The Cofactor-Dependent Pathways for {alpha}- and {beta}-Tubulins in Microtubule Biogenesis Are Functionally Different in Fission Yeast

The Cofactor-Dependent Pathways for ${alpha}$ - and ß-Tubulins in Microtubule Biogenesis Are Functionally Different in Fission Yeast

Pippa A. Radcliffe^1,a, Miguel Angel Garcia^a, and Takashi Toda^a
^a Laboratory of Cell Regulation, Imperial Cancer Research Fund, London WC2A 3PX, United Kingdom

Corresponding author: Takashi Toda, Laboratory of Cell Regulation, Imperial Cancer Research Fund, P.O. Box 123, 44 Lincoln's Inn Fields, London WC2A 3PX, United Kingdom., toda{at}europa.lif.icnet.uk (E-mail)

Communicating editor: P. RUSSELL

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The biogenesis of microtubules in the cell comprises a seriesof complex steps, including protein-folding reactions catalyzedby chaperonins. In addition a group of evolutionarily conservedproteins, called cofactors (A to E), is required for the productionof assembly-competent ${alpha}$ -/ß-tubulin heterodimers. Usingfission yeast, in which alp11⁺, alp1⁺, and alp21⁺, encodingthe homologs for cofactors B, D, and E, respectively, are essentialfor cell viability, we have undertaken the genetic analysisof alp31⁺, the homolog of cofactor A. Gene disruption analysisshows that, unlike the three genes mentioned above, alp31⁺ isdispensable for cell growth and division. Nonetheless, detailedanalysis of alp31-deleted cells demonstrates that Alp31^A isrequired for the maintenance of microtubule structures and,consequently, the proper control of growth polarity. alp31-deletedcells show genetic interactions with mutations in ß-tubulin,but not in ${alpha}$ -tubulin. Budding yeast cofactor A homolog RBL2 iscapable of suppressing the polarity defects of alp31-deletedcells. We conclude that the cofactor-dependent biogenesis ofmicrotubules comprises an essential and a nonessential pathway,both of which are required for microtubule integrity.

ALL eukaryotic cells utilize the microtubule cytoskeleton fora wide variety of cellular processes. Microtubules, biopolymersof ${alpha}$ - and ß-tubulins, initiate their assembly from specializedstructures in the cell called microtubule-organizing centers(MTOCs), and free ${alpha}$ /ß-heterodimers are then incorporatedinto their plus-ends. The biogenesis of microtubules in vivoconsists of a cascade of sequential reactions. After translationfrom mRNA, both ${alpha}$ - and ß-tubulins are captured in the cytosolby a group of chaperones, called chaperonins, which belong toa subfamily of GroEL and Hsp60 (CCT/TriC/c-cpn; ROMMELAEREet al. 1993 ; KUBOTA et al. 1994 ). Unlike actin and ${gamma}$ -tubulin,which also require the chaperonin complex for proper folding(GAO et al. 1992 ; MELKI et al. 1993 ; STERNLICHT et al. 1993), for the production of assembly competent ${alpha}$ -/ß-tubulinheterodimers, an additional set of proteins, called cofactors,is needed (CLEVELAND et al. 1978 ; GAO et al. 1993 , GAO etal. 1994 ). Molecular cloning of these cofactors from vertebrateshas revealed that they comprise multiple proteins, consistingof A, B, C, D, and E (LLOSA et al. 1996 ; MELKI et al. 1996; TIAN et al. 1996 , TIAN et al. 1997 ).

It has been proposed, on the basis of mammalian in vitro reactions,that the pathways leading to correctly folded ${alpha}$ /ß-heterodimerscomprise two symmetrical branches as summarized below. Afterrelease from the chaperonin complex (LEWIS et al. 1992 ; YAFFEet al. 1992 ), ${alpha}$ - and ß-tubulins initially follow distinctfolding pathways; ${alpha}$ -tubulins are captured by cofactor B, whileß-tubulin is captured by cofactor A, which are subsequentlyreplaced by cofactors E and D, respectively. The two pathwaysthen converge with the formation of a quaternary complex ( ${alpha}$ -tubulin/Eand ß-tubulin/D). Finally cofactor C binds the complexand upon GTP hydrolysis assembly-competent ${alpha}$ -/ß-tubulinheterodimers are released (LEWIS et al. 1997 ).

