ULTRASTRUCTURE AND CYTOCHEMISTRY OF EARLY SPERMATANGIAL DEVELOPMENT IN ANTITHAMNION NIPPONICUM (CERAMIACEAE,RHODOPHYTA)1

Spermatial development and differentiation of wall components were investigated by electron microscopy and cytochemical methods in Antithamnion nipponicum Yamada et Inagaki. The spermatium is composed of two parts, a globular head and two appendages projecting from near the basal portion. The appendages originate form spermatangial vesicles (SVs) and follow a developmental sequence beginning as amorphous material and ending as fully formed fibrous structures compressed with in the SVs. SV formation is due to contributions initially from endoplasmic reticulum and later form dictyosome-derived vesicles. Chemical differentiation of the spermatial wall occurs early in its development. Calcofluor white ST does not label spermatial walls, indicating an absence of cellulose polysaccharides, which are abundant in vegetative cell walls. Labeled lectins show that α-d -methyl manose and / or α-d -glucose as well as N-acetyl-glucosamine, β-d -galactose, and α-l -fucose moieties are present on the spermatial wall but not in the vegetative cell wall. The glyconjugate with α-d -methyl mannose and / or glucose residues, previously reported as a gamete recognition molecule in this species, is distributed along the surface of spermatia as well as in the SV during spermatangial development.     

STUDIES ON DEVELOPING AND RELEASED SPERMATIA IN THE RED ALGA,TIFFANIELLA SNYDERAE (RHODOPHYTA)1

Developing and released spermatia of the red alga, Tiffaniella snyderae (Farl.) Abb. were studied. Spermatia were observed under hydrodynamically defined conditions and found to be released from the exposed spermatangial heads in a spermatium-plus-strand unit that remained connected to the spermatangial head. Interactions of single-spermatial strands resulted in the formation of multi-spermatial strands as long as 600 μm with as many as 47 spermatia along their length; however, most were 100–200 μm with 8–21 spermatia. Strand length and number of spermatia were correlated. Spermatial strands contracted or extended and rotated as the water velocity past the plant was changed, and in still water the strands retracted into a clump on the spermatangial head surface. Each strand type exhibited a characteristic threshold water velocity at which it reached maximum length, and above which it broke and was carried away. Fluorescence microscopy showed that the strands did not contain nucleic acid (DNA) and could thus be differentiated from filamentous blue-green algal and bacterial epiphytes. Histochemical staining indicated that the strands and spermatial vesicles contained an acidic, sulfated polysaccharide. Chelation of Ca²⁺ with EGTA resulted in strand breakdown suggesting that this divalent cation may be involved in strand integrity. Scanning electron microscopy revealed that release from the spermatangia occurred through tears in the cuticle covering the spermatangial head if it was still present, or from exposed spermatangia. Individual spermatia were attached tangentially to a well-defined strand 0.64 μm in diameter in the contracted state to 0.2 μm in the extended state. Transmission electron microscopy of spermatangial heads showed that immature spermatangia were characterized by a centrally positioned nucleus and abundant ER cisternae filled with a moderately electron dense granular material. Later in development the spermatangia acquire two spermatial vesicles containing highly convoluted fibrillar contents. The cell becomes polarized with the nucleus displaced apically and the spermatial vesicles occupying the basal half of the spermatangium. At maturity one of the vesicles is released basally. Liberated spermatia contain a membrane-bound nucleus and mitochondria and are associated with an oblong accumulation of fibrous material similar in size and position to the strand observed with the SEM. These strands are discussed in relation to red algal fertilization and other phases of the red algal life-history.     

ELECTRON MICROSCOPIC OBSERVATIONS ON THE DIFFERENTIATION AND RELEASE OF SPERMATIA IN THE MARINE RED ALGA POLYSIPHONIA HENDRYI (CERAMIALES,RHODOMELACEAE)

Spermatial differentiation in Polysiphonia hendryi begins after nonpolar, avacuolate spermatia are cleaved from their mother cells. The spermatia and their mother cells are embedded within the spermatangium, a confluent wall matrix of the male branch. As the young spermatium enlarges and becomes ellipsoid, the wall fibrils of the spermatangium are compressed, forming a separating layer. Spermatia become polar with rough endoplasmic reticulum coalescing to form a large, fibrillar spermatial vacuole that becomes extracytoplasmic in later development. Following spermatial vacuole formation, dictyosomes form and deposit a spermatial wall, severing the spermatial mother-cell pit connection. Enlargement of younger spermatia, which are lateral to the older ones, squeezes the maturing spermatia, pushing them from the male branch, and leaving a scar that compresses and heals. Through this release mechanism, new sites are created for additional spermatial proliferation.     

