Gene Knockouts Reveal Separate Functions for Two Cytoplasmic Dyneins in Tetrahymena thermophila

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Vol. 10, Issue 3, 771-784, March 1999

Gene Knockouts Reveal Separate Functions for Two Cytoplasmic Dyneins in Tetrahymena thermophila

Seungwon Lee,^* Julie C. Wisniewski,^* William L. Dentler, and David J. Asai^*

^*Department of Biological Sciences, Purdue University, West Lafayette, Indiana 47907-1392; and Department of Molecular Biosciences, University of Kansas, Lawrence, Kansas 66045

Submitted August 6, 1998; Accepted November 18, 1998
Monitoring Editor: J. Richard McIntosh

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

In many organisms, there are multiple isoforms of cytoplasmic dynein heavy chains, and division of labor among the isoformswould provide a mechanism to regulate dynein function. The targeteddisruption of somatic genes in Tetrahymena thermophila presentsthe opportunity to determine the contributions of individual dyneinisoforms in a single cell that expresses multiple dynein heavychain genes. Substantial portions of two Tetrahymena cytoplasmicdynein heavy chain genes were cloned, and their motor domainswere sequenced. Tetrahymena DYH1 encodes the ubiquitous cytoplasmicdynein Dyh1, and DYH2 encodes a second cytoplasmic dynein isoform,Dyh2. The disruption of DYH1, but not DYH2, resulted in cellswith two detectable defects: 1) phagocytic activity was inhibited,and 2) the cells failed to distribute their chromosomes correctlyduring micronuclear mitosis. In contrast, the disruption of DYH2resulted in a loss of regulation of cell size and cell shape andin the apparent inability of the cells to repair their corticalcytoskeletons. We conclude that the two dyneins perform separatetasks in Tetrahymena.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Dynein is a molecular motor that transduces chemical energy into mechanical motion along microtubules. There are two functionalclasses of dynein: axonemal dynein that produces the propagatedbending of cilia and of eukaryotic flagella and nonaxonemal or"cytoplasmic" dynein that performs functions other than ciliarybeating. Cytoplasmic dynein is implicated in a variety of intracellularmovements, including fast retrograde transport (Schroer et al.,1989; Muresan et al., 1996), slow axonal transport (Clevelandand Hoffman, 1991; Dillman et al., 1996), mediation of the traffickingof membrane-bounded organelles (Corthesy-Theulaz et al., 1992;Aniento et al., 1993; Fath et al., 1994; Oda et al., 1995; Holleranet al., 1996), the organization and separation of the bipolarmitotic spindle (Verde et al., 1991; Vaisberg et al., 1993; Saunderset al., 1995; Echeverri et al., 1996), and postmitotic nuclearmigrations in yeast and filamentous fungi (Eshel et al., 1993;Li et al., 1993; Plamann et al., 1994; Xiang et al., 1994; Inoueet al., 1998).

The realization that dynein performs so many different tasks and the discovery that many organisms express multiple dyneinheavy chain genes lead to the hypothesis that different dyneinisoforms perform different cellular tasks (reviewed in Asai, 1996).Cilia and eukaryotic flagella provide clear examples of dyneinfunctional specialization (Piperno, 1990). The close coordinationof ~12 distinct axonemal dynein heavy chains produces axonemalbending (e.g., Piperno and Ramanis, 1991; Mastronarde et al.,1992; reviewed in Brokaw, 1994).

The functional specialization of the cytoplasmic dyneins is not well understood. All eukaryotes examined express homologuesof the ubiquitous Dyh1 (also called MAP1C, cDHC1, DHC1a), andsome organisms, including Saccharomyces, Aspergillus, Neurospora,and Dictyostelium, apparently have only this dynein. In the analysisof the family of dynein genes expressed in sea urchin, the catalyticdomain of a second putative cytoplasmic dynein heavy chain, originallycalled DYH1b and here referred to as Dyh2, was identified andpartly sequenced (Gibbons et al., 1994). Homologues of Dyh2 havesubsequently been identified in mammals, in which it has beencalled DLP4, DHC1b, and cDHC2 (Tanaka et al., 1995; Criswell etal., 1996; Criswell and Asai, 1998; Vaisberg et al., 1996). Thissecond cytoplasmic dynein isoform also has been identified inChlamydomonas (Pazour et al., 1999; Porter et al., 1999) and Caenorhabditiselegans (Wilson et al., 1994). In this manuscript, we describetwo Tetrahymena dynein heavy chain genes: DYH1 encodes Dyh1 proteinthat is the homologue of sea urchin 1a, and DYH2 encodes Dyh2that is the homologue of sea urchin 1b. To simplify the followingdiscussion, we use "Dyh1" and "Dyh2" to describe these isoformsthat, in the original manuscripts, were referred to by othernames.

Previous studies provide compelling evidence that Dyh2 is a bona fide cytoplasmic dynein. The gene encoding Dyh2 is expressedin unciliated tissues (Tanaka et al., 1995; Criswell et al., 1996;Vaisberg et al., 1996). The Dyh2 protein was immunolocalized tothe Golgi apparatus in unciliated fibroblasts (Vaisberg et al.,1996), and injection of antibodies to Dyh2 caused the dispersalof the Golgi apparatus (Vaisberg et al., 1996). The expressionof the gene encoding Dyh2 but not Dyh1 was shown to be upregulatedduring ciliogenesis in primary cultures of rat tracheal epithelialcells, and isoform-specific antibodies revealed that Dyh2 proteinaccumulated at the apical ends of these cells but appeared tobe excluded from the cilia (Cris-well et al., 1996).

