ECOLOGICAL CONSIDERATIONS OF DIATOM CELL MOTILITY. I. CHARACTERIZATION OF MOTILITY AND ADHESION IN FOUR DIATOM SPECIES1

To better determine the ecological role of motility in pennate diatoms, we quantitatively characterized several motility and adhesion properties of four species of motile pennate diatoms (Craticula sp., Pinnularia sp., Nitzschia sp., and Stauroneis sp.) isolated from the same freshwater pond. Using computer-assisted video microscopy, we measured speed, size/shape, functional adhesion, path curvature, and light sensitivity for these species, each of which shows a distinctive set of motile behaviors. The average speeds of Stauroneis, Pinnularia, Nitzschia, and Craticula cells are 4.6, 5.3, 10.4, and 10.0 μm · s^?1, respectively. Craticula and Nitzschia cells move in a relatively straight path (<4 degrees rotation per 100 μm movement), Stauroneis exhibits minor rotation (about 7 degrees per 100 μm movement), and Pinnularia rotates considerably during movement (about 22 degrees per 100 μm moved). Functional adhesion (as measured by the release rate of attached cells from the underside of an inverted coverslip) shows a half time for cell release of approximately 50 min for Craticula, 192 min for Pinnularia, and >1 day for Nitzschia and Stauroneis. Direction reversal at light/dark boundaries, which appears to be the main contributor to diatom Phototaxis, is most responsive for Craticula, Pinnularia, and Nitzschia at wavelengths around 500 nm. Craticula and Nitzschia cells are the most sensitive in the photophobic response, with over 60% of these cells responding to a 30-1x light/dark boundary at 500 nm, whereas Pinnularia cells are only moderately responsive at this irradiance, showing a maximal response of approximately 30% of cells at 450 nm. Stauroneis cells, in contrast, had a maximal photosensitive response at 700 nm, suggesting that this cell type may use a different response mechanism than the other three cell types. In addition, Craticula and Pinnularia show a net movement out of the light spot when illuminated at 650 nm, whereas Stauroneis shows a net movement out of the light spot when illuminated at 450 nm. Such quantitative characterizations of species-specific responses to environmental stimuli should give us a firm foundation for future studies analyzing the behavior of interspecies diatom competition for limited light or nutrient resources.     

CELL CYCLE DURATION IN THE MERISTEM OF NEPHROLEPIS BISERRATA STOLONS: THE ROLE OF THE APICAL CELL

The stolons of Nephrolepis biserrata (sw.) Schott are thin axes that grow rapidly (from 2 to 4 mm per day) in the controlled conditions applied. In the cylindro-conical meristem, three histological zones are defined. Cell cycle duration was determined for each zone by autoradiographic methods after incorporation of tritiated thymidine and confirmed by the colchicine-induced metaphase-accumulation technique. The apical cell and its derivatives (Zone 1) are mitotically more active (cell cycle duration: 80 hr) than the cells of the subapical zones (2 and 3), where cell cycle lengths are 142 hr and 95 hr respectively. These data, compared to previous results, give evidence for the main role played by the relative rate of division of the apical cell compared to that of lateral cells in the organization and the shape of the meristem of pteridophytes. Moreover, the apical cell appears to be unique in having a differentiated cytological aspect not usually associated with an intensely proliferating cell.     

GROWTH AND DIFFERENTIATION OF CYTOPLASMIC MEMBRANES IN THE COURSE OF LIPOPROTEIN GRANULE SYNTHESIS IN THE HEPATIC CELL : I. Elaboration of Elements of the Golgi Complex

The synthesis of "very low" density lipoprotein in liver cells is characterized by the fact that the synthesized products, mostly triglycerides, are processed in the form of discrete, size-limited granules or globules, about 400 A in diameter. The present investigation has been made possible in part by the use of a fixative (OsO₄ in bidistilled H₂O at pH 6.0, in the absence of electrolytes) particularly effective in preserving cytoplasmic membranes and lipids, and giving them high stainability and differential contrast. Under these technical conditions, the lipoprotein granules retain their morphology and high density to electrons practically unaltered, and may serve as tracers in determining their route of transport from the sites of synthesis, starting at the rough-smooth ER junctions, to the lumen of Golgi concentrating vesicles. From the observations, it may be deduced that, along with lipoprotein granule synthesis and transport, there are also production and transfer of new membranes in the form of tubular extensions of smooth ER network which, by progressive fusion and coalescence, participate in the elaboration of fenestrated plates and solid Golgi sacs. In contradistinction to the entire process of liver lipoprotein granule synthesis, transport, and segregation, as reported in the present paper, appears to constitute a developmental sequence which includes the following communicating compartments, in consecutive order: cisternae of rough ER where proteins and possibly phospholipids are synthesized, smooth ER network where triglycerides are synthesized and transported in the form of dense granules, fusion of smooth ER tubular extensions into Golgi fenestrated plates, and further coalescence into solid Golgi sacs, ending in the segregation of the granules in appended concentrating vesicles, or detached "secretory vesicles." It seems that it is this progressive evolution in growth and configuration of membranes which is reflected in the so called polarity, from forming to mature faces, of the Golgi apparatus.     

