250 (B) were unable to grow at 29°C, a temperature at which all three single alleles were viable. When myo2-gc cdc7-24 cells, which had been grown to early log phase at 25°C were shifted to the nonpermissive temperature Myo2 rings disappeared (C). When log phase myo2-gc sid2-250 cells were shifted to the nonpermissive temperature of 36°C, Myo2-GFP rings dispersed, but fluorescence remained as dots at the cell tips and cell equator (D). Bars, 10 µm.

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Figure 7. Cdc16 is required for the maintenance of the CAR. myo2-gc cdc16-116 cells were unable to grow at 29°C, a temperature that permitted growth in strains bearing either allele individually (A). myo2-gc cdc16-116 cells were grown to log phase at 25°C and then cultured at 36°C. Samples were taken at hourly time points and fixed to allow changes in the proportion of cells with Myo2-GFP rings ( $open circle$ , dotted line), contracted Myo2-GFP rings (

, solid line), septa (+ with dashed line), and aberrant septa (+ with solid line) to be examined (B). The proportion of cells containing Myo2-GFP rings declined over time. Rings assembled but subsequently collapsed (C) and the population of cells arrested with a single spot of Myo2-GFP fluorescence associated with septal material (D and E). cdc16-116 cells in a myo2⁺ background at the same 3-h time point are shown in the inset to E. The majority of cells had more than one morphologically normal septum. Bar, 10 µm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Unlike most conventional myosins, the tails of the two yeast myosin IIs consist of short stretches of alpha helix interruptedby proline residues, rather than a continuous extended structure(Bezanilla et al., 1997; May et al., 1998). Nevertheless, theMyo2 tail is involved in the formation of higher order structures(Naqvi et al., 1999; Bezanilla and Pollard, 2000). As with othermyosin IIs (Zang and Spudich, 1998; Yumura and Uyeda, 1997) and,indeed, some unconventional myosins (Reck-Peterson et al., 1999),localization of Myo2 is a function of the tail, neither the headdomain (Naqvi et al., 1999), nor the IQ region (Motegi et al.,2000), contributing to the recruitment of Myo2 to the CAR. Herewe confirm these previous findings and extend them to show thatthe C-terminal 77 amino acids of the Myo2 tail, a region witha high probability of forming coiled-coils (Bezanilla et al.,1997; May et al., 1998; Bezanilla and Pollard, 2000), is necessaryfor Myo2 localization. Constructs lacking this localization domain(Myo2^1-768, Myo2^1-819, Myo2^1-1228, Myo2^1-1335, Myo2^1228-1335 and Myo2^1228-1448) failed to localize to the CAR, whereas constructs containingthis region (the full-length protein Myo2^1-1526, Myo2^343-1526, and Myo2^1228-1526) did. Not only does the Myo2 tail domain direct the protein tothe CAR but also it prevents it from binding promiscuously toactin at the cell poles. Hence, the specificity of Myo2 recruitmentto the CAR resides within a distal tail fragment, which we referto as the LD. However, the LD alone (Myo2^1448-1526) failed to localize to the CAR. Thus, the LD is necessary butnot sufficient for the recruitment of Myo2 to the CAR and othertail sequences, as yet undefined, appear to contribute to thisprocess. Whether, as in Dictyostelium, the localization domainis also an assembly domain remains to be determined but the lackof toxicity of LD overexpression might suggest that it isnot.

Myo2 is known to be a phosphoprotein in vivo (McCollum et al., 1999). Examination of the localization domain sequence revealedtwo serine residues that lie within consensus phosphorylationsites for a number of protein kinases. Mutation of serine 1505to the nonphosphorylatable amino acid, alanine (S¹⁵⁰⁵A), reduced the efficiency of Myo2 localization but the most strikingfinding was that mutation of serine 1518 to alanine (S¹⁵¹⁸A) abolished both Myo2 localization and the toxicity of Myo2 overexpression.Myo2 carrying the mutation of the same residue to glutamic acid(S¹⁵¹⁸E) to mimic the effect of phosphorylation was recruited to theCAR, which contracted with apparently normal kinetics. This constructalso had reduced toxicity when overproduced. These results arguestrongly that Myo2 localization is regulated by phosphorylation.They also point to the toxicity of myo2⁺ overexpression being related to the phosphorylation state ofthe protein. Double staining of cells overproducing GFP-Myo2 withan actin antibody revealed that nonfunctional protein bound toand sequestered actin at the center of the cell but was unableto form rings (our unpublisheddata).