As do larger eukaryotes, the ciliated protozoan Tetrahymena thermophila expresses ~15 separate dynein heavy chain genes, includingones encoding Dyh1 and Dyh2 (Lee et al., 1997). The Tetrahymenamicrotubule cytoskeleton includes a cortical cage that helps todetermine cell size and shape and provides the framework for therows of ciliary basal bodies and other cytoplasmic microtubulesthat mediate intracellular movements including micronuclear mitosisand meiosis (reviewed in Frankel, 1999). Each cell has two functionallydistinct nuclei: the diploid germline micronucleus is transcriptionallysilent and therefore not required for vegetative growth, and thesomatic macronucleus contains ~45 copies of each gene and determinesthe phenotype of the cell. During vegetative growth, the celldivides every ~2.5 h during which an intranuclear mitotic spindlemediates the accurate separation of the five micronuclear chromosomes.However, unlike the micronucleus, the macronucleus divides amitotically,being pinched apart during cytokinesis. The amitotic divisionof the macronucleus separates the somatic genome imperfectly andcan lead to phenotypic assortment of a macronuclear allele (Sonneborn,1974). Because the micronucleus is not transcribed, the accuratesegregation of micronuclear chromosomes is not required for vegetativegrowth. Indeed, many species of Tetrahymena are amicronucleate;they are propagated vegetatively but cannot undergo sexual reproduction(Nanney and Simon, 1999).

Recent advances provide efficient methods to achieve macronuclear gene disruption in which a selectable marker is insertedinto the targeted chromosome exclusively by homologous recombination(Gaertig and Gorovsky, 1992; Cassidy-Hanley et al., 1997). Phenotypicassortment leads to the rapid and complete replacement of thewild-type gene if the targeted gene is not required for growthor to the incomplete elimination of an essential gene. In bothcases, the transformants remain viable, and even in the case ofan incomplete replacement, a phenotype may be observed. Thus Tetrahymenapresents the unique opportunity to focus on the cellular contributionsof an individual dynein in a cell with many dyneins. In the presentstudy, we have disrupted the macronuclear DYH1 and DYH2 genesindividually. These disruptions reveal that the two cytoplasmicdyneins are functionallyspecialized.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Nomenclature Used in This Manuscript

The nomenclature originally introduced in the sea urchin study (Gibbons et al., 1994) is useful because it organizes the dyneinheavy chains in a hierarchy based on the sequences of the catalyticdomains (see Gibbons, 1995). However, similarity between sequencesdoes not necessarily mean that the two dyneins are also functionallyrelated. Thus, we have adopted a nomenclature that is neutralin terms of dynein function and is in keeping with the recentlyadopted rules for naming Tetrahymena genes (Allen et al., 1998).

Cloning and Characterization of DYH1 and DYH2

Degenerate oligonucleotide primers corresponding to conserved sequences near the dynein P1 loop were used in RNA-directedPCR (reverse transcription [RT]-PCR) (Asai and Criswell, 1995).Sequencing of the 180-bp RT-PCR products identified several differentdynein heavy chain fragments, including ones whose deduced aminoacid sequences corresponded to those of Dyh1 and Dyh2 describedin other organisms. Genomic clones of Tetrahymena DYH1 and DYH2were obtained by screening a phage library constructed from wild-type(B2086) macronuclear DNA partially digested with BglII and ligatedinto the XhoI-half site of the lambda arms (LambdaGem-11, Promega,Madison, WI). Double-stranded DNA was purified (plasmid columns,Qiagen, Chatsworth, CA) and sequenced using Thermo Sequenase (Amersham,Cleveland, OH) or by the Purdue Center for DNA sequencing usingcycle-sequencing methods. Sequences were analyzed with the GCGsoftware package (version 9.1 [1997], University of Wisconsin,Madison, WI). Southern blots of genomic DNA and Northern blotsof total RNA (Chomczynski and Sacchi, 1987) were processed bystandard methods (Sambrook et al., 1989). The Northern blot ofRNA from reciliating cells (see Figure 2) was probed, strippedby treating the blot for 5 min with hot 0.1% SDS, and then reprobed.The intensities of the signals were estimated by densitometryusing ImageQuant (Molecular Dynamics, Sunnyvale,CA).

The intron-exon organizations of the genes were determined by RNA-directed PCR. RT-PCR using primers whose sequences werederived from the genomic sequence was used to produce overlappingcDNAs spanning the catalytic domains of DYH1 and DYH2. Approximately20 µg of total RNA from wild-type (B2086) cells was primed with100 pmol of random hexamers and reverse-transcribed (SuperscriptII, Life Technologies, Gaithersburg, MD). Approximately 1 µg ofthe resulting cDNA was then used as the template for each PCRreaction. The amplified cDNAs were purified andsequenced.

