LC2, the Chlamydomonas Homologue of the t Complex-encoded Protein Tctex2, Is Essential for Outer Dynein Arm Assembly

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Vol. 10, Issue 10, 3507-3520, October 1999

LC2, the Chlamydomonas Homologue of the t Complex-encoded Protein Tctex2, Is Essential for Outer Dynein Arm Assembly

Gregory J. Pazour,^* Anthony Koutoulis,^* Sharon E. Benashski, Bethany L. Dickert,^* Hong Sheng,^* Ramila S. Patel-King, Stephen M. King, and George B. Witman^*^§

^*Department of Cell Biology, University of Massachusetts Medical School, Worcester, Massachusetts 01655; Cell Biology Group, School of Plant Science, The University of Tasmania, Hobart, Tasmania 7001 Australia; and Department of Biochemistry, University of Connecticut Health Center, Farmington, Connecticut 06030-3305

Submitted June 7, 1999; Accepted July 30, 1999
Monitoring Editor: Tim Stearns

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Tctex2 is thought to be one of the distorter genes of the mouse t haplotype. This complex greatly biases the segregation ofthe chromosome that carries it such that in heterozygous +/t males,the t haplotype is transmitted to >95% of the offspring, a phenomenonknown as transmission ratio distortion. The LC2 outer dynein armlight chain of Chlamydomonas reinhardtii is a homologue of themouse protein Tctex2. We have identified Chlamydomonas insertionalmutants with deletions in the gene encoding LC2 and demonstratethat the LC2 gene is the same as the ODA12 gene, the product ofwhich had not been identified previously. Complete deletion ofthe LC2/ODA12 gene causes loss of all outer arms and a slow jerkyswimming phenotype. Transformation of the deletion mutant withthe cloned LC2/ODA12 gene restores the outer arms and rescuesthe motility phenotype. Therefore, LC2 is required for outer armassembly. The fact that LC2 is an essential subunit of flagellarouter dynein arms allows us to propose a detailed mechanism wherebytransmission ratio distortion is explained by the differentialbinding of mutant (t haplotype encoded) and wild-type dyneinsto the axonemal microtubules of t-bearing or wild-type sperm,with resulting differences in theirmotility.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Dynein ATPases are microtubule-based molecular motors that provide force for a variety of important cellular processes (reviewedby Holzbaur and Vallee, 1994; Witman et al., 1994). Cytoplasmicdyneins are involved in vesicle transport, Golgi localization,nuclear migration, spindle formation and orientation, mitosis,and flagellar assembly. Inner arm and outer arm axonemal dyneinsprovide the force for flagellar and ciliarybeating.

All characterized dyneins contain one or more heavy chains (HCs) that are associated with smaller polypeptides termed intermediatechains (ICs), light intermediate chains, and light chains (LCs).For example, Chlamydomonas outer arm dynein, which is the mostwell characterized axonemal dynein, contains three HCs, two ICs,and eight LCs (Table 1). Each HC has a globular head domain containingthe site for ATP hydrolysis and a fibrous stem domain that extendsto the base of the dynein, where the ICs and most of the LCs arelocated in a discrete complex. The heads of the HCs interact withthe B-tubule of the opposing doublet microtubule to generate force,whereas the ICs are involved in anchoring the dynein to the A-tubuleof the doublet microtubule (King et al., 1995; Wilkerson et al.,1995) and regulating dynein activity (Mitchell and Kang, 1993).In contrast, little is known regarding the function(s) of thedynein LCs.

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Table 1. Proteins associated with the outer dynein arm of Chlamydomonas

The need for more information on the dynein LCs has been underscored recently by 1) the discovery that LCs are associatedwith cytoplasmic dynein (King et al., 1996a), indicating thatthey are likely to have a universal role in dynein structure and/orfunction, and 2) the finding that two dynein LCs are encoded withina large region of mouse chromosome 17, which, in t mice, correspondsto the t haplotype (King et al., 1996b; Patel-King et al., 1997).The t haplotype has four inversions relative to the wild-typechromosome; these inversions suppress recombination, so that mutationsarising in the t haplotype are kept together (Silver, 1993). Thisportion of chromosome 17 has been the subject of intense studybecause the t haplotype is inherited in a non-Mendelian manner.Heterozygous +/t males transmit the t-bearing chromosome to >95%of their offspring, a phenomenon known as transmission ratio distortionor meiotic drive. This is due to the concerted action of threeor four t-encoded distorter genes acting on a t-encoded respondergene (Lyon, 1984). In the presence of the t responder, the t distortersact in an additive manner to increase the percent of offspringthat carry the t-bearing chromosome (for review, see Silver, 1985,1993). Apparently the t-encoded versions of the distorter andresponder genes contain mutations that give the t haplotype aselective advantage over the wild-type homologue. The identityand function of the responder gene product is unknown (Ewulonuet al., 1996), but two of the putative distorter gene products(Tctex1 and Tctex2) are dynein LCs. Tctex1 (Lader et al., 1989)is a homologue of a Chlamydomonas inner arm dynein LC (Harrisonet al., 1998) and also is a subunit of brain cytoplasmic dynein(King et al., 1996b). Tctex2 (Huw et al., 1995) is a homologueof a Chlamydomonas outer arm dynein LC termed LC2 (Patel-Kinget al., 1997). A third distorter gene product also may be a dyneinsubunit, because the Dnahc8 dynein HC (Vaughan et al., 1996) mapsat the site of the distorter gene Tcd2 (Harrison et al., 1998).Consequently, it has been hypothesized that the non-Mendeliantransmission of the t haplotype is due to its effect on spermmotility through dynein subunit interactions (Patel-King et al.,1997; Harrison et al., 1998). However, the mechanism by whichthis might work remainselusive.

Much information is now available on the structure of the Chlamydomonas outer dynein arm polypeptides, including the LCs.cDNAs encoding all 13 polypeptides in the outer arm have beenisolated and sequenced; similarly, sequences have been obtainedfor the cDNAs that encode three subunits of the outer dynein armdocking complex (ODA-DC), a heterotrimeric structure closely associatedwith the outer arm and necessary for outer arm assembly (Takadaand Kamiya, 1994; Takada et al., 1996; Koutoulis et al., 1997;Casey et al., 1998) (Table 1). In some cases, the sequences suggestpossible functions for their respective gene products. However,more definitive information on the roles of the outer arm polypeptideshas been obtained from analysis of mutants with defects in specificchains. Sixteen genes (ODA1-ODA14, PF13, and PF22) have been identifiedthat affect outer arm assembly. Mutations in the ODA genes causedefects in the outer dynein arms and slow jerky swimming (Kamiya,1988), whereas defects in the PF genes cause outer arm defectsand paralyzed flagella such that the cells are not motile (Huanget al., 1979). Five of these genes encode the three dynein HCsand two ICs of the outer arm; three others encode subunits ofthe ODA-DC (Table 1). An additional gene, FLA14, encodes LC8,an M_r 8000 LC that is a subunit of outer arm dynein and also ofcytoplasmic dynein, inner arm dynein I1, and myosin V (King andPatel-King, 1995b; King et al., 1996a; Espindola et al., 1996;Harrison et al., 1998; Pazour et al., 1998). Mutations in mostof the identified genes result in loss of the outer arm; deletionof FLA14 results in loss of intraflagellar transport (Rosenbaumet al., 1999) and defects in the assembly of inner and outer armsand radial spokes. Unfortunately, no mutations have been identifiedin the genes that encode LCs specific for the outer arm dynein,so there is no genetic data on the roles of LC1-LC7 in outer armassembly orfunction.

