Tubulin Sorting during Dimerization In Vivo

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Vol. 12, Issue 7, 2185-2194, July 2001

Tubulin Sorting during Dimerization In Vivo

Henry D. Hoyle,^* F. Rudolf Turner, Linda Brunick, and Elizabeth C. Raff

Department of Biology and Indiana Molecular Biology Institute, Indiana University, Bloomington, Indiana 47405

Submitted January 31, 2001; Accepted April 16, 2001
Monitoring Editor: J. Richard McIntosh

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

We demonstrate sorting of $beta$ -tubulins during dimerization in the Drosophila male germ line. Different $beta$ -tubulin isoforms exhibitdistinct affinities for $alpha$ -tubulin during dimerization. Our datasuggest that differences in dimerization properties are importantin determining isoform-specific microtubule functions. The differentialuse of $beta$ -tubulin during dimerization reveals structural parametersof the tubulin heterodimer not discernible in the resolved three-dimensionalstructure. We show that the variable $beta$ -tubulin carboxyl terminus,a surface feature in the heterodimer and in microtubules, andwhich is disordered in the crystallographic structure, is of keyimportance in forming a stable $alpha$ - $beta$ heterodimer. If the availabilityof $alpha$ -tubulin is limiting, $alpha$ - $beta$ dimers preferentially incorporateintact $beta$ -tubulins rather than a $beta$ -tubulin missing the carboxylterminus ( $beta$ 2 $Delta$ C). When $alpha$ -tubulin is not limiting, $beta$ 2 $Delta$ C forms stable $alpha$ - $beta$ heterodimers. Once dimers are formed, no further sorting occursduring microtubule assembly: $alpha$ - $beta$ 2 $Delta$ C dimers are incorporated intoaxonemes in proportion to their contribution to the total dimerpool. Co-incorporation of $beta$ 2 $Delta$ C and wild-type $beta$ 2-tubulin resultsin nonmotile axonemes because of a disruption of the periodicityof nontubulin axonemal elements. Our data show that the $beta$ -tubulincarboxyl terminus has two distinct roles: 1) forming the $alpha$ - $beta$ heterodimer,important for all microtubules and 2) providing contacts for nontubulincomponents required for specific microtubule structures, suchasaxonemes.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Microtubules support the assembly of cytoskeletal structures of diverse morphology and function. The basic building blocksof all microtubules are heterodimers composed of $alpha$ - and $beta$ -tubulinsencoded by multiple gene families. Studies of Drosophila developmenthave demonstrated functional specialization of microtubules assembledfrom differentially expressed $alpha$ - and $beta$ -tubulin isoforms (Hoyleand Raff, 1990; Matthews et al., 1993; Hoyle et al., 1995, 2000;Hutchens et al., 1997; Dettman et al., 2001). We have used Drosophilaspermatogenesis as a model system to compare the intrinsic capacityof different $alpha$ - and $beta$ -tubulins to assemble into different microtubules.In the Drosophila male germ line, a single $alpha$ - $beta$ heterodimer speciescomposed of the ubiquitous $alpha$ 84B-tubulin and the testis-specific $beta$ 2-tubulin, supports all postmitotic microtubule functions, includingassembly of the sperm tail flagellum, Drosophila's only motileaxoneme (Kemphues et al., 1979, 1980, 1982, 1983; Matthews etal., 1989). We have discovered that the constituent tubulins candetermine several levels of microtubule organization, includingmicrotubule protofilament number, morphology of specific setsof microtubules, and overall organization of axoneme superstructure(Fackenthal et al., 1993; Hoyle et al., 1995; Hutchens et al.,1997; Raff et al., 1997, 2000). These studies demonstrated thatdifferent $alpha$ - $beta$ dimers contribute to differences in microtubulearchitecture and function. Here we ask a more basic question:Does the process of $alpha$ - $beta$ dimerization discriminate between tubulinisotypes? To address this we have looked at the process of tubulindimerization in vivo in the Drosophila male germline.

Biochemical studies by Cowan, Lewis, and their colleagues identified components of the molecular machinery that guides formationof $alpha$ - $beta$ -tubulin heterodimers (Gao et al., 1992, 1994; Tian et al.,1996, 1997, 1999). After initial in vivo folding of nascent (orin vitro, denatured) tubulin subunits via TriC chaperonin, finalfolding and dimerization occur in a "dimerization machine," asupermolecular complex comprising $alpha$ - and $beta$ -tubulin and at leastfive tubulin-specific chaperones. Because the heterodimer is thestable form of native tubulin, biochemical preparations alwayscontain equimolar amounts of $alpha$ - and $beta$ -tubulin. With the Drosophilamale germ line we are able to determine the consequences for tubulindimerization in vivo when synthesis of $alpha$ - and $beta$ -tubulin is notequimolar (Hoyle et al., 1995; Hutchens et al., 1997).

In this study, we examined the role of the $beta$ -tubulin carboxyl terminus in the dimerization process. The isotype-defining carboxylterminus of Drosophila $beta$ 2-tubulin is required for axonemes butis not essential for the assembly of functional cytoplasmic microtubules,including spindles (Fackenthal et al., 1993; Hoyle et al., 1995;Nielsen et al., 2001). The $alpha$ - and $beta$ -carboxyl termini are not resolvedin the electron crystallographic structure of the $alpha$ - $beta$ tubulindimer. Both termini are surface features of the $alpha$ - $beta$ dimer andlie on the outside of the microtubule wall (Wolf et al., 1996;Nogales et al., 1998, 1999). The resolved intradimer contactsbetween $alpha$ - and $beta$ -tubulin thus support the prediction that theC termini are dispensable for the heterodimer. We tested thishypothesis for the $beta$ -tubulin subunit by comparing the abilityof $beta$ 2 $Delta$ C, a carboxyl terminus-truncated form of $beta$ 2-tubulin (Fackenthalet al., 1993), to form dimers when it was the sole $beta$ -tubulin inthe male germ cells or when different full-length $beta$ -tubulins werealso present. Our data show that the $beta$ -tubulin carboxyl terminusplays an important role in generating stable $alpha$ - $beta$ dimers and thatsorting between different $beta$ -tubulins takes place during dimerization.Competition between $beta$ 2 $Delta$ C and full-length $beta$ -tubulins revealed thatdifferent $beta$ -tubulin isoforms have distinct capacities for formingdimers with $alpha$ -tubulin. In vivo, many $beta$ -tubulins may be coexpressedin the same cell. We propose that isotype-specific differencesin the dimerization properties of different $beta$ -tubulins may playa key role in defining the cellular isoform content and, hence,in determining cell-type specific functions of the microtubulecytoskeleton.

