DNA synthesis and distribution in parthenogenetic bovine embryos

Parthenogenetically activated, in vitro-matured bovine oocytes and parthenogenotes obtained at 2 to 4 days post activation were analyzed by 3H-thymidine autoradiography for the timing of the S-phase and for distribution of newly replicated DNA, respectively. Spread pronuclear parthenogenotes revealed that the DNA synthesis in electrically stimulated oocytes commenced at 14 h post activation. At 20 to 24 h, a maximum number of labeled pronuclei was reached (25 to 38%), and DNA synthesis persisted in some parthenogenotes up to 30 h post activation. The DNA labeling detected on semi-thin sections showed that the distribution of newly synthesized DNA in the nuclei of 3- to 16-cell parthenogenotes was mostly irregular or abnormal, documenting that the apparent morphological normalcy of parthenogenotes was in contrast to the data concerning the DNA synthesis and distribution.     

Isolation of the protoplasts fromAsteraceae by means of xylonase

The enzyme xylonase was used to isolate the protoplasts from the leaves ofCalendula officinalis L.,Gazania splendens Moore,Tithonia rotundifolia Blake,Zinnia elegans Jacq- and from the petals ofDahlia variabilis (Willd.) Desf. The recovery of spherical undamaged protoplasts differed. The same method did not lead to the isolation of the protoplasts from callus cultures derived fromCalendula, Gazania andTithonia leaves respectively.     

Organogenesis in isolated carnation plant callus tissue cultivatedin vitro

Formation of stems both in callus tissue isolated from hypocotyl and in apical meristems culture of carnation plants (Dianthus caryophyllus L. ev. “Grenadin white, yellow, scarlet red, dark red and pink”) was evokedin vitro using chemically defined medium. The rooted stems were transferred into pots and cultivated under natural conditions.     

Cholinergic Neuronotrophic Factors: Fractionation Properties of an Extract from Selected Chick Embryonic Eye Tissues

Abstract: An aqueous extract derived from selected intraocular tissues of 15-day chick embryos contains a soluble macromolecular agent which is capable of ensuring the survival of 8-day chick embryonic ciliary ganglionic neurons in monolayer culture. When this ciliary neuronotrophic factor (CNTF) was concentrated using ultrafiltration and subjected to Sephadex G100 and G200 chromatography, activity was detected in most of the eluted fractions. A peak of the most active fractions was eluted in a region corresponding to a molecular weight of 35–40 ± 10³ and contained about 20-30% of the applied protein. CNTF activity bound readily to DE-52 cellulose resin at neutral pH and was eluted with NaCl in a narrow region containing about 20-40% of the applied protein. Gel electrophoretic staining profiles of the active DE52 fraction indicated considerable (but still only partial) simplification in protein composition. While significant CNTF activity losses were incurred in response to each of the above treatments, an active material could be conveniently generated in one working day in milligram amounts having a specific activity of 60,000 trophic units/mg protein. This trophic activity is in the same range as that of the only other known neuronotrophic factor, Nerve Growth Factor.     

Characterization of binding properties of the myelin-associated glycoprotein to extracellular matrix constituents.

The myelin-associated glycoprotein (MAG) can be obtained from adult mouse brain from detergent-lysates of a crude membrane fraction as a 96-100 kd form (detergent solubilized MAG), and from 100,000 g supernatants of homogenates as a 90-96 kd form (soluble MAG). The soluble form distributes into the Triton X-114-poor aqueous phase, while detergent-solubilized MAG predominantly enters the Triton X-114-rich phase. Both molecular forms bind to heparin in hypo- and isotonic buffers. Soluble MAG binds to several collagens (type G, I, II, III, IV, V, VI, IX) with a kd of 5.7 X 10(-8) M for collagen type IX and 2.0 X 10(-7) for collagen type IV. Binding of 125I-labeled MAG to collagen G can be completely inhibited by unlabeled MAG and collagen G, but not by heat-denatured collagen. MAG does not bind to itself, laminin, fibronectin, or the neural cell adhesion molecules L1 and N-CAM. Binding of MAG to collagen G is most effectively blocked by a high molecular weight dextran sulfate, heparan sulfate and heparin, with chondroitin sulfate and a low molecular weight dextran sulfate being less potent blockers. These findings are in agreement with previous observations on the localization of MAG in basal lamina and interstitial collagens of the sciatic nerve in situ.     