Targeted Disruption of Macronuclear DYH1 and DYH2

The neomycin-resistance gene was inserted into the coding region of each dynein gene using the p4T2-1 disruption plasmid (thegift of Dr. Marty Gorovsky, University of Rochester, Rochester,NY) that contains the histone 4 promoter region, the neomcyin-resistancecoding region, and the 3'-untranslated region of $beta$ tubulin. TheDYH1 disruption construct was made by inserting the neo gene atthe KpnI site, and the DYH2 disruption construct was made by deletingthe 1.8-kb EcoRV-EcoRV fragment and replacing it with the neogene (see Figure 3, a and b). Transformation was achieved by biolisticbombardment of mating cells (Cassidy-Hanley et al., 1997). Wild-typeB2086 and CU428.1CSHL cells (from Dr. Peter Bruns, Cornell University,Ithaca, NY) were starved in 10 mM Tris-Cl, pH 7.5, before theirmating. Ten to twelve hours after initiation of conjugation, thepaired cells were bombarded with the disruption plasmids coatedonto 1-µm gold particles (~3 mg of DNA per 1 g of particles) usingthe PDS-1000/He Biolistic Particle Delivery System particle gun(Bio-Rad, Richmond, CA). After bombardment, the cells were recoveredfor 3 h in Neff medium (0.25% proteose peptone, 0.25% yeast extract,0.5% dextrose, 0.03 mM FeCl₃) and then plated into Neff mediumsupplemented with paromomycin at 0.1 mg/ml. Transformants wereidentified after 3 d and then replated in progressively higherconcentrations of paromomycin. Chemicals were purchased from Sigma(St. Louis,MO).

Evaluation of the Phenotypes by Microscopy

Phagocytosis. Living cells were fed 2.16-µm fluorescent carboxylated polystyrene beads (Sigma, St. Louis, MO) by the use of the method describedby Batz and Wunderlich (1976). After 1 h of incubation with thebeads, the cells were washed, fixed in formaldehyde, and visualizedby confocal fluorescencemicroscopy.

4',6-Diamidino-2-phenylindole (DAPI) Staining. Cells were fixed in 3.7% formaldehyde and stained with DAPI. The DAPI-stained cells were examined and photographed with anepi-illumination fluorescence microscope using a 50-W Hglamp.

Indirect Immunofluorescence Microscopy. Cells were permeabilized and fixed in microtubule-stabilizing buffer (Cole and Stuart, 1999). To visualize the mitotic apparatuses,we double-stained the cells with mouse monoclonal anti-tubulinantibodies (Asai et al., 1982) and with rabbit anti-phosphorylatedhistone antibody (Upstate Biotechnology, Lake Placid, NY), whichstains only condensed chromatin (Lu et al., 1994). To visualizethe surface cilia, we stained the cells with monoclonal anti-tubulinantibodies. The antibody-stained cells were viewed by confocallaser fluorescence microscopy using a Bio-Rad MRC1024 instrumentequipped with a Kr/Arlaser.

Surface Areas. Cells were fixed in 2.5% glutaraldehyde in 100 mM NaCacodylate, pH 7.3. The cells were photographed using differential interferencecontrast optics, and the images were captured using a Dage (MichiganCity, IN) Nuvicon camera and Scion (Frederick, MD) frame-grabber.Measurements were made using the particle analysis program inNational Institutes of Health Image 1.61 (http://rsb.info.nih.gov/nih-image/).

Scanning Electron Microscopy. Cells were fixed in 2.5% glutaraldehyde and 1% OsO₄ in 100 mM NaCacodylate, pH 7.3, for 10 min, washed in water, stained with1% uranyl acetate for 1 h, and critical pointdried.

Reciliation Experiments Cells were deciliated by a modification of standard methods (Rosenbaum and Carlson, 1969). Exponentially growing culturesof cells were harvested by centrifugation (1000 × g, 2 min, roomtemperature) in oil tubes. The cell pellet was resuspended intwo volumes of ice-cold buffer A (10 mM EDTA, 50 mM sodium acetate,pH 6.0) and transferred to a sterile 50-ml tube containing 10ml of ice-cold sterile water and 0.5 ml of 0.2 M CaCl₂. The cellsuspension was gently agitated by end-over-end mixing for 45 s.The deciliated cells were then transferred to 600 ml of freshNeff medium and allowed to reciliate. In a Northern blot experiment(see Figure 2), the cells were allowed to reciliate for 2 h andthen deciliated again. Total RNA was isolated from the cells after45 min of recovery from the second deciliation. Total RNA wasalso isolated from mock-deciliated cells that were subjected tothe same treatments except that the calcium was omitted from thedeciliation steps. The deciliation and reciliation of the cellswere confirmed by observing the cells by bright-fieldmicroscopy.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Characterization of Tetrahymena DYH1 and DYH2

Short fragments of several Tetrahymena dynein heavy chain genes were obtained by the RT-PCR method using degenerate oligonucleotideprimers that correspond to conserved sequences. Comparison ofthese sequences with those of dynein isoforms from other organismsidentified the Tetrahymena genes encoding Dyh1 and Dyh2. The RT-PCRfragments were used to screen a Tetrahymena macronuclear genomiclibrary that yielded single lambda clones containing large portionsof DYH1 and DYH2. The DYH1 clone is ~17 kb in length, begins nearthe 5' end of the coding region, and extends past the 3' end ofthe gene. The DYH2 clone is ~15 kb in length, includes the 5'end of the coding region, but lacks 3-4 kb of the 3' end of thegene. The lambda inserts were mapped with restriction enzymes,and the central motor domains, which include the four P-loops,were sequenced. These sequences have been deposited in the database(GenBank accession numbers AF025312 and AF025313). To identifyunambiguously the open-reading frames, we sequenced overlappingcDNAs obtained by RNA-directed PCR. The comparisons between thegenomic sequences and the cDNA sequences identified several intronsin the central regions encoding the catalytic domains of bothdynein genes (see GenBank deposits). DYH1 has 10 introns of 50-64nucleotides (average length, 56); DYH2 has 12 introns of 50-108nucleotides (average length, 75). The intron-exon organizationsof the two genes aredistinct.