Unusual structures in the spermatial vesicles of the red algaErythrocystis montagnei

Electron microscopic observations on the membrane of the spermatial vesicles in the red algaErythrocystis montagnei are presented. A portion of this membrane is modified and more electron dense, with a layer of microtubules of about 20 nm. Generally, this membrane portion forms two paired bulges, appearing 3-shaped in cross-section. More rarely, two completely separate cylindrical bodies of about 0.3 µm diam. surrounded by membranes have been observed in the spermatial vesicles. The significance of these structures as possible vestigial remnants of flagella is discussed.     

ATTACHMENT AND FUSION OF GAMETES DURING FERTILIZATION OF PALMARIA SP. (RHODOPHYTA)1

Fertilization of cultured microscopic female gametophytes by spermatia from field-collected male gametophytes of Palmaria sp. was observed by light and transmission electron microscopy. Liberated spermatia had a prophase-arrested nucleus with a pair of polar rings. The protoplast of spermatia was covered with ca. a 3-μm-thick hyaline covering. After spermatium inoculation, the spermatial covering was attached specifically to the coat surrounding the cell wall of the trichogyne. The spermatial covering was eliminated only at the site of gamete attachment, resulting in direct attachment of the spermatial plasma membrane to the trichogyne within 5 min after spermatium inoculation. This direct attachment was followed by completion of spermatial nuclear division and cell wall formation. The polar rings disappeared before prometaphase. The cytoplasm of the binucleate spermatium invaded the trichogyne cell wall and subsequently fused with the trichogyne cytoplasm. The trichogyne could fuse with many spermatia, and many male nuclei (the derivative nuclei of spermatial nuclear division) could enter the trichogyne cytoplasm.     

Fertilization and the cytoskeleton in the red alga Bostrychia moritziana (Rhodomelaceae,Rhodophyta)

Time-lapse videomicroscopy was used to observe the effects of various cytoskeletal inhibitors on three important fertilization events in Bostrychia moritziana: spermatial mitosis, gamete fusion (formation of a fertilization pore) and nuclear migration along the trichogyne. The microtubule inhibitor oryzalin disrupted spermatial mitosis but had no other effect on fertilization. The actin inhibitors, jasplakinolide, cytochalasin B, latrunculin A and B and mycalolide B inhibited gamete fusion while BDM, a myosin-disrupting drug, inhibited all three major fertilization events. FL-Phallacidin was used to stain actin filaments in spermatia and trichogynes while microtubules were labelled with antibodies at appropriate stages of fertilization. Microtubules were only evident during spermatial nuclear division. Actin filaments were present in both trichogynes and spermatia throughout fertilization; they formed a discrete ring around the fertilization pore and ensheathed male nuclei as the latter migrated into and along the trichogyne. These results suggest that the actin/myosin system plays a role in the events of fertilization.     

PROGRESSION OF SPERMATIAL NUCLEAR DIVISION REQUIRES CALCIUM INFLUX DURING FERTILIZATION OF THE RED ALGA PALMARIA SP.1

During fertilization of the red alga Palmaria sp. (Palmariales), the prophase-arrested nucleus of the uninucleate spermatium resumes its division after direct attachment of the spermatium to the trichogyne of a carpogonium. Treatments that reduce Ca²⁺ influx inhibit the progression of spermatial nuclear division. The ratio of the number of spermatia released from prophase arrest (those in meta-phase to binucleate stages) to the total spermatia attached to trichogynes was significantly reduced by incubating the spermatia in the culture solution having low Ca²⁺ concentration. Similar inhibition was observed by addition of either inorganic (La³⁺ and Co²⁺) or organic (nifedipine and tetramethrin) Ca²⁺ channel inhibitors to the culture solution containing 10 mM Ca²⁺. These results indicate that the prophase/metaphase transition of spermatial nuclear division requires an influx of Ca²⁺ and suggest that Ca²⁺ acts as a second messenger to the mechanical or chemical stimulus that initiates mitotic progression of spermatia in this alga.     

