The sporophyte-gametophyte junction in the moss Acaulon muticum (Pottiaceae): EARLY STAGES OF DEVELOPMENT

The sporophyte-gametophyte junction in Acaulon muticum is composed of the sporophyte foot, the surrounding gametophyte vaginula, and an intervening placental space. At an early stage of development the foot has a large basal cell, characterized by extensive wall ingrowths beginning at the lowermost tip of the basal cell and extending along its tangential walls. Sporophyte cells in contact with the basal cell develop ingrowths on their outer tangential walls and on radial walls in contact with the basal cell. All sporophyte cells at this stage are characterized by numerous mitochondria, strands of endoplasmic reticulum, and dictyosomes, particularly in the cytoplasm adjacent to areas of extensive wall development. Plastids typically contain abundant starch reserves. As development proceeds, wall ingrowths become more extensive on all walls in the sporophyte foot but are never found on the upper wall of the basal cell in contact with the remainder of the sporophyte. Plastids in the foot contain fewer starch reserves later in development. Wall ingrowths are not visible in the cells of the gametophyte vaginula until well after extensive development has occurred in the sporophyte foot. Stacks or layers of endoplasmic reticulum are characteristic of the cells of the gametophyte vaginula, along with numerous mitochondria, dictyosomes, and well-developed plastids. Starch reserves typically are less abundant in cells of the gametophyte. The early development of extensive wall elaborations in the cells of the sporophyte foot, and particularly in the basal cell, may favor the rapid movement of water and nutrients from the gametophyte into the sporophyte at a time when rapid development in this minute, ephemeral moss is critical.     

Ultrastructure and development of the gametophyte vaginula-sporophyte foot complex in the liverwort Targionia hypophylla L.

The development of the placental complex including the gametophyte vaginula and the bulbous foot of the sporophyte in the liverwort Targionia hypophylla L. (Marchantiales) was studied by transmission electron microscopy. The vaginula and foot are separated by an intervening space and each consist of parenchymatous cells without intercellular spaces. Transfer cells begin to differentiate at the gametophyte-sporophyte interface just prior the onset of meiosis. While a single epidermal transfer-cell layer has developed in the foot by the end of meiosis, a multilayered pattern of transfer cells is formed in the vaginula. Gametophyte transfer cells have wall labyrinths which decrease in complexity with distance from the foot, lack plasmodesmata, and show signs of degeneration in the proximity of the foot. During meiosis, amyloplasts of both vaginula and foot lack starch and develop some thylakoid grana. In the subsequent stage of spore maturation, obliteration of the wall labyrinth occurs in both gametophyte and sporophyte transfer cells. The developmental pattern of the placental complex in Targionia is discussed in relation to that of mosses.     

The development of the placenta in the anthocerote Phaeoceros laevis (L.) Prosk

The development of the placenta in the anthocerote Phaeoceros laevis (L.) Prosk. was studied by transmission electron microscopy. By the time the sporophyte emerges from the involucre, a conspicuous placental region is formed by the intrusive growth of sporophyte foot haustorial cells into the adjacent gametophyte vaginula tissue. The separation of gametophyte cells by haustorial cells and their incorporation into the placenta are preceded by the loosening and swelling of their walls and the formation of a periplasmic space. This process causes the disruption of the plasmodesmata, and may eventually result in the complete isolation and consequent degeneration of the cells. Crystals are commonly observed in the vacuoles of gametophyte placental cells. Crystals become more abundant during cytoplasmic degeneration, and are released in the placental lacunae that result from the complete dissolution of gametophyte cells. During the subsequent phase of capsule elongation, the gametophyte placental cells that retain the symplastic connection with the adjoining gametophyte parenchyma develop a wall labyrinth typical of transfer cells. Obliteration of the wall labyrinth by deposition of lightly staining wall material is observed later in sporophyte development, in concomitance with capsule dehiscence. Crystals are negative to the periodic acid/thiocarbohydrazide/silver proteinate test for carbohydrates whilst they are completely digested by pepsin or protease, denoting protein composition.Abbreviation PATAg periodic acid/thiocarbohydrazide/silver proteinate     