There are three organisms from which substantial sequence information for both Dyh1 and Dyh2 has been determined: sea urchin(Gibbons et al., 1992, 1994), nematode (Wilson et al., 1994; Lyeet al., 1995), and Tetrahymena. The aligned catalytic domain sequencesof the six dyneins are shown in Figure 1. An asterisk marks aposition at which there is a conserved amino acid in the threeDyh1 sequences and a different conserved amino acid in the threeDyh2 sequences. The three Dyh1 sequences are more similar to oneanother than to any Dyh2 sequence, and the three Dyh2 sequencesare more similar to one another than to any Dyh1 sequence.

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Figure 1. Alignment of catalytic domain sequences of Dyh1 and Dyh2. The deduced amino acid sequences of Dyh1 and Dyh2 from Tripneustes gratilla (SU-1 and SU-2; accession numbers Z21941 and U03969), C. elegans (Ce-1 and Ce-2; accession numbers L33260 and Z75536), and Tetrahymena thermophila (Tt-1 and Tt-2; accession numbers AF025312 and AF025313) were aligned by the PILEUP program (GCG, University of Wisconsin). The four P-loops are identified. Each position (*) at which there is a conserved residue in the three Dyh1 sequences that is different from a conserved residue in the three Dyh2 sequences is identified.

Similar to what was found in sea urchin embryos (Gibbons et al., 1994) and rat tracheal epithelial cells (Criswell et al.,1996), DYH2 expression increased during ciliogenesis in Tetrahymena.Total RNA was obtained from mock- and twice-deciliated wild-type(B2086) cells. Northern blots revealed that the steady-state concentrationof DYH2 RNA, but not of DYH1 RNA, was increased in response todeciliation. The results of one such experiment are shown in Figure2. To circumvent potential variations caused by uneven loadingof the gel, we repeatedly probed and stripped the same blot. Asa positive control, the blot was also probed with a cDNA fragmentof ciliary dynein $beta$ heavy chain (the DYH4 gene). Deciliation interruptsthe growth of the cells, and a gene whose expression is reliablyunaltered is unavailable. Thus, this experiment provides a comparisonof the changes after deciliation in DYH1 and DYH2 expression butdoes not measure absolute levels of expression.

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Figure 2. Stimulation of DYH2 in response to deciliation. Total RNA was isolated from mock- and twice-deciliated wild-type cells. (a) The Northern blots were repeatedly probed, exposed to x-ray film, stripped, and then reprobed to obtain the data shown. The autoradiography signals were measured by densitometry. (b) The relative densities are plotted. The steady-state concentration of DYH2 RNA, but not that of DYH1, increased during reciliation. The positive control in this experiment was ciliary dynein $beta$ heavy chain DYH4 (accession number AF072878) that also increased in expression in response to deciliation.

KO-1 and KO-2 Are Targeted Knockouts of DYH1 and DYH2

The two cytoplasmic dynein genes were separately disrupted by inserting the neomycin-resistance gene into the coding region,which resulted in two gene knockout cell lines referred to asKO-1 and KO-2 (see Figure 3, a and b). Southern blots using dynein-specificprobes showed the loss of the appropriately sized fragment inthe KO cell lines, and the neo probe, which hybridized with onlya single band in each case, demonstrated that the neomycin-resistancegene was inserted only in the targeted genes (Figure 3, c andd). Northern blots showed the decreased expression of the targetedgene, but not of the untargeted gene, in each transformed cellline (Figure 3e). On the basis of the Southern and Northern analyses,the wild-type version of DYH2 appeared to be completely eliminatedin the KO-2 transformants. However, the wild-type version of DYH1could not be completely eliminated in the KO-1 transformants evenafter prolonged selection in paromomycin; thus, KO-1 is an incompleteknockout. Culturing the KO-1 cells without paromomycin for 3 dresulted in an increase in the copy number of the wild-type versionof DYH1 (Figure 3f). Therefore, it was possible to modulate thelevel of DYH1 by adjusting the selection pressure, and this modulationwas exploited in the following experiments.

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Figure 3. Targeted disruptions of DYH1 and DYH2. (a and b) Diagrams of portions of the macronuclear wild-type (WT) genes (top) and the disruption constructs (bottom) for DYH1 (a) and DYH2 (b). The DYH1 disruption construct was made by inserting the neomycin-resistance gene at the chromosomal KpnI site. The DYH2 disruption construct was made by deleting the EcoRV-EcoRV fragment and replacing it with the neomycin-resistance gene. In each diagram, the positions of the genes encoding the P-loops (P1-P4) are indicated. The locations of the gene-specific probes used in the Southern and Northern blots are underlined. (c and d) Southern blots demonstrating the targeted disruptions of the DYH1 (c) and DYH2 (d) genes. In each panel, the blot on the left was probed with the gene-specific probe and showed the loss of the appropriately sized hybridizing fragment in the KO cell lines. The blots on the right of each panel were probed with the coding region of the neomycin-resistance gene and showed that the neo gene was inserted in the appropriate locations. In each case, the neo probe hybridized with a single band. (e) Northern blots of total RNAs obtained from wild-type (B2086), KO-2, and KO-1 cells. The ~14.5-kb dynein heavy chain bands and the 1.4-kb neo bands were identified with gene-specific probes. The disruption of each dynein gene affected the expression of only the targeted gene. (f) Southern blots of DNAs from wild-type (B2086) and KO-1 cells probed with neo and DYH1. Genomic DNA digested with BglII was probed in this experiment. The paromomycin-selected KO-1 cells (lane labeled KO-1) possessed a large amount of the neo gene and very little of the wild-type version of DYH1. After growth for 3 d in the absence of paromomycin, the cells (lane labeled KO-1 rescued) possessed a high copy number of wild-type DYH1 and only a small amount of the neomycin-resistance gene. This experiment demonstrates that the KO-1 cells were incomplete knockouts of the DYH1 gene and that the copy number of the DYH1 gene could be manipulated by changing the selection pressure.