Gamete recognition during fertilization in a red alga,Antithamnion nipponicum

Summary Fertilization in the marine red algaAntithamnion nipponicum is a highly specific process involving non-motile male gametes, spermatia, and female receptive structures, carpogonia. FITC-lectin and Calcofluor white ST labelling show that the outer cell walls of spermatia differ from vegetative cells in carbohydrate composition. Specific binding of the lectins to spermatial walls was confirmed by lectin-gold labelling on thin sections. Gametic recognition inAntithamnion nipponicum is based on the interaction of a surface carbohydrate on the spermatia with a surface carbohydrate receptor on the trichogynes. Spermatial binding to trichogynes is inhibited by pre-incubation with concanavalin A and trichogyne receptors are blocked by the complementary carbohydrate -D-methyl mannose. The inhibitory effects of concanavalin A to spermatial binding of trichogynes is reversed by preincubation with -D-methyl mannose. The combination of long spermatial appendages and a carbohydrate-carbohydrate receptor-based gamete recognition mechanism make fertilization in this species an efficient process.     

ULTRASTRUCTURE OF SPERMATIUM LIBERATION IN THE MARINE RED ALGA PTILOTA DENSA1

The differentiation of male gametes of the marine red alga Ptilota densa was studied by electron microscopy. Mature primary spermatangia are enveloped by a single cell wall and possess a clearly polar subcellular organization. The nucleus is situated apical to large, striated, fibrous vacuoles which are apparently formed by the repeated fusion of dictyosome vesicles. The transformation and liberation of spermatia from spermatangia involve both the secretion of the fibrous vacuoles at the base of the cell and the subsequent rupturing of the spermatangial cell wall. Liberated spermatia are coated with a thin mucilage layer and contain numerous small vesicles and several mitochondria and dictyosomes. The nucleus is cup-shaped and generally lacks a limiting envelope. These findings are discussed in relation to other light and electron microscopic studies of differentiating spermatangia in red algae.     

THE ROLE OF F-ACTIN DURING FERTILIZATION IN THE RED ALGA AGLAOTHAMNION OOSUMIENSE (RHODOPHYTA)

The actin cytoskeletons in spermatia and trichogynes of Aglaothamnion oosumiense Itono were studied using fluorescein isothiocyanate (FITC) conjugated phalloidin and the cytoskeletal inhibitors, potassium iodide (KI), cytochalasin-B, and latrunculin-A. Microfilaments were localized to the distal ends of elongated spermatia and trichogynes and were more prominent in the trichogyne before spermatium binding. The actin cytoskeleton in spermatia and trichogynes was disrupted by treatment with 0.6 M KI, 100 μM cytochalasin-B, or 10 μM latrunculin-A. The actin cytoskeleton in trichogynes recovered within 24 h of removal from the inhibitor, but no recovery was observed in spermatia. Spermatial nuclei entered mitosis as soon as spermatia attached to the trichogyne. The greatest percentage (50%– 60%) of spermatia having completed mitosis was obtained at 60 min after spermatial binding to trichogynes. During mitosis, actin accumulated in the center of the spermatium, thereby separating the two daughter nuclei. Cytoskeletal inhibitors did not affect initial binding of spermatia to trichogynes but did block subsequent stages of fertilization, including spermatial mitosis and gamete fusion. The accumulation of cellulose or β-linked polysaccharide on the spermatial surface was also blocked by treatment with actin inhibitors. Exposure of the trichogyne to actin inhibitors after gamete fusion caused spermatial nuclei in trichogynes to stop moving and to condense. These results suggest that the microfilaments involved in nuclear division, cellulose deposition into the spermatial wall, gamete fusion, and migration of spermatial nuclei in trichogynes during fertilization in Aglaothamnion oosumiense.     