In an effort to learn more about the outer arm dynein LCs, we are taking a reverse genetics approach wherein we screen insertionalmutants for defects in these chains. Insertional mutagenesis inChlamydomonas is based on the fact that when Chlamydomonas istransformed, the exogenous DNA inserts at random into the nucleargenome and either disrupts a gene at the point of insertion or,more commonly, causes the deletion of a large block of DNA flankingthe insertion site (Tam and Lefebvre, 1993). In either case, theresult is a restriction fragment length polymorphism (RFLP) thatcan be detected in Southern blots using a DNA probe for the affectedgene. Inasmuch as cDNAs are available for all of the outer dyneinarm LCs, it should be possible to use these cDNAs to identifymutants with defects in the LC genes. Indeed, we recently usedthis approach to identify the mutants in which LC8 was deleted(Pazour et al., 1998).

In this work, we report two insertional mutants with defects in the gene encoding LC2, an outer arm dynein LC that is thehomologue of the mouse Tctex2 protein. This gene previously wasnamed ODA12 (Koutoulis et al., 1997), but its product was notidentified. Complete deletion of the LC2 gene results in completeloss of the outer dynein arm and impaired motility; transformationof the deletion mutant with the cloned LC2 gene restores the outerarm and rescues the motility phenotype. Therefore, LC2 has anessential role in outer arm assembly. This is the first mutationto be identified in an outer arm-specific LC, and the first evidencethat loss of a single dynein LC can have a deleterious effecton flagellar function. The results suggest a specific model inwhich mutant (t haplotype-encoded) and wild-type dyneins differentiallybind to axonemes of t-bearing or wild-type sperm, with resultingdifferences in their motility that ultimately lead to non-Mendeliantransmission of the tlocus.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Strains

Chlamydomonas reinhardtii strains used in this work include g1 (nit1, agg1, mt+) (Pazour et al., 1995), 1330.1 (ac14, nit1,NIT2, mt $-$ ) (Pazour, unpublished data), 137c (nit1, nit2, mt+),H8 $-$ (arg7, mt $-$ ), H11+ (arg7, mt+) (Tam and Lefebvre, 1993), CC2290(mt $-$ ) (Gross et al., 1988), CC2236 (oda5, mt+) (Kamiya, 1988),CC2240 (oda7, mt+) (Kamiya, 1988), CC2242 (oda8, mt+) (Kamiya,1988), CC2492 (pf13a, mt+) (Huang et al., 1979), and CC1382 (pf22,mt+) (Huang et al., 1979). Strains produced in the course of thisstudy include F56 (oda12-1::NIT1, ac14, nit1, mt $-$ ) and V3 (oda12-2::NIT1,nit1, mt+), generated by insertional mutagenesis of 1330.1 andg1, respectively, 2081.2 (oda12-1::NIT1, mt $-$ ; offspring of F56× 137c cross), 2567.1 (oda12-1::NIT1, arg7; offspring of 2081.2× H11+ cross), and transformants S1, S2, S3, S4, S5, and S20 obtainedby transforming 2567.1 with ODA12 genomic clones and pARG7.8 (Debuchyet al., 1989).

Growth Medium

Chlamydomonas was grown in the following media: M (Sager and Granick [1953] medium I altered to have 0.0022 M KH₂PO₄ and 0.00171M K₂HPO₄), M $-$ N (M medium without nitrogen), R (M medium plus0.0075 M sodium acetate), R + Arg (R medium plus 50 µg/ml arginine),SGII/NO₃ (Sager and Granick [1953] medium II modified to have0.003 M KNO₃ as the nitrogen source), and M $-$ N + KNO₃ (M $-$ Nmedium plus 0.003 M KNO₃).

Transformation

Transformation was performed using the glass bead method of Kindle (1990) as described by Pazour et al. (1995). The originalinsertional mutant library was made by transforming strains g1and 1330.1 with the linearized plasmid pGP505 containing the NIT1gene (Fernandez et al., 1989) as described previously (Pazouret al., 1995; Koutoulis et al., 1997). Strain 2567.1, an arg7derivative of F56, was cotransformed with the pARG7.8 plasmidcontaining the ARG7 gene (Debuchy et al., 1989) and phage or plasmidclones containing the LC2 gene. NIT1 transformants were selectedon SGII/NO₃ medium; ARG7 transformants were selected on Rmedium.

Analysis of Swimming Speeds

Swimming speed was calculated using an ExpertVision Motion Analysis (Santa Rosa, CA) system. Cells were observed with dimred illumination, and their positions were recorded every 67 msby the MotionAnalysis system (Moss et al., 1995). Subsequently,paths were determined, and the speed of individual cells was calculatedusing the speed operator. The final result is the average of >100cells.

Genetic Analysis

Mating and tetrad analyses were performed as described by Levine and Ebersold (1960) and Harris (1989). Cells of each matingtype were grown on solid medium (R or R + Arg) and resuspendedin M $-$ N liquid medium. After pellicles became apparent in 1 or2 d, the mixture was plated on solid M medium; the plates wereallowed to dry and placed in the dark for 6-10 d. Zygotes werehatched on solid R or R + Arg medium and dissected using a glassneedle. The meiotic progeny were allowed to grow for 3-5 d andthen transferred to 5 ml of liquid R or R + Arg medium. Cellswere allowed to grow for 2-5 d and then scored for motility bymicroscopic observation of cells illuminated with dim red light.The arg7 phenotype was scored by comparing cell growth on R versusR + Argmedium.

Electron Microscopy

Cells were fixed in glutaraldehyde (Hoops and Witman, 1983) and processed as described by Wilkerson et al. (1995).

Axoneme Isolation, Electrophoresis, and Immunoblotting

Wild-type and oda12 strains were deflagellated with dibucaine, and the resulting flagella were isolated by standard procedures(Witman, 1986). After demembranation with Nonidet P-40, axonemeswere placed in SDS sample buffer and heated at >95°C for severalminutes. All samples were electrophoresed in 5-15% acrylamidegradient gels (King et al., 1986). Gels were blotted to polyvinylidenedifluoride (PVDF) membrane (Immobilon-P; Millipore, Waters, Milford,MA) by the two-step procedure of Otter et al. (1987). To detectdynein polypeptides, blots were probed with monoclonal antibody1878A (specific for IC1; King et al., 1985), rabbit polyclonalEU51 (specific for IC140; Yang and Sale, 1998), or affinity-purifiedrabbit polyclonal antibody R5391 (specific for LC2; Patel-Kinget al., 1997) as described by Pazour et al. (1998).

