Uptake and nature of the intracellular binding of cyclosporin A in a murine thymoma cell line, BW5147

In a survey of malignant cell lines including a variety of leukemias and lymphomas, BW5147, a T lymphoma from the spontaneous virus-associated thymoma in AKR mice, was found to be the most sensitive to growth inhibition by cyclosporin A (Cs A). Inhibition of growth was cell cycle phase-independent and inhibition of macromolecular precursor uptake was relatively nonspecific. Uptake of radiolabeled Cs A by these cells was characterized by two components: one that appeared saturable at low drug concentrations (0.03 to 1.0 microgram/ml), and another that was nonsaturable at higher drug concentrations (1.0 microgram/ml or higher). Most of the drug concentrated by cells (70 to 80%) was located in the cytosol (100,000 X G supernatant of lysed cells). The apparent m.w. of the drug-macromolecule complex was 15,000 to 20,000 as determined by m.w. exclusion columns. This complex could also be formed by adding drug to cytosol prepared from unexposed cells. The low m.w. complex migrated on a preparative isoelectric focusing column to form two peaks with isoelectric points of 6.8 and 8.5. A method was developed to assay for the binding component, and a sequence of m.w. exclusion columns and isoelectric focusing was used to effect partial purification of the Cs A binding component.     

Properties of cloned promoters

Strong early bacteriophage T7 promoters A2 and A3 and also A2 and lac UV5 promoters with altered segments downstream the initiation of RNA start point were cloned using specially constructed plasmid vectors pBRS188 and PBRS240. The relative signal strengths of these promoters in vivo and in vitro were evaluated and the kinetic parameters of their interaction with RNA polymerase were determined. It has been shown that the nucleotide sequence of the transcribed region plays a significant role in specific promoter-RNA polymerase interaction and that the rate-limiting step of RNA synthesis initiation is different for various promoters.     

Escherichia coli and Pseudomonas putida RNA polymerases display identical contacts with promoters

Summary Methylation protection experiments with four promoters (P1 and P2 of the pBR322 plasmid, lacUV5 and lambda P₀) have shown that the RNA polymerases from Escherichia coli and Pseudomonas putida, while differing in the primary structure of the subunits involved in DNA binding, display identical patterns of DNA contacts. Nor do these enzymes differ in covalent cross-linking patterns with a partially apurinized promoter. We conclude that the two RNA polymerases have very similar structures of DNA binding centers. The evolutionary conservation of this structure may account for the fact that diverse RNA polymerases often recognize and efficiently use promoters of distant bacterial species.     

Seasonal changes in ovarian state in a eusocial halictine bee,Lasioglossum duplex,based on stages of the oldest oocytes in each ovariole (Hymenoptera: Halictidae)

Summary The changes in ovarian activity in the life cycle of the eusocial halictine beeLasioglossum (Evylaeus) duplex (Dalla Torre) was studied in both queens and workers by examining the stages of the terminal follicle in each of the six ovarioles. By this method, ovarian activities of both queens and workers were more quantitatively determined than by observation of gross ovarian features as usually conducted. Queen ovaries clearly exhibited two active periods, corresponding to the spring solitary phase and the summer eusocial phase, with distinctly greater activity in the latter. In ovaries of overwintering queens oosorption of young follicle was observed. Worker ovaries were found more active in orphan than in queenright colonies. The order of ovarian activity obtained from pooled data, summer queens>spring queens>orphan workers>queenright workers, was also recognized by comparison of individual females. Bionomics of the eusocial halictine beeLasioglossum duplex IX. Contribution No. 3107 from the Inst. Low Temp. Sci.     

Self-sustained rhythmic spike and wave activity and response of glial and nerve cells in the cat sensorimotor cortex

During acute experiments on unanesthetized cats, immobilized with myorelaxants, it was found that during rhythmic stimulation (8–14 Hz, duration: 10 sec) of the ventroposterolateral thalamic nucleus brief hyperpolarization is succeeded by depolarization in the pyramidal neurons of the sensorimotor cortex. Following this depolarization, rhythmic (approximately 3 Hz) paroxysmal depolarizing shifts in membrane potential are produced by ending stimulation, succeeded by protracted hyperpolarization and termination of rhythmic wave activity. Depolarization only is observed in glial cells, however, while hyperpolarization sets in after hyperpolarization is completed in the neurons. It is suggested that long-term changes in the membrane potential of cortical cells could make some contribution to the setting up and termination of rhythmic spike and wave activity.I. S. Beritashvili Institute of Physiology, Academy of Sciences of the Georgian SSR, Tbilisi. Translated from Neirofiziologiya, Vol. 18, No. 3, pp. 319–325, May–June, 1986.     

