The frequency of plasmodesmata increases early in the whole shoot apical meristem of Sinapis alba L. during floral transition

 The frequency of plasmodesmata increases in the shoot apical meristem of plants of Sinapis alba L. induced to flower by exposure to a single long day. This increase is observed within all cell layers (L1, L2, L3) as well as at the interfaces between these layers, and it occurs in both the central and peripheral zones of the shoot apical meristem. The extra plasmodesmata are formed only transiently, from 28 to 48 h after the start of the long day, and acropetally since they are detectable in L3 4 h before they are seen in L1 and L2. These observations indicate that (i) in the Sinapis shoot apical meristem at floral transition, there is an unfolding of a single field with increased plasmodesmatal connectivity, and (ii) this event is an early effect of the arrival at this meristem of the floral stimulus of leaf origin. Since (i) the wave of increased frequency of plasmodesmata is 12 h later than the wave of increased mitotic frequency (A. Jacqmard et al. 1998, Plant cell proliferation and its regulation in growth and development, pp. 67–78; Wiley), and (ii) the increase in frequency of plasmodesmata is observed in all cell walls, including in walls not deriving from recent divisions (periclinal walls separating the cell layers), it is concluded that the extra plasmodesmata seen at floral transition do not arise in the forming cell plate during mitosis and are thus of secondary origin. Received: 4 October 1999 / Accepted: 23 December 1999     

Integument cell differentiation in dandelions (<Emphasis Type="Italic">Taraxacum</Emphasis>, Asteraceae,Lactuceae) with special attention paid to plasmodesmata

The aim of the paper is to determine what happens with plasmodesmata when mucilage is secreted into the periplasmic space in plant cells. Ultrastructural analysis of the periendothelial zone mucilage cells was performed on examples of the ovule tissues of several sexual and apomictic Taraxacum species. The cytoplasm of the periendothelial zone cells was dense, filled by numerous organelles and profiles of rough endoplasmic reticulum and active Golgi dictyosomes with vesicles that contained fibrillar material. At the beginning of the differentiation process of the periendothelial zone, the cells were connected by primary plasmodesmata. However, during the differentiation and the thickening of the cell walls (mucilage deposition), the plasmodesmata become elongated and associated with cytoplasmic bridges. The cytoplasmic bridges may connect the protoplast to the plasmodesmata through the mucilage layers in order to maintain cell-to-cell communication during the differentiation of the periendothelial zone cells.     

Dynamic changes in the frequency and architecture of plasmodesmata during the sink-source transition in tobacco leaves

Summary The sink-source transition in tobacco leaves was studied noninvasively using transgenic plants expressing the green-fluorescent protein (GFP) under control of theArabidopsis thaliana SUC2 promoter, and also by imaging transgenic plants that constitutively expressed a tobacco mosaic virus movement protein (MP) fused to GFP (MP-GFP). The sink-source transition was measured on intact leaves and progressed basipetally at rates of up to 600 m/h. The transition was most rapid on the largest sink leaves. However, leaf size was a poor indicator of the current position of the sink-source transition. A quantitative study of plasmodesmatal frequencies revealed the loss of enormous numbers of simple plasmodemata during the sink-source transition. In contrast, branched plasmodesmata increased in frequency during the sink-source transition, particularly between periclinal cell walls of the spongy mesophyll. The progression of plasmodesmal branching, as mapped by the labelling of plasmodesmata with MP-GFP fusion, occurred asynchronously in different cell layers, commencing in trichomes and appearing lastly in periclinal cell walls of the palisade layer. It appears that dividing cells retain simple plasmodesmata for longer periods than nondividing cells. The rapid conversion of simple to branched plasmodesmata is discussed in relation to the capacity for macromolecular trafficking in developing leaf tissues.     

