Basal Body Duplication and Maintenance Require One Member of the Tetrahymena thermophila Centrin Gene Family

Alexander J. Stemm-Wolf^*, Garry Morgan^*, Thomas H. Giddings, Jr.^*, Erin A. White^*, Robb Marchione, Heather B. McDonald^||, and Mark Winey^*

^* Department of Molecular, Cellular, and Developmental Biology, University of Colorado–Boulder, Boulder, CO 80309; Department of Biology, Colgate University, Hamilton, NY 13346

Submitted October 22, 2004; Revised April 27, 2005; Accepted May 31, 2005
Monitoring Editor: Joseph Gall

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Centrins, small calcium binding EF-hand proteins, function inthe duplication of a variety of microtubule organizing centers.These include centrioles in humans, basal bodies in green algae,and spindle pole bodies in yeast. The ciliate Tetrahymena thermophilacontains at least four centrin genes as determined by sequencehomology, and these have distinct localization and expressionpatterns. CEN1's role at the basal body was examined more closely.The Cen1 protein localizes primarily to two locations: one isthe site at the base of the basal body where duplication isinitiated. The other is the transition zone between the basalbody and axoneme. CEN1 is an essential gene, the deletion ofwhich results in the loss of basal bodies, which is likely dueto defects in both basal body duplication and basal body maintenance.Analysis of the three other centrins indicates that two of themfunction at microtubule-rich structures unique to ciliates,whereas the fourth is not expressed under conditions examinedin this study, although when artificially expressed it localizesto basal bodies. This study provides evidence that in additionto its previously known function in the duplication of basalbodies, centrin is also important for the integrity of theseorganelles.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Centrins, also called caltractins, are widely conserved membersof the EF-hand superfamily of calcium-binding proteins (Salisbury,1995). Although sharing $~$ 50% identity with the ubiquitous calciumsensor calmodulin, centrins perform distinct functions withinthe eukaryotic cell. In particular, centrins have a varietyof roles at microtubule organizing centers (MTOCs) and microtubule-basedstructures (Salisbury, 1995; Vaughn and Harper, 1998; Chapmanet al., 2000). Additionally, centrins are constituents of calcium-responsivecontractile fibers found in many protists (Salisbury et al.,1984; Wright et al., 1985).

One of the widely recognized roles for centrin is in the duplicationof microtubule organizing centers, including centrosomes, basalbodies, and the yeast spindle pole body (Baum et al., 1986;Salisbury et al., 2002; Koblenz et al., 2003). Centrosomes consistof two orthogonally oriented centrioles surrounded by amorphouspericentriolar material from which spindle and astral microtubulesare organized. Centrioles are distinguished by 9-fold symmetryof microtubules in a "flower" arrangement, with the majorityof metazoans displaying triplet microtubules at these positions.Basal bodies are structurally similar to centrioles and differprimarily in the manner in which they organize microtubules.Cilia and flagella, which consist of nine doublet microtubulessurrounding a central microtubule pair, are nucleated from thedistal end of the basal body (reviewed in Beisson and Wright,2003). In some situations, it is the identical organelle thatacts as a centriole and then is converted to a basal body, orvice versa, at particular points in the life cycle of the cell.This is the case in many vertebrate cells where the oldest centrioleis capable of forming a single "9 + 0" cilium (known as theprimary cilium) that is assembled during the G₁ phase of thecell cycle and disassembled during mitosis (Jensen et al., 1987).The budding yeast spindle pole body is structurally distinctfrom the centriole and basal body. This trilaminar structureremains embedded within the nuclear envelope throughout thecell cycle. Spindle and astral microtubules emanate from theinner and outer plaques, respectively. Although dissimilar inappearance to the centrosome, the spindle pole body performsthe same task of organizing mitotic and meiotic spindles, andsome components of these organelles, including centrin, areconserved between these divergent organelles (Adams and Kilmartin,2000).

Temperature-sensitive mutations in the yeast centrin gene CDC31result in failure in an early step of spindle pole body duplicationand a cell cycle arrest in G₂/M phase, such that cells arrestwith a single, enlarged spindle pole body (SPB) (Byers, 1981;Baum et al., 1986). Like SPB duplication, basal body and centrioleduplication is dependent on centrin function, as demonstratedby RNA interference (RNAi) experiments in both human cells andChlamydomonas. Thus far, three centrin genes have been clonedfrom human cells (Lee and Huang, 1993; Errabolu et al., 1994;Middendorp et al., 1997). When human centrin2 levels are reducedby RNAi, cells exhibit defects in centriole duplication (Salisburyet al., 2002). The same is true when levels of the Chlamydomonascentrin (Vfl2) are decreased to 5% of the normal level. In thesecells, the number of basal bodies is reduced to $~$ 0.3 per cellfrom the normal condition of two per cell, indicating a failurein basal body duplication (Koblenz et al., 2003). Defects alsowere observed in the structure of remaining basal bodies, indicatinga possible role for centrin in basal body maturation or stability.

In addition to its essential role in MTOC duplication, centrinis involved in other cellular processes. In yeast, Cdc31 isrequired for Kic1 kinase activity that is important for propercell wall development (Sullivan et al., 1998). Cdc31 also isinvolved in mRNA export at the nuclear pore complex (Fischeret al., 2004). The contractile properties of centrin are importantin a number of structures, including the nucleus-basal bodyconnector and stellate fibers associated with Chlamydomonasbasal bodies (Sanders and Salisbury, 1989; Taillon et al., 1992;Sanders and Salisbury, 1994), and the infraciliary lattice,a contractile cortical network in Paramecium (Madeddu et al.,1996; Klotz et al., 1997). Centrin also has been associatedwith the inner dynein arm important for axonemal beating (LeDizetand Piperno, 1995; Guerra et al., 2003).

In some organisms, such as yeast and Chlamydomonas, the productof a single centrin gene carries out multiple functions. However,other species have multiple centrin genes that may encode productsthat are specialized to carry out different tasks or to carryout similar tasks at different stages of the life cycle. Inhumans, centrin1 expression is confined to the testes and retinalcells, whereas centrins 2 and 3 are more ubiquitously expressed(Hart et al., 1999; Laoukili et al., 2000). Strikingly, whena Leishmania centrin gene was deleted, one of the two lifestyleforms of this parasite was unable to duplicate its basal bodiesand was unable to progress through mitosis, whereas the otherwas unaffected, suggesting that a different centrin was activeduring this stage of its life cycle (Selvapandiyan et al., 2004).

Because the ciliate Tetrahymena thermophila has $~$ 750 basal bodiesper cell (Frankel, 2000; Frankel and Nelsen, 2001) and sophisticatedgenetic and molecular biological techniques are available forits study (Bruns and Cassidy-Hanley, 2000a,b; Gaertig and Kapler,2000; Hai et al., 2000), we turned to Tetrahymena to gain insightsinto basal body/centriole duplication. Centrin has been localizedto basal bodies and cilia in Tetrahymena, and a centrin genehas been cloned (Guerra et al., 2003). We independently clonedthis centrin gene, called CEN1, and have begun characterizingit and three other centrins we identified through sequence similarityin the recently sequenced Tetrahymena genome. By using fusionswith the green fluorescent protein (GFP) (Chalfie et al., 1994),we localized Cen1 and the second of the centrins (CEN2) to basalbodies. We created a null mutation in CEN1 and have shown itis required for basal body duplication and stability. Furthermore,we found that the third centrin (CEN3) localizes to specializedstructures in the oral apparatus, a complex network of cilia,and accessory structures that sweeps food into the cell. Thefourth centrin (CEN4) also localizes to these structures inthe oral apparatus as well as to contractile vacuole pores (theopenings for the contractile vacuoles that maintain the properosmolarity of the cells) and to basal bodies (Frankel, 2000).

