Regeneration of the active zone at the frog neuromuscular junction

The active zone is a unique specialization of the presynaptic membrane and is believed to be the site of transmitter release. The formation of the active zone and the relationship of this process to transmitter release were studied at reinnervated neuromuscular junctions in the frog. At different times after a nerve crush, the cutaneous pectoris muscles were examined with intracellular recording recording and freeze-fracture electron microscopy. The P face of a normal active zone typically consists of two double rows of particles lined up in a continuous segment located opposite a junctional fold. In the initial stage of reinnervation, clusters of large intramembrane particles surrounding membrane elevations appeared on the P face of nerve terminals. Like normal active zones, these clusters were aligned with junctional folds. Vesicle openings, which indicate transmitter release, were seen at these primitive active zones, even though intramembrane particles were not yet organized into the normal pattern of two double rows. The length of active zones at this stage was only approximately 15% of normal. During the secondary stage, every junction was reinnervated and most active zones had begun to organize into the normal pattern with normal orientation. Unlike normal, there were often two or more discontinuous short segments of active zone aligned with the same junctional fold. The total length of active zone per junctional fold increased to one-third of normal, mainly because of the greater number of segments. In the third stage, the number of active zone segments per junctional fold showed almost no change when compared with the secondary stage. However, individual segments elongated and increased the total length of all active zone segments per junctional fold to about two-thirds of the normal length. The dynamic process culminated in the final stage, during which elongating active zones appeared to join together and the number of active zone segments per junctional fold decreased to normal. Thus, in most regions, regeneration of the active zones was complete. These results suggest that the normal organization of two double rows is not necessary for the active zone to be functional. Furthermore, localization of regenerating active zones is related to junctional folds and/or their associated structures.     

Morphologic characteristics of intercellular junctions in early embryogenesis of mice

Dynamics concerning certain intercellular junctions have been followed during the preimplantation period of development in mouse embryos. The morphological analysis of the preimplantational embryos has demonstrated, that at the initial stages of cleavage (2-4 blastomeres) the cells make contacts by means of nonspecific junctions. Specialized intercellular junctions appear at the stage of 8 blastomeres and are presented as dotted tight and gap junctions. When the embryo is developing from the stage of 8 up to the stage of 16 blastomeres, certain connective complexes appear, consisting of dotted or cord-like tight and gap junctions. At the late morula stage, the external blastomeres in the apical part have contacts with each other by means of cingular tight junctions. In this place a connective complex might emerge; it is displayed as a tight junction and one or two gap junctions. At the blastocyst stage desmosomes and adhision zones appear. Between trophectodermal cells a connective complex arises; it is presented in the slice as a tight cingular junction, desmosomes (as a rule two) and an adhision zone. Between cells of the internal cellular mass the intercellular junctions are presented as dotted tight and gap junctions. Cells of the polar trophoectoderm and cells of the internal cellular mass could have contacts by means of gap and dotted tight junctions.     

Adenylate cyclase activity and cyclic AMP production in the outer and inner zones of the adrenal cortex

It has been reported that cells isolated from the inner zone of the guinea pig adrenal cortex fail to have a steroidogenic response to ACTH. To further explore this, adenylate cyclase activity of membrane particles and cAMP production by cells prepared from the inner and outer adrenocortical zones were determined. The cAMP response to ACTH and forskolin was similar for cells from both zones. Basal adenylate cyclase activity was significantly higher in the inner zone; and while absolute responses to ACTH, GppNHp, GTP, NaF, and forskolin were greater for the inner zone, relative responses were similar for the two zones. These observations suggest that the inner zone of the guinea pig adrenal cortex may have a defect in ACTH action at a step(s) beyond cAMP formation.     

