Microtubule reorganization,cell wall synthesis and establishment of the axis of elongation in regenerating protoplasts of the algaMougeotia

Summary Microtubule reorganization and cell wall deposition have been monitored during the first 30 hours of regeneration of protoplasts of the filamentous green algaMougeotia, using immunofluorescence microscopy to detect microtubules, and the cell-wall stain Tinopal LPW to detect the orientation of cell wall microfibrils. In the cylindrical cells of the alga, cortical microtubules lie in an ordered array, transverse to the long axis of the cells. In newly formed protoplasts, cortical microtubules exhibit some localized order, but within 1 hour microtubules become disordered. However, within 3 to 4 hours, microtubules are reorganized into a highly ordered, symmetrical array centered on two cortical foci. Cell wall synthesis is first detected during early microtubule reorganization. Oriented cell wall microfibrils, co-aligned with the microtubule array, appear subsequent to microtubule reorganization but before cell elongation begins. Most cells elongate in the period between 20 to 30 hours. Elongation is preceded by the aggregation of microtubules into a band intersecting both foci, and transverse to the incipient axis of elongation. The foci subsequently disappear, the microtubule band widens, and microfibrils are deposited in a band which is co-aligned with the band of microtubules. It is proposed that this band of microfibrils restricts lateral expansion of the cells and promotes elongation. Throughout the entire regeneration process inMougeotia, changes in microtubule organization precede and are paralleled by changes in cell wall organization. Protoplast regeneration inMougeotia is therefore a highly ordered process in which the orientation of the rapidly reorganized array of cortical microtubules establishes the future axis of elongation.     

The role of microtubules and cell-wall deposition in elongation of regenerating protoplasts of Mougeotia

Protoplasts of the filamentous green alga Mougeotia sp. are spherical when isolated and revert to their normal cylindrical cell shape during regeneration of a cell wall. Sections of protoplasts show that cortical microtubules are present at all times but examination of osmotically ruptured protoplasts by negative staining shows that the microtubules are initially free and become progressively cross-bridged to the plasma membrane during the first 3 h of protoplast culture. Cell-wall microfibrils areoobserved within 60 min when protoplasts are returned to growth medium; deposition of microfibrils that is predominantly transverse to the future axis of elongation is detectable after about 6 h of culture. When regenerating protoplasts are treated with either colchicine or isopropyl-N-phenyl carbamate, drugs which interfere with microtubule polymerization, they remain spherical and develop cell walls in which the microfibrils are randomly oriented.     

Orientation of microfibrils and microtubules in cortical parenchyma cells of poplar during elongation growth

Three types of microfibrillar orientation, namely parallel, perpendicular and oblique to the main cell axis were found not only in the innermost surface of but also throughout the developing wall. Furthermore, three types of microtubule orientation, namely parallel, perpendicular and oblique to the main cell axis, were found, coinciding with those of microfibrils. As a whole, the wall was shown to be a crossed polylamellate structure. These observations suggest that the orientation of microfibrils is determined at the time of wall formation, and not influenced by the extension of the wall.     

Electron diffraction from the primary wall of cotton fibers

Summary Electron diffraction patterns have been obtained from selected areas of disencrusted microfibrils isolated from the primary cell wall of cotton fibers. The resultant fiber diagram has the same meridional repeat distance as a corresponding pattern of secondary wall microfibrils but differs markedly in the equatorial reflections. The primary wall diagram displays only two strong equatorial reflections centered at 0.570 nm and 0.416 nm. The similarity of these spacings with those of cellulose IV suggests that the crystalline structure of the primary wall cellulose is similar to that of cellulose IV_I and is best explained in term of native cellulose I crystals having good longitudinal coherence (i.e., coherence along the length of the microfibrils) but with poor lateral organization of the network of inter chain hydrogen bonds. Similar results were also obtained for other primary wall specimens.     

The Cellulose System in the Cell Wall ofMicrasterias

The cellulose system of the cell wall ofMicrasterias denticulataandMicrasterias rotatawas analyzed by diffraction contrast transmission electron microscopy, electron diffraction, and X-ray analysis. The studies, achieved on disencrusted cell ghosts, confirmed that the cellulose microfibrils occurred in crisscrossed bands consisting of a number of parallel ribbon-like microfibrils. The individual microfibrils had thicknesses of 5 nm for a width of around 20 nm, but in some instances, two or three microfibrils merged into one another to yield larger monocrystalline domains reaching up to 60 nm in lateral size. The orientation of the cellulose ofMicrasteriasis very unusual, as it was found that in the cell wall, the equatorial crystallographic planes of cellulose having ad-spacing of 0.60 nm [(110) in the Iβ cellulose unit cell defined by Sugiyamaet al.,1991,Macromolecules24, 4168–4175] were oriented perpendicular to the cell wall surface. Up to now, such orientation has been found only inSpirogyra,another member of the Zygnemataceae group. The unusual structure of the secondary wall cellulose ofMicrasteriasmay be tentatively correlated with the unique organization of the terminal complexes, which in this alga occur as hexagonal arrays of rosettes.     

