The distribution of plasmodesmata in the phloem ofHevea brasiliensis in relation to laticifer loading

Summary Cell to cell connections, including plasmodesmata and perforations, were examined in the non-conducting secondary phloem ofHevea brasiliensis. Samples were taken from trunks of numerous trees, from several clones, and prepared for thin sectioning and transmission or scanning electron microscopy and as optical sections for fluorescence microscopy. Numerous plasmodesmata were found clustered in primary pit-fields between the ray and axial parenchyma cells. Between the laticifers and adjacent parenchyma sheath cells, structures corresponding to functional plasmodesmata were not observed. But some unusual structural features were occasionally seen in these walls. These observations are discussed in relation to the possible function of the cell types, and to the loss of latex on the tapping ofHevea. It is suggested that the loading of the laticifer might first require a symplastic pathway for the transport of metabolites, at the end of which the assimilates must enter the apoplast. A transmembrane active transport system then transfers the metabolites in the laticifer. The presumable role of parenchyma cells in the loading of laticifers is emphasized.     

The Endodermoid in Garlic Scape: Its Fine Structure and Physiological Function

In garlic scape there is a distinct boundary layer of cells between the cortex and stele. Its fine structure and possible ruction seem to agree with the endodermoid first defined by Esau[7], hence the frame. Lightand electron-microscopic examination and cytochemical test have revealed that this particular laryer is probably responsible for the withdrawal of cellular contents of parenchyma to the peripheral vascular bundles, during a long period of storage the excised withering scape would thoroughly exhaust itself to give rise to the new apical cloves. As already shown, the laticiferous tubes scattered throughout the cortex are always turgid, and their sap is rich of nutrients in variable proportion[3]. Possibility of mobilizing these nutrients by the aid of endodermoid to join in phloem transport also has been discussed.     

STRUCTURE AND ONTOGENY OF LATICIFERS IN CICHORIUM INTYBUS (COMPOSITAE)

The branched anastomosed laticifer system in the primary body of Cichorium intybus L. originates in embryos from files of laticiferous members at the boundary between phloic procambium and ground meristem. Upon seed germination, laticiferous members develop perforations in the end walls which become entirely resorbed. Perforations also develop in the longitudinal walls of contiguous laticiferous members and from lateral connections between developing laticifer branches. Additional laticiferous members originate as procambium differentiation proceeds, and their differentiation follows a continuous acropetal sequence in leaf primordia of the plumule. In roots, laticifers closely associated with sieve tubes in the secondary phloem originate from derivatives of fusiform initials in the vascular cambium. These laticifers develop wall perforations and in a mature condition resemble laticifers in the primary body. As the girth of the root increases, laticifers toward the periphery, unlike associated sieve tubes, resist crushing and obliteration. Laticifers vary in width from about 4 to 22 μm; the widest ones occur in involucral bracts and the narrowest ones in florets. There was no evidence that intrusive growth occurs during development of the laticifer system, although such growth may occur during development of occasional branches which extend through ground tissue independent of phloem and terminate in contact with the epidermis. Presence of amorphous callose deposits is related to aging of laticifers and mechanical injury.     

Intercellular Transport of Macro-Molecular Substances as a Means of Redistribution of Cellular Contents in Detatched Garlic Scape