ROLE OF SULFUR IN THE CELL DIVISION OF CHLORELLA, WITH SPECIAL REFERENCE TO THE SULFUR COMPOUNDS APPEARING DURING THE PROCESS OF CELL DIVISION. I.

1. The role of sulfur in the cell division of Chlorella was studiedby following the fate of the sulfur supplied to the sulfur-deficientcells using ³⁵S as a tracer.
2. The sulfur-deficient cells whichwere unable to perform celldivision were made capable of divisionby the provision of ³⁶S-labeledsulfate under non-photosynthesizingconditions. Soon after theprovision of sulfate the labeledsulfur went rapidly into thecold perchloric acid (PCA)-solublefraction of algal cells,almost entirely in the form of sulfateand/or some other inorganicsulfur substance (s). With the lapseof time, more or less remarkablechanges occurred in the patternof ³⁵S-distribution in differentfractions of cell material.It was noticed that, at the onsetof cell division, a sulfur-containingpeptide-nucleotide compound(s)(SPN), which has been reportedearlier, appeared in a largequantity in the cold PCA-solublefraction, and that its quantitydecreased gradually during thesubsequent process of cell division,suggesting that the compoundwas transformed into some othersubstance (s), presumably withits nucleotide moiety going intonucleic acids and the peptidemoiety going into some essentialproteins.
3. Another noteworthyphenomenon observed during the process ofcell division wasthe incorporation of ³⁶S in a group of hotPCA-soluble substances.These sulfur substances were revealedto be sulfur-containingnucleotidic compounds, which might possiblybe some essentialcomponents of, or substances in close relationto, deoxypentosenucleic acid (DNA).

(Received March 1, 1960; )     

MICRURGICAL STUDIES IN CELL PHYSIOLOGY : IV. COLORIMETRIC DETERMINATION OF THE NUCLEAR AND CYTOPLASMIC pH IN THE STARFISH EGG.

I. Cytoplasm. 1. The normal cytoplasmic pH, colorimetrically determined, of the starfish eggs in the unfertilized, fertilized, and first and second cleavage stages is 6.7 ± 0.1. 2. Cytolysis lowers the pH to a value 5.5 ± 0.1. 3. The cytolyzed material in time assumes the pH of its environing sea water. 4. The acid due to mechanical injury can also be detected in the environment of the egg. 5. Injury to the cytoplasm unaccompanied by visible disintegration causes an increase in acidity which is quickly neutralized. II. Germinal Vesicle. 6. The intranuclear pH, colorimetrically determined, of the immature Asterias egg is 7.5 ± 0.1. 7. Injury to the nucleus does not change its pH. 8. The spherical nuclear remnant which persists after injury gradually assumes the pH of its environment. III. Plasmalemma. 9. A dye to which the cell is normally impermeable can penetrate through a tear in the surface from an environment more acid than normal. This may be due to a difference in the formation of the plasmalemma in a normal and an acid medium.     

WATER RELATIONS IN THE CELL : I. THE CHLOROPLASTS OF NITELLA AND OF SPIROGYRA

Chloroplasts may contract under natural conditions and give up water to the rest of the cell, thus indicating changes in metabolism or constitution. Such contractions may be produced experimentally. In Nitella the chloroplasts are ellipsoid bodies which, under natural conditions, may contract to spheres with a loss of volume. This may be brought about by lead acetate, ferric chloride, and digitonin: the contraction may occur while the cell is alive. The contraction in lead acetate is reversible (in lead nitrate little or no contraction occurs). In Spirogyra the chloroplast is a long, spirally coiled ribbon which may contract under natural conditions to a short nearly straight rod with a loss of volume. This can be brought about by inorganic salts and in other ways while the cell is still alive.     

