The Ultrastructure of Protophloem Sieve Elements in Leaves of Aegilops comosa var. thessalica

The differentiation and obliteration of protophloem sieve elementsin leaves of the grass Aegilops comosa var. thessalica havebeen studied by electron microscopy. These elements differentiatesimilarly to metaphloem sieve elements of the same plant andother monocotyledons. Plasmalemma, smooth endoplasmic reticulum(ER), mitochondria, P-type plastids and sometimes nuclear remnantsconstitute the protoplasmic components at maturity, all areperipherally distributed. The differentiation of end walls intosieve plates and the presence of sieve areas on the lateralwalls indicate that protophloem sieve elements are componentsof sieve-tube. They may be functional for a brief period butsoon after their maturation they are compressed and finallyobliterated by the stretching of actively-growing surroundingcells. The protoplasmic components of mature elements degenerateand are destroyed during obliteration of the sieve elements. Aegilops comosa var. thessalica, protophloem, sieve elements, differentiation, ultrastructure     

Development of protophloem in roots ofAegilops comosa var.thessalica. I. Differential divisions and pre-prophase bands of microtubules

Summary The formative divisions of protophloem mother cells in roots of the grassAegilops comosa var.thessalica have been investigated by means of light and electron microscopy. Two successive differential divisions create protophloem poles consisting of a protophloem sieve element and two companion cells. Pre-prophase bands of microtubules appear in premitotic cells anticipating the plane of orientation of the cell plate and indicating the site where the daughter wall will join the parent one. Evidence is accumulated that the site previously occupied by pre-prophase band is bisected by the new wall. Structural asymmetries that could express polarity, like organelle displacement, were not observed in premitotic cells. A working hypothesis is proposed integrating the conclusions of the present study in a diagram correlating pre-prophase bands of microtubules and differential divisions.     

Sieve-Element Ontogeny in the Aerial Shoot of Equisetum hyemale L.

The aerial shoots of Equisetum hyemale L. var. affine (Engelm.)A. A. Eat. were examined with the electron microscope as partof a continuing study of sieveelement development in the lowervascular plants. Young E. hyemale sieve elements are distinguishablefrom all other cell types within the vascular system by thepresence of refractive spherules, proteinaceous bodies whichdevelop within dilated portions of the endoplasmic reticulum(ER). Details of cell wall thickening differ between protophloemand metaphloem sieve elements. Following cell wall thickeningthe ER increases in quantity and aggregates into stacks. Shortlythereafter, nuclear degeneration is initiated. During the periodof nuclear degeneration some cytoplasmic components-dictyosomes,microtubules and ribosomes-degenerate and disappear, while organellessuch as mitochondria and plastids persist. The latter undergostructural modifications and become parietal in distribution.Eventually the massive quantities of ER are reduced, leavingthe lumen of the cell clear in appearance. At maturity the plasmalemma-linedsieve element contains a parietal network of tubular ER, aswell as mitochondria, plastids, and refractive sphemh At thistime many of the spherules are discharged into the region ofthe wall. Sieveelement pores occur in both lateral and end walls.At maturity many pores are traversed by large numbers of ERmembranes. The metaphloem sieve elements of the mid-internodalregions apparently are sieve-tube members. The connections betweenmature protophloem sieve elements and pericycle cells are associatedwith massive wall thickenings on the pericyclecell side.     

ULTRASTRUCTURE OF DEVELOPING SIEVE ELEMENTS IN THLASPI ARVENSE L. I. THE IMMATURE STATE

Immature sieve elements of pennycress (Thlaspi arvense, Brassicaceae) were studied with the electron microscope in connection with studies on virus-infected plants. Immature sieve elements contained cytoplasm rich in organelles and other components: endoplasmic reticulum, dictyosomes and associated smooth and coated vesicles, mitochondria, plastids, ribosomes, microtubules, microfilaments, vacuoles, and nuclei that were sometimes lobed. Tubular P-protein (phloem protein) and one to three granular P-protein bodies also were present in the cytoplasm. Coated vesicles may be involved in formation of the granular P-protein body and in some aspect of cell wall development, for in the latter case, they were often seen united with the plasmalemma. The association of coated vesicles with the P-protein body is discussed with reference to proposed concepts of the origin and function of these vesicles.     