Differentiation of the Tapetum During Microsporogenesis in Tomato (Lycopersicon esculentum Mill.), with Special Reference to the Tapetal Cell Wall

During microsporogenesis and pollen maturation, the tapetumin anthers of tomato (Lycopersicon esculentum) underwent severalultrastructural changes and ultimately degenerated. The changesobserved related to the secretory function of the tapetum andto the transfer of materials from the cytoplasm to the surfaceof tapetal cells. Electron dense deposits, initially in thevacuoles, disappeared coincident with the appearance of orbiculeson the cell wall. The fibrillar wall of the tapetal cells loosened,presumably to facilitate transfer of materials through the wall.In Addition, membranous fragments were a consistent featurein the tapetum wall and may play a role in transport of materials.The cells of the inner tapetum (towards the connective) andouter tapetum (towards the epidermis) had different ultrastructuralfeatures. The cytoplasm of the outer tapetum was more electrondense and had a higher proportion of dictyosomes and mitochondriathan the inner tapetum, indicating the greater secretory natureof the outer tapetum. The plastids and mitochondria also differedin morphology between the two regions. Degenerations of thetapetal cytoplasm began by the vacuolate microspore stage. Atanthesis, cytoplasm was absent but the orbicular wall of thetapetum remained appressed to the wall of the middle layer ofthe anther.Copyright 1993, 1999 Academic Press Lycopersicon esculentum, microsporogenesis, pollen development, tapetum development, tomato, ultrastructure     

Seed Epidermis Development and Histochemistry in Solanum melongena L. and S. violaceum Ort.

Structure, development and histochemistry of the seed epidermiswere studied inSolanum melongena L. andS. violaceum Ort. usinglight and scanning electron microscopy. The epidermal cellsat the endosperm mother cell stage of ovule development hadthickened outer periclinal walls, consisting of two layers,a thin inner layer, and a thick outer layer. The latter whichstained positively for pectic substances became further thickenedduring the course of seed development; more so inS. melongena.The inner layer of the outer periclinal wall also was thickenedby depositions of cellulose but remained comparatively thin.The development of the inner periclinal and anticlinal wallstook place by the uneven deposition of concentric layers. Thesesecondary wall thickenings which appeared as pyramids in transversesection stained for cellulose, lignin and pectin. Further unevensecondary thickenings near the outer part of the anticlinalwalls resulted in the formation of projections which were hair-or ribbon-like in appearance. InS. melongena, these projectionsprogressed only a short distance from the anticlinal wall. InS.violaceum, on the other hand, they grew much longer formingstriations on the inside of the outer periclinal wall. InS.melongena, partial removal of the outer periclinal wall by enzymeetching exposed to surface view a beaded appearance of the cellboundaries. Complete erosion of the outer periclinal wall revealedthe hair-like projections of the underlying anticlinal walls.InS. violaceum, enzyme treatment exposed the striations whichformed bridge-like structures over the curves in the anticlinalwalls. Solanum melongena ; Solanum violaceum; seed epidermis; seed structure; seed development; cell wall histochemistry; cell wall projections; cell wall striations     

An Ultrastructural Study of The Embryo/Endosperm Interface in the Developing Seeds of Solanum nigrum L. Zygote to Mid Torpedo Stage

The early developmental sequences in the formation of the Zoneof Separation and Secretion in a hexaploid species of Solanumnigrum L. are described. Ultrastructural changes which occurredduring the development of the embryo/endosperm interface couldbe related to the different stages in the embryo's development.The first step was the completion of the cell wall around thechalazal end of the zygote; a thin wall was formed along theendosperm cell(s) abutting the zygote. From the mature zygotestage to the quadrant stage, minute plasmalemma invaginationsoccurred along the endosperm wall facing the zygote. These invaginationsenlarged, and from the mid-globular stage onwards became filledwith a fine fibrillar material; this material accumulated betweenthe endosperm cell wall and the plasmalemma before being releasedinto the developing periembryonic and intercellular spaces tobecome the extracellular matrix. Cell wall development in theendosperm cells abutting the embryo followed an unusual path.During the quadrant stage, whilst the outer embryo wall increasedin thickness due to vesicle fusion, the endosperm cell wallfacing the embryo showed a loosening of the wall fibrils aswell as partial separation of these same endosperm cells fromeach other. From the early-globular stage, the endosperm cellwalls opposite the embryo became electron-translucent, disappearinginto the extracellular matrix. Enzymic secretions by the embryomay account for the alteration in the abutting endosperm cellwalls. Enzymic activity may also explain the development ofa homogenous electron-opaque layer over the outer embryo wallas well as the differences in the width of the fibrillar layerwhich accumulated around the cotyledons as the embryo grew throughthe Zone of Separation and Secretion. The potential roles ofthe extracellular matrix are briefly discussed. Solanum nigrum L.; embryo/endosperm interface; Zone of Separation and Secretion; embryo development; cellular endosperm     

