The hepatic interleukin-6 receptor. Down-regulation of the interleukin-6 binding subunit (gp80) by its ligand.

Interleukin-6 (IL6) exerts its action via a cell surface receptor composed of an 80 kDa IL6-binding protein (gp80) and a 130 kDa polypeptide involved in signal transduction (gp130). We studied the role of gp80 in binding, internalization and down-regulation of the hepatic IL6-receptor (IL6R) by its ligand in human hepatoma cells (HepG2). Comparison of transfected HepG2 cells overexpressing gp80 with parental cells indicate that gp80 is responsible for low affinity binding (Kd = 500 pM) of IL6. Furthermore, gp80 is rate-limiting in internalization and degradation of IL6. Internalization resulted in a rapid down-regulation (t1/2 approximately 15-30 min) of IL6-binding sites at the cell surface. More than 80% of the internalized [125I]rhIL6 was degraded. The reappearance of IL6-binding sites at the cell surface required greater than 8 h and was sensitive to cycloheximide, suggesting that gp80 is not recycled after internalization. The down-regulation of the hepatic IL6R by its ligand might play an important role as a protection against overstimulation.     

The Standard Romanowsky-Giemsa Stain in Histology

A new and technically simple Romanowsky-Giemsa (RG) stain is proposed as a standardized technique for use in histology. An RG stock solution (pure azure B 7.5 g/l, eosin Y as eosinic acid 1.2 g/l in dimethylsulfoxide) is diluted to form the working solution with HBPES-buffer, pH 6. Staining time is 30-90 min after formolcalcium solution (or 2-4 hr after formaldehyde-organic acid mixtures). The resulting overstained sections are to be differentiated. A tannic acid-acetic acid combination in an isopropanol-water mixture was found to give optimum results within 100 sec. Subsequent dehydration is in isopropanol only. The staining pattern obtained is polychrome. The distribution of colors in detail is influenced by the modes of pre- and posttreatment. Of practical interest is the development of green and greenish blue colors on collagen fibrils which contrast strongly against the pink of sarcoplasm. For this and other reasons, this RG stain version seems suitable to replace the trichrome Gomori-type trichrome stains under appropriate processing conditions.     

Thermal acclimation and kinetics of a trypsin-like protease in eucarid crustaceans

Summary The properties of a trypsin-like protease in homogenates from midgut glands and gastric fluids of crustaceans were analyzed with special emphasis on thermal acclimation. For comparison, four species from different climatic regions were investigated: Ocypode ryderi (tropical), Cancer pagurus (temperate), Meganyctiphanes norvegica (subarctic-boreal), and Chorismus antarcticus (Antarctic). The pH optimum of the hydrolysis of N-benzoyl-l-arginine-p-nitroanilide is similar in all four species; at 25°C it ranged between pH 8 and 9.5. In the gastric fluids, pH was between 6.4 (Chorismus) and 7.7 (Ocypode); under experimental conditions at 25C, between 25% (Chorismus) and 95% (Ocypode) of maximal activity were observed at these pH values. Temperature optima of protease activity are independent from mean ambient temperature and were found to be around 50°C in Ocypode, 45°C in Cancer, 50–55°C in Meganyctiphanes, and 40°C in Chorismus. At temperatures near 0°C, temperate and tropical species show either a very low or even no activity at all, whereas the Antarctic and subarctic-boreal species display a residual activity of up to 15% of maximum activity. Under natural conditions, approximately 50% of maximal available enzymatic activity are eventually utilized. The kinetic parameters V _max and K _m depend on temperature and show distinct differences between the species. As an immediate response to temperature changes, the affinity for substrate decreases with elevated temperatures. Cold adaptation implies an effective utilization of energy in a low-energy system; the most prominent means of adaptation to low temperatures is the reduction of activation energy. Energies of activation in tropical temperate, and subarctic-boreal species (23.3–31.5 kJ·mol^-1) are significantly higher than in the Antarctic species (11.9–13.6 kJ·mol^-1). The enzymes were inhibited by N-tosyl-l-lysine chloromethyl ketone, copper sulfate, mercury chloride, and silver nitrate. In all enzymes, soybean trypsin inhibitor was the most effective inhibitor. Activation occurred after application of bovine serum albumin or calcium and magnesium chloride. The species-specific reactions after application of different protein or salt solutions support the hypothesis of decisive differences at the molecular level.Abbreviations BSA bovine serum albumin - E_a energy of activation - K _m Michaelis-Menten-constant - l-BAPA N-benzoyl-l-arginine-p-nitroanilide - SB soybean trypsin inhibitor - TLCK N-tosyl-l-lysine chloromethyl ketone - TRIS tris-(hydroxymethyl)-aminomethane - V _max maximal reaction velocity Contribution no. 409 of the Alfred-Wegener-Institute for Polar and Marine Research in Bremerhaven     