In fission yeast as in higher eukaryotes, microtubules playa crucial role in chromosome segregation (UMESONO et al. 1983A; TODA et al. 1984 ), distribution of the organella such asthe mitochondria and Golgi apparatus (AYSCOUGH et al. 1993 ; YAFFE et al. 1996 ), and cell polarity (UMESONO et al. 1983B; HIRAOKA et al. 1984 ; MATA and NURSE 1997 ; RADCLIFFE etal. 1998 ). In addition to chaperonins, all the cofactor homologsexcept for cofactor C exist in the genome and the homologs ofcofactors B, D, and E (Alp11, Alp1, and Alp21/Sto1, respectively)have all been shown to be involved in microtubule biogenesis(HIRATA et al. 1998 ; RADCLIFFE et al. 1998 , RADCLIFFE etal. 1999 , RADCLIFFE et al. 2000 ; GRISHCHUK and MCINTOSH1999 ; RADCLIFFE and TODA 2000 ). In contrast to the nonessentialroles of these cofactor homologs in budding yeast (HOYT et al.1990 , HOYT et al. 1997 ; STEARNS et al. 1990 ; URSIC andCULBERTSON 1991 ; ARCHER et al. 1995 ; TIAN et al. 1997 ),in fission yeast Alp11^B, Alp1^D, and Alp21^E are absolutely requiredfor cell viability and the absence of any one results in thefailure to maintain microtubule structures and in subsequentcell division defects (HIRATA et al. 1998 ; GRISHCHUK and MCINTOSH1999 ; RADCLIFFE et al. 1999 ).

Results obtained from studies in yeasts are mostly in line withthe pathways proposed from studies in higher systems; however,there apparently exists a significant difference. While thefindings from the two systems are consistent with the idea thatcofactors D and E act at the steps later than cofactor B, incontrast to the parallel roles of cofactors D and E in mammaliansystems, in fission yeast it is evident from genetic analysisthat Alp1^D functions downstream of Alp21^E (Alp11^B-Alp21^E-Alp1^D; RADCLIFFE et al. 1999 ; Table 1). This is in agreement withthe result from budding yeast (Pac2^E-Cin1^D; HOYT et al. 1997). In addition a subpopulation of Alp1^D, but not Alp21^E, colocalizeswith microtubules and biochemically behaves like microtubule-associatedproteins (MAPS; HIRATA et al. 1998 ; GRISHCHUK and MCINTOSH1999 ; RADCLIFFE et al. 1999 ). A further inconsistency isthat alp1 and cin1 mutants clearly show compromised ${alpha}$ -tubulinfunction rather than defects in ß-tubulin, such as a lowerlevel of ${alpha}$ -tubulin in these mutant cells (HOYT et al. 1990 ; RADCLIFFE et al. 1999 ; RADCLIFFE and TODA 2000 ). These resultssuggest that the pathways leading to heterodimer formation for ${alpha}$ - and ß-tubulins are not simply functionally symmetrical.

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Table 1. S. pombe cofactor homologs involved in the ${alpha}$ -tubulin pathway

To address the in vivo role of the ß-tubulin pathway,we have undertaken the genetic study of the cofactor A homologin fission yeast (designated alp31⁺). Cofactor A (Rbl2 in buddingyeast) has been shown to act specifically in the ß-tubulinpathway in parallel with cofactor B (Alf1 in budding yeast andAlp11 in fission yeast), which functions only for ${alpha}$ -tubulin (GAOet al. 1993 ; ARCHER et al. 1995 , ARCHER et al. 1998 ; MELKIet al. 1996 ; RADCLIFFE et al. 1999 ; RADCLIFFE and TODA 2000). Here we show that, in contrast to the alp11⁺ gene, alp31⁺is dispensable for cell viability. Nevertheless, Alp31 playsan important role in the maintenance of microtubule integrityand the determination of cell polarity. The analysis in fissionyeast presented here highlights the functional similaritiesand differences between the cofactor-dependent pathways for ${alpha}$ - and ß-tubulin in microtubule biogenesis.

MATERIALS AND METHODS

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Strains, media, and genetic methods:
Strains used in this study are listed in Table 2. YPD (2% dextrose,2% polypeptone, and 1% yeast extract) and YE5S were used asrich media. Standard methods were followed as described (MORENOet al. 1991 ).

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Table 2. S. pombe strains used in this study

Nucleic acids preparation and manipulation:
Standard molecular biology techniques were followed as described(SAMBROOK et al. 1989 ). Enzymes were used as recommended bythe suppliers (New England Biolabs, Beverly, MA). Nucleotidesequence data reported in this paper are in the DDBJ/EMBL/GenBankdatabases under accession no. AB029481 (alp31⁺).

Gene disruption:
The alp31⁺ gene was deleted using PCR-generated fragments (BAHLERet al. 1998 ). Dissection of asci from heterozygous diploidcells (PR21, Table 2) showed that alp31⁺ is a nonessentialgene as all four spores germinated and formed colonies. Resistancefor G418 segregated 2:2 and correct disruption of alp31⁺ wasconfirmed by PCR (PR23 and PR25).

Synthetic lethal interaction:
alp31-deleted cells ( ${Delta}$ alp31, PR31) were crossed with variousmutants defective in microtubule function. Mutants used includedcold-sensitive (cs) or temperature-sensitive (ts) ß-tubulinmutants (KM311-201, nda3-311 or DHH1828, nda3-1828, respectively),cs ${alpha}$ 1-tubulin mutant (KM52-201, nda2-52), and ts or deleted ${alpha}$ 2-tubulinmutant (DHH1377, atb2-1377 or ${Delta}$ atb2, atb2::LEU2, respectively).After tetrad dissection, spores were allowed to germinate at26° (ts) or 32° (cs).

