The Involvement of Glucose-6-Phosphatase in Mucilage Secretion by Root Cap Cells of Zea mays

In order to determine the involvement of glucose-6-phosphatasein mucilage secretion by root cap cells, we have cytochemicallylocalized the enzyme in columella and peripheral cells of rootcaps of Zea mays. Glucose-6-phosphatase is associated with theplasmalemma and cell wall of columella cells. As columella cellsdifferentiate into peripheral cells and begin to produce andsecrete mucilage, glucose-6-phosphatase staining intensifiesand becomes associated with the mucilage and, to a lesser extent,the cell wall. Cells being sloughed from the cap are characterizedby glucose-6-phosphatase staining being associated with thevacuole and plasmalemma. These changes in enzyme localizationduring cellular differentiation in root caps suggest that glucose-6-phosphataseis involved in the production and/or secretion of mucilage byperipheral cells of Z. mays. Zea mays, corn, glucose-6-phosphatase, columella cell, peripheral cell, mucilage, secretion, cytochemistry     

Sloughing of cap cells and carbon exudation from maize seedling roots in compacted sand

Sloughing of root cap cells and exudation of mucilage plays an important role in the penetration of compacted soils by roots. For the first time we have quantified the rate of sloughing of root cap cells in an abrasive growth medium that was compacted to create mechanical impedance to root growth. The number of maize ( Zea mays ) root cap cells sloughed into sand increased as a result of compaction, from 1930 to 3220 d⁻¹ per primary root. This represented a 12-fold increase in the number of cells sloughed per mm root extension (from 60 to >700). We estimated that the whole of the cap surface area was covered with detached cells in compacted sand, compared with c . 7% of the surface area in loose sand. This lubricating layer of sloughed cells and mucilage probably decreases frictional resistance to soil penetration. The total carbon deposited by the root was estimated at c . 110 μg g⁻¹ sand d⁻¹. Sloughed cells accounted for <10% of the total carbon, the vast majority of carbon being contained in mucilage exudates.     

Morphogenesis of the root cap in adventitious roots of Salix viminalis

The preformed root primordia in stems of Salk viminalis L. consist of undifferentiated cells. Forty-eight hours after activation of the primordia in cuttings a root cap meristem was initiated four to five cell tiers from the surface of the primordia. The cells distal to the meristem divided only in an anticlinal plane, while in the meristem they divided mostly periclinally but sometimes anticlinally. After 72 hours a columella was established and the amyloplasts began to sediment in response to gravity. Shortly after this stage the roots began to bend slightly downward, probably as a geo-tropic response. Six days after activation the root cap consisted of up to 15 tiers of cells. The ultrastucture of the cap cells just prior to emergence was studied in more detail. The plastids in the cells adjoining the root proper were typical proplastids. Distal to this cell tier starch accumulated in the plastids. In the fifth tier the amyloplasts were fully sedimented to the lowermost cell walls. The amount of ER increased with the distance from the initial cells and most of it was located at the distal periclinal cell wall. The nucleus and the vacuoles in the geo-sensitive cells occurred in the space above the sedimented amyloplasts. The cytoplasm was less electron opaque than in the initial cells and the mitochondria had more cristae. In the distal cells of the columella and the lateral root cap secretion of mucilage seemed to have started. Numerous large dictyosomes were associated with large vesicles containing a fibrillar or granular material. The plasmalemma lining the distal periclinal cell wall had separated from the wall. A fibrillar material was present between the plasmalemma and the wall and also in intercellular spaces outside the root cap.     

Cellular Differentiation and Tissue Partitioning in Caps of Primary and Lateral Roots of Helianthus annuus

Cellular and tissue volumes in caps of primary and lateral rootsof Helianthus annuus have been measured in order to determinequantitatively how tissues and their functions are partitionedin root caps. Patterns of change in cellular dimensions andvolumes are similar in caps of primary and lateral roots. Significantincreases in cellular dimensions and volume occur during thedifferentiation of columella cells and the innermost peripheralcells. There are no significant changes in cellular dimensionsas either (i) the production and secretion of mucilage begins,or (ii) cells are sloughed from the cap. Tissues are partitionedsimilarly in caps of primary and lateral roots. indeed, rootcaps allocate 7–8 per cent of their volume for regeneration(i.e. calyptrogen tissue), 16–19 per cent of their volumefor graviperception (i.e. columella tissue), and approx. 38per cent of their volume for the production and secretion ofmucilage. These results are discussed relative to patterns ofcellular differentiation and tissue function in root caps. Helianthus annuus, root caps, primary root, lateral root, calyptrogen, columella, peripheral cells, tissue partitioning     