Cloning the ODA12 Locus

To obtain genomic clones of the ODA12 locus, Chlamydomonas genomic DNA was partially digested with Sau3AI and size fractionatedby NaCl gradient centrifugation. The fraction containing DNA fragmentsin the 10- to 20-kbp range was ligated into the BamHI site ofLambda DashII (Stratagene, San Diego, CA) and packaged in vitrousing Gigapack II extracts (Stratagene). The library was screenedby hybridization with the LC2 cDNA, and three phage clones ( $lambda$ ODA12#8, $lambda$ ODA12#17, and $lambda$ ODA12#20) were obtained. The EcoRI insert of $lambda$ ODA12#17was subcloned into the EcoRI site of pKS+ (Stratagene) and namedpHS44. pBD14 was constructed by cloning the 3.1-kbp HindIII fragmentof pHS44 into the HindIII site of pKS+. pBD17 was constructedby cloning the 5.7-kbp KpnI-SalI fragment of pHS44 into pKS+ thathad been cut with SalI and KpnI.

Other Procedures

DNA was isolated by digesting ~0.3 ml of packed cells with 0.5 ml of proteinase K (1 mg/ml) in 5% sodium lauryl sulfate, 20mM EDTA, and 20 mM Tris, pH 7.5, at 50°C for 12-16 h. Ammoniumacetate was added to 1.5 M, the mixture was extracted once with50% phenol and 50% chloroform and once with chloroform, and thenthe DNA was precipitated with isopropyl alcohol. DNA was resuspendedin 10 mM Tris and 1.0 mM EDTA, pH 8.0, and digested with PstIor PvuII. Gel electrophoresis and Southern blotting were performedaccording to standard procedures (Sambrook et al., 1987).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Identification of Mutants with Defects in the LC2 Gene

We previously described the isolation of a large number of Chlamydomonas insertional mutants with defects in phototaxis, cellmotility, and flagellar assembly (Pazour et al., 1995, 1998; Koutouliset al., 1997). Because the mutations in these cell lines usuallyresult in RFLPs that can be detected in Southern blots probedwith cDNAs encoding parts of the affected genes, it has openedthe door to a reverse genetics approach wherein it is possibleto identify mutants with specific defects in cloned genes (Wilkersonet al., 1995; Pazour et al., 1998, 1999).

There are eight outer dynein arm LCs. cDNA clones encoding each of these have been isolated via protein sequence, but to dateonly one LC gene, FLA14, encoding LC8 (Pazour et al., 1998), hasbeen disrupted. We were particularly interested in finding a mutationthat affected LC2, the homologue of the mouse Tctex2 protein.In an attempt to identify such a mutant, we screened our entirecollection of Chlamydomonas insertional mutants by Southern blottingusing the LC2 cDNA as a probe. Chlamydomonas contains a singlecopy of the LC2 gene, which is cut once by PvuII (Patel-king etal., 1997). Thus, the LC2 cDNA detects two bands (0.9 and 3.5kbp) on Southern blots of wild-type genomic DNA cut with thisenzyme (Figure 1A).

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Figure 1. Southern blot showing RFLPs in F56 and V3. (A) Genomic DNA was isolated from slow-swimming insertional mutants, cut with PvuII, and analyzed by Southern blotting using the LC2 cDNA as a probe. This probe detects 0.9- and 3.5-kbp bands in most cell lines, including V5 and F55 (both containing a deletion of the ODA9 gene) and F57 (containing a disruption of an unidentified gene). However, both of these bands are missing in the F56 strain, and the lower band is missing in the V3 strain. (B) A probe (5' End) specific for the 5' UTR and entire coding region of the LC2 gene (see text) hybridizes to the upper band in DNA from both V5 and V3. A probe (3' End) specific for the 3' UTR of the LC2 gene hybridizes to the lower band in DNA from V5 but detects no band in DNA from V3, indicating that the deletion in V3 is at the 3' end of the gene.

One strain, F56, was missing both hybridizing bands (Figure 1A), indicating that the gene encoding LC2 is completely deletedin this strain. Previously, strain F56 had been briefly reportedto contain a mutation that caused complete loss of the outer dyneinarm and a slow-swimming phenotype (Koutoulis et al., 1997). Thismutant complemented oda1-oda11, pf13, and pf22 in stable diploids,indicating that it was defective in a new ODA gene, which wastermed ODA12 (Koutoulis et al., 1997; see below). The productof this gene was not identified, because no RFLPs were observedin Southern blots of F56 DNA probed with cDNAs encoding outerarm dynein HCs or ICs (Koutoulis et al., 1997). We similarly didnot detect RFLPs in Southern blots of F56 DNA probed with cDNAsencoding ODA-DC polypeptides or LCs other than LC2 (Pazour andWitman, unpublished data). Therefore, F56 does not appear to havea defect in any outer dynein arm-associated protein other thanLC2.

Another cell line, V3, was missing the smaller of the two hybridizing bands (Figure 1A). V3 also had a slow-swimming phenotype(see below). To determine which part of the gene is deleted inV3, probes specific to each end of the LC2 cDNA were made by PCRamplification of the LC2 cDNA with T3 and T7 primers, digestingthe product with PvuII, and gel-purifying the resulting 0.6- and0.4-kbp bands. PvuII cuts the LC2 cDNA at only one site, betweenG614 and C615 in the ~550-bp 3' untranslated region (UTR) (seePatel-King et al., 1997, their Figure 1). Therefore, the 0.6-kbpprobe corresponds to the 5' UTR, the entire coding sequence, anda small amount (~60 bp) of the 3' UTR; the 0.4-kbp probe correspondsto the remainder of the 3' UTR. The 5' probe detected the largerband in DNA from V3 cells and cells that were wild-type for LC2(Figure 1B). The 3' probe detected the smaller band in DNA fromcells that were wild-type for LC2 but did not hybridize with anyband in DNA from the V3 cells (Figure 1B). This indicates thatthe 3' end of the gene is deleted in V3. Because the promoterand amino-terminal coding region are retained, these cells havethe potential to produce at least a portion ofLC2.

The LC2 Locus Is Tightly Linked to ODA12

To determine whether the slow-swimming phenotype was linked to the disruption of LC2, the F56 and V3 lines were back-crossedto wild-type cells. The swimming defect appears to be caused bya single nuclear mutation as the Oda phenotype segregated 2:2in 25 tetrads obtained from a back-cross of F56. DNA was isolatedfrom 15 offspring of the F56 cross and 19 offspring of the V3cross and examined by Southern blotting using the LC2 cDNA asa probe. Figure 2 shows that whenever the LC2 gene was disrupted,the cells had an Oda-swimming phenotype. This strongly suggeststhat the ODA12 gene encodes LC2 of the outer dynein arm. The totaldeletion allele has been designated oda12-1; the partial deletionallele has been designated oda12-2.