Dynamics of the growth and maturation of oocytes and follicles in the ovaries of the cow

Chromosome despiralization and nucleolus vacuolization have been studied during the oocyte intensive growth. Oocyte and nucleolus growth has been found to stop at the secondary antral follicles with the diameter more than 1000 mkm. Chromosomal and nucleolar activity decreases at this stage. Chromosomes condense and concentrate around the nucleolus and chromatine mass (karyosphere) forms.     

Correlation between the amplitude of action potentials and the rate of conduction along axons of the output cells of the sensomotor cortex

Antidromic responses of neighbouring neurones in micro-areas of the sensorimotor cortex to the stimulation of fibers of the pyramidal tract as well as of the red nucleus and thalamic nuclei VPL and MGB, were studied in acute experiments on unanesthetized immobilized cats. Depending on the velocity of conduction along the axon, the neurones of all the categories were divided into fast and slow cells. When examining the two neuronal groups most differing in AP amplitude (N1 and N3), it was found that N1 neurones were mainly fast-conducting and N3 neurones-- slow-conducting. The conclusion is made that at multineuronal recording, each of the examined categories of the output neurones is characterized by positive correlation between AP amplitude and the axon conduction velocity and consequently, the size of the cell.     

Ultrastruktur und Bildung von Poren im Endothel von porösen und geschlossenen Kapillaren

Zusammenfassung An einer Reihe von normalen und pathologisch veränderten Organen wird die Porenstruktur, Porenbildung und Porenrückbildung elektronenmikroskopisch untersucht. Die Endothelpore ist eine Diskontinuität in der Endothelwand mit einem sehr konstanten Durchmesser von 500 Å. Das Diaphragma ist nur mit der äußeren Membranlamelle am Porenrand verbunden. Diaphragmalose Poren sind etwas größer (Ø650 Å), zeigen einen glatten Porenrand und kommen besonders in verdichteten Endothelteilen vor. Frustrane Poren münden blind in Vakuolen oder liegen in porösen Endothelfalten im Gefäßlumen. Die eigentliche Bildung der Poren geschieht immer in abgeflachten ( 800 Å) Endothelteilen. Die vorbereitende Abflachung geht jedoch in den verschiedenen Endothelzonen (Periksryon, dicker Endothelwand, Cytoplasmainseln) unterschiedliche Wege. Alle diese Vorgänge stellen Vesikulation in besonderer Lage und mit besonderer Fusionsrichtung der Vesikel dar. Wegen dieser Unterschiede wird die Endothelwand in 4 Zonen eingeteilt: Perikaryon; dicke, porenlose Wandteile mit cytoplasmatischen Vesikeln; dünne, porenhaltige Teile ohne Zellorganellen; dicke Cytoplasmainseln, die die porösen Wandteile voneinander trennen. Der Vorgang der Porenrückbildung bleibt unklar. Vielleicht besteht er in der Faltung des Endothels, die zu porösen Vakuolen führt. Die Porenbildung verändert die Endotheloberfläche nicht, kann aber das Cytoplasmavolumen vermindern. Der Aufbau des Diaphragmas sowie der Mechanismus und die auslösenden Faktoren der Porenbildung werden diskutiert.

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Summary Ultrastructure, formation and disappearance of endothelial pores was studied electron microscopically in several normal or experimentally changed organs. Pores being discontinuies in the endothelial wall have a very constant diameter of 500 Å. The diaphragm at the margin of the pore is in contact with only the outer lamella of the unit membrane. Pores without a diaphragm being somewhat larger (Ø 650 Å) show a smoother margin and are to be found in endothelia with dense cytoplasm. Frustrated pores form blind openings in vacuoles or are situated in porous endothelial folds within the vessel lumen. Pores alway are formed in flattened parts of endothelium ( 800 Å). In thick capillary walls the endothelium previously is flattened by vesiculation, which differs in different zones of the wall (Perikaryon, thick continuous endothelium, and cytoplasmic islands in porous capillaries) in location and direction of vesicle fusion. Because of these differences the endothelial wall is divided in 4 zones: Perikaryon; thick parts without pores containing cytoplasmic vesicles etc.; flattened, porous parts containing no cytoplasmic organelles; thick cytoplasmic islands which separate porous parts. The process removing pores is not clear. Perhaps they are removed by folding of the endothelial surface and formation porous vacuoles. Formation of pores dosn't enlarge or reduce the surface, but may reduce the cytoplasmic volume of endothelium. The nature of diaphragm as well as the mechanism and releasing factors of the formation of pores are discussed.

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