THE FINE STRUCTURE OF DIFFERENTIATING XYLEM ELEMENTS

Differentiating xylem elements of Avena coleoptiles have been examined by light and electron microscopy. Fixation in 2 per cent phosphate-buffered osmium tetroxide and in 6 per cent glutaraldehyde, followed by 2 per cent osmium tetroxide, revealed details of the cell wall and cytoplasmic fine structure. The localized secondary wall thickening identified the xylem elements and indicated their state of differentiation. These differentiating xylem elements have dense cytoplasmic contents in which the dictyosomes and elements of rough endoplasmic reticulum are especially numerous. Vesicles are associated with the dictyosomes and are found throughout the cytoplasm. In many cases, these vesicles have electron-opaque contents. "Microtubules" are abundant in the peripheral cytoplasm and are always associated with the secondary wall thickenings. These microtubules are oriented in a direction parallel to the microfibrillar direction of the thickenings. Other tubules are frequently found between the cell wall and the plasma membrane. Our results support the view that the morphological association of the "microtubules" with developing cell wall thickenings may have a functional significance, especially with respect to the orientation of the microfibrils. Dictyosomes and endoplasmic reticulum may have a function in some way connected with the synthetic mechanism of cell wall deposition.     

ULTRASTRUCTURE OF DEVELOPING SIEVE ELEMENTS IN THLASPI ARVENSE L. II. MATURATION

Developing sieve elements of pennycress (Thlaspi arvense L.) were studied with the electron microscope. The maturation of sieve elements involved loss of ribosomes from cytoplasm; degeneration of nulcei; modification of endoplasmic reticulum (ER); loss of tonoplast; and disappearance of dictyosomes and dictyosomes vesicles, coated vesicles, microtubules, and microbodies. Such changes produce a mature, presumably conducting cell that contains no nucleus or central vacuole but which retains a thin layer of peripheral cytoplasm with plastids, mitochondria, and smooth ER. Some similar changes have been described in a variety of developing sieve elements of angiosperms, but coated vesicles and microbodies previously have not been followed through sieve-element maturation. Likewise, few developmental studies have been made of plant sieve elements that exhibit two types of P-protein, the tubular type and the granular P-protein body.     

THE FINE STRUCTURE OF SIEVE ELEMENTS OF NEREOCYSTIS LÜTKEANA

The sieve elements of Nereocystis from the base of phylloids contain numerous small vesicles, cytoplasm, ribosomes, and the usual organelles and membrane systems, including nuclei, plastids, mitochondria, dictyosomes, and endoplasmic reticulum. They have a thick secondary wall layer which is deposited along the longitudinal walls and at the sieve plate excluding the sieve pores. The sieve pores range in diameter from 100 to 400 nm and are lined by plasmalemma. The sieve elements from the hollow basal parts of the pneumatocyst show essentially the same features but have larger and fewer vesicles, relatively little cytoplasm, larger sieve pores, 400–900 nm in diameter, and may lack a nucleus. In old sieve elements there are large deposits of callose on the sieve plate and along the longitudinal wall; the vesicles seem to break down, and the protoplast appears necrotic. It is concluded that the trumpet hyphae and sieve tubes are basically the same type of cell, and that the trumpet-shape of the sieve elements is due to their passive stretching during extension growth of the organ in which they occur. There are minor but significant differences among the sieve elements from different regions of the thallus which may reflect possible levels of structural specialization of the sieve elements within the same plant.     

