Centrin1 Is Required for Organelle Segregation and Cytokinesis in Trypanosoma brucei

Angamuthu Selvapandiyan^*^,, Praveen Kumar^,, James C. Morris, Jeffrey L. Salisbury^||, Ching C. Wang, and Hira L. Nakhasi^*

*Division of Emerging and Transfusion Transmitted Diseases, Center for Biologics Evaluation and Research, Food and Drug Administration, Bethesda, MD 20892; Department of Pharmaceutical Chemistry, University of California, San Francisco, CA 94143; Department of Genetics and Biochemistry, Clemson University, Clemson, SC 29634; and ^||Tumor Biology Program, Mayo Clinic College of Medicine, Rochester, MN 55905

Submitted January 12, 2007; Revised May 22, 2007; Accepted June 6, 2007
Monitoring Editor: Orna Cohen-Fix

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Centrin is a calcium-binding centrosome/basal body–associatedprotein involved in duplication and segregation of these organellesin eukaryotes. We had shown that disruption of one of the centringenes (centrin1) in Leishmania amastigotes resulted in failureof both basal body duplication and cytokinesis. Here, we undertookto define the role of centrin1 (TbCen1) in the duplication andsegregation of basal body and its associated organelles kinetoplastand Golgi, as well as its role in cytokinesis of the procyclicform of Trypanosoma brucei by depleting its protein using RNAinhibition methodology. TbCen1-depleted cells showed significantreduction in growth compared with control cells. Morphologicalanalysis of these cells showed they were large and pleomorphicwith multiple detached flagella. Both immunofluorescence assaysusing organelle-specific antibodies and electron microscopicanalysis showed that TbCen1-deficient cells contained multiplebasal bodies, kinetoplasts, Golgi, and nuclei. These multipleorganelles were, however, closely clustered together, indicatingduplication without segregation in the absence of centrin. Thisfailure in organelle segregation may be the likely cause ofinhibition of cytokinesis, suggesting for the first time a newand unique role for centrin in the segregation of organelleswithout affecting their multiplication in the procyclic formof T. brucei.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Centrin is a calcium-binding protein associated with microtubule-organizingcenters (MTOC), such as the centrosome of nonciliated cells,basal bodies of ciliated or flagellated cells, and spindle polebody of yeast cells (Salisbury et al., 1988; Spang et al., 1993;Salisbury, 1995; Wolfrum and Salisbury, 1998; Klink and Wolniak,2001). It is part of the filaments within and attached to suchorganelles that can contract in response to changes in Ca²⁺concentration as in Tetraselmis striata and Chlamydomonas reinhardtii(Salisbury et al., 1984; Wright et al., 1985). Thereby centrinis involved in duplication and segregation of centrosome/basalbodies and is important for cell division in eukaryotes (Erraboluet al., 1994; Salisbury, 1995). However, the basic mechanismof such centrin function is not known. There are several centringenes identified in different eukaryotes: one in Chlamydomonas(CrCen) and Saccharomyces cerevisiae (CDC31), four in mice (MmCen1-4),and three in humans (HsCen1-3; Huang et al., 1988; Erraboluet al., 1994; Salisbury, 1995; Gavet et al., 2003). The recentlycompleted genome database for two trypanosomatids, i.e., Trypanosomabrucei, causative agent of African sleeping sickness and Leishmaniamajor that causes cutaneous leishmaniasis disease in human (Berrimanet al., 2005; Ivens et al., 2005) and our own studies with L.donovani, causative agent of visceral leishmaniasis in human,have revealed that there are five putative centrin genes inthis group of organisms (Selvapandiyan et al., 2001, 2004).

Some of the centrins have been assigned particular functions.For example, one group of centrins, which includes human centrins(HsCen1 and 2), mouse centrins (MmCen1 and 2), C. reinhardtiicentrin (CrCen) and Paramecium centrins (PtCen2 and 3) is involvedin centrosome/basal body segregation (Middendorp et al., 1997;Koblenz et al., 2003; Ruiz et al., 2005). The other group containinghuman centrin3 (HsCen3), mouse centrin3 (MmCen3), yeast centrin(CDC31), and Leishmania centrin1 (LdCen1) plays a role in centrosome/basalbody duplication (Middendorp et al., 1997; Khalfan et al., 2000;Gavet et al., 2003; Selvapandiyan et al., 2004). Mouse centrin4(MmCen4) is involved in the basal body assembly in the brainependymal and choroidal ciliated cells (Gavet et al., 2003).Knockdown of centrin2 by ribonucleic acid inhibition (RNAi)in human cells and a centrin gene deletion in Tetrahymena thermophilayielded defects in centrosome/basal-body duplication and cellcycle progression (Salisbury et al., 2002; Stemm-Wolf et al.,2005; Tsang et al., 2006), whereas centrin disruption in Chlamydomonasled to aberrant numbers of basal bodies that interfered withcytokinesis (Koblenz et al., 2003). Centrins have also beenfound involved in other cellular processes such as maintenanceof membrane integrity and cell morphology in yeast (yeast centrin,CDC31; Ivanovska and Rose, 2001), homologous recombination andnucleotide excision repair in Arabidopsis (centrin2) and humans(HsCen2; Molinier et al., 2004; Nishi et al., 2005), nuclearmRNA export in yeast (CDC31; Fischer et al., 2004), genomicinstability via increased chromosome loss in C. reinhardtii(CrCen; Zamora and Marshall, 2005), Golgi duplication in T.brucei (TbCen2; He et al., 2005) and in defining the geometryof basal body duplication in Paramecium (PtCen2 and 3; Ruizet al., 2005).

Our earlier studies with Leishmania donovani have shown thatwhen the N-terminally (1-28 amino acids) deleted L. donovanicentrin protein (LdCen1) was overexpressed in the parasite,it had a dominant negative effect on the growth of the parasite,resulting in an enrichment of cells in the G2/M stage (Selvapandiyanet al., 2001). Further, a deletion of this gene in L. donovaniresulted in specific growth arrest in the amastigote form (astage that proliferates intracellularly in human macrophages)in vitro as well as ex vivo in human macrophages (Selvapandiyanet al., 2004). The growth arrested amastigotes were defectivein basal body duplication followed by a failure in cytokinesisresulting in large multinucleated cells (Selvapandiyan et al.,2004).

The eukaryotic cytoskeleton regulates important cellular functions,including the control of cell shape, cell movement, intracellulartransport, and cell division. Centrosome/basal body nucleatemicrotubules necessary for postmitotic changes, which includeorganelle repositioning and cytokinesis. The protozoan parasiteT. brucei has unique and precisely ordered microtubule-mediatedcytoskeletal structures. These include the subpellicular corsetof microtubules that maintain cell shape, the single flagellumthat exits the cell body through the flagellar pocket, the mitochondrialDNA (kinetoplast), the basal body, and the single nucleus (Robinsonet al., 1995). In addition basal bodies in T. brucei play arole, probably through microtubules, in determining the siteof the new Golgi and endoplasmic reticulum export site (He etal., 2004). The multiplication and segregation of these structuresare developmentally coordinated with great precision (Robinsonet al., 1995). They offer a great opportunity for studying therelationship between the organelles, and the proteins associatedwith them that are involved in their function.

