Centrin Is Necessary for the Formation of the Motile Apparatus in Spermatids of Marsilea

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Vol. 12, Issue 3, 761-776, March 2001

Centrin Is Necessary for the Formation of the Motile Apparatus in Spermatids of Marsilea

Vincent P. Klink, and Stephen M. Wolniak^*

Department of Cell Biology and Molecular Genetics, University of Maryland, College Park, Maryland 20742

Submitted June 12, 2000; Revised November 29, 2000; Accepted January 17, 2001
Monitoring Editor: Tim Stearns

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

During spermiogenesis in the water fern, Marsilea vestita, basal bodies are synthesized de novo in cells that lack preexistingcentrioles, in a particle known as a blepharoplast. We have focusedon basal body assembly in this organism, asking what componentsare required for blepharoplast formation. Spermiogenesis is arapid process that is activated by placing dry microspores intowater. Dry microspores contain large quantities of stored proteinand stored mRNA, and inhibitors reveal that certain proteins aretranslated from stored transcripts at specific times during development.Centrin translation accompanies blepharoplast appearance, while $beta$ -tubulin translation occurs later, during axonemal formation.In asking whether centrin is an essential component of the blepharoplast,we used antisense, sense, and double-stranded RNA probes madefrom the Marsilea centrin cDNA, MvCen1, to block centrin translation.We employed a novel method to introduce these RNAs directly intothe cells. Antisense and sense both arrest spermiogenesis whenblepharoplasts should appear, and dsRNA made from the same cDNAis an effective inhibitor at concentrations at least 10 timeslower than either of the single-stranded RNA used in these experiments.Blepharoplasts are undetectable and basal bodies fail to form.Antisense, sense, and dsRNA probes made from Marsilea $beta$ -tubulinpermitted normal development until axonemes form. In controls,antisense, sense, and dsRNA, made from a segment of HIV, had noeffect on spermiogenesis. Immunoblots suggest that translationalblocks induced by centrin-based RNA are gene specific and concentrationdependent, since neither $beta$ -tubulin- nor HIV-derived RNAs affectscentrin translation. The disruption of centrin translation affectsmicrotubule distributions in spermatids, since centrin appearsto control formation of the cytoskeleton and motile apparatus.These results show that centrin plays an essential role in theformation of a motile apparatus during spermiogenesis of M. vestita.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Throughout most of the eukaryotic realm, the formation of male gametes involves the synthesis and assembly of a motile apparatus.The motile apparatus comprises flagellar or ciliary axonemes,whose rapid beat frequency and precise beat shape are the consequenceof mechanochemical interactions between scores of proteins thatare arranged in a remarkably complex cylindrical array (Dutcher,1995). A controlling template for axonemal formation is the basalbody (Mizukami and Gall, 1966), which resides in the corticalcytoplasm at the base of the axoneme (Ringo, 1967; Fulton, 1971;Dibbayawan et al., 1995). Basal bodies closely resemble centrioles(Gould, 1975; Kuriyama and Borisy, 1981; Kochanski and Borisy,1990), and they are usually formed from or in close associationwith centrioles (Dirksen, 1991;Marshall and Rosenbaum, 2000),(however, see Fulton [1971]; Fulton and Dingle [1971]; Gould [1975]).The ubiquity of this association has led to the perception thatall basal bodies arise from these cytoplasmic organelles. Abouta century ago, however, lower plants were shown to produce motilemale gametes, in a process that involved the formation of basalbodies in cells that lacked preexisting centrioles (Webber, 1897,1901; Chamberlain, 1898; Sharp, 1914; Duckett, 1973; Hepler, 1976;Vaughn and Harper, 1998).

In the developing spermatids of lower plants, basal bodies form in a particle that was originally called the blepharoplast(Webber, 1897, 1901) because as the spermatids matured, it lookedlike an eyelash. Ultrastructural analyses reveal that, as a discretespherical particle in the cytosol, the blepharoplast is the precursorfor basal body assembly (Mizukami and Gall, 1966;Hepler, 1976;Doonanet al., 1986;Vaughn et al., 1993), and the elongated "eyelash"is actually a cytoskeletal array now known as a multilayered structure,or MLS (Carothers, 1975; Myles and Hepler, 1977; Duckett, 1973;Marc and Gunning, 1986, 1988; Hoffman and Vaughn, 1995; Wolniaket al., 2000; Klink and Wolniak, 2000), which is common to allplant spermatozoids. The uppermost stratum of the MLS is a ribbonof cross-linked microtubules that appears to control patternsof cell and nuclear elongation (Myles and Hepler, 1977, 1982)in the developing spermatid and is attached to the basal bodiesof the motile apparatus (Carothers, 1975; Hoffman and Vaughn,1995).

Recently, we have focused on blepharoplast formation and de novo basal body assembly in the male gametophytes of the waterfern, Marsilea vestita. In this organism, microspores, which aremeiotic products, are stored as dry structures that germinatewhen they are placed into an aqueous medium. The pattern of developmentin these male gametophytes is precise and synchronous; the entireprocess reaches completion in an 11-h period at 20°C (Mizukamiand Gall, 1966; Hepler, 1976). During the 1st 5.5 h after imbibition,there are 9 mitotic divisions that produce 39 cells, all containedwithin the original microspore wall (Sharp, 1914). One cell isa prothallial remnant, 6 of the cells are sterile jacket cells,and the remaining 32 cells are spermatids (Sharp, 1914, Hepler,1976, Pennell et al., 1986, 1988). During the next 5.5 h afterimbibition, the spermatids differentiate to become freely swimming,ciliated gametes (Myles and Hepler, 1977).

In our previous studies, we (Hart and Wolniak, 1998, 1999) extended earlier work (Hyams et al., 1983; Pennell et al., 1986,1988) that focused on patterns of transcription and translationin the gametophyte that are necessary for spermiogenesis. We showedthat dry microspores contain substantial quantities of storedproteins, like $alpha$ -, $beta$ - and $gamma$ -tubulin, and that spermiogenesis requiresthe translation of some new proteins from stored mRNA, such ascentrin (Hart and Wolniak, 1998). In the male gametophyte of M.vestita, significant quantities of centrin protein first beginto accumulate from the translation of stored mRNA, ~4 h afterthe spores are imbibed. In contrast, the translation of additional $beta$ -tubulin occurs > 8 h after imbibition, and appears necessaryfor axonemal formation, late in spermiogenesis (Hart and Wolniak,1998). Most new centrin protein synthesis coincides with the formationof the blepharoplast, at a stage when the cell division cyclesare nearing completion. Centrin abundance reaches maximal levelsat ~6 h after imbibition, as the basal bodies formed from theblepharoplast reach maturity and as the MLS begins to form. Thequestion that remains is whether centrin translation is an essentialprerequisite for formation of theblepharoplast.

Centrin is a calcium binding protein (Salisbury, 1995; Schiebel and Bornens, 1995) that resides in and around basal bodies(Baron et al., 1992; Taillon et al., 1992; Levy et al., 1996).It is synthesized during the assembly of a motile apparatus duringthe amoebo-flagellate transformation in Naegleria (Levy et al.,1998). Centrioles are preexisting structures in the amoebae. Centrinsthat participate in the organization and function of centrosomes(Middendorp et al., 2000) in higher organisms are also found inthe lumenal space of centrioles (Paoletti et al., 1996), but preciseroles for centrin in centrosomal and centriolar organization andfunction remain to be determined. During its ontogeny, the blepharoplastin M. vestita briefly serves as a functional centrosome, and thendifferentiates as a basal body factory (Hepler, 1976; Wolniaket al., 2000). Centrin proteins are related to basal body-associatedproteins in lower eukaryotes (Moudjou et al., 1991; Hart and Wolniak,1999), and they are also present in or near the blepharoplastand in or near the MLS of fern spermatids (Vaughn et al., 1993;Hoffman et al., 1994). Centrins interact with other proteins (Baronet al., 1991; Klotz et al., 1997), such as pericentrin (Doxseyet al., 1994), $gamma$ -tubulin, and cytoplasmic dynein (Purohit et al.,1999; Young et al., 2000).

