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Galls on the marine red alga Prionitislanceolata (Halymeniaceae): specific induction and subsequentdevelopment of an algal–bacterial symbiosis¹

^a Department ofBiology, University of California, Santa Cruz 1156 High Street, SantaCruz, CA 95064

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Gall formation in Prionitis lanceolata is associated with aspecific eubacterium (Proteobacteria [alphasubclass], Rhodobacter grouping), which, typical ofbacterial symbionts, has not yet been cultivated or isolated in pureculture. This investigation tested the hypothesis that P.lanceolata gall formation was caused by the associated eubacteriumusing a species-specific rDNA probe (S-S-P.l.sym-0949-a-A-25) toidentify and assay for symbiont presence during consecutive laboratoryinduction trials. Gall induction was quantified and whole-cell in situhybridization used to determine the relative percentage of symbioticeubacteria in inoculation homogenates. In situ hybridization ofsymbionts in sections allowed localization and monitoring of thismicrobe during gall development. Induction trial results indicate asignificant correlation between bacterial symbiont presence and gallinitiation (P = 0.00005). The gall bacterium comprisedthe majority of the eubacteria hybridized in laboratory inductionhomogenates (85–97%), in galls induced in the laboratoryand in three algal populations in nature. The evidence presented heredemonstrates the causative role of the identified eubacterium in gallinduction and formation. This investigation is significant in theapplication of molecular methods towards understanding the roles ofnoncultivable marine bacteria in marine algal–microbeinteractions.

Key Words: eubacteria • galls • Halymeniaceae • insitu hybridization • Prionitislanceolata • redalgae • symbiosis

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Prionitis lanceolata Harvey (Halymeniaceae, Rhodophyta) isan intertidal red alga that occurs commonly along the central coast ofCalifornia coast and is frequently found bearing small galls or tumors(1–15 mm) (Abbott and Hollenberg,1976). Individuals of this species are distributed fromsemipermanent upper intertidal tidepools to at least 20–25 msubtidally (Ashen, personal observations). Thalli are saxicolous, andfull grown size varies greatly from typically smaller upper intertidalspecimens (25–30 cm) to subtidal specimens that can reach <0.5m in length.

Galls on P. lanceolata are conspicuous in nature, appearingas small light-pink "domes" or "protuberances"and are typically restricted to thalli of the low intertidal andsubtidal zones (Apt and Gibor, 1989).Thalli exposed to high wave or surge action are usually found bearinggalls, the number of which varies per individual. Affected P.lanceolata appear to fall into two groups, with lightly affectedthalli bearing ~1–10 galls each and heavily affectedindividuals bearing less than ~100 each.

Galls on Prionitis were originally described from P.decipiens (Peru) as the parasitic red alga Lobocolaxdeformans Howe (Howe, 1914).Ultrastructural investigation of Lobocolax on P.lanceolata in central California revealed this "parasiticalga" to be a bacterial gall composed of hypertrophied algal cellscontaining aggregations of intercellular bacteria (1 x 2 µm insize) (McBride, Kugrens, and West,1974).

Gall induction and development on P. lanceolata were firstinvestigated by Apt and Gibor (1989), whoused size-fractionated homogenates of galls collected in nature todemonstrate the required presence of a "live infectiousparticle" of bacterial size (0.2–10 µm) for successfullaboratory induction (Apt and Gibor,1989). Wounding of the algal thallus to the medulla, followedby incubation with this homogenate allowed successful gall induction,but the specific microorganism responsible was not isolated or shown tobe the causative agent.

Bacterial gall formation has also been described from a number ofother red algal species, although there is little direct evidence forthe causative roles of any microorganism in gall formation (Andrews, 1977; Apt,1988) This is probably due to the generally recognizeddifficulties encountered when attempting to cultivate symbiotic bacteriaand isolate them in pure culture (Breznak,1984; Smith and Douglas, 1987;Bermudes, Chase, and Margulis, 1988;Apt and Gibor, 1989; Vetter, 1991). To date, only Cantcauzene (1930) has reported thedemonstration of the causative role of an isolated bacterium in algalgall formation.

