POLYGONAL ASPECTS OF CELL FACES. I. PENTAGONS AND HEXAGONS AS PREVAILING TYPES

Wheeler , George E. (Brooklyn Coll., Brooklyn, N. Y.) Polygonal aspects of cell faces. I. Pentagons and hexagons as prevailing types. Amer. Jour. Bot. 49(3): 246–252. Illus. 1962.—Different types of cell faces, classified as to polygon type (i.e., number of sides per face), may predominate in different samples of internal cells and of internal tissues; no single face type is exclusively predominant in all tissues. Pentagons usually are the most numerous type in the cell samples reported in the literature, but hexagons exceed them in some samples. Generally, these 2 “compete” for numerical supremacy. Perpetuation of an already-established, face-type dominance was studied, using data from the literature and from original diagrams. Cell-division orientation, i.e., the location and the relative positioning of new cell-division walls, was found to be the prime factor in maintaining the preponderant type. The polygon nature of the new wall is an additional, but less important, factor. Typical division events tend to favor pentagonal faces; but with an increase in cell division “regularity,” hexagons begin to rise in numbers. During the early stages in tissue differentiation, while mitosis is still occurring, one face type may replace another as the predominating type. Such a shift may be associated with the developmental characteristics of that tissue.     

POLYGONAL ASPECTS OF CELL FACES. III. CELL SIZE,CELL DIVISION,AND CELL FACE DISTRIBUTIONS

Wheeler , George E. (Brooklyn Coll., Brooklyn, New York.) Polygonal aspects of cell faces. III. Cell size, cell division, and cell face distributions. Amer. Jour. Bot. 50(8): 747–754. Illus. 1963.—The effects of cell size differences on cell face (polygon type) distributions, and the relationship of cell division to these effects were investigated, using published and original data. Only “relative” size was considered, i.e., the size of a body compared with the sizes of contiguous bodies. A preliminary study of mixtures including 2 sizes of nonliving bodies (bubbles or shot) showed that, with increase in number of smaller bodies relative to larger, 4- and 5-gons decrease and 6-gons increase on both large and small bodies (except for 5-gons on small bubbles). Since the cited papers on cells generally include no volume measurements, cell size was assumed to be proportional to number of faces; therefore, the cells from each sample were pooled in 3 groups of different ranges as to number of faces per cell. This device made evident the 4- and 5-gon decreases and the 6-gon increases with increasing size, but only in certain samples;- marked exceptions occurred among others. New data from 2 original samples showed, in general, the correlations described above, but again then; were exceptions. Discrepancies were found to arise from variable division patterns which affect face types both directly, and indirectly through division effects on cell size. It was concluded that relative size is generally less important in determining cell face distributions than are the more direct cell division events, and that size difference effects can be detected only if the other events operate minimally.     

Fine structural analysis of membrane changes during reaggregation culture of chick optic tectum

Thin section and freeze-fracture electron microscopy have been used to characterize the changes in membrane morphology of reaggregating cultures of chick optic tectum. The cells are rounded and freely dispersed at 0 hr after dissociation. Between 2 and 6 hr the cells become closely apposed on all sides by other cells and form small aggregates. At this time punta adhaerentia junctions and focal densities are seen along the membranes of neighboring cells. Between 1 and 5 days in vitro (DIV) neurites containing growth cone regions are present. At 5 DIV the first synaptic contacts are observed. Between 7 and 14 DIV, the number of synaptic contacts increase and fewer growth cone regions are observed. As early as 7 DIV profiles are observed which strongly resemble both astrocytic and oligodendroglial cell somata and processes. Freeze-fracture analysis of aggregates at 0–4 hr reveals a sparse particle distribution on the P and E faces of apposed cells. By 1 DIV small clusters of loosely packed, large sized particles are seen on the P face of apposed cell membranes which may represent junctional contacts. Apparent coated vesicle fusion sites are common on the P face at 1–2 DIV. By 7 DIV, E face particle arrays are seen on cell bodies and neurites which correspond to specializations characteristic of excitatory synaptic junctions. By 8–10 DIV particle arrays are seen on the P face of post-synaptic membrane which may represent inhibitory synaptic contacts. Other types of particle specializations seen in freeze-fracture replicas include: specializations characteristic of gap junctions between cells and orthogonal assemblies of particles thought to be characteristic of astrocytes.     