Dyh1, but Not Dyh2, Is Required for Phagocytic Activity in Tetrahymena

Normal feeding behavior in Tetrahymena begins at the oral apparatus where food particles are phagocytosed. The engulfed materialis then transported along the length of the cell, and the unusedmaterial is eventually expelled at the cytoproct located at theposterior end. This process requires ~2 h and can be easily visualizedby feeding the cells ~2-µm fluorescent latex beads (Batz and Wunderlich,1976). Using fluorescent beads, we performed a simple phagocytosisassay, and the results are shown in Figure 4. Cells were allowedto "feed" on the beads for 1 h and then washed, fixed, and counterstainedwith the nonspecific membrane dye 1,1'-dioctadecyl-3,3,3',3'-tetramethyloxycarbocyanineperchlorate (DiOC6, Sigma). The cells were then examined by confocalfluorescence microscopy. The KO-1 cells, but not the KO-2 cells,were mostly unable to take up the beads. The defect in phagocytosisexhibited by the KO-1 cells could be reversed by first growingthe KO-1 cells for 3 d in no paromomycin, a treatment that restoresthe wild-type copy number of the DYH1 gene (see Figure 3f, above).The inability of the drug-selected KO-1 cells to undergo phagocytosiswas not simply a side effect of the paromomycin because the KO-2cells, which continued to phagocytose the beads, were grown inthe same drug concentration as were the KO-1 cells (paromomycinat 10 mg/ml). Thus, Dyh1 is required for normal phagocytosis activity.

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Figure 4. Dyh1 is required for phagocytosis. Cells were incubated for 1 h with fluorescent latex beads, washed, fixed with formaldehyde, and counterstained with DiOC6. In these confocal fluorescence micrographs, the beads are red, and the membranes stained with DiOC6 are green. The KO-1 cells were unable to phagocytose the beads. However, KO-1 cells grown for 3 d in the absence of paromomycin (KO-1 rescued) possessed phagocytic activity. All photographs are at the same magnification (bar, in micrometers, in lower left corner of KO-2). Note the larger size of the KO-2 cells.

Dyh1, but Not Dyh2, Is Required for Chromosome Segregation during Micronuclear Mitosis

Cultures of vegetatively growing cells were fixed and stained with DAPI to assess their nuclear phenotypes. When the KO-1cells were grown in the presence of a high concentration of drug(paromomycin at 10 mg/ml), many of the cells lacked a distinctmicronucleus (Figure 5a). It is possible that these cells retaineda fragment of the micronucleus, which was obscured by the brightlystained macronucleus. In contrast, the KO-2 cells grown underthe same selection conditions possessed a normal-appearing micronucleus,thus demonstrating that the micronuclear effect in the KO-1 cellswas not a side effect of the paromomycin treatment. The relationshipbetween DYH1 and the micronuclear phenotype was further exploredby culturing the cells in different concentrations of paromomycin,staining the cells with DAPI, and scoring the cells for the presenceof a distinct micronucleus (Figure 5b). In this experiment, sampleswere coded and then scored (n > 200 for each treatment) by a studentwho did not know the code. Increasing the paromomycin concentrationresulted in a reduction in the proportion of KO-1 cells with adistinct micronucleus. In contrast, the same treatments had noeffect on the presence or appearance of the micronuclei in KO-2cells. Wild-type cells are sensitive to paromomycin and so wouldnot be a particularly meaningful control in this experiment. However,wild-type cells grown with no drug, fixed, and stained with DAPIrevealed numbers of micronuclei per cell similar to what was foundwith KO-2 cells. Because the copy number of the wild-type versionof DYH1 could be manipulated by adjusting the drug concentration(see Figure 3f), this result demonstrates that Dyh1 is requiredfor the maintenance of a normal micronucleus during vegetativegrowth.

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Figure 5. Many KO-1 cells lack a distinct micronucleus. (a) Fields of cells stained with DAPI and viewed by fluorescence microscopy. Most of the wild-type (B2086) and KO-2 cells contained a micronucleus (examples indicated with arrows), but most of the KO-1 cells did not. The KO-1 and KO-2 cells were grown for several weeks in paromomycin at 10 mg/ml before this experiment. (b) Effects of paromomycin concentration on the number of visible micronuclei per cell in KO-1 and KO-2. Cells were grown in paromomycin at 10 mg/ml and then transferred to medium containing different concentrations of the drug (0-10 mg/ml). After 3 d of vegetative growth, the cells were fixed and stained with DAPI. Approximately 200 cells at each drug concentration were viewed by fluorescence microscopy in a blind protocol. The number of distinct micronuclei in the KO-1 cells was affected by the paromomycin. At high concentrations of the drug, most of the KO-1 cells lacked a visible micronucleus, whereas in the absence of drug, most of the KO-1 cells had one micronucleus. The different paromomycin concentrations did not affect the micronuclear phenotype of the KO-2 cells, demonstrating that the effect in the KO-1 cells was not simply attributable to the drug. The KO-2 cells with two micronuclei included dividing cells in these nonsynchronized cultures.