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Figure 2. The motility defect in the F56 and V3 strains segregates with the defect in the LC2 gene. (A) The initial F56 isolate was crossed to 137c, and a slow-swimming offspring was isolated and crossed again to 137c. Twenty-five tetrads were dissected from this cross and scored for motility. The Oda phenotype segregated 2:2. DNA was isolated from the four products of one full tetrad and a single product of 11 additional tetrads, cut with PstI, and analyzed by Southern blotting using the LC2 cDNA as the probe. In every case, the Oda $-$ phenotype segregated with the deletion revealed by the LC2 cDNA, indicating that the motility defect is tightly linked to this deletion mutation. (B) V3 was crossed to H8 $-$ (Wild Type), and the resultant tetrads were dissected. DNA was isolated from the parental strains, the four products of one tetrad, and a single product of 15 additional tetrads, cut with PvuII, and analyzed by Southern blotting with the LC2 cDNA as the probe. Again, the Oda $-$ phenotype segregated with the deletion revealed by the LC2 cDNA.

The discovery that the LC2 locus is tightly linked and probably identical to ODA12 provided an opportunity to obtain independentproof that ODA12 is a novel gene. CC2290 is a wild-type C. reinhardtiiisolate that is highly interfertile with 137c-derived lab strainsbut divergent enough that it is easy to identify RFLPs betweenthe two strains (Gross et al., 1988). We identified an RFLP detectedby the LC2 cDNA probe in DNA of CC2290 versus the 137c-derivedstrains (Figure 3). We then compared the segregation of this RFLPwith the segregation of uncloned genes that affect the outer armin crosses between CC2290 and cell lines (derived from 137c) carryingmutations in the latter genes. Uncloned genes affecting the outerarm include ODA5, ODA7, ODA8, PF13, and PF22 (ODA1 [Takada etal., 1996] and ODA10 [Pazour, Koutoulis, and Witman, unpublisheddata] have been cloned but not yet published). Tetrads from thecrosses were dissected, the progeny were scored for motility,and DNA was isolated from one product of 10 different tetrads.The segregation of the LC2 PvuII RFLP was scored by Southern blottingand compared with the segregation of the motility defect. If theoda12 mutation is an allele of (or is tightly linked to) one ofthese genes, all offspring that have motility defects will havethe 137c version of the LC2 PvuII RFLP. However, if oda12 is notan allele of one of these genes, the motility defect will segregateindependently from the LC2 PvuII RFLP. As can be seen in Table2, the LC2 PvuII RFLP segregated independently of oda5, oda7,oda8, pf13, and pf22, confirming that ODA12 is a novel gene.

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Figure 3. LC2 cDNA detects an RFLP between 137c and CC2290 strains. DNA from the lab strain 137c and the wild isolate CC2290 was cut with PvuII and analyzed by Southern blotting using the LC2 cDNA as a probe. This probe detects two bands of ~3.5 and ~0.9 kbp in 137c but only a single band of ~2.5 kbp in CC2290.

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Table 2. Segregation of the LC2 RFLP

Phenotype of oda12 Cells

Most of the known defects in ODA1-ODA10 cause loss of the outer dynein arms. As a result, the cells swim in a jerky mannerat ~30% of the normal speed. These mutant cells also have an alteredphotoshock response. During photoshock, which is induced by aflash of bright light, wild-type cells stop swimming, switch toa flagellar waveform, and swim backward for a few milliseconds(Schmidt and Eckert, 1976). In contrast, oda mutants stop in responseto the flash but do not swim backward (Mitchell and Rosenbaum,1985).

oda12-1 cells swim in a typical oda-like manner. They are slower than normal and have a jerky appearance as they swim forward.The swimming pattern of oda12-2 cells is not as slow or jerkyas that of oda12-1 or other oda mutant cells. Swimming speedswere quantitatively measured with an ExpertVision Motion Analysissystem (Figure 4). The swimming speeds of wild-type (g1) cellsare broadly distributed with a mean of 114 µm/s. The mean swimmingspeed of oda12-1 cells is reduced to 39 µm/s, whereas the speedof oda12-2 cells is slightly faster at 49 µm/s. Both oda12-1 andoda12-2 cells show an altered photoshock response; when flashedwith light, they stop briefly and then resume forward swimmingwithout a period of backward swimming.

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Figure 4. Swimming speed of wild-type and oda12 mutant cells. The Speed Operator of the ExpertVision Motion Analysis system was used to calculate the swimming speed of individual cells. The histograms show the distribution of speeds within each sample. These are plotted as the percentage of cells in each of 10 20-µm/s bins between 0 and 200 µm/s. The mean swimming speed (in micrometers per second) for each sample also is shown. Note that the mean swimming speed of oda12-2 cells (49 µm/s) is slightly faster than that of oda12-1 cells (39 µm/s). More than 100 cells were analyzed for each cell type.

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Figure 5. LC2 is required for assembly of outer dynein arms. (A) Electron micrographs of cross-sections of flagella of wild-type g1 cells show prominent outer dynein arms (arrows) on all of the doublet microtubules except for doublet one (arrowhead), which does not normally have an outer dynein arm (Hoops and Witman, 1983

). In contrast, the outer dynein arms are completely missing in flagella of the oda12-1 mutant (F56). The number of outer dynein arms in flagella of oda12-2 cells (V3) is variable; in this section outer dynein arms (arrows) are seen on only three doublet microtubules. (B) Axonemes from wild-type and the two oda12 mutants were separated by SDS-PAGE, transferred to a PVDF membrane, and analyzed by Western blotting. The blots were probed with antisera to IC140 (an inner arm IC), IC1 (an outer arm IC), and LC2. The anti-IC140 antisera reacted equivalently with a 140-kDa band in all three lanes, indicating that each lane was loaded with an equal number of axonemes. Neither the anti-LC2 antibody nor the anti-IC1 antibody recognized bands of the appropriate size in the oda12-1 axonemes, confirming that this mutant is completely lacking the outer dynein arm. However, these two antibodies did reveal a small amount of IC1 and LC2 in the oda12-2 axonemes. The antibody to IC1 also reacts with a smaller band (*) (Fowkes and Mitchell, 1998

) that is not part of the outer arm and is not affected by the oda12 mutation. The bottom panel shows a longer exposure of the blot probed with the LC2 antibody to demonstrate the small amount of LC2 in the oda12-2 axonemes.