Development of mestome sheath cells in leaves ofAegilops comosa var.thessalica

Summary The development of mestome sheath cells ofAegilops comosa var.thessalica was studied by electron microscopy. Anatomical and cytological observations show that this grass belongs to the C₃ or non-Kranz plants. In the asymmetrically thickened walls of mestome sheath cells a suberized lamella is present. This lamella is deposited asynchronously. In the midrib and the large lateral bundles it appears first in the outer and inner walls and usually later in the radial walls. In the small lateral bundles its appearance is delayed in the inner walls of those cells situated on the xylem side. At maturity the suberized lamella is observed in all cell walls; however, in the small lateral bundles it is partly or totally absent from the walls of some cells situated on the xylem side. Tertiary wall formation is asynchronous as well, for it generally follows the deposition pattern of the suberized lamella.During the development of the mestome sheath cells microtubules show marked changes in their number and orientation, being fewer and longitudinal during suberin deposition. Dictyosomes are very active and may be involved in primary and tertiary wall formation. Endoplasmic reticulum cisternae are abundant and partly smooth, while plasmalemmasomes may function to reduce the plasmalemma extension. However, cytoplasmic structures that are clearly involved in suberin synthesis could not be identified.Suberized lamellae react strongly with silver hexamine. This is probably due to post-fixation with osmium tetroxide.On the basis of structural characteristics the mestome sheath may be regarded as an endodermis (cf., alsoFahn 1974). The significance of this view for water and assimilate exchange between the mesophyll and the bundle is discussed.This report represents a portion of a doctoral dissertation.     

CYTOLOGY OF DIFFERENTIATING TRACHEARY ELEMENTS I. ORGANELLES AND MEMBRANE SYSTEMS

The distribution of organelles, membrane systems, and ribosomes is not at any time obviously related to the pattern of secondary wall in helically thickened tracheary elements in leaves of Beta vulgaris L. (sugar beet) and Cucurbita maxima Duchesne, fixed with potassium permanganate and osmium tetroxide. During the differentiation of the secondary wall, cisternae of the endoplasmic reticulum and dictyosomes are particularly conspicuous, and the dictyosomes are associated with numerous vesicles. Similar vesicles appear to be in various stages of fusion with the secondary wall thickenings. The tracheary elements contain plastids which may include starch granules. Ribosomes occur free in the cytoplasm and in association with endoplasmic membranes.     

Structure and Development of Sieve Elements in the Root of Isoetes muricata Dur.

Root tissues of Isoetes muricata Dur. were fixed in glutaraldehydeand postfixed in osmium tetroxide for electron microscopy. Veryyoung root sieve elements can be distinguished from contiguousparenchyma cells by the presence of crystalline and/or fibrillarproteinaceous material in dilated cisternae of rough endoplasmicreticulum (ER). Similar crystalline-fibrillar material accumulatesin the perinuclear space. During differentiation, the portionsof ER enclosing this proteinaceous substance become smooth surfacedand migrate to the cell wall. Along the way many of them formmultivesicular bodies which fuse with the plasmalemma, dischargingtheir contents toward the wall. Nuclear degeneration is pycnotic.At maturity, the sieve element contains a degenerate, filiformnucleus, plastids, and mitochondria. In addition, the wall ofthe mature sieve element is lined by a plasmalemma and a parietalnetwork of smooth ER. Sieve-area pores are present in both endand lateral walls of mature sieve elements. Whereas a singlecluster of pores occurs in each end wall, the pores of the lateralwalls are solitary and few in number.     

PHLOEM OF PRIMITIVE ANGIOSPERMS. I. SIEVE-ELEMENT ONTOGENY IN THE PETIOLE OF LIRIODENDRON TULIPIFERA L. (MAGNOLIACEAE)

As part of a continuing study of sieve elements in primitive angiosperms, a study of this cell type was undertaken in Liriodendron tulipifera. A typical ontogenetic sequence was observed in which synthetic processes such as wall thickening are followed in time by cellular lysis of nucleus, ribosomes, microtubules, vacuoles, and dictyosomes. This lysis is selective in that certain cellular components (e.g., the plasmalemma) remain unaffected. Concomitant with lysis is the formation of sieve-area pores from plasmodesmata. Comparison of pore size on end and lateral walls indicates that the use of the term “sieve tube” rather than “sieve cell” to describe these elements is appropriate.     