Wandlabyrinthe im Sporophyten von Polytrichum

Zusammenfassung Die Wandlabyrinthe im Sporophyten dreier Polytrichum-Arten (P. commune, P. formosum und P. juniperinum) wurden im Elektronenmikroskop untersucht.In den äußeren 4–6 Zellreihen des Sporogonfußes nimmt der Differenzierungsgrad des Labyrinthes radial von innen nach außen zu.Bei Polytrichum formosum wurde eine Beziehung der Protuberanzenentstehung zur Lyse der Zellwand gefunden.Die Protuberanzen besitzen Schichtbau, ebenso wie die Wand, aus der sie hervorgehen. Sie sind auch in der späteren, mächtigen Wandauflagerung an ihrem Kontrast kenntlich (Polytrichum commune). Bei Polytrichum formosum entstehen, ausgehend von diesen ursprünglich isolierten Protuberanzen, in den Wandvorsprüngen Zonen starken Kontrastes, deren Umrisse jeweils den Appositionsgrenzen zu folgen scheinen. Im Gegensatz dazu treten bei Polytrichum juniperinum in der Wandsubstanz kontrastreiche Einschlüsse auf, die keinerlei Beziehung zum ursprünglichen Bau des Wandlabyrinths zeigen. Die Menge dieser Einschlüsse scheint von der Wachstumsintensität des Sporophyten abzuhängen, und es wurde vermutet, daß es sich dabei um Exkrete handelt.In der Wandsubstanz waren die verschiedensten Strukturen zu beobachten, deren Herkunft und Entstehungsmöglichkeiten diskutiert wurden.

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Wall labyrinths in the sporophyte of Polytrichum

Summary In the foot of the Polytrichum sporophyte the outer walls of the peripheral cells are coated with a labyrinth. In the outer 4–6 cell layers protuberances arising from the lamellated cell wall were found which are interpreted as initial stages of the labyrinth. In Polytrichum formosum there is a correlation between the lysis of the cell wall and the initiation of new protuberances. In the outer cell layers the protuberances increase more and more and fuse. In the external cells large aggregations of wall substances are deposited, in which the protuberances are seen as electron dense cores. In the wall substances of the external cells there are large inclusions of an electron dense material, the accumulation of which seems to be in relation to the growth intensity of the sporophyt. Some structures enclosed in the wall material seem to be membraneous elements.

     

An ultrastructural and cytochemical study of the wall-membrane apparatus of transfer cells using freeze-substitution

Summary A freeze-substitution technique is described which enables the ultrastructure of certain types of plant transfer cells to be preserved with minimal ice crystal damage. The ultrastructure of transfer cells fromFunaria, Lonicera, andSenecio after freeze-substitution has been compared with that of glutaraldehyde-osmium fixed material. The irregular clear zone between wall and plasma membrane, present in conventional preparations, is absent in freeze-substituted tissue. It is proposed that this interfacial zone is an artefact caused by expansion of wall ingrowth material during conventional fixation procedures. In transfer cells with a complex wall labyrinth the swelling of wall material severely disrupts the true structure of the wall-membrane apparatus and results in a large decrease in the surface to volume ratio of the protoplast. These findings are supported in the case ofFunaria by a freezefracture study. The reactivity of the plasma-membrane to the PTA/chromic acid stain is enhanced in freeze-substituted material. Use of theThiéry silver proteinate reagent in conjunction with freeze-substitution has revealed marked differences between the wall ingrowths ofFunaria sporophyte haustorium transfer cells and those ofLonicera nectary trichomes.     