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Strains, Culture Conditions, and Matings
T. thermophila strains B2086, CU427, and CU428 (all generousgifts from Dr. Peter Bruns, Cornell University, Ithaca, NY)were the starting point for new strain development. Strainswith constructs encoding GFP-Centrin fusion proteins were createdas described below. UCB8 and UCB9 are CEN1 knockout heterokaryons(described below). B*VI (gift from Dr. Aaron Turkewitz, Universityof Chicago, Chicago, IL) was used for star crosses in strainconstruction (Hai et al., 2000). All were grown in SSP (2% proteosepeptone, 0.1% yeast extract, 0.2% glucose, 0.003% FeEDTA) at30°C. Starvation media consisted of 10 mM Tris, pH 7.5 (Oriaset al., 2000). For matings, an equal number of cells of differentmating types, previously starved for 18 h, were mixed (Gaertigand Kapler, 2000).

Gene Identification and Sequence Analysis
To search for centrin genes in Tetrahymena, PCR using degenerateprimers EIK-F and VAK-R, designed to represent regions of highconservation between centrins, was conducted (Supplemental Table1 lists all primers used in this study). Standard molecularbiology techniques were used to isolate a centrin gene, whichwas subsequently reported by Guerra et al. (2003). To searchfor additional centrin genes, preliminary sequence data wereobtained from The Institute for Genomic Research Web site athttp://www.tigr.org. Tetrahymena CEN1 translated sequence wasused to query the Tetrahymena database using the tblastn program.CEN2 was found on sequence #8254664 between positions 498633and 499370, with possible introns spanning 498790–498909,499005–499063, and 499256–499320. CEN3 was foundon sequence #8253915 between positions 239917 and 240426. CEN4was found on sequence #8254437 between positions 298144 and298659. Sequences were compared and analyzed at the PasteurBioweb site (bioweb.pasteur.fr). ClustalW (Thompson et al.,1994) was used to align the sequences, and BOXSHADE (writtenby Hofmann and Baron) was used to create the image of the alignment.Using PHYLIP (Phylogeny Inference Package), protein distanceswere calculated with PROTDIST (Jones–Taylor–Thorntonmatrix), and a tree was constructed using NEIGHBORS followedby DRAWGRAM for image generation. For statistical analysis,1000 replicates were performed and bootstrap values were calculated.(Felsenstein, J. 2004. PHYLIP version 3.6. Distributed by theauthor, Department of Genome Sciences, University of Washington,Seattle, WA)

Plasmid Construction
As a starting point for the creation of a CEN1 knockout plasmid,pHM74 was constructed. A 2.1-kb fragment containing CEN1 wasamplified from genomic Tetrahymena DNA by PCR (Saiki et al.,1988) using primers RM13 and RM14, which were engineered toinclude unique BamHI and SacII sites at their respective 5'ends. This fragment, which begins 1 kb upstream of the CEN1start codon, was cloned into the BamHI and SacII sites of p4T2-1(Gaertig et al., 1994a) downstream of the NEO2 cassette. PrimersRM11 and RM12, which were engineered to contain unique KpnIand XhoI sites at their respective ends, were then used to amplifya 1.6-kb genomic fragment upstream of CEN1. This fragment wascloned into KpnI/XhoI-digested p4T2-1, upstream of the NEO2cassette, to create pHM74. pHM74 was digested with KpnI andBamHI, eliminating the NEO2 cassette and the 1.6-kb CEN1 upstreamregion. A KpnI-BamHI adapter from EZCloneSystems (New Orleans,LA) was used to recircularize the plasmid. This construct wasdigested with EcoRI to remove most of the CENI coding sequence,including the start codon, and blunted. A SmaI, EcoRV fragmentfrom pHM74 containing the NEO2 cassette was inserted into thisplasmid, creating pCentrin:NEO 1. To obtain more sequence downstreamof the CEN1 gene, a library of 3- to 4-kb PstI, EcoRI-digestedgenomic DNA was created in pBluescript KSII^– (Stratagene,La Jolla, CA) and transformed into Escherichia coli for colonylifts. A PCR fragment generated by amplification of pHM74 DNAwith primers RM10 and T7 was used as a probe. Lifts and labelingof the probe were conducted as per instructions for Hybond-N⁺nylon membrane and the AlkPhos direct labeling system (AmershamBiosciences, Piscataway, NJ). A clone was recovered with $~$ 3 kbof sequence downstream of CEN1, and a BglII, SacI fragment wascloned from this into pCentrin:NEO 1 to create pCentrin:NEO1+48.To use all of the upstream sequence available, a PCR fragmentfrom genomic DNA spanning the site where the NEO2 cassette hadbeen inserted in the sequence upstream of CEN1 was amplifiedwith primers NEORemove1 and NEORemove2, digested with BclI andSpeI, and inserted into similarly digested pHM74, creating pHM74-NEORemove.Finally, a BclI, KpnI fragment from this plasmid was ligatedinto similarly digested pCentrin:NEO1+48 to create pMicCentrinKO1.

For the plasmids encoding the GFP-centrin fusions, genomic DNAwas amplified with XhoI and ApaI sites engineered into the primersto allow cloning into similar sites in pVGF-1 (Wiley et al.,2000). Primers were used as follows: for CEN1, primers XhoI-5'Centrinand ApaI-3'Centrin; for CEN2, primers 5'XhoI TtCentrin2 and3'ApaI TtCentrin2; for CEN3, primers 5'XhoI TtCentrin3 and 3'ApaITtCentrin3; and for CEN4, primers 5'XhoI TtCentrin4 and 3'ApaITtCentrin4. Clones were sequenced at Macrogen (Seoul, Korea)to confirm that errors had not been introduced by PCR.

To create a version of CEN1 that could be expressed in E. coli,a PCR fragment containing the coding region of CEN1 was amplifiedfrom a Tetrahymena cDNA library (generous gift from Dr. AaronTurkewitz) using primers 5'BamHI-Centrin and 3'PstI-Centrin,which were engineered to contain the indicated restriction sites.This fragment was cloned into similarly digested pUC18. BecauseTetrahymena uses an alternative genetic code, in which UAA andUAG represent glutamine codons, it was necessary to modify theCEN1 sequence to allow expression in E. coli. Four glutaminecodons were changed to the canonical CAA or CAG codons usingthe U.S.E. site-directed mutagenesis system (Amersham Biosciences,Piscataway, NJ) with the following primers: CentSw1, CentSw2,CentSw3, and TMSelect. The resulting plasmid (pUC18-TtCentrinMFE)was digested with BamHI and PstI, and the CEN1 fragment wasligated into the pQE10 6-His fusion expression vector (QIAGEN,Valencia, CA), creating pQE10-CentrinMFE.

To create the CEN1 rescuing construct, a 1.0-kb BamHI, MfeICEN1 promoter region was excised from pHM74 and cloned intosimilarly digested pUC18-TtCentrinMFE. CEN1, with its promoter,was then excised from this construct with SmaI and SphI, blunted,and ligated into the blunted BsmBI site of grl3/4:BLAST (a constructthat replaces the GRL3 and GRL4 promoter region with the Bsrgene, which provides resistance to Blasticidin S, a generousgift from Aaron Turkewitz). Finally, the CEN1 3' untranslatedregion (UTR) was amplified by PCR of genomic DNA using primersCentrin_BstXI and BsmBI-dsCentrin and ligated into BstXI (partial),BsmBI-digested grl3/4:BLAST-PrCEN1 to create grl3/4:BLAST-PrCEN1–3'UTR.The resulting plasmid was sequenced to ensure no errors hadbeen introduced.

