On the Phospholipid Metabolism of Glial Cell Primary Cultures.

Abstract: Primary cultures were prepared from newborn rat brain. After 16-18 days, they consisted mainly of mature and immature astrocytes and oligodendrocytes, as judged by immunohistochemistry. To study the metabolism of ethanolamine glycerophospholipids, the cells were incubated with 1-[1-³H]alkyl- sn -glycero-3-phosphoethanolamine (1-alkyl-GPE), for 1–20 h. Five main products were formed: 1-alkyl-2-acyl-GPE; 1-alkyl-2-acyksn-glycero-3-phosphocholine (1-alkyl-2-acyl-GPC); 1-alkenyl-2-acyl-GPE (ethanolamine plasmalogen); 1-alkenyl-2-acyl-GPC (choline plasmalogen); and 1-alkyl-glycerol. Acylation of the substrate was the main reaction during the first 3 h of incubation, whereas desaturation to plasmaiogen reached a maximum after 12 h. Greater amounts of radioactivity were observed in the phosphatidylcholine fraction after longer incubation times. Only small amounts of choline plasmalogen were observed. The phosphatidylethanolamine fraction consisted of 26.5% diacyl-, 27.5% alkyl-acyl-, and 46.0% alkenyl-acyl- compounds, whereas the corresponding data for the phosphatidylcholine fraction were 78.5, 16.4, and 5.1%, respectively, after 20 h of incubation. Hydrolysis of the substrate to 1-alkyl-glycerol was a minor reaction.     

Über die Gefässe,die Faszikel und das Bindegewebe der Nerven während des Wachstums

Zusammenfassung Die Gefäße sprossen während zweier Wachstumsphasen in den Nerv ein: bei 11 cm langen Feten liegen 125 Gefäße innerhalb des N. tibialis (R. poplitea), auch bei 23 cm langen Feten finden sich etwa gleichviel Haargefäße im Endoneuralraum. Bei 39 cm langen Feten hat sich die Kapillarzahl etwa verdreifacht. Die Kapillarzahl pro Quadratmillimeter Endoneuralraum ist tabellarisch zusammengefaßt, die kritische Schichtdicke für einzelne Altersstufen errechnet worden.Bereits beim 11 cm langen Feten sind innerhalb des Nerven zarte Septen zu erkennen, aus denen sich bei 16 cm langen das Stratum lamellare perineurii entwickelt hat. Die Zahl der Lamellen vermehrt sich während des intrauterinen Lebens bis auf fünf. Das Stratum fibrosum perineurii et epineurii entwickelt sich erst beim über 35 cm langen Feten. Als erste Bindegewebsstruktur legen sich Teile des interfaszikulären Bindegewebes in Form von dreieckigen Zwickeln um die größeren Nervengefäße. Gleichzeitig runden sich die vorher eckig begrenzten Nervenfaserbündel ab. Während des intrauterinen Wachstums verdicken sich die Faszikel stetig. Allerdings schwanken Zahl und Durchmesser der Faszikel eines Nervs erheblich (Tabelle 2).Das Nervenbindegewebe nimmt während des Wachstums kontinuierlich zu (Tabelle 3). An der Umbiegungsstelle des N. tibialis sind die Faszikel vermehrt und verkleinert. Außerdem lassen sich mehr Bindegewebsanteile am Nervenquerschnitt ermitteln (Tabelle 4).In Injektionspräparaten von Nerven alter Menschen sind endoneurale Degenerationsherde (Renautsche Körperchen) aufgefunden worden. Da innerhalb der betroffenen Faszikel die Kapillarzahl um die Anzahl der Degenerationsherde vermindert ist, wird angenommen, daß diese Gebilde untergegangen und nekrobiotisch veränderten Kapillaren entsprechen.Diese Deutung wird gestützt durch Befunde an Kapillaren in der Umgebung der Degenerationsbezirke, deren Grundhäutchen verdickt und hyalinisiert sind.Im gelähmten Nerv nimmt das Bindegewebe relativ zur schrumpfenden Nervensubstanz zu.Herrn Professor Dr. Fritz Wassermann zum 80. Geburtstag in Verehrung gewidmet.     

Inhibition of Swarming of Proteus by Sodium Tetradecyl Sulfate, β-Phenethyl Alcohol,and p-Nitrophenylglycerine

The effects of sodium tetradecyl sulfate (STS), β-phenethyl alcohol (PEA), and p-nitrophenylglycerol (PNPG) on motility, swarming, flagellation, and growth of Proteus were examined. Growth-inhibitory concentrations (GIC) and swarming-inhibitory concentrations (SIC) were determined. A characterization of the swarming-inhibitory efficacy of these compounds was based on their GIC/SIC ratio and their concentration inhibition curves. Using the homologous series of sodium alkyl sulfates as a standard reference, we showed that PNPG was more effective than STS, which was the most effective of the homologous series. PEA was less effective than sodium decyl sulfate but more effective than sodium octyl sulfate. Motility tests in liquid medium and electron microscope investigations indicated that the modes of action of the three compounds, all of which effectively inhibit the swarming of Proteus, are different. Whereas STS and PEA inhibit swarming by inhibition of motility, PNPG seems to act on the swarming mechanism sensu strictori, without impairment of motility. STS immobilizes by inhibition of flagellum formation or by some lytic action on the flagella already synthesized. PEA acts by impairing flagellar function, but leaves the flagella morphologically intact.     