The apparent loss of the micronucleus in KO-1 cells during vegetative growth suggested that these cells were defective insome aspect of micronuclear mitosis. Normal cell division in Tetrahymenaoccurs in three discrete steps and is illustrated in Figure 6,top: 1) The condensed micronuclear chromosomes undergo an earlyanaphase A in which the two sets of daughter chromosomes are drawnto opposite ends of the micronucleus, 2) this is followed by anextensive anaphase B in which the two sets of chromosomes areseparated ~30 µm, and 3) after anaphase B, the cell undergoescytokinesis that results in one daughter micronucleus in eachcell and the pinching apart of the (amitotic) macronucleus.

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Figure 6. Dyh1 is required for normal micronuclear chromosome distribution during mitosis. Wild-type and KO-1 cells were fixed with formaldehyde, stained with DAPI, and viewed by fluorescence microscopy. To capture KO-1 cells with micronuclei, we grew the cells for 3 d in the absence of paromomycin, returned the cells to drug at 10 mg/ml for 1 d, and then fixed and stained the cells. A gallery of cells is shown in this figure; in each photograph, the dividing micronucleus is at the viewer's left. Top, wild-type micronuclear mitosis. Bottom, KO-1 micronuclear mitosis. In the wild-type cells, the two sets of chromosomes separated very early in mitosis. In the KO-1 cells, the chromosomes never segregated to opposite poles. Instead, chromosomal DNA was spread through the micronucleus as mitosis proceeded. This resulted in one or more thread-like DAPI-stained structures.

To determine how the micronuclei were lost in KO-1 cells, we grew the cells for 3 d in the absence of selection drug to restoreto the culture a significant number of cells with micronucleiand then returned the cells to paromomycin at 10 mg/ml and grewthem for another day in the drug to deplete them of wild-typeDYH1 gene. The cells were then fixed and stained with DAPI. Mostof the KO-1 cells examined lacked distinctly stained micronuclei.However, the few KO-1 cells with a micronucleus and fixed duringcell division displayed an aberrant micronuclear mitosis. In contrastto what was observed in wild-type cells, the KO-1 cells failedto segregate their chromosomes to opposite poles (Figure 6, bottom).Instead, the condensed chromosomes appeared to fill the lengthof the micronucleus, resulting in thread-like DAPI-stained materialas the micronuclei elongated. Occasionally more than one thread-likemicronucleus was observed in the same cell, suggesting that thecell had more than one micronucleus (or more than one micronuclearfragment). Wild-type cells also were occasionallymultimicronucleated.

To confirm the continued presence of spindle microtubules in the dividing KO-1 cells, we fixed and double-stained the cellswith monoclonal mouse anti-tubulin antibodies and rabbit anti-phosphorylatedhistone antibody that reacts only with condensed chromatin (Luet al., 1994). The micronuclei of the dividing KO-1 cells possessedwhat appeared to be normal spindles except that the chromosomeswere intertwined with the microtubules throughout the micronucleusinstead of being segregated at the poles (Figure 7).

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Figure 7. Double immunofluorescence microscopy of micronuclear mitotic apparatuses. Cells were permeabilized, fixed, and stained with anti-tubulin and anti-phosphorylated histone antibodies. The cells were viewed by confocal scanning laser fluorescence microscopy. The microtubules are green, the chromatin is red, and yellow is the superposition of the two stains. Top, wild-type micronuclear mitosis. Bottom, KO-1 micronuclear mitosis. Bar, 10 µm.

Dyh2 Contributes to the Maintenance of the Cortical Cytoskeleton

In contrast to the KO-1 cells, the KO-2 transformants underwent normal phagocytosis and micronuclear mitosis. However, theKO-2 cells were often aberrant in size and shape. Unlike wild-typeand KO-1 cells, the KO-2 cells varied widely in size, and manyof the KO-2 cells were significantly larger than the wild-typeand KO-1 cells (Figure 8). Scanning electron microscopy revealedthat many of the KO-2 cells were misshapen (Figure 9).

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Figure 8. Dyh2 contributes to cell size. Surface areas of wild-type (B2086), KO-1, and KO-2 cells were measured from cells photographed using differential interference contrast microscopy. The distributions by surface area for each cell type are shown in the graphs. The KO-2 cells were found to have a wide range of sizes, with many cells being significantly larger than wild-type and KO-1 cells. The slightly smaller size of the KO-1 cells relative to wild-type cells may be related to the involvement of Dyh1 in phagocytosis.

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Figure 9. Dyh2 contributes to cell shape. A gallery of KO-1 and KO-2 cells viewed by scanning electron microscopy are shown. Many KO-2 cells were misshapen. Bars, 6 µm.

The abnormal shapes of many of the KO-2 cells suggested possible defects in the integrity of the cortical cytoskeleton. Becausethe cortical cytoskeleton is responsible for the positioning ofthe ciliary basal bodies, we reasoned that the pattern of surfacecilia would reflect the organization of the underlying corticalmicrotubules. Wild-type, KO-1, and KO-2 cells were deciliatedwith a calcium shock and then returned to fresh media and allowedto reciliate. All three cell lines regrew cilia at approximatelythe same rate. However, unlike the normal pattern of cilia onthe wild-type and KO-1 cells, the cilia on the KO-2 cells oftenemerged randomly and not in the normal rows (Figure 10). This resultsuggests that the KO-2 cortical microtubules were disrupted duringthe calcium deciliation step and did not reform correctly duringthe time course of this experiment.

