ALGAL ASSEMBLAGES IN ANTARCTIC PACK ICE AND IN ICE-EDGE PLANKTON1

A significant amount of the primary production in the Southern Ocean and other ice-covered oceans takes place in localized ice edge plankton blooms. The dynamics of these blooms appear to be closely related to seasonal melting of sea ice. Algal cells released from the ice are a possible source of ice edge planktonic assemblages, but evidence for this “seeding” has been equivocal. We compared algal assemblages in ice and water in the Weddell Sea during the austral spring of 1983 at a receding ice edge with a well-developed ice edge bloom. The high degree of similarity between ice and water column assemblages, the spatial and temporal patterns in the distribution and abundances of species, and preliminary evidence for the viability and growth of ice-associated species provide evidence for seeding from sea ice of some species in Antarctica.     

A direct radioassay for pyruvate kinase activity

Pyruvate kinase catalyzes the conversion of phosphoenolpyruvate (PEP) to pyruvate. A direct radioassay for this enzyme using [14C]PEP as substrate has been developed. The product, [14C]pyruvate, can be separated from the substrate rapidly and easily by applying the mixture to a hydroxyapatite column, and eluting the [14C]pyruvate directly into a scintillation vial. The [14C]PEP is bound to the column which can be regenerated and used indefinitely. The assay is sensitive, rapid, and particularly well suited for the simultaneous assay of large numbers of samples.     

The fine structure of the microconidium of blastomyces dermatitidis

Aspects of the fine structure of the microconidium of the mycelial phase of the dimorphic fungal pathogenBlastomyces dermatitidis as seen by techniques of scanning and transmission electron microscopy are described and illustrated by electron micrographs. The conidia ofB. dermatitidis undergo changes in the ultrastructural appearance of the cell wall as the spore matures. The cell wall becomes irregular in its thickness and possesses two distinct layers. No discrete or unique surface spines or projections were evident when the conidium ofB. dermatitidis was viewed by scanning electron microscopy. Upon maturity there is a marked deposition of lipid material in large, multiple storage bodies which occupy much of the cytoplasmic area. However, the cytoplasmic organelles appear to retain their structural integrity.     

Drug—induced alterations in the ultrastructural organization of Histoplasma capsulatum and Blastomyces dermatitidis

Aspects of the fine structure as seen in thin section of yeastlike cells ofHistoplasma capsulatum andBlastomyces dermatitidis exposed to polyenic antibiotics are described and illustrated by electron micrographs. The exposure of log phase yeastlike cells to minimal fungicidal concentrations of both amphotericin B (Fungizone) and hamycin resulted in detectable alterations of the plasma membrane, and, to a lesser extent, the mitochondria. WithH. capsulatum, ultrastructural changes were observed to occur within 1 h exposure to amphotericin B. Marked degenerative changes and plasmolysis were observed to occur within 6 hrs exposure of the yeastlike cells to both polyenes. The observed changes in ultrastructural appearance are compatible with the concept of binding of the polyene with membrane sterol and subsequent damage due to alterations of permeability.     

Mitotic chromosome condensation in the sperm nucleus during post fertilization maturation division in urechis eggs

Changes in the morphology of the sperm nucleus in the egg cytoplasm are mong the immediate events in nucleocytoplasmic interactions during early embryogenesis. Soon after its entrance into the egg cytoplasm, the sperm nucleus of various organisms increases in size with the transformation of condensed chromatin to a diffuse state, resembling the chromatin of an interphase nucleus (2, 13, 15, 16). This is followed by a close association or fusion of male and female pronuclei (2, 13, 15, 16). Cytoplasmic influences on nuclear morphology have also been demonstrated clearly in nuclear transplantation and cell fusion studies (10, 11). Reactivation of the nucleus, such as the transplanted brain nucleus in Xenopus egg cytoplasm or the hen erythrocyte nucleus in interphase cytoplasm of HeLa cells, is accompanied by nuclear enlargement and chromatin dispersion (10, 11). However, premature mitotic-like chromosome condensation takes place in the nuclei of sperm or interphase cells fused with mitotic cells (9, 12). Thus, chromosome dispersion and condensation seem to depend on the state of the cytoplasm in which the nucleus is present. These observations imply that the initial morphological changes in the sperm nucleus after fertilization may very well be dependent on the state of maturation of eggs at the time of sperm entry. Unfertilized eggs of Urechis caupo, a marine echiuroid worm, are stored at the diakinesis stage. These eggs complete maturation division after insemination and this is followed by fusion of male and female pronuclei (5, 8). Therefore, Urechis caupo is a suitable organism in which to study the response of the sperm nucleus to the changing state of the egg cytoplasm during and after postfertilization maturation division.     

Electrotonic coupling between cercal afferents and giant interneurons in the American cockroach

Stimulation of the cercal nerve of the female American cockroach evokes a short-latency action potential in one giant axon in the ipsilateral connective of the ventral nerve cord. Neither procion yellow nor cobalt passes from the nerve cord into the cercal nerve, and the short-latency response disappears several weeks after removal of the cercus. Therefore, the short-latency spike is not due to a branch of the giant interneuron extending into the cercal nerve, but is presumably due to electrotonic coupling of cercal afferents to the giant. Responses of the presumed electrotonic junction to drugs, varied ionic concentrations and tonicity, and to cold are described. These responses and the impermeability of the junction to procion yellow suggest that the coupling is not by means of a gap junction. There is evidence for electrotonic coupling to another giant axon in the female, but this junction does not ordinarily transmit a spike. Electrotonic coupling is rare in males. In some females action potentials in giant interneurons excite cercal afferents electrically, and the afferents then re-excite the giants chemically. Electrotonic coupling may reduce fatigue and habituation of chemical synapses by depolarizing presynaptic terminals whenever the giants are active.     

Calcium-stimulated respiration and active calcium transport in the isolated chick chorioallantoic membrane

Summary Calcium markedly stimulates the respiration of the isolated chick chorioallantoic membrane. This stimulation of oxygen uptake appears to be closely associated with the membrane's active transcellular calcium transport mechanism. In the presence of 1mm Ca⁺⁺ the rate of uptake increases from 9.3±0.15 to 13.0±0.2 liters O₂/cm²/hr, an increase of about 40%. The calcium-stimulated respiration is specific for the ectodermal layer of cells, the known location of the calcium transport mechanism, and only occurs when the calcium transport mechanism is operative. Sr⁺⁺ and Mn⁺⁺ are transported by the tissue at a lower rate than Ca⁺⁺ and cause a smaller stimulation of oxygen consumption. Mg⁺⁺ and La³⁺ have no effect on tissue respiration. In the presence of Ca⁺⁺, the organic mercurialp-chloromercuribenzene sulfonate (PCMBS) inhibits calcium transport and specifically decreases the oxygen uptake of the ectoderm to a rate identical to that obtained in a calcium-free medium. Stripping the inner shell membrane away from the chorioallantoic membrane mimics these effects. The specificity and locus of action of these two inhibitors suggest that a vital component of the active transcellular calcium transport mechanism resides on or near the outer surface of the plasma membrane of the ectodermal cells and that sulfhydryl groups are important to the normal function of this component.