Suppression of ${Delta}$ alp31 by expression of the budding yeast RBL2 gene:
A ${Delta}$ alp31 strain (PR31) was cotransformed with pREP1 and pREP2or pREP1 and pA21A (RBL2-containing multicopy plasmids, obtainedfrom Dr. F. Solomon's laboratory). Leu⁺Ura⁺ transformants werestreaked on minimal medium and morphology was observed underphase-contrast microscopy.

Overexpression and epitope-tagging:
The entire open reading frame (ORF) of the alp31⁺ gene was clonedby PCR into pREP1 under control of the nmt1 promoter (MAUNDRELL1990 ), yielding pREP1-alp31⁺. pREP1-alp31⁺ is functional, asit is capable of suppressing the morphological defects of alp31-deletedcells. To epitope-tag alp31⁺, GST was tagged at the C terminusof Alp31 using a PCR-based method (BAHLER et al. 1998 ). Taggingdoes not interfere with Alp31 function, as the cell morphologyof a strain containing Alp31-GST is normal. Cells containingpREP1-alp31⁺ were grown in thiamine-free minimal medium for24 hr and processed for immunofluorescence microscopy.

Immunochemical assays:
Antibodies used in this study were as follows: mouse monoclonalanti-Cdc2 antibody (obtained from Dr. Hiroyuki Yamano), mousemonoclonal anti-HA antibodies (16B12, BAbCO), mouse monoclonalanti- ${alpha}$ -tubulin antibody (TAT-1, provided by Dr. Keith Gull),mouse monoclonal anti-ß-tubulin antibody (KMX-1, providedby Dr. Keith Gull), and rabbit polyclonal anti-GST antibody(G7781; Sigma Chemical Co., St. Louis, MO). Preparation of rabbitpolyclonal anti-Alp11 antibody was described previously (RADCLIFFEet al. 1999 ). Horseradish peroxidase-conjugated goat anti-rabbitIgG, goat anti-mouse IgG (Bio-Rad Laboratories Ltd., Hercules,CA), and a chemiluminescence system (ECL; Amersham PharmaciaBiotech Ltd., Buckinghamshire, UK) were used to detect boundantibody. Fission yeast whole cell extracts were prepared usingglass beads to disrupt cells as described before (RADCLIFFEet al. 1998 ).

Gel filtration chromatography:
Gel filtration chromatography was performed on a Superose-6column (Amersham Pharmacia Biotech Ltd.) in buffer A (20 mMTris-HCl, pH 7.5, 20% glycerol, 0.1 mM EDTA, 1 mM mercaptoethanol,5 mM ATP plus a cocktail of inhibitors). The column was equilibratedwith two column volumes of buffer A containing 100 mM NaCl.To determine molecular weight, a parallel column was run withstandards consisting of dextran (2000 kD), thyroglobulin (669kD), ${alpha}$ -amylase (232 kD), and ovalbumin (43 kD). Fractions (50µl each) were separated by SDS-PAGE and fractionated proteinswere detected with individual antibodies.

Indirect immunofluorescence microscopy:
Cells were fixed with methanol and primary antibodies (TAT-1)were applied, followed by Cy3-conjugated sheep anti-mouse IgG(Sigma). Microtubules were viewed with a chilled video-ratedCCD camera (model C5985, Hamamatsu, Japan) connected to a computer(Apple Power Macintosh G3/400, Cupertino, CA). Images were processedby use of Adobe Photoshop (version 4).

RESULTS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The cofactor A homolog in fission yeast:
A homology search using human cofactor A as a query againstthe Schizosaccharomyces pombe genome database revealed thatfission yeast contains one ORF that encodes a homologous protein(30% identity and 52% similarity; Fig 1A). This value is closeto that between budding yeast Rbl2 and vertebrate cofactor A(29% identity and 57% similarity; ARCHER et al. 1995 ). Thecorresponding gene was designated alp31⁺ (altered polarity 31,as the gene is involved in growth polarity control, see below).The computer-assisted analysis of potential secondary structurespredicted that Alp31 and vertebrate cofactor A contain two internalcoiled-coil regions as shown in Fig 1B.

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Figure 1. Alp31 is a homolog of cofactor A. (A) Amino acid sequence comparison of fission yeast Alp31, human cofactor A, and budding yeast Rbl2. Amino acid residues, either identical (black) or conserved (gray), are emphasized. (B) Predicted coiled-coil structure of Alp31 and human cofactor A. Coiled-coil probability was determined by the Macstripe 2.0 program using window lengths of 21 amino acid residues.