Is centrin translation in gametophytes of M. vestita an essential and rate-limiting factor for blepharoplast formation? Totest for a centrin requirement, we blocked centrin translationin developing male gametophytes of M. vestita in vivo by employingantisense RNA (Holt et al., 1988) that was made from our MvCen1centrin cDNA clone (Hart and Wolniak, 1999). We devised a novelprotocol for the introduction of our constructs into the cytosolof the gametophytes. Our control experiments, using sense constructs,revealed inhibitory effects that resembled those observed in Caenorhabditiselegans and other organisms (Fire et al., 1998; Kennerdell andCarthew, 1998; Montgomery and Fire, 1998; Montgomery et al., 1998;Tabara et al., 1998, 1999; Ngo et al., 1998; Bashirullah et al.,1999; Driver et al., 1999; Fire, 1999; Misquitta and Paterson,1999; Sanchez-Alvorado and Newmark, 1999; Boscher and Labouesse,2000; Klink and Wolniak, 2000; Sharp and Zamore, 2000; Wiannyand Zernicka-Goetz, 2000), prompting us to generate double-strandedRNA (dsRNA) constructs as a means to assess whether the effectswere the result of RNA interference (RNAi). Since no one had heretoforeadded dsRNA directly to plant cells, a portion of our experimentaldesign required an assessment of the efficacy of the approach;to this end, we performed a variety of additional controls, includingtreatments of cells with antisense, sense, and dsRNA derived froma $beta$ -tubulin cDNA obtained from our library, and a noncoding segmentof HIV. Tubulin was selected because its pattern of new translationdiffers from that of centrin, and HIV was selected because itrepresents a transcript that should be irrelevant in the ferngametophyte.

In this paper, we show that centrin translation is necessary for the formation of the blepharoplast, and for differentiationof the motile apparatus in the developing spermatid of M. vestita.This is the 1st demonstration of a critical function for centrinprotein during the formation of the motile apparatus in a highereukaryote. To perform RNAi experiments, we developed a novel methodof introducing these constructs into the cells, by treating thedry spores with various RNAs at the time of imbibition. We includea large number of control experiments to assess the specificityof the response in the context of the underlying biology. Becausethis is the 1st demonstration that the direct addition of dsRNAto plant cells results in altered patterns of translation, ourexperimental design also assesses the efficacy of thisapproach.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Sporocarps, the dried structures containing the microspores and megaspores of M. vestita, were originally obtained from Dr.Peter Hepler (University of Massachusetts, Amherst, MA). The originalsource of sporocarps is a natural population of ferns growingat Lake Laganita, at Stanford, CA (Hepler, 1976). In addition,10 ponds in the greenhouses at the University of Maryland havebeen constructed and used to generate additional quantities ofsporocarps. Sporocarps were ground with three 1-s bursts in acommercial coffee grinder (Braun, model KSM2, Lynnfield, MA) andsifted through 425 µm and 212 µm wire sieves to separate the microsporesfrom the megaspores. Microspores were cultured in a shaking waterbath (New Brunswick Scientific, Gyrorotary, Model G7, New Brunswick,NJ) maintained at 20°C (Brinkmann Lauda, model RM6, Westburg,NY) at a concentration of 10 mg/10 ml of Laetsch's medium (Laetsch,1967). $alpha$ -Amanitin and cycloheximide (Sigma, St. Louis, MO) wereused at concentrations of 1, 10, and 100 µM.

RNAi Experiments

A full-length, 750 base pair (bp) centrin cDNA (MvCen1 accession # U92973) was originally isolated from our cDNA libraryduring a heterologous screen, and previously characterized (Hartand Wolniak, 1998). A 3'-truncated centrin cDNA was prepared fromMvCen1 by KpnI (Life Technologies, Rockville, MD) cleavage producinga construct ~250 bp in length. The truncated centrin cDNA clonewas transcribed in vitro according to manufacturers instructions(Epicentre Technologies, T3, T7 Ampliscribe transcription kit,Madison, WI). RNA was prepared using protocols adapted from Fireet al. (1998). In parallel, we made comparable 250 bp 5'-truncatedsense, antisense and dsRNA probes from a $beta$ -tubulin cDNA that weisolated from our M. vestita library. We made 250 bp sense, antisense,and dsRNAs from a cDNA that encodes a random sequence from theHIV genome (kindly provided by Dr. Jeffrey deStefano, Universityof Maryland, College Park, MD) for use in a series of negativecontrol experiments. Sequence analysis of this HIV-derived proberevealed no homologies with M. vestita (our unpublishedresults).

Four milligrams of dry microspores were added to 1 ml of sterile water with either sense, antisense, or double-stranded RNAat a concentration of 2000, 200, 20, 2 µg/ml, or untreated in2-ml centrifuge tubes. Spores were agitated on an Orbitron agitator(model 260200, Boekel Industries, Feasterville, PA) with aerationfor a period of 8 h at 20°C. Alternatively, after incubation inthe 2-ml microcentrifuge tubes, we transferred the microsporesto 50-ml flasks containing 25 ml of medium. For all of these experiments,the cells were harvested 8 h after imbibition and processed forstructural observations, or fractionated for biochemical analysis,as describedbelow.

Histology

Excess culture medium was removed from the flask with a pipette, and spores were pooled into a volume of 1 ml and transferredto 2-ml centrifuge tubes. For fixation, 8% paraformaldehyde pH7.4 in PBS was diluted 1:1 with the culture medium containingspores to bring the final concentration of paraformaldehyde to4%. The spore walls were fractured in a stainless steel mortarand pestle, and the cells were fixed according to protocols originallydescribed by Hepler (1976). The spores were then transferred toa microcentrifuge tube and allowed to settle without centrifugation.Spores were washed 3 times in PBS (15 min each wash) and dehydratedthrough 10, 20, 30, 40, 50, 60, and 70% ethanol in PBS (45 mineach). Dehydration proceeded through 80% and 90% ethanol in distilledwater (45 min each) followed by 3 changes of 100% ethanol. Infiltrationand polymerization in polymethacrylate was performed with proceduresdescribed by Baskin et al., (1992).

Immunocytochemistry

Male gametophytes from M. vestita exhibit high amounts of autofluorescence from spore wall and cytoplasmic polyphenolics,thereby prompting us to employ immunogold histochemistry. Methacrylatesections (1-2 µm) were placed on cleaned glass microscope slidesin drops of water and allowed to adhere to the glass by dryingat 40°C on a slide warmer. The plastic was then removed by deep-etchingin chloroform for 2 h, followed by a 30-min acetone treatment.The sections were incubated with PBS pH 7.4 (three 5-min incubations)and blocked with a solution containing 1.0% BSA fraction V (FischerScientific, Pittsburg, PA), 7.5% glycine (Fischer Scientific),5.0% Idaho Spuds (Pillsbury, Minneapolis, MN), and 5.0% Carnationnonfat dried milk (Nestle; Solon, OH) in PBS. Slides were transferredto PBS (three 5-min incubations) followed by one 5-min incubationin PBST (PBS with 0.1% Tween 20). Anticentrin (1:50 in PBST) monoclonalantibody 20H5, directed against Chlamydomonas reinhardtii, (agift of Dr. Jeffery Salisbury, Mayo Clinic, Rochester, MN), anti- $alpha$ / $beta$ -tubulinmonoclonal antibodies (Amersham, Buckinghamshire, UK - 1:100 inPBST), and anti-P28 antibody (a gift of Dr. Gianni Piperno, Mt.Sinai School of Medicine, NY), were added to the sections andincubated for 1 h in a humid chamber at room temperature. Slideswere transferred to PBST (three 5-min incubations). Gold-conjugatedantimouse secondary antibodies (Research Diagnostics, Flanders,NJ; 1:500 in PBST) were incubated on sections in a humid chamberfor 1 h at room temperature for detection of anticentrin and anti- $beta$ -tubulinantibodies. Gold-conjugated antirabbit IgG secondary antibodies(Research Diagnostics) were used for the detection of P28. Slideswere transferred to PBST (three 5-min incubations) followed byimmersion in distilled water (three 5-min changes). This transferwas done according to the manufacturer's instructions, since silverprecipitation occurs nonspecifically because of salts presentin wash solutions. Silver enhancement was performed for 15 min,followed by three 5-min washes in distilledwater.