A genomic sequence search in the T. brucei database (Berrimanet al., 2005) revealed the presence of five putative centringenes in these organisms (TbCen1-5). The functions of two ofthese centrins (TbCen2 and 3) have been recently reported (Heet al., 2005). TbCen2, which is localized at the basal bodyand a bilobed structure close to the Golgi, is responsible forthe duplication of both basal body and the Golgi. TbCen3, whichis localized at the basal body of the parasite, is also responsiblefor the duplication of the basal body in T. brucei (He et al.,2005). Here, we characterize the localization and function ofTbCen1 in T. brucei. Our studies reveal that TbCen1 is localizedat the basal body and a bilobed structure close to the Golgi.TbCen1 depletion affects cell growth and results in impairmentof the appropriate segregation of basal bodies and nucleus,along with the arrest in the movement of the other basal body–associatedorganelles, viz., kinetoplasts and Golgi. In addition, we observedearly on detachment of flagella, which is part of basal bodycomplex. The outcome of such a defect leads to loss of cytokinesis,resulting in enlarged cell size. Our studies also revealed thatdepletion in TbCen1 does not affect the duplication of basalbody, kinetoplast, Golgi, and nucleus, unlike TbCen2. This suggeststhat TbCen1 may have a unique role in overall organelle segregationand not in organelle duplication.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In Vitro Culture of Parasites
T. brucei procyclic form strain 29-13 that harbors integratedgenes for T7 RNA polymerase and tetracycline repressor (Wirtzet al., 1999) was used. The parasites were grown in SDM-79 mediumsupplemented with 10% fetal bovine serum during normal growthand 15% during transfection and clonal selection. G418 (15 µg/ml)and hygromycin B (50 µg/ml) were added in the medium topreserve T7 RNA polymerase and tetracycline repressor gene constructswithin the cells. The parasites were grown and harvested asdescribed previously (Morris et al., 2004).

Gene Cloning and Transfection of Parasites for RNAi
Gene characterization via cognate mRNA degradation (RNAi) andarrest of translation is a routinely followed molecular techniqueas described in certain eukaryotes (Ullu et al., 2004). Thisis achieved through plasmid construct carrying a unique portionof the gene, which after transfection in cell generates double-strandedRNA of the gene upon induction (currently with tetracycline),which then targets the cognate native mRNA for degradation.Specifically in this study to amplify PCR fragment of TbCen1gene for developing RNAi construct, gene-specific forward andreverse primers were designed utilizing the putative centrinsequence from the T. brucei genome sequence databank (Berrimanet al., 2005). Oligos were designed (Supplementary Table S1)in which the amplicon constitutes a portion from the 5' untranslatedregion (from –69 base pairs) of the genes into approximatelythe middle of the open reading frame (ORF; +278 base pairs)with HindIII and XhoI restriction sites added to the terminiof the PCR fragments. The PCR amplified fragment was a 347-basepair unique sequence that had no significant sequence identitywith the rest of the T. brucei genome sequences. The fragmentwas subcloned into the HindIII and XhoI sites of the pZJM vector(Wang et al., 2000). The recombinant plasmid was linearizedwith NotI and DNA transfection carried out on the procyclicform of T. brucei using a published procedure (Morris et al.,2004) using a BTX ECM 630 Electroporator (BTX, San Diego, CA,500 V and 275 µF). Transfectants were selected in thepresence of 2.5 µg/ml phleomycin and a clonal cell linewas obtained by limiting dilutions. For induction of RNAi, thecloned stable transfectant that reached a constant growth rateafter at least three regular subpassages was cultured in thepresence of 1.0 µg/ml tetracycline. For monitoring cellgrowth, the cells were counted at different time intervals usinga Coulter Z1 particle counter (Beckman Coulter, Fullerton, CA)with a starting culture of 1 x 10⁵ cells/ml. To include countingof larger cells that appear during RNAi, an aperture settingbetween 6.5 and 30 µm was used.

Isolation of RNA and Northern Blot Analysis
To examine the specific reduction in centrin transcription duringRNAi induction, the cloned stable transfectant, either uninducedor induced with tetracycline for 3 d, was analyzed for TbCen1mRNA level using Northern blot analysis. The membrane was rehybridizedwith ${alpha}$ -tubulin gene-specific probe as loading control, and withTbCen2-5 gene-specific probes to confirm the specific inhibitionof TbCen1 transcript. Probes were designed (Supplementary TableS1) in such a way that the amplicon constitute a portion fromthe middle of the ORF, not including the region selected forRNAi. The signal intensity was quantitated using a PhosphorImager system (Molecular Dynamics, Amersham Pharmacia Biotech,Piscataway, NJ) as described previously (Selvapandiyan et al.,2001).

Ectopic Expression of Centrins in T. brucei
In the absence of specific antibodies expression of a gene isroutinely monitored by the localization of an ectopic expressionof that protein through an expression plasmid (Selvapandiyanet al., 2001). Such proteins are usually expressed with tagsequences that help in the specific identification of protein'slocalization. To ectopically express TbCen1 in the procyclic-formT. brucei, the TbCen1 gene ORF was amplified using the primersdescribed in Supplementary Table S2 and cloned into pLEW100(Wirtz et al., 1999) in frame with either three concatamerichemagglutinin (HA) tag sequences (Pati, 1992; pLEW100-HA) ora cyan fluorescent protein (CFP; Chudakov et al., 2004) tagsequence (pLEW100-CFP) at the 3'-end. The authenticity of thePCR products was confirmed by DNA sequencing. The constructswere transfected into the T. brucei 29-13 for integration inthe genome as described above (Wirtz et al., 1999). The proteinsoverexpressed by addition of 0.5 µg/ml tetracycline wereanalyzed by Western blot analysis (Selvapandiyan et al., 2001).

Flow Cytometry
Procyclics inoculated at 1 x 10⁵ cells/ml were allowed to growand the cultures were harvested at 0, 3, and 5 d, fixed withparaformaldehyde, stained with propidium iodide (PI), and analyzedby flow cytometry according to the procedure described previously(Tu and Wang, 2004; Raslova et al., 2006). Cells were analyzedfor populations with 2C, 4C, and >4C as a measure of relativeDNA content. The stained cell samples were also examined withan Olympus phase-contrast and fluorescence microscope (Olympus,Melville, NY) to count the number of nuclei and kinetoplastsin individual cells from a population of 200 cells.