The regulation of myosin II function by tail phosphorylation has hitherto only been described in amoebae (reviewed in Brzeskaand Korn, 1996). In Acanthamoeba, myosin II activity is negativelyregulated by phosphorylation of a C-terminal, nonhelical regionof its heavy chain (Collins et al., 1982; Ganguly et al., 1992).In Dictyostelium, filament assembly and the recruitment of myosinII to the contractile ring require the phosphorylation of threethreonine residues at the C terminus (Egelhoff et al., 1991; Leeet al., 1994; Sabry et al., 1997; Shu et al., 1999) by at leasttwo myosin II heavy chain kinases (Ravid and Spudich, 1989, 1992;Kolman et al., 1996). Mutation of all three sites (Egelhoff etal., 1993) or, indeed, just one of them (Nock et al. 2000), abolishesmyosin function. In fission yeast also, a single charge changeabolishes the assembly of Myo2 into the CAR. The recruitment ofMyo2 to the CAR must be coordinated with the signal transductionpathway leading to septum formation, the septation initiationnetwork. This includes a number of protein kinases, Plo1 (Okhuraet al., 1995; Bahler et al., 1998a; Mulvihill et al., 1999), Cdc7(Fankhauser and Simanis, 1994), Sid 1 (Guertin et al., 2000),and Sid 2 (Sparks et al., 1999), and their associated regulators(reviewed in Gould and Simanis, 1997; Le Goff et al., 1999; Balasubramanianet al., 2000). Any or all of the above are potential fission yeastmyosin II heavy chain kinases. We have shown previously a geneticinteraction between myo2 and cdc7 mutants (May et al., 1997; Mulvihillet al., 2000) and that the efficiency of septation driven by overexpressionof Spg1, the GTPase activator of Cdc7 (Schmidt et al., 1997),or inactivation of Cdc16, one of the components of the Spg1 GTPase-activatingprotein (Furge et al., 1998), is substantially reduced in themutant myo2-E1 (Mulvihill et al., 2000). In this report we showdirectly that the CAR is dependent for its integrity upon SINfunction. Myo2 rings formed with more or less normal efficiencyin cdc7-24 and cdc7-A20 at the permissive temperature but wereabolished at a temperature at which Cdc7 kinase activity is substantiallyreduced (Fankhauser and Simanis, 1994). Strikingly, the dependencyof CAR formation on Cdc7, but not Sid2, was bypassed in Myo2S¹⁵¹⁸E. Thus, both Cdc7 and Sid2 are potential myosin II heavy chainkinases whose functions are required for Myo2 localization tothe CAR but only Cdc7 phosphorylates S1518, whereas Sid2 is directedto other residue(s), possibly including S1505. These results clearlyrequire direct biochemical confirmation. We are also aware thatalthough Sid2 has been shown to be associated with the CAR (seebelow), Cdc7 has not (Sohrmann et al., 1998) and the full storyof the relationship between Myo2 and its presumptive kinase awaitsfurtherstudy.

CAR contraction in living fission yeast cells has been followed with the use of GFP-tagged Myo2 and Myp2 (Kitayama et al.,1997; Bezanilla et al., 2000; Mulvihill et al., 2000) and by Balasubramanianet al. (1997) who made a GFP fusion protein with the Myo2 lightchain Cdc4 (McCollum et al., 1995, 1999). In none of these caseswas the GFP reporter under the control of the endogenous promoter,moreover, cells retained the endogenous myo2⁺ gene. We therefore created the strain myo2-gc in which the chromosomalcopy of myo2⁺ is fused to GFP and thus produces only the chimeric protein atendogenous levels. myo2-gc showed normal growth and cytokinesisin all growth conditions tested and mated normally. Hence, wewere able to introduce the mutation into a variety of geneticbackgrounds. myo2-gc was synthetically lethal with mutants intwo of the SIN kinases, cdc7-24 and sid2-25 at the semipermissivetemperature. We were unable to generate the double mutant myo2-gcsid1-25 and we interpret this as indicating a very strong geneticinteraction between these two alleles. That myo2-gc, in whichGFP is fused to the C terminus of Myo2, has a cryptic cytokinesisphenotype is perhaps not surprising given the importance of thisregion of the tail for Myo2 localization (this report). Raisingmyo2-gc cdc7-24 and myo2-gc sid2-25 to the restrictive temperaturehad a striking effect on Myo2 organization; rings disappearedat 36°C as they did when GFP-Myo2 was expressed from aplasmid.