alp31⁺ is a nonessential gene:
As a first step in addressing the cellular function of alp31⁺,gene disruption was performed. The entire ORF of one of thetwo chromosomal alp31⁺ genes in a diploid was deleted (PR21; Table 2) and tetrad analysis was performed. In contrast toour previous results, which demonstrated that the cofactor B,D, and E homologs encoding alp11⁺, alp1⁺, and alp21⁺, respectively,are essential for cell viability (HIRATA et al. 1998 ; RADCLIFFEet al. 1999 ), the alp31-deleted ( ${Delta}$ alp31) cells were viable (Fig 2A). ${Delta}$ alp31 cells were neither ts nor cs. Their doubling timewas 150 min in rich medium at 30°, whereas that of wildtype was 130 min (Fig 2B), showing a modestly prolonged celldivision. The absence of Alp31 did not alter sensitivity toantimicrotubular drugs (Fig 2C). However, a small population(2–5%) of ${Delta}$ alp31 cells showed either bent or branched morphology(arrowheads in Fig 2D, a and c), which has never been observedin wild-type cells (Fig 2D, Fig B and Fig D) and is indicativeof growth polarity defects ascribable to compromised microtubulefunction (UMESONO et al. 1983B ; HIRAOKA et al. 1984 ). Thisresult suggested that the fission yeast cofactor A homolog,although not essential, plays a role in microtubule integrity.

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Figure 2. alp31⁺ is not essential for cell viability. (A) Gene disruption of alp31⁺. A set of four segregants (a, b, c, and d: PR23, PR22, PR25, and PR24, respectively; Table 2) dissected from one ascus were grown on a rich YE5S plate at 29° (top) or at 36° (bottom), or on a YE5S plate containing 100 µg/ml of G418 (middle). (B) Growth curve of an alp31-deleted strain. Wild-type (PR22) or ${Delta}$ alp31 (PR23) cells were grown in rich liquid medium at 30° and cell number was measured. (C) Wild-type (WT, HM123) and alp31-deleted strains ( ${Delta}$ alp31, PR26) were spotted onto rich YPD (-TBZ, left) or YPD plates containing 20 µg/ml of thiabendazole (+TBZ, right) as serial dilutions (10⁶ cells in the top row and then diluted 10-fold in each subsequent spot below) and incubated at 30°. (D) Cell morphology of alp31-deleted mutants. Phase-contrast micrograph of cells taken from plates in A was presented. Branched cells are marked by arrowheads. Bar, 10 µm.

alp31-deleted cells have unstable microtubule structures but normal cellular levels of tubulins:
The altered morphology of ${Delta}$ alp31 cells suggests that microtubulefunction is somehow compromised. To examine this possibility,indirect immunofluorescence microscopy was performed using antitubulinantibody. It was found that microtubules are indeed defectivein ${Delta}$ alp31. Using standard fixation conditions under which filamentousmicrotubules of wild-type cells were easily visualized (Fig 3A,bottom), no intact microtubules were evident, instead eithershort, dotted, or misoriented microtubules were observed (top).It appears that microtubules become highly unstable in the absenceof Alp31^A.

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Figure 3. alp31-deleted cells have unstable microtubules and are sensitive to increased levels of the cofactor E homolog Alp21. (A) Defective microtubule structures in the alp31 disruptant. ${Delta}$ alp31 (top) or wild-type cells (bottom) were fixed, stained with anti-tubulin antibody (TAT-1, left), and processed for immunofluorescence microscopy. Chromosomal DNAs were stained with 4',6-diamidino-2-phenylin-dale (DAPI; right). Bar, 10 µm. (B) Tubulin levels. Cell extracts were prepared from ${Delta}$ alp31 (lane 1), wild type (lane 2), or wild type containing an empty plasmid (lane 3), or plasmid containing nmt1-alp31⁺ (pREP1-alp31⁺, lane 4, 24 hr in minimal medium). Immunoblotting was performed with anti-ß-tubulin antibody (KMX-1), anti- ${alpha}$ -tubulin antibody (TAT-1), or anti-Cdc2 antibody. (C) Lethal overexpression of alp21⁺ in ${Delta}$ alp31 cells. ${Delta}$ alp31 cells containing the plasmids (clockwise from top) pREP1-alp21⁺, pREP1-alp11⁺, pREP1, pDB(alp1⁺), pREP1-alp31⁺, pREP1, or pREP1-alp1⁺ were streaked on minimal plates in the presence (left plate) or absence (middle) of thiamine and incubated at 26° for 3 days.

We showed previously that the temperature-sensitive alp1 andalp11 mutants, in which microtubules fail to assemble at therestrictive temperature, show reduced levels of ${alpha}$ -tubulin (RADCLIFFEet al. 1999 ). To examine whether a similar phenomenon occurredin ${Delta}$ alp31 cells, immunoblotting was performed against extractsprepared from this mutant. In contrast to the finding for thealp1 and alp11 mutants, the amount of either ${alpha}$ -tubulin or ß-tubulindid not alter significantly in this mutant (Fig 3B). This resultis in line with the relatively mild phenotypes of a ${Delta}$ alp31 strainand supports the view that the pathway in which Alp31^A is involvedplays a more minor role than Alp11^B, Alp21^E, and Alp1^D.