Because we observed that tubulins were sorted during dimerization, we wondered whether further sorting would occur duringmicrotubule assembly. We found no evidence for this. Once formed, $beta$ 2 $Delta$ C-containing dimers were incorporated into axonemes at thesame ratio as they were present in the total dimer pool. As weshow here, these $beta$ 2 $Delta$ C-containing axonemes are structurally andfunctionally compromised, revealing that the periodicity of theinteractions of the $beta$ -tubulin carboxyl termini with nontubulincomponents is an essential feature of axonemearchitecture.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Drosophila Stocks

Stocks were maintained at 25°C to avoid temperature-induced effects on male fertility. The $beta$ 2-tubulin null allele, $beta$ 2^null, was described by Fackenthal et al. (1993). The deficiency chromosomethat deletes the $alpha$ 84B-tubulin gene, Df(3R)Scx⁴, was described by Hazelrigg and Kaufman (1983); for clarity,we have herein designated this as Df( $alpha$ 84B). Other Drosophila stocksare described in FlyBase (1999).

Gene Constructs

The transgenic construct p[ $beta$ 2 $Delta$ C] consists of the $beta$ 2 gene with stop codons engineered at amino acid positions 432 and 433,resulting in the deletion of the 15 carboxyl-terminal residues(construct B2t.432, Fackenthal et al., 1993). p[ $beta$ 2 $Delta$ C] supportsexpression of $beta$ 2 $Delta$ C-tubulin in the postmitotic male germ line ata level equivalent to the endogenous $beta$ 2-tubulin. Pulse-chase experimentshave shown that the intrinsic stability of $beta$ 2 $Delta$ C is only slightlyless than that of $beta$ 2 (Fackenthal et al., 1993; note that the pulse-chaseexperiments were performed under conditions where $alpha$ -tubulin wasnot limiting; see DISCUSSION and Figure 2.).

As described previously, the transgenic constructs p[ $beta$ 1], p[ $beta$ 3], and p[ $alpha$ 85E] were constructed with the use of a "testis vector"containing 2.1 kb of $beta$ 2 5' and 1.5 kb of $beta$ 2 3' sequences flankingthe indicated heterologous coding sequence. These $beta$ 2 regulatorysequences control expression of the inserted coding sequence atthe same level and tissue specificity as the endogenous $beta$ 2-tubulin(Hoyle et al., 1995; Hutchens et al., 1997; Raff et al., 2000).The transgenic construct p[ $alpha$ 84B] consists of the wild-type $alpha$ 84B-codingsequence and sufficient flanking genomic sequence to direct fullywild-type expression of $alpha$ 84B in the male germ line (Matthews etal., 1993; Hutchens et al., 1997).

Analysis of Drosophila Testis Tubulins

In the Drosophila testis, the ubiquitous $beta$ -tubulin, $beta$ 1, is the only $beta$ -tubulin expressed in the early, mitotic stages of spermatogenesis(Bialojan et al., 1984; Kaltschmidt et al., 1991). Before meiosis, $beta$ 1 is replaced by the testis-specific isoform, $beta$ 2-tubulin. $beta$ 2is then required for all microtubules, including meiotic spindles,all cytoplasmic microtubules, and the motile sperm tail axoneme(Kemphues et al., 1979, 1980, 1982, 1983). Both $beta$ 1 and $beta$ 2 dimerizewith $alpha$ 84B-tubulin, the only $alpha$ -tubulin expressed in the Drosophilamale germ line (Matthews et al., 1989). After the onset of spermatogenesisin late larval development, the testes become filled with developingspermatids. In the work presented here, all testes are from 1-day-oldadults, in which total testis proteins primarily represent postmitoticstages. The major tubulins in adult testes are thus postmitoticallyexpressed species, which consist of the endogenous isoforms $alpha$ 84Band $beta$ 2, or heterologous tubulins expressed from transgenic constructscontrolled by $beta$ 2 regulatoryelements.

Samples for two-dimensional gel analysis and immunoblotting were prepared from 1-day-old males as described by Hoyle and Raff(1990). Four testes labeled for 1 h with [³⁵S]methionine plus six unlabeled testes were used for each gelsample. Isoelectric focusing gradients were established with theuse of a 2:1 ratio of wide range (pH 3.0-10) to narrow range (pH4.0-6.0) ampholytes (Fluka, Buchs, Switzerland). Antibodies usedwere a commercial anti- $beta$ antibody (N357, Amersham Pharmacia Biotech,Piscataway, NJ) and anti- $alpha$ antibody (N356, Amersham PharmaciaBiotech); as previously documented, these antisera react withendogenous Drosophila testis tubulins and all experimental $beta$ -tubulinsused in this study (Hoyle et al., 1995; Hutchens et al., 1997;Raff et al., 2000). Primary antibodies were detected with theuse of a horseradish peroxidase-conjugated goat-anti-mouse secondaryantibody (Jackson ImmunoResearch, West Grove, PA) and detectedwith the use of 4-chloro-1-napthol and hydrogenperoxide.

In each experiment, the [³⁵S]methionine signal for each tubulin species provided a direct measure of the levels of synthesisduring 1 h of labeling. Antibody-staining signals on the sameblot provided a direct measure of the amount of each tubulin speciesthat accumulated in the stable tubulin pool during spermatid maturation,a process that takes 5 days (Lindsley and Tokuyasu, 1980). Comparisonbetween [³⁵S]methionine signal and antibody signal thus revealed the relativeextent of stable dimers formed by each tubulin species present.Different sites of insertion were tested for each gene construct.Multiple blots were run for each gene combination; all gave thedescribedphenotypes.

Determination of Male Fertility

Virgin males were collected and held away from females for 5 days. Sperm production was assayed by dissecting the reproductivetract and scoring for the presence of motile sperm in the seminalvesicles by light microscopy as described previously (Hoyle andRaff, 1990; Hoyle et al., 1995; Hutchens et al., 1997).

Electron Microscopy

Testes from 1-day-old males were fixed overnight in 2.5% gluteraldehyde and 0.1 M cacodylate, stained with 2% osmium tetroxideand 0.5% uranyl acetate, dehydrated, and imbedded in DER resin(Electron Microscopy Sciences, Fort Washington, PA). Sectioningand transmission electron microscopy were done by standardmethods.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The $beta$ -Tubulin Carboxyl Terminus Participates in Formation of Stable $alpha$ - $beta$ Heterodimers

We have used the Drosophila postmitotic male germ cells as an experimental system that allows us to assay tubulin dimerizationunder conditions where endogenous or heterologous tubulins canbe expressed at specific levels. The stable form of soluble tubulinis the $alpha$ - $beta$ heterodimer. In Drosophila, free, monomeric $alpha$ - or $beta$ -tubulinis degraded immediately after synthesis (Kemphues et al., 1982;Hoyle et al., 1995; Hutchens et al., 1997). We have previouslyshown that synthesis of both $alpha$ - and $beta$ -tubulin is directly proportionalto gene dose in the postmitotic male germ cells (Hoyle and Raff,1990; Hoyle et al., 1995). We have shown that this holds truefor the endogenous germ line tubulins, $beta$ 2 and $alpha$ 84B, as well asfor $beta$ 2 $Delta$ C and transgenic genes driven by $beta$ 2 regulatory sequences(see MATERIALS AND METHODS; Hoyle and Raff, 1990; Fackenthal etal., 1993; Hoyle et al., 1995; Hutchens et al., 1997; Raff etal., 2000). In wild-type testes, the quantity of $alpha$ matches thequantity of $beta$ , but the one "synthesis unit" per gene still holdstrue under experimental conditions in which the gene dose of $alpha$ does not equal the gene dose of $beta$ (Hutchens et al., 1997). Thus,as illustrated in Figure 1, we can examine the formation of stabletubulin dimers in vivo under conditions in which $alpha$ - and $beta$ -tubulinsynthesis is not balanced.

