Male-male pairs in Greylag Geese (Anser anser)

Summary For almost two decades a flock of 130 free-flying Greylag Geese (Anser anser) has been the focus of detailed ethological investigations at the Konrad Lorenz Institut in Grünau im Almtal, Austria. Gander pairs, i. e. male-male pairs, represent a prominent social unit in this flock and were the subject of a detailed behavioral investigation. Analysis of the composition and dynamics of the flock over a 15 year period indicated that the incidence of homosexual pairings closely paralleled the male bias of the sex ratio. The behavior of ganders in gander pairs was investigated and compared to that of gander and goose in heterosexual pairs. The behavior of the two males in a gander pair (1) was comparable in most aspects, (2) was similar to the behavior of the gander in heterosexual pairs, and (3) differed greatly from that of the heterosexually paired goose. Therefore, pseudo-female behavior in one partner cannot account for the formation of a pairbond between two males. As a unit, gander pairs were characterized by a higher frequency of offensive agonistic behavior compared to heterosexual pairs and spent significantly more time peripheral to, and away from the flock than did heterosexual pairs.

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Zusammenfassung Das Sozialgefüge einer Schar Graugänse ist weitaus komplizierter, als es das monogame Fortpflanzungssystem erwarten ließe (Collias &Jahn 1959,Fischer 1965,Kalas 1979,Rutschke 1982). Ganterpaare, die häufig über Jahre hinweg bestehen bleiben, sind für tiersoziologische Untersuchungen interessant, weil ihre Funktion nicht im Rahmen der Fortpflanzung gesehen werden kann. Welche Bedingung begünstigen die Bildung von Ganterpaaren, und welche Verhaltensmechanismen tragen zum Entstehen und zur Aufrechterhaltung dieser Verbindung bei? Die Zusammensetzung der Grünauer Graugansschar 1973–1988 zeigt, daß die Anzahl der Ganterpaare von einem Überschuß von Männchen in der Schar abhängt. Das Verhalten von 6 Ganterpaaren wurde untersucht und mit dem von heterosexuellen Paaren verglichen. Innerhalb eines Ganterpaares entsprachen sich die Partner in der Häufigkeit von agonistischem sowie sozial-bindendem Verhalten. Homo- und heterosexuell verpaarte Ganter zeigten sich im Verhalten vergleichbar. Der Ganter eines Ganterpaares unterschied sich jedoch in der Häufigkeit aller untersuchten Verhaltensweisen von dem der heterosexuell verpaarten Gans. Folgende Schlußfolgerungen und Hypothesen bieten sich an: (1) Pseudo-weibliches Verhalten bei einem der Ganter scheint nicht die Bildung von Ganterpaaren erklären zu können. Beide Ganter verhalten sich rein männlich und behandeln den Partner so, als ob dieser ein Weibchen wäre. (2) Ein Mangel an gegengeschlechtlichen Schargenossen fördert die Bildung von homosexuellen Paaren und aufzuchtsbekannte Vögel werden dabei vorgezogen. (3) Ein Zusammenschluß mit einem gleichgeschlechtlichen Artgenossen sollte, verglichen mit der Möglichkeit alleine zu bleiben, eine überlegene Strategie darstellen, da unverpaarte Gänse geringeren Zugang zu Futterquellen haben und eher Raubtieren zum Opfer fallen. (4) Homosexuelle Paare könnten als ein Puffersystem für Ganter angesehen werden, vor allem zu Zeiten in denen das Geschlechtsverhältnis in Richtung der Männchen verschoben ist. (5) Aggression des Ganters richtet sich generell gegen andere männliche Schargenossen. Die Bildung von Ganterpaaren, also besonders aggressiven Paaren, könnte daher dazu beitragen, Ganter aus der Schar zu vertreiben und ein Übermaß von Männchen in der Schar zu verhindern. (6) Da wir zeigen konnten, daß sich homosexuelle Paare oft am Rande der Schar aufhalten und dabei häufig sichern, könnte solchen Paaren eine Art Wächterfunktion zukommen. (7) Andererseits ist es durchaus möglich, daß Ganterpaare bloß ein Epiphenomen einer Graugansschar mit einem Überschuß an Männchen darstellen.