Nuclear origin of the mitotic spindle in the oogenesis of Oligotrophus schmidti (Cecidomyiidae; Diptera)

In the oogenesis of the gall midge Oligotrophus schmidti, a material assumed to be precursor material of the first maturation division spindle appears in the middle area of the early diplotene nucleus in close association with the chromosomes. At the beginning of the growth stage of the oocyte this material together with the chromosomes is transported as a characteristic ring-shaped body toward the nuclear membrane. Having approached the nuclear membrane the ring material spreads all over its inner surface. Next, it differentiates into a continuous cortical layer of a non-chromosomal material and the chromosomal vesicles. The cortical layer, about 1, thick, is appressed tightly to the inner surface of the nuclear membrane, being delimited against the nuclear sap by a membrane-like boundary. At the end of diakinesis the chromosomes congregate in the middle area of the nucleus, and at the same time the spindle organizing activity of kinetochores begins. At the early stages of its development the spindle is a compound structure, consisting of a number of individual spindles, each of them being organized by a separate group of chromosomes. Changes in the structure of the cortical layer before and during prometaphase spindle formation are interpreted to indicate that the precursor material of the spindle is dissolved and diffuses into the nuclear sap. The nuclear membrane and the remnants of the cortical layer do not disappear until late prometaphase when the process of spindle formation is nearly completed.Dedicated to Professor Jakob Seiler on the occasion of his eightieth birthday.     

FINE STRUCTURE OF THE SPERMATOZOON OF HYDROIDES HEXAGONUS (ANNELIDA), WITH SPECIAL REFERENCE TO THE ACROSOMAL REGION

This paper describes in some detail the structure of the acrosomal region of the spermatozoon of Hydroides as a basis for subsequent papers which will deal with the structural changes which this region undergoes during fertilization. The material was osmium-fixed and mild centrifugation was used to aggregate the spermatozoa from collection to final embedding. The studies concern also the acrosomal regions of frozen-thawed sperm prepared by a method which previously had yielded extracts with egg membrane lytic activity. The plasma membrane closely envelops four readily recognizable regions of the spermatozoon: acrosomal, nuclear, mitochondrial, and flagellar. The acrosome consists of an acrosomal vesicle which is bounded by a single continuous membrane, and its periphery is distinguishable into inner, intermediate, and outer zones. The inner and intermediate zones form a pocket into which the narrowed apex of the nucleus intrudes. Granular material adjoins the inner surface of the acrosomal membrane, and this material is characteristically different for each zone. Centrally, the acrosomal vesicle is spanned by an acrosomal granule: its base is at the inner zone and its apex at the outer zone. The apex of the acrosomal granule flares out and touches the acrosomal membrane over a limited area. In this limited area the adjoining granular material of the outer zone is lacking. The acrosomal membrane of the inner zone is invaginated into about fifteen short tubules. The acrosomal membrane of the outer zone is closely surrounded by the plasma membrane. At the apex of the acrosomal region a small apical vesicle is sandwiched between the plasma membrane and the acrosomal membrane. Numerous frozen-thawed specimens and occasional specimens not so treated show acrosomal regions at the apex of which there is a well defined opening or orifice. Around the rim or lip of this orifice plasma and acrosomal membranes may even be fused into a continuum. The evidence indicates that the apical vesicle and the parts of the plasma and acrosomal membranes which surround it constitute a lid, and the rim of this lid constitutes a natural "fracture line" or rim of dehiscence. Should fracture occur, the lid would be removed and the acrosomal vesicle would be open to the exterior.     

泥螺卵黄发生过程中线粒体的变化

利用透射电镜（TEM）技术研究了泥螺卵黄发生过程中线粒体的形态结构的变化特点,结果表明,从卵黄发生早期到晚期,卵母细胞内线粒体经历了从外部形态到内部结构的一系列变化。卵黄合成初期的卵母细胞内,线粒体多,结构典型,仅部分线粒体外膜破裂,嵴 和内膜逐渐消失,卵黄发生中期,线粒体基质空泡化,嵴和内膜消失,腔内充满颗粒状物质,最后演变成卵黄颗粒,随着卵母细胞的发育,卵黄颗粒的数量和直径逐渐增加,卵黄发生后期,卵质中胞器不发达,细胞质中充满卵黄颗粒,在卵黄颗粒之间仅有少量线粒体存在,提供细胞代谢所需的能量,此外,对线粒体在卵黄形成中的功能,去向及行为变化等 进行了讨论。     

Ultrastructure and cytochemistry study of the yolk syncytial layer in the alevin of trout (Salmo fario trutta L.) after hatching