A detached garlic scape in long storage will eventually give rise to a whorl of freshy aerial cloves at its apex (Text fig. 2). This can only be brought about at the expense of the stalk proper, where withering starts from the lower end and extends gradually upward until the whole stalk is completely exhausted. The material transfer involved must be mainly concerned with the redistribution and reultilization of cellular contents from the senescing stalk to the growing cloves. The present systematic investigation on the whole process is primarily based upon serial microscopic and electronmicroscopic examination on conducting channels and withering parenchyma. Our previous investigations on garlic have shown that the exhaustive withdrawl of cellular contents from the senescing tissue is finally accomIished by intercellular movement of the partially disassembled protoplasm itself. The present result are essentially in agreement with such a general scheme. Light and electron-micrographs that show nuclear material and other macro-molecular substances tranversing through the plasmodesmata are rather common. The high resolving electronmicrographs have enabled us to detect the finer details in intercellular transport as given below: 1. Filamentous and fluffy material, somewhat similar in structure to P-protein in sieve tube, can be found in abundance in senescing parenchyma cells in which the demar- kations between protoplasmic components gradually become indistinct. The filamentous material is in transit through plasmodesmata between parenchyma cells and also between parenchyma and sieve tube (Plate Ⅱ, 16, 18). 2. Withdrawl of cellular contents from the deteriorating parenchyma may assume the form of vesicular transport through plasmodesmata (Plate Ⅰ 9, 10, 11). Some of the vesicles are simply filled with vacuolar sap; some fully packed with prefabricated material of maeromolecolar structure; and some actually loaded with disassembled protoplasmic fragments. 3. Fully packed vesicles as well as disassembled protoplasmie components (including disintegrated nucleus, degenerated mitoehondrion, etc.) may extrude into the intercellular spaces and may invade the vessel eavity (Plate Ⅱ, 12, 13, 20; Plate Ⅲ, 21, 22, 23, 24). The fine structure of the moving protoplasm in the vessel is quite distinct from that of the residual deposits which may cause plugging in the same cavity (Plate Ⅲ, 25, 26).     

Histochemical study of trans-polyisoprene accumulation by spectral confocal laser scanning microscopy and a specific dye showing fluorescence solvatochromism in the rubber-producing plant, Eucommia ulmoides Oliver

A microscopic technique combining spectral confocal laser scanning microscopy with a lipophilic fluorescent dye, Nile red, which can emit trans-polyisoprene specific fluorescence, was developed, and unmixed images of synthesized trans-polyisoprene in situ in Eucommia ulmoides were successfully obtained. The images showed that trans-polyisoprene was initially synthesized as granules in non-articulated laticifers that changed shape to fibers during laticifer maturation. Non-articulated laticifers are developed from single laticiferous cells, which are differentiated from surrounding parenchyma cells in the cambium. Therefore, these observations suggested that trans-polyisoprene biosynthesis first started in laticifer cells as granules and then the granules accumulated and fused in the inner space of the laticifers over time. Finally, laticifers were filled with the synthesized trans-polyisoprene, which formed a fibrous structure fitting the laticifers shape. Both trans- and cis-polyisoprene are among the most important polymers naturally produced by plants, and this microscopic technique combined with histological study should provide useful information in the fields of plant histology, bioindustry and phytochemistry.     

ORIGIN AND EARLY DEVELOPMENT OF NONARTICULATED LATICIFERS IN EMBRYOS OF EUPHORBIA MARGINATA

In E. marginata 12 nonarticulated laticifer initials arise in the cotyledonary node of the young embryo during the early heart stage. The initials arise progressively in the developing embryo, the first laticifers differentiating simultaneously with or shortly before the elements of the pro-cambium. The laticifers occupy a position lateral to the six procambial strands which are formed in the embryo. Upon subsequent growth each laticifer becomes vacuolated and nuclear division unaccompanied by cytokinesis results in the formation of a coenocytic protoplast. The enlarging laticifer produces several branches, one growing into the cotyledon, another growing down along the hypocotyl penetrating toward the root meristem, and one or several growing along intercellular spaces of adjacent cells. No fusion of these branches with one another or adjoining parenchyma cells was observed.     

Laticifers: An historical perspective

This review describes the development of the laticifer concept, with emphasis upon the nonarticulated type, from early observations of plant exudates and “juices” to the presentation of laticifers by Esau (1953). Classical writers and herbalists described practical applications of these substances. With the advent of the microscope early investigators believed that these substances occurred in structures present in most, if not all, plants and, wrongly, equated these structures to the circulatory system in animals. Introduction of the term, latex, into botany derived from its early use as a term for a blood component by physicians, and not for analogy to milk. However, the origin of the terms, laticifer and laticiferous, remains uncertain. Initial studies of laticifers were marked by the controversy of whether they represented intercellular spaces or elongated cells. Confirmation of their cellular character led to the designation of nonarticulated and articulated laticifers. Nonarticulated laticifers were shown to arise during early embryogeny in some plants. The ontogenetic origin of the articulated laticifer was unclear to early workers, but new laticifers were detected to be formed by cambium activity. Nonarticulated laticifers were described to develop by intrusive growth whereby tips of the cell penetrated between adjacent cells. The coenocytic condition of the nonarticulated laticifer resulted from nuclear divisions along the cell positioned in the growth region of the shoot and the subsequent distribution of the daughter nuclei along the length of the cell.     