Immunofluorescence Analysis
For the immunofluorescence experiments, cells were preparedand analyzed under a fluorescence microscope following the proceduredescribed previously (Kumar and Wang, 2006). Paraformaldehydefixed midlog T. brucei cells were stained with anti-LdCen1 (rabbitpolyclonal antibody [pAb] against L. donovani LdCen1; Selvapandiyanet al., 2001; 1:300 dilution) for staining TbCen1; YL1/2 (ratmAb against yeast tyrosinated- ${alpha}$ -tubulin from Chemicon, Temecula,CA; 1:400 dilution; Kilmartin et al., 1982) for staining thebasal body; L8C4 (anti-paraflagellar rod antibodies from Dr.Keith Gull, Oxford University; 1:4 dilution; Kohl et al., 1999)to stain the flagella; GRASP (pAb against Golgi reassembly stackingprotein from Dr. Graham Warren, Yale University School of medicine;1:500 dilution; He et al., 2004) to stain Golgi; anti-HA-Tag(from Santa Cruz Biotechnology, Santa Cruz, CA, sc-7392; 1:500dilution) to stain ectopically expressed HA-tagged TbCen1 proteins.Appropriate secondary antibodies (anti-rat Alexa Flour 488 A-21208,anti-mouse Alexa Flour 488 A-21422, anti-mouse Alexa Flour 588A-21422, and anti-rabbit Alexa Flour 488 A11008 [GenBank] ; all from MolecularProbes [Invitrogen, Carlsbad, CA]) were used at 1:500 dilutions.

Electron Microscopy
Parasites harvested at appropriate time periods from culturewere prepared and examined by electron microscopy as describedpreviously (Lingle et al., 1998; Lee et al., 2002).

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Sequence Analysis and Nomenclature of T. brucei Centrins
The five putative T. brucei centrin ORF sequences obtained fromGeneDB were compared with the characterized three human, fourmouse, one yeast, and one Chlamydomonas centrin genes by ClustalW(Figure 1A). For comparison we have also included the Leishmaniacentrin counterparts (L. donovani centrin [Selvapandiyan etal., 2001] and five putative L. major centrins [www.genedb.org])in the analysis. Based on the sequence similarity and clustalanalysis, the centrins from L. donovani (AAL01153 [GenBank] ), L. major(LmjF22.1410), and T. brucei (XP_845964 [GenBank] ) that share 97–100%sequence similarity (Supplementary Data: Supplementary TableS3) fall in the same cluster with HsCen1, HsCen2, MmCen1, MmCen2,and CrCen in the phylogenetic tree (Figure 1B) were designatedas LdCen1, LmCen1, and TbCen1, respectively. Centrin1 sequencesfrom the trypanosomatid family are smaller in size, in comparisonto all the other centrins in the eukaryotes, because of a shorterN terminal region (Figure 1A). Similarly, the L. major and T.brucei centrins (LmjF07.0710; XP_824555) that share 71% similaritiesto both HsCen2 and MmCen2 were designated as LmCen2 and TbCen2,respectively. Leishmania centrin (LmjF34.2390) and T. bruceicentrin (XP_825248), which have 67–71% similarity withHsCen3 and MmCen3 and coexist with HsCen3, MmCen3, and CDC31in the phylogeny, were designated as LmCen3 and TbCen3, respectively.Recently, He et al. (2005) named the five centrins of T. bruceibased on their homology to only Chlamydomonas centrin. Accordingto their nomenclature TbCen1 is homologous to human or mousecentrin 3. This nomenclature is at odds with the known nomenclaturefor centrins from different organisms; therefore, in this reportwe have used centrin nomenclature that is consistent with allother organisms, based on the above-mentioned extensive sequenceand phylogenetic analysis. Thus, we referred centrin1 of Heet al. (2005) as TbCen3 in the present study. Both, Leishmaniaand T. brucei centrins 1-3, similar to HsCen1-3, also have EF-handsI and IV as two putative calcium-binding sites predicted bythe motif analysis program (http://molbio.info.nih.gov/molbio/;Figure 1A). The Leishmania and T. brucei centrins (LmjF32.0660;XP_829446 [GenBank] ) with a single putative calcium-binding site (EF-handI) were designated as LmCen4 and TbCen4, respectively, whereas,the Leishmania and T. brucei centrins (LmjF36.6; XP_823096 [GenBank] ),with no predicted calcium-binding site, were designated as LiCen5and TbCen5, respectively (Figure 1B). The mouse has a uniquecentrin MmCen4, which is more closely related to mammalian centrin2and 3 but is expressed exclusively in the basal bodies of theependymal and choroidal ciliated cells (Gavet et al., 2003).However none of the kinetoplastid members have such a centrinhomolog. The use of such a uniform nomenclature will be ultimatelybeneficial in comparing the functions of centrins across differentorganisms.

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Figure 1. (A) Multiple alignment of centrin protein sequences of T. brucei (TbCen), L. donovani (LdCen), L. major (LmCen), Chlamydomonas (CrCen), yeast (CDC31), mouse (MmCen), and human (HsCen). The sequence names with the accession numbers are as follows: TbCen1 (XP_824270), TbCen2 (XP_824555), TbCen3 (XP_825248), TbCen4 (XP_829446), TbCen5 (XP_823096), LdCen1 (AAL01153), LmCen1 (LmjF22.1410), LmCen2 (LmjF07.0710), LmCen3 (LmjF34.2390), LmCen4 (LmjF32.0660), LmCen5 (LmjF36.6), CrCen (P05434), CDC31 (NP-014 900), MmCen1 (NP_031619), MmCen2 (NP_062278), MmCen3 (AAH54097), MmCen4 (CAI26236), HsCen1 (AAH29515), HsCen2 (NP_004335), and HsCen3 (O15182). The accession numbers of T. brucei, L. donovani, Chlamydomonas, yeast, and human are from GenPept data bank. The accession numbers of L. major are from www.genedb.org. The alignment was generated utilizing ClustalW of MacVector 7.2.2 program. Amino acids are listed in the standard one-letter code, and residues identical to TbCen1 are indicated by dashes. The gray boxes (EF-hands I and IV) are the putative Ca²⁺-binding domains. (B) Dendrogram of complete protein sequences of centrins mentioned above were generated in the MacVector 7.2.2 program, utilizing the systematic bootstrap unweighted pair group method with arithmetic mean. The numbers on the nodes indicate the percent of times the respective centrins grouped together in 1000 bootstrap samples in the program.