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Figure 10. Disruption of surface ciliary pattern in reciliated KO-2 cells. Wild-type (B2086), KO-1, and KO-2 cells were deciliated with calcium and then returned to Neff medium. At the indicated times after deciliation, the cells were fixed and stained with anti-tubulin antibodies and then viewed by confocal laser scanning fluorescence microscopy. The wild-type and KO-1 cells regrew their cilia in rows corresponding to the longitudinal cortical microtubules. In contrast, the KO-2 cells regrew their cilia in a disorganized manner.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

In this study, we have taken advantage of the nuclear dimorphism and targeted replacement of somatic genes in Tetrahymenathermophila to dissect the roles of two cytoplasmic dyneins inthe same cell. The disruption of DYH1 resulted in a loss of phagocyticactivity and a mitotic defect in which the chromosomes failedto segregate during anaphase A. In contrast, the disruption ofDYH2 affected the ability of the cell to maintain the corticalmicrotubule cytoskeleton. We conclude that the two dyneins performdistinct functions in Tetrahymena.

Heretofore, most of the genetics of cytoplasmic dynein has focused on the ubiquitous cytoplasmic Dyh1. In organisms with onlyone dynein gene, including budding yeast and filamentous fungi,disruption of Dyh1 produces defects in mitotic spindle positioningand postmitotic nuclear movements, but the cells remain viable(Eshel et al., 1993; Li et al., 1993; Plamann et al., 1994; Xianget al., 1994; Inoue et al., 1998). In contrast, in organisms withmultiple dyneins-Drosophila (Gepner et al., 1996), mouse (Haradaet al., 1998), and now Tetrahymena-Dyh1 appears to be requiredfor normalgrowth.

Dyh1 and Phagocytosis

Our finding that KO-1 cells were defective in the phagocytosis of fluorescent beads is consistent with previous results obtainedin other systems in which cytoplasmic dynein has been implicatedin the retrograde trafficking of membrane-bounded organelles andvesicles (e.g., Schroer et al., 1989; Oda et al., 1995; Muresanet al., 1996). If the KO-1 cells were able to complete phagocytosisbut were then blocked in the subsequent transport of the vesiclesto the cytoproct, we would expect to find an accumulation of fluorescentbeads at the anterior end of the cells, but this was not observed.Thus, our results demonstrate a requirement for Dyh1 in the engulfmentof the beads but do not reveal whether dynein is also involvedin vesicle transport. Because Tetrahymena can take up nutrientsby alternate mechanisms (Rasmussen and Orias, 1975), it is notclear whether the effect on phagocytosis is the reason DYH1 isapparently an essential gene. The lack of phagocytic activitywas not simply caused by a loss of the oral apparatus, which canoccur when the micronucleus is completely eliminated (Haremakiet al., 1996), because anti-tubulin immunofluorescence microscopyrevealed the presence of an oral apparatus in the KO-1 and KO-2cells.

Dyh1 and Chromosome Distribution

During micronuclear anaphase A in wild-type cells, the two sets of chromosomes are drawn to opposite ends of the micronucleusby kinetochore microtubules (LaFountain and Davidson, 1979, 1980).After chromosome segregation, the micronucleus travels from thecenter of the cell to near the cortex where it undergoes a dramaticelongation, growing from a length of 1-2 µm to >30 µm. Micronuclearelongation is driven by the extension and rearrangement of theintranuclear spindle microtubules that are located between thetwo sets of chromosomes and by the stretching of the micronucleussurface along longitudinally oriented cortical microtubules (Jaeckel-Williams,1978). In our experiments, the disruption of DYH1 blocked chromosomedistribution but did not affect micronuclear elongation, and thedisruption of DYH2 had no discernible effect on any aspect ofmitosis. Thus, in Tetrahymena, dynein appears not to be involvedin the migration of the dividing micronucleus from the centerof the cell to near the surface, in the extension of the mitoticspindle, or in the stretching of the micronucleus along corticalmicrotubules.

In the dividing KO-1 cells, the micronuclear chromosomes failed to segregate, implying that Dyh1 is required for the effectiveattachment of the chromosomes to the kinetochore microtubulesor for normal chromosome movement to the opposite poles afterkinetochore attachment. Experiments in other organisms have shownthat dynein activity is associated with the kinetochore (Pfarret al., 1990; Rieder and Alexander, 1990; Steuer et al., 1990;Echeverri et al., 1996). We are currently developing reagentswith which to visualize the Dyh1 protein in Tetrahymena cells;the location of dynein relative to the mitotic apparatus willbe important in understanding the mechanism by which Dyh1 participatesin anaphaseA.

Because the micronuclear genome is not transcribed, the inaccurate segregation of chromosomes during micronuclear mitosiswould not be expected to affect the phenotype of the daughtercells, and micronuclear aneuploidy would be detected only aftermating when a new macronucleus is formed. Such a cell might beanalogous to nullisomic or "star" strains that lack substantialportions of the micronuclear genome (Bruns et al., 1983). However,in experiments in which the entire micronucleus is eliminatedat one time, the progeny do not survive (Haremaki et al., 1996).Thus, a culture of KO-1 cells is likely to be unstable becausethe micronuclei are randomly fragmented at every cell division;if too much of the micronucleus is lost, then the cell may notsurvive. The KO-1 cells illustrate the potential of Tetrahymenaas a model system with which to dissect mitotic mechanisms: 1)anaphase A and B are temporally well resolved, 2) mutations canbe generated by targeted gene disruptions, and 3) mutations affectingmitosis do not immediately affect the viability of thecell.