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Figure 1. Monomeric tubulins are unstable in the Drosophila male germ line. Total testis proteins from 1-day-old males were labeled with [³⁵S]methionine, separated by two-dimensional gel electrophoresis, blotted, and immunostained as described in MATERIALS AND METHODS. Left, autoradiograms showing labeled proteins. Right, the same blots stained with anti- $alpha$ -tubulin and anti- $beta$ -tubulin antibodies, showing stable testis tubulins. The $alpha$ signal is from $alpha$ 84B-tubulin (Matthews et al., 1989

; Hutchens et al., 1997

). (A) Testes from males with one functional copy of the wild-type $beta$ 2-tubulin gene in a wild-type $alpha$ 84B background (genes present: $beta$ 2⁺/ $beta$ 2^null; $alpha$ 84B⁺/ $alpha$ 84B⁺). The stable form of soluble tubulin is the $alpha$ - $beta$ heterodimer: the amount of stable $alpha$ 84B corresponds to the total amount of stable $beta$ -tubulin, primarily $beta$ 2-tubulin for this genotype. (B) Testes from $beta$ 2-null males (genes present: $beta$ 2^null/ $beta$ 2^null; $alpha$ 84B⁺/ $alpha$ 84B⁺). These males are sterile: each gonial cell produces 16 spermatocytes via four rounds of mitosis, but then spermatogenesis fails. $beta$ 2-Tubulin is not synthesized (arrows denote the normal position of $beta$ 2); the mature spermatocytes do not assemble meiotic spindles, and spermatids do not assemble axonemes or any other postmitotic microtubules. $alpha$ 84B is synthesized in the postmitotic cells (left), but in the absence of any $beta$ 2, there can be no formation of $alpha$ - $beta$ dimers and almost all of the newly synthesized $alpha$ 84B is rapidly degraded and fails to accumulate (right). The small amount of antibody-stained $alpha$ 84B represents $alpha$ 84B- $beta$ 1 dimers in premeiotic cells.

We tested the role of the $beta$ -tubulin C terminus in dimerization in experiments in which intact $beta$ -tubulins competed for dimerizationwith $alpha$ -tubulin with $beta$ 2 $Delta$ C, a truncated $beta$ 2-tubulin missing onlythe final 15 amino acids that constitute the variable C-terminalisotype-defining domain (Fackenthal et al., 1993). Figure 2 andTable 1 summarize experiments in which we determined the abilityof $beta$ 2 $Delta$ C to form stable dimers under conditions in which the availabilityof total $alpha$ - and $beta$ -tubulins was varied. We found that, when $beta$ 2 $Delta$ Cwas coexpressed with any full-length $beta$ -tubulin under conditionsin which $alpha$ -tubulin was limiting (i.e., the total $alpha$ -tubulin poolwas less than the total $beta$ -tubulin pool), the $beta$ 2 $Delta$ C component ofthe $beta$ -tubulin pool failed to dimerize, and $beta$ 2 $Delta$ C was degraded.Conversely, when $alpha$ -tubulin was not limiting, $beta$ 2 $Delta$ C formed stableheterodimers. We have found that stable $alpha$ - $beta$ 2 $Delta$ C heterodimers areincorporated into axonemes. This results in male sterility if $beta$ 2 $Delta$ C makes up more than one-third of the stable dimer pool (discussedbelow). We therefore used male sterility as a second assay forthe formation of stable $alpha$ - $beta$ 2 $Delta$ C dimers (Table 1).

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Figure 2. $beta$ 2 $Delta$ C-tubulin is stable only when $alpha$ -tubulin is not limiting. Two-dimensional gels of total testis proteins from 1-day-old males, prepared as described in MATERIALS AND METHODS. Left, autoradiograms showing [³⁵S]methionine-labeled proteins. Right, the same blots stained with anti- $alpha$ -tubulin and anti- $beta$ -tubulin antibodies, showing stable testis tubulins. (A) Testis proteins from sterile males with two gene doses of $alpha$ 84B (wild type at the $alpha$ 84B locus), one copy of $beta$ 2 $Delta$ C, and no $beta$ 2-tubulin (genes present: p[ $beta$ 2 $Delta$ C]; $beta$ 2^null/ $beta$ 2^null; $alpha$ 84B⁺/ $alpha$ 84B⁺). $beta$ 2 $Delta$ C is the only $beta$ -tubulin synthesized in the postmitotic cells and is stable (comparable to the stability of $beta$ 2 itself shown in Figure 1A). Arrow denotes the normal position of $beta$ 2. (B) Testis proteins from fertile males that are wild type at the $alpha$ 84B and $beta$ 2 loci and also carrying one copy of p[ $beta$ 2 $Delta$ C] (genes present: p[ $beta$ 2 $Delta$ C]; $beta$ 2⁺/ $beta$ 2⁺; $alpha$ 84B⁺/ $alpha$ 84B⁺). There are two gene doses of $alpha$ -tubulin and three gene doses of total $beta$ -tubulin. $beta$ 2 $Delta$ C is synthesized but is unstable; stable tubulin in the postmitotic cells consists primarily of $alpha$ 84B- $beta$ 2 dimers. $beta$ 1 staining reflects the contribution of premeiotic germ cells to total testis tubulins. The amount of total protein on this gel is large enough to also allow detection of the endogenous $beta$ 3-tubulin present in the somatic cyst cells (Kimble et al., 1989