The rhizosphere in Zea: new insight into its structure and development

Some of the nodal roots of field-grown Zea mays L. bear a persistent soil sheath along their entire length underground except for a glistening white soil-free zone which extends approximately 25 mm behind the root cap. These roots are generally unbranched. The histology of the surface and the rhizosphere of the sheathed roots has been examined by correlated light and electron microscopy. All mature peripheral tissues including root hairs, are largely intact and apparently alive where enclosed by the soil sheath. The sheath is permeated by extracellular mucilage which is histochemically distinct from the mucilage at the epidermal surface, but similar to that produced by the root cap. Isolated cells resembling those sloughed from the sides of the root cap persist in the soil sheath along the length of these roots. Fresh whole mounts of the sheath show that these detached cells may be alive and streaming vigorously even at some distance from the root cap. Rhizosphere mucilage is associated with the isolated cells.To whom correspondence should be addressed     

CELLULAR VOLUME AND TISSUE PARTITIONING IN CAPS OF PRIMARY ROOTS OF ZEA MAYS

Cellular and tissue volumes were measured in caps of primary roots of Zea mays. There is an 850% increase in cellular volume as cellular function changes from that of being meristematic (i.e., calyptrogen cells) to graviperception (i.e., columella cells), and a 22% increase in cellular volume during the functional transition from graviperception to the production and secretion of mucilage. Cellular volume does not change significantly after cells cease mucilage production and are sloughed from the cap. Root caps of Z. mays allocate 7.5% of their volume for regeneration, 14.9% for graviperception, 24.3% for the transition of function from graviperception to mucilage production and secretion, and 38.7% for the production and secretion of mucilage. The remaining 14.5% of the cap volume is comprised of cells being sloughed from the cap.     

Characterizing Pathways by Which Gravitropic Effectors Could Move from the Root Cap to the Root of Primary Roots of Zea mays

Plasmodesmata linking the root cap and root in primary rootsZea mays are restricted to approx. 400 protodermal cells borderingapprox. 110000 µm² of the calyptrogen of the root cap.This area is less than 10% of the cross-sectional area of theroot-tip at the cap junction. Therefore, gravitropic effectorsmoving from the root cap to the root can move symplasticallyonly through a relatively small area in the centre of the root.Decapped roots are non-responsive to gravity. However, decappedroots whose caps are replaced immediately after decapping arestrongly graviresponsive. Thus, gravicurvature occurs only whenthe root cap contacts the root, and symplastic continuity betweenthe cap and root is not required for gravicurvature. Completelyremoving mucilage from the root tip renders the root non-responsiveto gravity. Taken together, these data suggest that gravitropiceffectors move apoplastically through mucilage from the capto the root. Calyptrogen, open meristem, protoderm, root cap, root gravitropism, Zea mays     

Root apical organization inArabidopsis thaliana 1. Root cap and protoderm

Summary We investigated the development of the root cap and protoderm inArabidopsis thaliana root tips.A. Thaliana roots have closed apical organization with the peripheral root cap, columella root cap and protoderm developing from the dermatogen/calyptrogen histogen. The columella root cap arises from columella initials. The initials for the peripheral root cap and protoderm are arranged in a collar and the initiation event for these cells occurs in a sequential pattern that is coordinated with the columella initials. The resulting root cap appears as a series of interconnected spiraling cones. The protoderm, in three-dimensions, is a cylinder composed of cell files made up of packets of cells. The number of cell files within the protoderm cylinder increases as the root ages from one to two weeks. The coordinated division sequence of the dermatogen/calyptrogen and the increase in the number of protoderm cell files are both features of post-embryonic development within the primary root meristem.Abbreviations RCP root cap/protoderm - CI columella initial - PI protoderm initial     

Cell division patterns of the protoderm and root cap in the “closed” root apical meristem ofArabidopsis thaliana