Histochemical study of detailed laticifer structure and rubber biosynthesis-related protein localization in <Emphasis Type="Italic">Hevea brasiliensis</Emphasis> using spectral confocal laser scanning microscopy

In Hevea brasiliensis, laticifers produce and accumulate rubber particles. Despite observation using histochemical methods, development stage structure and structures with ceasing functions have rarely been described. Spectral confocal laser scanning microscopy with Nile red staining simplifies laticifer structure observation in tangential sections while enhancing the resolution. Laticifer and ray images were extracted from unmixed images and used to monitor changes during growth. A laticifer network structure developed from increased anastomoses between adjoining laticifers outside of the conducting phloem, but because of increased radial division and growth of rays, the network structure ruptured and disintegrated. We also investigated immunohistochemical localization of two rubber particle-associated proteins in the laticifers: small rubber particle protein (SRPP) and rubber elongation factor (REF). Mature bark test results show that SRPP is localized only in the laticifer layers in the conducting phloem; REF is localized in all laticifer layers. Because SRPP plays a positive role in rubber biosynthesis, results show that the rubber biosynthesis capability of laticifers is concentrated where rays and the sieve tube actively transport metabolites.     

宁夏枸杞果实韧皮部及其周围细胞超微结构研究

应用透射电镜技术研究了宁夏枸杞果实韧皮部细胞的超微结构变化。结果表明:(1)随着枸杞果实的发育成熟,果实维管组织中的韧皮部筛分子筛域逐渐变宽,筛孔大而多,通过筛孔的物质运输十分活跃;筛分子和伴胞间有胞间连丝联系,伴胞属传递细胞类型,与其相邻韧皮薄壁细胞和果肉薄壁细胞连接处的细胞界面发生质膜内突,整个筛分子/伴胞复合体与韧皮薄壁细胞之间形成共质体隔离,韧皮部糖分的卸载方式主要以质外体途径进行。(2)韧皮薄壁细胞间的胞间连丝较多,而韧皮薄壁细胞与果肉薄壁细胞的胞间连丝相对较少,但果肉薄壁细胞间几乎无胞间连丝;果肉薄壁细胞之间胞间隙较大,细胞壁和质膜内突间形成较大的质外体空间,为质外体的糖分运输创造了条件。(3)筛管、伴胞、韧皮薄壁细胞和果肉薄壁细胞中丰富的囊泡以及活跃的囊泡运输现象,暗示囊泡也参与了果实糖分的运输过程。研究推测,枸杞果实韧皮部同化物的卸载方式以及卸载后的同化物运输主要以质外体途径为主。     

Ultrastructure of Non-Articulated Laticifers in Allamanda violacea

Ultrastructure studies on the differentiation of non-articulatedbranched laticifers in Allamanda violacea Gardn. were carriedout. Growing laticifers show sequential changes. In the earlystage, the laticifers possess electron dense cytoplasm, abundantmitochondria, ER, ribosomes, small vacuoles, nucleus and plastidwith starch-grains. The ER dilates to form small vacuoles whichcoalesce at the later stages. A large central vacuole is formedin the mature laticifers due to the cellular autophagy of cytoplasmincluding the cell organelles. At this stage, the mitochondriapossess a few cristae and plastids with plastoglobuli and smallstarch grains. Towards the end of differentiation the cytoplasmis restricted to a thin parietal layer along the cell wall,the remaining organelles being either reduced in number or degenerate.Plasmodesmata and primary pit fields are occasionally observedbetween the laticifer and the adjacent parenchyma cell. Allamanda violacea, laticifers, ultrastructure     

Immunolocalization of beta-D-glucans,pectins, and arabinogalactan-proteins during intrusive growth and elongation of nonarticulated laticifers in Asclepias speciosa Torr

