Chromatin elimination in the hypotrichous ciliate Stylonychia mytilus

Chromatin elimination in the hypotrichous ciliate Stylonychia mytilus was studied by means of electron microscopy using a microspreading procedure. In the polytene chromosomes of the macronuclear anlagen three organization patterns are observed: Bands of various size composed of 300 Å chromatin fibers, large blocks of 300 Å nucleofilaments which probably represent the heterochromatic regions of the chromosome and axial 120 Å filaments. Those DNA sequences which become eliminated belong to the 300 Å fiber type. The eliminated chromatin occurs in the form of rings of variable size corresponding to a DNA content between 18 and 160 Kb while the axial 120 Å filaments appear to be preserved.     

Phytoferritin in plastids of the cambial zone of willow

Summary Crystalline and paracrystalline arrays of electron-opaque granules have been found in plastids of the cambial zone and its immediate derivatives in crack willow (Salix fragilis L.). These granules have a diameter of 55 to 70 Å and, when in crystalline arrangement, show a centre to centre spacing of 100 Å with adjacent, slightly curved, or linear rows running parallel. The 70 Å particles have a substructure of four to six subunits 15 Å in diameter. These units are arranged around an electron-translucent core 20 Å diameter. It is suggested that this complex is phytoferritin. It is assumed that the electron-translucent area around the opaque granules represents the proteinaceous shell characteristic of both plant and animal ferritin as described by other authors. The phytoferritin is commonly found spread in a thin, regular, array over the surface of plastoglobuli in the plastids.It is further suggested that the phytoferritin is an iron-protein complex which allows the plant to store iron in non-toxic form. This theory would be in accord with the presence of phytoferritin in plastids which appear to be morphologically mature but which, on account of their position within the stem, would not be expected to be photosynthetically very active.     

Nucleotide sequences and unusual electrophoretic behavior of the W chromosome-specific repeating DNA units of the domestic fowl,Gallus gallus domesticus

Nucleotide sequences of three independently cloned repeating units of the W chromosome-specific repettive DNA sequences (XhoI family) of the chicken were determined. All three units are 717 bp long with XhoI sites at both ends. There are only 21 sites out of 717 bases where a single base change occurs in one of the three clones. Each of these repeating units consists of 34 tandem repeats of about 21 bp. Sequences of some members of these internal repeats are not well conserved, but the majority of the repeats are characterized by the presence of (A)_3–5 and (T)_3–5 clusters separated by 6–7 relatively G+C-rich base pairs. One striking feature of the cloned 717 bp repeating units is that they migrate unusually slowly on electrophoresis in polyacrylamide gels. The same feature is also shown by a genomic population of the 0.7 kb repeating units recovered from XhoI digests of the genomic DNA of the female chicken. This anomalous behavior is attributed to the occurrence of DNA curvatures because of the above sequence characteristics and partial recovery of the electrophoretic mobility in the presence of distamycin A. Another feature of the 717 bp repeating unit is the presence of 438 and 159 nucleotide-long open reading frames (ORFs) at each end of the unit. A possible function of the XhoI family sequences in the heterochromatization of the W chromosome and the significance of the ORFs are discussed.     

Electron microscopical observations on the brush border of proximal tubule cells of mammalian kidney

Summary The ultrastructure of the plasma membrane and the core of microvilli of proximal tubule cells has been investigated by electron microscopy using sectioned and negatively stained material. By the technique of negative staining, a particulated coat is disclosed on the outside of the plasma membrane of microvilli of brush borders isolated from rat, rabbit and ox. This coat is composed of 30 to 60 Å particles and is 150 to 300 Å thick and appears to be a distinguishing feature for the luminal plasma membrane (brush border) of proximal tubule cells. The plasma membrane of the basal part of tubule cells is found to be smooth. By thin sectioning, an axial bundle of 50 to 70 Å diameter filaments regularly arranged in an 1+6 configuration, one axially located filament being surrounded by a ring of six, is disclosed. The distance from the ring of filaments to the inner surface of the plasma membrane is 250–300 Å, the diameter of the ring 300 Å and the center-to-center distance between filaments 120 Å. Negative staining also discloses 60 Å filaments in microvilli of isolated brush borders. Broken off, single microvilli (fingerstalls) are observed with thin filaments projecting from their broken ends. Filaments up to 1 in length are seen. At high magnification, the filaments appear beaded and show strong resemblance with actin filaments isolated from skeletal muscle. Based on present evidence, it is postulated that microvilli constituting renal brush borders possess contractile properties, which may play a role in the absorption process operating at the luminal part of the cells.The authors are indebted to Miss Kirsten Sjöberg for skilled technical assistance, and to the Danish State Research Foundation and the Tuborg Foundation for financial support.     