Summary The peripheral root cap and protoderm inArabidopsis thaliana are organized into modular packets of cells derived from formative T-divisions of the root cap/protoderm (RCP) initials and subsequent proliferative divisions of their daughter cells. Each module consists of protoderm and peripheral root cap packets derived from the same periclinal T-division event of an RCP initial. Anatomical analyses are used to interpret the history of extensively coordinated cell divisions producing this modular construction. Within a given layer of root cap, the columella and RCP initials divided in a centrifugal sequence from the innermost columella initials toward the RCP initials. All RCP initials in the lineages around the circumference of the root divided nearly simultaneously in waves to form one module prior to the next wave of initial divisions forming a younger module. The peripheral root cap and protoderm packets within each module completed four rounds of proliferative divisions in the axial plane to produce, on average, 16 cells per packet in the basalmost modules in axial view. Peripheral root cap and protoderm cells predominantly in the T-type (trichoblast) lineages also underwent radial divisions as they were displaced basipetally. The regularity in the cellular pattern within the modules suggests a timing mechanism controlling highly coordinated cell division in the initials and their daughter cells.Abbreviations RAM root apical meristem - RCP root cap protoderm - prc peripheral root cap     

Geoperception in primary and lateral roots of Phaseolus vulgaris (Fabaceae). I. Structure of columella cells

Primary roots of Phaseolus vulgaris (Fabaceae) are positively geotropic, while lateral roots are not responsive to gravity In order to elucidate the structural basis for this differential georesponse, we have performed a qualitative and quantitative analysis of the ultrastructure of columella cells of primary and lateral roots of P. vulgaris. Root systems were fixed in situ so as not to disturb the ultrastructure of the columella cells. The columellas of primary roots are more extensive than those of lateral roots. The volumes of columella cells of primary roots are approximately twice those of columella cells of lateral roots. However, columella cells of primary roots contain greater absolute volumes and numbers of all cellular components examined than do columella cells of lateral roots. Also, the relative volumes of cellular components in columella cells of primary and lateral roots are statistically indistinguishable. The endoplasmic reticulum is sparse and distributed randomly in both types of columella cells. Both types of columella cells contain numerous sedimented amyloplasts, none of which contact the cell wall or form complexes with other cellular organelles. Therefore, positive geotropism by roots must be due to a factor(s) other than the presence of sedimented amyloplasts alone. Furthermore, it is unlikely that amyloplasts and plasmodesmata form a multi-valve system that controls the movement of growth regulating substances through the root cap.     

Structure of Columella Cells in Primary and Lateral Roots of Ricinus communis (Euphorbiaceae)

Horizontally oriented primary roots of Ricinus communis aremore graviresponsive than similarly oriented lateral roots.The more pronounced graviresponsiveness of primary roots ispositively correlated with their caps having a more extensivecolumella tissue than caps of lateral roots. Individual columellacells of primary roots contain 2.6 times more protoplasm thando columella cells of lateral roots. Similarly, the absolutevolumes of all cellular components in columella cells of primaryroots are larger than those of lateral roots. However, thereare no statistically significant differences in the relativevolumes of any cellular component in columella cells of primaryvs lateral roots. Endoplasmic reticulum is distributed randomlyin columella cells of both types of roots. Columella cells ofprimary and lateral roots contain numerous sedimented amyloplastswhich do not consistently contact any cellular structure. Nucleitend to be located in the middle thirds of the columella cells,and the vacuole is found in largest concentrations in the middleand upper thirds of columella cells of both types of roots.The largest protoplasmic volumes of mitochondria occur in thelower thirds of columella cells, and dictyosomes are found insimilar concentrations throughout the cells. There is no significantdifference in the intracellular distributions of organellesin columella cells of primary vs lateral roots. We believe thatthe differing graviresponsiveness of primary vs lateral rootsof R. communis is probably due to factors other than the structuresof their individual columella cells. Ricinus communis, columella, graviperception, graviresponsiveness, roots, root cap     

The Locations and Amounts of Endogenous lons and Elements in the Cap and Elongating Zone of Horizontally Oriented Roots of Zea mays L: An Electron-probe EDS Study