LC2 Is Required for Assembly of the Outer Dynein Arm

Previously, we briefly reported that the oda12-1 mutant was lacking the outer dynein arms (Koutoulis et al., 1997), a defectconsistent with the swimming phenotype described above. Electronmicroscopic analysis indicates that whereas oda12-1 cells lackall of the outer dynein arms, oda12-2 cells are much more variable(Figure 5A). Some flagellar cross-sections have no outer dyneinarms, whereas others have significant numbers. This indicatesthat the partial deletion does not completely abolish the assemblyof outerarms.

Western blot analysis was used to more quantitatively assess the loss of outer dynein arms in oda12-1 and oda12-2 cells. Axonemeswere isolated from wild-type cells and from each of the mutants.Equal amounts of protein (standardized to tubulin) were separatedby SDS-PAGE and transferred to a PVDF membrane. The blot was firstprobed with an antibody to an inner dynein arm subunit (IC140)that should not be affected by the oda12 mutations. All threelanes had similar amounts of this antigen, confirming that equalnumbers of axonemes had been loaded in each lane on the gel (Figure5B). The blot was then probed with antibodies to outer dyneinarm subunits IC1 and LC2 (Figure 5B). Both proteins were readilydetected in axonemes of wild-type cells. In contrast, neitherprotein was detected in axonemes of oda12-1 cells, confirmingthat LC2 and the outer dynein arm is completely missing in thismutant. However, small amounts of IC1 and LC2 were detected inoda12-2 cells; the oda12-2 LC2 appeared to migrate with the samerelative mobility as the wild-type LC2. Therefore, oda12-2 cellsproduce small amounts of apparently full-length LC2. This is sufficientto permit assembly of some outer arms, although the loss of outerarms appears to be more severe than indicated by electronmicroscopy.

The oda12 Phenotype Can Be Rescued by Transformation with DNA Encoding LC2

To determine whether the oda12 phenotype is due specifically to loss of LC2, we assayed the ability of the LC2 gene to restorethe wild-type phenotype to oda12 mutant cells. Three genomic clonesencoding LC2 were isolated from a $lambda$ phage library using the LC2cDNA clone as a probe. Two of these, $lambda$ ODA12#17 and $lambda$ ODA12#20,had very similar restriction patterns. The third, $lambda$ ODA12#8, wasshifted along the chromosome slightly from the first two (Figure6A). The LC2 coding region (as determined by hybridization) iscontained completely within a 3.1-kbp HindIII fragment commonto all three clones (Figure 6A, dark bar). DNA from each of thesethree $lambda$ phage was transformed into the cell line 2567.1 (whichcarries oda12-1 and arg7 mutations), along with DNA containingthe ARG7 gene. Individual ARG7 transformants were screened bylight microscopy to determine whether the oda12 motility phenotypehad been rescued as a result of cotransformation with the phageDNA. All three phage clones were able to rescue the defect (Figure6A), indicating that each carried the complete ODA12 gene. Theinsert from $lambda$ ODA12#17 was subcloned into a plasmid vector andnamed pHS44; as expected, this also was able to rescue the motilitydefect. The locus was further refined by subcloning the 5.7-kbpKpnI-SalI and the 3.1-kbp HindIII fragments, which were termedpBD17 and pBD14, respectively. Both of these fragments complementedthe oda12 defect (Figure 6A), indicating that ODA12 is locatedwithin the 3.1-kbp fragment that also contained the LC2 codingregion as determined by hybridization. This data provide verystrong evidence that the outer dynein arm defect of oda12 is theresult of the LC2 deletion.

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Figure 6. Rescue of oda12 by transformation. (A) Map of the ODA12 locus. Three genomic $lambda$ phage clones ( $lambda$ ODA12#8, $lambda$ ODA12#17, and $lambda$ ODA12#20) were isolated and mapped. The EcoRI sites at the ends of the clones are derived from the vector. The LC2 coding region (dark bar) was determined by hybridization with the cDNA clone. The 16-kbp insert from $lambda$ ODA12#17 was cloned into pKS+ and named pHS44. The 5.7-kbp KpnI-SalI and 3.1-kbp HindIII fragments of pHS44 were subcloned and named pBD17 and pBD14. The number of cell lines in which the Oda $-$ phenotype was rescued out of the total number of ARG7 transformants screened is shown on the right. (B) Swimming speeds of transformed cell lines. The Speed Operator of the ExpertVision Motion Analysis system was used to calculate the swimming speed of five transformed lines (S1-S5). The histograms show the distribution of speeds within each sample. These are plotted as a percentage ofcells in each of 10 20-µm/s bins between 0 and 200 µm/s. The mean swimming speed (micrometers per second) for each sample also is shown. More than 100 cells were analyzed for each cell line. (C) Segregation of the exogenous copy of ODA12. oda12-1, arg7 strains were transformed with genomic clones of the ODA12 gene. One transformant (S20) that showed wild-type swimming speeds was mated to an oda12-1 strain of the opposite mating type, and tetrads were dissected. The offspring were scored for motility, and DNA was isolated from them. The DNA was cut with PvuII and analyzed by Southern blotting using the LC2 cDNA as a probe. The probe hybridizes with two bands in DNA from wild-type cells but does not hybridize with any band in DNA from oda12-1 cells (see Figure 1). Analysis of one full tetrad and a single product from each of 12 additional tetrads showed that fast-swimming cells (Oda+) had the LC2-hybridizing bands, whereas the slow-swimming cells (Oda $-$ ) were missing these bands. (D) Electron microscopy of flagella of transformed cells. Transformant S3, which swims at a speed similar to that of wild-type (cf. Figure 4 and B), has a full complement of outer dynein arms (left panel, arrows). In contrast, cells of transformed strain S1, which have a wide range of swimming speeds (Figure 6B), have variable numbers of outer dynein arms (right panel, arrows).

The swimming speed of five independent transformants was measured. All swam faster than the oda12-1 mutant line and had recoveredthe ability to swim backward when photoshocked. TransformantsS3 (from $lambda$ ODA12#20), S4 (from $lambda$ ODA12#20), and S5 (from $lambda$ ODA12#8)were similar to wild-type in both mean swimming speed and thedistribution of swimming speeds (cf. Figures 4 and 6B). TransformantS2 (from $lambda$ ODA12#17) was similar to wild-type except for a greaternumber of very slow cells that reduced its mean speed to 82 µm/s(Figure 6B). The swimming speeds of transformant S1 (from $lambda$ ODA12#17)were very broadly distributed around a mean of 81 µm/s (Figure6B). The mixed distribution of swimming speeds seen in the S1and S2 populations was not the result of an impure culture, becausethe cells were cloned from a single cell before analysis. Morelikely, it was the result of gene silencing, whereby newly integratedgenes in some Chlamydomonas cells become transcriptionally inactivated(Cerutti et al. 1997).