Recently, the bacterial symbiont associated with gall formation onP. lanceolata, was identified by whole-cell in situhybridization using a fluorescently labeled, species-specific ribosomalRNA-targeted oligodeoxynucleotide probe (S-S-P.l.sym-0949-a-A-25)(Ashen and Goff, 1996). Phylogeneticinference based on 16S rDNA sequence comparisons suggests that thiseubacterium is most closely related to other gall-forming bacterialsymbionts from the genus Prionitis and the marine algalepiphyte isolated from Japan, Roseobacter denitrificans (alphasubclass of the Proteobacteria) (Shiba,1992; Ashen and Goff,1996)

The current investigation of P. lanceolata gall inductionemployed whole-cell in situ hybridization to investigate the causativerole of the gall symbiont in tumor formation. In situ hybridization isparticularly suited to investigations of symbiotic associations wherethe cultivation and isolation of the microbial partner has not beenachieved (Amann et al., 1991; Hahn, Amann, and Zeyer, 1993; Amann, Ludwig, and Schleifer, 1995). The algalhost response during gall development was also investigated using insitu hybridization in section and in standard preparations for lightmicroscopy. The possibility that the bacterial symbiont is notrestricted intercellularly but undergoes an intracellular phase incertain regions of gall proliferation or at particular times during gallformation was also re-investigated in preparations for transmissionelectron microscopy (TEM) (McBride, Kugrens, andWest, 1974).

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Satisfaction of Koch's postulates
The demonstration of the causative role of the P. lanceolatasymbiont in gall induction was carried without cultivation or isolationof this organism in pure culture with whole-cell in situ hybridizationsubstituted as a measure of absolute identification. This modificationof Koch's postulates allowed a specific microorganism to beidentified and monitored during sequential rounds of gall initiation anddevelopment (Fig. 1). Gallscollected from nature were used to induce gall formation on nonaffectedthalli. Galls induced successfully were then used to induce a secondround of gall formation. At each step whole-cell in situ hybridizationwas used to identify the gall symbiont and monitor the presence ofnonsymbiotic eubacteria.

View larger version (30K): [in this window] [in a new window]   Fig. 1. Flow chart depicting sequential gall inductions and in situ hybridizations carried out in this study. Gall inductions were performed sequentially with in situ hybridization used to identify symbiotic bacteria from induction homogenates and sections of induced galls. Figure Abbreviations: c, cortex: dc, dead cells: e, epideral cortex: ic, intracellular bacteria: g, gall: m, medulla: p, autofluorescent particles: u, unaffected tissue: ws, wound site.

Laboratory gallinduction from field-collected material
Galls used for laboratory induction trials were prepared as follows.Galls were excised from thalli collected at Lover's Pt. and washedten times in sterile seawater (0.22 µm filtered). Galls (~5 gfresh mass) were homogenized in a sterile mortar and pestle andresuspended in 45 mL sterile seawater in 50-mL Falcon tubes on ice.Algal thalli were prepared as follows. Blade tips (5–10 cm) wereexcised from thalli that had been kept in indoor flow tanks for 2 mo;these thalli showed no evidence of gall formation. Thalli were wipedclean of surface epiphytes and wounded to the medulla by injection ofgall homogenate. Negative controls were prepared simultaneously usingblade tips taken from the same individual thalli. Sterile seawater wassubstituted as an inoculum. Inoculated blades were incubated in 50-mLFalcon tubes containing gall homogenate at 12°C for 2–3 h.After incubation, blade tips were immobilized in short lengths of tygontubing epoxyed to the flat face of a cement brick. This assemblage wasincubated in an indoor seawater tank with high ambient flow andaeration. Induction trials were performed six times, totaling ~600inoculation events. Successful induction was scored as a percentage ofinoculated sites that formed pigmented cell masses associated withintercellular bacteria.

Laboratory gall induction from experimentally inducedgalls
Bacterial galls (60) induced in the laboratory were harvested after 8wk, rinsed, and homogenized (6–8 each) with sterile tissuegrinders (Kontes, Vineyard, New Jersey) in sterile 1.5-mL Eppendorftubes containing 200 µL of sterile seawater. The volume of gallhomogenate in each tube was increased to 1.5 mL with sterile seawaterand the samples pooled, yielding a final volume of 12 mL. Subsamples (2x 1 mL) were fixed for whole-cell in situ hybridization and theremainder brought to 45 mL in sterile seawater. This suspension was usedto initiate a second round of gall induction on P. lanceolatablade tips. Inoculated blades were incubated as above and scored after 8wk as a percentage of galls successfully formed in inoculationsites.