A cytochemical and immunocytochemical analysis of the wall labyrinth apparatus in leaf transfer cells in Elodea canadensis

Background and Aims

Transfer cells are plant cells specialized in apoplast/symplast transport and characterized by a distinctive wall labyrinth apparatus. The molecular architecture and biochemistry of the labyrinth apparatus are poorly known. The leaf lamina in the aquatic angiosperm Elodea canadensis consists of only two cell layers, with the abaxial cells developing as transfer cells. The present study investigated biochemical properties of wall ingrowths and associated plasmalemma in these cells.

Methods

Leaves of Elodea were examined by light and electron microscopy and ATPase activity was localized cytochemically. Immunogold electron microscopy was employed to localize carbohydrate epitopes associated with major cell wall polysaccharides and glycoproteins.

Key Results

The plasmalemma associated with the wall labyrinth is strongly enriched in light-dependent ATPase activity. The wall ingrowths and an underlying wall layer share an LM11 epitope probably associated with glucuronoarabinoxylan and a CCRC-M7 epitope typically associated with rhamnogalacturonan I. No labelling was observed with LM10, an antibody that recognizes low-substituted and unsubstituted xylan, a polysaccharide consistently associated with secondary cell walls. The JIM5 and JIM7 epitopes, associated with homogalacturonan with different degrees of methylation, appear to be absent in the wall labyrinth but present in the rest of cell walls.

Conclusions

The wall labyrinth apparatus of leaf transfer cells in Elodea is a specialized structure with distinctive biochemical properties. The high level of light-dependent ATPase activity in the plasmalemma lining the wall labyrinth is consistent with a formerly suggested role of leaf transfer cells in enhancing inorganic carbon inflow. The wall labyrinth is a part of the primary cell wall. The discovery that the wall ingrowths in Elodea have an antibody-binding pattern divergent, in part, from that of the rest of cell wall suggests that their carbohydrate composition is modulated in relation to transfer cell functioning.     

芡实种子萌发期子叶传递细胞发育的初步研究

芡实种子萌发期,子叶吸收外胚乳中养分供萌发和幼苗发育,具有吸器的功能。在种子萌发过程中,子叶的部分表皮细胞发育为传递细胞。其壁内突的生长以外切向壁为多,形成壁内突的造壁物质主要由高尔基体合成,并由其溢出的囊泡运送的。     

Ontogeny of external glands in the bladderwortUtricularia monanthos

Summary The development of external glands on traps and stolons ofU. monanthos has been studied using transmission electron microscopy. During early differentiation of the epidermis some cells remain narrow and develop a protuberance which subsequently divides into a terminal and a pedestal cell, with the remainder of the original cell forming the basal epidermal cell of the gland. The lateral wall of the pedestal cell soon becomes densely impregnated throughout its thickness, and this is followed by the formation of discontinuous cuticular deposits within the primary wall of the terminal cell. The outer wall of the terminal cell then usually undergoes extensive secondary wall thickening beginning with the formation of ingrowths which for a period characterize the cell as a transfer cell. Later, at the stage when traps begin capturing prey, these ingrowths are overlain by further layers of secondary wall material. Concomitantly, in the pedestal cell, wall ingrowths become fully differentiated on the outer transverse wall and persist throughout the remaining life of the gland.The function of external glands during early ontogeny is discussed. At the stage when the terminal cell is differentiated as a transfer cell it is suggested that the gland is mainly responsible for absorbing solutes from the external medium. Once traps commence capturing prey the gland may become modified for a rôle in water secretion, facilitated by the differentiation of the pedestal cell as a transfer cell, and by the formation of a thick outer wall in the terminal cell.     