Protein Expression and Antibody Generation
pQE10-CentrinMFE was transformed into the E. coli strain M15,and a culture was grown in 500 ml of Luria Broth + 0.2% glucosewith 50 µg/ml kanamycin and 100 µg/ml ampicillin.At an OD₆₀₀ of 0.4, cells were cooled to room temperature for1 h. Isopropyl ${beta}$ -D-thiogalactoside was added to 0.3 mM and inductionwas allowed to proceed for 2.5 h. Cells were pelleted, washedonce with phosphate-buffered saline (PBS), and stored frozen.Pellets were thawed, and resuspended in 10 ml of PBS containing1 mM phenylmethylsulfonyl fluoride, 0.5 µg/ml leupeptin,1 µg/ml aprotinin, and 1 µg/ml pepstatin A. Lysozymewas added to 200 µg/ml before a 10-min incubation on ice.Cells were sonicated five times for 15 s each with 1-min intervalsof rest on ice and centrifuged 15 min at 10,000 x g at 4°C.The supernatant was loaded onto a column containing Talon resin(BD Biosciences Clontech, Palo Alto, CA) equilibrated in PBS,and fractions were eluted in PBS + 200 mM imidozole. Fractionswith Cen1 were pooled, and 1 mg was sent to Animal Pharm (Healdsburg,CA), for antibody generation in rabbits.

Northern Blot Analysis
RNA was isolated using the TRI Reagent (Molecular Research Center,Cincinnati, OH) as per the manufacturer's instructions. Samples(each containing 10 µg of RNA) were run on formaldehydegels and transferred to Hybond N⁺ (Amersham Biosciences) in20x SSC (Ausubel et al., 1997). Northern blots were probed withrandomly primed [ ${alpha}$ -³²P]dATP-labeled fragments (Feinberg and Vogelstein,1983), which were obtained by amplification by PCR of genomicDNA with the primers used to create the GFP fusions describedabove. Probes were specific for the target sequences as determinedby Southern blot analysis of total DNA (our unpublished data).

Western Blot Analysis
Cells were lysed in buffer as described previously (Williams,2000), and whole cell extracts were run on 12.5% or 11.5% standardLaemmli acrylamide gels (Ausubel et al., 1997) along with BenchMarkprestained molecular weight standards (Invitrogen, Carlsbad,CA). Proteins were electrophoretically transferred to Immobilon-Pmembrane and blotted according to the manufacturer's instructions(Millipore, Billerica, MA). Membranes were incubated with antibodiesdiluted in Tris-buffered saline containing 0.05% Tween and 1%bovine serum albumin for 1 h at room temperature. Primary antibodies(either serum from bleed 4 of a Cen1-injected rabbit, an anti-GFPmonoclonal antibody [mAb] [B34 from Abcam, Cambridge, MA]),or an anti- ${alpha}$ -tubulin mAb (12G10; a kind gift of Joseph Frankel,University of Iowa, Iowa City, IA) were diluted 1:2000, 1:5000,and 1:1000, respectively. Secondary antibodies (anti-rabbitIR800 [Li-Cor Biosciences, Lincoln, NE], anti-mouse Alexa680(Molecular Probes, Eugene, OR), anti Mouse horseradish peroxidase[HRP], and anti-rabbit HRP [Pierce Chemical, Rockford, IL])were diluted 1:10,000. Blots were visualized either on a Li-CorOdyssey scanner or by SuperSignal West Pico chemiluminescentsubstrate (Pierce Chemical) and exposure to film.

Macronuclear Transformations
Plasmids encoding GFP-centrin fusions were transformed intothe developing macronucleus during late stages of conjugationof strains B2086 and CU428 by electroporation (Gaertig and Kapler,2000). Paromomycin-resistant cells were selected and viewedon the fluorescence microscope. The cen1 ${Delta}$ rescuing constructwas transformed into the developing macronucleus of the strainsUCB8 and UCB9 during conjugation by electroporation, using KpnI,XhoI-digested grl3/4:BLAST-prCEN1–3'UTR, followed by selectionwith Blasticidin S (InvivoGen, San Diego, CA).

Micronuclear Knockout and Heterokaryon Generation
pMicCentrinKO1 was digested with SacI and introduced into themicronucleus of B2086- and CU428-conjugating cells by biolisticbombardment as described previously (Bruns and Cassidy-Hanley,2000a). To check for proper integration of the CEN1 knockoutconstruct, total Tetrahymena DNA was isolated (Gaertig et al.,1994b) and digested with NsiI and PstI. Standard Southern blotanalysis was performed using a probe representing sequence upstreamof the transforming fragment. The probe was generated by PCRamplification with primers CentrinUS1 and CentrinUS2 and labeledby the AlkPhos Direct (Amersham Biosciences) labeling system.Crosses to confirm that the transformation occurred in the micronucleuswere performed, and the knockout heterokaryon was constructed,as described previously (Hai et al., 2000) with the modificationthat an outcross was performed on the original transformantstrains to rid them of an apparent micronuclear aneuploidy beforemating with B*VI.

Analysis of cen1 ${Delta}$ Cells
Cultures containing equal numbers of UCB8 and UCB9 cells werestarved and mixed. Ten hours after mixing, an equal volume of2x SPP (1% proteose peptone, 0.1% yeast extract, 0.2% glucose,0.003% FeEDTA final) was added. Seventeen hours after mixing,paromomycin was added to 120 µg/ml to select against cellsthat had not gone through conjugation. Samples were removedfor Western blotting at 6-, 25-, 50-, 75-, and 96-h time points.Samples were removed from separate mating cultures and preparedfor immunofluorescence microscopy at 17-, 24-, 48-, and 72-htime points. Wild-type (WT) cells were treated with paromomycinas a control. To determine whether cells could continue to growwithout Cen1, individual conjugating pairs were isolated into30-µl drops of SPPA media, and cells were counted at 50and 75 h.

Fluorescence Microscopy
Cells containing the GFP-Centrin fusions were placed on slidesand allowed to dry just until cells no longer swam. GFP-Cen1cells were from logarithmic cultures, GFP-Cen2 cells were fromdense cultures, and GFP-Cen3 and GFP-Cen4 were from starvedcultures, as dense and starved cultures had less nonspecificbackground signal. Immunofluorescence microscopy was performedas described previously (Stuart and Cole, 2000). Cells werefixed with both formaldehyde and EtOH as described previously.Fixed cells were visualized on Antibody slides (Bellco Glass,Vineland, NJ). Antibodies were diluted in PBS + 1% bovine serumalbumin. Tetrahymena Cen1 antibody was diluted 1:1000, the 20H5monoclonal centrin antibody raised against Chlamydomonas centrin(a generous gift from Dr. J. Salisbury, Mayo Clinic, Rochester,MN) was diluted 1:2500, the antibody against polyglutamylation(a generous gift from Dr. M. Gorovsky) (Shang et al., 2002)was diluted 1:500, and the 12G10 mAb against ${alpha}$ -tubulin (a generousgift of Dr. J. Frankel, University of Rochester, Rochester,NY) was diluted 1:50. Secondary antibodies were used at a 1:1000dilution and included goat anti-rabbit Alexa594, goat anti-rabbitAlexa488, and donkey anti-mouse Alexa488 (Molecular Probes).Antibody incubations were carried out at room temperature for1 h, or alternatively, overnight at 4°C. To visualize DNA,4,6-diamidino-2-phenylindole (DAPI) was applied to the cellsat 1 µg/ml for 3 min. After each antibody incubation,cells were washed six times with PBS + 0.1% bovine serum albumin.Standard fluorescence microscopy was carried out using a LeicaDMRXA/RF4/V automated microscope with a Cooke Sensi-Cam digitalcamera. Images were collected and subjected to no neighborsor nearest neighbors deconvolution algorithms using the Slidebooksoftware package (Intelligent Imaging Innovations, Denver, CO).