Protein Extraction

Microspores were grown in Laetsch's (1967) medium or in distilled water. Protein extractions were performed on dry sporesas previously described (Hart and Wolniak, 1998), and on sporescultured for 30 min at 4°C, and then grown for varying intervalsfrom 1 to 11 h, at 20°C in a shaking water bath. Spores were grownat a density of 1 mg/ml of culture medium. Male gametophytes werecollected by centrifugation at 9000 × g for 10 min. Protein extraction,SDS PAGE and protein transfers onto PVDF membranes (ImmobilionP, Millipore, Bedford, MA) for immunoblotting were performed accordingto procedures described earlier (Hart and Wolniak, 1998). Proteinconcentrations were measured using assays developed by Bradford(1976).

Immunoblotting

PVDF membranes were wetted in methanol for 30 s and transferred to PBS at pH7.4 (three 5-min incubations). Blocking and antibodyincubations were the same as those used for immunocytochemistry.Primary antibody concentrations were 1:100 (centrin 20H5 monoclonalantibody), 1:500 (anti- $alpha$ / $beta$ -tubulin antibodies), and 1:250 (anti-P28antibodies). Antispecies horseradish peroxidase secondary antibodies(Amersham) were diluted 1:1500 in PBST and membranes were incubatedin a humid chamber for 1 h at room temperature. Membranes weretransferred to PBST (three 10-min incubations and one 20-min incubation).Chemiluminescence detection of binding was performed using a 1:1dilution of ECL (Amersham) on Kodak X-OMAT AR film (Eastman Kodak,Rochester, NY), or with a STORM 840 PhosphorImager (MolecularDynamics, Sunnyvale,CA).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Development of the Male Gametophyte

The pattern of development of the male gametophyte of Marsilea vestita, first described by Sharp (1914), consists of a phaseof cytoplasmic polarization (Figures 1 and 2) followed by a seriesof rapid cell divisions (Figure 2), and then, a phase of gametedifferentiation (Myles and Hepler, 1977). The entire process lasts~11 h and is initiated by placing dry microspores into water ora defined aqueous medium (Laetsch, 1967). At the earliest stageof development, a centrally positioned nucleus is surrounded bydozens of starch-containing plastids (Figures 1a and 2a). Beforethe 1st mitotic division, the cytoplasm of the hydrated microsporebecomes reorganized so that the plastids become situated along1 side of the cell (Figures 1b and 2b). The nucleus becomes repositionedaway from the clustered plastids, and undergoes the 1st mitoticdivision (Figure 2c), which creates a remnant prothallial cellthat does not divide further. The other cell of the gametophyteproceeds to enter a series of 8 additional cell division cyclesthat are completed by 5.5 h after imbibition and incubation at20°C (Figure 2, d-k). The 9 division cycles ultimately partitionthe cytoplasm within the spore wall into a total of 39 cells,32 of which are spermatids, clustered into 2 groups of 16 cells.These spermatogenous masses are surrounded by 6 sterile jacketcells, which represent the antheridial wall. A fate map (Figure2, lower panel) shows how further proliferation does not occurin the prothallial and sterile jacket cells, once they are formed.After completion of the cell divisions, the jacket cells becomeless conspicuous over time as the spermatids enlarge, separatefrom each other, and mature (Myles and Hepler, 1977). Before thelast cell division, each blepharoplast, visible as a discreteparticle in the cytosol of each spermatocyte, splits into 2 parts,and functions as centrosomes for the last mitotic spindle (Hepler,1976). The blepharoplasts disperse and then reform in each ofthe spermatids, where they become involved in basal body formation(Mizukami and Gall, 1966; Hepler, 1976). During the next 5.5 hafter imbibition, each of the spermatids develops a motile apparatus(Hepler, 1976), and undergoes extensive elongation and coilingof the nucleus (Myles and Hepler, 1977, 1982). The elongated nucleusand the motile apparatus ultimately reside at the anterior endof the gamete (Myles and Hepler, 1977). Each mature spermatozoidpossesses ~140 cilia placed along the distal face of its coiledcell body.

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Figure 1. The microgametophyte of M. vestita at and after the time of imbibition. (a) At the time of imbibition, the male gametophyte of M. vestita consists of a single cell that is contained within the microspore wall. A large centrally positioned nucleus is surrounded by dozens of starch-containing plastids. (b) Spermiogenesis is initiated by placing the spore into an aqueous medium, and all of the development occurs within the spore wall. At 30-45 min after imbibition, there is a change in the organization of the cytoplasm: the plastids become aggregated along 1 side of the microspore and the nucleus becomes displaced toward the opposite side of the gametophyte. Images photographed with Phase Contrast optics. Bar = 25 µm.

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Figure 2. Drawings of the cell division patterns during development of the male gametophyte of M. vestita. (a) Microspores at the time of imbibition. The nucleus is depicted as a black circle, and the plastids are depicted as open ellipses. (b) The gametophyte before the 1st division, when cytoplasmic reorganization occurs. (c) After the 1st mitotic division, a prothallial cell (bottom)is cut off from the rest of the gametophyte and no longer divides. (d) The 2nd division gives rise to 2 antheridial initials, essentially of equal size. (e-g) Each antheridial initial undergoes a series of unequal divisions that produce the 3 sterile jacket cells. None of the jacket cells can proliferate further. (h) Each primary spermatogenous cell undergoes a symmetric division. (i) The 2 spermatogenous cells in each antheridium undergoes a symmetric division to produce 4 spermatocyte mother cells. By this stage, the jacket cells become far less conspicuous and they eventually degenerate. (j) The 4 spermatocyte mother cells in each antheridium undergo a division to produce 8 spermatocytes. At this stage, a blepharoplast (dot) appears in each spermatocyte, and then it rapidly disappears (see Hepler [1976]). Later, the blepharoplasts reform, split and function as the centrosomes for the next mitotic cycle, when each spermatocyte undergoes a division that produces 16 spermatids in each antheridium. (Lower panel) A fate map of gametophyte development during spermiogenesis in M. vestita. During the 1st 5.5 h, the gametophytes undergo 9 mitotic division cycles to produce a total of 39 cells, 32 of which are spermatids. The vegetative prothallial cell and the sterile jacket cells lose the capability to proliferate after they are formed. The dotted lines indicate continued proliferation in an identical segment of the gametophyte. The antheridial initials, the primary spermatogenous cells, and their progeny proliferate to produce a total of 32 spermatids.

Translational and Transcriptional Inhibitors Block Spermiogenesis at Different Stages

We first tested whether specific stages of spermiogenesis are reliant upon transcription and translation. We compared thepattern of normal gametophyte development in untreated cells fixedat various points after imbibition (Figure 3, a-c) to that ofgametophytes treated with $alpha$ -amanitin, an inhibitor of RNA polymeraseII, (Figure 3, d and e), or with the translational inhibitor,cycloheximide (Figure 3f). Each of these general inhibitors wasadded to the cells at the time of imbibition, and remained presentuntil the time of fixation. The segregation of plastids to theperiphery of the gametophyte, a process that precedes the 1stdivision in untreated microspores (Figure 1b) also occurs in gametophytestreated with $alpha$ -amanitin (our unpublished results), and by 4 hof incubation in the inhibitor, these cells form blepharoplasts(our unpublished results). Treatment with $alpha$ -amanitin is followedby a normal pattern of cell division (Figure 3, d and e) and spermatidmaturation (our unpublished results), but the developmental processis arrested before spermatozoid release (Hyams et al., 1983; Hartand Wolniak, 1998). In contrast, gametophytes treated with 10µM cycloheximide fail to exhibit any cytoplasmic changes or celldivisions; even after 11 h, the gametophyte is unicellular, witha large, centrally placed nucleus and with plastids scatteredaround the periphery of the cell (Figure 3f). Thus, male gametophytedevelopment is blocked at a very early stage in the absence oftranslation and much of spermatid development is dependent onthe translation of stored mRNA.