Sequential development of pathogens in the maize tarspot disease complex

The tarspot complex is caused by the interaction of Phyllachora maydis and Monographella maydis. Coniothyrium phyllachorae, possibly a mycoparasite, is found in older ascostromata of P. maydis, which always appears first causing tarspot. M. maydis follows and is responsible for the damaging fisheye symptom. The fisheye symptom is always associated with a tarspot in the center of the lesion, whereas 12 to 20% of the Phyllachora ascostromata remained free of M. maydis. Inoculations of maize leaves with the Microdochium anamorph of the Monographella (usually produced in lesions) failed to produce infections. Some infections with M. maydis were, however, obtained under unusual conditions in the field. Inoculations onto tarspots in the laboratory were unsuccessful, but in field experiments inoculations with conidia of M. maydis enhanced severity of the tarspot complex. Fisheye symptoms of the complex naturally appear 2 to 7 days after the manifestation of P. maydis. This is followed a week later by the appearance of M. maydis which became predominant in the lesions and is associated with empty perithecia of P. maydis. In the early stages of the tarspots pycnidia of the anamorph of P. maydis, Linochora sp., could occasionally be observed. Ascomata of M. maydis were rare in the field. Of the 36 genetic materials of CIMMYT tested, 30 developed the fisheye symptom, 4 tarspots only and 2 remained free of symptoms     

Co-localization of vimentin and cytokeratins in M-cells of rabbit gut-associated lymphoid tissue (GALT)

Summary The occurrence of cytokeratins, vimentin, and desmin in the dome epithelia and adjacent non-dome epithelia in four locations of gut-associated lymphoid tissues (GALT) of adult and newborn rabbits (Peyer's patches, sacculus rotundus, caecal lymphoid patches and appendix) was studied with monoclonal antibodies, using the indirect immunoperoxidase technique. In all locations investigated in adult animals, antibodies specific for vimentin labelled (1) M-cells, which engulf intraepithelial lymphocytes, (2) columnar epithelial cells at the base of the domes lacking an apparent contact with lymphocytes (immature M-cells), and (3) flat cells, which lie in the lamina propria under the dome epithelium, and which line the basal lamina with thin cytoplasmic processes. In newborn rabbits, columnar epithelial cells resembling the immature M-cells of adults were selectively stained with vimentin antibodies. In M-cells, the strongest immunoreactivity was present in the perinuclear region and close to the pocket membrane, whereas the most apical and most basal parts of the cytoplasm showed no vimentin-immunoreactivity. Enterocytes in the dome epithelium and in the non-dome epithelium were vimentin-negative. M-cells and enterocytes bound antibodies against cytokeratin peptides 18 and 19 in adults and newborn animals. Compared with enterocytes, M-cells showed less intense staining for cytokeratins. Dome epithelia and no-dome epithelia did not contain desmin-immunoreactive cells. The results suggest that vimentin is a sensitive marker for M-cells in rabbit GALT.     

Rapid induction of phenylalanine ammonia-lyase and chalcone synthase mRNAs during fungus infection of soybean (Glycine max L.) roots or elicitor treatment of soybean cell cultures at the onset of phytoalexin synthesis

The differential regulation of the activities and amounts of mRNAs for two enzymes involved in isoflavonoid phytoalexin biosynthesis in soybean was studied during the early stages after inoculation of primary roots with zoospores from either race 1 (incompatible, host resistant) or race 3 (compatible, host susceptible) of Phytophthora megasperma f.sp. glycinea, the causal fungus of root rot disease. In the incompatible interaction, cloned cDNAs were used to demonstrate that the amounts of phenylalanine ammonia-lyase and chalcone synthase mRNAs increased rapidly at the time of penetration of fungal germ tubes into epidermal cell layers (1–2 h after inoculation) concomitant with the onset of phytoalxxin accumulation; highest levels were reached after about 7 h. In the compatible interaction, only a slight early enhancement of mRNA levels was found and no further increase occurred until about 9 h after inoculation. The time course for changes in the activity of chalcone synthase mRNA also showed major differences between the incompatible and compatible interaction. The observed kinetics for the stimulation of mRNA expression related to phytoalexin synthesis in soybean roots lends further support to the hypothesis that phytoalexin production is an early defense response in the incompatible plant-fungus interaction. The kinetics for the enhancement of mRNA expression after treatment of soybean cell suspension cultures with a glucan elicitor derived from P. megasperma cell walls was similar to that measured during the early stages of the resistant response of soybean roots.Abbreviations cDNA copy DNA - CHS chalcone synthase - PAL phenylalanine ammonia-lyase     