Fine structure of spermatial surface in the red alga Antithamnion nipponicum (Rhodophyta)

In the ceramiacean red alga Antithamnion nipponicum Yamada et Inagaki, the structure of the spermatial covering and appendages was examined using confocal laser scanning microscopy, scanning and transmission electron microscopy. The liberated spermatium was subspherical, ca 4.5 μm in size with a colorless covering 2.7–3.0‐μm thick. Two flexible, ribbon‐like appendages arose from the periphery of the spermatial covering. The appendages averaged 80 μm in length and were 0.5–0.6 μm width in most parts. Each appendage consisted of a number of thin longitudinal fibrils. Concanavalin A conjugated with fluorescein isothiocyanate, colloidal gold orferritin, bound specifically with the inner layer of spermatial covering and spermatial appendages. When the liberated spermatia were incubated with mature female gametophytes, the spermatial appendages entangled around the tricho‐gyne.     

LEACHIELLA PACIFICA,GEN. ET SP. NOV., A NEW PARASITIC RED ALGA FROM WASHINGTON AND CALIFORNIA

Leachiella pacifica, gen. et sp. nov., a marine alloparasitic red alga is described from Washington and California. Several species of Polysiphonia and Pterosiphonia are hosts for this parasite. The thallus is a white, multiaxial, unbranched pustule with rhizoidal filaments that ramify between host cells, forming numerous secondary pit connections with host cells. All reproductive structures develop from outer cortical cells. Tetrasporocytes, situated on stalk cells, undergo simultaneous, tetrahedral cleavage to form tetraspores. Spermatia are formed continuously by oblique cleavages of the elongate spermatial generating cells. This results in spermatial clusters consisting of 4–8 spermatia in an alternate arrangement. Carposporophyte development is procarpial. The carpogonium is part of a six-celled branch including a sterile cell that is formed by the basal cell. The carpogonial branch is attached laterally to an obovate supporting cell that also forms an auxiliary cell, presumably formed prior to fertilization. After fertilization the carpogonium temporarily fuses with the auxiliary cell apparently to transfer the diploid nucleus and initiate further fusion with the subtending supporting cell to form an incipient fusion cell. The auxiliary cell portion of this fusion cell divides to form gonimoblast initials that continue to divide, forming gonimoblast filaments whose terminal cells differentiate into carpospores. The remainder of the fusion cell enlarges by continual fusion with adjacent vegetative cells. The resultant carposporophyte consists of a basal, multinucleate fusion cell supporting a hemispherical cluster of gonimoblast filaments with terminally borne carpospores. Vegetatively, Leachiella resembles several other parasitic red algae but it is clearly separated by the procarp, carposporophyte development and structure, and tetrasporocyte cleavage.     

THE ULTRASTRUCTURE OF CARPOSPOROGENESIS IN THE MARINE HEMIPARASITIC RED ALGA ERYTHROCYSTIS SACCATA1

The ultrastructure of carposporogenesis for Erythrocystis saccata is described. The fusion and gonimoblast cells contain few organelles, and chloroplasts are in a proplastid state, with pit plugs between gonimoblast cells dissolving early in development. Carpospore development may be separated into 3 stages, the first stage being characterized by the appearance of straight-profiled dictyosomes, fibrous vesicles, and an increase of discoid thylakoids within the chloroplasts. During the second, stage the dictyosomes assume a curved profile and striped vesicles are formed by the endoplasmic reticulum. The third stage is initiated by the disappearance of striped vesicles and the appearance of straight-profiled dictyosomes secreting vesicles with cores. Mature carpospores consist of many cored vesicles, fibrous vesicles, and floridean starch grains. A single wall layer surrounds each carpospore since the carposporangial wall becomes incorporated into a mucilaginous matrix surrounding the spores.     