Fluorescent in situhybridization of symbiotic bacteria
Galls from P. lanceolata collected from the state beach inCarmel and Lighthouse Point in Santa Cruz were excised from host thalliand cored by sterile dissection. Cores were washed five times in sterileseawater and homogenized in Eppendorf tubes as above. Specimens werefixed, dehydrated, and attached to 10-well Teflon-coated hybridizationslides as described previously (Ashen and Goff,1996). Identification of the gall symbiont was then carriedout by dual hybridization using a 5' TAMARA-conjugated universaleubacterial probe (S-D-Bact-0338-a-A-18) and a 5'fluorescein-conjugated symbiont-specific probe (S-S-P.l.sym-0949-a-A-25)(DeLong, 1993; Ashen and Goff, 1996). Hybridizations and washeswere performed at 43°C in 0.2 x SET (30 mmol/L NaCl, 2mmol/L Na₂EDTA, 4 mmol/L Tris base) as describedpreviously, mounted in 3:1 Citifluor:DAPI (0.5 µg/mL4,6-Diamidino-2-phenylindole), sealed with nail polish, and imaged on anOlympus IMT2 inverted photoscope using a Biorad 600 laser confocalimaging system and an Olympus S-Plan-apo 60x, oil objective(Ashen and Goff, 1996). Excitationwavelengths were 510 nm, corresponding to the maximal excitationwavelength of fluorescein and 560 nm, corresponding to that of TAMRA(the excitation wavelength of this proprietary chromophore is equivalentto that of rhodamine) (Applied Biosystems, Foster City, California).Slides were stored dark at 4°C for up to 2 mo with little to nonoticeable loss of fluorescence. Agrobacterium tumefaciens andRoseobacter denitrificans cells were included on the sameslides to control for oligonucleotide probe specificity.

Homogenates used to investigate the bacterial role in gall inductionwere prepared, fixed, hybridized, and imaged as above. Images of labeledcells were captured from single transects across individual wells of thehybridization slides (ten random fields of view, 2x zoom). Therelative percentage of symbiotic bacteria among the total eubacteriahybridized was determined in each induction homogenate by merging of thered and green fluorescence signals produced by each excitationwavelength and subtraction of cells hybridized only by the universaleubacterial probe from the total hybridizedeubacteria.

In situhybridization: paraffin sections using a digoxigenin-labeledoligonucleotide
Field-collected and laboratory-induced galls were excised from algalthalli, dissected, and fixed for 3–16 h in a 1:1 mixture ofbuffered paraformaldehyde (8%) and seawater at 4°C (Ashen and Goff, 1996). Laboratory-inducedspecimens were fixed at 2, 3, 4, 6, and 8 wk after inoculation.Specimens were washed twice in 1x phosphate-buffered saline (PBS)for 10 min each and dehydrated in a graded ethanol series (Sambrook, Fritsch, and Maniatis, 1989). Theethanol was replaced by three washes in xylenes (20 min each) and thespecimens gradually infiltrated with Periplast plus (Oxford Scientific,St. Louis, Missouri). Infiltration was completed through three changesof Periplast over 48 h and embedded blocs stored for up to 4 mo(4°C) before sectioning.

Sections (5 µm) were adhered overnight at 45°C to acid-washed,3-aminopropyltriethoxysilane (Sigma, St. Louis, Missouri) coated glassslides and stored at -20°C for no longer than 1 mo. Forhybridization a number of previously used protocols available in themicrobial and botanical literature were combined and modified (Cary et al., 1993; Hahn,Amann, and Zeyer, 1993; Polz et al.,1994; Dubilier et al.1995). Specimens were brought to 25°C, deparaffinized inthree changes of xylenes (30 min total) and rehydrated through ethanolto deionized water. Sections were treated with freshly prepared HCl(0.2mol/L for 20 min at 25°C), rinsed in 1x PBS andneutralized in 2x SSC (0.3 mol/L NaCl, 30 mmol/L sodiumcitrate) for 20 min at 25°C. This was followed by two rinses ofdeionized water and incubation in TE-100 (100 mmol/L Tris-HCl, 5mmol/L Na₂EDTA [pH 7.5]) for 5 min at25°C.