Nonarticulated laticifers are latex-containing cells that elongate indefinitely and grow intrusively between the walls of meristematic cells. To identify biochemical mechanisms involved in the growth of nonarticulated laticifers, we have analyzed the distribution of various polysaccharides and proteoglycans in walls of meristematic cells in contact with laticifers, nonadjacent to laticifers, and in laticifer walls. In the shoot apex of Asclepias speciosa, the levels of callose and a (1-->4)-beta-galactan epitope are lower in meristematic walls in contact with laticifers than in nonadjacent walls. In contrast, we did not detect a decline in xyloglucan, homogalacturonan, and arabinogalactan-protein epitopes upon contact of meristematic cells with laticifers. Laticifer elongation is also associated with the development of a homogalacturonan-rich middle lamella between laticifers and their neighboring cells. Furthermore, laticifers lay down walls that differ from those of their surrounding cells. This is particularly evident for epitopes in rhamnogalacturonan I. A (1-->5)-alpha-arabinan epitope in this pectin is more abundant in laticifers than meristematic cells, while the opposite is observed for a (1-->4)-beta-galactan epitope. Also, different cell wall components exhibit distinct distribution patterns within laticifer walls. The (1-->5)-alpha-arabinan epitope is distributed throughout the laticifer walls while certain homogalacturonan and arabinogalactan-protein epitopes are preferentially located in particular regions of laticifer walls. Taken together, our results indicate that laticifer penetration causes changes in the walls of meristematic cells and that there are differences in wall composition within laticifer walls and between laticifers and their surrounding cells.     

A morphometric analysis of the phloem-unloading pathway in developing tobacco leaves

A morphometric analysis of developing leaves of Nicotiana tabacum L. was conducted to determine whether imported photoassimilates could be unloaded by symplastic transport and whether interruption of symplastic transport could account for termination of import. Five classes of veins were recognized, based on numbers of cells in transverse section. Photoassimilate is unloaded primarily from Class III veins in tissue nearing the end of the sink phase of development. Smaller veins (Class IV and V) do not transport or unload photoassimilate in sink tissue because the sieve elements of these veins are immature until after the tissue stops importing. In Class III veins the sieve element-companion cell (SE-CC) complexes are surrounded by phloem parenchyma which abuts the bundle sheath. Along the most obvious unloading route, from SE-CC complex to phloem parenchyma to bundle sheath to mesophyll cells, the frequency of plasmodesmata at each interface increases. To determine whether this pattern of plasmodesmatal contact is consistent with symplastic unloading we first demonstrated, by derivation from Fick's law that the rate of diffusion from a compartment is proportional to a number N which is equal to the ratio of surface area to volume of the compartment multiplied by the frequency of pores (plasmodesmata) which connect it to the next compartment. N was calculated for each compartment within the vein which has the SE-CC complex as its center, and was shown to be statistically the same in all cases except one. These observations are consistent with a symplastic unloading route. As the leaf tissue matures and stops importing, plasmodesmatal frequency along the unloading route decreases and contact area between cells also decreases as intercellular spaces enlarge. As a result, the number of plasmodesmata between the SE-CC complex and the first layer of mesophyll cells declines in nonimporting tissue to 34% of the number found in importing tissue, indicating that loss of symplastic continuity between the phloem and surrounding cells plays a role in termination of photoassimilate unloading.Abbreviation SE-CC sieve element-companion cell     

文冠果果实韧皮部及其周围薄壁细胞的超微结构观察及功能分析

该研究应用透射电镜技术,对生长发育过程中的文冠果果实的韧皮部及其周围薄壁细胞的超微结构进行了观察,以探讨文冠果果实同化物韧皮部卸载的细胞学路径及其机理。结果显示:(1)文冠果果实发育过程中,筛分子细胞胞腔较空,几乎没有细胞器,但有类似于囊泡的丝状不定型物存在;伴胞胞质浓密且细胞器丰富,液泡化程度不一,大多数存在多个小液泡;薄壁细胞具有中央大液泡,发育中期富含线粒体、高尔基体、内质网等细胞器,并存在囊泡运输现象,发育后期细胞器发生降解,说明随着果实生长发育,果实内物质代谢和转运活跃程度逐渐下降。(2)果实发育过程中筛分子和伴胞之间始终有胞间连丝,薄壁细胞之间也一直存在大量的胞间连丝,而筛分子-伴胞复合体与薄壁细胞之间只有在果实发育前期和后期存在一定数量的胞间连丝,发育中期却几乎没有胞间连丝。研究结果表明,文冠果果实发育过程中同化物韧皮部卸载路径可能发生了共质体途径-质外体途径-共质体途径的转变。     

Localization of cell wall polysaccharides in nonarticulated laticifers ofAsclepias speciosa Torr.