Immunoelectron Microscopy
Tetrahymena cells were pelleted, frozen under high pressurein a BAL-TEC HPM-010 high-pressure freezer, freeze substitutedin 0.25% gluteraldehyde/0.1% uranyl acetate, and embedded inLowicryl HM20. Serial sections (55 nm) were taken and labeledwith 1:200 dilutions of primary antibody in 1% nonfat milk phosphate-bufferedsaline/Tween 20, which included an affinity-purified rabbitanti-GFP primary antibody (a gift from Jason Kahana, LudwigInstitute for Cancer Research, New York, NY, and Pamela Silver,Dana-Farber Cancer Institute, Boston, MA) and the Cen1 antibodydescribed above. A 1:20 dilution of 15-nm gold-conjugated goatanti-rabbit secondary antibody (Ted Pella, Redding, CA) wasused. Grids were stained with uranyl acetate and lead citrateand were visualized in a Philips CM10 electron microscope.

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Identification of a Tetrahymena Centrin Gene Family
We wished to isolate the T. thermophila centrin gene for analysiswith respect to its potential role at basal bodies. A fragmentwas amplified by PCR from Tetrahymena genomic DNA using degenerateprimers designed based on the alignment of several publishedcentrins (see Materials and Methods). Flanking sequences werecloned by inverse PCR, and DNA sequencing revealed the fragmentto be a centrin gene. During the course of this work, this centringene was independently reported by Guerra et al. (2003). Werefer to this gene as CEN1.

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Figure 1. Comparison of centrins from different organisms. Tt, T. thermophila; Hs, Homo sapiens; Mm, Mus musculus; Cr, Chlamydomonas reinhardtii; Pt, P. tetraurelia; Cdc31 from S. cerevisiae; Cmd, calmodulin. (A) Twelve representative centrins were aligned along with two calmodulin proteins. Residues where 50% or more are identical between the proteins are shaded black, and residues where 50% or more are similar are shaded gray. (B) The centrin and calmodulin sequences were subjected to phylogenetic analysis using the Neighbor-Joining method; 1000 replicates were performed, and a representative unrooted tree is displayed as a dendogram. Bootstrap values are displayed as percentages at each node and indicate how often the separation delineated by the branching occurred. Bar = 0.1 substitutions per one amino acid (see Materials and Methods).

The corresponding protein sequence of CEN1 was used as a queryto search the recently sequenced Tetrahymena genome at The Institutefor Genomic Research (TIGR, www.tigr.org), and three additionalpotential centrin genes were identified. Two of these genes,called CEN3 and CEN4 herein, contain 510 and 515 base pairs,respectively, of uninterrupted protein coding sequence. Theremaining gene, CEN2, contains 492 base pairs of coding sequencewith three introns predicted by the protein alignment and standardsplicing rules (Alberts et al., 2002

). All three centrins hadpredicted molecular masses of 19.5 kDa, which is similar toCen1's molecular mass of 19.4 kDa. The translated sequenceswere aligned with a variety of characterized centrins as wellas the Tetrahymena and human calmodulins and placed in a phylogenetictree (see Materials and Methods) (Figure 1). The phylogeneticanalysis revealed three distinct branches: one for the calmodulins,one for two centrins identified in the ciliate Paramecium tetraureliaand CEN3 and CEN4 from Tetrahymena, and the third for all theremaining centrins included in the analysis. Of the Tetrahymenacentrins, Cen1 is most similar to the Chlamydomonas centrinand human Centrin2, which are involved in duplication of basalbodies and centrioles, respectively (Salisbury et al., 2002

;Koblenz et al., 2003

). Cen2 is most closely related to buddingyeast Cdc31, which is essential for spindle pole body duplication,and to human Centrin3. Cen3 and Cen4 are similar to centrinsfound in the infraciliary lattice of the ciliate P. tetraurelia(Klotz et al., 1997

), and this more distantly related branchof the centrin family may be unique to the ciliates.

We checked for expression of these sequences to confirm thatthey encoded genes. Initially, PCR was carried out on a cDNAlibrary generated from vegetatively growing cells, and an unclonedcDNA preparation also from vegetatively growing cells. In bothcases, amplification of sequence resulting from primers specificto CEN1, CEN3, and CEN4 was observed, but not for primers specificto CEN2, which are capable of amplification of CEN2 from thegenome (Figure 2A; our unpublished data). Five clones from eachof these PCR products were sequenced, confirming that the primersused were specific for the targeted sequences. To determinewhether CEN2 was expressed during other stages of the Tetrahymenalife cycle and to examine expression patterns for the threeother centrins, RNA was isolated from vegetatively growing cells,cells in starvation media, and cells at various time pointsthrough the mating cycle (conjugation) for Northern analysiswith probes derived from each of the four centrin genes (Figure 2B).CEN1, CEN3, and CEN4 have similar expression profiles:bands of the expected size are observed during vegetative growth,and the intensity of these bands decreases in cells in starvationmedia, which were no longer dividing. During conjugation, whichoccurred in a starvation medium, expression increases to levelsapproximately twice those seen during logarithmic growth, peaking9 h after initiation of mating. During conjugation, cells losethe oral apparatus, and its reformation is an early event afterconjugants separate (Kiersnowska et al., 1993); the increasein the centrins's expression during later stages of conjugationcould play a role in this process. Among the centrin genes,CEN1 seems to have the highest expression levels, followed byCEN4 and then CEN3, although it is possible that differencesin band intensity may be the result of the ability of each probeto recognize the appropriate message. Because mRNA was detectedfor CEN1, CEN3, and CEN4, these sequences represent three bonafide members of a Centrin family in Tetrahymena. CEN2 expressionwas not detected for this limited set of conditions, althoughthis result does not preclude expression during other untestedgrowth conditions.

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Figure 2. Expression of genes in the Tetrahymena centrin family. (A) PCR products using primers specific for CEN1, CEN2, CEN3, and CEN4 on cDNA from cells during vegetative growth displayed on an agarose gel. Sizes of select marker (M) bands are displayed in kilobase pairs. (B) Northern blot analysis of RNA from vegetatively growing cells (V), starved cells (S), and conjugating cells at various time points after initiation of mating (2, 4, 6, 9, 18 h) (see Materials and Methods). Similar amounts of total RNA were loaded as assessed by absorbance spectroscopy and ethidium bromide staining our unpublished data).

GFP Tagging and Localization of Tetrahymena Centrin Family Members
To understand more about the functions of the centrin genes,we attempted to localize their products within the cell. Eachgene was fused at its N terminus to the GFP (Chalfie et al.,1994) in the vector pVGF1 (Wiley et al., 2000). This vectoris based on a ribosomal DNA processing vector in which rDNAsequences on the plasmid, into which the GFP fusion is inserted,are processed in the developing macronucleus, resulting in amplificationand strong expression (Karrer, 2000). An N-terminal GFP-centrinfusion protein has been reported previously to localize correctlyto centrioles in cell culture, and a C-terminal centrin-GFPfusion protein localized to Chlamydamonas basal bodies (Whiteet al., 2000; Ruiz-Binder et al., 2002), although these fusionsare probably not fully functional (Ruiz-Binder et al., 2002;Kilmartin, 2003). Although Cen2 mRNA is not normally detectableduring vegetative growth, we tagged this protein along withthe others to gain some understanding of where it might functionif expressed. Transformants were recovered for each construct,and live cells were imaged by fluorescence microscopy. GFP-Cen1and GFP-Cen2 both localized to the oral apparatus, a complexcytoskeletal structure rich in basal bodies, microtubule structures,and other nonmicrotubule-based filaments (Sattler and Staehelin,1976; Frankel, 2000) and to cortical rows in a pattern similarto that observed for basal bodies. Interestingly, transformationof both constructs resulted in an apparent disorganization ofthe cortical rows, such that the rows sometimes ended prematurely,or curled around in unusual patterns, suggestive of a dominant-negativephenotype (Figure 4A, a and b). Consistent with these constructsbeing deleterious alleles, the transformants grew slowly, andneither construct was stably maintained over the course of extendedvegetative growth. Nonetheless, Cen1 and Cen2 seem to localizeto basal bodies.