Following equilibration, sections were treated with lysozyme (1mg/mLin TE-100 for 30 min at 25°C) in a humidchamber under parafilm coverslips. Slides were rinsed twice with TE-100and prehybridized in 150 µL prehybridization buffer (6x SSC,0.2% SDS, 5x Denhart's, 100 µg/mL shearedsalmon sperm DNA, and 25 µg/mL yeast tRNA) at 43°C underparafilm coverslips. The prehybridization buffer was replaced after 2 hby 100 µL hybridization buffer, identical in composition butcontaining either S-S-P.l.sym-0949-a-A-25 or an Alvinellapompjiana specific probe 5' labeled with digoxigenin-11-dUTP(final concentration = 75 ng/section) (Cary et al., 1993). Sections were then hybridizedovernight at 43°C under parafilm coverslips. Sections oflaboratory-induced galls to which no oligonucleotide probe was added andsections of P. lanceolata wounded with sterile seawater andhybridized with S-S-P.l.sym-0949-a-A-25 were included as negativecontrols.

After hybridization, specimens were washed at 43°C as follows:2x SSC, once for 30 min and once for 1 h; 0.2x SSC, twicefor 1.5 h each. Digoxigenin moieties conjugated to hybridizedoligonucleotides were detected using an antidigoxigenin antibody (FABfragment) conjugated to alkaline phosphatase (Boehringer Mannheim,Indianapolis, Indiana). The activity of alkaline phosphatase isvisualized colorimetrically as a dark precipitate following reactionwith 5-bromo-4-chloro-3-indolyl-phosphate-4-toluidine salt/4-Nitroblue tetrazolium chloride (BCIP/NBT) as per the manufacturersrecommendations (Boehringer Mannheim). Specimens were dehydrated throughethanol and xylenes, mounted in Permount (Fisher), and photographedusing a Leitz Diaplan microscope equipped with PL-fluotar objectives andKodachrome 160T color slide film.

Light and epifluorescence microscopy
P. lanceolata galls (laboratory-induced andfield-collected), uninfected vegetative thalli, and seawater inoculatedthalli were embedded in JB4 plus resin (Ted Pella, Redwood City,California) and prepared for light and epifluorescence microscopy usingstandard techniques (McCully, Goff, and Adshead,1980; Goff and Zuccarello,1994). Galls induced in the laboratory were also prepared forlight microscopy by squashing following the methodology of Goff and Zuccarello (1994).

Sections (3 µm) were stained directly with 1% aniline blue(aq), toluidine blue O (pH 4.4 in benzoate buffer), or the nucleic acidfluorochrome DAPI (0.1–0.5 µg/mL in filtered seawater)(McCully, Goff, and Adshead, 1980).Paraffin sections (5 µm) were deparaffinized in xylenes, rehydratedthrough a graded ethanol series, and stained as above. DAPI-treatedsections were mounted in Citifluor (Ted Pella), observed on a Leitzdiaplan microscope equipped with PL-fluotar objectives, and photographedusing Kodachrome color slide film (ASA 160T or elite 400) (Goff and Zuccarello,1994).

Transmissionelectron microscopy
Laboratory-induced and field-collected material were prepared fortransmission electron microscopy using chemical fixation protocolsdescribed previously and modified as described below (Bozzola and Russell, 1992; Goff and Zuccarello, 1994). Specimens weretransferred from 70% acetone to 2% uranyl acetate in70% methanol (w/v) and en bloc stained overnight at 4°Cin the dark. Dehydration in acetone was completed and gradualinfiltration with Spurr's resin completed over 1–2 wk. Silversections were cut on a Sorvall Porter-Blum Ultra MT-2, collected oncopper grids, stained for 5–10 min with Sato's lead stain,and observed and photographed on a JEOL JEM-100B electron microscope at80 kV.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Laboratory induction
Gall formation on P. lanceolata was observed in all sixinduction trials within 2–3 wk of inoculation (Table 1). Initial stages of gallformation were seen as pigmented regions within inoculated thalli(Fig. 2). Thick section ofthese regions revealed dense masses of small, abnormally shaped,pigmented cells (pink) forming within the thallus interior (Fig. 3). Developing galls were notfirmly embedded in the algal thallus and were easily separated bydissection needle. Galls were also observed to distend from the plane ofthick section, indicating their containment under pressure within theunaffected thallus. When squashed, gall tissue liberated copious numbersof bacteria of uniform morphology (1 x 2 µm) and algal cellsthat retained a large numbers of symbionts adhering to theirsurfaces.

