Covalent labelling of histones with aurothiomalate. Gold-labelled H2A-H2B dimers assemble to octamers, which form crystalline helical tubes

Histone octamers were covalently labelled with aurothiomalate at amino groups by the method of carbodiimide activation. The labelling procedure was demonstrated to result in the specific covalent coupling through a single bond of the heavy metal atom label to protein amino groups. Such octamers were dissociated to yield soluble H2A-H2B dimers containing three gold atoms per dimer. The dimers were reconstituted with native H3-H4 tetramers to form labelled octamers, which were crystallized to form helical tubes. This strongly suggests that this procedure resulted in minimal changes of protein conformation.     

Cardiac sarcoplasmic reticulum contains a low-affinity site for phenylalkylamines

The distribution of the bovine cardiac binding sites for the organic calcium-channel blockers was studied. Crude microsomal membranes were separated into three fractions, which contained mainly membranes derived from sarcolemma, 'junctional' sarcoplasmic reticulum containing transversal tubuli, and free sarcoplasmic reticulum. The high-affinity binding site for the dihydropyridines, determined in the presence of nitrobenzylthioinosine, was enriched 12-fold and 17-fold in sarcolemma and junctional sarcoplasmic reticulum. The binding sites for the phenylalkylamines, determined with [3H]verapamil or [3H](-)desmethoxyverapamil, were enriched 1.5-3.4-fold in sarcolemma and junctional sarcoplasmic reticulum but 6-10-fold in free sarcoplasmic reticulum. The phenylalkylamine-binding site, present in free sarcoplasmic reticulum, was partially destroyed by chymotrypsin or phospholipase A2 and C treatment. Specific binding was proportional to the concentration of the added membrane protein. The binding of (-)desmethoxyverapamil was half-maximally inhibited by 6.5 mM calcium chloride and was optimal in the presence of 5 mM EGTA. In three out of five preparations (-)desmethoxyverapamil bound to a single site with an apparent Kd value of 191 +/- 42.8 nM and a density of 34.5 +/- 7.7 pmol/mg protein. In two out of five preparations an additional high-affinity site (Kd approximately 0.67 nM) was detected. The low-affinity site bound other phenylalkylamines, but stereospecific binding of phenylalkylamines was not observed. Binding of phenylalkylamines to the low-affinity site was inhibited by some but not all calmodulin 'antagonists'. Furthermore dihydropyridines did not affect the binding of (--)desmethoxyverapamil suggesting that the low-affinity site differs considerably from the high-affinity sarcolemmal site. These results suggest that free sarcoplasmic reticulum contains a binding site for phenylalkylamines at a relative high density, which is not related to the high-affinity site present in the voltage-dependent calcium channel.     

Steroid sulfatase. Biosynthesis and processing in normal and mutant fibroblasts

Antibodies raised against steroid sulfatase purified from human placenta were used to follow the biosynthesis of this enzyme in human skin fibroblasts. Steroid sulfatase is synthesized as a membrane-bound Mr-63 500 polypeptide with asparagine-linked oligosaccharide chains. Within 2 days, newly synthesized steroid sulfatase is processed to a mature Mr-61 000 form. The decrease in size is due to processing of the oligosaccharide chains, which are cleavable by endoglucosaminidase H in both the early and the mature form of steroid sulfatase. The processing involves mannosidase(s) sensitive to 1-deoxy-manno-nojirimycin. The half-life of the steroid sulfatase polypeptides is 4 days. Synthesis of steroid-sulfatase-related polypeptides and steroid sulfatase activity were not detectable in fibroblasts from four patients with X-linked ichthyosis.     

The extracellular matrix proteins laminin and fibronectin modify the AMPase activity of 5'-nucleotidase from chicken gizzard smooth muscle

Laminin and fibronectin, but not collagen, affect the AMPase activity of the purified transmembrane protein 5'-nucleotidase. Laminin stimulates whereas fibronectin inhibits the AMPase activity of this ectoenzyme. The AMPase-modulating effects by these components of the extracellular matrix require a preincubation period of several hours when detergent-solubilized 5'-nucleotidase is employed, they can, however, instantaneously be elicited with liposome-incorporated 5'-nucleotidase.     