To confirm that the rescue of the Oda $-$ phenotype was due to integration of the cloned DNA and not suppression of the mutantphenotype, transformant S20 (obtained by transformation of 2507.1with pHS44), which has wild-type motility, was crossed to an oda12-1line and the resultant tetrads dissected. Motility of the offspringwas scored, and DNA was isolated and analyzed by Southern blottingusing the LC2 cDNA as a probe (Figure 6C). This probe revealedthat the two PvuII restriction fragments observed in wild-typecells, but missing in the oda12-1 line, were restored in the rescuedcell lines. Analysis of one full tetrad and single products of12 additional tetrads showed that whenever the two PvuII bandswere present, the cells swam with wild-type speeds. This indicatesthat restoration of the phenotype is due to the clonedDNA.

Transformants S1 and S3 were examined by electron microscopy to determine whether the outer dynein arms had been restored(Figure 6D). Transformant S3, which had a distribution of swimmingspeeds similar to that of wild type, had a full complement ofouter dynein arms. In contrast, cells of the transformant S1,which had a broader distribution of swimming speed and a lowermean swimming speed, showed a corresponding variability in therestoration of arms. Most of the flagellar cross-sections showedintermediate numbers of arms, but in a few, no arms were present,suggesting that the intermediate swimming speed was due to restorationof only some of the outer dyneinarms.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In this report we describe, for the first time, mutations in the C. reinhardtii gene encoding LC2, an LC that is specificfor the outer dynein arm. Deletion of this gene leads to lossof the outer dynein arm and impaired flagellar motility. The LC2gene is the Chlamydomonas homologue of mouse Tctex2 (Patel-Kinget al., 1997), which has been identified as one of the distortergenes of the t haplotype (Huw et al., 1995). The finding thatLC2 is essential for outer arm assembly supports the hypothesisthat some of the phenotypes expressed by t haplotypes are dueto interactions between defective dynein polypeptides and suggestsa specific model by which this mightoccur.

Function of LC2

Although mutations are known for each of the HCs and ICs of the Chlamydomonas outer dynein arm, previously a mutation hasbeen identified in only one gene (FLA14) that encodes an outerarm LC, LC8 (Pazour et al., 1998). However, LC8 also is a componentof inner arm dynein, cytoplasmic dynein, and myosin (Espindolaet al., 1996; King et al., 1996a; Harrison et al., 1998), andknockout of the LC8 gene has pleiotropic effects that are difficultto interpret in terms of the specific role of LC8 in the outerdynein arm. In contrast, LC2 appears to be specific for the outerarm. Complete deletion of the LC2 gene causes a complete lossof the outer dynein arm, with no other structural changes in theflagellar axoneme. Loss of the outer arms in this mutant causesa decrease in swimming speed to ~34% of that of wild-type cells,a reduction similar to what has been observed for other mutationsthat cause complete loss of the outer dynein arm (Mitchell andRosenbaum, 1985; Kamiya, 1988). Loss of the outer arm also causesloss of the ability to swim backward during the photoshock response,as reported previously for a mutant with a defect in the outerarm (Mitchell and Rosenbaum, 1985).

It is most remarkable that LC2, which has a mass of only 15.8 kDa (King and Patel-King, 1995a), is absolutely essential forassembly of the outer dynein arm, which contains at least 13 differentpolypeptides and has a total mass of ~2 MDa (Table 1; Witmanet al., 1983). Two independent lines of evidence indicate thatLC2 is a component of the IC-LC complex (Mitchell and Rosenbaum,1986; King and Witman, 1990; Witman et al., 1992), which is locatedat the base of the dynein (King and Witman, 1990). First, LC2is associated with the $beta$ subunit of the outer dynein arm (Pfisterand Witman, 1984) and is retained in the Chlamydomonas mutantoda4-s7, which expresses only the NH₂-terminal one-third of the $beta$ HC (Sakakibara et al., 1993). This portion of the $beta$ HC formsthe stem and base of the outer arm dynein (Witman et al., 1994)and binds the IC-LC complex (King and Witman, 1989). Second, afterdissociation of the outer arm dynein with nonionic detergent,LC2 was immunoprecipitated as part of an aggregate with IC1, IC2,and another LC (Mitchell and Rosenbaum, 1986). Therefore, by virtueof its location in the arm, LC2 is in a position to interact directlywith tubulin or the ODA-DC and might be required for binding apreassembled outer dynein arm to the doublet microtubule. Alternatively,LC2 might be required for preassembly of the outer dynein armin the cytoplasm (Fowkes and Mitchell, 1998), for stability ofthe preassembled complex, or even for transport of the preassembledcomplex into the flagellum. Whatever the precise reason, the currentfindings demonstrate that LC2 has an important role in dyneinassembly. It is likely that the LCs of other dyneins have equallyimportant roles in the complexes of which they are apart.

LC2 is Encoded by ODA12

We previously identified a novel Chlamydomonas gene, ODA12, that was necessary for outer arm assembly (Koutoulis et al., 1997);however, the product of this gene was not determined. The followingevidence now indicates that ODA12 encodes LC2: 1) Southern hybridizationshowed that the gene encoding LC2 is completely deleted in theoriginal oda12 mutant strain; 2) the defining phenotype of oda12cells segregated with the LC2 deletion in crosses between oda12and wild-type cells; and 3) the oda12 phenotype was rescued bytransformation of oda12 cells with a small (3.1-kbp) genomic DNAclone containing the LC2 gene. Thus, the phenotype observed foroda12 cells is due to the deletion of the LC2gene.

The current findings also confirm that ODA12 is a novel gene, distinct from any of the other ODA or similar genes that havebeen reported. Previously, we reported that cDNA clones encodingODA1, ODA2, ODA3, ODA4, ODA6, ODA9, and ODA11 detected no RFLPsin oda12 versus wild-type strains, and that oda12 complementedoda1, oda3, oda5, oda7, oda8, oda10, pf13, and pf22 in stablediploids (Koutoulis et al., 1997). Similarly, we determined thatcDNA clones encoding the unpublished genes ODA13 and ODA14 (Table1) did not detect RFLPs in oda12 versus wild-type strains (Pazourand Witman, unpublished results). We now have used the LC2 cDNAas a physical marker for the ODA12 gene and find that an RFLP,detected by the cDNA in CC2290 versus 137c-derived strains, segregatesindependently of oda5, oda7, oda8, pf13, and pf22. These resultsprovide additional evidence that ODA12 cannot be the same as anyof thosegenes.