RNAi-induced Reduction of Specific TbCen1 mRNA
To characterize TbCen1 function for the first time, we knockeddown the mRNA level of this centrin using RNAi methodology inthe procyclic stage of the parasite. Northern blot analysisof RNA obtained from the tetracycline-induced culture on daythree revealed the reduction of the cognate mRNA level (Figure 2A).As a loading control, the membrane was also reprobed with a ${alpha}$ -tubulin gene fragment, and its mRNA level was quantitated.After normalizing the centrin band intensity with the intensityof the ${alpha}$ -tubulin mRNA control, the reduction in the amount ofcentrin mRNAs in the tetracycline-induced culture compared withthe uninduced culture was $~$ 92%. Rehybridizing the membrane withprobes of other centrin genes (TbCen2-5) showed that the mRNAlevels of these genes were not affected. As an additional confirmation,based on the observation that LdCen1 antibody, cross-reactswith TbCen1 (Supplementary Figure S1), we measured the levelof TbCen1 protein in the uninduced and the induced cells. Asignificant reduction in the level of TbCen1 protein was alsoobserved in the induced cells (Figure 2B).

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Figure 2. (A) Northern blots of RNA from induced and uninduced TbCen1 culture. Membrane containing 12 µg total RNA from 3-d uninduced (Un) and induced (I) cells was used. Membrane for TbCen1, in addition to hybridization with either specific centrin DNA or ${alpha}$ -tubulin (Ngo et al., 1998

) probes was reprobed with probes of TbCen2-5 to confirm on the specific inhibition of only the TbCen1 transcript. (B) Western blots on the parasite lysates showing reduction in the protein level of TbCen1 during RNAi induction by anti-LdCen1 Ab (top) and the loading control showing the level of ${alpha}$ -tubulin by anti-tubulin Ab (bottom). Un, uninduced; In, induced. In each lane 20 µg of total extracted proteins were loaded. (C) The effect of TbCen1 knockdown on the in vitro growth of T. brucei procyclics. The cells were grown with (I) or without (Un) tetracycline. The data represent the means of ± SD of three independent experiments. *p < 0.04. (D) Geimsa-stained images of the control and TbCen1-depleted cells, 4 d after RNAi induction. Scale bar for both images, 5 µm. AF, attached flagella; DF, detached flagella.

TbCen1 Is Essential for the Growth of the Parasite
The effect of reduction in TbCen1 level on the growth of theTbCen1 RNAi cells was monitored by counting cell number dailyfor 6 d after RNAi induction (Figure 2C). The tetracycline-inducedparasites started showing the growth defect on day 3 comparedwith uninduced control cells. Cell density on day 5 was 11%of the control for TbCen1-depleted cells. There was no increasein the cell numbers of the RNAi-induced TbCen1 parasites afterday 5, whereas the uninduced culture continued to grow throughoutthe experiment. Thus, TbCen1 RNAi-expressing cells showed areduced growth rate after induction compared with the uninducedcells. Geimsa-stained TbCen1-depleted cells at day 4 in culture,under microscope, showed that the cells were large, pleomorphicin shape and had multidetached flagella, unlike the uninducedcells that were uniform in shape with one or two attached flagellum,depending on the cell cycle stage (Figure 2D and see Figure 9).

TbCen1 Depletion Arrests Cytokinesis Resulting in Large Cells with Multiple Organelles
To determine the cause of growth arrest, the RNAi-induced TbCen1cells along with uninduced cells as control were stained withPI and subjected to flow cytometry to analyze for relative DNAcontent (C) at different time intervals in culture (Figure 3A).The percent of cells having 2C, 4C, and >4C were calculatedand the data are shown in Figure 3B. The analysis revealed thatthe TbCen1 RNAi cultures displayed gradual increase in the numberof cells with >4C (Figure 3, A and B). Approximately 15%of TbCen1 RNAi-induced cells had >4C at day 3 compared with3% of the cells at day 0 and the percentage of >4C cellsincreased to up to 45% at day 5 (Figure 3B). The increase inthe >4C cell population coincided with the simultaneous decreasein 2C cells with progression of TbCen1 depletion (Figure 3,A and B). In Figure 3A the 5-d time point the far left-handedge of the figure shows cells having less than 2C, which usuallyrepresent dying cells, as was observed previously in LdCen1-depletedL. donovani amastigotes (Selvapandiyan et al., 2004).

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Figure 3. Fluorescence-activated cell sorting analysis for relative DNA content of TbCen1-depleted cells. The percentage of cells that contain two times the DNA content (2C), four times (4C), and more than 4 times (>4C) were measured at each time point and are shown. (A) The corresponding cell frequency units obtained directly from the flow cytometry analysis are shown. (B) Histograms with the quantitated values of the cell populations are shown. Data represent the means of ± SD of three independent experiments.

As a first step to analyze the organization of various organellesof both control and TbCen1-depleted cells, the cells at day4 after induction were stained with DAPI to identify the nucleiand kinetoplasts and with L8C4 antibody (antibodies to paraflagellarrod, which is a complex lattice-like structure running alongsidethe axoneme in the flagellum of T. brucei; Bastin et al., 1998

)to visualize the flagella. The stained cells were observed undera fluorescence microscope for organelle position. The majorityof the uninduced or wild-type cells showed a single kinetoplast(the mitochondrial genome), a single nucleus with one flagellum(Figure 4A, top). However, TbCen1-depleted cells have multinuclei,multikinetoplasts, and multiflagella in each cell (Figure 4A,bottom). Such cells were also large and highly pleomorphic (Figure 4A,bottom), as opposed to the control cells that were small andtwisted (Figure 4A, top). With such large cells, we noticedmultiple detached flagella along with the attached flagellum(Figure 4A, bottom). We presume that such an attached flagellumcould be the initial flagellum of the cells before the inductionof RNAi. To monitor the progression of organelle replication,we counted the number of nuclei, kinetoplasts, basal bodies,Golgi, and flagella in centrin-depleted cells until day 4 afterinduction. A gradual increase in the number of cells with multiplenuclei and multiple kinetoplasts (>2K2N) was observed fromday 3 onward in the centrin-depleted cultures, coupled witha concomitant decrease in cells with one nucleus and one kinetoplast(1K1N; Figure 4C). We also observed cells with two kinetoplastsand one nucleus (2K1N), two kinetoplasts and two nuclei (2K2N),one kinetoplast and no nucleus (1K0N: zoid) and one kinetoplastand two nuclei (1K2N) as intermediate populations before finallythe majority (>70%) of them on day 4 became >2K2N cells(Figure 4C).