137 Gamete Recognition and Sexual Isolation in a Red Alga,Aglaothamnion Byssoides (Rhdophyta)

The binding of fluorescein isothiocyanate (FITC) conjugated lectins to gametes of Aglaothamnion byssoides Itono during the fertilization was studied by the use of confocal microscope. The physiological effects of lectins and carbohydrates on gamete binding were also examined. Three lectins, concanavalin A (ConA), Soybean agglutinin (SBA) and wheat germ agglutinin (WGA) bound to the surface of spermatia, but each lectin labeled different region of the spermatium. SBA bound only to the spermatial appendages but ConA bound to the whole spermatial surface except spermatial appendages. WGA labeled narrow region which connects spermatial body and appendages. During fertilization, ConA and WGA specific substances on the spermatial surface moved towards the area contacting with trichogyne and accumulated on the surface of fertilization canal. Spermatial binding to trichogynes was inhibited by pre‐incubation of spermatia with SBA, while trichogyne receptors were blocked by the complementary carbohydrate, N‐acetyl‐D‐galactosamine. WGA and its complementary carbohydrate had little effect on gamete binding. For searching the step of sexual isolation, crossing experiment was performed between Aglaothamnion byssoides and twelve other red algal species. Results showed that the gamete recognition was genus‐specific: the gametes bound freely with their partners of the same genus. When two species from same genus were crossed, sexual isolation occurs gradually during the fertilization process. Therefore, sexual isolation in red algae appears to be determined by multi‐step process and gamete binding is the initial step.     

80 Purification and characterization of male and female gamete recognition molecules of a marine red alga aglaothamnion oosumiense

In red algae, fertilization begins with gamete‐gamete contact between the trichogyne cell wall of the female carpogonium and spermatial coverings. During the fertilization in Aglaothamnion oosumiense, reproductive cells interact with each other through sex specific adhesion molecules on the surface of spermatia and trichogyne. The gamete binding is highly selective suggesting the presence of recognition factors along their surfaces. In the previous studies, we have reported that spermatial binding to trichogynes of a red alga, Aglaothamnion oosumiense is mediated by a lectin‐carbohydrate complementary system. Spermatial binding to trichogynes was inhibited by pre‐incubation of trichogynes with N‐acetyl‐D‐galactosamine and D‐glucose and hence lectins specific to these sugars were expected to present on the surfaces of trichogyne cell wall. We have isolated a new lectin from Aglaothamnion oosumiense by the use of agarose bound N‐acetyl‐D‐galactosamine affinity chromatography and named it as rhodobindin. Rhodobindin agglutinated human erythrocytes as well as spermatia of Aglaothmanion oosumiense. The agglutinating activity of this lectin was inhibited by N‐acetyl‐D‐galactosamine and N‐acetyl‐D‐glucosamine. SDS‐PAGE results showed that this lectin may be monomeric. The molecular weight was determined as 21,876 dalton by matrix‐assisted laser desorption ionization (MALDI) mass‐spectrometry. N‐terminal amino acid sequence of the lectin was analyzed and revealed to have no identity with those of known proteins. The complementary male glycoprotein was also isolated and purified by the use of SBA‐agarose affinity chromatography. The subtractive cloning was carried out to characterize the recognition molecules.     

Isolation and Characterization of a Sex-Specific Lectin in a Marine Red Alga,Aglaothamnion oosumiense Itono

In red algae, spermatial binding to female trichogynes is mediated by a lectin-carbohydrate complementary system. Aglaothamnion oosumiense is a microscopic filamentous red alga. The gamete recognition and binding occur at the surface of the hairlike trichogyne on the female carpogonium. Male spermatia are nonmotile. Previous studies suggested the presence of a lectin responsible for gamete recognition on the surface of female trychogynes. A novel N-acetyl-d-galactosamine-specific protein was isolated from female plants of A. oosumiense by affinity chromatography and named AOL1. The lectin was monomeric and did not agglutinate horse blood or human erythrocytes. The N-terminal amino acid sequence of the protein was analyzed, and degenerate primers were designed. A full-length cDNA encoding the lectin was obtained using rapid amplification of cDNA ends-PCR (RACE-PCR). The cDNA was 1,095 bp in length and coded for a protein of 259 amino acids with a deduced molecular mass of 21.4 kDa, which agreed well with the protein data. PCR analysis using genomic DNA showed that both male and female plants have this gene. However, Northern blotting and two-dimensional electrophoresis showed that this protein was expressed 12 to 15 times more in female plants. The lectin inhibited spermatial binding to the trichogynes when preincubated with spermatia, suggesting its involvement in gamete binding.     