The generation of curved clathrin coats from flat plaques

Flat clathrin lattices or 'plaques' are commonly believed to be the precursors to clathrin-coated buds and vesicles. The sequence of steps carrying the flat hexagonal lattice into a highly curved polyhedral cage with exactly 12 pentagons remains elusive, however, and the large numbers of disrupted interclathrin connections in previously proposed conversion pathways make these scenarios rather unlikely. The recent notion that clathrin can make controlled small conformational transitions opens new avenues. Simulations with a self-assembling clathrin model suggest that localized conformational changes in a plaque can create sufficiently strong stresses for a dome-like fragment to break apart. The released fragment, which is strongly curved but still hexagonal, may subsequently grow into a cage by recruiting free triskelia from the cytoplasm, thus building all 12 pentagonal faces without recourse to complex topological changes. The critical assembly concentration in a slightly acidic in vitro solution is used to estimate the binding energy of a cage at 25-40 k(B) T/clathrin.     

Nonatomic solvent-driven Voronoi tessellation of proteins: an open tool to analyze protein folds

A three-dimensional Voronoi tessellation of folded proteins is used to analyze geometrical and topological properties of a set of proteins. To each amino acid is associated a central point surrounded by a Voronoi cell. Voronoi cells describe the packing of the amino acids. Special attention is given to reproduction of the protein surface. Once the Voronoi cells are built, a lot of tools from geometrical analysis can be applied to investigate the protein structure; volume of cells, number of faces per cell, and number of sides per face are the usual signatures of the protein structure. A distinct difference between faces related to primary, secondary, and tertiary structures has been observed. Faces threaded by the main-chain have on average more than six edges, whereas those related to helical packing of the amino acid chain have less than five edges. The faces on the protein surface have on average five edges within 1% error. The average number of faces on the protein surface for a given type of amino acid brings a new point of view in the characterization of the exposition to the solvent and the classification of amino acid as hydrophilic or hydrophobic. It may be a convenient tool for model validation.     

The histochemistry of the avian parathyroid and ultimobranchial glands. I. Carbohydrates and proteins

Synopsis The non-enzyme histochemistry of the closely related parathyroid and ultimobranchial glands of the domestic fowl has been studied.The parathyroid cells and the ultimobranchial C cells gave only weakly positive reactions in tests for specific amino-acid residues. The rather stronger reactions found in the C cells were probably related to their content of polypeptide secretory granules. Carbohydrate and lipid stains also gave only negative or weakly positive reactions although the parathyroid cells did contain some free lipid.The lining cells of the ultimobranchial vesicles may be either actively secreting or inactive and cystic. Active cells contain large numbers of granules that are composed of large amounts of sulphated acid mucopolysaccharides, moderate amounts of mucoproteins and small amounts of neutral mucopolysaccharides and glycogen. Both the granular and colloidal secretions of these cells appeared to be identical in composition to the intracellular granules. The vesicular lining cells and their secretions showed strong but variable reactions for sulphydryl, disulphide and amino groups.The intermediate cell strands, which connect the ultimobranchial parathyroid foci with the vesicles, showed a range of reactions intermediate between those exhibited by parathyroid and vesicular cells.The results are discussed in relation to the structure and function of the various cell types.     

Mechanically facilitated cell-cell electrofusion.

Apparatus and methods were developed to enable mechanically facilitated cell-cell electrofusion to be performed. The apparatus and methods mechanically place cells in contact before fusion. The key component of this fusion system was a newly developed fusion chamber. The chamber was composed of two functionally identical electrodes that were housed in a multi-layer structure. The layers functioned as support for the electrodes. They also allowed adjustment of the distance between opposing electrode faces. The electrodes were constructed in a manner that allowed cells to be deposited, by vacuum, onto each face. Electrode faces were positioned at a predetermined distance from each other to mechanically force cell-cell contact between the deposited cells. Fusion was induced by delivering direct current pulses to the juxtaposed cells. Fusion products were detected and quantitated by flow cytometry. Details of the chamber design and a protocol for using the fusion chamber are given. Mechanically facilitated cell-cell electrofusion was demonstrated by using the chamber to produce fusion products from like fusion partners. The practical applicability of the chamber was demonstrated by fusing unlike cell types. Mechanically facilitated cell-cell electrofusion is not specific to the cells used in this study; the chamber can be adapted for use with other cell types.     