SEQUENCE AND PATTERN OF LATERAL ROOT FORMATION IN FIVE SELECTED SPECIES

The proximal-distal distribution of the lateral roots of five species was studied. A detailed investigation was carried out on two of the five species, Ceratopteris thalictroides and Cucurbita maxima. A definite pattern of lateral root arrangement, with a degree of variability related to the number of protoxylem poles, was found in all of the species studied. In the fern Ceratopteris, lateral root initiation was found to be related to the segmentation of the apical cell, which in turn determines the distribution of the laterals. In this species the lateral roots occur in a predictable sequence and they are grouped in pairs. In the angiosperms studied, the pattern of lateral root distribution seemed to depend primarily upon a rather strict longitudinal relationship between the lateral root primordia formed opposite any one protoxylem pole. In Cucurbita maxima, 93.7 ± 5.02% of the lateral root primordia observed were in a specific sequence. The laterals of this species are also arranged in groups. In the other plants studied, Arachis hypogaea, Victoria trickeri, and Eichhornia crassipes, the laterals were not as regularly arranged, but nevertheless they were found to be arranged in groups along the main root axis and not randomly dispersed. Factors controlling the spacing of lateral root primordia include their relationship with the developing vascular system, a direct effect of the parent root apex, and an effect of older lateral root primordia in the same sector of the root.     

Microtubule organization,mesophyll cell morphogenesis,and intercellular space formation inAdiantum capillus veneris leaflets

Summary Mesophyll cells (MCs) ofAdiantum capillus veneris are elongated and highly asymmetric, bearing several lateral branches and forming a meshwork resembling aerenchyma. Young MCs are polyhedral and display oppositely arranged walls and transverse cortical microtubules (Mts). Their morphogenesis is accomplished in three stages. At first they become cylindrical. Intercellular space (IS) canals, containing PAS-positive material, open through their junctions and expand laterally. During the second stage the cortical Mts form a reticulum of bundles, externally of which an identical reticulum of wall thickenings, containing bundles of parallel cellulose microfibrils, emerges. MCs do not grow in girth in the regions of wall thickenings, where constrictions form and new ISs open. Thus, MCs obtain a multi-lobed form. At the third morphogenetic stage MCs display a multi-axial growth. During this process, additional Mt rings are assembled at the base of cell lobes accompanied by similarly organized wall thickenings-cellulose microfibrils. Consequently, cell lobes elongate to form lateral branches, where MCs attach one another, while the IS labyrinth broadens considerably. Colchicine treatment, destroying Mts, inhibits MC morphogenesis and the concomitant IS expansion, but does not affect IS canal formation. These observations show that: (a) MC morphogenesis inA. capillus veneris is an impressive phenomenon accurately controlled by highly organized cortical Mt systems. (b) The disposition of Mt bundles between neighbouring MCs is highly coordinated, (c) The perinuclear cytoplasm does not appear to be involved in cortical Mt formation. Cortical sites seem to participate in Mt bundling, (d) Although extensive IS canals open before Mt bundling, the Mtdependent MC morphogenesis contributes in IS formation.Abbreviations EM electron microscopy - ER endoplasmic reticulum - IS intercellular space - MC mesophyll cell - MSB microtubule stabilizing buffer - Mt microtubule - PBS phosphate buffered saline     

STABILITY AND COLCHICINE EFFECT OF WALL MICROFIBRILLAR ALIGNMENT IN THE NITELLA RHIZOID

The cell wall of the Nitella rhizoid was stripped to make wedges of various thicknesses. Polarizing and interference microscopes were used to examine the post-deposition orientation of wall microfibrils. The fibrils appeared to maintain alignment after they were deposited. Since during growth the rhizoid wall elements are static in the cylindrical part or extend isotropically in the dome (Chen, 1973), these observations provide indirect evidence that the fibrillar reorientation observed in the Nitella internode is due to a passive reorientation during the predominant longitudinal cell elongation (Gertel and Green, 1977). The static microfibrils of the secondary wall of rhizoid, however, reoriented under the influence of colchicine, the alignment becoming almost random after 48 hrs. The disturbance of alignment started in the region adjacent to the plasma membrane, increasing in thickness with prolonged treatment.     