Dyh2 and the Maintenance of the Cytoskeleton

The disruption of DYH2 produced an intriguing phenotype, quite distinct from the effects of disrupting DYH1. The KO-2 cellswere defective in the maintenance of their cortical cytoskeletons.This apparent loss of regulation led to wide variations in cellsize and shape. One interpretation of these results is that Dyh2participates in the repair and remodeling of the Tetrahymena cytoskeleton,which must be reformed at each cell division (every 2.5 h at 30°C).The putative repair function of Dyh2 was most evident in the reciliationexperiment. The cells were deciliated with a brief exposure toa high concentration of calcium ion, a treatment that disruptedthe cortical microtubules that arrange the ciliary basal bodiesor kinetids. The pattern of reciliation revealed that the underlyingcytoskeleton remained disorganized in the KO-2 cells. An importantfuture problem will be to determine what cargoes Dyh2 carriesto perform this task. The result in Tetrahymena is reminiscentof findings in Dictyostelium discoideum and Saccharomyces cerevisiaein which overexpression of the dynein globular head domain affectedthe microtubule cytoskeleton and cell polarity (Koonce and Samso,1996; Shaw et al., 1997). Slime mold and yeast have only one dynein,Dyh1, whereas Tetrahymena uses a separate dynein, Dyh2, to organizethe cytoskeleton, thus underscoring the division of labor achievedwith multiple dyneinisoforms.

In nonciliated fibroblasts, Dyh2 was shown to participate in the organization of the Golgi apparatus (Vaisberg et al., 1996).In Tetrahymena thermophila, the Golgi apparatus is located atand organized by the cortical cytoskeleton (Kurz and Tiedtke,1993). If Dyh2 is important in maintaining the cortical cytoskeleton,then the absence of Dyh2 might have an indirect effect on Golgifunction. However, we have observed no noticeable defect in regulatedexocytosis (Chilcoat et al., 1996) in the KO-2cells.

In sea urchin embryos, rat tracheal epithelial cells, and Tetrahymena, the steady-state concentration of transcripts encodingDyh2 increased during cilia formation. This implies that Dyh2is either a component of the cilia or is involved in ciliogenesis,perhaps carrying ciliary precursors to the site of their incorporation.We therefore expected that the elimination of DYH2 expressionwould have an effect on cilia formation in Tetrahymena. However,the KO-2 cells were able to regenerate their cilia with approximatelynormal kinetics, and no gross abnormality in the KO-2 ciliaryaxonemes was detected by electron microscopic analysis. This resultis particularly intriguing because of the recent reports thatdisruption of the gene encoding Dyh2 in Chlamydomonas resultsin abnormal flagella (Pazour et al., 1999; Porter et al., 1999).If Dyh2 is used for cytoskeletal remodeling as we suggest, itsimpact may be observed in different places depending on the organism.In Tetrahymena, most of the cilia are terminal organelles thatdo not shorten or elongate, and remodeling occurs mostly in thecortical cytoskeleton. However, in Chlamydomonas, remodeling occursin the flagella, which must be able to change in length constantlyin response to environmental cues and for cell division (see Tuxhornet al., 1998).

Complexity of Dynein Functions: Genes and Environment

The techniques of modern molecular biology have provided the means to identify rapidly the dynein heavy chain genes in severalmodel organisms. Although we do not yet have a complete understandingof the structure-function relationships of dynein heavy chainsin organisms with multiple dyneins, it is reasonable to expectthat there is functional specialization among the dynein isoforms,as has been documented for the kinesin family of microtubule motors(reviewed in Cole and Scholey, 1995; Vale and Fletterick, 1997).The genetic dissection of the several axonemal dyneins demonstratestheir individual specializations (reviewed in Piperno, 1990; Asaiand Brokaw, 1993; Brokaw, 1994), and isoform-specific antibodiessuggest separate tasks for three different cytoplasmic dyneinsin vertebrate cells (Vaisberg et al., 1996). The present studyextends this idea by providing a clear example of the divisionof labor between two cytoplasmic dyneins within the samecell.

Although there is specialization among dynein isoforms within a single cell, it is appropriate to consider cellular contextas a second important element in the determination of dynein function.A particular dynein isoform may do different things in differentcontexts. For example, Dyh2 appears to perform distinct tasksin unciliated fibroblasts versus ciliated epithelial cells andin Tetrahymena versus Chlamydomonas. Another striking exampleis the apparent involvement of dynein $beta$ heavy chain in the establishmentof visceral handedness at a time when the embryonic cells maynot be ciliated (Supp et al., 1997). The contextual regulationof dynein function suggests that it is not simply the heavy chainisoform sequence that determines function. Rather, what a dyneindoes in a particular cell may also be controlled by other factors,including interaction with specific dynein subunits and dyneinaccessory proteins, and by posttranslational modifications ofdyneinsubunits.

	ACKNOWLEDGMENTS

We are grateful for the helpful advice of many persons, including Kerry Bloom, Peter Bruns, Jim Forney, Joe Frankel, MartyGorovsky, Mike Koonce, Mary Porter, Conly Rieder, Aaron Turkewitz,and Norm Williams. David Wilkes and Jifan Chen began the TetrahymenaRNA-directed PCR analysis, Dana Ahn helped with the experimentsummarized in Figure 5, and Sunkyung Lee contributed to the resultsshown in Figure 10. This work was supported by research grantsfrom the National Institutes of Health (to W.L.D.) and the AmericanCancer Society and National Science Foundation (to D.J.A.).

	FOOTNOTES

Corresponding author. E-mail address: dasai{at}bilbo.bio.purdue.edu.

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DISCUSSION
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