A stereologic electron microscope study of “tubular myelin figures” in alveolar fluids of rat lungs

Summary The three-dimensional structure of a composite material found in alveolar exudate of oxygen poisoned lungs but also present in normal lungs is stereologically analysed. It is composed of tubules of 450 Å diameter which are tightly packed in a quadratic lattice. The wall of the tub vile is formed by four-winged osmiophilic filaments which are located in the corners of the quadratic lattice; their interior is made up of a hydrophilic substance which contains either a tubule or a filament of moderate electron density. The osmiophilic substance of the walls is continuous with associated myelin figures which can be resolved into lamellae with a periodicity of 42 Å and can thus be considered to be water crystals of phospholipids. The nature of the content of the tubules, which presumably exerts the formative force on the phospholipid lamellae to form tubules, remains undetermined.Dedicated to Prof. W. Bargmann in honor of his 60th birthday.The research reported here has been sponsored by the Schweizerischer Nationalfonds zur Förderung der wissenschaftlichen Forschung (Nr. 2569); by the Stiftung für wissenschaftliche Forschung an der Universität Zürich; by the National Institutes of Health, USPHS, through grant RF-57; and the 6570th Aerospace Medical Research Laboratories under contract AF 61(052)-784 through the European Office of Aerospace Research (OAR), United States Air Force.     

A tridentate bis(pyrazolyl) ligand binds to Cu(II), without using the pyrazole group: a very unusual coordination mode of the ligand Hbdmpb, 1,3-bis(3,5-dimethylpyrazol-1-yl)-2-butanoic acid

A new pyrazole-based ligand, namely 1,3-bis(3,5-dimethylpyrazol-1-yl)-2-butanoic acid (Hbdmpb) was synthesised together with its copper complex Na[Cu(bdmpb)₂(OOCCH₃)H₂O] · 4H₂O. Both the free ligand and its Cu compound were fully characterised and their crystal structures were determined by X-ray analysis. The free-ligand molecular structure is uneventful. The Cu compound is highly unusual, as the pyrazole nitrogen atoms do not bind to the Cu ion. The copper(II) ion is coordinated by four nearly coplanar oxygen atoms from two dehydronated ligands bdmpb (CuO(1a) 1.942(4), CuO(1b) 1.933(4) Å), a monodentate acetate group (CuO(1) 1.927(3) Å) and a water molecule (CuO(1w) 1.937(4) Å). The nitrogen atoms of the pyrazole rings do not coordinate to the metal center, but instead are involved in strong intramolecular hydrogen bonds. The coordinated water molecule is strongly H-bonded to two pyrazole N atoms from two bdmpb ligands (N(12a) ? HO(1w) 2.762(7), N(12b) ? HO(1w) 2.774(7) Å). The other two pyrazole N atoms with a lone pair are hydrogen-bonded to water molecules in the lattice (N(22a) ? HO(2w) 2.763(7), N(22b) ? HO(6w) 2.892(7) Å). The sodium ion is six-coordinated by the oxygen atom O(2) of the acetato ligand and by five water molecules. The EPR spectrum recorded in the solid state shows a characteristic signal for an axial anisotropic S = 1/2 species. The spectrum recorded in methanol glass confirms the absence of the coordination of pyrazole nitrogen atoms to the copper centers.     