; Hoyle and Raff, 1990

). (C) Testis proteins from fertile males that are wild type at the $alpha$ 84B and $beta$ 2 loci but also carrying four copies of p[ $beta$ 2 $Delta$ C]. There are two gene doses of $alpha$ -tubulin and six total gene doses of $beta$ -tubulin. There is more stable $beta$ 2 $Delta$ C than in the genotype shown in Figure 2B, but the amount of stable $beta$ 2 $Delta$ C is less than $beta$ 2 and much less than when $beta$ 2 $Delta$ C is the only $beta$ -tubulin available in the postmitotic cells (compare with Figure 2A). (D) Testis proteins from sterile males carrying one copy each of p[ $beta$ 2 $Delta$ C] and $beta$ 2 and wild type at the $alpha$ 84B locus (genes present: p[ $beta$ 2 $Delta$ C]; $beta$ 2⁺/ $beta$ 2^null; $alpha$ 84B⁺/ $alpha$ 84B⁺). There are two total gene doses of $beta$ -tubulin and two gene doses of $alpha$ -tubulin. $beta$ 2 $Delta$ C is stable, accumulating to an amount only slightly less than endogenous $beta$ 2. (E) Testis proteins from sterile males carrying one copy of p[ $alpha$ 84B], one copy of p[ $beta$ 2 $Delta$ C], and wild type at the endogenous $alpha$ 84B and $beta$ 2 loci (genes present: p[ $beta$ 2 $Delta$ C]; p[ $alpha$ 84B]; $beta$ 2⁺/ $beta$ 2⁺; $alpha$ 84B⁺/ $alpha$ 84B⁺). There are three total gene doses of $alpha$ -tubulin and three total gene doses of $beta$ -tubulin. $beta$ 2 $Delta$ C is stable. (F) Testis proteins from sterile males with one gene dose each of $beta$ 2 $Delta$ C, $alpha$ 84B and $beta$ 2 (genes present: p[ $beta$ 2 $Delta$ C]; $beta$ 2⁺/ $beta$ 2^null; $alpha$ 84B⁺/Df[ $alpha$ 84B]). There are two gene doses of total $beta$ -tubulin but only one gene dose of $alpha$ -tubulin. The rates of $beta$ 2 $Delta$ C and endogenous $beta$ 2 synthesis are comparable (left). However, $beta$ 2 $Delta$ C is unstable (right). (G) Testis proteins from fertile males carrying two gene doses of $alpha$ 84B and one gene dose each of $beta$ 2, $beta$ 2 $Delta$ C, and transgenic $beta$ 1 (genes present: p[ $beta$ 2 $Delta$ C]; p[ $beta$ 1]; $beta$ 2⁺/ $beta$ 2^null; $alpha$ 84B⁺/ $alpha$ 84B⁺). There are three gene doses of total $beta$ -tubulin and only two gene doses of $alpha$ -tubulin. The stability of $beta$ 2 $Delta$ C is reduced but to a lesser degree than when $beta$ 2 is the sole competing full-length $beta$ -tubulin (compare B and C). (H) Testis proteins from males carrying two gene doses of $alpha$ 84B and one gene dose each of $beta$ 2, $beta$ 2 $Delta$ C and transgenic $beta$ 3 (genes present: p[ $beta$ 2 $Delta$ C]; p[ $beta$ 3]; $beta$ 2⁺/ $beta$ 2^null; $alpha$ 84B⁺/ $alpha$ 84B⁺). There are three gene doses of total $beta$ -tubulin and only two gene doses of $alpha$ -tubulin. The stability of $beta$ 2 $Delta$ C is reduced, comparable to the genotype in G. (Note that males with equal gene doses of p[ $beta$ 3]and $beta$ 2 are sterile with or without $beta$ 2 $Delta$ C; see Table 1, lines 18 and 19.)

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Table 1. The $beta$ -tubulin carboxyl terminus functions in forming stable $alpha$ , $beta$ -tubulin heterodimers

Figure 2A shows that, when $beta$ 2 $Delta$ C was the only $beta$ -tubulin expressed in the postmitotic germ cells, $beta$ 2 $Delta$ C formed stable dimerswith $alpha$ 84B-tubulin. Under these conditions, $beta$ 2 $Delta$ C is itself stable(Table 1, lines 1and 2) and rescues the instability of $alpha$ 84B,which is otherwise unstable in the absence of endogenous $beta$ 2 (asshown in Figure 1B). $beta$ 2 $Delta$ C-containing heterodimers can be assembledinto microtubule arrays that exhibit at least partial function,including meiotic spindles and the cytoplasmic microtubules thatmediate mitochondrial elongation. However, $beta$ 2 $Delta$ C cannot assembleaxonemes (Figure 3; Fackenthal et al., 1993). Here we report experimentsin which coexpression of $beta$ 2 $Delta$ C and intact $beta$ -tubulins reveals anew role for the C terminus in stabilization of heterodimers.Our data thus show that, although dimerization and microtubuleassembly per se are not dependent on the $beta$ -tubulin C terminus,it nonetheless plays a crucial role in stability of the heterodimerand control of the specificity of microtubule assembly in vivo.

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Figure 3. Microtubule assembly capacity of $beta$ 2 $Delta$ C. Cross-sections of intermediate stage elongating spermatids. (A) Spermatid from a wild-type fertile male showing the normal architecture of an intermediate stage axoneme. The canonical nine doublet microtubules plus two central pair microtubules have been assembled, and the nine accessory microtubules (Ac) associated with the B tubule of each doublet are nearly completed. Inner and outer dynein arms are present on the A tubules of each doublet. Radial spokes are present between the doublets and the central pair complex (see Figure 5A for more detail). Arrow indicates cytoplasmic microtubules that at this stage surround the two mitochondrial derivatives (MD), in which typical electron-dense material has just begun to accumulate. (B) Spermatid from a sterile male in which $beta$ 2 $Delta$ C is the only $beta$ -tubulin in the postmitotic germ cells (male with one copy of p[ $beta$ 2 $Delta$ C] in a $beta$ 2-null background; see Figure 2A). Mitochondria-associated cytoplasmic microtubules are present (arrow), but axonemes are not formed. Clusters of axonemal microtubules (arrowheads) are dispersed in the cytoplasm. These clusters include doublets with multiple nascent accessory tubules (Ac¹). ( $beta$ 2 $Delta$ C does not support completion of closed accessory microtubules [Raff et al., 2000

].) There is no higher-order axonemal organization, and there are no dynein arms, radial spokes, or other nontubulin axoneme components normally associated with doublet microtubules. Microtubules with nascent accessory tubules can also be seen associated with the mitochondrial derivatives (Ac²). Such misplaced doublet-like microtubules are never seen in wild-type spermatids. Scale bar, 100 nm for A and B.

Figure 2B shows that $beta$ 2 $Delta$ C was not stable if full-length $beta$ 2 was also present at wild-type levels and $alpha$ -tubulin was thereforelimiting (Table 1, line 4). These males have two gene doses of $alpha$ -tubulin and three total gene doses of $beta$ -tubulin. $beta$ 2 $Delta$ C synthesiswas the same with or without synthesis of endogenous $beta$ 2 (in Figure2, compare B and A), but when $alpha$ -tubulin is limiting, endogenousfull-length $beta$ 2 and $beta$ 2 $Delta$ C must compete to form $alpha$ - $beta$ heterodimers. $beta$ 2 $Delta$ C is outcompeted, fails to dimerize, and is degraded. The extentto which $beta$ 2 $Delta$ C tubulin is excluded from the dimer pool when $alpha$ -tubulinis limiting is illustrated by comparing B and C in Figure 2. Figure2B shows testis tubulins in males with two copies of both $alpha$ 84Band full-length $beta$ 2, plus a single copy of $beta$ 2 $Delta$ C. Only a trace amountof stable $beta$ 2 $Delta$ C was accumulated (i.e., dimerized with $alpha$ -tubulin).Figure 2C shows testis tubulins in males with two copies of both $alpha$ 84B and $beta$ 2, but with four copies of $beta$ 2 $Delta$ C (Table 1, line 6).The amount of stable $beta$ 2 $Delta$ C is increased but is still much lessthan the amount of stable $beta$ 2. Thus, intact $beta$ 2 can outcompete $beta$ 2 $Delta$ Cfor dimerization even when synthesis of $beta$ 2 $Delta$ C exceeds $beta$ 2.