Über die reaktiven Veränderungen des Trabeculum corneosclerale im Primatenauge nach Einwirkung von Hyaluronidase

Zusammenfassung Einmalige Injektionen von 75–150 IE Hyaluronidase in die Augenvorder-kammer oder den Glaskörper führten am Trabekelwerk höherer Affen (Cercopithecus aeth.) in wenigen Tagen zur Auflösung der homogenen Substanzen des Lamellenkernes und zur Ablösung der Trabekelendothelien. Stellenweise wurden die Trabekel vollständig aufgelöst. Die abgelösten Trabekelendothelien zeigten elektronenmikroskopisch eine Vermehrung des Retikulum und der freien Ribosomen. Phagocytierte Zelleinschlüsse waren nachzuweisen. Die vergrößerten Kerne enthielten zahlreiche Nukleoli und wenig Chromatin. Inflammatorische Reaktionen waren nicht erkennbar. Stellenweise kam es zur Bildung größerer Symplasmen mit zahlreichen, aktivierten Kernen. Je nach Dosis regenerierte das Zell- und Lamellensystem des Trabekelwerkes in 7–10 Tagen vollständig.Durch mehrmalige Injektionen von Hyaluronidase in den Glaskörper konnten außer den beschriebenen Auflösungs- und Reparationsvorgängen erstmalig am Trabekelwerk auch proliferative Prozesse ausgelöst werden, die teilweise zur vollständigen Verlötung des Kammerwinkels und Obliteration des Schlemmschen Kanals führten. Der Mechanismus dieses Proliferationseffektes wird diskutiert.Ein Teil dieser Untersuchungen wurde in dankenswerter Weise durch die Deutsche Forschungsgemeinschaft unterstützt.     

Isolation of the vitellogenin-binding protein from locust ovaries

A rapid, efficient procedure for the isolation and purification of the vitellogenin binding protein from locust ovarian membranes is described. After solubilization with the nonionic detergent octyl-β-D-glucoside and removal of the detergent, the binding protein is subjected to affinity chromatography on vitellogenin coupled covalently to Affi-Gel 15. The binding protein is eluted with suramin and EDTA at low pH value. Sodium dodecyl sulfate (SDS) polyacrylamide gel electrophoresis reveals a polypeptide with a molecular weight of 156,000 in the eluted fraction. By ligand blotting this polypeptide could be identified as the vitellogenin binding protein. It retains its high-affinity binding properties. The specific binding of vitellogenin increases from 4.8 μg (intact ovarian membranes) to 170.9 μg (affinity purified binding protein) per mg membrane protein, which corresponds to a purification factor of 35.     

Blood–Brain Barrier Permeability to Sodium. Modification by Glucose or Insulin?

In order to explore the pathogenetic mechanism underlying the changes in blood-brain barrier sodium transport in experimental diabetes, the effects of hyperglycemia and of hypoinsulinemia were studied in nondiabetic rats. In untreated diabetes, the neocortical blood-brain barrier permeability for sodium decreased by 20% (5.6 +/- 0.7 versus 7.0 +/- 0.8 X 10(5) ml/g/s) as compared to controls. Intravenous infusion of 50% glucose for 2 h was associated with a decrease in the blood-brain barrier permeability to sodium (5.4 +/- 1.2 X 10(5) ml/g/s), whereas rats treated with an inhibitor of insulin-secretion (SMS 201-995, a somatostatin-analogue) had normal sodium permeability (7.3 +/- 2.0 X 10(5) ml/g/s). Acute insulin treatment of diabetic rats normalized the sodium permeability within a few hours as compared to a separate control group (7.7 +/- 1.1 versus 6.9 +/- 1.4 X 10(5) ml/g/s). To elucidate whether the abnormal blood-brain barrier passage is caused by a metabolic effect of glucose or by the concomitant hyperosmolality, rats were made hyperosmolar by intravenous injection of 50% mannitol. Although not statistically significant, blood-brain barrier sodium permeability increased in hyperosmolar rats as compared to the control rats (8.3 +/- 1.0 and 7.0 +/- 1.9 X 10(5) ml/g/s, respectively). It is concluded that either hyperglycemia per se or a glucose metabolite is responsible for the blood-brain barrier abnormality which occurs in diabetes. Further, we suggest that the specific decrease of sodium permeability could be the result of glucose-mediated inhibition of the Na+K+-ATPase localized at the blood-brain barrier.     

An inhibitor of elongation factor G (EF-G) GTPase present in the ribosome wash of Escherichia coli: a complex of initiation factors IF1 and IF3?

An inhibitor of elongation factor G (EF-G) GTPase isolated from the ribosome wash of Escherichia coli was shown to stimulate the poly(A,U,G)- and initiation factor 2 (IF2)-dependent binding of N-formyl-[35S]Met-tRNAfMet to ribosomes. In the presence of saturating amounts of the EF-G GTPase inhibitor, neither addition of initiation factor 1 (IF1) nor addition of initiation factor 3 (IF3) caused a further stimulation of the formation of N-formyl-[35S]Met-tRNAfMET/poly(A,U,G)/ribosome complexes. Both IF1 and IF3 were shown to inhibit ribosome-dependent EF-G GTPase, especially when both initiation factors were added either in absence or in the presence of initiation factor 2 (IF2), poly(A,U,G) and N-formyl-Met-tRNAfMet. Therefore, we conclude that the EF-G GTPase inhibitor consisting of two polypeptide subunits with apparent molecular masses of 23,000 and 10,000 Da is a complex of initiation factors IF1 and IF3. The inhibition of EF-G GTPAse by IF3, but not the effects of IF1 in the presence or absence of IF3 could be reversed by increasing the Mg(2+)-concentration as already shown for the EF-G GTPase inhibitor. Therefore, IF1 as well as the EF-G GTPase inhibitor do not influence the ribosome-dependent EF-G GTPase by affecting the association of ribosomal subunits.