Morphometric analysis of the surface cells of rabbit corneal epithelium by scanning electron microscopy

The corneal surface of female New Zealand white rabbits (1.9-2.6 kg) was examined at x500 magnification by scanning electron microscopy. A total of 112 micrographs, taken as sequential sets from the center to the edge of the corneal surface from 8 different animals, was analyzed using a digitizer pad. Each cell was identified by the number of immediately bordering cells and by the nature of its electron reflex (light, medium, dark). Analysis of areas of the cells by number of bordering cells (number of cell sides) reveals a wide range of areas and skewed distributions especially when the number of sides is 5 or less. Overall, the cell-surface area increases as the number of cell sides increases. However, analyses of the mean surface areas for cells with different numbers of sides and additionally grouped by electron reflex suggests the existence of three separate populations of cells at the corneal surface. The possible etiology and dynamics of this complex cell mosaic are discussed in relation to circadian rhythms and to resurfacing of the cornea following mechanical trauma, ultraviolet radiation, and toxic chemical exposure.     

Magnetosome chain arrangement and stability in magnetotactic cocci

We have studied the disposition of chains of magnetosomes inside magnetotactic cocci with light and electron microscopy. Light microscopy of isolated cocci indicated that the chains of magnetosomes are disposed on opposite sides of the cell. Electron spectroscopic imaging of whole unprocessed bacteria, showed the magnetosome chains in the cells. Freeze-etching of the cell surface allowed the observation of the close association of the chain with the cell surface. During the replication process of the freeze-etching, the magnetosome chains remained attached to the replicas, which indicates that chains were very close to the cell surface before freezing. We provide evidence that the large area of the contact faces between magnetosomes in a chain may provide an extra mechanical stability that helps keep the magnetosomes in chains even after isolation from the bacteria. Comparison with pointed magnetosomes from different cocci present in the same samples showed that the maintenance of linear chains is more difficult to be achieved because of the geometry of the crystals.     

Charge distribution on the S layer of Bacillus stearothermophilus NRS 1536/3c and importance of charged groups for morphogenesis and function.

The distribution and functional significance of charged groups on the outer and inner faces of the S layer from Bacillus stearothermophilus NRS 1536/3c was investigated. Chemical modification of the exposed amino or carboxyl groups was performed on whole cells, isolated S layers self-assembled in vitro, and cell wall fragments (S layer attached to the peptidoglycan-containing sacculus). Without chemical modification, S layer self-assembly products could be labeled with polycationic ferritin, while S layers on whole cells could not. Following treatment with glutaraldehyde, whole cells were uniformly labeled with polycationic ferritin. Whole cells treated with glutaraldehyde and glycine methyl ester in the presence of carbodiimide did not bind polycationic ferritin significantly above background. Treatment of cell wall fragments with amino-specific, homobifunctional cross-linkers or with carbodiimide alone rendered the S layer protein nonextractable with sodium dodecyl sulfate. After amidation of the accessible carboxyl groups, the modified, guanidine hydrochloride-extractable S layer protomers did not self-assemble into regularly structured lattices. N-Amidination with ethylacetimidate did not interfere with the self-assembly of the isolated protomers. N-Acetylation resulted in a considerable destabilization of the S layer lattice, as seen by the release of a large amount of modified protomers during the reaction. N-Succinylation led to a complete disintegration of the protein lattice. These results indicated that only the inner face of the S layer carried a net negative charge. On both faces, free amino and carboxyl groups of adjacent protomers were arranged in proximity so as to contribute by electrostatic interactions to the cohesion of the protomers in the two-dimensional array. The native charge of the protomers was required for both the in vitro self-assembly of the isolated subunits and the maintenance of the structural integrity of the S layer lattice. Among other functions, the biological significance of the S layers may be in masking the electronegative charge of the cell wall proper.     