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     

The shoot apical meristem of Sinapis alba L. expands its central symplasmic field during the floral transition

The shoot apical meristem (SAM) is functionally subdivided into zones with distinct tasks. During vegetative growth the peripheral zone of the meristem gives rise to leaf primordia that develop into dorsiventral leaves under the influence of signals from the central zone. During the floral transition the function of the SAM is altered and its peripheral zone starts to form floral structures in a specific pattern. This requires alterations in the signal networks that coordinate the activities of the peripheral and central zone of the SAM. These signal networks are partly housed in the symplasmic space of the SAM. Dye-coupling experiments demonstrate that in the superficial layer of the Sinapis alba meristem this space is radially subdivided. The cells of the central zone are coupled into a symplasmic field, which is shielded from the peripheral zone by the positional closing of plasmodesmata. In the vegetative meristems, most of these central symplasmic fields have a triangular geometry and are relatively small in size. Plants that are induced to flower by exposure to a single long day alter the geometry as well as the size of their central symplasmic field. After two subsequent days under short photoperiod the central symplasmic fields exhibit a circular form. Simultaneously, their size strongly increases both in an absolute sense and relative to the enlarging meristem. The geometric change in the fields is hypothesized to be due to recruitment of extra initial cells, required to support the increase in phyllotactic complexity. The proportional increase in field size is interpreted as an adjustment in the balance between the central and peripheral zone of the SAM, accompanying the shift from leaf production to flower formation.     

Development of the endosperm in rice (Oryza sativa L.): Cellularization

The syncytial endosperm of rice undergoes cellularization according to a regular morphogenetic plan. At 3 days after pollination (dap) mitosis in the peripheral synctium ceases. Radial systems of microtubules emanating from interphase nuclei define nuclear-cytoplasmic domains (NCDs) which develop axes perpendicular, to the embryo sac wall. Free-growing anticlinal walls between adjacent NCDs compart-mentalize the cytoplasm into open-ended alveoli which are overtopped by syncytial cytoplasm adjacent to the central vacuole. At 4 dap, mitosis resumes as a wave originating adjacent to the vascular bundle. The spindles are oriented parallel to the alveolar walls and cell plates formed in association with interzonal phragmoplasts result in periclinal walls that cut off a peripheral layer of cells and an inner layer of alveoli displaced toward the center. Polarized growth of the newly formed alveoli and elongation of the anticlinal walls occurs during interphase. The next wave of cell division in the alveoli proceeds as the first and a second cylinder of cells is cut off inside the peripheral layer. The periods of polarized growth/anticlinal wall elongation alternating with periclinal cell division are repeated 3–4 times until the grain is filled by 5 dap.     

Cytokinin application to the shoot apical meristem of Sinapis alba enhances secondary plasmodesmata formation

A single application of cytokinin benzyladenine causes a threefold increase in the frequency of plasmodesmata in the vegetative shoot apical meristem (SAM) of Sinapis alba plants. This increase is observed 20 h after application within all cell layers (L1, L2, L3) as well as at the interfaces between these layers. Evidence is presented indicating that cytokinin promotes mainly the formation of new secondary plasmodesmata. A similar increase in the frequency of secondary plasmodesmata was observed in the Sinapis SAM during the floral transition induced by a single long day, suggesting that this effect of the long day is mediated by cytokinin.     

ULTRASTRUCTURE OF THE EPIDERMIS OF DEVELOPING COTTON (GOSSYPIUM) SEEDS: SUBERIN,PITS, PLASMODESMATA,AND THEIR IMPLICATION FOR ASSIMILATE TRANSPORT INTO COTTON FIBERS