Ultrastructure of the “fringe-layer”, the innermost epidermis of cotton seed coats

Summary The inner epidermis of the inner integument of cotton seed coats (fringe-layer) and the cuticles between this cell layer and the nucellus were examined in the light and electron microscope at different times of their development. The cells of the fringe-layer contain only small vacuoles and their cytoplasm is densely packed with organelles and free and membrane-bound polysomes. The lateral walls contain many plasmodesmata. At the time when the fruit capsules stop growing, the fringe-cells produce a cell wall labyrinth, resembling that of transfer cells. The cell wall labyrinth is restricted to the lateral walls. The differentiated state of the fringe-cells is short-lived. At about the time of elaboration of the cell wall labyrinth most of them become progressively vacuolated, lignify, and lose their cytoplasmic constituents. The development of the fringe-layer is well correlated with other developmental events in the inner integument, but not with the filling of embryo and endosperm with reserve substances.At anthesis, the fringe-layer and nucellus are covered by a thin cuticle proper of about 20 nm. After anthesis, the nucellar cells start to produce a cuticular layer of considerable, but variable, thickness (0.25–2.5 m), containing a polysaccharide network.In drying seeds the cells of the fringe-layer disrupt. The thin outer tangential wall remains attached to the seed coat. The rest of the cell, together with the cuticles and the collapsed cells of the nucellus, form a protective layer around embryo and endosperm, remaining attached to the seed coat at the chalazal end.     

Absorption of Some Amino Acids by Sporophytes Isolated from Polytrichum formosum and Ultrastructural Characteristics of the Haustorium Transfer Cells

The absorption of ¹⁴C-labelled amino acids (glycine, threonineand -aminoisobutyric acid) by the isolated sporophyte of Polytrichumformosum takes place mainly in the haustorium. The isolationof the sporophyte does not alter the absorption capacity ofits haustorium nor its ultrastructure, in particular that ofits peripheral transfer cells. amino acids, transfer cells, sporophyte, Polytrichum formosum, haustorium     

Transfer cells and flange cells in sinkers of the mistletoePhoradendron macrophyllum (Viscaceae), and their novel combination

Summary The unusual thick-walled cells in contact with host and parasite vessels, first noted by Calvin 1967 in sinkers (structures composed of tracheary elements and parenchyma that originate from parasite bark strands that grow centripetally to the host vascular cambium and become embedded by successive development of xylem) of the mistletoePhoradendron macrophyllum (Englem.) Cockerell, have been investigated by modern methods of microscopy. The wall is thickest in cells abutting large-diameter host vessels, less so against smaller host vessels and those abutting sinker vessels. Transmission electron microscopy reveals the wall to be complex, consisting of a basement primary wall, upon which two developments of secondary-wall material occur. These are represented by lignified thickenings, in the form of flanges, and a labyrinth of wall ingrowths characteristic of a transfer cell. The wall ingrowths occur mostly in the primary-wall regions between the flanges, but when in contact with a large host vessel the ingrowths also differentiate on top of the flanges. Cells with such a transfer cell labyrinth have not been previously reported in the endophytic system of a mistletoe. The cells are confined to the xylary portion of the primary haustorium and sinkers. InP. macrophyllum, however, the cells differ from ordinary transfer cells in that they have differentiated as part of a flange parenchyma cell. This arrangement represents a novel anatomical situation. The name flange-walled transfer cell is used for these cells. The xylem of primary haustorium and sinkers also contain numerous ordinary flange cells. In both flange-walled transfer cells and ordinary flange cells the flanges are lignified and form a reticulate pattern of thickenings, separated by rounded areas of primary pit fields. The extent of development of the flange wall can vary in different parts of a sinker. At the host interface, the existence of a flange-walled transfer cell in direct contact with a vessel reflects a site associated with high loading into the parasite. Similarly, a labyrinth against a sinker vessel indicates a site of unloading from surrounding sinker tissue into the vessel for subsequent longdistance transport within the parasite.Dedicated to the memory of Dr. Katherine Esau (1898–1997)     