After hatching, the yolk syncytial layer of Salmo fario trutta may be subdivided into two zones, namely, the vitellolysis zone (containing numerous yolk platelets), and the cytoplasmic zone (where yolk platelets are rare). In the vitellolysis zone, two stages in the utilization of the yolk are observed: 1) The first stage, comprises the formation of yolk platelets from coalescent yolk by spherical cutting out and basal scission. This process seems to be achieved by the invagination of fibrillar elements into the coalescent yolk to form individual yolk platelets surrounded by a limiting membrane. 2) The second stage essentially consists of the extrusion or budding of yolk matter from a yolk platelet. Again, where the yolk matter leaves a platelet, fibrillar elements are evident and show an alkaline phosphatase activity. The platelets of the vitellolysis zone have a homogeneous content and variable diameter; they never acquire a heterogeneous and polymorphic aspect which could be interpreted as an intermediate stage in their degradation.     

Electron microscopic studies of the development of kinetes in Theileria annulata Dschunkowsky & Luhs, 1904 (Sporozoa, Piroplasmea).

Gamogony of Theileria annulata Dschunkowsky & Luhs occurs within the intestine of nymphs of the tick Hyalomma anatolicum excavatum Koch. After the 5th day post repletionem (p.r.) of the ticks spherical and ovoid parasites were found within the intestinal cells. These stages were thought to represent fertilized macrogametes. These underwent a transformation process leading ultimately to the differentiation of a motile stage, the kinete, which leaves the intestinal cells on the 14th-17th day p.r. and penetrates the alveoles of the salivary glands. The transformation of the stationary into a motile stage takes place by formation of a growing protrusion (= anlage) into an inner, enlarging vacuole. During this process the limiting membrane of the vacuole serves as the outer membrane of the developing motile stage, whereas the 2 inner membranes of its pellicle are newly formed. The steps of this differentiation in T. annulata are compared to the process of ookinete formation in haemosporina.     

Electron Microscopic Studies of the Development of Kinetes in Theileria annulata Dschunkowsky & Luhs, 1904 (Sporozoa, Piroplasmea)

SYNOPSIS. Gamogony of Theileria annulata Dschunkowsky & Luhs occurs within the intestine of nymphs of the tick Hyalomma anatolicum excavatum Koch. After the 5th day post repletionem (p.r.) of the ticks spherical and ovoid parasites were found within the intestinal cells. These stages were thought to represent fertilized macrogametes. These underwent a transformation process leading ultimately to the differentiation of a motile stage, the kinete , which leaves the intestinal cells on the 14th-17th day p.r. and penetrates the alveoles of the salivary glands. The transformation of the stationary into a motile stage takes place by formation of a growing protrusion (= anlage) into an inner, enlarging vacuole. During this process the limiting membrane of the vacuole serves as the outer membrane of the developing motile stage, whereas the 2 inner membranes of its pellicle are newly formed. The steps of this differentiation in T. annulata are compared to the process of ookinete formation in haemosporina.     

The fine structure of meiotic chromosome polarization and pairing in Locusta migratoria spermatocytes

At the leptotene stage of meiotic prophase in Locusta spermatocytes (2n=22 telocentric autosomes + X-chromosome), each chromosome forms an axial core. The 44 ends of the autosomal cores are all attached to the nuclear membrane in a small region opposite the two pairs of centrioles of the juxtanuclear mitochondrial mass. At later stages of meiotic prophase, the cores of homologous chromosomes synapse into synaptinemal complexes. Synapsis is initiated near the nuclear membrane, in the centromeric and the non-centromeric ends of the chromosomes. Homologous cores have their attachment points close together and some cores are co-aligned prior to synapsis. At subsequent stages of zygotene, the number of synaptinemal complexes at the membrane increases, while the number of unpaired axial cores diminishes. At pachytene, all 11 bivalents are attached to the membrane at both ends, so that there are 22 synaptinemal complexes at the membrane near the centrioles. Because each bivalent makes a complete loop, the configuration of the classic Bouquet stage is produced. The X-chromosome has a poorly defined single core at pachytene which also attaches to the nuclear membrane. These observations are based on consecutive serial sections (50 to 100) through the centriolar zone of the spermatocytes. Labeling experiments demonstrated that tritiated thymidine was incorporated in the chromatin of young spermatocytes prior to the formation of the axial cores at leptotene. It is concluded that premeiotic DNA synthesis is completed well in advance of pairing of homologous chromosomes, as marked by the formation of synaptinemal complexes.     