To further examine the effect of loss of Alp31^A, in particularin terms of the disturbance of the relative stoichiometry amongcofactors, each cofactor homolog was overproduced in ${Delta}$ alp31 cells.In addition to Alp1^D and Alp11^B, which have been shown to betoxic even in a wild-type background (HIRATA et al. 1998 ; RADCLIFFE et al. 1999 ), it was found that Alp21^E, which doesnot interfere with the growth of wild-type cells, completelyinhibits colony formation in ${Delta}$ alp31 cells (Fig 3C). Thus Alp31^Ais important for maintaining viability under the conditionswhere the level of Alp21^E is increased. It is of note that multicopyplasmids containing nda2⁺ ( ${alpha}$ 1-tubulin) or nda3⁺ (ß-tubulin)were not capable of suppressing the morphological defects of ${Delta}$ alp31 cells.

Genetic interaction between alp31 deletion and mutations in genes involved in microtubule function:
To examine the interaction between Alp31 and tubulins, geneticcrosses were performed between ${Delta}$ alp31 and ts or cs tubulin mutantssuch as cs nda2 (encoding ${alpha}$ 1-tubulin; TODA et al. 1984 ), deletedor ts atb2 ( ${alpha}$ 2-tubulin; ADACHI et al. 1986 ; RADCLIFFE et al.1998 ), and ts or cs nda3 (ß-tubulin; HIRAOKA et al.1984 ; RADCLIFFE et al. 1998 ). Strong synthetic interactionswere found with both ts and cs ß-tubulin mutants. ${Delta}$ alp31was synthetically lethal with ts nda3-1828 (Fig 4A), and inthe case of cs nda3-311, double mutants were not capable offorming colonies at 26° (Fig 4B), which was permissive foran nda3-311 single mutant. On the other hand, mutants defectivein ${alpha}$ -tubulin genes did not show synthetic phenotypes (Table 3).These results suggest that Alp31, although nonessential, isinvolved in the ß-tubulin pathway as reported for otherorganisms (ARCHER et al. 1995 ; LEWIS et al. 1997 ).

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Figure 4. Genetic interaction of alp31-deleted mutant and rescue by budding yeast RBL2. (A) Synthetic lethal interaction between alp31 deletion and ts nda3. Tetrad analyses between ${Delta}$ alp31 (PR31) and nda3-1828 (DHH1828) strains were performed and spores were germinated at 26°. Segregation patterns (TT, tetratype; PD; parental ditype; NPD, nonparental ditype) of each tetrad (numbers 1–8) are shown. Nonviable spores are all ${Delta}$ alp31nda3-1828 double mutants. (B) Synthetic interaction between alp31 deletion and cs nda3. Four different segregants (HM123, PR31, KM311-201, and TP509-1B) were streaked on rich plates and incubated at 30° (left) or 26° (middle) for 4 days. (C) Suppression of the morphological defects of ${Delta}$ alp31 by RBL2. Cell morphology of ${Delta}$ alp31 (PR31) containing vectors (pREP1 and pREP2, left) or plasmids carrying RBL2 (pREP1 and pA21A, right) is shown. Bar, 10 µm.

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Table 3. Genetic interaction between alp31 and mutations in tubulin genes

To examine whether cofactor A from another organism is capableof complementing ${Delta}$ alp31, multicopy plasmids containing the buddingyeast RBL2 gene were introduced into ${Delta}$ alp31 cells. Compared tothe altered cell morphology of transformants containing emptyvectors only (Fig 4C, left), ${Delta}$ alp31 cells expressing RBL2 showedalmost normal cylindrical shape (right), indicating that RBL2suppressed the polarity defects of ${Delta}$ alp31 cells. Therefore, notonly from structural similarity, but also on the basis of functionalcomplementation, Alp31 is the fission yeast homolog of cofactorA.

Ectopic overexpression of alp31⁺ is toxic and results in abnormal microtubules:
To examine the phenotypes arising from overproduction of Alp31^A,the entire ORF of the alp31⁺ gene was inserted into plasmidscontaining the thiamine-repressible nmt1 promoter (pREP1-alp31⁺).It was found that alp31⁺ is deleterious to the cell as Alp31^A-overproducingcells show elongated, sometimes bent, morphology (Fig 5A). Itis of note that pREP1-alp31⁺ did not perturb growth or colonyformation; the abnormally elongated Alp31^A-overproducing cellscould manage to divide and form colonies (Fig 5C).

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Figure 5. Ectopic overproduction of Alp31 results in compromised microtubule structures. (A) Cell morphology of Alp31-overproducing cells. Wild-type cells containing an empty vector (pREP1, left) or plasmid containing nmt1-alp31⁺ (pREP1-alp31⁺, right) were grown in the absence of thiamine (derepressed conditions) for 24 hr at 30°. (B) Defective microtubules in Alp31-overproducing cells. Cultures used in A were fixed and processed for immunofluorescence microscopy using anti-tubulin antibody (TAT-1, top). Chromosomal DNAs were stained with DAPI (bottom). Bar, 10 µm. (C) Toxic overproduction of Alp31 in ß-tubulin mutant. pREP1-alp31⁺ was introduced into wild type, ${Delta}$ alp31, or ts nda3-1828 mutants. Transformants were streaked on minimal plates in the presence (left) or absence (middle) of thiamine and incubated at 26° for 4 days.