On the polarity of cellulose in the cell wall of Valonia

The orientation of the triclinic phase of cellulose in the cell wall of Valonia ventricosa J. Agardh was investigated by X-ray- and electron-diffraction analysis. In addition to the well-documented uniplanar-axial organization of the cell wall which requires that the a ^* axis should be always perpendicular to the wall surface, the direction of this axis was also found to be pointing outward from the plasma membrane side of the wall. This unidirectionality was persistent throughout the various layers that constitute the cell wall and also for the three microfibrillar orientations that occur in Valonia cell walls. The unidirectionality of the a ^* axis indicates, in particular, that the Valonia cellulose microfibrils are not twisted along their axis. These observations are consistent with a cellulose biosynthetic scheme where a close association exists between terminal-complex orientations and those of the cellulose microfibrils. In this context, the unidirectionality of the a ^* axis of cellulose seems to be related to the restricted mobility of the terminal complexes which are able to slide in the plasma membrane but not to rotate along their long axis.Abbreviations TC terminal complex This work was initiated during a visit of J.F.R at Grenoble in the framework of a France-Québec exchange program. J.S. was recipient of a CNRS fellowship. The diagram in Fig. 8 was kindly drawn for us by Miss Yukie Saito from the Department of Forest Products, the University of Tokyo.     

LIGNIFICATION DURING SECONDARY WALL FORMATION IN COLEUS: AN ELECTRON MICROSCOPIC STUDY

The fine structure of lignin deposition was examined in developing secondary walls of wound vessel members in Coleus. KMnO₄, which was used as the fixative, selectively reacts with the lignin component of the cell wall and thus can be used as a highly sensitive electron stain to follow the course of lignification during secondary wall deposition. Lignin was first detected as conspicuuos electron-opaque granules in the primary wall in the region where the secondary wall thickening arises and as fine granular striations extending into the very young secondary wall. As the secondary wall develops lignification becomes progressively more extensive. In cross sections the lignified secondary wall appears as concentric, fine granular striations; in tangent al or oblique sections it is seen as delicate, beaded fibrils paralleling the long axis of the thickening. High magnification of tangential or oblique sections shows that the fibrillar appearance is due to the presence of alternating light and dark layers each approximately 25-35 A wide. It is assumed that the light layers are the cellulose microfibrils and the dark regions contain lignin which fills the space between the microfibrils. KMnO₄, by selectively reacting with lignin, thus negatively stains the cellulose microfibrils revealing their orientation and dimensions.     

Effects of 3-Indolylacetic Acid and 3-Indolylacetonitrile on the Growth of Excised Tomato Roots

1. The inhibition by IAA (3-indolylacetic acid) and by IAN (3-indolylacetonitrile)of the growth of excised tomato roots cultured for 7 days at27 C. in a modified White's medium is described. 510^–9g./ml, IAA or 510^–6 g./ml, IAN cause approx, 50 per cent,inhibition of the linear growth of the main axis. With IAA decreasein number of laterals closely parallels the decrease in lineargrowth of the main axis; with IAN reduction in linear growthof the main axis occurs at concentrations above 10^–8 whereasnumber of laterals does not decrease until the concentrationexceeds 10^–6.
2. Study of the course of cell elongationin the exodermal cellsshowed that in the standard medium andin media containing 510^–9IAA or 510^–6 IAN theprocess takes about 7 hours; thefinal cell lengths in IAA andIAN media are lower than in standardmedium owing to a slowerrate of elongation. The decrease inlinear growth of the mainaxis in presence of IAA could be accountedfor by the decreasein cell length; this was not the case withIAN. The implicationsof this are considered.
3. Determinations of the distance (mm.)between, and of the numberof exodermal cells separating, theadjacent laterals in oneorthostichy showed that IAN enhancesthe frequency of lateralswhereas this is either unaffectedor decreased by IAA. The enhancementof lateral frequency inIAN arises from shortening of the cellsof the main axis anddecrease in the number of cells separatingadjacent laterals.
4. The results are considered to support the view that IAN haseffects on root growth different from those of IAA. Study ofthe degree of inhibition of main axis growth and of alterationsin lateral frequency resulting from treatment with mixturesof IAA and IAN provided data which could also be most easilyexplained on this hypothesis.