Biliary lipid secretion in patients with heterozygous familial hypercholesterolemia and combined hyperlipidemia. Influence of bezafibrate and fenofibrate

Serum and biliary lipid metabolism were examined in 13 patients with different types of hyperlipoproteinemia before and after 4 weeks of treatment with either bezafibrate or fenofibrate. In patients with heterozygous familial hypercholesterolemia (FH), bezafibrate (n = 5) and fenofibrate (n = 7) produced a similar significant reduction of total cholesterol, LDL-cholesterol, and triglycerides by 21, 23, and 32%, respectively. In patients with familial combined hyperlipidemia (CHL), only triglycerides decreased markedly. Biliary lipid secretion rates in patients with heterozygous FH were not different from those of young male volunteers, indicating that a reduction of hepatic LDL receptors did not affect hepatic elimination of cholesterol or bile acids. Biliary cholesterol secretion increased significantly from 57 to 75 mg/hr during bezafibrate therapy (n = 8) and from 62 to 71 mg/hr during fenofibrate therapy (n = 9). No consistent change in bile acid or phospholipid secretion was observed. The elevated output of biliary cholesterol increased cholesterol saturation significantly from 147 to 185% and from 152 to 173% during administration of bezafibrate and fenofibrate, respectively. The present study indicates that treatment with bezafibrate or fenofibrate is effective in lowering LDL cholesterol in patients with heterozygous FH, but both drugs increase cholesterol saturation of bile, which might enhance the risk of cholesterol gallstone formation.     

Localization of eosinophil cationic protein, major basic protein, and eosinophil peroxidase in human eosinophils by immunoelectron microscopic technique

An immunoelectron microscopic technique using protein A-gold as a specific marker was used for precise intracellular localization of eosinophil granule proteins. Eosinophils from healthy individuals were isolated in metrizamide gradients. Eosinophil cationic protein (ECP) and eosinophil peroxidase (EPO) were clearly located in the matrix of the large crystalloid-containing granules. In addition, ECP was probably present in the small granules of eosinophils. Major basic protein (MBP) was present in the crystalloid structure of specific granules. This method can be applied in studies of eosinophil degranulation to trace the release of biological effector molecules.     