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Figure 3. Development of the male gametophyte of M. vestita in normal medium, or in medium containing either $alpha$ -amanitin or cycloheximide. Cells were fixed at various times after imbibition. (a) Untreated gametophyte, fixed after the 3rd cell division, 90 min after imbibition. Each of the antheridial initials has already produced the 1st of 3 sterile jacket cells, which are rich in plastids. (b) Untreated gametophyte, fixed after the 9th cell division, 5 h after imbibition. This 2 µm section depicts 14 of the 32 spermatids. The jacket cells are becoming less conspicuous. (c) Untreated gametophyte, fixed at 8 h after imbibition. The spermatids had initiated nuclear elongation at the time of fixation. (d) A gametophyte incubated with $alpha$ -amanitin at the time of imbibition and fixed 4 h later. (e) A gametophyte incubated with $alpha$ -amanitin at the time of imbibition and fixed 8 h later. All of the mitotic division cycles have occurred in these gametophytes. (f) A gametophyte incubated with cycloheximide at the time of imbibition and fixed 10 h later. There have been no cell divisions. Moreover, there have been no apparent changes in cytoplasmic or nuclear organization in the presence of this inhibitor. All images photographed with DIC. Bar = 25 µm.

Centrin, $beta$ -Tubulin, and P28 Proteins Accumulate at Different Times and in Different Places

Our inhibitor experiments show that spermiogenesis is dependent on translation of stored mRNA. Our earlier studies (Hart andWolniak, 1998), show that new translation of centrin and $beta$ -tubulinoccur at different stages of spermiogenesis and suggest that specificproteins are made at particular times in the developing gametophyte.We screened immunoblots of gametophyte protein isolates with anumber of antibodies directed against cytoskeletal, axonemal,and centrosomal antigens, asking if centrin is the only new proteinmade midway through spermiogenesis, at the time of blepharoplastformation. We found that a ciliary inner-arm component, knownas P28 (LeDizet and Piperno, 1995), binds to a single proteinband on our blots in the proper molecular weight range, and thereis a large increase in the abundance of this antigen ~5 h afterimbibition. Unlike centrin, P28 is undetectable in gametophytesthat have been imbibed for < 4 h, and reaches maximal levels ofabundance ~6 h after imbibition (our unpublished results). Weperformed a series of in situ immunolocalizations on male gametophytesof M. vestita as a means to determine the distribution of theseproteins during spermiogenesis. Untreated gametophytes were fixedat various times after imbibition, and then embedded, sectioned,and labeled with antibodies directed against centrin (Figure 4,a-c), $beta$ -tubulin (Figure 4, d-f), and P28 (Figure 4, g-i). Anticentrinantibody labeling of gametophytes fixed at the time of imbibition(Figure 4a) is weak but specific, and reveals a perinuclear distribution.Thereafter (Figure 4, b and c), anticentrin antibody labelingis restricted to the spermatogenous mass; the sterile jacket cells,located around and between the spermatogenous cells, are not labeledwith the anticentrin antibody (Figure 4b). At 4 h after imbibition,some of the anticentrin antibody is aggregated in the blepharoplasts(Figure 4b, arrows), highlighting its association with, or presencein the blepharoplast (Hoffman et al., 1994). By 8 h after imbibition,the distribution is intense, and again, perinuclear, with mostof the label in the anterior region of each spermatid (Figure4c).

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Figure 4. Immunolocalizations reveal differences in the distributions of various antigens in the male gametophytes over time. Gametophytes were fixed immediately after imbibition (a, d, and g), 4 h after imbibition (b, e, and h), and 8 h after imbibition (c, f, and g) in culture medium. After sectioning at a thickness of < 4 µm and acetone-extraction of the plastic embedding medium, the cells were labeled with anticentrin antibody (a-c), anti- $beta$ -tubulin antibody (d-f), or anti-P28 antibody (g-i). Secondary gold-conjugated antibodies and silver enhancement were used to image antibody binding. (a) Centrin is detectable at low levels in cells at the time of imbibition and is present near the centrally positioned nucleus. (b) By 4 h after imbibition, dark aggregates of anticentrin antibody can be seen in spermatogenous cells; because of their abundance (1 per cell), their proximity to the unlabeled nucleus, and their size, these aggregates represent blepharoplasts (arrows). (c) By 8 h after imbibition, anticentrin antibody is abundant in the spermatids, in a roughly-perinuclear distribution. Most of the antibody ultimately resides in the apical portion of each forming spermatozoid, as it reaches maturity (our unpublished results). (d) In contrast to centrin, $beta$ -tubulin is abundant and scattered through the cytosol from the time that the spores imbibe water. (e) By 4 h after imbibition, the cytoplasm of the spermatogenous cells is heavily labeled with anti- $beta$ -tubulin antibody, while the surrounding sterile jacket cells exhibit almost no labeling. The dense labeling in 3 of the spermatids (arrowheads) shows the position of the blepharoplasts, which are sufficiently mature to exhibit anti- $beta$ -tubulin labeling. Each of the blepharoplasts is adjacent to a nucleus, represented by a nonlabeled zone in each spermatid. (f) By 8 h after imbibition, the spermatids of the sectioned gametophyte show dense labeling with anti- $beta$ -tubulin antibody at their outer edges. In some sections, the pattern resembles a clover leaf, and denotes the formation of the microtubule ribbon that is assembling on dorsal side of the developing cell (see Myles and Hepler, [1977]). (g) P28 is not detectable in newly imbibed microspores. (h) At 4 h after imbibition, the cytoplasm of both spermatogenous and sterile jacket cells is heavily labeled with anti-P28 antibodies, but blepharoplasts are not detectable in these cells. (i) At 8 h after imbibition, anti-P28 antibody is abundant in all cells of the gametophyte. All images photographed with DIC. Bar = 25 µm.

Immunolabeling with anti- $beta$ -tubulin antibody reveals a uniform distribution throughout the cytosolic compartment of the singlecell gametophyte a few min after imbibition (Figure 4d). The labelbecomes restricted to the spermatogenous cells of the gametophyteby 4 h after imbibition (Figure 4e), with no label apparent inthe surrounding sterile jacket cells (see Figure 2g). Within thespermatogenous cells, aggregates of anti- $beta$ -tubulin antibody aggregateat each blepharoplast (Figure 4e, arrows). Blepharoplast stainingwith anti- $beta$ -tubulin antibody reveals that the structure is reachingmaturity (Doonan et al., 1986; Pennell et al., 1986; Hoffman andVaughn, 1995). By 8 h after imbibition, the anti- $beta$ -tubulin antibodylabel becomes localized in the anterior portions of the spermatids(Figure 4f). In 1-3 µm sections of gametophytes labeled with anti- $beta$ -tubulinantibody, the most intense labeling often circumscribes the spermatogenousmass. This pattern of labeling is consistent with the positioningof the MLS and the forming microtubule ribbon that ultimatelyresides on the dorsal face of the cell body of each mature gamete(Myles and Hepler, 1977); at the light microscopic level of resolution,the pattern often resembles acloverleaf.

The anti-P28 antibody label is not detectable in gametophytes imbibed for < 4 h (Figure 4g). Thereafter, the P28 antigen accumulatesboth in spermatogenous and sterile cells (Figure 4h), and by 8h after imbibition, the label is uniformly distributed throughoutthe gametophyte (Figure 4i) though it seems to be more abundantin the spermatids, especially in the anterior regions of the forminggametes. We found that in gametophytes treated with $alpha$ -amanitinat the time of imbibition, the distribution and abundance of labelingwith anticentrin, anti- $beta$ -tubulin, or anti-P28 antibodies was notdiscernibly different from that observed in untreated gametophytesfixed at the same times during development (our unpublishedresults).

We observed no labeling with anticentrin or anti-P28 antibodies in gametophytes that had been imbibed with cycloheximide (ourunpublished results). Cycloheximide-treated gametophytes exhibitrandom cytoplasmic labeling with anti- $beta$ -tubulin antibodies, butwe were unable to detect any aggregation of the anti- $beta$ -tubulinantibody label in blepharoplast-like particles, even 10 h afterimbibition (our unpublishedresults).