     

The change of pattern in microfibril arrangement on the inner surface of the cell wall of Closterium acerosum during cell growth

Closterium acerosum (Schrank) Ehrenberg cells cultured on cycles of 16 h light and 8 h dark, undergo cell division synchronously in the dark period. After cell division, the symmetry of the daughter semicells is restored by controlled expansion, the time required for this restoration, 3.5–4 h, being relatively constant. The restoration of the symmetry is achieved by highly oriented surface expansion occurring along the entire length of the new semicell. During early semicell expansion, for about 2.5 h, microfibrils are deposited parallel to one another and transversely to the cell axis on the inner surface of the new wall. Wall microtubules running parallel to the transversely oriented microfibrils are observed during this period. About 2.5 h after septum formation, preceding the cessation of cell elongation, bundles of 7–11 microfibrils running in various directions begin to overlay the parallel-arranged microfibrils already deposited. In the fully elongated cells, no wall microtubules are observed.     

Spatial relationship between microtubules and plasma-membrane rosettes during the deposition of primary wall microfibrils in Closterium sp.

The mechanism by which cortical microtubules (MTs) control the orientation of cellulose microfibril deposition in elongating plant cells was investigated in cells of the green alga, Closterium sp., preserved by ultrarapid freezing. Cellulose microfibrils deposited during formation of the primary cell wall are oriented circumferentially, parallel to cortical MTs underlying the plasma membrane. Some of the microfibrils curve away from the prevailing circumferential orientation but then return to it. Freeze-fracture electron microscopy shows short rows of particle rosettes on the P-face of the plasma membrane, also oriented perpendicular to the long axis of the cell. Previous studies of algae and higher plants have provided evidence that such rosettes are involved in the deposition of cellulose microfibrils. The position of the rosettes relative to the underlying MTs was visualized by deep etching, which caused much of the plasma membrane to collapse. Membrane supported by the MTs and small areas around the rosettes resisted collapse. The rosettes were found between, or adjacent to, MTs, not directly on top of them. Rows of rosettes were often at a slight angle to the MTs. Some evidence of a periodic structure connecting the MTs to the plasma membrane was apparent in freeze-etch micrographs. We propose that rosettes are not actively or directly guided by MTs, but instead move within membrane channels delimited by cortical MTs attached to the plasma membrane, propelled by forces derived from the polymerization and crystallization of cellulose microfibrils. More widely spaced MTs presumably allow greater lateral freedom of movement of the rosette complexes and result in a more meandering pattern of deposition of the cellulose fibrils in the cell wall.Abbreviations E-face exoplasmic fracture face - MT microtubule - P-face protoplasmic fracture-face     

LONGITUDINAL MICROFIBRILLAR ALIGNMENT IN THE WALL OF CYLINDRICAL NITELLA RHIZOIDAL CELLS: OBSERVATION UNDER POLARIZING AND INTERFERENCE MICROSCOPES

Polarizing and interference microscopes were employed to measure overall orientation of microfibrils and dry matter (expressed in optical thickness) in the cell wall of Nitella rhizoids. The microfibrils are aligned predominantly parallel to the cell's long axis (positively birefrengent), except in the apical dome where the arrangement appears to be random. The optical thickness, however, is greater at the very tip and the base region. The wall contains about 50-60% of acid extractable amorphous, noncrystalline substance. This extraction does not make a significant change in the alignment, but the remaining dry matter becomes less at the tip and increases slightly toward the base. The alignment parallel to the direction of cell growth in the rhizoidal cell is different from that of the elongating Nitella internodal cell where the alignment is transverse.     

Wiedereinführung vonBryopsis lyngbyei (Bryopsidales,Chlorophyta) als selbständige Art

Zusammenfassung 1. Die bisher in der Algenflora Helgolands alsBryopsis plumosa (Huds.) C. Ag. geführte Art wurde alsBryopsis lyngbyei Hornemann erkannt.2. Der Umriß der dicht zweizeilig gefiederten Art ist einer Vogelfeder ähnlich.Bryopsis lyngbyei ist diözisch; ihr Lebenszyklus schließt ein fadenförmiges Sporophytenstadium ein, das nur stephanokonte Zoosporen erzeugt.3. Die negativen Kreuzungsversuche mit Herkünften vonBryopsis plumosa europäischer Küstenabschnitte erweisen die Selbständigkeit vonBryopsis lyngbyei.

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Reestablishment ofBryopsis lyngbyei (Bryopsidales, Chlorophyta) as separate species

This study investigates the taxonomic status of a Helgoland species hitherto regarded asBryopsis plumosa (Huds.)Ag. The habitus of the plant concerned agrees well with that of the original specimens ofBryopsis lyngbyei Hornemann in the Botanical Museum of Copenhagen. Pinnules arise distichously from the axis; the life cycle of the dioecious species includes a filamentous sporophytic stage which produces only stephanokontic zoids. Crosses with samples ofBryopsis plumosa from European coasts were unsuccessful; thusBryopsis lyngbyei is evidently a separate species.