PHOTOCONTROL OF THE ORIENTATION OF CELL DIVISION IN ADIANTUM. I. EFFECTS OF THE DARK AND RED PERIODS IN THE APICAL CELL OF GAMETOPHYTES

When protonemata of Adiantum capillus-veneris L. which had been grown filamentously under continuous red light were transferred to continuous white light, the apical cell divided transversely twice, but the 3rd division was longitudinal. An intervening period of darkness lasting from 0 to 90 hr either between the 1st and the 2nd cell division or between the 2nd and the 3rd one did not affect the number of protonemata in which the 3rd cell division was longitudinal. The insertion of red light instead of darkness greatly decreased the percentage of 1st longitudinal divisions occurring at the 3rd division, and increased the number of transverse divisions. Fifty percent reduction of induction of 1st longitudinal division was caused by ca. 50 hr exposure to red light between 1st and 2nd division and by ca. 20 hr between 2nd and 3rd division, and total loss was induced by an exposure of ca. 100 hr or longer to red light in the former and by ca. 40 hr longer in the latter. Thus, by using an appropriate intervening dark period or exposure to red light, the orientation and timing of cell division could be controlled in apical cell of the fern protonemata.     

THE THEORY OF DIFFUSION IN CELL MODELS : II. SOLUTION OF THE STEADY STATE FOR THREE DIFFUSING SUBSTANCES

The differential equations describing diffusion in cell models have been extended to include the simultaneous penetration of water and two salts. These equations have been solved for the steady state. Values for the concentrations in the steady state which may be computed from the equations compare favorably with the experimental values obtained by Osterhout, Kamerling, and Stanley. Moreover, it has been shown elsewhere that the solution for the steady state is essential to a discussion of the volume change or "growth" of phase C in the models and, by analogy, in living cells.     

THE ROLE OF ANTIBIOTICS IN THE DECOMPOSITION OF SAWDUST: I. INHIBITION OF THE GROWTH OF CELLULOSE-DECOMPOSING BACTERIA

It has been shown that 'deal' sawdust contains substances which inhibit the growth of cellulose-decomposing bacteria of the genera Sporocytophaga and Cellulomonas , the former being the more sensitive. The substances can be extracted with water or a mildly alkaline solution of inorganic salts, the latter being rather more effective. The extracted material is acidic but still exhibits activity even after neutralization, especially towards Sporocytophaga. Sawdust which has been extracted with water or the alkaline solution, or neutralized by admixture with calcium carbonate, no longer prevents the growth of Cellulomonas on added filter paper cellulose, although there is a delay before the attack becomes evident, but Sporocytophaga is still completely inhibited under all three conditions.     

MICROTUBULE BIOGENESIS AND CELL SHAPE IN OCHROMONAS : I. The Distribution of Cytoplasmic and Mitotic Microtubules

In the first of two companion papers which attempt to correlate microtubules and their nucleating sites with developmental and cell division patterns in the unicellular flagellate, Ochromonas, the distribution of cytoplasmic and mitotic microtubules and various kinetosome-related fibers are detailed. Of the five kinetosome-related fibers, which have been found in Ochromonas, two, the kineto-beak fibers and the rhizoplast fibers are utilized as attachment sites for distinct groups of microtubules. The set of microtubules attached to the kineto-beak fibers apparently shape the anterior beak region of the cell whereas the rhizoplast microtubules appear to extend into and shape the tail in vegetative cells. In mitotic cells a rhizoplast is found at each spindle pole apparently serving as foci for the spindle microtubules. These findings are discussed in relation to the less well defined attachment sites for vegetative and mitotic microtubules in other kinds of cells. It is noted that the effects of depolymerizing microtubules in vivo might be easily quantitated in whole populations since no external wall or pellicle contributes to the maintenance or the biogenesis of the characteristic cell form of Ochromonas.     

MICROTUBULES IN THE FORMATION AND DEVELOPMENT OF THE PRIMARY MESENCHYME IN ARBACIA PUNCTULATA : I. The Distribution of Microtubules

Prior to gastrulation, the microtubules in the presumptive primary mesenchyme cells appear to diverge from points (satellites) in close association with the basal body of the cilium; from here most of the microtubules extend basally down the lateral margins of the cell. As these cells begin their migration into the blastocoel, they lose their cilia and adopt a spherical form. At the center of these newly formed mesenchyme cells is a centriole on which the microtubules directly converge and from which they radiate in all directions. Later these same cells develop slender pseudopodia containing large numbers of microtubules; the pseudopodia come into contact and fuse to form a "cable" of cytoplasm. Microtubules are now distributed parallel to the long axis of the cable and parallel to the stalks which connect the cell bodies of the mesenchyme cells to the cable. Microtubules are no longer connected to the centrioles in the cell bodies. On the basis of these observations we suggest that microtubules are a morphological expression of a framework which opeartes to shape cells. Since at each stage in the developmental sequence microtubules appear to originate (or insert) on different sites in the cytoplasm, the possibility is discussed that these sites may ultimately control the distribution of the microtubules and thus the developmental sequence of form changes.     