Formation of siliceous spicules in the marine demosponge <Emphasis Type="Italic">Suberites domuncula</Emphasis>

The siliceous skeleton of demosponges is constructed of spicules. We have studied the formation of spicules in primmorphs from Suberites domuncula. Scanning electron microscopy and transmission electron-microscopical (TEM) analyses have revealed, in the center of the spicules, an axial canal that is 0.3–1.6 m wide and filled with an axial filament. This filament is composed of the enzyme silicatein, which synthesizes the spicules. TEM analysis has shown that spicule formation starts intracellularly and ends extracellularly in the mesohyl. At the initial stage, the axial canal is composed only of silicatein, whereas membranous structures and fibrils (10–15 nm in width) can later also be identified, suggesting that intracellular components protrude into the axial canal. Antibodies against silicatein have been applied for Western blotting; intracellularly, silicatein is processed to the mature form (24 kDa), whereas the pro-enzyme with the propeptide (33 kDa) is detected extracellularly. Silicatein undergoes phosphorylation at five sites. Immunohistological analysis has shown that silicatein exists in the axial canal (axial filament) and on the surface of the spicules, suggesting that they grow by apposition. Finally, we have demonstrated that the enzymic reaction of silicatein is inhibited by anti-silicatein antibodies. These data provide, for the first time, a comprehensive outline of spicule formation.This work was supported by grants from the European Commission (SILIBIOTEC), the Deutsche Forschungsgemeinschaft, the Bundesministerium für Bildung und Forschung Germany (project: Center of Excellence BIOTECmarin) and the International Human Frontier Science Program.     

The fine structure of the pellicle ofEuglena gracilis as revealed by freeze-etching

Summary The ultrastructure of the pellicle ofEuglena gracilis (Klebs) Z strain was studied using the freeze-etching technique and the results were correlated with data obtained from thin sections of fixed material.Examination of freeze-etched pellicles reveals an outer particulate layer and an inner striated layer. The particles of the outer layer measure approximately 150 Å in diameter. The striations of the inner layer are about 50 Å wide and are separated from each other by about 35 Å. A broad repeating pattern is also visible with a periodicity of about 450 Å. When deep etching is employed, a smooth outer layer is seen covering the particulate layer. This is probably the outer surface of the plasma membrane. Mucilage is present on the outer surface of the cell and is seen as a substructure of threads superposed on the smooth layer of plasma membrane.Thin sectioning also shows a striated layer interior to the plasma membrane. This appears to be identical to the striated layer seen after freeze-etching.     

Long link induction between the microtubules of the manchette in intermediate stages of spermiogenesis

Summary Links unusual for their length and variable morphology have been described between manchette microtubules in late stages of rat spermiogenesis. In earlier stages of rat spermiogenesis obvious links longer than 160 Å are rare, the majority being 80 or 120 Å in length. The most easily discernible geometric pattern in cross-sections of assemblies of manchette microtubules in intermediate stages of rat spermiogenesis is that of linear arrays sometimes resulting in long and irregularly folded chains of closely linked microtubules. Colcemid disrupts these arrays and is responsible for the formation of more complex geometric patterns. Six hours after drug administration the manchette is dramatically reduced in length. Sheet-like links of variable dimensions and >160 Å in length interconnect not only microtubules but C-type microtubules as well as other links. These links are similar in morphology to those found in later stages of rat spermiogenesis. It is suggested that the formation of these links may perhaps be dependent upon aspects of microtubule disassembly.Supported by a grant to E. A. MacKinnon by the Medical Research Council of Canada.     