In theory, this simple yet novel assay of ring stability can be used to monitor, in living cells, the effect of any potentialregulator of cytokinetic actomyosin ring formation for which amutation is available. This is shown particularly clearly in thecase of cdc16-116 in which the SIN pathway is hyperactivated.Whereas cdc16-116 in a myo2⁺ background formed multiple septa as described originally by Minetet al. (1981), in myo2-gc cdc16-116 cells mostly failed to formmore than one septum and the morphology of the septa formed wasmarkedly aberrant. Such cells were found to contain a single tightspot of GFP fluorescence. Closer analysis revealed that the CARwas unstable in this background and the spot of GFP-Myo2 was thefinal stage of CAR collapse. Taken together, our results suggesta model in which the assembly of the CAR and its subsequent contractionis under the control of the SIN pathway. We envisage that recruitmentof Myo2 to the CAR is positively regulated by phosphorylationby both Cdc7 and Sid2, whereas CAR ring contraction is regulatedby other SIN kinases and phosphatases. Based on their structuralinterdependence at the spindle poles, Guertin et al. (2000) envisagethat the SIN proteins form a simple linear pathway with the orderCdc16/Byr4, Spg1, Cdc7, Sid1, and Sid2 that activates the cellwall $beta$ -glucan Cps1 (Balasubramanian et al., 2000). We envisagethe SIN proteins forming a complex in which the components interactin a variety of ways and which modifies a number of substrates,one of which is Myo2. The cytokinesis defect of cdc7 mutants islikely due to the failure to phosphorylate S1518; this inhibitsCAR formation and septation is consequently abolished. Myo2S¹⁵¹⁸E forms rings n the absence of Cdc7 function but these are unableto contract and other modifications must take place to initiatethis process. cdc7 mutants form actin ring (Le Goff et al., 1999),suggesting that actin and Myo2 are brought to the CAR by differentmechanisms.

The SIN pathway in fission yeast closely corresponds to the mitotic exit network in budding yeast (Hoyt, 2000). Lippincottet al. (2001) recently demonstrated a role for the TEM1 GTPase(the homolog of Spg1 in S. pombe) in CAR dynamics in budding yeast.The relationship between mitosis and cytokinesis is very differentin the two yeasts. Nevertheless, a role for the SIN/mitotic exitnetwork pathway in the control of CAR formation and function appearsto be conserved. Our findings do not exclude the possibility thatMyo2 is phosphorylated at other sites by protein kinases otherthan those in the septation pathway. In Dictyostelium, myosinII is phosphorylated by a myosin heavy chain specific proteinkinase C (Matto-Yelin et al., 1997) and the fission yeast proteinkinase C homolog Pck2 localizes to the division site at cytokinesis(Sayers et al., 2000). Myo2 is not regulated by phosphorylationof conserved sites in its essential light chain Cdc4 (McCollumet al., 1999) and the regulatory light chain Rlc1 lacks the serineat amino acid position 19 that is associated with the regulationof Myo2 function in nonmuscle cells (Bresnick, 1999). As notedby others (Bresnick, 1999; Prokopenko et al., 2000), it is likelythat several signaling pathways converge on cytokinesis. Fissionyeast are emerging as a powerful tool in which to dissect someof theseprocesses.

	ACKNOWLEDGMENTS

We are extremely grateful to Viesturs Simanis, Dan McCollum, and Mohan Balasubramanian for strains; Yannick Gachet and JonathanMillar for advice and encouragement; and Vasanti Amin for technicalassistance. This study was supported by Wellcome Trust grant 046707to J.S.H.

	FOOTNOTES

^* Present address: Université Paul Sabatier, Toulouse,France.

Corresponding author. E-mail address: j.hyams{at}ucl.ac.uk.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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