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Figure 4. Localization of GFP-centrin fusion proteins. (A) Fluorescence signal of live cells: a, GFP-Cen1; b, GFP-Cen2; c, GFP-Cen3; and d, GFP-Cen4. The oral apparatus is on the right side in each image. In a and to a greater extent b, cortical rows are affected by the overexpression of the GFP fusion protein. The strong signal in c is at the oral apparatus primarily in the oral crescent, internal to the undulating membrane, and in the apical band. These same regions are visible in d. The contractile vacuole pores are the two small circles near the posterior of the cell. Bar, 10 µm. (B) Immunoelectron microscopy with a GFP antibody and a 15-nm gold-conjugated secondary antibody. Arrowheads indicate representative concentrations of gold particles. a and b, GFP-Cen1 localization; c and d, GFP-Cen2 localization. kf, kinetodesmal fiber; pc, postciliary microtubules; bb, basal body; c, cilia. Representative cross-sectional (a and c) and longitudinal views (b and d) of basal bodies are shown. e and f, localization to the fine-filamentous reticulum of GFP-Cen3, with f also showing some localization along the oral ribs. Ffr, fine-filamentous reticulum; rw, ribbed wall; or, oral-ribs. GFP-Cen4 localization is shown in g, h, and i. g, localization in the fine filamentous reticulum of the oral apparatus. h, sections of both contractile vacuole pores as well as some associated microtubules. cvp, contractile vacuole pore; mt, microtubules; cv, contractile vacuole. h, two basal bodies in cross section with signal apparent along the kinetodesmal fibers.

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Figure 3. Schematic drawings of centrin containing structures. (A) A basal body from a cortical row is represented along with some of the structures associated with it. bb, basal body; kf, kinetodesmal fiber; tm, transverse microtubules; pc, postciliary microtubules. (B) Some of the structures within the oral apparatus are represented. Um, undulating membrane; m, membranelles, of which there are three; or, oral-rib (gray in diagram); df, deep-fiber; ffr, fine-filamentous reticulum (striped in diagram). The undulating membrane and membranelles contain basal bodies and cilia. The oral-rib is a sheet of microtubules along the inside of the oral apparatus cavity beneath the undulating membrane, edged with ribbed walls (not labeled). The deep-fiber consists of a subset of microtubules that continue inward from the oral-rib into the cell. The fine-filamentous reticulum lies beneath the oral ribs.

In contrast, GFP-Cen3 and GFP-Cen4 transformants did not haveany obvious growth defects. The fluorescence signal for Cen3and Cen4 fusion proteins also was strikingly different fromthat of the other centrin fusions. GFP-Cen3 localized primarilyto the oral apparatus. However, this fluorescence signal wasdistinct from the GFP-Cen1 and GFP-Cen2 signal at the oral apparatus,which was punctate and in all likelihood originated from GFPsignal at the oral apparatus basal bodies. Rather, the GFP-Cen3signal was found in a crescent-shaped region to the cell's leftof the undulating membrane and extended along the deep rootlet.Signal also was present at the three membranelles of the oralapparatus, and in a crescent-shaped band at the apical tip ofthe cell (Figures 3B and 4A, c). GFP-Cen4 also localized tothe structures where GFP-Cen3 was observed as well as to thecontractile vacuole pores (CVPs) through which the contractilevacuole expels fluid at the posterior of the cell (Frankel,2000

). Additionally, faint signal was observed along the corticalrows, reminiscent of basal body localization (Figure 4A, d).

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Figure 5. Reactivity of the Cen1 antibody. (A) Western immunoblot analysis using the Cen1 antibody as a probe on recombinant 6-histidine–tagged Centrin (lane 1) and Tetrahymena whole cell extract (wce) from cells in logarithmic growth (lane 2). The reactivity of the preimmune serum on wce also is shown (lane 3). (B) Reactivity of the Cen1 antibody with the overexpressed GFP-centrin fusion proteins. Whole cell extracts from strains expressing different fusion proteins were probed with either the Cen1 antibody (left) or a GFP antibody (right). Because the fusion proteins are overexpressed, the signal overwhelms the endogenous Centrin signal, which is visible with longer exposures. Select marker bands are noted and sizes are in kilodaltons.

We examined cells by immunoelectron microscopy to better resolvethe localization of the four centrin fusions. Cells were preparedfor electromicroscopy by high-pressure freezing and freeze substitution,and sections were stained using an antibody that recognizesGFP followed by a secondary antibody conjugated to 15-nm goldparticles (see Materials and Methods). GFP-Cen1 is abundantat the base of the basal body adjacent to the kinetodesmal fiber,a nonmicrotubule-based striated rootlet that extends from thebasal body toward the anterior of the cell, at the locationwhere new basal body formation occurs (Figures 3A and 4B, a and b)(Allen, 1969

). Additionally, signal was observed alongthe length of the basal body, with a second concentration atthe transition zone between the basal body and the ciliary axoneme.Transition zone localization for centrin has been reported inChlamydomonas (Sanders and Salisbury, 1994

). The overall signalfrom GFP-Cen2 was significantly weaker than that for GFP-Cen1in this experiment, but when multiple images were analyzed signalwas detected in a pattern similar to that of GFP-Cen1 (Figure 4B, c and d).GFP-Cen3 and GFP-Cen4 both localized primarilyto the region directly underneath the ribbed wall and the oral-ribswithin the oral apparatus that corresponds to the fine filamentousreticulum (Williams and Luft, 1968

; Williams and Bakowska, 1982

)(Figures 3B and 4B, e–g), and GFP-Cen4 signal was clearlydetected at the contractile vacuole pores (Figure 4B, h). WeakGFP-Cen4 signal also was observed at the basal bodies, primarilyon the kinetodesmal fiber (Figure 4B, i). When a strain notexpressing GFP was submitted to identical antibody incubations,there was almost no background signal apparent, supporting theauthenticity of the localization data (our unpublished data).

Together, the localization of the GFP fusion proteins and theexpression patterns of the different centrins suggest that eachmember of the Tetrahymena centrin family has a unique role withinthe cell. The possibility remains that there is some redundancyamong the centrin genes, particularly between CEN3 and CEN4,because their protein products have similar distributions withinthe oral apparatus. Because our primary interest is the roleof centrin in basal body duplication during vegetative growth,we chose to focus on Cen1. Of the four Tetrahymena centrins,Cen1 is most similar to human centrin2, which is required forcentriole duplication. Furthermore, we have shown that Cen1is expressed strongly during logarithmic growth, and a GFP fusionprotein localizes to basal bodies at the precise location whereinitiation of basal body duplication is thought to occur (Allen,1969).

Basal Body Localization of Endogenous Cen1
A polyclonal antibody was raised against full-length 6-histidine–taggedCen1 (see Materials and Methods) and initially characterizedby Western blot analysis. The antibody detected recombinant6-histidine–tagged Cen1 (Figure 5A, lane 1), and a bandthe size expected for centrin (19.5 kDa) in a whole cell Tetrahymenaextract (lane 2). We then took advantage of the GFP-centrinfusion strains, to examine the antibody's reactivity with eachindividual Tetrahymena centrin family member. GFP adds approximately27 kDa to the molecular mass of the protein, thus allowing foreasy separation of the tagged allele from the endogenous proteins,which all have a molecular mass of 19.5 kDa. To control forthe individual expression level of each protein, antibody recognizingthe GFP tag was used as a control. As expected, the Cen1 antibodystrongly recognized GFP-Cen1 (Figure 5B, left). The antibodyhad minimal cross-reactivity with GFP-Cen3 and slightly morecross reactivity with GFP-Cen2 and GFP-Cen4 compared with theGFP probed immunoblot. Endogenous centrin was clearly visiblewith the Cen1 antibody on longer exposures (our unpublisheddata). We therefore concluded that our antibody is largely specificto Cen1, but it may interact with the other centrins at a low-to-moderatelevel.