The instability of $beta$ 2 $Delta$ C can be "rescued" by reducing the endogenous $beta$ 2 gene dosage so that $alpha$ -tubulin is no longer limiting.Figure 2D shows synthesis and accumulation of testis tubulinsin males that are wild-type for $alpha$ 84B and have one copy each of $beta$ 2 $Delta$ C and the endogenous $beta$ 2 gene. There are two gene doses of $alpha$ -tubulinand two total gene doses of $beta$ -tubulin (Table 1, line 8). Figure2D, right, shows that the amount of accumulated $beta$ 2 $Delta$ C is only slightlyless than the amount of $beta$ 2. Thus, if $alpha$ -tubulin is not limiting, $beta$ 2 $Delta$ C can form stable dimers even in the presence of $beta$ 2.

A second means of stabilizing $beta$ 2 $Delta$ C is to increase the level of $alpha$ 84B-tubulin. Figure 2E shows synthesis and accumulation of $beta$ 2 $Delta$ C in males that are wild-type at the $alpha$ 84B and $beta$ 2 loci and alsocarry one copy of $beta$ 2 $Delta$ C, plus an additional transgenic copy ofthe $alpha$ 84B gene (Matthews et al., 1993; Hutchens et al., 1997).This results in three total gene doses of $alpha$ -tubulin and threetotal gene doses of $beta$ -tubulin (Table 1, line 9). Once again,as in Figure 2D, $alpha$ 84B is not limiting, and $beta$ 2 $Delta$ C forms stable dimers.In a separate experiment, we used a different $alpha$ -tubulin isoformto increase the total $alpha$ -tubulin pool (Table 1, lines 11 and 12). $alpha$ 85E-tubulin is a developmentally regulated isoform that is notexpressed in the wild-type male germ line (Matthews et al., 1990).We have previously shown that the transgenic construct p[ $alpha$ 85E]expresses $alpha$ 85E in the postmitotic male germ line at a level equivalentto the endogenous $alpha$ 84B (Hutchens et al., 1997). Increasing thelevel of $alpha$ -tubulin in the testes by expressing one copy of p[ $alpha$ 85E]in males together with one copy of p[ $beta$ 2 $Delta$ C] and two copies eachof $alpha$ 84B and $beta$ 2 also resulted in accumulation of stable $beta$ 2 $Delta$ C, similarto when three doses of $alpha$ 84B were present. $alpha$ 85E is not a normalpartner for $beta$ 2 in wild-type males; nevertheless, $alpha$ 85E can rescuethe instability of $beta$ 2 $Delta$ C about as well as can $alpha$ 84B.

A reciprocal experiment showed that reducing the level of endogenous $alpha$ -tubulin destabilizes $beta$ 2 $Delta$ C. Figure 2F shows synthesisand accumulation of testis tubulins in males with one copy ofthe endogenous $beta$ 2 gene, one copy of $beta$ 2 $Delta$ C, and only one copy of $alpha$ 84B-tubulin. In this genotype, $alpha$ -tubulin is once again limiting, $beta$ 2 outcompetes $beta$ 2 $Delta$ C to form $alpha$ - $beta$ dimers, and $beta$ 2 $Delta$ C is degraded (Table1, line14).

Different $beta$ -Tubulin Isoforms Exhibit Differing Potential for Dimerization

The ability of full-length $beta$ 2-tubulin to outcompete $beta$ 2 $Delta$ C for dimerization with $alpha$ 84B revealed that the $beta$ 2 carboxyl terminusis important in forming stable $alpha$ - $beta$ dimers. We next wished to askwhether these results reflect a general role of the $beta$ -tubulincarboxyl terminus in dimerization. We therefore tested the abilityof two other Drosophila $beta$ -tubulin isoforms, $beta$ 1- and $beta$ 3-tubulin,to compete with $beta$ 2 $Delta$ C for dimerization in the male germ line. Neither $beta$ 1 nor $beta$ 3 is normally expressed in the postmitotic male germ line;however, both are partners with $alpha$ 84B elsewhere (Kimble et al.,1989; Matthews et al., 1989; Dettman et al., 1996, 2001). We madeuse of the transgenic constructs p[ $beta$ 1] and p[ $beta$ 3] to express $beta$ 1or $beta$ 3 in the postmitotic male germ cells at a level equivalentto that of endogenous $beta$ 2 (see MATERIALS AND METHODS; Hoyle etal., 1995; Raff et al., 2000).

Figure 2, G and H, show that $beta$ 1 and $beta$ 3 outcompete $beta$ 2 $Delta$ C for dimerization with $alpha$ 84B. In the testes of the males in these experiments,two copies of full-length $beta$ -tubulin and one copy of $beta$ 2 $Delta$ C wereexpressed in the presence of two copies of $alpha$ 84B. Total full-length $beta$ -tubulin thus consists of one gene dose of $beta$ 2 plus one gene doseof either $beta$ 1 or $beta$ 3. In Figure 2, B, G, and H, the relative affinityof each full-length $beta$ -tubulin for dimerization with $alpha$ 84B is judgedby the degree to which $beta$ 2 $Delta$ C is excluded from the dimer pool andsubsequently degraded. Figure 2B shows that $beta$ 2 $Delta$ C is almost completelydegraded in the presence of two copies each of $alpha$ 84B and $beta$ 2. InFigure 2, comparison of B with G or H shows that, when one genedose of $beta$ 2 is replaced by one gene dose of either $beta$ 1 (Table 1,line 17) or $beta$ 3 (Table 1, line 19), $beta$ 2 $Delta$ C is still degraded butto a lesser extent than when $beta$ 2 is the sole competitor. Thus,in the context of the male germ line, any $beta$ -tubulin may act toprovide $alpha$ - $beta$ dimer stability, but the endogenous $beta$ 2 works best.The amount of stable $beta$ 2 $Delta$ C is about the same in Figure 2, G andH, indicating that $beta$ 1 and $beta$ 3 are approximately equal in theirability to compete with $beta$ 2 $Delta$ C for dimerization with $alpha$ 84B.

Sorting between Tubulins Occurs Only during Dimerization, Not during Microtubule Assembly

Instability of $beta$ 2 $Delta$ C appears to result from competition with $beta$ 2 during passage through the tubulin-specific chaperone supercomplexor "dimer-making machine." An alternative explanation is thatsome or all of the instability of $beta$ 2 $Delta$ C results from preferentialuse of $alpha$ 84B- $beta$ 2 over $alpha$ 84B- $beta$ 2 $Delta$ C heterodimers in the assembly ofaxonemes and concomitant degradation of the unused $alpha$ 84B- $beta$ 2 $Delta$ C dimers.To distinguish between these two models, we compared the relativeamounts of $beta$ 2 $Delta$ C in testes and in the seminal vesicles from malesof the same fertile $beta$ 2 $Delta$ C-expressing genotype. The testes containonly immature spermatids; mature sperm exit the testes and arestored in the seminal vesicle. In the testes there exists a solubletubulin heterodimer pool used to assemble several transient microtubulearrays including the meiotic spindle and two classes of cytoplasmicmicrotubules, as well as the axoneme microtubules. The solubletubulin, together with the rest of the cytoplasm, is lost duringspermatid individualization just before the mature sperm enterthe seminal vesicle. In the seminal vesicle, 100% of both $alpha$ - and $beta$ -tubulin is present in the form of stable axoneme microtubules.If $alpha$ 84B- $beta$ 2 dimers are preferentially incorporated into microtubulesand $alpha$ 84B- $beta$ 2 $Delta$ C dimers are excluded and eventually degraded, thenthere should be no $beta$ 2 $Delta$ C found in sperm. This is not the case.Figure 2B shows the relative amounts of stable $alpha$ 84B, $beta$ 2, and $beta$ 2 $Delta$ Cin total tubulins from testes of fertile males with one copy of $beta$ 2 $Delta$ C in an otherwise wild-type background. Figure 4A shows thetubulins found in mature sperm isolated from the seminal vesiclesof wild-type males. Figure 4B shows the amount of $beta$ 2 $Delta$ C in maturesperm isolated from seminal vesicles of males of the same genotypeas in Figure 2B. Comparison of Figure 2B with Figure 4B showsthat the amount of $beta$ 2 $Delta$ C relative to $beta$ 2 is about the same in totaltestis tubulins and in tubulins assembled into axonemes of maturemotile sperm.