View larger version (61K): [in this window] [in a new window]   Figs. 2–4. Laboratory gall induction. 2. Induction site with newly forming gall visible underneath (g) 3. Cross section of a gall induction site at ~6 wk showing lateral proliferation of gall induction. 4. Cross section of a control inoculation showing the algal cells involved in the healing response. Scale bars = 5 mm.

Fluorescentin situ hybridization of symbiotic bacteria
Whole-cell in situ hybridization was successful in confirming theidentity of the bacteria associated with all galls tested in nature andinduced in the laboratory as well as in characterizing the relativepercentage of eubacterial gall symbionts from induction homogenates.Bacteria from galls collected at Carmel and Lighthouse Pt., Santa Cruz,were hybridized by both S-S-P.l.sym-0949-a-A-25 andS-D-Bact-0338-a-A-18r. Agrobacterium and Roseobactercells included as controls were hybridized by S-D-Bact-0338-a-A-18r butnever S-S-P.l.sym-0949-a-A-25. Assays of gall induction homogenates(galls collected in nature) using S-S-P.l.sym-0949-a-A-25 identified arange of 85–90% (±3%) of the hybridizableeubacteria as the P. lanceolata symbiont (Table 2) (Figs. 5–6). The relativepercentage of eubacterial symbionts in homogenates prepared fromlaboratory-induced galls was 97% (±3%) (Table 2).

View larger version (90K): [in this window] [in a new window]   Figs. 5–6. Whole-cell in situ hybridization of bacterial symbionts with S-D-Bact-0338-a-A-18 and S-S-P.l.sym-0949-a-A-25. 5. Hybridized gall induction homogenate upon 560 nm excitation (TAMRA). Note labeled bacteria (arrowheads) and autofluorescent particles (p). 6. The same field of view upon 510 nm excitation (fluorescein). Autofluorescent particles and a number of eubacterial cells hybridized by S-D-Bact-0338-a-A-18 are no longer evident (arrowheads). Scale bars = 15 µm.

Light andepifluorescence microscopy
Several distinct cell layers were seen in cross sections ofunaffected P. lanceolata thallus (Fig. 7). The epidermal region oftightly packed cells was subdivided into epidermal cortex and corticallayers, which were underlain by a loosely woven, filamentous medulla.The epidermal cortex was composed of 3–4 layers of tightly packed,isodiametric cells (5–10 µm), each of which was derived fromthe cortex, a region composed of 3–5 cell layers of increasingdiameter (10–50 µm). Cells in this region formed extensivesecondary pit connections with each other. The central region of theunaffected P. lanceolata thallus was composed of a loose,filamentous medulla (Figs.7–8). Thallus expansion during growth resulted in a"network" of cells composed of stellate regions connected byfilamentous projections (Fig.8).

View larger version (173K): [in this window] [in a new window]   Figs. 7–11. Healing response observed in control inoculations of P. lanceolata thalli. 7. The normal appearance of P. lanceolata vegetative epidermis (e), cortex (c), and medulla (m) in cross section. The early stages of gall formation are evident deep within the thallus interior (g). Scale bar = 125 µm. 8. Longitudinal section of the P. lanceolata medulla, unaffected thallus. Cells that have fused during the process of secondary pit connection formation are elongated during normal growth of the thallus (solid arrow). Scale bar = 40 µm. 9. Cross section of a healing P. lanceolata control inoculation reveals the invasion of the wound site (ws) by unspecified bacteria and the algal wound response, which has sealed off the thallus interior. Scale bar = 125 µm. 10. Cross section of the algal healing response illustrating cortical cell division and the subsequent anticlinal organization of newly produced cell files with respect to the wound site. Scale bar = 60 µm. 11. Cross section of dead algal cells (dc) filled with unspecified, invasive bacteria (solid arrow) that are excluded from the thallus interior during the algal healing response. Despite extensive bacterial invasion the dead algal cells trapped by the healing response maintain a relatively normal cell morphology. Scale bar = 60 µm.