To examine whether overproduction of Alp31^A results in defectsin microtubule integrity, immunofluorescence microscopy wasperformed with anti-tubulin antibody. Staining of these alp31⁺-overexpressingcells with anti-tubulin antibody revealed that in the majorityof cells no intact microtubules were present, instead none,shorter, or dotted microtubule structures were evident (Fig 5B).In spite of their defective microtubules, the total amountof tubulin molecules was unaltered in Alp31^A-overproducing cells(Fig 3B, lane 4). It is concluded that an excess amount of Alp31^Adisrupts normal microtubules, leading to growth polarity defectswithout affecting the overall level of ${alpha}$ - and ß-tubulinmolecules.

To examine the effect of excess Alp31^A in a ß-tubulinmutant, pREP1-alp31⁺ was introduced into a ts nda3 strain. Asshown in Fig 5C, overproduction of Alp31^A resulted in inhibitionof colony formation in the absence of thiamine. Similar experimentswere performed in ts ${alpha}$ 2-tubulin mutants, but no strong toxicitywas observed (Table 3). These results indicate that the cellularlevel of Alp31^A has to be precisely regulated, that either aloss or excess of the protein results in defects in microtubuleintegrity, and that Alp31^A shows genetic interactions with ß-tubulin,but not ${alpha}$ -tubulin.

Alp31^A does not coprecipitate with Alp1^D, Alp11^B, or tubulins:
As shown previously (RADCLIFFE et al. 1999 ), Alp11^B binds ${alpha}$ -tubulinin the cell. We sought to find out whether Alp31^A forms a stablecomplex with ß-tubulin. To this end, the chromosomal alp31⁺gene was tagged with GST at its C terminus (MATERIALS AND METHODS).Tagging did not interfere with Alp31 function, as a haploidstrain containing Alp31-GST did not show any discernible abnormalityin cell morphology (PR27; Table 2). Immunoblotting using anti-GSTantibody showed that a tagged strain specifically contains animmunoreactive band of 50 kD that corresponded to the predictedsize of Alp31-GST (25 + 25 kD; Fig 6A). Also, a doubly taggedstrain containing Alp1-HA and Alp31-GST was constructed (PR28).Using these strains, immunoprecipitation was performed withanti-GST antibody. Neither Alp1^D and Alp11^B nor ${alpha}$ -/ß-tubulinco-immunoprecipitated (Fig 6B, lanes 4 and 6, note that somelevel of ${alpha}$ - and ß-tubulins precipitated nonspecificallyby binding to beads). Furthermore, reciprocal immunoprecipitationexperiments using anti-HA as a primary antibody showed thatAlp1^D does not coprecipitate with Alp31^A or ${alpha}$ - or ß-tubulin(lanes 10 and 12). This shows a clear difference between theproperties of Alp31^A and of Alp11^B, which tightly binds ${alpha}$ -tubulinunder the same conditions (RADCLIFFE et al. 1999 ).

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Figure 6. Characterization of the Alp31 protein. (A) Identification of the alp31⁺ gene product by chromosomal tagging. The chromosomal alp31⁺ gene was tagged with GST at its C terminus. Cell extracts were prepared from the parental (untagged) strain (lane 1) or three independent tagged strains (PR27, lanes 2–4), and immunoblotting was performed with anti-GST antibody. Alp31-GST (50 kD) is emphasized with an arrow and a nonspecific band (22 kD) is marked with a black dot. The position of size markers is shown at the right. (B) Lack of interaction between Alp31 and the other cofactors and tubulins. Cell extracts were prepared from an untagged wild-type (lanes 1 and 7), singly tagged (Alp31-GST, PR27, lanes 2, 6, 8, and 12), or doubly tagged strain (Alp31-GST Alp1-HA, PR28, lanes 3, 4, 5, 9, 10, and 11). Immunoprecipitation was performed with either anti-GST (lanes 4, 6, and 7), anti-HA antibody (lanes 10 and 12), or mock treatment (beads only, lanes 5 and 11). Precipitated proteins were detected with anti-HA, anti-ß-tubulin, anti-GST, anti-Alp11 or anti- ${alpha}$ -tubulin antibodies. Total cell extracts (corresponding to 1/30 amount used for immunoprecipitation) were also run (lanes 1, 2, 3, 8, and 9).

Alp31^A exists in a complex distinct from Alp1^D, Alp11^B, and tubulins:
Next, the native size of Alp31 was analyzed by gel filtrationchromatography. As shown in Fig 7, it was found that Alp31^Adid not cofractionate with any of the proteins examined (Alp1^D,Alp11^B, and tubulins) and existed predominantly in fractionsbetween tubulins and Alp11^B (fractions 21–23; Fig 7).This is consistent with the previous results showing that Alp31^Aforms a stable interaction with neither Alp11^B and Alp1^D nortubulins (by immunoprecipitation; Fig 6B). It is of note thata subpopulation of Alp1^D, Alp11^B, and tubulins (and Alp21^E; RADCLIFFE et al. 1999 ) exists in a large complex (>20S), butthis is not the case with Alp31^A, although at a smaller position(200–300 kD), Alp31^A appeared to cofractionate with ${alpha}$ -tubulin(lanes 21–23) and also ß-tubulin (RADCLIFFE andTODA 2000 ).