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Figure 4. (A and B) Microscopic images of control and TbCen1-depleted procyclic cells from day 4 cultures. In each cell, DAPI stained kinetoplasts (K) and nuclei (N), the L8C4 stained flagella (F), YL1/2 stained basal bodies (B), and GRASP stained Golgi (G). AF, attached flagellum; DF, detached flagellum. All the images are the same scale (scale bars, 5 µm). (C) Bar graph showing increase in the proportion of multinucleated and multikinetoplast cells with days after RNAi knockdown of TbCen1. Cells after different days of TbCen1 RNAi induction were stained with PI and examined by fluorescence microscope for tabulation of the cells with different number of kinetoplasts (K) and nuclei (N). (D) Percentage of TbCen1-depleted cells with multiflagella. Cells after different days of TbCen1 RNAi induction were observed under microscope under bright field, and the cells that contained more than two flagella were counted. For both B and C at least 250 total cells were observed for the quantitation at each time point. The data represent the means of ± SD of three independent experiments. (E and F) Percent of cells on day 3 and 4, which show varying number of basal bodies (E) and Golgi (F). The data only shows the number of mature basal bodies that were stained with YL1/2 Ab and were easily visible than the probasal bodies and GRASP that stains the Golgi as in B. In each case more than 125 cells were analyzed.

We also observed that the TbCen1-depleted cells in culture continueto grow in size, with continuous replication of kinetoplastsand nuclei until the nutrients are depleted in the medium (Figures 2Dand 4C). Because the TbCen1 RNAi cells have multiflagella, wequantitated them in a separate analysis. Almost 60% of the TbCen1-depletedcells on day 4 had more than two flagella (Figure 4D). Previously,we had observed that knockdown of LdCen1 expression in L. donovaniamastigotes affected basal body duplication. Further, coordinatedbiogenesis of basal body and Golgi has been recently shown inT. brucei (Field et al., 2000

; He et al., 2004

). To determinethe fate of basal bodies and Golgi in the TbCen1-depleted T.brucei cells, an immunofluorescence analysis was conducted onsuch cells using YL1/2 antibody that stains the basal bodiesand GRASP antibody that stains the Golgi. Most of the uninducedcells show a pair of basal bodies and single Golgi (Figure 4B,top). However, majority of TbCen1-depleted cells displayed multibasalbodies and multi-Golgi (Figure 4B, bottom). Careful quantificationof the basal body and Golgi number in the centrin-depleted cellson day 3 and 4 revealed the existence of cells with one, two,or more than two mature basal bodies and Golgi. Approximately60% of cells with more than two basal bodies and Golgi on day4 after RNAi induction were observed with concomitant decreasein the cells with two basal bodies and two Golgi (Figure 4,E and F).

To further confirm the abnormal morphological characteristicsof TbCen1-depleted cells, we examined such cells by electronmicroscopy (EM). The features of multibasal bodies, multikinetoplasts,multiflagella, and multinuclei observed in the TbCen1-depletedcells by immunofluorescence microscopy were confirmed by theEM studies (Figure 5, B–D). The uninduced cells mostlyhad a single nucleus, kinetoplast and basal body (Figure 5A).In a limited number of observations the EM morphology of theflagellar pocket in the TbCen1-depleted cells appears to benormal (Figure 5E). Although the newly formed flagella are detachedtype in TbCen1 RNAi cells (Figure 6A), the 9 + 2 arrangementof the microtubules of the axoneme and paraflagellar rod (Bastinet al., 2000) is not affected (Figure 5F) and appears similarto the attached flagellum (Figure 5G). All these observationsclearly demonstrate the failure of cell division in the TbCen1-depletedT. brucei cells, which resulted in increase in number of thecellular organelles with concomitant increase in cell size.

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Figure 5. Electron microscopy of centrin-depleted cells. (a) A nondividing control cell shows single flagellum, basal body, and kinetoplast. (b–d) TbCen1-depleted cells with multinuclei, multibasal bodies, and multikinetoplasts are sequentially displayed in images. Inset in d is more representation of divided kinetoplasts. (e) Similar cell showing the unaffected flagellar pocket with the old attached flagellum and a cross section of a newly formed detached flagellum. (f) The cross section of detached flagella from TbCen1-depleted cells showing the paraflagellar rod and the unaffected 9 + 2 microtubule structure in the flagellar axoneme (inset). (g) The cross section of an attached flagellum of a centrin-depleted cell showing the typical regions of paraflagellar rod and the axoneme that shows the 9 + 2 arrangement of microtubules. F, flagellum; P, flagellar pocket; B, basal body; K, kinetoplast; N, nucleus; R, paraflagellar rod; A, axoneme. Cells in all experiments were from 5 d after RNAi induction, except in d, where the inset of f and g are from 2 d after RNAi induction. Scale bars, (a and c–f) 500 nm; (b), 2 µm; and (g) 250 nm.

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Figure 6. Effect on the attachment of the newly formed flagella in the TbCen1 RNAi cells. (A) DAPI-stained cells; (B) Geimsa-stained cells. More than 40 cells were used for the analysis. AF, attached flagella; DF, detached flagella; K, kinetoplast; N, nucleus. Scale bars, 5 µm.

TbCen1 Depletion Affects Flagellar Attachment
Centrin-depleted cells showed newly formed flagella that wereof detached type although the original flagellum in such cellswas still seen as attached (Figure 2D). To find out whetherthe detachment of the flagella in the centrin RNAi cells iseither a primary or a secondary effect of centrin depletion,we analyzed cells at early stages of RNAi induction. Carefulobservation of 2K2N cells on day 2 of RNAi induction revealedthat the very first new flagella of more than 90% of such cells,where the kinetoplasts did not segregate, showed detached flagellumin addition to the old attached flagellum (Figure 6A, top, andB, right). Similarly in 4K2N centrin RNAi cells, we observedthree new detached flagella (Figure 6A, bottom). These resultssuggest that flagellar detachment is an early event in the TbCen1-depletedcells and occurs concomitantly with the failure of segregationof basal-bodies, flagellum, and kinetoplast.

TbCen1 Is Associated with the Basal Bodies
To ascertain the localization of TbCen1 in T. brucei, we carriedout immunofluorescence analysis. Using anti-LdCen1 Ab (Selvapandiyanet al., 2001), which cross-reacts specifically to TbCen1 proteinin a Western blot analysis (Supplementary Figure S1), we noticedstaining at the basal body region (Figure 7A). However, in additionto the basal body, the anti-LdCen1 Ab also stained an additionalarea (a bilobed structure) next to the basal body. To confirmthat the localization of TbCen1 in the bilobed structure wasnot an aberrant observation, we ectopically expressed 1) TbCen1fused with an HA tag (TbCen1-HA) using a pLEW100-HA vector and2) TbCen1 fused with CFP using a pLEW100-CFP vector in the parasite.The parasites that express either TbCen1-HA or TbCen1-CFP showednormal growth compared with control cells, and the expressionof both the fusion proteins was observed in over 90% of thecells using immunofluorescence analysis (data not shown). Theanti-HA Ab-stained TbCen1 at both the basal body and the bilobedstructure (Figure 7B). The fluorescent TbCen1-CFP also similarlylocalized at the basal body and the bilobed structure (Figure 7C).The TbCen1-CFP localization was monitored in the live cellsby fluorescence microscope. Using three different immunolocalizationapproaches for TbCen1 clearly suggesting that TbCen1 localizesboth in the basal body region and to a bilobed structure. Inaddition, it also suggests that TbCen1 localization to bilobedstructure is not due to overexpression of the protein becausesuch localization was found in nonoverexpressing cells (Figure 7A).Previously, it was reported that TbCen2 is also localized tothe both basal body and a bilobed structure that is in closeproximity with the Golgi apparatus (He et al., 2005). Usingboth GRASP, an antibody that stains Golgi, and anti-HA Ab, whichlocalizes TbCen1, we confirmed that the bilobed structure isalso in close proximity to Golgi in the transfected T. bruceicells (Figure 7D). However, the reason for the localizationof TbCen1 (in this study) and TbCen2 (in He et al., 2005) atthe bilobed structure along with basal body and its relevanceto the function of these proteins is not known at this time.