Summary Asclepias speciosa Torr, has latex-containing cells known as nonarticulated laticifers. In stem sections of this species, we have analyzed the cell walls of nonarticulated laticifers and surrounding cells with various stains, lectins, and monoclonal antibodies. These analyses revealed that laticifer walls are rich in (1→4) β-D-glucans and pectin polymers. Immunolocalization of pectic epitopes with the antihomogalacturonan antibodies JIM5 and JIM7 produced distinct labeling patterns. JIM7 labeled all cells including laticifers, while JIM5 only labeled mature epidermal cells and xylem elements. Two antibodies, LM5 and LM6, which recognize rhamnogalacturonan I epitopes distinctly labeled laticifer walls. LM6, which binds to a (l→5) α-arabinan epitope, labeled laticifer walls more intensely than walls of other cells. LM5, which recognizes a (1→4) β-D-galac-tan epitope, did not label laticifer segments at the shoot apex but labeled more mature portions of laticifers. Also the LM5 antibody did not label cells at the shoot apical meristem, but as cells grew and matured the LM5 epitope was expressed in all cells. LM2, a monoclonal antibody that binds to β-D-glucuronic acid residues in arabinogalactan proteins, did not label laticifers but specifically labeled sieve tubes. Sieve tubes were also specifically labeled byRicinus communis agglutinin, a lectin that binds to terminal β-D-galactosyl residues. Taken together, the analyses conducted showed that laticifer walls have distinctive cytochemical properties and that these properties change along the length of laticifers. In addition, this study revealed differences in the expression of pectin and arabinogalactan protein epitopes during shoot development or among different cell types.     

Laticifer Differentiation in Hevea brasiliensis: Induction by Exogenous Jasmonic Acid and Linolenic Acid

Laticifer differentiation of Hevea brasiliensis was investigatedby application of lanolin containing jasmonic acid (JA) or otherchemicals to the surface of young stems in epicormic shoots.The young stems had primary laticifers and no secondary laticifers.When applied to extending young stems, JA led to a significantincrease in primary laticifer number but did not induce secondarylaticifer differentiation. Secondary laticifer differentiationand a less significant increase in primary laticifer numberwere caused by JA application to the extended young stems. Theinduction of the secondary laticifers was dependent on the concentrationof JA applied. Cambium cell division leading to the formationof secondary phloem was not accelerated by JA treatment. Treatedbark tissues showed no visible changes except for the additionallaticifers, which were normal in ultrastructure. The secondarylaticifers were also induced by the application of linolenicacid, a precursor of JA biosynthesis. Abscisic acid, ethephonand salicylic acid had no detectable effect on laticifer differentiation.Copyright 2000 Annals of Botany Company Hevea brasiliensis, laticifer differentiation, jasmonic acid, linolenic acid, vascular cambium.     

THE STRUCTURE AND DEVELOPMENT OF AN UNUSUAL TYPE OF ARTICULATED LATICIFER IN MAMMILLARIA (CACTACEAE)

Although the laticifers of several species of Mammillaria can technically be classified as being of the articulated type, they differ significantly from all other reported articulated laticifers. They are derived from cells which differentiate only in older tissues, never in meristematic or young regions. The development involves the complete lysis of masses of cells, not just the perforation or resorption of the end walls in a single file of cells. At maturity, the laticifer lumen is lined with a one-to-several layered epithelium which may be quite thick. The laticifers increase in diameter with age, apparently by the lysis of the inner epithelial cells. Laticifers occur in the pith, cortex and tubercles of the vegetative body but were not observed in the roots, flower parts or in seedlings up to eight months old. Seven species were studied, all of which have “milky sap.” and the laticifers of each were virtually identical to the laticifers of the others.     