RNAi Specifically Inhibits Centrin Translation and Disrupts Spermiogenesis

In this study, we were most interested in asking whether centrin translation is necessary for blepharoplast formation andsubsequent assembly of the motile apparatus. To address this question,we employed antisense strategies, introducing our RNA constructsinto the cells at the time of imbibition by immersing the dryspores into RNA-containing solutions. We found that gametophytedevelopment was arrested as a function of the concentration ofcentrin antisense RNA added to the microspores. In contrast tountreated gametophytes fixed at 8 h after imbibition, when thedivisions are completed and spermatid maturation is well underway (Figure 5a), we found that high concentrations (2 mg/ml) ofantisense centrin RNA probes arrested the vast majority of gametophytesin the 1-cell stage of development, with no segregation of plastidsto 1 end of the cell (Figure 5b). Most (70%) of the gametophytespresent in these large cultures, containing thousands of spores,when treated with the antisense probe, became arrested in prophaseof the 1st mitotic division, with condensed chromosomes (Figure5b), but lacking apparent spindles. For our initial set of controls,we used sense versions of the same RNA, and treated large populationsof microspores under identical conditions. Most of the gametophytes(>85%) treated with high concentrations of the sense probe failedto reach prophase of the 1st mitotic division by 8 h (our unpublishedresults); these cells closely resembled the microspores that hadbeen imbibed in cycloheximide (Figure 3f).

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Figure 5. A high concentration of centrin-based RNA probes arrests development of the male gametophytes of Marsilea vestita. At 8 h after imbibition, untreated gametophytes (a) consist of 39 cells, 32 of which are developing spermatids. Twelve spermatids are visible in this section of a gametophyte. (b) Gametophytes that were imbibed in a solution containing 2 mg/ml antisense centrin RNA and fixed at 8 h were arrested in the 1st mitotic division, with condensed chromosomes (dark structures in the center of the cell), but with no apparent spindles. Images photographed with phase contrast optics. Bar = 25 µm.

In the gametophytes imbibed in the presence of low concentrations (2-20 µg/ml) of centrin antisense or sense probes, we observednormal cytoplasmic partitioning into sterile plastid-containingjacket cells and spermatogenous cells. The early phases of celldivision cycles appeared to progress normally. However, 40 to50% of these gametophytes contained fewer cells than untreatedcontrols, suggesting that they had failed to complete all 9 divisioncycles. Intermediate concentrations of centrin antisense or senseRNA (200 µg/ml) resulted in a block to development in virtuallyall of the gametophytes, with > 75% of the cells blocked afterthe 7th mitotic division. Irrespective of the concentration ofprobe used, the spermatogenous cells failed to develop furtherif they were arrested before they completed all of their divisioncycles (our unpublished results, seebelow).

The unexpected anomalies observed with our sense probes also led us to suspect that these gametophytes were sensitive to RNAinterference (RNAi) effects (Fire et al., 1998) and prompted usto evaluate whether the presence of small quantities of centrindsRNA might be the factor responsible for the observed inhibitionof development. We treated microspores at the time of imbibitionwith several different concentrations of centrin dsRNA. Microsporeswere cultured in high (2 mg/ml) concentrations of dsRNA (centrin),similar to those used in sense and antisense experiments. Thesegametophytes failed to undergo mitosis for > 10 h after imbibition.Arrest of development appeared to coincide with prophase of the1st mitotic division. Nuclear envelope breakdown did not occur,but chromatin was condensed, in a manner similar to that observedafter treatments in antisense centrin RNA. Gametophytes developingin intermediate concentrations of centrin dsRNA (200 µg/ml) undergo6 or 7 division cycles to produce spermatocyte mother cells orspermatocytes that have plastids localized to the posterior ofthe cells. These plastids are closely aggregated and the cellshave a diffuse region of cytoplasm terminated by an anterior nucleusthat fails to undergo coiling. Intermediate concentrations ofdsRNA produced arrested development in > 80% of the gametophytesbefore all of the division cycles were completed. Low concentrationsof centrin dsRNA (2 µg/ml) arrested development for ~50% of thegametophytes after the 6th or 7th division, but in these populationsof treated cells, we saw high variation in the stage of arrest(our unpublished results). Whether or not the gametophytes developedbeyond the 7th division cycle in the presence of centrin dsRNA,the spermatogenous cells failed to undergo coiling of the cellbody or to produce anterior ciliary arrays (our unpublished results).With an apparent concentration-dependent effect on development,it became necessary to assess protein abundance as a functionof added-RNA concentration on immunoblots and protein distributionsin the treated cells byimmunolocalizations.

In order to determine whether the centrin based RNA constructs were affecting translation in different concentration rangesor at different stages during development, we performed a seriesof dose response studies with centrin RNA probes and populationsof cells. We isolated proteins from treated gametophytes 8 h afterimbibition for analysis on immunoblots (Figure 6A). We found thatcentrin dsRNA was at least 10 times more effective in preventingtranslation of centrin mRNA than centrin sense RNA or centrinantisense RNA in these populations of cells assayed 8 h afterimbibition. None of the centrin RNA treatments affected the accumulationof P28 protein in the gametophytes.

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Figure 6. Centrin translation is inhibited specifically and in a concentration-dependent manner by treatment of gametophytes with RNA probes made from MvCen1. Immunoblots of protein isolates obtained at 8 h after imbibition from populations of gametophytes treated with different concentrations of antisense RNA (lanes 1-4), sense RNA (lanes 5-8) or dsRNA (lanes 9-12). RNA probes were made from MvCen1 cDNA (A), which encodes centrin from Marsilea male gametophytes (Hart and Wolniak, 1998

), from MvB-Tub cDNA (B), which encodes a $beta$ -tubulin from Marsilea male gametophytes, and from a 250 bp random sequence present in the viral genome of HIV (kindly provided by Dr. J. DeStefano, University of Maryland) (C). The concentration of RNA was 1.5 mg/ml was in lanes 1, 5, and 9. The concentration of RNA was 150 µg/ml in lanes 2, 6, and 10. The concentration of RNA was 15 µg/ml in lanes 3, 7, and 1. The concentration of RNA was 1.5 µg/ml in lanes 4, 8, and 12. The immunoblots were probed with anticentrin antibody (upper blot in each pairing) and anti-P28 antibody (lower blot in each pairing). Binding was detected by ECF fluorescence imaging with the STORM PhosphorImager as described in the text. Lane 13 depicts a protein isolate that was obtained from untreated gametophytes, 8 h after imbibition, run in parallel with the RNA-treated spores. (Cells from these populations of control gametophytes revealed normal immunolabeling patterns with anticentrin antibody $---$ see Figure 4). The anticentrin antibody binding in control lanes should be compared separately with binding intensities in the same blots with the same populations of cells treated for MvCen1, Mv $beta$ -tub, and HIV. Though we loaded the same amounts of protein from identical cell populations onto gels, and then labeled and imaged them identically, comparisons of intensities between experiments on different blots is invalid because of nonlinearities in antigen binding and amplified fluorescence detection. (A) MvCen-derived RNA probes reduce the amount of centrin translated by the gametophytes as an inverse function of RNA probe concentration. The use of dsRNA derived from MvCen1 is at least 10 times more effective in blocking centrin translation than either sense or antisense RNA made from the same cDNA. P28 translation is not affected by the presence of MvCen-derived RNA probes. (B and C) RNA probes derived from either Mv $beta$ -tub or HIV are without significant effect on the abundance of either centrin or P28 after 8 h.

The effect of centrin dsRNA is highly specific; we found that antisense, sense and dsRNA derived from M. vestita $beta$ -tubulinhad no effect on the abundance of centrin protein in the developinggametophytes at 8 h after imbibition (Figure 6B). Moreover, inthe presence of our $beta$ -tubulin RNA constructs, we found that thepattern of centrin translation/accumulation through gametophytedevelopment was not distinctly different from that described inuntreated cells (Hart and Wolniak, 1998). Centrin protein wasdetectable at very low levels from 0-3 h after imbibition, withan increase in apparent translation at 4 h after imbibition, reachingmaximal abundance by ~6 h after imbibition in the gametophytes,whether they were treated with antisense, sense, or dsRNA madefrom M. vestita $beta$ -tubulin cDNA (Figure 6B). Centrin levels remainedhigh and constant thereafter. As expected, none of the $beta$ -tubulinRNA treatments affected the accumulation of P28 protein in thegametophytes. RNA made from a cDNA that encodes a random fragmentof the HIV genome were also without effect on the amount of centrinor P28 protein made in the gametophytes (Figure 6C), further attestingto the high specificity of the effects observed with centrindsRNA.