View larger version (210K): [in this window] [in a new window]   Figs. 12–17. Gall formation in P. lanceolata in response to bacterial symbiont invasion. 12. Cross section of algal medullary cell proliferation ~2 wk postinoculation. Scale bar = 20 µm. Note the formation of bud initial cells by medullary filaments (solid arrows) in the region of gall induction 13. Cross section of developing gall within algal thallus. The disorganized production of cell files occurs with no particular orientation relative to surrounding unaffected cells (solid arrows). Scale bar = 40 µm. 14. Cross section of gall-affected cells showing extensive secondary connections between gall-induced Prionitis cortical and subcortical cells (solid arrows). Scale bar = 20 µm. 15. DAPI-stained cross section of an expanding gall. The proliferation of symbiont cells (solid arrow) into the intercellular spaces adjacent to the forming gall is apparent. Scale bar = 40 µm. 16. DAPI-stained cross section of a newly forming gall (~2 wk) within the base of an inoculation site. The proliferation of bacterial symbionts into intercellular spaces (solid arrow) and the division of an algal cortical cell nuclei are apparent. The volume of the vacuole within the gall induced cell has been much reduced. Scale bar = 20 µm. 17. Cross section of dividing medullary cells (solid arrows). Scale bar = 20 µm.

Gall-induced medullary cells and bacterial symbionts were foundconsistently in close proximity to each other, suggesting that contactmay be involved in the induction response (<5 µm) (Fig. 17). Symbiotic bacteria were alsoassociated with the hypertrophy and hyperplasia of algal cortical andsubcortical cells, although specific cell-to-cell contact was notobserved in all cases (Figs.18–20). In regions adjacent to and surrounding gallproliferation (<20 µm) filamentous medullary cells that did notappear affected (these cells retained their normal elongate morphologyand were not induced to divide or produce bud initial cells) bybacterial infection were physically displaced by the expanding gall(Fig. 21).

View larger version (212K): [in this window] [in a new window]   Figs. 18–22. Cellular responses observed in gall formation. 18. A grazing cross section of cortical (c) cell division induced by symbiotic bacteria (solid arrow) at the base of an inoculation site ~2–3 wk postinduction. Scale bar = 20 µm. 19. Cross section of an expanding gall. The hypertrophic response of a cell from the algal cortex in response to the presence of symbiotic bacteria has resulted in the production and ramification of filaments of this induced cell with the forming gall callus (solid arrows). Scale bar = 15 µm. 20. Cross section of induction, division, and extensive secondary connection of gall-affected cortical cells ~6 wk postinduction. Scale bar = 40 µm. 21. Cross section of gall formation ~4 wk postinduction. Unaffected medullary cells adjacent to the expanding gall have been shunted aside (solid arrows). Scale bar = 100 µm. 22. Symbiotic bacteria appear intracellular in this image (ic). Medullary cells in several adjacent regions have also been induced to form bud initial cells and secondary pit connections by nearby symbiotic bacteria (solid arrows). Scale bar = 125 µm.

In situ hybridization: paraffin sections using adigoxigenin-labeled oligonucleotide
Hybridization of both field-collected and laboratory-induced gallswith S-S-P.l.sym-0949-a-A-25 localized a single intercellular bacterialmorphotype (Fig. 23).Hybridized cells were uniform and of the same size as whole cellshybridized in gall induction homogenates. The Alvinellaepibiont probe did not hybridize to any bacteria in sections of P.lanceolata galls (Fig.24). No bacteria were detected in sections not hybridized withan oligonucleotide. This confirmed the specificity of the colorimetricdetection method used (data not shown). Similarly, hybridization ofnegative control wound sites with S-S-P.l.sym-0949-a-A-25 did not detectthe gall bacterium. The gall symbiont was also localized in sections ofdeveloping, laboratory-induced galls (2–3 and 6 wk postinduction)(Figs. 25–28). Nobacteria in these sections were detected either by hybridization withthe Alvinella epibiont-specific probe or in the absence of anoligonucleotide.

View larger version (209K): [in this window] [in a new window]   Figs. 23–28.  In situ localization of P. lanceolata symbiotic gall bacteria. 23. Bacterial symbionts (solid arrow) are localized intercellularly in a cross section of a gall collected from nature. Scale bar = 25 µm. 24. Cross section of an in situ hybridization of a control inoculation site. No bacteria are hybridized by the species-specific Alvinella pompeijana symbiont probe. Scale bar = 40 µm 25. Cross section of a laboratory gall induction site ~2 wk postwounding. Hybridized bacteria are present basally in the wound site (solid arrow). Scale bar = 150 µm. 26. Close-up of the inoculation site depicted in Fig. 25 . The disorganized growth and proliferation of algal cells in this region are evident (ws). Scale bar = 40 µm. 27. Cross section of a forming gall after ~4 wk. Symbiotic bacteria are absent from the region of unaffected algal cells (u). Scale bar = 20 µm. 28. Cross section of a forming gall mass (g) trapped beneath a healed inoculation site (ws) (~5 wk). Note again the restriction of symbionts to gall-affected regions of the thallus interior. Scale bar = 60 µm.