Intercellular Symplastic Connection and Isolation of the Unloading Zone in Flesh of the Developing Grape Berry

The uhrastructure and intercellular connection of the sugar unloading zone (i. e. the phloem in the dorsal vascular bundle and the phloem-surrounding the assimilate sink-cells) of grape ( Vitis vinifera x V. labrusca cv. Jingchao) berry was observed via transmission electron microscopy. The results showed that during the early developmental stages of grape berry, numerous plasmodesmata were found in the phloem between sieve element (SE) and companion cell (CC), between SE/CC complexes, between SE/CC complex and phloem parenchyma cell and in between phloem parenchyma cells, which made the phloem a symplastic integration, facilitating sugar unloading from sieve elements into both companion cells and phloem parenchyma cells via a symplastic pathway. On the contrary, there was almost no plasmodesma between phloem and its surrounding flesh photoassimilate sink-cells, neither in between the flesh photoassimilate sink-cells giving rise to a symplastic isolation both between phloem and its surrounding flesh photoassimilate sink-cells, as well as among the flesh photoassimilate sink-cells. This indicated that both the sugar unloading from phloem and pestphloem transport of sugars should be mainly via an apoplastic pathway. Dining the ripening stage, most of the plasmodesmata between SE/CC complex and the surrounding phloem parenchyma cells were shown to be blocked by the electron-opaque globules, and a phenomenon of plasmolysis was found in a number of companion cells, indicating a symplastic isolation between SE/CC complex and its surrounding parenchynm cells during this phase. The symplastic isolation between the whole phloem and its surrounding photoassimilate sink-cells during the early developmental stages shifted to a symplastic isolation within the phloem during the ripening phase, and thus the symplastic pathway of sugar unloading from SE/CC complex during the early development stages should be replaced by a dominant apoplastic unloading pathway from SE/CC complex in concordance.     

FOSSIL LATICIFERS FROM EOCENE BROWN COAL DEPOSITS OF THE GEISELTAL

Thick mats of cellular remains from Eocene brown coal deposits of the Geiseltal near Halle, DDR, were determined to be fossil nonarticulated laticifers. Nuclear magnetic resonance analyses of intact strands showed they consisted of eis-1,4-configuration rubber representing the polymerized isoprenoid contents of individual laticifers. Only remains of laticifers are present; other cells are absent as a result of biodegradation. The long laticifers, often with a surrounding cell wall, retained a tubular shape during their preservation. The isoprenoid content, which filled the entire lumen, possessed a cribriform structural character. The interstices within the rubber represent areas of former protoplasm of the cell. Various configurations in the protoplasm molded by the rubber during the initial phase of fossilization appear as negative images of former nuclei, organelles, and possibly membrane surfaces. The laticifer axes possess branches of several configurations comparable in morphology to those in branched, nonarticulated laticifers in extant plants. Acetone extracts of the rubber contents analyzed by gas-liquid chromatography identified the presence of several hydrocarbons which form a characteristic profile for the laticifer. It is suggested that the distinctive cellular micromorphology, rubber configuration, and hydrocarbon profile of these laticifers can be employed as markers in comparative studies with extant plants to identify the generic or species origin of these laticifers.     

MITOSIS IN THE NON-ARTICULATED LATICIFER OF EUPHORBIA MARGINATA

The multinucleate condition in the non-articulated laticifers of embryos of Euphorbia marginata arises as a result of mitosis. Successive stages of mitosis in the nuclei of the laticifer appear in the form of a wave. No sequence of mitotic stages has been noticed in the neighboring longitudinal tiers of cells. This difference in the mitotic pattern in the laticifer and other parenchymatous cells of the embryo suggests that the synthesis of factor(s) responsible for triggering mitosis occurs within the laticifer and does not diffuse to the surrounding cells. The mitotic waves originate distally from the meristems, either in the cotyledonary or hypocotyl portion of the laticifer, and move uni- or bidirectionally along its longitudinal axis. The mitotic stimulus does not start simultaneously in all the laticifers. The variable velocity of the mitotic substance results in aphasic mitotic waves in laticifers of the same embryo. Mitotic aberrations have not been observed in the dividing nuclei of the laticifer. A chromosome estimation made from a polar view of metaphase does not suggest polyploidization in the observed laticifers.