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Figure 7. Size fractionation of the Alp31 protein. Gel filtration chromatography. Soluble extracts from a doubly tagged strain (Alp31-GST Alp1-HA, PR28) were separated through a Superose-6 column and fractions were analyzed by immunoblotting with anti-Alp11, anti-GST, anti-HA, and anti- ${alpha}$ -tubulin antibodies. Total extract (10 µg) was also run (far left lane). Numbers above (1–35) correspond to fraction numbers. Positions of size markers (43, 232, 669, and 2000 kD) are also shown.

Taken together, the data show that Alp31^A plays an importantrole in microtubule integrity; however, compared to Alp11^B,Alp21^E, and Alp1^D, which are indispensable for maintaining ${alpha}$ -tubulinlevels, microtubule structures, and cell survival, its requirementis less stringent.

DISCUSSION

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Our analysis highlights a clear differentiation between ${alpha}$ - andß-tubulins in their requirement for cofactors in the microtubulebiogenesis pathways. We have shown that cells lacking Alp31^A,the cofactor A homolog (structural and functional), grow anddivide despite morphological defects. The possibility that fissionyeast has another homolog for cofactor A is not formally excluded;however, it is unlikely, as a homology search against the fissionyeast genome database shows Alp31 is the only homolog (>98%of the genomic sequence has been completed; the Sanger Centre,Hixton, UK). Nonessentiality of Alp31^A is in clear contrastto findings for Alp11^B, which is absolutely required for celldivision and viability (Fig 8). It has been proposed that cofactorA is a cochaperonin, which interacts with ß-tubulin releasedfrom chaperonin complexes (GAO et al. 1994 ). Furthermore byanalogy to the role of cofactor B for ${alpha}$ -tubulin (TIAN et al.1997 ; RADCLIFFE et al. 1999 ), cofactor A may function tomaintain a reservoir of partially folded ß-tubulins (ARCHERet al. 1995 ; TIAN et al. 1996 ). This explains why overproductionof Alp31^A results in the disappearance of intact microtubulestructures associated with cell polarity defects; excess Alp31^Amay sequester a pool of free ß-tubulin molecules. Consistentwith this, we have shown that the overproduction of Alp31^A resultsin greater toxicity in strains containing mutations in ß-tubulin.Compared to Alp11^B, which contains a conserved motif (CLIP-170domain) responsible for binding ${alpha}$ -tubulin (LEWIS et al. 1997; FEIERBACH et al. 1999 ; RADCLIFFE et al. 1999 ), the aminoacid sequence of Alp31^A does not give any significant cluesas to putative protein-protein interactions, except that itcontains two coiled-coil domains with structural similaritiesto the DnaJ protein (this study; LLOSA et al. 1996 ; MELKIet al. 1996 ). It seems likely that the binding properties ofcofactor A/ß-tubulin and cofactor B/ ${alpha}$ -tubulin differ atthe molecular level.

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Figure 8. Essential and nonessential pathways for in vivo microtubule biogenesis. The two pathways required for microtubule biogenesis in fission yeast are shown. Small shaded circles surrounding ${alpha}$ - and ß-tubulin molecules represent the chaperonin complex. The linear sequential pathway (top) in which the cofactor homologs Alp11^B, Alp21^E, and Alp1^D are involved mainly functions to control ${alpha}$ -tubulin availability. Alp41 is a conserved GTPase, which functions prior to Alp1^D, probably in concert with Alp21^E (RADCLIFFE et al. 2000

). Without these proteins, cells fail to maintain normal ${alpha}$ -tubulin levels and lose microtubule structures, resulting in cell division defects. On the other hand, the role of Alp31^A in microtubule integrity, however, is dispensable. Alp31 is most likely to function, like its homologs in other organisms, in the ß-tubulin-dependent pathway.

Genetic analysis highly suggests that Alp31^A regulates the ß-tubulinpathway, rather than the ${alpha}$ -tubulin pathway, in which Alp11^B,Alp21^E, and Alp1^D are involved. This notion is consistent withthe proposed role of cofactor A in the correct folding of ß-tubulin(LEWIS et al. 1997 ). alp31-deleted cells have compromised microtubules;no intact cytoplasmic microtubules were observed under immunofluorescencemicroscopy. There is evidence that fission yeast cells can growwithout cytoplasmic microtubules (SAWIN and NURSE 1998 ). However,mitotic spindles are absolutely essential for cell division.It is possible that Alp31^A is mainly involved in the integrityof cytoplasmic microtubules and its requirement for spindleformation is less stringent. The reason that Alp31^A is dispensable,therefore, might be ascribable to the differential requirementfor Alp31^A between cytoplasmic and spindle microtubules. ${Delta}$ alp31cells are sensitive to ectopic overexpression of Alp21^E, thebasis of which is currently unknown. It is possible that furtherunbalance of the stoichiometry of molecules between functional ${alpha}$ - and ß-tubulins, caused by the combination of overproducedAlp21^E and the absence of Alp31^A, is deleterious for the cell.