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Figure 7. (A) Immunolocalization of TbCen1 in the procyclics of T. brucei 29-13 using anti-LdCen1 Ab (stains LdCen1 at the basal body in L. donovani (Selvapandiyan et al., 2004

) stains here the basal body and the bilobe. (B) Localization of TbCen1-HA proteins in T. brucei 29-13 procyclic cells transformed with pLEW100-TbCen1. Staining with anti-HA Ab stains the basal body and the bilobe, and YL1/2 stains the basal body. (C) Fluorescent images of a live T. brucei cell ectopically expressing TbCen-CFP are stained with cyan, and kinetoplast was stained with SYTO Green-Fluorescent Nucleic Acid Stain (Molecular Probes, Invitrogen). (D) Localization of TbCen1 with respect to Golgi. Cells were stained with GRASP to stain the Golgi and anti-HA Ab to stain TbCen1-HA at the basal body and the bilobe. In all, the parasites obtained were from midlog culture and also stained with DAPI for the nuclei and the kinetoplasts. K, kinetoplast; N, nucleus; B, basal body; G, Golgi; L, bilobe. Scale bar in all, 5 µm.

TbCen1 Is Involved in Segregation of Organelles Necessary for Completion of Cytokinesis
Previously we showed that disruption of a L. donovani centrin(LdCen1) affected basal body duplication, which in turn affectedcytokinesis in the amastigote form of L. donovani (Selvapandiyanet al., 2004

). In this study we explored the effect of TbCen1depletion on the basal body duplication and segregation, alongwith the segregation of other organelles, such as kinetoplasts,nuclei, and Golgi in the procyclic form of TbCen1-depleted cells.Immunofluorescence analysis was carried out using YL1/2 andGRASP antibodies for identifying basal bodies and Golgi, respectively.Control cells displayed a normal segregation pattern of theduplicated basal bodies and the divided kinetoplasts (Figure 8A,magnified portion in 8A and 8B, and Figure 9A), which is a prerequisitefor the initiation of cytokinesis (Robinson and Gull, 1991

).Careful observation of TbCen1 RNAi cells revealed the absenceof segregation of the duplicated basal bodies and kinetoplastcomplex (Figures 8, C and D, and 9B). The magnified portionin Figure 8C shows the basal bodies that have gone through asecond round of duplication without segregation. High-resolutionEM of TbCen1-depleted cells also showed multiple number of basalbodies and kinetoplasts grouped in one area (Figure 5, c andd). Basal-body migration pattern in the normal T. brucei cellswas described previously (Robinson et al., 1995

). On the basisof that study we have measured the migration of basal bodiesin TbCen1 RNAi cells at the two-nucleated stage. At day 3 afterRNAi induction the quantitation revealed that $~$ 75% of the cellscontained the basal bodies that were close to each other andnot separated as in the uninduced cells (Figure 8E). The twonucleated cells with multiple nonseparated basal bodies continuedto increase from day 3 to day 4. These results clearly indicatea defect in basal body segregation after centrin depletion.Using a Golgi-specific antibody, GRASP, we found normal duplicationof Golgi similar to other organelles in the TbCen1-depletedcells (Figure 8, F and G). We have also noticed more than onenew Golgi structures stained with GRASP in both the control(data not shown) and the centrin-depleted cells (Figure 8G markedas g), as observed by He et al. (2004)

during the normal T.brucei cell cycle. However, in TbCen1-depleted cells, therewas an abnormal segregation of Golgi as was observed with otherorganelles in such cells compared with control (Figure 8, Fand G). In conclusion, depletion of TbCen1 did not affect organelleduplication but interfered with their segregation.

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Figure 8. Effects on the duplication and segregation of basal bodies, kinetoplasts, Golgi, and nuclei in TbCen1-depleted cells. The cells were stained with DAPI for nuclei and kinetoplasts, GRASP for Golgi, and YL1/2 for basal bodies. (A–D) In A and C the separate enlarged areas at right show the number and position of the duplicated basal bodies and the divided kinetoplasts. Note that the divided basal bodies and the kinetoplasts in image C are not as well separated compared with the cell in B. (E) Histogram showing the percent of TbCen1 RNAi cells with two basal bodies that are either normal or defective in their separation were analyzed on days 3 and 4. The images show the type of the cells used in the analysis. Note the cells that show basal bodies defective in separation have already two nuclei in them. More than 40 cells were used for the analysis. (F and G) Effects on the duplication and segregation of the Golgi in TbCen1-depleted parasite (G) compared with control (F). Note that the divided two Golgi in image G are not as well separated as the two Golgi seen in the F. The time point at which the cells analyzed after induction was day 2 for A–C and F and day 3 for D and I. B, basal body; K, kinetoplast; G, Golgi; N, nucleus; g, additional Golgi structures as described (He et al., 2004

). Scale bars, 5 µm.

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Figure 9. Schematic diagram of the segregation of the organelles and its failure in the absence of TbCen1 in T. brucei procyclic form. (A) Normal cell division. (B) The arrest of organelle segregation and cytokinesis upon depletion of TbCen1.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Trypanosomatids Have Unique Centrin Genes
Eukaryotic cells are reported to have a varying numbers of centringenes, for example, one in Chlamydomonas and yeast, three inhumans, and four in mice (Wolfrum and Salisbury, 1998

; Gavetet al., 2003

). The genomic sequences of T. brucei and Leishmaniareveal the presence of five putative centrins in their genome.The protein sequence homology among the five genes within trypanosomatidsis very low (35–54% similarity). However, each gene displayssignificant similarity to its homologue among other speciesof trypanosomatids, suggesting diversification of this centrinfamily early in evolution. All five genes in trypanosomatidshave variable amino-terminal extensions. The amino-terminalregions are thought to confer functional diversity to centrins(Salisbury, 1995

; Wiech et al., 1996

). Shorter amino-terminalextension seen either in TbCen1, LdCen1, or LmCen1, seems uniqueto the Trypanosomatid family among the eukaryotes. Similarly,TbCen4 (and its Leishmania counterpart), which has one putativecalcium-binding site, and TbCen5, which has no putative calcium-bindingsite, branched off early in the phylogenetic tree from a commoncentrin ancestor, are unique to this family. Further in thephylogenetic analysis the centrins that possess two putativecalcium-binding sites branch into two clusters. One clustercomprises all the centrins 1 and 2 and MmCen4. The other clusterincludes all the centrins 3 and CdC31. These observations suggestthat the unique structure of each of centrin gene might playdifferent functional roles. Therefore, further characterizationof each T. brucei centrin is important for understanding trypanosomebiology.