Radiosensitive mutants of yeast-Saccharomyces with disruptions in the cell division cycle. Cell inactivation by restrictive temperature, ultra-violet and ionizing radiation in relation to the passage of the generated cycle

Three thermo- and radiosensitive mutants of yeast-Saccharomyces were used to study cell inactivation under the effect of elevated temperature, UV-light, and ionizing radiation. The forms of cell inactivation were shown to be identical with all the factors under study and to resemble lethal "terminal phenotypes" of Hartwell cds mutants. It is suggested that the cell division cycle is blocked due to the disorders in the system of gene product synthesis and not to defects in the enzymes themselves.     

Muskoxen in the high Arctic-temporal and spatial differences in body size

The life history of ungulates is affected by factors such as climate, population density and resource availability. With focus on the muskoxen Ovibos moschatus living in Kangerlussuaq in western Greenland, Jameson Land in north-eastern Greenland and on Banks and Victoria Islands in northern Canada, we tested spatial variation in life-history traits measured by mandibular growth. In accordance with expectations, we found that muskoxen in the southernmost and low Arctic area (Kangerlussuaq) grew faster, matured earlier, reproduced earlier, reached larger adult size and additionally had a higher reproduction than muskoxen living in the more northern areas. In the Kangerlussuaq population, mandible lengths in adult males changed temporally with density, with significant smaller adult males present in high population densities in western Greenland. It was especially the male mandible lengths that responded to environmental factors. In females, spatial differences were less pronounced than in males and is probably explained by females facing a trade-off between investment in own growth and reproduction, whereas a large body size is more important for the males, which are exposed to sexual selection. This explanation was, furthermore, supported by the fact that the calf percentage was higher in western Greenland than in any of the other studied areas in spite of the density-dependent effects detected within the male gender.     

Chemotaxonomic discrimination among the fungal genera Tolypocladium, beauveria and Paecilomyces

Fungi of the genera Beauveria and Paecilomyces were found to produce cyclotetradepsipeptides, beauverolides. Production of beauverolides was not detected at the genus Tolypocladium. Analysis of beauverolides therefore provides a very simple chemotaxonomic test which seems to be suitable for fast discrimination between the genera Beauveria vs Tolypocladium and complementing morphological examination. A GC-MS study of β-hydroxy acid distribution in the beauverolide hydrolyzates revealed that all strains prdouce γ-methyl-β-hydroxy acids only. Their occurrence thus cannot be used as a taxonomic marker of different species within the genera Beauveria and Paecilomyces.     

Quantification of angiogenesis in estrogen receptor-positive and negative breast carcinoma

Background

The objective of this study was to evaluate angiogenesis according to CD34 antigen expression in estrogen receptor (ER)-positive and negative breast carcinomas.

Methods

This study comprised 64 cases of infiltrating ductal carcinoma in postmenopausal women divided into two groups: Group A: ER-positive, n = 35; and Group B: ER-negative, n = 29. The anti-CD34 monoclonal antibody was used as a marker for endothelial cells. Microvessel count was carried out in 10 fields per slide using a 40× objective lens (magnification 400×). Statistical analysis of the data was performed using Student's t-test (p < 0.05).

Results

The mean number of vessels stained with the anti-CD34 antibody in the estrogen receptor-positive and negative tumors was 23.51 ± 1.15 and 40.24 ± 0.42, respectively. The number of microvessels was significantly greater in the estrogen receptor-negative tumors (p < 0.001).

Conclusion

ER-negative tumors have significantly greater CD34 antigen expression compared to ER-positive tumors.