The basal part of cotton fibers (Gossypium arboreum and G. hirsutum) was studied with light and electron microscopy in order to improve the understanding of assimilate transport into the fibers during the deposition of the cellulosic secondary wall. Although the distal parts of white cotton fibers are not suberized, a variable amount of suberin was found at the fiber base. This suberin is typically deposited in concentric layers, alternating with polysaccharides. Numerous pits occur in the base of cotton fibers and in ordinary epidermal cells in the periclinal and anticlinal walls. About 25% of the length of periclinal walls is occupied by pits, but only 2% of the anticlinal walls, being pitted mainly in their proximal part. In suberized walls the deposition of suberin is not reduced in the pit region. The pits, whether or not suberized, contain plasmodesmata (22 ± 2.3 and 27 ± 3.3 · μm^−-2 in the periclinal and anticlinal walls of the white lint cultivar of G. hirsutum). Transport of assimilates into the fibers through the symplast is therefore possible. This transport may occur directly from mesophyll cells to fibers, or indirectly via ordinary epidermal cells. The minimum amount of assimilates transported into individual fibers during the phase of secondary wall deposition could be estimated (1.3 pg · fiber^−-1 · sec^−-1), as well as the corresponding symplastic flux of assimilates through the periclinal cell wall, neglecting a possible transport through the anticlinal walls (10^−-3 pg · μm^−-2 · sec^−-1). It is postulated that in the green lint genotype of G. hirsutum and in wild cotton species (not studied in this paper), the uptake of assimilates into the fibers occurs through the symplast, the apoplastic pathway being excluded by the suberization of the fibers during secondary wall formation. Although cultivated, white-linted cotton species may use the same pathway, loading of assimilates from the apoplast is theoretically also possible, and the relative contribution of both pathways has to be determined experimentally.     

THE FINE STRUCTURE OF THE TRIGGER HAIR IN VENUS'S FLYTRAP

Trigger hairs of Dionaea muscipula fixed in glutaraldehyde and OsO₄ were prepared for study in the electron microscope. Electron micrographs of the active zone of the trigger hair reveal three regions in which the cells differ in size, shape, and cytoplasmic content. Each region contains large numbers of protein bodies and mitochondria with densely packed tubular cristae. Vacuole-like structures containing protein bodies or an anastomosing system of cisternae, or occasionally both, are also present. Found only in the indentation cells is a complex, whorled endoplasmic reticulum. A concentric lamellar arrangement of the endoplasmic reticulum around the vacuolar structures is often observed. The lateral walls of the indentation cells are disproportionately thick while end walls are thin. The basal walls of these cells contain many plasmodesmata. Plasmodesmata in the anticlinal and podium cells pass through constricted zones in the cell wall and are particularly numerous in the peripheral podium cells. The possible functional significance of these structures is discussed.     

Microtubules and morphogenesis in stomata of the water fernAzolla: An unusual mode of guard cell and pore development

Summary A mature stomate of the water fernAzolla consists of a single apparently unspecialized annular guard cell (GC) with two nuclei surrounding an elongated pore aligned longitudinally in the leaf. During development, the guard mother cell develops a preprophase band (PPB) of microtubules (MTs) oriented transverse to the leaf axis. This is followed by a cell plate which fuses with the parental walls at the PPB site. Subsequently only the central part of the cell plate is consolidated, while the parts to either side become perforated and tenuous and may disperse completely, forming a single composite GC.Meanwhile, a dense array of MTs appears along both faces of the central part of the new wall, oriented normal to the leaf surface. Further MT arrays radiate out across the periclinal walls from the region of the consolidated cell plate. Putative MT nucleating sites are seen along the cell edges between these anticlinal and periclinal arrays. Polarized light microscopy reveals cellulose deposition parallel to the periclinal MT arrays. At the same time lamellar material is deposited within the new anticlinal wall. As the GC complex elongates, a split appears in these lamellae creating an initially transverse slit which then opens up to become first circular and ultimately an elongated pore aligned in the long axis of the leaf,i.e., at right angles to the wall in which it originated. The radiating pattern of cellulose microfibrils in the periclinal walls contributes to the shaping of the pore. Elongation at the apical and basal ends of the GC is restricted by longitudinal microfibril orientation, while that at the sides is facilitated by transverse alignment.     