CELL KINETICS IN THE SEBACEOUS GLANDS OF THE MOUSE. I. THE GLANDS IN RESTING SKIN

Cell proliferation, differentiation and migration have been studied in the sebaceous glands of DBA-2 mice in the resting (telogen) phase of hair growth. Cells labelled by a single injection of tritiated thymidine start to leave the glands of adult male mice 5 days later. About 80% of the proliferative cells in the basal layer have a cell cycle time of 40 hr or less. In 18% of the proliferative cells G₁ is at least 4 days long and 16% have a G₂ phase longer than 17 hr. The S phase is about 7.5 hr long and cells spend at least 21 hr in the basal layer before migrating into the differentiating cell region. The glands of mature female and immature mice are smaller than those of the mature male. They have fewer, smaller cells and a much lower labelling index.     

ROLE OF SULFUR IN THE CELL DIVISION OF CHLORELLA, WITH SPECIAL REFERENCE TO THE SULFUR COMPOUNDS APPEARING DURING THE PROCESS OF CELL DIVISION II.

1. Chlorella cells, which had been grown synchronously undersulfur-deficient conditions and thus rendered unable to performcell division, were made capable of nuclear and cellular divisionby being supplied with ³⁵S-labeled sulfate and nitrate underphotosynthesizing conditions, and the fate of sulfur duringthese recovery processes was followed. 2. When the S-starved cells were provided with sulfate aloneunder photosynthesizing conditions, cells grew appreciably inmass performing nuclear division but remaining incapable ofcellular division. During these processes most of the ³⁵S wasfound to be incorporated into the protein fraction of algalcells. 3. When the cells which had been stalemated at the above-mentionedstage were supplied with nitrate, they grew further in massand eventually performed cellular division. During this periodthe ³⁵S was found to be distributed not only in the proteinfraction, but also in an appreciable amount in the cold andhot acid-soluble fractions. 4. By paper-electrophoretic experiments it was found that thenature of the sulfur substances appearing in the hot acid-solublefraction changed strikingly during the process of cellular division.Zone electrophoresis and an anion-exchange chromatography ofthese substance isolated from the cells at the completion ofcellular division, disclosed that they were most probably deoxypentosepolynucleotides containing sulfur in some form yet unidentified. 5. It was demonstrated that there exist some antagonistic relationsbetween the protein synthesis and the formation of these sulfur-containingdeoxypentose polynucleotides, and that the former predominatesunder photosynthesizing conditions while the latter outweighsunder nonphotosynthesizing conditions. (Received August 9, 1960; )     

STRUCTURE AND DEVELOPMENT OF THE CHLOROPLAST IN CHLAMYDOMONAS : I. THE NORMAL GREEN CELL

The cytoplasmic organization of a normal green strain of the alga Chlamydomonas reinhardi has been investigated with the electron microscope using thin sections of OsO₄ fixed material. The detailed organization of the chloroplast has been of special interest. The chloroplast, a cup-shaped organelle, surrounded by a double membrane, consists of: (1) discs about 1 micron in diameter, considered to represent the basic structural unit of the chloroplast, and each composed of a pair of membranes joined at their ends to form a flat closed vesicle; the discs are grouped into stacks resembling the grana of higher plants; (2) matrix material of low density in which the discs are embedded; (3) starch grains; (4) the pyrenoid, a non-lamellar region associated with starch synthesis, and containing tubules which connect with the lamellae; (5) the eyespot, a differentiated region containing two or three plates of hexagonally packed, carotenoid-containing granules, located between discs, and associated with phototaxis. In addition to the chloroplast, the cytoplasm contains various membranous and granular components, including mitochondria, endoplasmic reticulum, and dictyosomes, identified on the basis of morphological comparability with structures seen in animal cells. The nucleus, not investigated in detail in this study, contains a large, granular nucleolus and is surrounded by a nuclear envelope which is provided with pores and exhibits instances of continuity with the endoplasmic reticulum of the cytoplasm.     