To examine localization of endogenous Cen1, we used the Cen1antibody for immunofluorescence and immunoelectron microscopy.Immunofluorescence was performed on cells from a logarithmicculture (Figure 6A) using our rabbit polyclonal antibody (anti-Cen1),and a mAb (20H5) that recognizes centrins from a variety ofspecies and has previously been used to localize centrin inTetrahymena (Jerka-Dziadosz et al., 1995; Guerra et al., 2003).Staining patterns from each antibody were very similar but notidentical. Both recognized the basal bodies along the corticalrows and in the oral apparatus, but the 20H5 antibody recognizedadditional structures that the Cen1 antibody did not. The signalfrom 20H5 was observed at the oral crescent (corresponding tothe fine filamentous reticulum) and also at the apical filamentousband (Jerka-Dziadosz, 1981; Jerka-Dziadosz et al., 1995). Boththese structures were revealed by GFP-Cen3 and GFP-Cen4. However,the 20H5 antibody did not recognize the contractile vacuolepores, raising the possibility that this antibody can recognizeCen1 and Cen3, but not Cen4, or that Cen4 is not accessibleto the antibody at the CVPs. Consistent with this interpretation,the 20H5 antibody strongly recognized Cen1 and Cen3 by Westernblot analysis, whereas showing moderate affinity to Cen4 andvirtually no affinity for Cen2 (our unpublished data). Likethe GFP-Cen1 data, data from the Cen1 antibody indicates thatCen1 localizes specifically to basal bodies.

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Figure 6. Cen1 localization at basal bodies. (A) Immunofluorescence microscopy using the Cen1 antibody and the monoclonal centrin antibody 20H5 raised against Chlamydamonas centrin. DNA is visualized with DAPI. Bar, 10 µm. (B) Serial section immunoelectron microscopy of a basal body in cross section with the Cen1 antibody. Panels proceed from the axoneme distal part of the basal body (a) and track upwards through the structure. Figure 3A serves as a reference for some of the basal body associated structures that are present. Certain basal body associated structures are identified in sections where they are most prominent, although this does not preclude these same structures from being visible in other sections. cw, cartwheel; kf, kinetodesmal fiber; pc, postciliary microtubules; tz, transition zone; tm, transverse microtubules; c, cilia; bb, basal body. Centrin concentrates on the transverse microtubules that are seen obliquely, on the kinetodesmal fiber, and at the transition zone (k). (C) Serial section immunoelectron microscopy of three basal bodies in longitudinal section.

To map Cen1 localization within basal bodies, immunoelectronmicroscopy was performed on serial sections of cells from alogarithmic culture using the Cen1 polyclonal antibody. Thisanalysis on endogenous levels of Cen1 revealed a similar localizationpattern to that observed with the GFP-Cen1 strain. Serial sectionsthrough six basal bodies where examined. At the basal body,there are two major centers of Cen1 concentration. The firstis at the base of the basal body, along and adjacent to thekinetodesmal fiber (Figures 3A, 6B, a–e, and 6C, a–c).At the very base of the basal body (most distal to the axoneme),this signal is immediately adjacent to the basal body (Figure 6B, a),the site of new basal body formation (Allen, 1969).As the cross-sectional serial sections are tracked through thebasal body, this signal moves away from the basal body, followinga path along the transverse microtubules that extend to theadjacent cortical row (for reference, see Figures 3A and 6B, c–j).There is also a moderate amount of signal from theCen1 antibody within the basal body cylinder that extends thelength of the basal body immediately adjacent to basal bodymicrotubules (Figure 6B, g–j). The second concentrationof Cen1 occurs at the transition zone between the basal bodyand the axoneme (Figure 6B, k). These localization patternsalso were observed in longitudinal sections (Figure 5C, a–c).

Cen1 Is Required for Basal Body Duplication and Maintenance in Tetrahymena
Both Cen1's localization to the base of the basal body whereduplication is initiated, and the disruption of the corticalrows caused by overexpression of the GFP-Cen1 fusion protein,are suggestive that Cen1 has an important role at the basalbody. To assess this more directly, a null strain was created.We replaced CEN1 with the NEO2 drug resistance cassette, whichprovides resistance to paromomycin (Gaertig et al., 1994a),in the diploid micronucleus by homologous recombination (Brunsand Cassidy-Hanley, 2000a), as confirmed by Southern analysis(Figure 7A). This strain was then used to create a knockoutheterokaryon (Hai et al., 2000), a strain homozygous for theknockout in the micronucleus, but containing only wild-typeCEN1 in the expressed macronucleus. When two such strains withdifferent mating types are mated to each other, a new macronucleusis formed based on the DNA of the germline micronuclei of theparent strains. The resulting progeny lack the CEN1 gene, havingthe NEO2 gene cassette in its place (Figure 7A). CEN1 knockoutheterokaryon strains UCB8 and UCB9 were mated to each other,and 120 µg/ml paromomycin was added to select for cellsthat had proceeded successfully through mating and developmentof progeny. The cell density of the culture increased only slightlyby 72 h after initiation of mating (starting at 2.5 x 10⁵ cells/ml,and increasing to 2.8 x 10⁵ cells/ml), and eventually all cellsdied, either due to sensitivity to paromomycin (nonmating, parentalcells) or due to the lack of Cen1 (progeny). No "survivors"were observed in these cultures, indicating that none of theother centrins can substitute for Cen1 in its essential function.Western blot analysis confirmed that Cen1 protein levels werereduced significantly by 50 h after mating and that the reductionin Cen1 protein levels continued over time (Figure 7B). TheseWestern blot results further indicate that either the antibodyis very specific for Cen1 and/or Cen1 is the predominantly expressedcentrin in cells, because the decrease in Cen1 was not maskedby the other centrins.

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Figure 7. Cen1 protein levels decrease when CEN1 is deleted. (A) Southern blot analysis of the CEN1 locus. The fragment used for transformation extends from the SacI site to the PstI site with the NEO2 cassette replacing CEN1. Total Tetrahymena DNA from wild-type cells (lane 1), the micronuclear transformant (lane 2), and progeny from the knockout heterokaryon strains rescued by CEN1 transformed at a second genomic location (lane 3) was digested with NsiI and PstI. The sizes of select marker bands (M) are noted in kilobase pairs. (B) Western blot analysis of progeny from the cen1 ${Delta}$ knockout heterokaryon strains UCB8 and UCB9 (cen1 ${Delta}$ ) and of the progeny from wild-type strains B2086 and CU428 (CEN1). Cen1 is visualized with the Cen1 polyclonal antibody, and a mAb to ${alpha}$ -tubulin is used as a loading control. V, vegetative growth; S, starvation; numbers correspond to hours after parental cells were mixed. Marker bands are noted, and sizes are in kilodaltons.