Patterns of Development Are Altered Specifically by RNAi Treatments With abnormal cell division patterns resulting from an induced block to centrin translation following the addition of centrinRNA (Figure 6), we assayed for altered abundance and distributionof centrin (Figure 7), $beta$ -tubulin (Figure 8), and P28 (Figure 9)by in situ immunolabeling after the gametophytes had been imbibedwith 1 of the RNA probes. We assayed fixed and sectioned cellsthat had been treated with 200 µg/ml sense, or antisense RNA transcribedfrom centrin or $beta$ -tubulin cDNAs obtained from M. vestita. We used20 µg/ml dsRNA as standard treatments on other populations ofcells. In parallel, we fixed and sectioned cells that had beentreated with sense, antisense or dsRNA derived from a 250 basesegment of the HIV genome, added at the same concentrations. Inall cases, 4 mg of cells were treated in 1 ml of RNA-containingsolution and the gametophytes were fixed 8 h after imbibition.Intermediate concentrations (200 µg/ml) of centrin sense (Figures7a and 8a) and antisense (Figures 7b and 8b), enabled gametophytesto undergo some of their mitotic divisions. Because developmentwas uniformly arrested with intermediate concentrations of oursense and antisense RNA probes, it became the focus of our effortsto assess induced changes in development. At these concentrationswith our centrin-based RNA probes, we observed arrested developmentfor the vast majority of gametophytes, which, at most, stoppedwith the 7th cell division cycle. In these gametophytes, the spermatocytemother cells that were present in the antheridia did not undergofurther differentiation. Blepharoplasts, clearly labeled in untreatedgametophytes (Figure 4, b and e) were never observed, and in theirabsence, the subsequent formation of basal bodies (and then, amotile apparatus) could not be expected.

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Figure 7. Immunolocalizations with anticentrin antibody reveal that centrin-derived RNA probes affect development and the accumulation/aggregation patterns of centrin protein. Gametophytes were imbibed with solutions containing MvCen1-derived sense RNA (a), MvCen1-derived antisense RNA (b), or MvCen1-derived dsRNA (c). No centrin protein is detectable in the gametophytes that were treated with centrin RNA probes. In addition, the gametophytes failed to undergo all 9 mitotic division cycles. Gametophytes were imbibed with solutions containing Mv $beta$ -tubulin-derived sense RNA (d), Mv $beta$ -tubulin-derived antisense RNA (e), or Mv $beta$ -tubulin-derived dsRNA (f). Anticentrin antibody labeling reveals that centrin protein accumulation and distribution is not altered by the presence of the Mv $beta$ -tubulin-derived RNA probes. Gametophytes were imbibed with solutions containing HIV-derived sense RNA (g), HIV-derived antisense RNA (h), or HIV-derived dsRNA (i). Anticentrin antibody accumulation and distribution is not altered by the presence of the HIV-derived RNA probes. All images photographed with DIC. Bar = 25 µm.

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Figure 8. Immunolocalizations with anti- $beta$ -tubulin antibody reveal that centrin-derived RNA probes affect development and the aggregation patterns of $beta$ -tubulin protein. Gametophytes were imbibed with solutions containing MvCen1-derived sense RNA (8a), MvCen1-derived antisense RNA (8b), or MvCen1-derived dsRNA (8c). Anti- $beta$ -tubulin antibody staining is diffuse in these gametophytes. Moreover, the gametophytes have undergone fewer than the normal 9 division cycles. Gametophytes were imbibed with solutions containing Mv $beta$ -tubulin-derived sense RNA (8d), Mv $beta$ -tubulin-derived antisense RNA (8e), or Mv $beta$ -tubulin-derived dsRNA (8f). Anti- $beta$ -tubulin antibody accumulation and distribution is not altered by the presence of the Mv $beta$ -tubulin-derived RNA probes, up through 8 h after imbibition. Gametophytes were imbibed with solutions containing HIV-derived sense RNA (8g), HIV-derived antisense RNA (8h), or HIV-derived dsRNA (8i). Anti- $beta$ -tubulin antibody accumulation and distribution is not altered by the presence of the HIV-derived RNA probes. All images were photographed with DIC. Bar = 25 µm.

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Figure 9. Immunolocalizations with anti-P28 antibody reveal that our RNA probes exert no effect on development and the aggregation patterns of P28 protein. Gametophytes were imbibed with solutions containing MvCen1-derived dsRNA (9a), Mv $beta$ -tubulin-derived dsRNA (9b), or HIV-derived dsRNA (9c). All images photographed with DIC. Bar = 25 µm.

In contrast to centrin, the abundance of $beta$ -tubulin protein does not change substantially until late in spermiogenesis, whenit exhibits an increase in abundance that coincides with the formationof ciliary axonemes (Hart and Wolniak 1998

). Thus, in the presenceof introduced $beta$ -tubulin RNA, we anticipated no disruption of spermiogenesisat least up to the stage where substantial levels of newly made $beta$ -tubulin were detectable, ~10 h after imbibition. The additionof $beta$ -tubulin sense (Figures 7d and 8d), antisense (Figures 7eand 8e) or dsRNA (Figures 7f, 8f, and 9b) probes to dry microsporesat the time of imbibition was followed by a normal pattern ofdevelopment that included all 9 division cycles. Thereafter, thespermatids appeared to develop normally up to 8 h after imbibition.During this late phase of spermiogenesis, we began to observesubtle anomalies in the spermatozoids that are not the focus ofthispaper.

Centrin and $beta$ -Tubulin Are Affected Differently by RNAi

When immunolabeled with anticentrin antibody, we observed no centrin staining in gametophytes that had been imbibed with sense(Figure 7a), antisense (Figure 7b) or dsRNA (Figure 7c) made fromour centrin cDNA. In the absence of labeling with anticentrinantibody in gametophytes treated with centrin sense, antisense,or dsRNA probes, we were unable to detect conspicuous blepharoplastlabeling in untreated gametophytes (Figure 4b, arrows). In contrast,when gametophytes were treated with sense (Figure 7d), antisense(Figure 7e), or dsRNA (Figure 7f) that had been made from a M.vestita $beta$ -tubulin cDNA, we found intense anticentrin antibodylabeling in the spermatids. The distribution of centrin antigenin these cells appeared very similar to that in untreated cells(Figure 4c) that had been fixed at 8 h after imbibition, sectioned,and immunolabeled. Similarly, the presence of sense (Figure 7g),antisense (Figure 7h), or dsRNA (Figure 7i) made from a 250 basesegment of the HIV genome had no apparent effects on centrin abundanceor on spermatiddevelopment.

When gametophytes treated with centrin sense (Figure 8a), antisense (Figure 8b), or dsRNA (Figure 8c) were immunolabeled withanti- $beta$ -tubulin antibody, we found diffuse cytoplasmic tubulinstaining in the spermatogenous cells. The tubulin aggregationpattern did not resemble the intense antitubulin labeling of blepharoplasts,seen in untreated cells at 4 h after imbibition (Figure 4e), orthe anti- $beta$ -tubulin antibody labeling that is typical of spermatidsobserved 8 h after imbibition (Figure 4f), which in some sections,resembles a clover-leaf pattern. Instead, we saw a marked reductionof anti- $beta$ -tubulin antibody label intensity in these cells, a resultwe interpret as indicative of reduced microtubule organizationin the gametophyte, rather than lowered $beta$ -tubulin abundance. Thepattern of anti- $beta$ -tubulin antibody labeling in gametophytes treatedwith sense (Figure 8d), antisense (Figure 8e), or dsRNA (Figure8f) made from our $beta$ -tubulin cDNA all appear markedly differentfrom the gametophytes treated with centrin RNA probes (Figure8, a-c). In the presence of the $beta$ -tubulin RNA probes, there isno apparent disruption of spermiogenesis or $beta$ -tubulin aggregationin the spermatids (Figure 8, d-f) through 8 h after imbibition.Gametophytes treated with $beta$ -tubulin RNAs begin to display anomaliesin spermiogenesis 9-10 h after imbibition, when the cells areactively engaged in axonemal formation (our unpublished results).As expected, treatments of gametophytes with RNA probes made fromHIV had no effect on the abundance or distribution of $beta$ -tubulin(Figure 8, g-i) in the normally developing spermatids, (wherenearly mature gametes are present in Figure 8g, and the clover-leafpattern of anti- $beta$ -tubulin can be seen in Figure 8 (h andi).