THE ROLE OF LIGHT IN HISTOGENESIS AND DIFFERENTIATION IN THE SHOOT OF PISUM SATIVUM. I. THE APICAL REGION

Thomson , B. F., and P. M. Miller . (Connecticut Coll., New London.) The role of light in histogenesis and differentiation in the shoot of Pisum sativum. I. The apical region. Amer. Jour. Bot. 49(3): 303–310. Illus. 1962.—Seedlings of Pisum sativum grown under constant conditions and kept in total darkness or exposed daily to red or white light were harvested at the same plastochron age and examined histologically to determine what specific aspects of histogenesis and differentiation are affected by light. The tissue organization of the shoot apex is the same in all light conditions to a point below the 2 youngest leaf primordia. The first detectable difference is a slight thickening of the internode in light due to more and larger cells. The first effect on longitudinal growth appears below the fourth youngest primordium and consists of an increase of internode length in light-grown plants. This is associated with a greater distance between the apex and the first mature protoxylem. The distance from apex to the first pith, provascular strands, and protophloem and the distances between the 4 youngest leaf primordia are not affected by light.     

FINE STRUCTURE OF CELL DIVISION IN CHLAMYDOMONAS REINHARDI : Basal Bodies and Microtubules

Cell division in log-phase cultures of the unicellular, biflagellate alga, Chlamydomonas reinhardi, has been studied with the electron microscope. The two basal bodies of the cell replicate prior to cytokinesis; stages in basal body formation are presented. At the time of cell division, the original basal bodies detach from the flagella, and the four basal bodies appear to be involved in the orientation of the plane of the cleavage furrow. Four sets of microtubules participate in cell division. Spindle microtubules are involved in a mitosis that is marked by the presence of an intact nuclear envelope. A band of microtubules arcs over the mitotic nucleus, indicating the future cleavage plane. A third set of microtubules appears between the daughter nuclei at telophase, and microtubules comprising the "cleavage apparatus" radiate from the basal bodies and extend along both sides of the cleavage furrow during cytokinesis. Features of cell division in C. reinhardi are discussed and related to cell division in other organisms. It is proposed that microtubules participate in the formation of the cleavage furrow in C. reinhardi.     

THE ULTRASTRUCTURE OF PHYCOPELTIS (CHROOLEPIDACEAE: CHLOROPHYTA). I. SPOROPOLLENIN IN THE CELL WALLS

Electron microscope observations on Phycopeltis epiphyton, a subaerial green alga found growing on the leaves of vascular plants and bryophytes, revealed the presence of a densely staining material within the inner and outer zones of the cell walls. This material resists acetolysis, is degraded by chromic acid, is unaffected by ethanolamine and exhibits secondary fluorescence when stained with the fluorochrome Primuline. These characteristics, together with infrared absorption spectra indicate that, on the basis of currently accepted criteria, the densely staining material is a sporopollenin and that it is a major component of the cell wall. Tests for cellulose, chitin, and lignin were negative, and little if any silica is present. It is suggested that negative results in tests for cellulose may be due to a masking effect by the sporopollenin. Comparison of the fine structure of the cell walls of P. epiphyton, pollen grains, and algal cells (known to contain sporopollenin) supports the suggestion that sporopollenin deposition on “unit membranes” is universal. Morphological similarity among sporopollenin lamellae in P. epiphyton, pollen grains, spores of land plants, and the trilaminar sporopollenin sheath in Chlorella, Scenedesmus, and Pediastrum indicates that the structures may be analogous. As in pollen grains, sporopollenin may provide protection against desiccation and parasitism. It may also be involved in the adhesion of Phycopeltis to host plants and in the adhesion between adjacent filaments of the thallus.     

CHANGES IN THE STABILITY AND POTENTIAL OF CELL SUSPENSIONS : I. THE STABILITY AND POTENTIAL OF BACTERIUM COLI.

1. Stability and potential of Bacterium coli suspensions depend, not only on the strain of the organism and the medium in which it is suspended, but also on the previous treatment of the suspension, and the length of time it has been in the medium. 2. When treated at acid reactions, the negative charge on the bacteria is diminished; with some strains, a positive charge is acquired. Changes in stability accompany the changes in potential. 3. Washing acid-treated bacteria at neutral or slightly alkaline reactions does not restore the original potential; the zone of flocculation is moved toward the alkaline side. 4. These changes are due to two factors: the extraction of a soluble protein which combines with the surfaces of the cells, and a further irreversible change of the cell or its membrane.     

THE POSSIBLE ROLE OF A FIBROUS BODY IN THE GENERATIVE CELL OF THE POLLEN GRAIN OF TILLANDSIA CAPUT-MEDUSAE MORR. (BROMELIACEAE)

The occurrence of a fibrous body in the generative cell of the pollen grain of Tillandsia caputmedusae Morr. (Bromeliaceae) is pointed out and its possible role is indicated.