Modulation of Ca2+-mediated K+-gating of erythrocyte ghosts by external Ca-EGTA

Using 86Rb+ as a marker for K+ permeability, we find that extracellular Ca-EGTA influences the rate of 86Rb+ efflux from erythrocyte ghosts preloaded with 86Rb+ and "buffered" Ca2+. At an internal free Ca2+, where the rate of 86Rb+ efflux is minimal and uninfluenced by either external EGTA or external Ca2+, external Ca-EGTA at 0.2-0.5 mM can raise the flux rate to as high as can be attained by raising internal Ca2+, in the presence of an excess externally either of Ca2+ or of EGTA. Higher concentrations of Ca-EGTA (up to 1-2 mM) diminish the flux rate. External Ca-EDTA or Mg-EDTA can substitute for Ca-EGTA in enhancing and suppressing flux rate. The peak rate is insensitive to external free Ca2+ but depends on internal Ca2+; internal Mg-EDTA does not substitute for internal Ca-EGTA. Thus, the erythrocyte membrane is asymmetric with respect to its interaction with Ca2+ and Ca-EGTA. Also, 22Na+ does not substitute for 86Rb+. The peak rate of 86Rb+ flux produced by external Ca-EGTA is diminished by chlorpromazine (0.1 mM) and augmented by 1-propranolol (25 microM), in the same way as the rate produced by increasing internal Ca2+. The results suggest that external Ca-EGTA enhances the affinity of internal Ca2+ for its receptor(s) which operate the K+-gate at the inner surface of the membrane. At external concentrations of Ca-EGTA above 1-2 mM, 86Rb+ flux rate again rises with increase of Ca-EGTA. This phenomenon does not depend upon internal Ca2+, is not affected by chlorpromazine or by 1-propranolol, and is associated with an enhanced permeability to 22Na+, inulin, and haemoglobin.     

PLASMOLYSIS,HECHTIAN STRAND FORMATION,AND LOCALIZED MEMBRANE‐WALL ADHESIONS IN THE DESMID,CLOSTERIUM ACEROSUM (CHLOROPHYTA)1

Closterium acerosum Ehrenberg (Chlorophyta) produced a distinct network of thin cytoplasmic strands, or Hechtian strands, upon controlled plasmolysis in a sucrose solution. The strands persisted for 30 min or longer and could be visualized with both LM and EM. Near the plasma membrane of the polar zones of plasmolyzing protoplasts, the strands formed a “lattice”‐like arrangement with interstrand spacing of 120–130 nm. The strands terminated at the fibrous zone of the inner cell wall stratum. Although actin cables could be found attached to the plasma membrane upon rhodamine phalloidin labeling of membrane ghosts, neither microfilaments nor microtubules were found in Hechtian strands at any stage of development. The formation of strands was not disrupted by centrifugation at 8000 g or by repeated cycles of plasmolysis‐deplasmolysis. Application of microtubule‐ or microfilament‐affecting agents or various proteolytic/polysaccharide‐degrading enzymes did not disrupt the formation of strands. Cold treatment of cells resulted in the formation of Hechtian strands.     

Role of cytoplasmic ATP in the restoration and maintenance of a membrane permeability barrier in transformed mammalian cells

Addition of ATP to medium surrounding intact, transformed 3T3 cells activates the formation of aqueous channels in the plasma membrane. This results in efflux of nucleotide pools and ions and entry into the cytosol of charged, phosphorylated species. In such permeabilized cells, glycolysis is totally dependent on the external addition of glucose, inorganic phosphate, ADP, K+, Mg2+ and NAD+ which restore lactic acid formation to levels found in untreated cells. As expected, such reconstitution of glycolytic activity is found to restore intracellular ATP levels. This is accompanied by sealing of the membrane channels so that efflux of nucleotide pools ceases. Pyruvate, a substrate for mitochondrial ATP synthesis, when provided along with ADP and inorganic phosphate also produces sealing of the membrane channels. On the other hand, reactivation of pentose phosphate shunt activity, which does not lead to ATP synthesis, does not induce restoration of the membrane permeability barrier. Furthermore, compounds which lower the internal ATP pool prevent sealing, and also render the plasma membrane more sensitive to external ATP (Rozengurt and Heppel, '79). Sealing of aqueous channels following restoration of the internal ATP pool is associated with phosphorylation of the inner membrane surface, and is unaffected by inhibitors of protein synthesis, microfilament or microtubular assembly. These results indicate the probable role of intracellular ATP in the restoration and/or maintenance of an active membrane barrier against efflux of small molecules and ions in transformed 3T3 cells.     