Die Bestandsentwicklung von Kleinv?geln in Mitteleuropa: Analyse von Fangzahlen

Zusammenfassung Im Mettnau-Reit-Illmitz-Programm (MRI-Programm) der Vogelwarte Radolfzell wurden von 1974–1983 auf drei Fangstationen in Süddeutschland, Norddeutschland und Ostösterreich (Abb. 1) 184 939 Vögel von 37 Kleinvogelarten gefangen. Die Fänge erfolgten jährlich während der gesamten Wegzugperiode von Ende Juni bis Anfang November an Durchzüglern in Japannetzen unter strikter und umfassender Standardisierung aller Fang- und Arbeitsmethoden. Die Fangzahlen (Tab. 1, Abb. 2–6) werden in fünf Regressionsanalysen (Tab. 2–9) auf systematische Änderungen untersucht.Von insgesamt 496 errechenbaren Koeffizienten waren 317 oder 63,9% negativ und nur 179 oder 38,1 % positiv. Bei 34 der 37 untersuchten Arten ließen sich signifikante Trends errechnen. Sie sind für 20 oder 54 % dieser Arten ausschließlich oder überwiegend negativ. 14 Arten zeigten mindestens auf zwei Stationen negative Trends. Nur für insgesamt 10 Arten ließen sich überwiegend positive Trends errechnen. Faßt man negative Trends und Tendenzen (Vorzeichen) zusammen, so ergibt sich für 26 oder 70 % der untersuchten Arten ein negatives Bild. Dieses stark negative Gewicht ist im statistischen Sinne keine zufällige Erscheinung. Da die Bestandszunahmen die Abnahmen nicht aufwiegen konnten, zeigten auch die jährlichen Gesamtfangzahlen aller drei Stationen negative Trends. Die mittlere jährliche Abnahme betrug auf den Stationen Mettnau, Reit und Illmitz etwa 1,6 %. Die Tendenzen und Trends der einzelnen Arten stimmen auf den drei Stationen weitgehend überein. Sie lassen für ihr Zustandekommen auf weitgehend gleichförmige Ursachen bei den durch Mitteleuropa wandernden Populationen schließen.Die Fangzahlen und Literaturdaten zeigen, daß beträchtliche Teile unserer Kleinvogelwelt von Rückgangserscheinungen betroffen sind, wie wir sie von vielen Großvogelarten seit langem kennen. Bei einer Reihe von Arten sind die Abnahmen gravierend und die jährlichen Fangzahlen inzwischen so niedrig, daß sich bei ihnen mit den in den 70er Jahren konzipierten Fanganlagen eine Reihe von Fragestellungen nicht mehr untersuchen lassen. Wir können der weiteren Entwicklung der Bestände unserer derzeit noch artenreichen Kleinvogelwelt — wie der vieler Großvögel — nur mit größter Sorge entgegensehen. Die Ursachen der Rückgänge sind weitgehend unbekannt, und demzufolge mangelt es fast vollständig an geeigneten Gegenmaßnahmen. Bisherige Schutzmaßnahmen haben die Rückgänge nicht aufhalten können. Künftiger Vogelschutz wird sich folglich weitergehender Maßnahmen bedienen müssen.

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The development of songbird populations in central Europe: Analysis of trapping data

Summary In the Mettnau-Reit-Illmitz-Program (MRI-Program) of the Vogelwarte Radolfzell 184 939 birds of 37 songbird species were caught in the period 1974–1983 on three trapping stations in S. and N. Germany and E. Austria (Fig. 1). Trapping of passage migrants in mist nets occurred annually from the end of June to the beginning of November, the entire autumn migratory period. All trapping and working methods were strictly and comprehensively standardized. The trapping figures (Tab. 1, Fig. 2–6) were analyzed with respect to systematic alterations to gain information about changes in the population levels of species migrating through central Europe. The investigation is based above all on five regression analyses (Tab. 2–9).The most important individual results are: out of a total of 496 coefficients which could be calculated 317 or 63.9 % were negative and only 179 or 38.1 % positive. For 34 of the 37 investigated species significant trends could be calculated. In 20 or 54 % of these species they were (exclusively or predominately) negative. 14 species showed negative trends at least at two stations. Mainly positive trends could be found in only 10 species. Taking negative trends and tendencies (negative signs) together, 26 or 70 % of the species were included. This strongly negative bias is not accidental in a statistical sense. Since the increases could not balance the declines, the annual trapping totals of all three stations also showed negative trends. The mean annual decline in the stations Mettnau, Reit and Illmitz was about 1.6 %. Trends and tendencies of the species show a high degree of agreement for the three stations. This suggests that in the species migrating through central Europe rather uniform factors control the population levels. From the most recent literature results, it appears that most of the species with declining trapping figures in the MRI-Program demonstrate decreases elsewhere.The trapping figures of the MRI-Program and data from the literature together clearly indicate that considerable parts of our small birds are affected by declines as have been known in many large bird species for long time. In a number of species the decreases have been quite dramatic and their annual trapping totals are now so low that a number of problems can no longer be studied. We should be alarmed when considering this negative development among our small birds as we must be with respect to many large bird species. The reasons for the declines are almost unkown and thus there is lack of appropriate counter-measures. Hitherto existing efforts for conservation which are briefly discussed have not been able to prevent the decline. Consequently, bird conservation in the future has to be based on more effective methods. Proposals, briefly raised, will be discussed in a forthcoming paper.