On the ultrastructure of differentiating secondary xylem in willow

Summary Studies of differentiating xylem inSalix fragilis L. show the immediate cambial derivatives to be ultrastructurally similar. The Golgi apparatus is important at all stages of wall synthesis, possibly producing (amongst other substances) hemicellulose material which is carried to the wall in vesicles or multivesicular bodies. The endoplasmic reticulum also contributes one or more components to the developing wall: at some stages during differentiation the endoplasmic reticulum produces electron opaque bodies which appear to be guided towards the wall by microtubules. Compact structures formed from concentric membranes (myelin-like bodies) have been found joined to rough endoplasmic reticulum, but their presence is not explained.Two types of plasmalemma elaboration occur: invagination of the plasmalemma itself to form vesicles which may contain cytoplasmic material; and vesicles between the plasmalemma and cell wall which are the result of single vesicles or multivesicular bodies traversing the plasmalemma. Both systems provide a means for transporting cytoplasmic material across the plasmalemma.Microtubules have been seen associated with all vesicles derived from the cytoplasm which appear to be moving towards the wall. The presence of microtubules may generally be explained in terms of orientation of vesicles, even if they also happen coincidentally to parallel the supposed orientation of microfibrils in the wall itself. It is possible to resolve connections between the microtubules and the plasmalemma.     

Differentiation and Ultrastructure of the Protophloem Sieve Elements of Minor Veins in the Maize Leaves: Changes in the Protoplast

Protophloem sieve element differentiation in the minor veins of the maize ( Zea mays L. ) leaves was first evidenced as an increase of the wall thickness, which began in the comers of the cell and then extended to other parts of the wall, and the appearance of long rough endoplasmic reticulum cistemae distributed throughout the cytoplasm, and then the presence of characteristic crystalloid inclusions within the plastids. As differentiation progressed, long cisternae of rough endoplasmic reticulum appeared to transform into shorter forms and eventually aggregated into small stacks, losing their ribosomes during the process. The nuclei degenerated, although frequently persisted until very late in differentiation the stages of maturation, as darkly stained amorphous aggregates surrounded by double nuclear envelope or only inner membrane of nuclear envelope. Subsequently, the nuclear envelope collapsed and became discontinuous. At the beginning of nuclear degeneration the perinuclear spaces were partly dilated and sometimes the outer nuclear envelope in the dilated portions then ruptured, and was accompanied by the disappearance of the cytoplasmic portion near it. During the peried of nuclear degeneration, in addition to the endoplasmic reticulum, plastids and mitochondria underwent structural modification, while components such as ribosomes, cytoplasmic ground substances, vacuoles and dictyosomes disintegrated and disappeared. At maturity, the surviving protoplasmic components, including plasmalemma, mitochondria, small stacked smooth endoplasmic reticulum and P-type plastids with crystalloids, became parietal in position. As differentiation of adjacent metaphloem sieve elements proceeded, the protoplasmic components of the mature protophloem sieve elements progresively degenerated and finally obliterated.     

Protoplasmic Changes in Cambial Cells Induced by a Tracheid-Differentiation Factor from Pine Needles