Localization of T. brucei TbCen1
Centrins have been localized to the basal-body region in theflagellated eukaryotes, such as Chlamydomonas (CrCen; Salisbury,1995), Leishmania (LdCen1; Selvapandiyan et al., 2001), Paramecium(PtCen2 and 3; Ruiz et al., 2005), and T. brucei (TbCen2; Heet al., 2005). We have similarly found that TbCen1 is localizedto the basal body region of T. brucei. In addition, we observedTbCen1 is also localized at a bilobed structure close to theGolgi. The additional localization of Tbcen1 to a bilobed structurein close proximity to the Golgi has also been observed withTbCen2 but not for TbCen3 (He et al., 2005). At present littleis known about the localization of TbCen4 and TbCen5. The functionalsignificance of some of the T. brucei centrins localizing atthe bilobed structure in addition to the basal body is not knownand needs further investigation.

TbCen1 Depletion Leads to Pleomorphic Cell Shape and Detached Flagella
The pleomorphic shape observed in LdCen1 deleted Leishmania(Selvapandiyan et al., 2004) and TbCen1-depleted T. brucei inthe current study has also been observed in S. cerevisiae. Forexample, mutations in yeast centrin (CdC31p) have generatedcells defective in spindle pole body biogenesis with large-buddedcell morphology (Sullivan et al., 1998; Ivanovska and Rose,2001). Other structural proteins besides centrin have also beenshown to be important for the cell morphology of T. brucei.For example, depletion of a flagellar adhesion protein (Fla1)seen at the flagellum attachment zone (LaCount et al., 2002)or the cytoskeletal protein ${alpha}$ -tubulin (Ngo et al., 1998) causesparasites to lose their shape because of failure in cell division.Whether the loss of shape in the centrin-depleted protozoanparasites (Leishmania and T. brucei) is a direct effect fromloss of centrin or an indirect effect due to the uncontrolledenlargement of cell size needs to be further examined.

TbCen1-depleted T. brucei cells also displayed detached flagellain addition to the original attached flagellum. A similar phenotypewas observed in Fla1 deficient T. brucei cells (LaCount et al.,2002). However, in the present study, the Fla1 level was unaffectedin the TbCen1-depleted cells with detached flagellum (SupplementaryFigure S2). Because Fla1 is apparently not affected in TbCen1-depletedT. brucei cells and TbCen1 is not localized between flagellumand flagellum attachment zone (FAZ) like Fla1 (LaCount et al.,2002), the flagellar detachment due to TbCen1 depletion couldbe an indirect effect. However, it has been shown that the FAZfilament originates close to basal body area and occurs aroundthe time, when the probasal body matures and new axoneme extendsand is essential in determining the process of cytokinesis inT. brucei (Kohl et al., 1999; LaCount et al., 2002). In thepresent study depletion of TbCen1 in T. brucei resulted in thedetachment of new flagellum at an early stage (day 2 after RNAiinduction) of failure in segregation of the basal body suggestingthe role of centrin in flagellum attachment and its requirementin cytokinesis. Role of flagellum in basal body and kinetoplastsegregation has also been previously demonstrated by eitheraltering the expression of intraflagellar transport proteinsresulting in either short or lost flagella (Kohl et al., 2003)or by ablation of axonemal proteins which alter flagellar mobility(Dawe et al., 2005).

It is also known that the centrin associated centrosome/basalbody regulates the number, spatial arrangement, and stabilityof microtubules responsible for cell polarity and shape in othereukaryotes (Lingle and Salisbury, 1999). The flagellum's positionand polarity along with the subpellicular cytoskeleton enablesthe morphogenesis of the distinct flagellar pocket (Gull, 2003).However in our limited EM studies to analyze flagellar pocketmorphology, we were not able to conclusively determine whetherTbCen1 depletion had any effect on the overall structure ofthe flagellar pocket in such cells.

TbCen1 Is Involved in Organelle Segregation
TbCen1 depletion by RNAi revealed that it is important for thegrowth of T. brucei procyclic form. The parasites depleted forTbCen1 stopped dividing and the cells became enlarged and highlypleomorphic with multiple detached flagella. Such parasiteshad multiple basal bodies, kinetoplasts, Golgi, and nuclei,suggesting that there was no effect on organelle multiplicationbut a defect in cytokinesis. The fate of large cells eventuallyled to cell death, as indicated by the increased number of cellswith less than 2C DNA content. Similar phenomenon was observedin L. donovani centrin disrupted amastigotes (Selvapandiyanet al., 2004).

Organelles like the flagellum, basal bodies, mitochondrion,Golgi, and nucleus must duplicate and segregate during eachcell division in the protozoan parasite (Robinson et al., 1995;Gull, 1999). The sequence of events that occur during cell divisionin the procyclic form of T. brucei are maturation and duplicationof the basal bodies, division of kinetoplast and nucleus, assemblyand emergence of a new flagellum followed by segregation ofthe linked organelles (flagellum, basal bodies, and kinetoplast),a prerequisite for cytokinesis (Robinson et al., 1995; Kohland Gull, 1998; Gull, 1999), and are depicted in Figure 9. Inthe centrin-depleted T. brucei cells, we have observed no effecton the multiplication of the linked-organelles, as indicatedby a majority of cells ( $~$ 80%) with multikinetoplasts and multinuclei(>2K2N) on day 4, but a significant defect in their segregationleading to loss of cytokinesis. Interestingly, we have noticeda significant population (40%) of cells with 1K2N only at day3 and not at day 4. The increase in the cell population withonly single kinetoplast (in 1K2N) observed by DAPI is most probablydue to a lack of enough segregation of the divided kinetoplastsat day 3 because DAPI staining is not sufficiently sensitiveto distinguish a single kinetoplast from a duplicated kinetoplast.However, at day 4 cells the duplicated kinetoplasts are separatedenough to be counted as >2K2N (Figure 4C). A similar increasein the 1K2N population was observed because of the failure ofnuclear segregation, leading to both the nuclei remaining inone daughter cell and leaving the second daughter cell withone kinetoplasts and no nucleus (1K0N; Ploubidou et al., 1999).However, we did not observe an increase in 1K0N population inTbCen1-depleted cells. Our observation that the divided kinetoplastsoften staying close together without separation in the TbCen1-depletedcells was further substantiated by the EM analysis in Figure 5D.Therefore, the increase in number of cells with multibasal bodies,multiflagella, and multi-Golgi as the RNAi induction proceedsreinforces the idea that there is no defect in the duplicationof these organelles after depletion of TbCen1.