The in vivo dispensability of Alp31^A may correlate to the previousresults reported for the folding pathways in vertebrates fromin vitro data. In this system, although cofactor A binds partiallyfolded ß-tubulin intermediates, it does not participatein folding reactions per se when reactions are performed usingpurified components (TIAN et al. 1996 ). In contrast the requirementof cofactor B is more stringent both in vitro and in vivo (RADCLIFFEet al. 1999 ). It is possible that, upon release from chaperonincomplexes, unlike ${alpha}$ -tubulin, ß-tubulin can be folded byitself to some extent without cofactor A, such that it is ina conformational state capable of interacting with other cofactorsand ${alpha}$ -tubulin. This view is consistent with the fact that ß-tubulinappears more stable than ${alpha}$ -tubulin in the absence of cofactorfunction in fission yeast cells (this study; RADCLIFFE et al.1999 ) and that overproduction of ß-tubulin is in generalmore toxic than that of ${alpha}$ -tubulin (HIRAOKA et al. 1984 ; BURKEet al. 1989 ; KATZ et al. 1990 ; WEINSTEIN and SOLOMON 1990).

We failed to see a physical interaction between Alp31^A and ß-tubulinby immunoprecipitation, as opposed to results reported for counterpartsin other organisms (mammalian cofactor A and budding yeast Rbl2; ARCHER et al. 1995 , ARCHER et al. 1998 ; LEWIS et al. 1997; VEGA et al. 1998 ). Gel filtration chromatography shows thatan interaction between Alp31^A and ß-tubulin might be eitherweaker or more delicate in fission yeast. Given the defectivephenotypes of alp31-deleted cells, however, it is unambiguousthat alp31⁺ is involved in microtubule integrity in the cell.These defects include altered cell shape (bent or branched),synthetic lethal interaction with mutations in ß-tubulin,hypersensitivity to the overproduction of, usually nontoxic,Alp21^E, and unstable microtubule structures. The cell shapedefects seen in ${Delta}$ alp31 cells are reminiscent of microtubule defectsin fission yeast (UMESONO et al. 1983B ; HIRAOKA et al. 1984; MATA and NURSE 1997 ; RADCLIFFE et al. 1998 ; SAWIN andNURSE 1998 ). It is of note that, although overproduction ofAlp21^E has no discernible effects in wild-type cells (RADCLIFFEet al. 1999 ), it is toxic in the cold-sensitive nda2-52 mutant(defective in ${alpha}$ 1-tubulin; GRISHCHUK and MCINTOSH 1999 ). Therefore,although the cellular levels of both ${alpha}$ - and ß-tubulin moleculesappear normal, the quality of tubulins must be somehow compromisedin the absence of Alp31^A.

In summary we have shown that the cofactor-dependent microtubulebiogenesis in vivo requires two separate pathways, one essential(Alp11^B-Alp21^E-Alp1^D) and the other nonessential (Alp31^A; Fig 8).These results strongly imply that ${alpha}$ - and ß-tubulinsshould not be regarded simply as evolutionarily duplicated partners,instead these two proteins must be functionally and biochemicallydistinct. It is well established that, in addition to theirasymmetrical positioning in ${alpha}$ /ß-heterodimers along microtubulepolymers, with regards to GTP binding, these two proteins differ;while ${alpha}$ -tubulin-GTP is nonexchangeable, GTP bound by ß-tubulinis exchangeable and also hydrolyzable (BURNS and FARRELL 1996). These differences may explain why most of the antimitoticdrugs acting through microtubules, such as thiabendazole compounds,colchicine, and paclitaxel, target ß-tubulin, rather than ${alpha}$ -tubulin (UMESONO et al. 1983B ; RAO et al. 1994 ; BAI etal. 1996 ). The screening of new drugs that affect microtubuleintegrity via cofactor functions might be a novel avenue foragriculture or pharmaceutics toward the improvement of foodproduction or remedies for microtubule-related human diseases.

FOOTNOTES

¹ Present address: Oxford Biomedica (UK) Ltd., Oxford OX44GA,United Kingdom.

ACKNOWLEDGMENTS

We thank Drs. Kate Compton, Keith Gull, Paul Nurse, Frank Solomon,and Hiroyuki Yamano for providing materials used in this study.We thank Dr. Jacqueline Hayles for critical reading of the manuscriptand useful suggestions. M.A.G. was supported by a European MolecularBiology Organization long-term fellowship.

Manuscript received December 18, 1999; Accepted for publication May 22, 2000.

LITERATURE CITED

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
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