Nucellar projection transfer cells in the developing wheat grain

Summary Transfer cells in the nucellar projection of wheat grains at 25 ±3 days after anthesis have been examined using light and electron microscopy. Within the nucellar tissue, a sequential increase in non-polarized wall ingrowth differentiation and cytoplasmic density was evident. Cells located near the pigment strand were the least differentiated. The degree of differentiation increased progressively in cells further removed from the pigment strand and the cells bordering the endosperm cavity had degenerated. Four stages of transfer cell development were identified at the light microscope level. Wall ingrowth differentiation followed a sequence from a papillate form through increased branching (antler-shaped ingrowths) which ultimately anastomosed to form a complex labyrinth. The final stage of wall ingrowth differentiation was compression which resulted in massive ingrowths. In parallel with wall ingrowth deposition cytoplasmic density increased. During wall deposition, paramural and multivesicular bodies were prominent and were in close association with the wall ingrowths. The degeneration phase involved infilling of cytoplasmic islets within the wall ingrowths. This was accompanied by complete loss of the protoplast. The significance of this transfer cell development for sucrose efflux to the endosperm cavity was assessed by computing potential sucrose fluxes across the plasma membrane surface areas of the nucellar projection cells. Transfer cell development amplified the total plasma membrane surface area by 22 fold. The potential sucrose flux, when compared with maximal rates of facilitated membrane transport of sugars, indicated spare capacity for sucrose efflux to the endosperm cavity. Indeed, when the total flux was partitioned between the nucellar projection cells at the three stages of transfer cell development, the fully differentiated stage III cells located proximally to the endosperm cavity alone exhibited spare transport capacity. Stage II cells could accommodate the total rate of sucrose transfer, but stage I cells could not. It is concluded that the nucellar projection tissue of wheat provides a unique opportunity to study transfer cell development and the functional role of these cells in supporting sucrose transport.Abbreviations CSPMSA cross sectional plasma membrane surface area - LPMSA longitudinal plasma membrane surface area - PTS tri-sodium 3-hydroxy-5,8,10-pyrenetrisulfonate     

Studies on Mature Seeds of Cuscuta pedicellata and C. campestris by Electron Microscopy

The seeds of Cuscuta pedicellata have been investigated by transmissionand scanning electron microscopy. Additional observations havebeen made on seeds of C. campestris by SEM only. The seed coatconsists of an outer single epidermis, two different palisadelayers, and an inner multiparenchyma layer. The outer epidermalwall in C. pedicellata has a thick cuticle and zones rich inpectic substances. The thicker ‘U-shaped’ cell wallsin the outer palisade layer are strengthened by a wall layerof hemicellulose. The inner palisade layer has thick walledcells with a ‘light line’. The inner cell wall ofthe compressed multiparenchyma layer has a thin cuticle. A fairlythick cuticle is positioned directly on the endosperm surface.The aleurone cell walls are different from the remaining endospermwalls. The latter are thick and believed to be of galactomannans.There is a ‘clear’ zone between the plasmalemmaand the cell wall in the aleurone cells. The embryo cells arepacked with lipids and proteins. In Cuscuta campestris mostendosperm has been absorbed during the seed development. Theembryo apex has two minute leaf primordia. The features of theCuscuta seeds are discussed in relation to functional and environmentalconditions. Cuscuta pedicellata, Cuscuta campestris, seed, seed coat, cuticle, cell walls, endosperm, aleurone cells, galactomannan, embryo, TEM, SEM     

Ultrastructure and Development of Oil Idioblasts in Annona muricata L.

The ultrastructure and development of oil idioblasts in theshoot apex and leaves in Annona muricata L. are described, andthree arbitrary developmental stages are distinguished: cellsin which no additional cell wall layers have been depositedagainst the initial primary cell wall, possessing an electron-translucentcytoplasm and distinct plastids which lack thylakoids (stage1); cells in which a suberized layer has been deposited againstthe primary wall (stage 2, the cytoplasm resembles that of thepreceding stage), and cells in which an additional inner walllayer has been deposited against the suberized layer, whichincreases in thickness with development (stage 3). In this stagean oil cavity is formed, surrounded by the plasmalemma, andattached to a bell-like protrusion of the inner wall layer,the cupule. A complex membranous structure occurs next to thecupule. Smooth tubular endoplasmic reticulum (ER), appearingas linearly arranged tubules, and groups of crystalline bodieswith an almost hexagonal outline are present. The final stagewas further subdivided into three subgroups (a, b, c) basedon the extent of the oil cavity, its contents, and the compositionof the cytoplasm, and increasing thickness of the inner walllayer. The oil is probably synthesized in the plastids, releasedinto the cytoplasm, and then passed through the plasmalemmasurrounding the oil cavity. Oil idioblasts, Annona muricata L., suberized layer, inner wall layer, oil cavity, cupule, smooth tubular ER, crystalline bodies     