Differential growth resulting in the specification of different types of cellular architecture in root meristems

Symplastic growth of plant organs may be described by a continuous growth tensor field. In tensorial analysis of meristems, the trajectories of periclinal and anticlinal cell walls represent trajectories of the principal directions of growth (PDGs); this follows from the maintenance of mutual orthogonality between periclinal and anticlinal wall trajectories during growth. Periclinal and anticlinal cell divisions are also oriented in the principal planes of growth. The growth tensor for the root apex is specified in such a way that the principal directions of the tensor fit the pattern of periclinal and anticlinal walls in the apex, and that the grid formed by material particles aligned along PDG trajectories preserve this alignment during growth. Two growth tensors are formulated--one giving a maximum and the other giving a minimum of the volumetric relative elemental growth rate at the region of the initial cell(s). Temporal sequences of deformation of a grid formed by lines coinciding with the principal directions of growth are shown. The formation of cellular patterns in root apices is simulated. Two types of patterns are obtained: one with an apical cell and merophytes, and another with files of cells converging towards a quiescent centre.     

Rearrangements of F-actin during Stomatogenesis Visualised by Confocal Microscopy in Fixed and Permeabilised Tradescantia Leaf Epidermis

Abstract: New details of F-actin organisation in leaf epidermal and stomatal cells were revealed by rhodamine — and fluorescein — phalloidin staining of fixed epidermal peels of Tradescantia virginiana and visualisation by confocal microscopy. Non-specialised epidermal cells contain highly organised arrays of fine cortical actin filaments aligned in transverse or oblique orientations. In interphase guard mother cells (GMCs), the arrangement of cortical F-actin changes on the periclinal and anticlinal cell walls at different times during differentiation. Initially, cortical F-actin on the periclinal surfaces is oriented transversely and F-actin is evenly distributed around the anticlinal walls. Following polarisation of the adjacent subsidiary mother cells (SMCs), actin in GMCs concentrates on the lateral anticlinal walls, but not on the transverse walls. Subsequently, F-actin on the periclinal walls reorients to radial and then longitudinal. Organisation of F-actin in SMCs appears to be influenced by the adjacent GMCs and co-ordination in F-actin arrangements in cells of the stomatal complex continues through to the formation of the guard cell pair. Our studies indicate that actin bands marking the division site in prophase cells, and detected in microinjected living material, are a particularly labile subset of F-actin. Actin bands were difficult to preserve, even when aldehyde fixation was avoided, in contrast to all interphase and mitotic F-actin.     

Sucrose-Caused Changes in the Frequency and Localization of Anticlinal Divisions in the Cambial Zone of Silver Birch

This study continues our previous experiments intended to elucidate the role of sucrose in a figured wood formation in silver birch (Betula pendula Roth var. carelica). The purpose of the study was the investigation of the role of sucrose in the regulation of cell division in the cambial zone. Using an earlier-developed technique, sucrose solutions of different concentrations have been delivered into trunk tissues of silver birch. A microscopic analysis of samples collected 28 days after the beginning of the experiment has shown that an increased sucrose concentration in an exogenous solution causes an increase in the frequency of anticlinal cell divisions in the cambial zone. In the case of high sucrose concentrations (10 or 20%), the zone of anticlinal divisions is significantly wider than in variants with low sucrose concentrations, since anticlinal divisions are observed on both phloem and xylem sides and at a larger distance from rays. A comparison of the obtained results with the previous experiments shows that the increased frequency of anticlinal divisions in cambial cells observed in the case of application of 10 or 20% sucrose solutions coincides with an increased parenchymatization of tissues. A revealed localization of anticlinal divisions within the cambial zone indicates that, in the case of the exogenous sucrose uptake, the morphogenesis of conductive tissues in silver birch (Betula pendula Roth var. pendula) occurs in the same way as in Karelian birch (Betula pendula Roth var. carelica). Data presented in this paper agree with the earlier hypothesis that the formation of figured wood similar to that of Karelian birch occurs due to increased sucrose content in trunk tissues.     