A long-wavelength absorbing form of protochlorophyll and crystalloids in the inner seed coat of Luffa cylindrica

The inner seed coat of seeds of Luffa cylindrica (L.) Roem. (cv. Luffa sponge vine) was used to study the development of the protochlorophyll-containing plastids during different stages of maturity of the fruits. The inner seed coats had an absorption spectrum with a main peak in the red region at 675 nm and a shoulder at 630 nm. The fourth derivative spectrum gave a clear peak at 630 nm and also a small additional peak at 650 nm. An acetone extract showed a peak at 626 nm and a Soret band at 440 nm indicating that the main pigment in the seed coat was protochlorophyll. The ultrastructure of the protochlorophyll-containing plastids changed during maturation of the seed. In the young stage an elaborate membrane system was present. In a more mature stage the membrane system degenerated and crystalloids were formed. Some of these crystalloids seemed to develop into plastoglobuli in the most mature stage.     

Platelet activation and cytoskeletal reorganization: high voltage electron microscopic examination of intact and Triton-extracted whole mounts

The sequential changes in the three-dimensional organization of the filamentous components of human platelets following surface activation were investigated in whole-mount preparations. Examination of intact and Triton-extracted platelets by high voltage electron microscopy provides morphological evidence of increased polymerization of actin into the filamentous form and an increased organization of the cytoskeletal elements after activation. The structure of resting platelets consists of the circumferential band of microtubules and a small number of microfilaments randomly arranged throughout a dense cytoplasmic matrix. Increased spreading is accompanied by cytoskeletal reorganization resulting in the development of distinct ultrastructural zones including the peripheral web, the outer filamentous zone, the "trabecular-like" inner filamentous zone, and the granulomere . These zones are present only in well-spread platelets during the late stages of surface activation and are retained following Triton extraction. Extraction of the less stable cytoplasmic components provides additional information about the underlying structure and filament interactions within each zone.     

Immunohistochemical study of fibronectin localization during the formation of the vascular coat under the influence of the pigment epithelium in chick embryos

The role of fibronectin (FN) in cell interactions of retinal pigment epithelium (RPE) and mesenchyme surrounding the optic cup during choroid formation in chick embryos was studied by indirect immunofluorescence using antibodies against FN. Experimental coloboma of retina and choroid was used as a model. During the initial stages of coloboma the regions structured like retina rudiment appear in the outer layer of the optic cup. Such regions were formed in microphthalmic eyes obtained by excision of lens from the eyes of 3.5 day old chick embryos (stage 21). At stage 21 bright FN-specific immunofluorescence was observed in basal membrane located along the external surface of the normally differentiated RPE. Later on, FN-specific immunofluorescence appeared in mesenchyme condensing along the RPE. The most intensive FN-specific immunofluorescence was observed in chorio-capillary layer of choroid after 5-7 days of incubation. In microphthalmic eyes retina-like regions of RPE and adjacent mesenchyme showed negative reaction, and the choroid was not formed from the adjacent mesenchyme in such zones. The data obtained suggest that the presence of normally differentiated RPE producing FN-containing basal membrane is necessary for the formation of chorio-capillary layer of the choroid in chick embryos.     

Specific protein synthesis in cellular differentiation: III. The eggshell proteins of Drosophila melanogaster and their program of synthesis

The eggshell of Drosophila melanogaster is composed of a set of proteins synthesized by the follicular epithelium during the last third of oogenesis and organized into an inner zone (vitelline membrane) and an outer zone (chorion). To study these proteins, the authors developed techniques for mass-isolating follicles of mixed stages, mature (stage 14) follicles, chorion from stage 14 follicles, and chorion and vitelline membrane from laid eggs. The eggshell is composed mainly of protein and is unusually rich in proline and alanine. Six proteins of the chorion have been identified on polyacrylamide gels. The program of synthesis of these proteins was studied by incubating follicles of different developmental stages in culture with ³H-labeled amino acids and displaying the labeled proteins on gels with the aid of autofluorography. The proteins are synthesized in a specific overlapping sequence during stages 10–14, a period when chorion deposition is known to occur. In addition, putative vitelline membrane proteins have been identified by their preferential incorporation of [³H]proline and [³H]alanine during stages of active vitelline membrane synthesis.     