Microspore ofSecale cereale as a transfer cell type

Summary In the mature microspore ofSecale cereale, a set of wall ingrowths deposited as the first (outer) intine layer between exine and the microspore plasma membrane, are revealed by electron microscopy. The wall ingrowths form a girdle in the vicinity of the apertural region at the external pole of microspore which is in contact with the tapetum, so the microspore can be considered as a transfer cell which is polarized. After microspore division the second (inner) intine layer is deposited by the vegetative cell and forms a labyrinth of branched wall ingrowths. As a result, the periphery of a vegetative cell is also irregular and appears as very thin plasmatubules or evaginations delimited by plasma membrane and penetrating the pollen wall.The possible functions of the microspore as a transfer cell and the wall-membrane system of the vegetative cell are discussed.     

Pollen Wall Development of Xiphidium coeruleum (Haemodoraceae) and its Systematic Implications

The development of the pollen grain wall in Xiphidium coeruleum(Haemodoraceae) was studied using TEM and cytochemical stainingtechniques. Microsporocyte ontogeny initiates with the degradationof the cellulosic cell wall and subsequent deposition of a thickcallosic cell wall. Following callose deposition, successivemeiosis occurs, resulting in a tetragonal tetrad of microspores.during meiosis, the cell walls of the tapetum break down, releasingthe syncytial periplasmodium. Irregular non-sporopollenous globularbodies are deposited in this peripheral periplasmodium, whichis rich in ER, golgi bodies, vesicles, and characteristic starchplastids. Within the microspore cytoplasm, vesicles, golgi bodies,and plastids are plentiful during the early tetrad stage. Atthis time the plasma membrane of the microspore develops characteristicevaginations. An extracellular membrane, the ‘white line’,is secreted outside the microspore plasma membrane, followedby callose wall degradation. Bead-like deposits of exine orprimexine are deposited at points along the ‘white line’simultaneously on inner and outer surfaces and opposite theoriginal plasma membrane evaginations. The bead-like exine depositscontinue to grow during the release of the microspores and developinto laterally appressed, rod-shaped ektexinous elements havinga tangentially oriented commissure, the vestige of the original‘white line’. The mature intine is two-layered,the outer exintine containing radially oriented vesicular structures,which are apparently derived from plasma membrane extensions.Exine development in Xiphidium is similar to ‘nexine 1’development in Lilium and may have evolved from an ancestraltectate-columellate condition by the loss of the sexine. Walldevelopment in members of the Zingiberales is strikingly similarto that reported here for the Haemodoraceae—evidence ofa possible relationship between the two taxa. Xiphidium coeruleum, Haemodoraceae, pollen, tapetum, development, exine     

The Rest Period of Rhododendron Flower Buds: III. CYTOLOGICAL STUDIES ON THE ACCUMULATION AND BREAKDOWN OF PROTEIN BODIES AND AMYLOPLASTS DURING FLOWER DEVELOPMENT

Rhododendron flower development occurs in three easily definedstages: a pre-rest stage, during which petal growth is mainlyby cell elongation; an indeterminate rest period; and an after-reststage, that begins when the flowers resume growth and ends atanthesis. Early in the pre-rest stage of development, protein bodies andamyloplasts accumulate in the petals. The epidermal cells accumulateonly protein bodies and the mesophyll cells accumulate amyloplaststhat have a few small protein bodies around the periphery. Thesubepidermal cells and the cells around the vascular bundlesaccumulate both large protein bodies and amyloplasts. Duringthe rest period there is a cessation of cell elongation andthe reserve protein bodies and amyloplasts remain intact. The protein bodies in all of the cells including those aroundthe amyloplasts are proteolized early in the after-rest stageof development. Digestion of the starch granules occurs whenthe petals are about one-half their final size. Epidermal-cell expansion during after-rest is relatively uniform;the walls between adjacent epidermal cells remain attached toeach other. The mesophyll cells elongate irregularly and thewalls of adjacent cells separate giving rise to large intercellularspaces. At anthesis the petal cells consist of a cell wall, a parietalcytoplasm, and a large central vacuole.