We used quantitative electron-probe energy-dispersive x-raymicroanalysis to localize endogenous Na, Cl, K, P, S, Mg andCa in cryofixed and freeze-dried cryosections of the cap (i.e.the putative site of graviperception) and elongating zone (i.e.site of gravicurvature) of horizontally oriented roots of Zeamays. Ca, Na, Cl, K and Mg accumulate along the lower side ofcaps of horizontally oriented roots. The most dramatic asymmetriesof these ions occur in the apoplast, especially the mucilage.We could not detect any significant differences in the concentrationsof these ions in the central cytoplasm of columella cells alongthe upper and lower sides of caps of horizontally-oriented roots.However, the increased amounts of Na, Cl, K and Mg in the longitudinalwalls of columella cells along the lower side of the cap suggestthat these ions may move down through the columella tissue ofhorizontally-oriented roots. Ca also accumulates (largely inthe mucilage) along the lower side of the elongating zone ofhorizontally-oriented roots, while Na, P, Cl and K tend to accumulatealong the upper side of the elongating zone. Of these ions,only K increases in concentration in the cytoplasm and longitudinalwalls of cortical cells in the upper vs lower sides of the elongatingzone. These results indicate that (1) gravity-induced asymmetriesof ions differ significantly in the cap and elongating zoneof graviresponding roots, (2) Ca accumulates along the lowerside of the cap and elongating zone of graviresponding roots,(3) increased growth of the upper side of the elongating zoneof horizontally-oriented roots correlates positively with increasedamounts of K in the cytoplasm and longitudinal walls of corticalcells, and (4) the apoplast (especially the mucilage) may bean important component of the pathway via which ions move ingraviresponding rots of Zea mays. These results are discussedrelative to mechanisms for graviperception and gravicurvatureof roots. Corn, gravitropism (root), ions, x-ray microanalysis, Zea mays     

Deoxyribonucleic Acid synthesis in root cap cells of cultured roots of convolvulus

Isolated cultured roots of Convolvulus arvensis L. were incubated in 0.2 microcurie per milliliter methyl-³H-thymidine for 14 hours, for 64 hours, or for 14 hours followed by transfer to fresh nutrient medium without tritiated thymidine. Autoradiographs of serial, longitudinal sections of roots which were continuously incubated with tritiated thymidine showed that cells of the root cap columella did not undergo DNA synthesis after their formation from the root cap initials. In roots pulse-labeled with tritiated thymidine, the movement of labeled cells through the root cap columella was followed. Labeled cells were displaced at a constant rate of 72 microns per day over a period of 6 to 9 days before they were sloughed off from the root cap. The specialized role of the root cap cells in relation to their distinctive metabolism and longevity is discussed.     

The Root Cap: Cell Dynamics, Cell Differentiation and Cap Function

The root cap is a universal feature of angiosperm, gymnosperm, and pteridophyte roots. Besides providing protection against abrasive damage to the root tip, the root cap is also involved in the simultaneous perception of a number of signals – pressure, moisture, gravity, and perhaps others – that modulate growth in the main body of the root. These signals, which originate in the external environment, are transduced by the cap and are then transported from the cap to the root. Root gravitropism is one much studied response to an external signal. In the present paper, consideration is given to the structure of the root cap and, in particular, to how the meristematic initial cells of both the central cap columella and the lateral portion of the cap which surrounds the columella are organized in relation to the production of new cells. The subsequent differentiation and development of these cells is associated with their displacement through the cap and their eventual release, as “border cells”, from the cap periphery. Mutations, particularly in Arabidopsis, are increasingly playing a part in defining not only the pattern of genetic activity within different cells of the cap but also in revealing how the corresponding wild-type proteins relate to the range of functions of the cap. Notable in this respect have been analyses of the early events of root gravitropism. The ability to image auxin and auxin permeases within the cap and elsewhere in the root has also extended our understanding of this growth response. Images of auxin distribution may, in addition, help extend ideas concerning the positional controls of cell division and cell differentiation within the cap. However, firm information relating to these controls is scarce, though there are intriguing suggestions of some kind of physiological link between the border cells surrounding the cap and mitotic activity in the cap meristem. Open questions concern the structure and functional interrelationships between the root and the cap which surmounts it, and also the means by which the cap transduces the environmental signals that are of critical importance for the growth of the individual roots, and collectively for the shaping of the root system.     

How roots perceive and respond to gravity

Graviperception by plant roots is believed to occur via the sedimentation of amyloplasts in columella cells of the root cap. This physical stimulus results in an accumulation of calcium on the lower side of the cap, which in turn induces gravicurvature. In this paper we present a model for root gravitropism integrating gravity-induced changes in electrical potential, cytochemical localization of calcium in cells of gravistimulated roots, and the interdependence of calcium and auxin movement. Key features of the model are that 1) gravity-induced redistribution of calcium is an early event in the transduction mechanism, and 2) apoplastic movement of calcium through the root-cap mucilage may be an important component of the pathway for calcium movement.     

Fucose in the surface deposits of axenic and field grown roots ofZea mays L.