Specificity of RNAi

We performed in situ immunolabeling with anti-P28 antibody on fixed, sectioned gametophytes that had been imbibed with thedsRNA probes made from M. vestita centrin cDNA (Figure 9a), M.vestita $beta$ -tubulin cDNA (Figure 9b), and HIV cDNA (Figure 9c).The obvious expectation from the addition of irrelevant (noncoding,nonhomologous) RNA probes from HIV to these cells is that we wouldobserve no effect on spermiogenesis. We found that the abundanceand the distribution of P28 (Figure 9, a-c) were normal throughoutspermiogenesis, a result consistent with our immunoblot studies(Figure 6).

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

We have found that the translation of centrin from stored mRNA is necessary for the formation of the blepharoplast in themale gametophyte of M. vestita. By employing general pharmacologicalblocks to transcription and translation, we expand upon our earlierobservations (Hart and Wolniak, 1998) to show how spermiogenesisin this organism is dependent upon the translation of stored mRNAs.Our RNAi experiments show an essential link between centrin translationand the formation of basal bodies in a developing eukaryotic gamete.Centrin antisense, sense, and dsRNA probes inhibit centrin translationin a gene-specific and concentration-dependent manner. CentrindsRNA is at least 10 times more effective than either antisenseor sense centrin RNA in preventing centrin translation. In thepresence of the centrin-derived RNAs, blepharoplasts fail to form,and there is a pronounced disruption in the formation of the motileapparatus. Antisense, sense, or dsRNA made from Marsilea $beta$ -tubulincDNA only affects development late in the process, when new $beta$ -tubulintranslation appears to occur (Hart and Wolniak, 1998). Blocksto centrin translation affect the distribution of $beta$ -tubulin, becausethese proteins are both present in the blepharoplast and the MLS(Vaughn et al., 1993), and because appear to interact with eachother. The addition of HIV RNA exerts no effect on translationalpatterns in the gametophytes, and is without effect on the spermatozoiddevelopment. Thus, our blocks to centrin translation with centrin-derivedRNA probes reveal that centrin translation is necessary for blepharoplastformation, and that the centrin protein controls or affects cytoskeletalpatterning and formation of the motileapparatus.

Centrin Translation Is Essential for Spermiogenesis

The blepharoplast is a particle unique in the spermatogenous cells of lower plants; it functions briefly as a centrosome,and then it serves as the site for de novo basal body formation.In its capacity as a centrosome for the ultimate division in normally-developingmale gametophytes of M. vestita, the blepharoplast resides atspindle poles for just a few minutes (Sharp, 1914; Hepler, 1976).During basal body formation, the particle is recognizable for~60 min, a time during which it can be immunolabeled with anticentrin(Figure 4b) and then antitubulin (Figure 4e) antibodies. Centrinhas already been shown to associate with the blepharoplast andMLS by EM immunolabeling (Vaughn et al., 1993; Hoffman et al.,1994) and antitubulin antibody labels the blepharoplast only asbasal bodies become recognizable (Doonan et al., 1986). The diagnosticpattern of immunolabeling with anti- $beta$ -tubulin antibody duringlater time points in spermiogenesis is in an intense Ag/Au depositthat resembles a cloverleaf pattern in sectioned gametophytes(Figures 4f and 8, d and e, h and i), and signifies the formationof the MLS and its microtubule ribbon along the anterior endsof the spermatids. Deviations from this distinctive labeling pattern(Figure 8, a-c) are indicative of anomalies that occurred earlierin development. In the absence of centrin translation, the gametophytesfail to undergo all 9 mitotic division cycles, blepharoplast formationfails to occur, and spermiogenesis is arrested before the assemblyof a motile apparatus. In the absence of centrin translation,there is no aggregation of the anti- $beta$ -tubulin antibody label (Figure4e) that overlies each organized blepharoplast, and the clover-leafpattern of anti- $beta$ -tubulin antibody labeling fails toform.

If cycloheximide is present in the imbibition medium, all gametophyte development is arrested for extended periods (Figure3f), and no new centrin is translated (Hart and Wolniak, 1998).High concentrations of antisense, sense and dsRNA (centrin) presentin the imbibition medium also arrest gametophytes in the singlecell stage. High concentrations of antisense centrin RNA blockedthe gametophytes at prophase of the 1st division, while senseand dsRNA probes arrested the gametophytes before the 1st division.Perhaps, the probes act through different mechanisms. At highconcentrations, centrin antisense RNA appears to act in a gene-specificmanner, to lower or block centrin translation necessary for theearly division cycles. Small amounts of newly made centrin proteinwere detectable on immunoblots from untreated gametophytes, shortlyafter imbibition (Hart and Wolniak, 1998); this centrin proteinmay be involved in mitotic spindle organization. Centrin appearsto function in the organization of mitotic spindles in a varietyof organisms (Taillon et al., 1992; Weich et al., 1996; Salisbury,1995; Middendorp et al., 2000), and plays a prominent role inbasal body formation during Naegleria amebo-flagellate transformations(Levy et al., 1996, 1998). Centrin has been immunolocalized inthe blepharoplast and the MLS of plant spermatozoids (Vaughn etal., 1993; Hoffman et al., 1994; Hoffman and Vaughn, 1995), butour current work provides the 1st clues about this protein inthe formation of thesearrays.

Earlier, we (Hart and Wolniak, 1998, 1999) proposed that spermiogenesis in M. vestita relied heavily on the translation ofstored mRNAs at specific times during development. Here, our combinationof inhibitor and RNAi strategies with immunolabeling reveal thatthe translation of stored mRNAs occurs at the beginning of developmentfrom the time that spores are imbibing culture medium. Sporescultured in the presence of cycloheximide and in high concentrationsof either centrin sense RNA or centrin dsRNA all fail to exhibitnuclear migration, plastid reorganization and chromatin condensation,a result suggesting that the initiation of development is controlledby yet-to-be-characterized, untranslated stored mRNAs. It is strikingthat no development of the gametophyte occurs in the presenceof only stored protein (Figure 3f). We suspect that a number oftranslation products, in addition to centrin, made early in gametophytedevelopment are important components in processes that are manifestedmorphologically as the segregation of the cytoplasm into spermatogenousand sterile domains that become partitionedlater.

The Specificity of RNAi and the Requirement of Centrin for Spermiogenesis

Because we had opted to perform direct additions of RNAs to our gametophytes, it was necessary to establish the efficacy ofour RNAi approach, by including multiple negative and positivecontrols in the experimental design. We employed sense RNA andantisense RNA in addition to the dsRNA in parallel dose-responseexperiments for multiple genes (Figure 6). By assaying for thepresence and distribution of centrin, $beta$ -tubulin, and P28 in identicallytreated cells with immunolocalizations (Figures 7-9), we are ableto match developmental anomalies with specific changes in antigendistributions. By comparing centrin abundance on immunoblots madefrom cells treated with each of the RNA probes (Figure 6), weconclude that the inhibitions of centrin-derived RNA probes arealmost certainly gene-specific and definitely concentration-dependent.

At low concentrations, our centrin-based RNA probes may prevent centrin translation in sufficient quantities for blepharoplastformation. In the absence of blepharoplasts, we observe no furtherprogression in spermiogenesis; usually we fail to see the final2 cell division cycles in the gametophyte. We suspect that mitoticarrest after the 7th division cycle provides an indication thatthe blepharoplast somehow controls mitotic progression in thefinal stages of proliferation in the gametophyte. The blepharoplastserves as a centrosome for the 9th division in this organism (Hepler,1976). Centrin has been linked to centrosomal duplication (Jarvikand Suhan, 1991; Middendorp et al., 2000), so perhaps in its absence,duplication of the forming blepharoplast is blocked at this stage,and subsequent formation of the mitotic spindle is prevented.Since mature blepharoplasts produce basal bodies, formation ofbasal bodies and ciliary axonemes is precluded after these treatments.We see no indication of basal body formation, or ciliogenesisin gametophytes that were blocked with our centrin-basedRNAs.