Conformation of the high molecular weight form ofDunaliella salina phosphofructokinase in solution by means of small-angle X-ray diffraction and viscosity measurements

Summary The intrinsic viscosity of phosphofructokinase fromDunaliella salina in different states of aggregation was determined. The instrinsic viscosity [], of the biologically active tetramer, with a molecular weight of 320,000, was found to be 6.5 ml·g^–1 at 4°C. Moreover, for the inactive dimer, with a molecular weight of 160,000, a value of []=8.0 ml·g^–1 was determined. The high molecular weight aggregate of phosphofructokinase fromDunaliella salina, that shows little activity, has an intrinsic viscosity of 23.2 ml·g^–1, which is significantly higher than that found for the active tetramer and the inactive dimer.Small angle X-ray scattering experiments in solution of this high molecular from of phosphofructokinase fromDunaliella salina reveal a radius of gyration of the cross section ofR _c=49.0 Å at an ionic strength of 0.15 M and_pH 7.2. Furthermore, a comparison of the values obtained for the tetramer and the radius of gyration (R _g=52.9 Å) with those of typical spherical proteins (3–4 ml·g^–1) shows that the values of [] andR _g are significantly larger for the high molecular weight form of phosphofructokinase than for the spherical proteins. The high intrinsic viscosity of the polymeric form of phosphofructokinase suggests an end-to-end aggregation consisting of monomeric units with heights,h=80–90 Å, and a cylindrical diameter of approximately 140.0 Å, resulting in a long rod of a total length of 1,800 Å and a molecular weight of two million. On the basis of the experimentally observedR _c and [] values, using a prolate ellipsoid of revolution as a model, the hydrodynamic volume and the hydration, the axial ratio could be determined to be 12. The native tetrameric form contains 0.4 g H₂O/g protein, whereas the higher aggregate structure corresponds to a hydration of 0.60 g H₂O/g protein.     

Structures from powders: Diflorasone diacetate

Diflorasone diacetate, a steroid anti-inflammatory drug (marketed as Diacort^® or Florone^® by Pfizer) and used in the treatment of skin disorders, can be prepared as anhydrous form, DD1 (as deposited in the US pharmacopoeia), or as a monohydrated phase, DDW. Heating the DDW form above 90 °C, a mixture of DD1 and of a new anhydrous polymorph, DD2 is obtained. Further heating of this mixture, or of pure DD1, up to 230 °C (only a few degrees before melting!), generates an elusive anhydrous DD3 polymorph. Their crystal structures, determined uniquely from laboratory powder diffraction data, show the isomorphous character of the DDW and DD1 forms, while the DD2 and DD3 polymorphs crystallize with markedly different unit cells. Crystals of the DD1, DD2 and DDW forms are orthorhombic, P2₁2₁2₁, a = 29.386(1) Å; b = 10.4310(9) Å, c = 8.1422(7) Å, V = 2495.8(3) Å³ for DD1; a = 15.2639(10) Å; b = 11.7506(7) Å, c = 13.8931(11) Å, V = 2491.9(3) Å³ for DD2; a = 30.311(2) Å; b = 10.6150(9) Å, c = 7.9337(7) Å, V = 2552.7(4) Å³ for DDW; while the lattice parameters for the monoclinic P2₁DD3 species are a = 11.5276(10) Å; b = 13.8135(11) Å, c = 7.8973(7) Å, β = 103.053(6)°, V = 1225.0(2) Å³. These compounds have also been fully characterized by thermo analytical methods, as well by ¹³C, ¹⁹F, and ¹H NMR spectroscopy.     

Ultrastructure of the eosinophil granule-internum; the problem of reversed relative density

Summary An electron microscope study was made of the specific granules of eosinophil leucocytes in mouse bone marrow. A crystal lattice was apparent in the granule-internum, with a repeating pattern of about 30 Å. The presence of this lattice in stained material in which the usual densities of internum and externum were reversed is taken as supporting the hypothesis that the reversal is a negative staining effect. Very occasionally a myelin-like inclusion was also seen in eosinophil granules.     

Fine structure ofPenicillium megasporum conidiospores

Summary An investigation was conducted on the fine structure ofP. megasporum conidiospores using both chemical fixation and the freeze-etching techniques. The spore cell wall was shown to consist of several layers, one of which is chiefly fibrillar in nature. The surface of the spore appears to be covered by ordered arrays of rodlets which are embedded in or resting upon a thin layer of homogenous material. At higher magnification, these rodlets appear as linear arrays of particles approximately 50 Å in diameter. This layer may be of a cutaneous nature. In addition, the plasma membrane was shown to be covered by particles, some of which appear to migrate to the inner layer of the cell wall. Numerous invaginations of the plasma membrane were also seen.On leave of absence from the Department of Botany, University Nijmegen, Holland.On leave of absence from the Department of Botany, Brigham Young University, Provo, Utah.     