Transmissionelectron microscopy
Despite an extensive survey of laboratory-induced galls (2 and 4 wkpostinoculation) no evidence of an intracellular stage of bacterialproliferation was observed. Gall-affected cells contained reducedvacuoles and enlarged plastids in comparison to nonaffected cells.Symbiotic bacteria were found consistently in intercellular spaces andwere always surrounded by an electron-transparent region. This regionformed an external layer similar in appearance to other bacterialexopolysaccharide layers, making complete infiltration of gall tissuesextremely problematic and resulting in the intermittent loss ofbacterial cells from sections.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
The causative role of a specific microorganism in the formation ofgalls on P. lanceolata, without prior cultivation andisolation, has been established by application of a whole-cell in situhybridization methodology. Briefly stated, the strict satisfaction ofKoch's postulates for the demonstration of the causative agent indisease requires the following. The suspected agent must always be foundin association with the expressed symptomology, isolated and identifiedfrom the disease, reinoculated to demonstrate reformation of thedisease, and ultimately reisolated and reidentified (Andrews and Goff, 1985). In this investigation,modification of Koch's postulates was required as this gallsymbiont has yet to be cultured or reliably cultivated using standardmicrobial techniques. In the context of the P. lanceolata gallsymbiosis, disease may be viewed as an intimate association thatmanifests pathogenic symptoms and may involve a necrotrophism in therelationship of one symbiont to the other.

The metabolic consequences of gall formation for either P.lanceolata or its bacterial symbiont remain unknown. Thehypertrophied growth of gall-induced algal cells apparently provides adesirable microhabitat for the growth and proliferation of the bacterialsymbiont. Observations of the host alga in nature, however, suggest thatthere is little to no ecological consequence to the gall-bearing thallus(Ashen, personal observations). The subtidal population at Pacific Grovecontains both gall and nongall-bearing individuals, which can be eithersmall, perennating thalli or large (>1 m) 1st-yr thalli regardless ofbacterial presence. The extent of gall formation on a particularindividual is extremely variable but ranges from several (5–10)galls to hundreds of galls per thallus, irrespective of size.Gall-affected thalli were not obviously different from nonaffectedindividuals except for the localized effects of gall formation (Ashen,personal observations).

Gall formation in nature appears to affect between 45 and 70%of the thalli from a given location (Apt and Gibor,1989). Extensive collection of P. lanceolatathroughout California suggests that gall formation is common on algalthalli (perhaps >80%) from low intertidal to subtidal zones,which experience moderate to high wave action (Ashen, personalobservations). Thalli in other littoral regimes were rarely observed tobear galls.

The genus Prionitis is highly pleiomorphic with the speciesP. lanceolata being an extreme example. Thallus morphology isapparently related to position within the intertidal, with lowerintertidal and subtidal thalli manifesting a more cylindrical and lessbranched habit (Abbott and Hollenberg,1976). Galls were consistently found on thalli of thismorphology and were never observed on mid-to-high intertidal individualscharacterized by flatter, wider blades and increasing proliferation ofmarginal bladelets.

The presence of a single, predominant eubacterial phylotype (16s rDNAsignature) was confirmed on all collected individuals of P.lanceolata from in and around Monterey Bay, California. Thespecies-specificity of particular regions of the 16S rDNA sequence hasbeen demonstrated and widely applied to the investigation of specificmicroorganisms in a wide range of symbiotic associations (Amann et al., 1991; Distel, DeLong, and Waterbury, 1991; Cary et al., 1993; DeLong,1993; Hahn, Amann, and Zeyer,1993; Amann, Ludwig, and Schleifer,1995; Dubilier et al.,1995; Fischer et al., 1995;Ashen and Goff, 1996; Bianciotto et al., 1996). Gall formation onP. lanceolata has not been found in the absence of theidentified gall symbiont. This supports the hypothesis that gallformation is a species-specific phenomenon requiring the presence of aparticular eubacterium and satisfies Koch's first postulate for thedemonstrated presence of the disease agent in all cases of manifestsymptomology.