Structure and development of stellate trichomes in Andradea ftoribunda Fr. Allem. (Nyctaginaceae)

LOURO, R. P., MIGUENS, F. C. & MACHADO, R. D., 1992. Structure and development of stellate trichomes in Andradea ftoribunda Fr. Allem. (Nyctaginaceae). Trichomes occur on both faces of young leaves. They are peltate-stellate on the abaxial face, and comprise a stalk and radiating cells with a rudimentary central apex. On the adaxial face the trichomes arc stellate with a large apex comprising one to three cells. In both cases the stalk is formed by three to six cells of which the most distal may contain a tannoid substance. In the adult leaf only the abaxial surface exhibits stellate trichomes, with two to three celled stalks. The central region of radial cells is depressed. On the adaxial side the hairs are shed during maturation of the leaf.     

Functional micromorphology of petals of <Emphasis Type="Italic">Chaenomeles japonica</Emphasis> exposed to humid and cold season

In this study, micro- and nano-traits of petal epidermises of flowers of Chaenomeles japonica extended under environmental conditions, during the humid and cold period of the year, are presented. The outer (abaxial) and the inner (adaxial) epidermises of petals of C. japonica consist of convex and papillae cells, respectively, that are covered by epicuticular wrinkled relief further ornamented by submicron motifs, forming interfaces between floral tissues and environment. Structural epidermal features of the petal relief at the nanoscale level reveal different functionality on the two sides of the corolla. The cuticular folds of convex epidermal cells display declining water retention on the outer petal surface and the exposed side of the corolla to the environmental conditions. The cuticular folds of papillae epidermal cells increase in size the inner petal surface, in comparison with the outer surface; such traits facilitate light absorption and enhanced the contact area among folds and curvatures at the inner side of the corolla. It appears that nanometric surface structures of petals may be important adaptive features of C. japonica flowers, contributing to their performance in the field.     

The eyespot of the flagellateTetraselmis cordiformis stein (Chlorophyceae): Structural spezialization of the outer chloroplast membrane and its possible significance in phototaxis of green algae

Summary The eyespot region of the flagellateTetraselmis cordiformis Stein (Chlorophyceae) was investigated with the freeze-fracture technique. The only fracture faces observed in this region were the two complementary fracture faces (PF and EF) of the outer chloroplast envelope membrane. Intramembranous particle numbers on both fracture faces of this membrane were significantly higher in the eyespot region as compared to regions outside the eye-spot. Higher numbers of particles on the PF face in the eyespot region were mainly caused by an increase in particle numbers of the size class 6–8 mm, while on the EF face particle size distribution was not significantly different between eyespot and other regions. Functional implications are discussed and evidence is presented that the outer chloroplast envelope membrane may be the site of photoreceptor location in green algal phototaxis.     

Rotary-Shadowed Freeze-Fracture Replicas: A Simple Method for the Analysis of Fracture Faces

In rotary-shadowed freeze-fracture replicas, intramembrane particles on the periphery of a membrane fracture face are not uniformly shadowed from all sides. Those eccentrically positioned intramembrane particles with a net centripetally directed shadowing are on a convex fracture face. In contrast, those eccentrically positioned intramembrane particles with a net centrifugally directed shadowing are on a concave fracture face. Centrally positioned intramembrane particles on convex faces are uniformly shadowed from all sides; however, central depressions of concave faces are often unshadowed.     

假瘤蕨属（水龙骨科）植物叶表皮特征的比较研究

在光镜和扫描电镜下观察了假瘤蕨属2系、5亚系的24种植物的叶表皮。结果表明,叶表皮细胞形状不规则,垂周壁波曲状。下生气孔,气孔类型有极细胞型、共环极细胞型、腋下细胞型、聚腋下细胞型和不规则型,常伴生出现。在扫描电镜下,叶表皮气孔器外拱盖内缘为浅波状、少平滑;一些种的保卫细胞两端有“T”型加厚;角质膜波状有条纹,有时附有颗粒。叶表皮的一些特征对该属部分种的区分有一定的参考价值。叶表皮的微形态特征,如气孔器类型和垂周壁类型特征不能用来界定假瘤蕨属的系和亚系。     