Summary The location of materials containing terminal fucose residues on the surface of axenic and field grown roots of corn has been determined.Binding patterns of FITC-labelled,Lotus purpureus Moench lectin indicate the presence of the fucose residues in the cell walls and mucilage of the peripheral region of the root cap. During development, fucose residues also appear in the outer periclinal walls and overlying mucilage of columnar epidermal cells. Surface material rich in these residues persists between the mature root hairs but is not found on their surface. Fucose-rich mucilage is present on the exposed surface of aerial roots and at the point where they enter the soil. No lectin binding residues are indicated elsewhere in the roots.     

Domain-specific and cell type-specific localization of two types of cell wall matrix polysaccharides in the clover root tip

Using immunocytochemical techniques and antibodies that specifically recognize xyloglucan (anti-XG), polygalacturonic acid/rhamnogalacturonan I (anti-PGA/RG-I), and methylesterified pectins (JIM 7), we have shown that these polysaccharides are differentially synthesized and localized during cell development and differentiation in the clover root tip. In cortical cells XG epitopes are present at a threefold greater density in the newly formed cross walls than in the older longitudinal walls, and PGA/RG-I epitopes are detected solely in the expanded middle lamella of cortical cell corners, even after pretreatment of sections with pectinmethylesterase to uncover masked epitopes. These results suggest that in cortical cells XG and PGA/RG-I are differentially localized not only to particular wall domains, but also to particular cell walls. In contrast to their nonoverlapping distribution in cortical cells, XG epitopes and PGA/RG-I epitopes largely colocalize in the epidermal cell walls. The results also demonstrate that the middle lamella of the longitudinal walls shared by epidermal cells and by epidermal and cortical cells constitutes a barrier to the diffusion of cell wall and mucilage molecules. Synthesis of XG and PGA/RG-I epitope-containing polysaccharides also varies during cellular differentiation in the root cap. The differentiation of gravitropic columella cells into mucilage-secreting peripheral cells is marked by a dramatic increase in the synthesis and secretion of molecules containing XG and PGA/RG-I epitopes. In contrast, JIM 7 epitopes are present at abundant levels in columella cell walls, but are not detectable in peripheral cell walls or in secreted mucilage. There were also changes in the cisternal labeling of the Golgi stacks during cellular differentiation in the root tip. Whereas PGA/RG-I epitopes are detected primarily in cis- and medial Golgi cisternae in cortical cells (Moore, P. J., K. M. M. Swords, M. A. Lynch, and L. A. Staehelin. 1991. J. Cell Biol. 112:589-602), they are localized predominantly in the trans-Golgi cisternae and the trans-Golgi network in epidermal and peripheral root cap cells. These observations suggest that during cellular differentiation the plant Golgi apparatus can be both structurally and functionally reorganized.     

SLOUGHED PERIPHERAL ROOT CAP CELLS: YIELD FROM DIFFERENT SPECIES AND CALLUS FORMATION FROM SINGLE CELLS

Peripheral root cap cells can be isolated by gentle agitation of the root in water for less than 60 sec. Filtration of the detached cells through a 30-μm mesh screen results in a suspension of single cells. Yields of peripheral root cap cells from 28 species in 10 families ranged from fewer than 10 per root from tobacco to more than 5,000 per root from pine. The viability of freshly isolated cells from most species, including legumes and cereals, was 85% to 95%. Cultured cells from pea and soybean exhibited cytoplasmic streaming for more than a month. When incubated at an initial density of 10⁵ cells per ml of liquid B5(P) medium, 6% to 8% of isolated pea root cap cells divided and grew into callus.     

Localization of Phenolic Compounds in the Root Cap Columella of Six-year-old Dry Seeds of Brassica napus during Imbibition and Germination

In 6-year-old seeds of Brassica napus the columella cells haveno necroses and resemble in structure the cells of the 2-year-oldembryo. The outermost layer of the columella shows a structuresimilar to that of the lateral region of the root cap, as itcontains protein bodies, rare in layers of the columella closerto the promeristem, which, in turn, contain numerous mitochondriaand plastids. Phenolic compounds in the dry embryo are on thesurface of the root cap in the space between the plasmalemmaand the cell wall, and in small vesicles which presumably remainedfrom degradation of ER. Imbibition promotes further extrusionof phenolics outside the plasma membrane. Long sheets of ERare visible after 9 h imbibition. After 24 h phenolics of moredense structure are localized in some dilated parts of the ER.This suggests that new production of defence compounds startswithin 24 h in water, a few hours earlier than in 2-year-oldseeds.Copyright 1994, 1999 Academic Press Brassica napus, phenolics, root columella, germination