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Figure 4. $alpha$ 84B- $beta$ 2 $Delta$ C dimers are incorporated into axonemes at the same ratio at which they are present in the total testis tubulin pool. Mature motile sperm were isolated from the seminal vesicles of 14 1-week-old virgin males; sperm proteins were separated by two-dimensional gel electrophoresis, blotted, and immunostained as described in MATERIALS AND METHODS. (A) Tubulins from wild-type sperm. Both $alpha$ 84B and $beta$ 2 undergo posttranslational modification (Piperno and Fuller, 1985

; Eddé et al., 1990

; Hutchens et al., 1997

). (B) Tubulins in sperm from fertile males carrying one copy of p[ $beta$ 2 $Delta$ C] but otherwise wild-type at the $alpha$ 84B and $beta$ 2 loci. Total testis tubulins from males of this genotype are shown in Figure 2B. Comparison of the $beta$ 2 $Delta$ C signals with that in Figure 2B shows the same relative amount of stable $beta$ 2 $Delta$ C-tubulin.

We therefore conclude that once made $alpha$ 84B- $beta$ 2 $Delta$ C dimers are not preferentially excluded from microtubules and that incorporationof $alpha$ 84B- $beta$ 2 $Delta$ C into axonemes directly reflects the proportion of $alpha$ 84B- $beta$ 2 $Delta$ C dimer in the soluble $alpha$ - $beta$ dimer pool. This result indicatesthat competition between $beta$ 2 $Delta$ C and full-length $beta$ -tubulin occursonly in the dimer-making machine; the axoneme-making machineryis less picky. This is in agreement with studies showing thatectopic $beta$ 1 and $beta$ 3 are incorporated into axonemes at the same genedose at which they are expressed (Hoyle and Raff, 1990; Hoyleet al., 1995; Raff et al., 2000). Moreover, ectopic $beta$ 1 is uniformlydistributed along the length of the axoneme; there is no preferentialincorporation of endogenous $beta$ 2 (Nielsen et al., 2001). In thecase of ectopic $beta$ 3 expression, $alpha$ 84B- $beta$ 3 dimers by themselves failto support axoneme assembly and co-incorporation with endogenous $beta$ 2 results in dominant male sterility (Hoyle and Raff, 1990),just as is the case with $beta$ 2 $Delta$ C.

$beta$ 2 $Delta$ C Disrupts the Periodicity of Organization of Nontubulin Components of the Axoneme

As discussed above, when it is the only $beta$ -tubulin in the postmitotic germ cells, $beta$ 2 $Delta$ C can support assembly and partial functionof meiotic spindles and some classes of cytoplasmic microtubules(Fackenthal et al., 1993). However, $beta$ 2 $Delta$ C alone cannot supportthe testis-specific functions that are unique to the $beta$ 2 isoform(Fackenthal et al., 1993). $beta$ 2 $Delta$ C can support assembly of doubletmicrotubules, but it cannot support axoneme morphogenesis (Figure3), nor can it support microtubule-mediated shaping of the spermnuclei.

Analysis of genotypes in which $beta$ 2 $Delta$ C is coexpressed with intact $beta$ 2 allowed us to discern some of the specific roles of the $beta$ 2-specific C terminus in axonemes. When $beta$ 2 $Delta$ C is co-incorporatedwith $beta$ 2, meiotic spindles and cytoplasmic microtubules are fullyfunctional, and intact full-length axonemes are assembled. A smallamount of $beta$ 2 $Delta$ C is compatible with axoneme motility. Figure 2Cshows that, in testes of males with four gene doses of $beta$ 2 $Delta$ C inan otherwise wild-type background, some $beta$ 2 $Delta$ C accumulates in thetotal stable $beta$ -tubulin pool. These males are fertile but of reducedfecundity relative to wild-type (Table 1, line 6). However, when $alpha$ -tubulin is not limiting and $beta$ 2 $Delta$ C-containing dimers constitutea third or more of the total stable $beta$ -tubulin pool, males areinvariably sterile (e.g., Table 1, lines 8, 9, and 12). Thissterility provides another indicator that there is no sortingof dimers during microtubule assembly and that $beta$ 2 $Delta$ C is being builtintoaxonemes.

In sterile males in which $beta$ 2 $Delta$ C makes up 30% of the stable $beta$ -tubulin pool, axonemes are assembled and mature individualizedsperm are formed, but the axonemes are not motile and sperm donot enter the seminal vesicles. This seems paradoxical: $beta$ 2 $Delta$ C ismissing the carboxyl terminus, and yet $beta$ 2 $Delta$ C-mediated sterilityis a dominant phenotype. At the light microscope level, the spermlook normal (albeit motionless) and reach the wild-type lengthof ~1.8 mm. Viewed in cross-section by electron microscopy, the $beta$ 2 $Delta$ C-containing axonemes are indistinguishable from wild-typeaxonemes at all stages. Figure 5 compares the ultrastructure ofwild-type axonemes with nonmotile axonemes from sterile malescarrying three copies of $alpha$ 84B, one copy of $beta$ 2 $Delta$ C, and two copiesof $beta$ 2 (the genotype shown in Figure 2E; Table 1, line 9). Figure5A shows a cross-section of a mature wild-type 9 + 2 axoneme.The cross-section of a nonmotile $beta$ 2 $Delta$ C-containing axoneme in Figure5B has all of the wild-type axonemal structures, including doubletmicrotubules, inner and outer dynein arms, radial spokes, andthe central pair complex.