The optic lobe of Drosophila melanogaster. I. A Golgi analysis of wild-type structure

Summary Golgi studies of the neurons in the optic lobes of Drosophila melanogaster reveal a large number of neuronal cell types. These can be classified as either columnar or tangential. Columnar elements establish the retinotopic maps of the lamina, medulla, and lobula-complex neuropiles. They are classified according to the position of their cell bodies, the number, width, and level of their arborizations, and their projection areas. Tangential elements are oriented perpendicularly to the columns. The arborizations of different tangential neurons are restricted to different layers of the optic neuropiles, within such layers their dendritic fields may span the entire retinotopic field or only part of it. The abundance of cell types inside each of the columnar units of the optic lobe is discussed with regard to its possible functional significance. By means of their stratified arborizations the columnar neurons form what appear to be multiple sets of retinotopically organized parallel information processing networks. It is suggested that these parallel networks filter different kinds of visual information and thus represent structurally separated functional subunits of the optic lobe. Such a parallel organization of visual functions increases the sites for function-specific gene actions and may explain the behavioral phenotypes of recently isolated structural mutants of the optic lobe.     

Gamma-Glutamyl Transpeptidase Does Not Act As a Cystine Transporter in Brain Microvessels

Gamma-glutamyl transpeptidase (GGTP) is highly enriched in blood-brain barrier (BBB) microvessels. According to the most cited hypothesis its functional role is amino acid transport across the BBB. To test this hypothesis the influence of GGTP inhibition on cystine uptake was measured in isolated brain microvessels. Adult porcine brain microvessels were enzymatically isolated, resulting in an enrichment of GGTP from 3 to 85 U/mg protein. The inhibitors 0.1 mM AT-125 combined with 20 mM hippurate reduced the GGPT enzyme activity by more than 98%. However this inhibition did not influence the uptake of [³⁵S]-cystine, which is the substrate with the highest affinity in the GGTP-reaction. Instead increased glutathione (GSH) levels and elevated [³⁵S] release were found. These results show that GGTP does not mediate the transport of cystine into brain microvessels in vitro and suggest that GGTP plays a role in cellular GSH metabolism.     

Recycling of a glycosylphosphatidylinositol-anchored heparan sulphate proteoglycan (glypican) in skin fibroblasts

We have used suramin and brefeldin A to investigate the natureof a heparan sulphate proteoglycan that appears to recycle fromthe cell surface to intracellular compartments which synthesizenew heparan sulphate chains. Suramin, which would block internalizationand deglycanation of a putative recycling cell surface proteoglycan,markedly increases the yield of a membrane-bound proteoglycanwith a core protein of 60–70 kDa and unusually long heparansulphate side chains. When transport of newly made core proteinsto their Golgi sites for glycosaminoglycan assembly is blocked,by using brefeldin A, [³H]glucosamine and [³⁵S]sulphate incorporationinto cell surface-bound heparan sulphate proteoglycan can stilltake place. After chemical biotinylation of cell surface proteinsin brefeldin A-treated cells, followed by metabolic [³⁵S]sulphationin the presence of the same drug, biotin-tagged [³⁵S]proteoglycancan be demonstrated, indicating the presence of recycling proteoglycanspecies. By prelabelling cells with [³H]leucine or [³H]inositolin the presence of suramin, followed by chase labelling with[³⁵S]sulphate in the presence of brefeldin A, a ³H- and ³⁵S-labelled,hydrophobic heparan sulphate proteoglycan with a core proteinof 60–65 kDa is obtained. The proteoglycan loses its hydrophobicitywhen glucosamineinositol bonds are cleaved, indicating thatit is membrane bound via a glycosylphosphatidylinositol anchor.However, treatment with phosphatidylinositol-specific phospholipaseC has no effect, suggesting that the inositol moiety may beacylated. We propose that a portion of the lipid-anchored proteoglycanglypican is internalized, recycled via the Golgi, where heparansulphate chains are added, and finally re-deposited at the cellsurface. glycosylphosphatidylinositol-anchored glypican heparan sulphate proteoglycan recycling