High concentrations of the centrin sense RNA and centrin dsRNA in the gametophytes may be affecting development through aneffective, specific block of centrin translation. It was not surprisingthat the centrin RNA probes are inhibitory, given the fact thatspermiogenesis represents a complex developmental program thatis reliant on the translation of certain kinds of stored mRNAwithin a tight time regime. We believe that our centrin RNAs couldalso alter pool sizes of transcripts in the gametophyte, and affectoverall rates of centrin translation through multiple mechanisms.It is reasonable to suspect that the cells possess surveillancemechanisms to detect anomalous quantities or types of RNAs thatcould be disruptive to the developmental program. The mechanismof inhibition by centrin sense RNA is probably linked to the presenceof small amounts of dsRNA present in the transcription mixture,since dsRNA made from the same probe is even more effective atinhibiting development at the same stage. The effects of highdoses of both sense and antisense centrin RNA were less dramaticthan comparable concentrations of centrin dsRNA (Figure 6A), suggestingthat inhibition is the consequence specific RNAi mechanisms affectingtranslational activities in the cells. Similar multi-tiered effectshave been observed in other organisms (Fire et al., 1998). Thespecificity of the response of this developmental program to thepresence of centrin-based RNA probes is highlighted by the inabilityof our $beta$ -tubulin RNA probes to affect development within 8 h ofimbibition, or of our HIV-based RNA probes to evoke any anomaliesinspermiogenesis.

Intermediate concentrations of antisense centrin RNA usually allow 7 division cycles to reach completion before gametophytedevelopment is arrested. At this stage of development, we wouldhave expected to see blepharoplasts form, but they fail to appear.Since the cells fail to label with anticentrin antibody, we assumethat there is insufficient centrin protein present in the gametophytefor detection of the antigen. We performed immunolabeling on thesegametophytes with anti- $beta$ -tubulin, looking for tubulin aggregationsthat are diagnostic of blepharoplast maturation (Doonan et al.,1986), but we failed to see any aggregates that hinted at organizedblepharoplast assembly. This result was expected because tubulinadditions to the blepharoplast occur late in the ontogeny of theorganelle (Hepler, 1976; Doonan et al., 1986). Thus, we are ledto conclude that at intermediate concentrations, our centrin antisenseprobes are acting specifically on centrin translation and thatcentrin synthesis is a necessary prerequisite for blepharoplastformation.

Our centrin dsRNA treatments block the translation of stored centrin mRNA at concentrations ~10-100 times lower than eithersense or antisense RNA (Figure 6). The increased potency of inhibitionby dsRNA is a hallmark of RNAi effects in a variety of eukaryoticorganisms (Kennerdell and Carthew, 1998; Montgomery et al., 1998;Montgomery and Fire, 1998). After the addition of our centrin-basedRNA probes, it is clear that the block to development occurs ator just before the stage of blepharoplast formation, and the furtherelaboration of the motile apparatus or maturation of the gametesis arrested. We suspect that the anomalies in $beta$ -tubulin distributionin cells imbibed with centrin sense (Figure 8d), antisense (Figure8e) or dsRNA (Figure 8f) is the consequence of the role of centrinprotein in controlling microtubule assembly patterns in the developingspermatid (Vaughn et al., 1993; Vaughn and Harper, 1998). In contrastto a block of centrin translation, development is not dramaticallyaltered through 8 h after imbibition by the presence of antisense,sense or dsRNA made from a $beta$ -tubulin cDNA isolated from our gametophytelibrary. Our earlier work showed that new $beta$ -tubulin is not translateduntil late in spermiogenesis, when the spermatids are assemblingciliary axonemes (Hart and Wolniak, 1998). Presumably at thatstage of development, this protein becomes limiting for axonemalgrowth.

Rapid, Efficient, Direct Uptake of Drugs and RNA into Gametophytes during Imbibition

The blocks to spermiogenesis we observe require entry of cycloheximide or these RNAs into the cytosol of the gametophyte.We have found that molecules as large as 450+ bp RNAs will enterthe dry microspores rapidly at the time of imbibition. Pettitt(1979) showed that dry megaspores from M. vestita were permeableto large iron particles at the time of imbibition, and that theparticles would accumulate in cytosolic space of the gametophyteif they were present in the aqueous medium at the time the dryspores were immersed in the suspension. The drugs or RNAs usedin our experiments were present in the aqueous medium at the timethe dry microspores were added. Uptake of the probes appears tobe rapid and uniform in a population of cells. We can vary RNAconcentration in replicate experiments and treat cells directlywith RNA, as opposed to being reliant upon expression of an insertin a transformed organism (Waterhouse et al., 1998; Chuang andMeyerowitz, 2000). The level of permeability we observe may bewidespread among gametophytes whose germination immediately followsimbibition by dry spores. Thus, in an extension of these particleuptake experiments (Pettitt, 1979), and our previous drug andradiolabel experiments (Hart and Wolniak, 1998), it seems clearthat our RNAi probes enter the cells of the gametophytes at thetime of imbibition. The utility and efficacy of macromolecularuptake by dry spores at the time of imbibition provides a powerfulmeans with which to perform a variety of experimentaltreatments.

To ensure specificity with our RNAi treatments, we performed in vitro transcriptions from those portions of the centrin and $beta$ -tubulin transcripts that exhibit the lowest similarity to relatedgenes. Centrin appears to be a single-copy or few-copy gene ingametophytes of M. vestita (Hart and Wolniak, 1999). Both centrinand $beta$ -tubulin RNAs were made from cDNAs isolated from our M. vestitalibrary. Clearly, these factors contribute substantially to thespecificity of theresponse.

	ACKNOWLEDGMENTS

We gratefully acknowledge support for this work from the National Science Foundation (MCB-9809950, MCB-9904435). We are gratefulto Dr. Peter Hepler for providing us with our initial supply ofsporocarps. In addition, we appreciate the efforts of Drs. JeffDeStefano, Peter Hart, Jeff Salisbury, Berl Oakley, and GianniPiperno, who supplied us with probes that proved to be invaluableduring various phases of this study. A number of our colleaguesat the University of Maryland, including Chia-Wei Tsai, Jeff Molkand Drs. Eric Baehrecke, Margaret De Cuevas, Bill Jeffery, SteveMount, and Heven Sze have provided us with input, suggestions,and comments at various stages of this project. Their interest,support and encouragement has helped us extend this work in anumber of importantdirections.

	FOOTNOTES

^* Corresponding author: sw36{at}umail.umd.edu.

*Corresponding author: sw36{at}umail.umd.edu.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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				A. Selvapandiyan, A. Debrabant, R. Duncan, J. Muller, P. Salotra, G. Sreenivas, J. L. Salisbury, and H. L. Nakhasi Centrin Gene Disruption Impairs Stage-specific Basal Body Duplication and Cell Cycle Progression in Leishmania J. Biol. Chem., June 11, 2004; 279(24): 25703 - 25710. [Abstract] [Full Text] [PDF]

				B. Koblenz, J. Schoppmeier, A. Grunow, and K.-F. Lechtreck Centrin deficiency in Chlamydomonas causes defects in basal body replication, segregation and maturation J. Cell Sci., July 1, 2003; 116(13): 2635 - 2646. [Abstract] [Full Text] [PDF]

				S. C. Stout, G. B. Clark, S. Archer-Evans, and S. J. Roux Rapid and Efficient Suppression of Gene Expression in a Single-Cell Model System, Ceratopteris richardii Plant Physiology, March 1, 2003; 131(3): 1165 - 1168. [Full Text] [PDF]

				A. Selvapandiyan, R. Duncan, A. Debrabant, S. Bertholet, G. Sreenivas, N. S. Negi, P. Salotra, and H. L. Nakhasi Expression of a Mutant Form of Leishmania donovani Centrin Reduces the Growth of the Parasite J. Biol. Chem., November 9, 2001; 276(46): 43253 - 43261. [Abstract] [Full Text] [PDF]

				C. W. Tsai and S. M. Wolniak Cell cycle arrest allows centrin translation but not basal body formation during spermiogenesis in Marsilea J. Cell Sci., January 12, 2001; 114(23): 4265 - 4272. [Abstract] [Full Text] [PDF]