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Figure 5. $beta$ 2 $Delta$ C causes dominant defects in the axial organization of the axoneme. Axonemes in nearly mature spermatids before individualization. Cross-sections (A and B) and longitudinal sections (C-F) of axonemes from wild-type males (A, C, and E) and sterile males with three copies of $alpha$ 84B, one copy of $beta$ 2 $Delta$ C, and two copies of $beta$ 2 (B, D, and F; this is the same genotype as in Figure 2E and Table 1, line 9). (A) Wild-type axoneme showing the major components including the A and B tubules of the doublets, the accessory microtubules (Ac) associated with each B tubule, the central pair complex (CP), and the radial spokes (Sp) and spoke heads (SH). Other components include the inner and outer dynein arms associated with each A tubule, the membrane surrounding the axoneme (m), and the luminal filaments within the accessory and central pair tubules (which appear in cross-section as a "dot" or filling in the microtubule lumen). (B) $beta$ 2 $Delta$ C-containing axoneme. In cross-section, axonemes from males of this genotype appear wild type. (C and E) Longitudinal sections through wild-type axonemes at the plane of the central pair complex. The regular spacing of the radial spokes (arrowheads) can be seen along the entire length of each section. Within the central pair complex there is a "beads-on-a-string" element with a periodicity of ~15 nm. (D) Longitudinal section through a $beta$ 2 $Delta$ C-containing axoneme showing mild disorganization. Some radial spokes have a wild-type spacing (arrowheads) and some are irregularly spaced and misshapen (bracket). In addition, the beads-on-a-string element is not present along most of the top edge of the central pair complex, and there is a gap in the middle along the bottom edge (compare with A). (F) Longitudinal section through a region of a second $beta$ 2 $Delta$ C-containing axoneme that is more disorganized than the axoneme in D. Very few wild-type radial spokes are present; most spokes are misshapen and irregularly spaced. There are gaps where spokes are either above or below the plane of section or are missing entirely. The beads-on-a-string element of the central pair complex is largely disrupted. Scale bar, 50 nm, for all panels.

However, the sterility can be explained by defects seen in longitudinal sections of axonemes. Figure 5, C and E, shows longitudinalsections of wild-type axonemes with the regular array of radialspokes and an element repeated at 15-nm intervals within the centralpair complex. Both of these regular axial arrays are disruptedin the $beta$ 2 $Delta$ C-containing axonemes shown in Figure 5, D and F. Radialspokes are present, but their spacing is uneven and some spokesappear to be out of the plane of section. The spoke heads appearirregular in shape and many do not appear to contact the centralpair complex. The 15-nm repeat element is lost in patches alongthe $beta$ 2 $Delta$ C-containing central pair complexes. All axonemal microtubulesare present and appear fully wild-type in cross-section. Thus,it appears that nontubulin components of the axoneme have failedto form all of the correct associations with microtubules containing $beta$ 2 $Delta$ C.

When $beta$ 2 $Delta$ C is increased from 30 to 50% of the stable $beta$ -tubulin pool, defects become readily apparent in axonemes examined incross-section. These defects include severe examples of the typesof radial spoke defects and central pair complex defects thatcan be detected only in longitudinal section when $beta$ 2 $Delta$ C is just30% of the stable $beta$ -tubulin pool. Figure 6 shows the ultrastructureof nonmotile axonemes from sterile males carrying two copies of $alpha$ 84B, one copy of $beta$ 2 $Delta$ C, and one copy of $beta$ 2 (the genotype shownin Figure 2D; Table 1, line 8). The axoneme shown in Figure 6Ais missing two radial spoke heads. In addition, three intact spokesare not in contact with the central pair complex. The axonemein Figure 6B is missing a spoke head as well as the entire centralpair complex, including the central pair microtubules. Althoughmany axonemes are defective, there is no clear ordering or patternamong the defects. We observed normal central pair complexes associatedwith defective spokes, normal spokes in axonemes with defectivecentral pair complexes, and normal spokes and central pair complexesassociated with defective outer doublet complexes.

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Figure 6. Axoneme defects increase with increased levels of stable $beta$ 2 $Delta$ C. Cross-sections of axonemes containing equal amounts of $beta$ 2 $Delta$ C and $beta$ 2-tubulin show defects in the central pair complex and radial spokes. Axonemes in A and B are from sterile males with two copies of $alpha$ 84B, one copy of $beta$ 2 $Delta$ C, and one copy of $beta$ 2 (this is the same genotype as in Figure 2D and Table 1, line 8). (A) An axoneme missing two spoke heads (SH) normally found adjacent to the central pair complex. In addition, three intact spokes are detached from the central pair complex (arrows). (B) An axoneme missing the central pair complex (CP) as well as a single spoke head (arrow). One accessory microtubule lacks the electron-dense material that would normally connect it to the adjacent doublet (arrowhead). Scale bar, 50 nm, for both panels.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

To determine the functional roles of the $beta$ -tubulin carboxyl terminus, we expressed a carboxyl-truncated $beta$ -tubulin in the Drosophilamale germ line under conditions where synthesis of $alpha$ - and $beta$ -tubulinsare not equimolar. Our data show that the $beta$ -tubulin C terminusis important in generating stable $alpha$ - $beta$ dimers in vivo. A varietyof full-length $alpha$ - and $beta$ -tubulins are stable when expressed ectopicallyin the wild-type male germ line at nonequimolar ratios of $alpha$ - and $beta$ -tubulin (Hoyle and Raff, 1990; Hoyle et al., 1995; Hutchenset al., 1997; Raff et al., 1997, 2000). We have found that thecarboxyl terminus-truncated $beta$ -tubulin, $beta$ 2 $Delta$ C, forms stable dimersonly when $alpha$ -tubulin is not limiting, i.e., when the total genedose of intact $beta$ -tubulin plus $beta$ 2 $Delta$ C is less than or equal to thetotal $alpha$ -tubulin gene dose. If the total $beta$ -tubulin gene dose exceedsthe total $alpha$ -tubulin gene dose, intact $beta$ -tubulins are preferentiallydimerized. In such conditions, $beta$ 2 $Delta$ C fails to dimerize and is degraded.This contrasts with results of in vitro experiments using rabbitreticulocyte extracts to express a murine $beta$ -tubulin missing thelast 12 carboxyl residues (Fontalba et al., 1995). In the in vitrosystem, the newly synthesized truncated $beta$ -tubulin was not ableto form $alpha$ - $beta$ heterodimers and was released from the chaperone complex,undegraded, as amonomer.

In this study, we have found that different $beta$ -tubulin isoforms possess different affinities for dimerization with $alpha$ -tubulin.Our data demonstrate that the carboxyl terminus is key in establishingstable heterodimers. However, just as sequence differences betweendifferent $beta$ -tubulin isoforms in regions other than the C terminusare important in determining isoform-specific function in microtubuleassembly, internal sequence differences may also contribute todifferential dimerizationproperties.

Our data support the interpretation that differences in dimerization properties are important in determining isoform-specificmicrotubule functions. Thus, we found that $beta$ 2 was better at competingwith $beta$ 2 $Delta$ C than either of the other two full-length $beta$ -tubulin isoformswe tested. The finding that endogenous $beta$ 2 has greater affinitythan $beta$ 1 for $alpha$ 84B suggests a developmental role for $beta$ -tubulin sortingduring dimerization. $beta$ 1 is expressed in primary spermatocytesand is rapidly replaced by $beta$ 2 before meiosis (Kemphues et al.,1982). Tian et al. (1999) have shown that heterodimeric tubulinscan exchange in vitro by recycling through the dimer-making machine.At the onset of $beta$ 2 synthesis the $beta$ 1 gene is no longer expressed;however, each spermatocyte still contains $beta$ 1 protein. One of severalpossible mechanisms by which $beta$ 2 could replace this residual $beta$ 1would be for $beta$ 2 to outcompete $beta$ 1 for dimerization duringrecycling.