Ultrastructure of spermatozoa of Peregrinus maidis (Homoptera,Delphacidae)

Summary The spermatozoa of Peregrinus maidis Ashm. are thread-like, approximately 650 long and 1 wide including the head (approximately 28 ).The main part of the spermatozoa consists of two mitochondria derivatives, a central body between them, the axial filament complex, and a newly found element consisting of two wing-shaped bodies. Each mitochondrion derivative shows a peripheral and an inner part. The peripheral part is formed by cristae arranged perpendicularly to the long axis of the spermatozoon. The cristae are approximately 70 Å wide. The dense layers between them measure approximately 280 Å. The inner part of the mitochondrion derivative shows a crystalline array, formed by sub-units of approximately 100 Å diameter. The wing-shaped bodies consist of tubular elements.The head has an elongated nucleus with an electron transparent space inside. At the anterior end of the nucleus lies a tapered acrosome. This appears fibrous and parts of the acrosome fibers seem to run along the nucleus. Acknowledgements. The authors wish to thank Dr. G. H. Bergold for suggestions and support, Drs. J. André, D. W. Fawcett, P. Maillet and G. F. Meyer for very helpful discussion. They are also grateful to Mr. O. Suárez for assistance in the preparation of the organs of P. maidis and to Mrs. M. de Pingarrón for technical assistance.     

The fine structure of the kinetochore of a mammalian cell in vitro

The chromosomes of Chinese hamster cells were examined with the electron microscope and the following observations were made concerning the structure and organization of the kinetochore. — The kinetochore consists of a dense core 200–300 Å in diameter surrounded hy a less dense zone 200–600 Å wide. The dense core consists of a pair of axial fibrils 50–80 Å in diameter which may be coiled together in a cohelical manner. The less dense zone about the axial elements is composed of numerous microfibrils which loop out at right angles to the axial fibrils. Together the structures comprise a lampbrush-like filament which extends along the surface of each chromatid. Some sections suggested that two such filaments may be present on each chromatid. The fine structure of kinetochores associated with spindle filaments was essentially the same as those free of filaments. The structure and organization of the kinetochore of these mammalian cells was compared to that of lampbrush chromosomes of certain amphibian oöcytes, dipteran polytene chromosome puffs, and the synaptinemal complex seen during meiotic prophase.The authors also wish to thank Dr. Arthur Cole of the Department of Physics for the use of his electron microscope facilities and for his helpful criticism.     

Structure of actin paracrystals induced by nerve growth factor

When nerve growth factor is added to F-actin, well-ordered bundles of filaments are formed. These bundles are observed even at low concentrations of NGF²¹, but when N-bromosuccinimide-treated NGF, a biologically inactive form of the protein is used, a much higher concentration is required to produce aggregation. Moreover, the bundles induced by the modified NGF are not very well ordered and show amorphous aggregates attached at various points.Electron microscopy of paracrystals induced by native NGF shows that, although they resemble pure actin paracrystals induced by Mg²⁺, the interfilament spacing is larger and bridges connect the filaments. Optical diffraction patterns show, in addition to the off-meridional reflections characteristic of the actin helix, meridional reflections on the first and fourth layer-lines, at axial spacings of 37 and 9 nm. Measurements of the axial positions of the layer-lines show that the actin helical symmetry is not significantly different from that in pure actin paracrystals. The presence of the meridional reflections indicates that groups of two or three bridges with spacing 9 nm or nearly 9 nm are arranged along the bundles at a repeating interval of 37 nm.Actin filament bundles have been observed in several non-muscle cells, and specific actin-binding proteins have been identified as responsible for this aggregation. Our in vitro observations show that the biologically active form of NGF interacts with actin and organizes it into well-ordered paracrystalline arrays. The in vitro formation of NGF-actin complexes may be related to the in vivo mechanism of action of this growth factor.     