ULTRASTRUCTURE OF TETRASPOROGENESIS IN THE PARASITIC RED ALGA LEVRINGIELLA GARDNERI (SETCHELL) KYLIN12

Ultrastructural studies on tetraspore formation in Levringiella gardneri revealed that 3 stages may be recognized during their formation. The youngest stage consists of a uninucleate tetraspore mother cell with synaptonemal complexes present during early prophase of meiosis I. Mitochondria are aggregated around the nucleus, dictyosome activity is low, and chloroplasts occur in the peripheral cytoplasm. A 4-nucleate tetraspore mother cell is formed prior to tetrahedral cell cleavage, and an increase in the number of chloroplasts and mitochondria occurs. Small straight-profiled dictyosomes secrete vesicles into larger fibrous vesicles or contribute material to the developing tetraspore wall. During the second stage of tetraspore formation, striated vesicles form within endoplasmic reticulum, semicircular profiled dictyosomes secrete vesicles for fibrous vesicles or wall material, and starch formation increases. The final stage is characterized by the disappearance of striated vesicles, presence of straight, large dictyosomes which secrete cored vesicles, and an abundance of starch grains. Cleavage is usually complete at this stage and the tetraspore wall consists of a narrow outer layer of fibrillar material and an inner, electron transparent layer. These spores are surrounded by a tetrasporangial wall which was the original wall surrounding the tetraspore mother cell.     

138 Molecular Evolution of Glutamine Synthetase In Protists

The binding of fluorescein isothiocyanate (FITC) conjugated lectins to gametes of Aglaothamnion byssoides Itono during the fertilization was studied by the use of confocal microscope. The physiological effects of lectins and carbohydrates on gamete binding were also examined. Three lectins, concanavalin A (ConA), Soybean agglutinin (SBA) and wheat germ agglutinin (WGA) bound to the surface of spermatia, but each lectin labeled different region of the spermatium. SBA bound only to the spermatial appendages but ConA bound to the whole spermatial surface except spermatial appendages. WGA labeled narrow region which connects spermatial body and appendages. During fertilization, ConA and WGA specific substances on the spermatial surface moved towards the area contacting with trichogyne and accumulated on the surface of fertilization canal. Spermatial binding to trichogynes was inhibited by pre-incubation of spermatia with SBA, while trichogyne receptors were blocked by the complementary carbohydrate, N-acetyl-D-galactosamine. WGA and its complementary carbohydrate had little effect on gamete binding. For searching the step of sexual isolation, crossing experiment was performed between Aglaothamnion byssoides and twelve other red algal species. Results showed that the gamete recognition was genus-specific: the gametes bound freely with their partners of the same genus. When two species from same genus were crossed, sexual isolation occurs gradually during the fertilization process. Therefore, sexual isolation in red algae appears to be determined by multi-step process and gamete binding is the initial step.     

Differentiation of Male Gametes in Gracilaria verrucosa (Rhodophyta, Gracilariales)

The development of male gametes (spermacia) in the red alga Gracilaria verrucosa has been studied using methods of transmission electron microscopy. Early spermatangia located along the wall of the conceptacle show an elongated shape in the thin sections. In the central part of the electron-dense cytoplasm of these cells there is a nucleus; numerous fibrous vesicles are arranged in the periphery. During the process of differentiation, the spermatangia become more rounded in shape and a large spermatangial vesicle is developed. The subsequent development of spermatium is accompanied by polarization of the spermatangium and the subsequent excretion of the spermatangial vesicle. The spermatia are oval cells containing a nucleus and fibrous vesicles. The process of differentiation of male gametes in G. verrucosa does not differ from that in five species of the genus Gracilaria, where it has already been studied. However, any conclusions about the degree of similarity between the spermatia in all the studied species can be made only after a detailed comparative analysis of the ultrastructural characteristics of these gametes.     

Ultrastructure,biogenesis, and functions of extrusive organelles in selected non-ciliate protists

Summary The ultrastructural features, biogenesis and functions of several selected protist extrusive organelles are discussed. Most of the review focuses on some common extrusive organelles that were not considered by Hausmann and several types which have been described since that review of 16 years ago. For convenience, extrusomes are categorized as projectile or mucocyst extrusomes. The projectile extrusomes are further subdivided into non-penetrating and cell penetrating extrusomes. This review is restricted to projectile extrusomes such as ejectisomes, the microsporidian invasion apparatus, and the gun cell of oomycetes. Mucocysts include the apicomplexan rhoptries, the K₂ bodies of oomycetes, and the spermatial vesicles and adhesive vesicles of red algae. The possible phylogenetic importance of some extrusive organelles is briefly considered.