The equal affinities of $beta$ 1 and $beta$ 3 for $alpha$ 84B are also consistent with the developmental coexpression of these two isoforms inseveral cell types during development (Kimble et al., 1989, 1990;Dettman et al., 1996, 2001; Hoyle et al., 2000). We have previouslyshown that $beta$ 1 and $beta$ 3 are coassembled into the same microtubulesin vivo (Hoyle et al., 2000). This would not be possible if either $beta$ 1 or $beta$ 3 could strongly outcompete the other for dimerizationwith $alpha$ -tubulin.

The $beta$ 2-specific carboxyl terminus is essential for assembly of the sperm tail flagella, the only motile axoneme in Drosophila.The 15 carboxyl residues missing from $beta$ 2 $Delta$ C include the axonememotif present in all $beta$ -tubulins incorporated into motile axonemes(Raff et al., 1997), as well as sites of posttranslational modificationknown to be important for axoneme motility (Xia et al., 2000).The axoneme motif specifies the central pair microtubules (Nielsenet al., 2001). Here, we have found that even when full-length $beta$ 2 makes up the majority of the $beta$ -tubulin present, incorporationof stable $beta$ 2 $Delta$ C into axoneme microtubules disrupts the organizationof the central pair complex and the radial spokes. Studies ofparalyzed flagella mutants of Chlamydomonas have shown these twoaxonemal structures to be involved in regulating axoneme motility(reviewed by Smith and Lefebvre, 1997; Porter and Sale, 2000).A nontubulin component found in the central pair complex of awide range of species is the central pair projection (Witman etal., 1978). Transient contact between the radial spokes and thecentral pair projections is thought to play an important rolein the regulation of dynein and the generation of the complexflagellar waveform (Smith and Lefebvre, 1997).

The identity of the repeated element found in the Drosophila central pair complex is not known. However, its disruption by $beta$ 2 $Delta$ C, as well as the disruption of the radial spokes, impliesthat both components are in contact with the carboxyl terminusof $beta$ -tubulin in wild-type axonemes, either directly or indirectlythrough other protein-protein interactions. In our experiments,all nontubulin components present are wild type. When the radialspokes or central pair components are themselves mutant, as isthe case with Chlamydomonas paralyzed flagellar mutants, the mutationsare recessive. In contrast, when $beta$ 2 subunits lacking the carboxylterminus are incorporated at random into axonemes, the consequenceis a dominant disruption of axoneme motility. It appears thatfor each $alpha$ 84B- $beta$ 2 $Delta$ C dimer incorporated into an axoneme microtubule,there is a stoichiometric loss of interaction with nontubulincomponents of the axoneme. When 30% of the $beta$ -tubulin lacks thecarboxyl terminus, the loss of organization becomes too greatto permit axoneme function, and sperm become nonmotile. The higherthe percentage of truncated $beta$ -tubulin incorporated into the axoneme,the more severe are the defects. Axonemes from males in which $beta$ 2 $Delta$ C is 50% of total $beta$ -tubulin exhibit the same kind of defectsthat occurred in sterile males with 30% $beta$ 2 $Delta$ C but to a much moremarked degree, readily apparent in axoneme cross-sections.

We have discovered that the $beta$ 2-tubulin carboxyl terminus plays two distinct roles. In its first role, the acidic carboxylterminus is important for producing a stable $alpha$ - $beta$ heterodimer.The generalized nature of this requirement is reflected by thefact that any acidic carboxyl terminus seems to work; $beta$ 1- and $beta$ 3-tubulin both form stable $alpha$ - $beta$ dimers in the male germ line.Thus, although the $beta$ -tubulin carboxyl terminus is the hypervariable,isotype-defining region of the molecule (Sullivan and Cleveland,1986), the wrong carboxyl terminus seems to be better than nocarboxyl terminus. In a distinct second role, the carboxyl terminusis involved in interactions between intact microtubules and nontubulincomponents required to generate the architecture of specific microtubule-basedstructures. $beta$ 2 $Delta$ C by itself fails to support any axonemal organization(Fackenthal et al., 1993; Nielsen et al., 2001). However, notjust any carboxyl terminus can support this function: other full-lengthDrosophila $beta$ -tubulin isoforms cannot replace $beta$ 2 for axoneme function(Hoyle and Raff, 1990; Hoyle et al., 1995; Raff et al., 2000).In contrast, the carboxyl terminus is not required for genericmicrotubule functions: $beta$ 2 $Delta$ C can support assembly of functionalmeiotic spindles as well as the cytoplasmic microtubules associatedwith elongation of the mitochondrial derivative (Fackenthal etal., 1993; Figure 3B). It should be noted that these generic functionscan also be fully or partially supplied by other Drosophila isoforms(Hoyle and Raff, 1990; Hoyle et al., 1995; Raff et al., 2000).

Our data demonstrate that competition between $beta$ 2 $Delta$ C and intact $beta$ -tubulins takes place during dimerization and not during subsequentmicrotubule assembly. However, competition between full-length $beta$ -tubulin and $beta$ 2 $Delta$ C could occur at several steps in the dimerizationprocess. Our work does not distinguish between competition forbinding with cytosolic chaperonin, competition for cofactors ofthe dimer-making machine, or direct competition between $beta$ 2 and $beta$ 2 $Delta$ C for $alpha$ 84B. However, the resolved three-dimensional structureof the $alpha$ - $beta$ dimer allows for the possibility that the unresolved $beta$ -tubulin carboxyl residues are in contact with the $alpha$ -tubulinmoiety of the same $alpha$ - $beta$ dimer (Nogales et al., 1998). Direct competitionbetween $beta$ -tubulins for binding to $alpha$ is consistent with our findingthat different $beta$ -tubulin isoforms exhibit differential abilityto form $alpha$ - $beta$ dimers. This model suggests the possibility that $alpha$ -tubulinresidues contacted by the $beta$ -tubulin carboxyl terminus play a directrole in stabilizing the $alpha$ - $beta$ dimer. The resolved structure predictsthese $alpha$ -tubulin residues to be non-carboxyl-terminal residues.As is the case with $beta$ -tubulin, the $alpha$ -tubulin carboxyl terminusis also unresolved in both the structures of the heterodimer andthe microtubule (Nogales et al., 1998, 1999). The 11 unresolved $alpha$ residues are in position to contact $beta$ -tubulin in another heterodimer,either in the same protofilament or perhaps in an adjacent protofilament(Nogales et al., 1998). This leads to the prediction that the $alpha$ -tubulin carboxyl terminus will be of relatively little importancein forming or stabilizing intrasubunit associations in the dimerbut may be involved in interdimer associations in the protofilamentsubstructure ofmicrotubules.

	ACKNOWLEDGMENTS

We thank Mark Nielsen for many lively and helpful discussions of our data and Mark and Bill Saxton for critical reading ofthe manuscript. This work was supported by a research grant toE.C.R. from the U.S. Public HealthService.

	FOOTNOTES

^* Corresponding author. E-mail address: hhoyle{at}bio.indiana.edu.

Present address: Biology Department, Wesleyan University, Middletown, CT06459.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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