The predominant eubacterium identified in induction homogenates fromgalls collected in nature (85–95%) was the P.lanceolata proteobacterial symbiont. The low percentage ofextraneous eubacteria detected in these homogenates were undoubtedlybacterial epiphytes, ubiquitous among intertidal algae (Provasoli and Pintner, 1980; Tatewaki, Provasoli, and Pintner, 1983;Shiba, 1992). Laboratory induction usingthe above homogenates showed a significant correlation between thepresence of the identified symbiotic eubacterium and gall formation.Wound sites that were inoculated with sterile seawater formed galls asmall percentage of the time (4%). This was likely due to theincubation of P. lanceolata blade tips in ambient seawater. Theassumption at present is that the gall symbiont is present in the watercolumn and was able to enter the wound sites of the control bladesbefore they had healed.

In situ identification of the P. lanceolata symbiont fromgalls collected in nature satisfies Koch's second postulate byidentifying the suspected disease agent. The need for pure cultureisolation has been required traditionally to ensure that only a singleorganism is involved in reinfection trials. In this case moleculartechniques were used to identify an uncultivable microorganism andmonitor that organism in re-infection trials. While not the onlyeubacterium present in "natural" induction homogenates, theidentified gall symbiont was the numerically predominant microbe and wassubsequently identified in situ, in proliferating stages of thereforming association.

Whole-cell in situ hybridization of the gall symbiont withS-S-P.l.sym-0949-a-A-25 confirmed the presence of this specificeubacterium in laboratory-induced galls Symbionts in homogenates ofinduced galls comprised a higher percentage of the hybridizableeubacteria than in homogenates of galls collected in nature(97%). This was probably due to removal of these galls fromaffected thalli shortly after eruption through the thallus surface,affording epiphytes only a short time for colonization. Localization ofthe bacterial symbiont was performed in section throughout the course ofthe induction trials. The in situ monitoring, during consecutive roundsof laboratory induction, satisfies Koch's third and fourthpostulates by demonstration of the disease symptomology in the reformedassociation in response to the presence of a specific, suspected diseaseagent.

The overall timing of cellular events involved in gall developmentand formation may be characterized as follows. The production ofepidermal cell layers from the cortex adjacent to the inoculation siteis generally complete within 2–4 wk, sealing the thallus interiorfrom the external environment. In situ hybridization confirms that theeubacteria lying within the wound site and observed to proliferateintercellularly from the inoculation site are the gall symbiont.Bacterial induction of algal hypertrophy does not appear to be localizedin one region of the wound site but is related to symbiont proximity.Expansion of gall-induced tissues continues within the thallus throughthe 4th wk, with increasing numbers of cells of the algal cortex,subcortex, and medulla induced to hypertrophy and hyperplasia by contactwith the proliferating gall. The finding of cortical cell induction hasnot been reported elsewhere where red algal gall induction anddevelopment have been examined.

Eruption of the gall mass through the algal epidermis occurs~8–12 wk after inoculation. Release from the thallus exterioris followed by a marked change in the orientation of gall-induced cells,with growth expanding externally in anticlinal, albeit irregular filesto form the gall mass observable in nature. This is an apparentlyphysical response resulting from the release of pressure on theexpanding gall mass once the surface of the algal thallus has beenbreached.

The evidence presented here demonstrates the causative role of aspecific eubacterial phylotype in gall induction and formation on P.lanceolata. This microorganism is associated with all cases of gallformation on P. lanceolata. It can be specifically identifiedand comprises the vast majority of metabolically active bacterial cellsin homogenates from field-collected and laboratory-induced galls. Thepresence of this eubacterium is significant for the reformation of thegall symbiosis, and this microbe has been identified in situ, as theonly eubacterium present in consecutive rounds of gall induction andformation.

	FOOTNOTES

 
¹ The authors thank Bill Sullivan, Charles Daniel, Diane Okamuro, Betsy Steele, Jonathan Krupp and the Microscopy and Imaging Facility, Guessippee Zuccarello, Debbie Moon, David Garrison, and Marcia Gowing (UCSC). Funds for this research and publication were provided by the Office of Naval Research-Assert (grant number N00014-92-J-1462) and by the National Science Foundation (Systematic Biology Program number BSR 940411) to L.J.G. and by Friends of Long Marine Lab, Sigma Xi and the UCSC Department of Biology grants to J.B.A.

² Author for correspondence, current address: Mail Stop 239-12, NASA/Ames Research Center, Moffett Field, CA 94035-1000.

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