Direct differentiation of ‘dormant’ fusiform cambialcells (fees) into tracheids in stem cuttings of Pinus contortaDougl. was investigated by light and transmission electron microscopy.In cuttings from which all but one pair of needles had beenremoved, differentiation occurred close to the needle tracewithout prior cell division or expansion. The highly osmiophillic,granular cytoplasm of differentiating fees exhibited numerousmitochondria, dictyosomes and endoplasmic reticulum (ER) cisternaeand was enriched with vesicles and polyribosomes. The protoplasmdid not become highly vacuolated, as it normally does, untildifferentiating tracheids were approaching maturation. During differentiation, secondary walls were deposited in feesas ribs of annular and spiralled thickenings and also as borderedpit-likestructures devoid of margo and torus and lacking the typicallamellar structure of secondary-xylem tracheids. The fee plasmamembrane at sites of secondary-wall growth was in dynamic flux,dilated vesicles derived from both ER and dictyosomes apparentlyfusing with it at these locations. In addition, electron-denseblebs were invariably plasma membrane-associated and appearedto be exocytotic; these blebs became rare during autolysis andthey were never seen in non-differentiating cells. Depositionof oriented nascent cellulose microfibrils appeared to occurin the absence of associated cortical microtubules. As secondary-walldeposition neared completion, vacuoles derived from rough ERgrew and fused; concomitantly, the protoplasm disappeared resultingin fully autolysed tracheids. Auxin (indol-3-ylacetic acid, IAA) promoted the gel-like protoplasmof dormant fees to became highly vacuolated, and cell divisionand expansion followed; however, tracheid differentiation didnot occur. Polyribosomes, rough ER, and dictysomes were lessabundant than in differentiating fees and the cytoplasm of auxin-treatedfees was fine grained and less densely stained. The electron-denseexocytotic blebs found at the plasmalemma in differentiatingfees were not induced by IAA treatment. Fees of control cuttingsenlarged somewhat and became more vacuolated but otherwise remaineddormant. Key words: Cambium, exocytosis, Gymnospermae, ultrastructure, xylogenesis     

STRUCTURE AND DEVELOPMENT OF THE SIEVE ELEMENT IN THE STEM OF LYCOPODIUM LUCIDULUM

Stem tissue of Lycopodium lucidulum Michx. was fixed in glutaraldehyde and postfixed in osmium tetroxide for electron microscopy. Although their protoplasts contain similar components, immature sieve elements can be distinguished from parenchymatous elements of the phloem at an early stage by their thick walls and correspondingly high population of dictyosomes and dictyosome vesicles. Late in maturation the sieve-element walls undergo a reduction in thickness, apparently due to an “erosion” or hydrolysis of wall material. At maturity, the plasmalemma-lined sieve elements contain plastids with a system of much convoluted inner membranes, mitochondria, and remnants of nuclei. Although the endoplasmic reticulum (ER) in most mature sieve elements was vesiculate, in the better preserved ones the ER formed a tubular network closely appressed to the plasmalemma. The sieve elements lack refractive spherules and P-protein. The protoplasts of contiguous sieve elements are connected with one another by pores of variable diameter, aggregated in sieve areas. As there is no consistent difference between pore size in end and lateral walls these elements are considered as sieve cells.     

Abnormal structure of protophloem sieve-element cell wall in colchicine-treated roots of Triticum aestivum L.

The structural aberrations of the cell walls of protophloem sieve elements (PSEs) in roots of wheat (Triticum aestivum L. cv. Maris Huntsman) caused by the anti-microtubule drug colchicine were investigated by electron microscopy. The initial effect of the drug on cell wall development was found to be an exceptionally rough wall surface, presumably caused by an uncontrolled fusion of Golgi vesicles with the plasma membrane. Cellulose microfibrils, which in normal PSEs are aligned transversely to the long axis and parallel to the cortical microtubules, in colchicine-treated PSEs display a predominant longitudinal orientation. The pattern of wall development is disturbed by deposition of wall material also within the sieve pores of the sieve-pore/plasmodesmata complexes, resulting in evenly thickened walls instead of the normal uneven layers, and in narrowing the sieve pores to the size of plasmodesmata. In prolonged and continuous colchicine treatment, PSEs develop unusual wall ingrowths projecting deeply into the cytoplasm, creating an extraordinary cell type not found in normal roots. The results confirm the view of microtubule involvement in the proper deposition and orientation of cellulose microfibrils, and in the normal patterning of the cell wall thickenings of differentiating PSEs.Abbreviations c colchicine-treated - PSE protophloem sieve element The author is grateful to Dr. B. Galatis, Dr. P. Apostolakos and Dr. C. Katsaros, Institute of General Botany, University of Athens, Greece, for helpful discussions and suggestions, and for the generous gift of the colchicine used here. This work was carried out in the Department of Botany, University of Thessaloniki, Greece, while observations were also made in the Lehrstuhl für Zellenlehre, University of Heidelberg, Germany, and in the Department of Botany, University of Georgia, USA. The author is thankful to Prof. E. Schnepf (Zellenlehre, Heidelberg, Germany) and Prof. B.A. Palevitz (Department of Botany, University of Athens, Ga., USA), for generously providing access to their equipment and facilities. The work was financially supported in part by the Stiftung Volkswagenwerk and by the Research Committee, University of Thessaloniki (No 7537).     