Nerve-purkinje fiber relationship in the moderator band of bovine and caprine heart

Summary The moderator band in the heart of the ox and goat contains bundles of Purkinje fibers and nerve fibers separated by connective tissue. The axons are mostly unmyelinated and embedded in the cytoplasm of Schwann cells.Small bundles of axons run close to the Purkinje fibers. The axons dilate into varicosities 0.5 to 1.6 in diameter (mean 0.95 ), containing three types of vesicles: 1) agranular vesicles with a diameter of 400–500 Å, 2) large dense-cored vesicles with a diameter of 800–1200 Å, 3) small dense-cored vesicles with a diameter of 500 Å. Most varicosities contain agranular vesicles together with a few large dense-cored vesicles.The gap between the varicosities and the nearest Purkinje fiber is unusually wide and normally varies between 0.3 and 0.8 . No intimate nerve-Purkinje fiber contacts, with a cleft of 200 Å, were observed.     

Structural aspects of amitosis: a light and electron microscope study of the isolated macronuclei of Paramecium aurelia and Tetrahymena pyriformis

Thin sections show the macronuclei of Paramecium aurelia and Tetrahymena pyriformis to contain two types of bodies. The smaller, measuring 0.1–0.2 in diameter, have been resolved in the light microscope by first removing the macronuclei from the cells in the presence of Mg⁺⁺, then chelating that divalent cation with EDTA, resulting in expansion of the nuclear material. By staining with methyl green, Azure B, and the Feulgen procedure, the small bodies were shown to contain DNA. In whole mounts these small bodies appear to be joined to one another producing a complex network suspended in which are the larger bodies, or nucleoli. — Macronuclei from both ciliates were isolated in large quantities and purified for spreading on an air-water interface. When the nuclei burst from surface tension forces and are examined with the electron microscope, the DNA containing bodies remain attached to one another by means of 100 Å fibrils. The pattern of attachment is non-linear. Occasionally individual DNA-containing bodies loosen revealing a coil resembling both in shape and dimensions the 250 Å coil characteristic of eucaryotic chromatin. The substructure of the 250 Å coil has not been directly observed. However, the frequent association of pairs of 100 Å fibrils makes it likely that two such fibrils are tightly complexed in the 250 Å coil. The 100 Å fibril, in turn, contains two 20 Å strands, each presumably a DNA double helix. — In Paramecium each small body of the macronucleus contains approximately one chromosome-equivalent of DNA. The fact that these small bodies are joined to form large structured masses of chromatin within the macronucleus indicates that the distribution of genetic material is not random. It is possible that, similar to bacteria, entire genomes segregate as units, thus accounting for successful amitotic division.This work was supported by a Predoctoral Fellowship to the author from the National Institutes of Health, U.S. Public Health Service, and by grant GM-13882 (NIH-USPHS) to Dr. Daniel Mazia.     

Aktomyosinartige Filamente im Teilungsmakronukleus des Ciliaten Ichthyophthirius Multifiliis

Just before nuclear division, the chromosomal elements within the large, highly polyploid macronucleus of I. multifiliis carry out rotational movements. Electron micrographs of cells fixed during the rotational movements show islets filled with microfilaments in various states of aggregation. Both thick (80–200 Å) and thin (30–80 Å) filaments occur, either as a highly dense network or as straight, in part parallel, filaments embedded in a filamentous network of lower density. Other islets of the macronucleus contain large and dense aggregates of filaments, sometimes with globular particles measuring 50–60 Å arranged along the thick filaments, occasionally forming cross-bridges with the thinner ones. — After incubation of the cells before fixation in a contractionsolution containing 0.002 M ATP, all nuclear islets show a nearly uniform appear ance of filamentous aggregates: numerous long and thick filaments are arranged in parallel with thin filaments with which they are in some parts connected by bridges. The probable myosinoid and actinoid nature of thick and thin filaments is discussed. It is suggested that the pre-divisional intranuclear rotational movement is a mechanism to avoid aneuploidy by producing a random arrangement of replicated hereditary units prior to division.