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Mit Unterstützung der Deutschen Forschungsgemeinschaft und gefördert mit Hilfe von Forschungsmitteln des Landes Niedersachsen. 15. Mitteilung aus dem MRI-Programm     

Laser cross-linking of nucleic acids to proteins. Methodology and first applications to the phage T4 DNA replication system

Single-pulse (approximately 8 ns) ultraviolet laser excitation of protein-nucleic acid complexes can result in efficient and rapid covalent cross-linking of proteins to nucleic acids. The reaction produces no nucleic acid-nucleic acid or protein-protein cross-links, and no nucleic acid degradation. The efficiency of cross-linking is dependent on the wavelength of the exciting radiation, on the nucleotide composition of the nucleic acid, and on the total photon flux. The yield of cross-links/laser pulse is largest between 245 and 280 nm; cross-links are obtained with far UV photons (200-240 nm) as well, but in this range appreciable protein degradation is also observed. The method has been calibrated using the phage T4-coded gene 32 (single-stranded DNA-binding) protein interaction with oligonucleotides, for which binding constants have been measured previously by standard physical chemical methods (Kowalczykowski, S. C., Lonberg, N., Newport, J. W., and von Hippel, P. H. (1981) J. Mol. Biol. 145, 75-104). Photoactivation occurs primarily through the nucleotide residues of DNA and RNA at excitation wavelengths greater than 245 nm, with reaction through thymidine being greatly favored. The nucleotide residues may be ranked in order of decreasing photoreactivity as: dT much greater than dC greater than rU greater than rC, dA, dG. Cross-linking appears to be a single-photon process and occurs through single nucleotide (dT) residues; pyrimidine dimer formation is not involved. Preliminary studies of the individual proteins of the five-protein T4 DNA replication complex show that gene 43 protein (polymerase), gene 32 protein, and gene 44 and 45 (polymerase accessory) proteins all make contact with DNA, and can be cross-linked to it, whereas gene 62 (polymerase accessory) protein cannot. A survey of other nucleic acid-binding proteins has shown that E. coli RNA polymerase, DNA polymerase I, and rho protein can all be cross-linked to various nucleic acids by the laser technique. The potential uses of this procedure in probing protein-nucleic acid interactions are discussed.     

A sodium dodecyl sulfate-gradient gel electrophoresis system that separates polypeptides in the molecular weight range of 1500 to 100,000

A sodium dodecyl sulfate-polyacrylamide gradient gel system is described. It combines a linear gradient in polyacrylamide from 10.2 to 30.2% in the separating gel and the discontinuous ammediol/glycine buffer system suggested by Bury (A. F. Bury, 1981, J. Chromatogr. 213, 491-500). This urea-free electrophoretic system provides high resolution and clean separation patterns of proteins and polypeptides with molecular weights from 1500 to 100,000. It is especially suited for studying complex mixtures of proteins and proteolytic fragments, in particular with regard to immunoelectrotransfer blot techniques.     

Combined administration of human corticotropin-releasing factor and lysine vasopressin induces cortisol escape from dexamethasone suppression in healthy subjects

Inadequate suppression of plasma cortisol after 1-2 mg dexamethasone is frequently observed in depressive patients. To further investigate the pathophysiology underlying cortisol nonsuppression after dexamethasone we compared cortisol and corticotropin (ACTH) response to human corticotropin-releasing factor (h-CRF), lysine vasopressin (LVP), and a concurrent administration of both peptides after pretreatment with 1.5 mg dexamethasone in six male controls. Neither h-CRF nor LVP were able to produce a marked elevation of dexamethasone suppressed plasma cortisol and ACTH. If both peptides were administered in combination, a substantial escape of plasma cortisol from dexamethasone suppression was observed. ACTH responses changed in concordance with those of cortisol indicating that the LVP-CRF interaction takes place at the pituitary level. Our finding is consistent with a multihormonal control of pituitary-adrenal activity and bears several implications for interpretation of dexamethasone suppression test results in depressive illness.