     

Effects of colchicine on cell shape and on microfibril arrangement in the cell wall of Closterium acerosum

Cell morphogenesis in Closterium acerosum (Schrank) Ehrenberg was greatly influenced by colchicine. Addition of colchicine to the medium led to production of tadpole-shaped cells, by decreasing the length and increasing the thickness of the new semicells. Transversely oriented wall microtubules and microfibrils, characteristic of normally elongating semicells, were not observed in colchicine-treated semicells, randomly oriented microfibrils being present instead. About 3.5 h after septum formation, the randomly oriented microfibrils began to be overlaid by bundles of microfibrils as seen in normal semicells at the later stage of elongation. When colchicine treatment was terminated 1 h after septum formation, cell elongation was partially restored and microfibrils were deposited parallel to each other and transversely to the cell axis, indicating that the effect of colchicine on microfibril arrangement in growing semicells is reversible.     

Colchicine-induced expansion ofVaucheria cell apex. Alteration from isotropic to transversally anisotropic growth

The tip-growth ofVaucheria geminata was analyzed. The elemental rate of surface expansion (RERE) at the very apex of this alga cell reaches ca. 100% min⁻¹. The expansion is almost isotropic; i.e. the both meridional and latitudinal components of RERE are almost equal. An antimicrotubular reagent, colchicine, caused expansion at the actively growing cell apex of this alga. This drug did not change the surface expansion rate, but altered the polarity of cell wall expansion from isotropic to transversally anisotropic. The orientation of cell wall microfibrils is random at the apex but axial at the basal cylindrical part of the cell. Colchicine did not change the fluence-response relationship for the first positive phototropism.     

Cellulose microfibril orientation and cell shaping in developing guard cells of Allium: The role of microtubules and ion accumulation

Summary The role of microtubules and ions in cell shaping was investigated in differentiating guard cells of Allium using light and electron microscopy and cytochemistry. Microtubules appear soon after cytokinesis in a discrete zone close to the plasmalemma adjacent to the common wall between guard cells. The microtubules fan out from this zone, which corresponds to the future pore site, towards the other sides of the cell. Soon new cellulose microfibrils are deposited on the wall adjacent to the microtubules and oriented parallel to them. As the wall thickens, the shape of the cell shifts from cylindrical to kidney-like. Studies with polarized light show that guard cells gradually assume a birefringence pattern during development characteristic of wall microfibrils radiating away from the pore site. Retardation increases from 10 Å when cells just begin to take shape, to 80–100 Å at maturity. Both microfibril and microtubule orientation remain constant during development. Observations on aberrant cells including those produced under the influence of drugs such as colchicine, which leads to loss of microtubules, abnormal wall thickenings and disruption of wall birefringence, further support the role of microtubules in cell shaping through their function in the localization of wall deposition and the orientation of cellulose microfibrils in the new wall layer. Potassium first appears in guard mother cells before division and rapidly accumulates afterwards during cell shaping, as judged by the cobaltinitrite reaction. Some chloride and perhaps organic acid anions also accumulate. Thus, these ions, which are known to play a role in the function of mature guard cells, also seem to be important in the early growth and shaping of these cells.Abbreviations IPC isopropyl-N-phenylcarbamate - CB cytochalasin B - GMC guard mother cell - MTOC microtubule organizing center     

Lattice images from ultrathin sections of cellulose microfibrils in the cell wall of Valonia macrophysa Kütz.

The crystalline ultrastructure and orientation of cellulose microfibrils in the cell wall of Valonia macrophysa were investigated by means of high-resolution electron microscopy of ultrathin (approx. 28 nm) sections. With careful selection of imaging conditions, ultrastructural aspects of the cell wall that had remained unresolved in previous studies were worked out by direct imaging of crystal lattice of cellulose microfibrils. It was confirmed that each microfibril is a single crystal having a lateral dimension of 20·20 nm², because lattice images of 0.39 nm resolution were clearly recorded with no major disruption in the whole area of the cross section of the microfibril. There was no evidence for the existence of 3.5-nm elementary fibrils which have been considered to be basic crystallographic and morphological units of cellulose in general. It was also confirmed that the axial directions (crystallographic fiber direction) of adjacent microfibrils in each single lamella of the cell wall are opposite to each other.