Effects of sheep urine on growth characteristics of different life form plants in a Chinese steppe grassland

The effects of sheep urine deposition volume (0, 1, 2 or 4 L/m²) and deposition stage of plant growth (vegetative or reproductive) on the number and size of tillers/branches and the biomass of Stipa bungeana, Artemisia capillaries and Lespedeza davurica in a Chinese steppe grassland were determined. The results indicate that the response of the three plant species to sheep urine deposition differs, and is influenced by both urine deposition volume and deposition stage of plant growth. Urine deposition had a short-term scorch effect on grassland plants, which mainly occurred in the inner zone of urine patches. Urine application had a long-term positive effect on S. bungeana and a long-term negative effect on A. capillaries and L. davurica, which lasted at least two years and decreased with decrease in urine deposition volume. All species growing in the inner zone of urine patches were scorched by sheep urine deposition, some species in the marginal zone of patches were also scorched, while no species were scorched in the outer zones. The reproductive and vegetative stages of A. capillaries and the reproductive stages of S. bungeana and L. davurica were sensitive to sheep urine deposition.     

Effects of sheep urine on growth characteristics of different life form plants in a Chinese steppe grassland

The effects of sheep urine deposition volume (0, 1, 2 or 4 L/m²) and deposition stage of plant growth (vegetative or reproductive) on the number and size of tillers/branches and the biomass of Stipa bungeana, Artemisia capillaries and Lespedeza davurica in a Chinese steppe grassland were determined. The results indicate that the response of the three plant species to sheep urine deposition differs, and is influenced by both urine deposition volume and deposition stage of plant growth. Urine deposition had a short-term scorch effect on grassland plants, which mainly occurred in the inner zone of urine patches. Urine application had a long-term positive effect on S. bungeana and a long-term negative effect on A. capillaries and L. davurica, which lasted at least two years and decreased with decrease in urine deposition volume. All species growing in the inner zone of urine patches were scorched by sheep urine deposition, some species in the marginal zone of patches were also scorched, while no species were scorched in the outer zones. The reproductive and vegetative stages of A. capillaries and the reproductive stages of S. bungeana and L. davurica were sensitive to sheep urine deposition.     

Evidence for an intermediate type of spermatozoon: ultrastructural studies of spermiogenesis in the cuttlefishRossia macrosoma (Cephalopoda,Decabrachia)

Summary Testes and spermatophores of the decapod cephalopodRossia macrosoma have been investigated by electron microscopy. Cytochemical analysis, by use of the periodic acid thiosemicarbazide-silver proteinate (PA-TSC-SP) technique, allows the precise localization of glycogen within the spermatozoon. Nuclear morphogenesis occurs in three stages (termed A, B and C), resulting in the transformation of the nucleus from an ovoid shape (stage A) into an elongated form (stages B and C). Prior to elongation of the spermatid nucleus, the spheroidal proacrosome, derived from the Golgi complex, becomes located at the apex of the nucleus. Later, the proacrosome elongates and its internal contents differentiate into an apical vesicle, electron-dense rod and electron-lucent subacrosomal fossa. A longitudinal microtubular manchette is closely associated with the elongating proacrosome. At this stage, the spermatid nucleus also elongates and its associated microtubular manchette is continuous with that surrounding the proacrosome. Large quantities of glycogen granules,-particles, about 130–145 Å in diameter, occur in the midpiece in relation to both the specialized external plasma membrane of the mitochondrial sleeve and within or around the axonome in the tail piece. We compare the features of spermiogenesis and the spermatozoon ofR. macrosoma with those documented in the literature for species from a number of phyla with the so-called primitive type of spermatozoon and which practise external fertilization, and the modified type in species practising internal fertilization. We suggest that the spermatozoon and spermiogenesis ofRossia demonstrates characteristics intermediate between these two groups and that the spermatozoon should be classified as an intermediate type.