Rotary-shadowed freeze-fracture replicas: a simple method for the analysis of fracture faces

In rotary-shadowed freeze-fracture replicas, intramembrane particles on the periphery of a membrane fracture face are not uniformly shadowed from all sides. Those eccentrically positioned intramembrane particles with a net centripetally directed shadowing are on a convex fracture face. In contrast, those eccentrically positioned intramembrane particles with a net centrifugally directed shadowing are on a concave fracture face. Centrally positioned intramembrane particles on convex faces are uniformly shadowed from all sides; however, central depressions of concave faces are often unshadowed.     

假瘤蕨属 (水龙骨科) 植物叶表皮特征的比较研究

在光镜和扫描电镜下观察了假瘤蕨属2系、5亚系的24种植物的叶表皮。结果表明,叶表皮细胞形状不规则,垂周壁波曲状。下生气孔,气孔类型有极细胞型、共环极细胞型、腋下细胞型、聚腋下细胞型和不规则型,常伴生出现。在扫描电镜下,叶表皮气孔器外拱盖内缘为浅波状、少平滑;一些种的保卫细胞两端有“T”型加厚;角质膜波状有条纹,有时附有颗粒。叶表皮的一些特征对该属部分种的区分有一定的参考价值。叶表皮的微形态特征,如气孔器类型和垂周壁类型特征不能用来界定假瘤蕨属的系和亚系。     

Culture and filtration methods for obtaining Pneumocystis carinii trophozoites and cysts.

Two methods for acquisition of Pneumocystis carinii (Pc) trophozoites and cysts are reported. One method, the isolation of Pc from infected rat lung, provides large numbers of trophozoites and cysts but retains rat proteins. Ground lung is filtered through a series of Nucleopore filters from 10 to 3 microns; 1 g of rat lung yields an average of 1.1 x 10(9) Pc trophozoites and 1 x 10(7) cysts. The second method, propagation of Pc in culture with human embryonic lung cells on microcarrier beads, provides Pc trophozoites which are relatively free of host lung material. Cultured organisms may be filtered to remove rare culture monolayer cells. Organisms harvested from filtered lung are free from intact host cells and cell nuclei, however, host cell proteins and host DNA remain. Organisms from culture have minimal host contamination.     

Use of glass beads and CF 11 cellulose for removal of leukocytes from malaria-infected human blood in field settings.

Passage of malaria-infected blood through a two-layered column composed of acid-washed glass beads and CF 11 cellulose removes white cells from parasitized blood. However, because use of glass beads and CF 11 cellulose requires filtration of infected blood separately through these two resins and the addition of ADP, the procedure is time-consuming and may be inappropriate for use in the field, especially when large numbers of blood samples are to be treated. Our modification of this process yields parasitized cells free of contaminating leukocytes, and because of its operational simplicity, large numbers of blood samples can be processed. Our procedure also compares well with those using expensive commercial Sepacell resins in its ability to separate leukocytes from whole blood. As a test of usefulness in molecular biologic investigations, the parasites obtained from the blood of malaria-infected patients using the modified procedure yield genomic DNA whose single copy gene, the circumsporozoite gene, efficiently amplifies by polymerase chain reaction.     

The function of the golgi complex in transitional epithelium. Synthesis of the thick cell membrane

The superficial squamous cells of rat transitional epithelium are limited, on their luminal face, by an asymmetrically thickened membrane. Patches of similar thick membrane are found in the walls of the Golgi cisternae and it is suggested that the Golgi system is the site of assembly of the thick plasma membrane. This implies membrane flow from the Golgi apparatus to the cell surface, and there is indirect evidence that the membrane is transported in the form of fusiform vacuoles, derived from the Golgi cisternae, which fuse with, and become part of, the free cell membrane. Uptake of injected Imferon shows that similar, large, thick-walled vacuoles may be formed by invagination of the free cell surface. Some of these vacuoles are subsequently transformed into multivesicular bodies and autophagic vacuoles. The formation of other large heterogeneous bodies is described, and some of these are shown to have acid phosphatase activity.