A coordination in the biogenesis of Golgi and basal bodies hasbeen previously suggested (Field et al., 2000; He et al., 2004).For example, in T. brucei, duplication of the basal bodies wasfollowed by the formation of a new Golgi near to the new basalbody. An inhibition of the separation of the basal bodies andkinetoplasts by anistomicin-p, which inhibits the microtubulemorphogenesis, also inhibited separation of the old and newGolgi in T. brucei (He et al., 2004). From the above-mentionedobservations it is apparent that segregation of various organellesis interdependent and the basal body plays a control role inthis process. Further, the failure of segregation that we observedwith both the duplicated basal bodies and kinetoplasts soonafter the induction of RNAi is probably the cause of the defectin the initiation of cytokinesis. Involvement of centrins inthe segregation of basal bodies/centrosome is known in human,mouse, Chlamydomonas, and Paramecium (Middendorp et al., 1997;Koblenz et al., 2003; Ruiz et al., 2005). However, in the presentstudy the role of TbCen1 in the segregation of other organelles(kinetoplast and Golgi) besides basal body has been demonstratedin T. brucei. Hence from our studies the localization of TbCen1to the basal body and its depletion affecting the segregationof all the associated organelles suggest the importance of thisprotein in the completion of cell cycle in T. brucei.

We observed that nuclear division occurs despite arrest in cytokinesisin centrin-depleted T. brucei cells. This confirms previousobservations by others that nuclear division and cell divisionin both T. brucei and Leishmania are not linked processes (Ploubidouet al., 1999; Selvapandiyan et al., 2004; Kumar and Wang, 2006).It is known that the nuclear division in Trypanosomes is dueto the spindles that are intranuclear in origin and not dueto the basal body nucleating microtubules (Ogbadoyi et al.,2000). The divided nuclei, which were not repositioned in theTbCen1-depleted cells as they were in the uninduced controlcells but remained as a cluster in the centrin-depleted cells,suggest that the repositioning of the divided nuclei might requirea distinct unknown mechanism that needs the presence of TbCen1.

It has been shown that the position of the spindle pole body(basal body counterpart in yeast) after segregation determinesthe division cleavage plane and cytokinesis (Hoyt, 2000). Postanaphaserepositioning of the centrosome in HeLa cells controls the releaseof central microtubules from the midbody and the completionof cell division (Piel et al., 2001). The involvement of thespindle pole body nucleating microtubules in the nuclear migrationand repositioning needed for cell division in Aspergillus nidulanshas been also shown (Oakley et al., 1990; Xiang and Fischer,2004). Centrin depletion in Chlamydomonas cells resulted inaberrant numbers of basal bodies, which disturbed the microtubularcytoskeleton independent of the mitotic spindle and arrestedcytokinesis (Koblenz et al., 2003). In addition, a precedentfor centrin-associated fibers interacting with microtubuleshas been established in Chlamydomonas (Sanders and Salisbury,1989, 1994). These studies describe the association betweencentrin and microtubules and may explain the observed failurein organelle segregation in the T. brucei centrin-depleted cells.Therefore, in the future studies, it will be of interest todetermine the effect on microtubule assembly in the absenceof centrin and its effect on trypanosomatid organelle segregation.

Differential Function of Centrins in Trypanosomatids
TbCen1-depleted cells showed continued duplication of basalbodies and kinetoplasts in the absence of cytokinesis, whereas,the TbCen2- and 3-depleted cells showed defects both in theduplication of basal bodies and kinetoplast (He et al., 2005).In the L. donovani amastigote form, another member of the trypanosomatidfamily, there is a failure in the duplication of basal bodieswithout affecting kinetoplast division in the absence of LdCen1(Selvapandiyan et al., 2004). There are additional differencesbetween T. brucei and L. donovani. For example, the knockoutfor LdCen1 in L. donovani only affected the growth of amastigotestage parasites and not the in vitro growth of the insect formpromastigote (Selvapandiyan et al., 2004), whereas, in T. bruceiwe see a distinct change in the phenotype of the insect stageprocyclic form upon depletion of centrins. At this time thefunction of centrins in the bloodstream form of T. brucei isnot known. It is possible that the differences in function amongcentrins in trypanosomatids could be due to structural differences.The variable amino-terminus, which is thought to confer functionaldiversity to centrins (Salisbury, 1995; Wiech et al., 1996),may be involved in the functional differences. Therefore, itwill be of interest to find how differences in centrins amongT. brucei and Leishmania, which cause various diseases, resultin the functional differences.

The results in this study indicate that the primary event thatoccurs in the absence of TbCen1 could be the failure of thesegregation of the linked organelles (basal bodies, flagellum,kinetoplasts, and Golgi). The detachment of new flagella, arrestin cytokinesis, and the enlargement of cell size due to repeatedorganelle multiplication could be the associated events andmay be occurring simultaneously. In conclusion, the presentstudy describes a novel function for TbCen1, which is the involvementin the spatial positioning of multiple organelles that is requiredfor the initiation of cytokinesis in T. brucei. Such a centrinfunction may be unique in T. brucei among the eukaryotes, probablydue to a primitive centrin-dependent mechanism of coordinationin the biogenesis of the organelles seen in this evolutionarilyancient protozoan parasite.

ACKNOWLEDGMENTS

We acknowledge Paul T. Englund (Johns Hopkins School of Medicine,Baltimore, MD) for providing plasmid vector pZJM; and GeorgeA.M. Cross (The Rockefeller University, New York, NY), GrahamWarren (Yale University School of Medicine, New Haven, CT),and Keith Gull (University of Oxford, Oxford, United Kingdom)for providing anti-flagellum adhesion protein (Fla1), anti-Golgireassembly stacking protein (GRASP), and anti-paraflagellarrod (L8C4) antibodies, respectively. We also acknowledge RobertDuncan and Alain Debrabant (Division of Emerging and Transfusionand Transmitted Diseases, Center for Biologics Evaluation andResearch, Food and Drug Administration, Bethesda, MD) for criticalreading of the manuscript.

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E07-01-0022)on June 13, 2007.

The online version of thisarticle contains supplemental material at MBC Online (http://www.molbiolcell.org).

These authors contributed equally to this work.

Address correspondence to: Hira L. Nakhasi (hira.nakhasi{at}fda.hhs.gov) or Angamuthu Selvapandiyan (angamuthu.selvapandiyan{at}fda.hhs.gov).

Abbreviations used: HA, hemagglutinin; DAPI, 4'6-diamidino-2-phenylindole; ORF, open reading frame; pAb, polyclonal antibodies; EM, electron microscopy.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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