With the discovery that the ODA12 gene product is an outer dynein arm LC, only four known ODA genes (ODA5, ODA7, ODA8, andODA10) and two known PF genes (PF13 and PF22) that affect outerarm assembly have yet to have their products identified. It willbe of great interest to determine the products of these genesand their roles in outer arm assembly. It may not be coincidentalthat the products of six ODA or ODA-like genes are still unknown,whereas mutations have not yet been reported for an identicalnumber of outer dynein arm LCs (Table 1). The current findingsunderscore the possibility that some of these other LCs also couldbe critical for dynein assembly. The ease with which a reversegenetics approach may be applied to Chlamydomonas should greatlyfacilitate the identification of mutants with defects in thesepolypeptides.

oda12-2 Is a Hypomorphic Allele

The results presented here show that the oda12 mutation originally reported by Koutoulis et al. (1997) is a complete deletionof the LC2 gene; this allele has been designated oda12-1. Herewe also describe a second allele (oda12-2) in which only the 3'end of the LC2 gene is deleted. Ultrastructural analysis revealedthat the oda12-2 mutant assembles only a few outer arms on itsdoublet microtubules (Figure 5A). Presumably because some outerarms are present, oda12-2 cells swim slightly faster than oda12-1cells (Figure 4A). Western blot analysis confirmed that the outerdynein arm polypeptide IC1 is greatly diminished but not entirelymissing in axonemes of oda12-2 (Figure 5B). Interestingly, a smallamount of approximately full-length LC2 also is present in theoda12-2 axoneme. That an apparently full-length product is synthesizedsuggests that the oda12-2 deletion removes most or all of the3' UTR but little if any of the coding sequence. The 3' UTR ofeukaryotic mRNAs has several important functions, including controlof mRNA stability (Beelman and Parker, 1995; Decker and Parker,1995; Wickens et al., 1997) and mRNA localization (Wilhelm andVale, 1993; Decker and Parker, 1995). A defect in either of thesefunctions likely would result in the production of reduced amountsof LC2, which in turn would permit assembly of reduced numbersof outer arms. The incorporation of small amounts of LC2 alongwith equally small amounts of IC1 into the oda12-2 axonemes isconsistent with LC2 being absolutely essential for outer dyneinarmassembly.

Dynein Defects and t Haplotype Phenotypes

The mouse t haplotype is an ~30-Mb region of chromosome 17 containing numerous genes and defined by the presence of four inversionsrelative to the wild-type homologue, so that recombination issuppressed and the entire region usually segregates as a singleunit (Olds-Clarke and Johnson, 1993; Silver, 1993). One of themost intriguing phenotypes of the t haplotype is that heterozygous+/t males transmit the t haplotype-bearing version of chromosome17 to >95% of their progeny. Analysis of partial t haplotypesresulting from rare recombination events within the t complexindicate that this transmission ratio distortion, or meiotic drive,is the result of two or three distorter genes, located in differentparts of the t haplotype, acting on a single responder gene, termedTcr (t complex responder) (Lyon, 1984). The distorter genes canact cis or trans on the responder gene, and their effects areadditive. The result of these interactions is to increase theprobability of transmission of the chromosome carrying the t haplotyperespondergene.

The discovery that some of the candidate distorter genes encode dynein LCs has prompted a model that explains the t haplotypephenotype on the basis of interactions between dyneins and otheraxonemal components (Patel-King et al., 1997; Harrison et al.,1998). The current finding that LC2 is important for dynein assemblypermits the model to be described in more specific terms (Figure7). In this model, the responder gene encodes a protein (Tcr)that is expressed in the haploid nucleus and remains associatedwith that nucleus throughout the remainder of spermiogenesis.Because soluble components can diffuse through the intercellularbridges that connect developing spermatids, this protein mustbecome rapidly associated with some structural component of thespermatid, such as the basal body or the elongating axoneme, toprevent its diffusion to neighboring spermatids. Ultimately, Tcrmust interact with the dynein arms. For the sake of simplicity,we will assume that Tcr is part of an axonemal component suchas the ODA-DC (Takada and Kamiya, 1994; Koutoulis et al., 1997)or the dynein regulatory complex (Gardner et al., 1994; Pipernoet al., 1994) that interacts directly with the dynein arms, butit could interact with the arms indirectly, as through a basalbody-associated templating activity that determines the locationof the outer dynein arm binding sites on the doublet microtubule.In contrast, the distorter proteins, which include subunits ofthe inner and outer dynein arms, diffuse through the intercellularbridges, so that both wild-type and mutant (t haplotype-encoded)dyneins are preassembled in the cytoplasm of both spermatids bearingthe wild-type responder (Tcr⁺) and spermatids bearing the t haplotype-encoded responder (Tcr^t).

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Figure 7. Model for mouse t phenotypes based on dynein-axoneme interactions. In all cases, the distorter gene (d) products, which are dynein subunits, are free to diffuse (arrows) through the intercellular bridges that connect developing spermatids. However, the responder gene (Tcr) product quickly assembles onto the axoneme and thus remains associated with the nucleus that encoded it. Wild-type and t-encoded proteins are indicated by open and filled symbols, respectively. t-encoded dyneins contain mutations that affect their assembly and/or function; the t-encoded responder contains mutations that affect its ability to bind t-encoded dyneins. (A) In developing spermatids of heterozygous +/t mice, the mutated t responder binds only wild-type dyneins, preventing incorporation of mutant dyneins into the axoneme associated with the nucleus carrying the t haplotype. In contrast, the wild-type responder binds both wild-type and mutant dyneins; the mutant dyneins "poison" the axoneme into which they are incorporated. As a result, the sperm bearing the t haplotype has slightly impaired motility (because of the presence of the mutant responder), but the sperm with the wild-type homologue has greatly impaired motility. The sperm bearing the t haplotype is much more likely to reach and fertilize an egg, thus leading to transmission ratio distortion. (B) In spermatids of homozygous t/t mice, all dyneins produced are defective and bind poorly to the t-encoded responder. The resulting sperm are nonmotile, and the mice are sterile. (In this case, all spermatids are identical, so only one is shown.) (C) In mice containing a partial t haplotype with a t-encoded responder, but no t-encoded distorters, only wild-type dyneins are produced and assembled into the axonemes. Sperm carrying Tcr^t and sperm carrying Tcr⁺ are both motile, although the former will suffer a competitive disadvantage because of the presence of the t-encoded responder in their axonemes.

The model predicts that Tcr^t binds wild-type dynein strongly but mutant dynein less efficiently. In +/t mice (Figure 7A), bothtypes of dyneins will be present in the cytoplasm of the developingspermatid. The wild-type dyneins will out-compete the mutant dyneinsfor binding sites on the Tcr^t-containing axoneme, with the result that these axonemes willassemble a nearly normal complement of arms and have motilitythat is only slightly impaired because of the presence of Tcr^t (see below). In contrast, the model predicts that Tcr⁺ binds both wild-type and mutant dyneins equally, with the resultthat both types of dyneins will be assembled into the Tcr⁺-containing axonemes. Because of the presence of many mutant dyneinsin these latter axonemes, the resulting sperm will be much lessefficient than those containing Tcr^t in some critical aspect of motility, resulting in transmissionratiodistortion.

A second phenotype of the t haplotype that is readily accounted for by this model is that t/t males are sterile (Figure 7B).t/t males will produce only mutant dynein, which has a low affinityfor Tcr^t. As a result, few arms will be assembled into the axoneme, andif they are assembled they will be defective. The resulting spermwill have aberrant or no motility and be unable to fertilize anegg.