The ability of cen1 ${Delta}$ cells to divide was tested by mating UCB8and UCB9 cen1 ${Delta}$ knockout heterokaryon strains and isolating individualconjugating pairs into small drops of media. As a control, B2086and CU428 cells (both wild-type for CEN1) were subjected tothe same procedure. Cells were counted after 50 h of growthand checked again at 75 h, and an estimate as to how many divisionseach cell had completed was made. Both wild-type and cen1 ${Delta}$ cellshad a significant population of cells that were completely unableto divide after conjugation (29 and 55%, respectively). Mostwild-type cells went on to form stable vegetative cultures (62%).In contrast, none of the cen1 ${Delta}$ cells progressed to form a stablevegetative culture. However, of the 45% that did divide afterconjugation, more than half divided approximately three times.Therefore, at least some of the cen1 ${Delta}$ strains were able to undergoseveral cell divisions before arresting and eventually dying.

The effect of the lack of Cen1 on basal body integrity was observedby fixing and staining cells at various time points after matingwith both the 20H5 monoclonal centrin antibody and an antibodyraised against a polyglutamic acid peptide that recognizes atubulin modification, polyglutamylation, that is abundant atbasal bodies (Shang et al., 2002) (Figure 8). The number ofcells with an obviously reduced number of basal bodies comparedwith wild-type was counted at each time point. Cells proceededthrough conjugation without apparent problems, and 17 h afterinitiation of mating the cells had separated and looked normal.However, 24 h after mating, some cells displayed reduced centrinsignal and fewer basal bodies along the cortical rows. By 48h, cells had fewer basal bodies, and by 72 h most of the cellsshowed a severe phenotype, including loss of most basal bodies,disorganization of the remainder along the cortical rows, andloss of the oral apparatus. Cell division intermediates wereobserved in the samples, and although these cells looked capableof completing the division cycle, because they did not accumulateat later time points, they were unable to form a new oral apparatusand had fewer basal bodies, especially in the posterior halfof the cell (Supplemental Figure 1A). Additionally, there wassignal from the polyglutamic acid antibody at locations wherethere was no centrin signal, indicating that there was no longerenough Cen1 to localize to all of the remaining basal bodies.

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Figure 8. Deletion of CEN1 results in a failure to duplicate basal bodies. cen1 ${Delta}$ knockout heterokaryon strains UCB8 and UCB9 were mated, and their progeny were analyzed at 17-, 24-, 48-, and 72-h time points by immunofluorescence microscopy. The monoclonal centrin antibody 20H5 was used along with an antibody that recognizes polyglutamic acid, which is prominent on modified tubulin at basal bodies. DNA is visualized with DAPI. WT is strain CU428 in logarithmic growth. Percentages refer to the proportion of cells with reduced numbers of basal bodies, with the images shown being representative (n = 200). Rescue refers to UCB8 x UCB9 progeny that were rescued by CEN1 transformed into a second site in the genome. In the WT and 17-h samples, 100% of cells had an apparently normal number of basal bodies. The oral apparatus is oriented on the right side of each panel. Bar, 10 µm.

To ensure that the loss of basal bodies was due to the lackof Cen1, and not the result of the introduction of paromomycinto the cultures, three controls were performed. First, UCB8and UCB9 cen1 ${Delta}$ knockout heterokaryon strains were mated to eachother, and the resulting culture was allowed to progress inthe absence of drug, allowing parental, unmated cells to largelyovertake the population. Nevertheless, the loss of centrin signaland basal bodies was still observed in some cells, whereas ina wild-type control, cross-centrin signal remained high throughoutthe population (Supplemental Figure 1B; our unpublished data).In the second control, a wild-type strain was subjected to 120µg/ml paromomycin and observed at time points after additionof drug similar to those used in the experiment with the knockoutstrains. Although dying cells often had disorganized basal bodies,these cells were distinct from cen1 knockout cells in that centrinsignal remained strong, and these cells were small and rounded(Supplemental Figure 1C). In the third control, a constructthat reintroduces CEN1 at the GRL3/4 locus (Verbsky and Turkewitz,1998) rescued cen1 ${Delta}$ cells. UCB8 and UCB9 cells were mated, andthis construct was transformed into the developing macronucleusby electroporation. Transformants were recovered that were resistantboth to blasticidin S, which selects for the bsr gene used inthis construct, and to paromomycin, which selects for the NEO2cassette used to disrupt CEN1 (Figure 7A; our unpublished data).Rescued cultures grew normally and were subjected to immunofluorescencemicroscopy (Figure 8, bottom). The cortical rows and oral apparatusin these cells were indistinguishable from wild type, indicatingthat when Cen1 is restored to these cells, they no longer havebasal body defects.

The immunofluorescence data on the cen1 ${Delta}$ strain strongly suggeststhat basal bodies are absent from these cells at later timepoints. However, fluorescence signal at late time points wasstill observed, more so with the antibody to polyglutamic acid,and the question remained whether this signal was at basal bodies,or some identifiable remnant of basal bodies. To address thisissue, electron microscopy was performed on cells processed68 h after the initial mixing of the two knockout heterokaryonstrains. Fewer basal bodies were observed in sections from thecen1 knockout strains compared with a wild-type control cross.When basal bodies were detected, they often seemed incompletewithout cilia attached (Figure 9A). Occasionally the electrondense structures associated with the base of the basal bodywere present without all of the microtubules that normally comprisea basal body (our unpublished data). Immunoelectron microscopywith the Cen1 antibody revealed that basal bodies with moreCen1 were better preserved than basal bodies with less antibodysignal (our unpublished data). The possibility that Cen1 isimportant for maintenance of basal bodies was addressed furtherby immunofluorescence microscopy using an antibody to ${alpha}$ -tubulin,which detects cilia, a marker for a functioning basal body,as well as basal bodies. By 48 h after the initiation of matingof cen1 ${Delta}$ cells, many punctate spots reminiscent of basal bodiesremained but a large percentage of these did not have attachedcilia, indicating the absence of functional basal bodies atthese sites (Figure 9B). Together, the results from the micronuclearknockout strains indicate that centrin is important for boththe duplication and stability of basal bodies.

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Figure 9. Cen1 is required for basal body maintenance. (A) Serial sections of a cen1 ${Delta}$ cell (top) and a cell from a wild-type control cross (bottom). The asterisks (*) (top left) indicate the location of one incomplete basal body and a second site of interest. The basal body (top left) does not nucleate a cilium and seems disorganized at its base. The material at the bottom right is unrecognizable as a basal body, although it is present where a basal body would be expected given the location of the mitochondrion on the right (m) and the indentation in the cell surface. In the wild-type panels, three basal bodies (*), two with cilia clearly attached, are visible. Basal bodies are between mitochondria (m), and the cilia emerge from indentations in the cell surface. Bar, 0.5 µm. (B) ${alpha}$ -Tubulin localization in cen1 ${Delta}$ cells. Times are after mating initiation of the cen1 ${Delta}$ knockout heterokaryon strains, and cells were stained with a mAb raised against ${alpha}$ -tubulin (12G10). By 48 h, many apparent basal bodies do not have cilia attached. Bar, 10 µm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION ACKNOWLEDGMENTS REFERENCES

We report the initial characterization of a family of four centringenes in the ciliate T. thermophila. Two of these genes areclosely related to the majority of the centrin genes found inother organisms, whereas the other two are related to the centringenes identified in another ciliate, P. tetraurelia. Ciliatescontain many distinct and highly specialized cytoskeletal structures.In Tetrahymena, these include basal bodies, cilia, micronuclearspindles, macronuclear microtubule arrays, a cortical networkorganized around the basal bodies of the ciliary rows, the contractilevacuole pores, and the complex microtubule and filamentous structuresthat comprise the oral apparatus (Gaertig et al., 1993

; Frankel,2000

). Because centrins play multiple roles at structures associatedwith microtubules (Taillon et al., 1992