Microtubule and actin filament organization during stomatal morphogenesis in the fernAsplenium nidus

Summary The newly-formed guard cell mother cells (GMCs) ofAsplenium nidus are small, lens-shaped and are formed by one or two asymmetrical divisions. Their growth axis is parallel to the plane of their future division, a process during which the internal periclinal wall (IPW) is detached from the partner wall of the underlying cell(s). This oriented GMC expansion occurs transversely to a microfibril bundle, which is deposited externally to a U-like microtubule (Mt) bundle and a co-localized actin filament (Af) bundle. They line the IPW and the major part of the anticlinal walls. The deposition of the microfibril bundle is followed by the slight constriction of the internal part of the GMCs and the broadening of the substomatal cavity. The IPW forms a distinct bulging distal to the neighbouring leaf margin, as well as a less defined proximal one. During the IPW bulging, the Mts and Afs under the external periclinal wall (EPW) attain a radial organization. This is followed by thinning of the central EPW region, which becomes impregnated with a callose-like glucan. The rest of the EPW becomes unequally thickened. The disintegration of the U-like Mt bundle is succeeded by the organization of radial Mt and Af arrays under the IPW. The radial Mt systems, controlling the alignment of the newly-deposited microfibrils, allow the GMC to assume a round paradermal profile. The GMCs form a preprophase Mt band (PPB) perpendicular to the interphase U-like Mt bundle. The anticlinal PPB portions appear first and those lining the periclinal walls later. The cytoplasm adjacent to the latter walls retain the radial Mt systems during early preprophase, simultaneously with the anticlinal PPB portions. The observations suggest that the GMCs of the fernA. nidus obtain a unique form, as a result of a particular polarity established in the cortical cytoplasm of the periclinal walls, in which Mts and Afs appear involved. This polarity persists in cell division and is inherited to guard cells (GCs). It provides primary morphogenetic information not only to GMCs but also to GCs.Abbreviations Af actin filament - EPW external periclinal wall - GC guard cell - GMC guard cell mother cell - IPW internal periclinal wall - Mt microtubule - MTOC microtubule organizing centre - PPB preprophase microtubule band     

Seed testa micromorphology of thirty‐eight species of Allium (Amaryllidaceae) from central Asia,and its taxonomic implications

Micromorphological characteristics of the seed testa of 38 species belonging to 19 sections and seven subgenera of Allium from central Asia have been evaluated with a scanning electron microscope (SEM). Several taxonomically significant characters were found. The results showed that the epidermis consists of polygonal cells with different dimensions, that the cellular arrangement is tight or loose with or without reticulate tissue, and that the arrangement of cells is regular or irregular. The main variation was found in the anticlinal walls, of which the outline could be straight, straight to arched, arched or undulating like an S or U. Convex and (or) concave verrucate periclinal walls occurred in all species investigated. Based on the characteristics of the anticlinal and periclinal walls of the 38 species, six groups of Allium were distinguished, and a dichotomous key for them is presented. The cellular arrangement and periclinal and anticlinal wall traits of the 38 species of Allium were found stable and distinct within a species, but showed great differences among species. We conclude that seed epidermal characteristics provide useful and important information for distinguishing species of Allium, and thus they have taxonomic significance.     

Differential Growth in Periclinal and Anticlinal Walls during Lobe Formation in Arabidopsis Cotyledon Pavement Cells

Lobe development in the epidermal pavement cells of Arabidopsis thaliana cotyledons and leaves is thought to take place via tip-like growth on the concave side of lobes driven by localized concentrations of actin filaments and associated proteins, with a predicted role for cortical microtubules in establishing the direction of restricted growth at the convex side. We used homologous landmarks fixed to the outer walls of pavement cells and thin-plate spline analysis to demonstrate that lobes form by differential growth of both the anticlinal and periclinal walls. Most lobes formed within the first 24 h of the cotyledons unfurling, during the period of rapid cell expansion. Cortical microtubules adjacent to the periclinal wall were persistently enriched at the convex side of lobes during development where growth was anisotropic and were less concentrated or absent at the concave side where growth was promoted. Alternating microtubule-enriched and microtubule-free zones at the periclinal wall in neighboring cells predicted sites of new lobes. There was no particular arrangement of cortical actin filaments that could predict where lobes would form. However, drug studies demonstrate that both filamentous actin and microtubules are required for lobe formation.     