In an analysis of partial t haplotypes, it was observed that if a t-encoded responder was present on one chromosome, withno t-encoded distorters acting on it cis or trans, then that chromosomewas transmitted at a low ratio (11-17%) (Lyon, 1984). This suggeststhat the mutant responder itself impairs the motility of Tcr^t-bearing sperm. This also is compatible with our model (Figure7C). In spermatids of such mice, only wild-type dynein is present,and it binds to both Tcr^t- and Tcr⁺-containing axonemes. The resulting Tcr^t-containing sperm will have slightly impaired motility as a resultof having Tcr^t in their axonemes. This motility will not be so compromised thatthe sperm are unable to fertilize an egg and not as defectiveas that of Tcr⁺-containing spermatids with a mixture of mutant and wild-typedyneins (see Figure 7A). Nevertheless, they will have a competitivedisadvantage, compared with Tcr⁺-containing sperm with only wild-type dyneins, in reaching andfertilizing theegg.

The sperm motility phenotypes predicted by this model are in good agreement with observations of sperm from +/t and t/t mice(summarized by Harrison et al., 1998). For example, sperm fromt/t mice rarely exhibit a regular beat pattern and have littleprogressive motility, whereas the mean swimming speed of spermfrom +/t mice is intermediate between that of t/t and +/+ mice(Olds-Clarke and Johnson, 1993). Moreover, sperm from +/t miceseparate into two subpopulations, one having nearly normal motilityand the other having abnormal motility (Olds-Clarke and Johnson,1993); the former may correspond to Tcr^t-containing sperm, and the latter may correspond to Tcr⁺-containing sperm. Certainly these motility defects could be accountedfor by defects in dynein arm assembly and/or function. As indicatedby our analysis of the oda12-2 mutant compared with oda12-1 andwild-type cells, intermediate levels of outer dynein arms canresult in intermediate swimming speeds. Furthermore, Chlamydomonascells with defects in both the inner and outer arms have a moresevere phenotype than those with a defect in either arm alone(Kamiya et al., 1989), which is consistent with the additive effectsof the distorter genes in mice (Lyon, 1984). Finally, at leastsome of the motility defects observed in sperm of +/t mice aredependent on Ca²⁺ (Olds-Clarke and Johnson, 1993), and both inner and outer dyneinarms are involved in Ca²⁺-mediated changes in flagellar waveform. For example, in Chlamydomonas,the inner arms are involved in phototactic steering (King andDutcher, 1997), and mutants with defects in the outer arm aredefective in backward swimming during photoshock (Mitchell andRosenbaum, 1985; this report); both of these responses are mediatedby Ca²⁺.

Conclusion

The above model should be readily testable by further molecular genetic and biochemical studies of t haplotype-bearing mice.Of particular importance will be identification of the productsof the Tcr gene and of the remaining distorter genes. In any case,the findings presented here demonstrate for the first time thata defect in a dynein LC can have a profound effect on outer armassembly. It is likely that the LCs have equally important rolesin other dyneins. Because oda12-1 is a null mutant, it shouldnow be possible to investigate LC function by in vitro mutagenesisof the ODA12 gene, followed by transformation of the modifiedgene into the oda12-1 mutant, where the modified gene productshould be assembled into an outer dynein arm. The effects of theLC modification on flagellar movement and dynein activity in vitrocould then bedetermined.

	ACKNOWLEDGMENTS

We thank Dr. J. Aghajanian (Worcester Foundation for Biomedical Research, Shrewsbury, MA) for the electron microscopy presentedin this study and Drs. P. Yang and W. Sale (Emory University,Atlanta, GA) for the gift of the anti-IC140 antibody. These studieswere supported by grants from the National Institutes of Health(GM30626 to G.B.W. and GM51293 to S.M.K.) and the Campbell andHall Charity Fund (to G.B.W.).

	FOOTNOTES

^§ Corresponding author. E-mail address: george.witman{at}umassmed.edu.

ABBREVIATIONS

Abbreviations used: HC, heavy chain; IC, intermediate chain; LC, light chain; ODA-DC, outer dynein arm docking complex; PVDF, polyvinylidene difluoride; RFLP, restriction fragment length polymorphism; UTR, untranslated region.

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King, S.J., and Dutcher, S.K. (1997). Phosphoregulation of an inner dynein arm complex in Chlamydomonas reinhardtii is altered in phototactic mutant strains. J. Cell Biol. 136, 177-191[Abstract/Free Full Text].
King, S.M., Barbarese, E., Dillman, J.F., III, Patel-King, R.S., Carson, J.H., and Pfister, K.K. (1996a). Brain cytoplasmic and flagellar outer arm dyneins share a highly conserved M_r 8,000 light chain. J. Biol. Chem. 271, 19358-19366[Abstract/Free Full Text].
King, S.M., Dillman, J.F., III, Benashski, S.E., Lye, R.J., Patel-King, R.S., and Pfister, K.K. (1996b). The mouse t-complex-encoded protein Tctex-1 is a light chain of brain cytoplasmic dynein. J. Biol. Chem. 271, 32281-32287[Abstract/Free Full Text].
King, S.M., Otter, T., and Witman, G.B. (1985). Characterization of monoclonal antibodies against Chlamydomonas flagellar dyneins by high-resolution protein blotting. Proc. Natl. Acad. Sci. USA 82, 4717-4721[Abstract/Free Full Text].
King, S.M., Otter, T., and Witman, G.B. (1986). Purification and characterization of Chlamydomonas flagellar dyneins. Methods Enzymol. 134, 291-306[Medline].
King, S.M., and Patel-King, R.S. (1995a). Identification of a Ca²⁺-binding light chain within Chlamydomonas outer arm dynein. J. Cell Sci. 108, 3757-3764[Abstract].
King, S.M., and Patel-King, R.S. (1995b). The M_r = 8,000 and 11,000 outer arm dynein light chains from Chlamydomonas flagella have cytoplasmic homologues. J. Biol. Chem. 270, 11445-11452[Abstract/Free Full Text].
King, S.M., Patel-King, R.S., Wilkerson, C.G., and Witman, G.B. (1995). The 78,000-Mr intermediate chain of Chlamydomonas outer arm dynein is a microtubule-binding protein. J. Cell Biol. 131, 399-409[Abstract/Free Full Text].
King, S.M., and Witman, G.B. (1989). Molecular structure of Chlamydomonas outer arm dynein. In: Cell Movement, vol. I: The Dynein ATPases, ed. F.D. Warner, P. Satir, and L.R. Gibbons, New York: Alan R. Liss, 61-75.
King, S.M., and Witman, G.B. (1990). Localization of an intermediate chain of outer arm dynein by immunoelectron microscopy. J. Biol. Chem. 265, 19807-19811[Abstract/Free Full Text].
Koutoulis, A., Pazour, G.J., Wilkerson, C.G., Inab