), it would not be surprisingif specialized centrins evolved along with some of these structuresunique to ciliates. For example, GFP-Cen3 localizes predominantlyto the fine filamentous reticulum of the oral apparatus anda band at the apex of the cell, and GFP-Cen4 localizes primarilyto these structures and to the contractile vacuole pores. Thesestructures are involved in dynamic processes: the undulatingmembrane of the oral apparatus sweeps media (food) into theoral cavity, whereas when the contractile vacuole expands, contracts,and ruptures, fluid is expelled through the CVPs maintainingthe cell's proper osmolarity. The function of the apical bandis not known; it is distinct from the contractile division furrowring, although it, too, may be contractile and involved in regulatingcell shape (Jerka-Dziadosz, 1981

). In Paramecium multimicrnucleatum,the number of contractile vacuoles increases in response toan increased amount of calcium in the environment (Iwamoto etal., 2003

). The assumption is that this is a response with whichthe cell rids itself of excess calcium, but it is possible thatcalcium, through centrin, more directly stimulates the assemblyof this structure. Although the roles for Cen3 and Cen4 at thefine filamentous reticulum and the contractile vacuole poreare not known, it is possible the contractile properties ofcentrin affect the dynamic properties of these structures (Salisburyet al., 1984

). Additionally, Tetrahymena Cen1 along with innerarm dynein is involved in ciliary beat changes in response tocalcium (Hennessey et al., 2002

; Guerra et al., 2003

), and perhapscentrins at the fine filamentous reticulum perform a similartask for this structure.

Tetrahymena CEN1 and CEN2 are on branches of the centrin treethat are most widely conserved throughout the eukaryotic world,and here we examined the function of Cen1 in MTOC duplication.Centrin is required for this process in species as diverse asyeast, green algae, and humans (Baum et al., 1986; Salisburyet al., 2002; Koblenz et al., 2003). Although GFP-Cen1 and GFP-Cen2both localize to basal bodies, CEN2 is not normally expressedduring vegetative growth, or conjugation. This situation maybe similar to that in humans, in which centrin1 expression islimited to the testes and retinal cells (Hart et al., 1999).We have not determined whether CEN2 is expressed under differentconditions, or not at all, although the similarity to othercentrins, in particular yeast Cdc31 and human centrin3, leadsus to suspect that it is a functional gene. CEN1, however, ishighly expressed in vegetative and mating cells. Localizationof the endogenous protein places the majority of Cen1 at twopositions on the basal body. One is at the transition zone betweenthe basal body and the axoneme of the cilium, as has been reportedin Chlamydomonas (Sanders and Salisbury, 1994). The second isat the base of the basal body adjacent to the kinetodesmal fiberwhere probasal body formation is initiated (Allen, 1969). Disruptionof CEN1 led to the progressive loss of basal bodies. Of thebasal bodies that remained, many were defective and unable toact as MTOCs for the cilia. Cen1 is a stable molecule, and smallamounts of Cen1 remained even 72 h after mating initiation ofthe knockout heterokaryon strains. Therefore, our experimentsexamine the results of a slow depletion of Cen1. As Cen1 decreased,cells were unable to fill their cortical rows with the propernumber of basal bodies, or to form a new oral apparatus, suggestingthe requirement for Cen1 in the duplication of basal bodies.

The deterioration of the remaining basal bodies indicates thatCen1 also is required for proper basal body maintenance. Thedepletion of ${gamma}$ -tubulin yielded a related phenotype, demonstratingthe necessity for this protein in basal body maintenance aswell as basal body duplication. When ${gamma}$ -tubulin is depleted, oralapparatus basal bodies are lost before cortical basal bodies,suggesting that turnover of ${gamma}$ -tubulin is more rapid in the oralapparatus than at the basal bodies of the cortical rows, andrequired for these organelles' stability (Shang et al., 2002).The CEN1 knockout strain had no such hierarchy of loss, indicatingthat turnover of Cen1 is not significantly different at basalbodies along the cortical rows and basal bodies at the oralapparatus. Instead, Cen1 seems to be very stably associatedwith basal bodies and plays some role in preserving these organelles.Hence, a cen1 ${Delta}$ cell preparing for division can have one existingoral apparatus that seems normal and a highly aberrant developingoral apparatus (Supplemental Figure 1A). We do not know whetherCen1's roles in basal body duplication and maintenance can beseparated, but it is tempting to speculate that Cen1 localizationto the base of the basal body is important for duplication,whereas localization to the transition zone is important forbasal body maintenance and function. Future work on Cen1 bindingpartners will shed light on this issue.

Our experiments did not reveal any association between the Tetrahymenacentrin proteins and the micronucleus. This is somewhat surprisingbecause centrins are found at mitotic spindle poles in a widerange of organisms. This supports the previous finding thatcentrin was not detected with ${gamma}$ -tubulin at the micronucleus (Shanget al., 2002). However, centrin antibodies tested to date havenot revealed centrin localization at the contractile vacuolepores, and our analysis of Cen4 indicates that it is likelypresent at this structure. Thus, the possibility remains thatthe experiments have not been sensitive enough to reveal centrinat spindle poles. Also, the GFP tag could interfere with centrinlocalization to the spindle pole in Tetrahymena. Another possibilityis that there are yet more Tetrahymena centrin genes encodingisoforms that are at the spindle pole. Finally, it is possiblethat Tetrahymena does not require centrin for its mitotic apparatus.Few components of the Tetrahymena mitotic apparatus have beenidentified, and this issue may take some time to resolve.

We have shown there exists a family of Tetrahymena centrin geneswith at least three bona fide members based on expression. Twoof the centrins likely function at specialized fibrillar structuresin the oral apparatus and the apical tip, and one of these alsomay act at the contractile vacuole pore. The predominant centrin,encoded by CEN1, localizes to basal bodies, and is requiredfor their duplication and maintenance. The genetic malleabilityof these cells will likely lead to further insights into themechanisms by which Cen1 functions at the basal body, and Cen3and Cen4 function at their respective locations in the cell.

ACKNOWLEDGMENTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

This manuscript and our understanding of the Tetrahymena cytoskeletonwere greatly enhanced by Joe Frankel's careful reading and advice.We thank Chandler Fulton, Joe Frankel, Jeffrey Salisbury, andMarty Goroversusky for antibodies; Peter Bruns and Aaron Turkewitzfor strains; and Jacek Gaertig and Aaron Turkewitz for cDNApreparations. David Prescott, Eric Cole, Aaron Turkewitz, MengChao Yao, Joe Frankel, and Jacek Gaertig were very helpful withadvice on the molecular biology, genetics, and/or cytology ofTetrahymena. Preliminary sequence data were obtained from TheInstitute for Genomic Research Web site at http://www.tigr.org.Ed Orias and Jonathan Eisen helped with genome sequence issues.We are particularly indebted to Craig Weaver at Martek Biosciences(Boulder, CO) for help with their Bio-Rad PDS-1000/He BiolisticsApparatus. Danielle Perry was instrumental in expressing Cen1in E. coli. Catherine Lozupone helped with the phylogeneticanalysis of the centrin family. We also thank Michele Jonesand Chad Pearson for helpful comments on the manuscript, andthe members of the laboratory for support. This work has beensupported by National Institutes of Health Grant GM-067898 (toM. W.). Early phases of the project at Colgate University weresupported by National Science Foundation Grant MCB-9727240 (toH.B.M.).

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E04–10–0919)on June 8, 2005.

The online version of this article contains supplemental materialat MBC Online (http://www.molbiolcell.org).

Present address: Institute for Molecular Bioscience, Universityof Queensland, Brisbane QLD 4072, Australia

Present address: SUNY Upstate Medical University, 750 East AdamsSt., Syracuse, NY 13210-2375

^|| Present address: The American Association for the Advancementof Science, 1200 New York Ave. NW, Washington, DC 20005.

Address correspondence to: Mark Winey (mark.winey{at}colorado.edu).

REFERENCES