Comparative Structure of Companion Cells and Phloem Parenchyma Cells in Mimosa pudica L.

The phloem of Mimosa pudica L. furnishes an example of definablediversification of the parenchymatic members of the tissue intocompanion cells and parenchyma cells. The companion cells havedense protoplasts which contain the typical organelles of plantcells, including chloroplasts and many ribosomes. The sieveelements and companion cells are interconnected by numerousbranched plasmodesmata. The companion cells degenerate whenthe associated sieve elements cease to function. The parenchymacells have less dense protoplasts than the companion cells.In many parenchyma cells the rough endoplasmic reticulum assumesa tubular form, and bundles of microfilaments are present. Thecytoplasmic ribosomes occur in groups apparently held togetherby fibrils. Chloroplasts, mitochondria (some are exceptionallylong), dictyosomes, microbodies, and microtubules are the othercell components. Whether the parenchyma cells are ontogeneticallyrelated to the sieve elements or not, they do not degeneratewhen the sieve element ceases to function.     

Histochemical and Ultrastructural Observations on the Nacreous Walls of the Sieve Elements of Atrichum undulatum

The nacreous walls of the sieve elements of Atrichum undulatumare composed of a loose fibrillar matrix. Histochemically, thesewalls have cellulose, pectins, proteins, phospholipids, andRNA as components. Ultrastructurally, the walls contain fragmentsof the plasmalemma and what appear to be aggregations of endoplasmicreticulum and vesicles. The unusual presence of these cytoplasmiccomponents appears to explain the positive histochernical testsfor proteins and RNA.     

Endoplasmic Reticulum-dictyosome Involvement in the Origin of Refractive Spherules in Sieve Elements of Davallia fijiensis Hook

Young sieve elements from petioles and rachises of Davalliafijiensis Hook were examined with an electron microscope. Evidencewas obtained that implicated both the endoplasmic reticulum(ER) and the Golgi apparatus in the formation of refractivespherules. Numerous connections were observed between smooth,tubular ER and peripheral tubules of the dictyosomes, indicatingthat these two cytoplasmic components are parts of a singleendomembrane system. Davallia fijiensis Hook, endomembrane system, endoplasmic reticulum, dictyosome, refractive spherule, sieve element     

Structure and cytochemistry of the procambium in Salix buds during dormancy and dormancy breaking

This report presents a combined investigation of ultrastructural and enzymatic changes in the procambium from late winter to early spring. In January the procambial cells of dormant Salix buds have a convoluted plasma membrane with many plasmalemmasomes, numerous lipid bodies, large stacks of rough ER and plastids surrounded by smooth ER profiles. Several small lysosomes show activity of ATPase and acid phosphatases. In addition ER, nuclear envelopes, dictyosomes, and thylakoids have ATPase activity, and ER and plasmalemma, and nuclei also show acid phosphatase activity. In February metabolism seems to increase as indicated by lysosomes with membranous formations, dilated ER, nuclear envelopes, spiny vesicles, and polysomes. ATPase activity occurs in plasmalemma and vacuoles, and acid phosphatases in the middle lamella region of walls, in plasmalemma, vacuoles, ER, and nuclei. At the end of March, when growth starts inside the buds, but before they break, the stacks of rough ER disappear, and the vacuoles coalesce. Most of the lipid bodies have disappeared and the plastids have accumulated starch. Cell division and differentiation of procambial cells to protophloem and protoxylem have started. The distribution of ATPase increases; activity is found in walls and plasmalemma, and only a few small vacuoles still have ATPase and acid phosphatase activity. Notable is the appearance of ATPase in mitochondrial cristae and nucleoli and the occurrence of rather high levels also in endomembranes and dictyosomes.