Ectopic expression of Arabidopsis CYCD2 and CYCD3 in tobacco has distinct effects on the structural organization of the shoot apical meristem

Transgenic tobacco lines expressing Arath-CYCD2 or Arath-CYCD3 genes under a cauliflower mosaic virus 35S promoter are modified in the timing of their development, but not in the phenotype of their vegetative organs. They display an increased rate of leaf initiation, which is shown to be associated with distinct changes in the structural organization of their shoot apical meristem (SAM). Constitutive expression of Arath-CYCD2 leads to a progressive modification of the SAM structural organization with predominant periclinal divisions in the L3 layer and to the loss of the classical cytophysiological zonation, the central zone being reduced to the central cells of the L1 and L2 layers. These changes reveal a particular sensitivity of the corpus cells (L3) to Arath-CYCD2 over-expression and suggest a role for CYCD2 in controlling the planes of cell division in these cells. The SAM structural modifications in the Arath-CYCD3 over-expressing lines are less drastic; only an increased cell number together with a reduced cell size, particularly in the L1 layer, characterizes the peripheral zones. This could be related to the shortening of the G1-phase duration that renders cell growth incomplete between successive mitoses. Cell proliferation continues beyond the SAM in the developing internodes and confers a delayed senescence to Arath-CYCD3 over-expressing juvenile tissues. In addition, the ploidy levels of mature stem tissues in both types of transgenic lines are unaffected, suggesting that the studied G1 to S cell-cycle genes have no effect on the extent of endoreduplication in tobacco stem tissues.     

Floral transition as a sequence of growth changes in different components of the shoot apical meristem ofChenopodium rubrum

The changes in cell division rate were studied in different components of the shoot apex ofChenopodium rubrum during short-day photoperiodic induction and after the inductive treatments. Induced and vegetative apices were compared. Accumulation of metaphases by colchicine treatment was used to compare the mean cell cycle duration in different components of the apex. A direct method of evaluating the increase in cell number obtained by anticlinal or periclinal divisions was applied if the corresponding components of induced and non-induced apices had to be compared. The short-day treatment prolonged the cell cycle more in the peripheral zone than in the central zone and still more in the leaf primordia. The importance of changing growth relations for floral transition was shown particularly if the induced plants were compared with the vegetative control with interrupted dark periods. Induced plants transferred to continuous light showed further changes in the rates of cell division. The cell cycle was shortened more in the central zone than in the peripheral zone,i.e. there was a further shift in growth relations within the apical dome. The cell cycle in the leaf and bud primordia was also shortened if compared with the vegetative control, the acceleration being stronger in the bud primordia. There was a subsequent retardation in cell division in the leaf primordia formed during and after the inductive treatment if the plants were fully induced. An inhibition of the oldest bud primordia was observed in fully induced apices, as well.     

The generation and consolidation of a radial array of cortical microtubules in developing guard cells of Allium cepa L.

The initiation and development of a radial array of microtubules (MTs) in guard cells of A. cepa was studied using immunofluorescence microscopy of tubulin in isolated epidermal layers. Soon after the completion of cytokinesis, MTs originate in the cortex adjacent to a central strip of the new, anticlinically oriented ventral wall separating the two guard cells. Cortical MTs extend from the mid-region of the central strip toward the cell edge where the ventral wall joins the inner periclinal wall. They then spread in a fan-like formation along the periclinal wall and gradually extend along the lateral and end walls as well. Many MTs criss-cross at various angles as they arc past the edge formed by the junction of the ventral and periclinal walls, but they do not terminate there, indicating that, contrary to previous report, the edge is not involved in MT initiation. Instead, the mid-region of the central strip appears to function as a planar MT-organizing zone. Initially, MTs radiate from this zone through the inner cytoplasm as well as the cortex. During cell expansion, however, the cortical MTs increasingly predominate and consolidate into relatively thick, long bundles, while the frequency of non-cortical MTs diminishes. The apparent density of MTs per unit surface area is maintained as the cells expand and gradually flex into an elliptical shape. The guard cells eventually separate completely at the pore site. The entire process is accomplished within about 12 h.Abbreviations DIC differential interference contrast - GC guard cell - MT microtubule To whom correspondence should be addressed.