     

Detection of enteroviruses in groundwater with the polymerase chain reaction.

Standard methods for the detection of enteroviruses in environmental samples involve the use of cell culture, which is expensive and time-consuming. The polymerase chain reaction (PCR) is an attractive method for the detection of enteroviruses in water because primary cell culture is not needed and the increased sensitivity of PCR allows detection of the low numbers of target DNAs and RNAs usually found in environmental samples. However, environmental samples often contain substances that inhibit PCR amplification of target DNA and RNA. Procedures that remove substances that interfere with the amplification process need to be developed if PCR is to be successfully applied to environmental samples. An RNA-PCR assay for the detection of enteroviruses in water was developed and used to test a variety of groundwater concentrates and humic acid solutions seeded with poliovirus type 1. The groundwater samples and humic acid solutions were treated with Sephadex G-50, Sephadex G-100, Sephadex G-200, Chelex-100 resin, and a mixed bed resin to remove PCR-inhibitory material from the samples. Sephadex G-100 in combination with Chelex-100 was found to be very effective in removing inhibitory factors for the detection of enteroviruses in groundwater concentrates by PCR. Viruses were detected in two of the groundwater concentrates by the RNA-PCR assay after treatment with Sephadex G-100 plus Chelex-100. This was confirmed by tissue culture, suggesting that the treatment protocol and, subsequently, the RNA-PCR assay are applicable for the detection of enteroviruses in environmental samples.     

Characterisation of a 34 kD protein from potato cyst nematodes, using monoclonal antibodies with potential for species diagnosis

Two monoclonal antibodies, which differentially recognise the two species of potato cyst nematodes (PCN), Globodera pallida and G. rostochiensis, are described. They have been shown to have potential for quantification of these two species, recognising proteins of the same molecular weight (34 kD) in both species. Further investigation showed these proteins to have isoelectric points at pH values of 5.7 in G. pallida and 5.9 in G. rostochiensis, in common with the proteins used by Fleming & Marks (1983) to differentiate the species of PCN. They are likely to be structurally very similar, with the same physiological function (and therefore similar concentrations) in the two species. In cross-reactivity tests with a wide range of soil nematode species, the antibodies reacted strongly only with species of the genus Globodera, and thereby confirmed their potential as the basis of a quantitative immunoassay likely to be useful in management of PCN populations.     

Crystal structure of human annexin I at 2.5 A resolution.

cDNA coding for N-terminally truncated human annexin I, a member of the family of Ca(2+)-dependent phospholipid binding proteins, has been cloned and expressed in Escherichia coli. The expressed protein is biologically active, and has been purified and crystallized in space group P2(1)2(1)2(1) with cell dimensions a = 139.36 A, b = 67.50 A, and c = 42.11 A. The crystal structure has been determined by molecular replacement at 3.0 A resolution using the annexin V core structure as the search model. The average backbone deviation between these two structures is 2.34 A. The structure has been refined to an R-factor of 17.7% at 2.5 A resolution. Six calcium sites have been identified in the annexin I structure. Each is located in the loop region of the helix-loop-helix motif. Two of the six calcium sites in annexin I are not occupied in the annexin V structure. The superpositions of the corresponding loop regions in the four domains show that the calcium binding loops in annexin I can be divided into two classes: type II and type III. Both classes are different from the well-known EF-hand motif (type I).     

Food intake and mass gain of hand-reared brown bear cubs

Five orphaned European brown bear cubs (Ursus arctos) from 3 litters were hand-reared from the ages of 1–4 months. Body mass initially ranged from 1.7 to 2.8 kg. Growth rates were monitored with reference to diet. Over a period of 3 years, 6 different feed formulas were used. The first 4 formulas were given with bottles until an average age of 133 days. Conversion to mass in the first 10 months ranged from 3.5 to 32.0 g of food per gram of body mass (or 38.1–192.6 kJ of gross energy/gram body mass), and was affected by type of diet. High fat content increased, whereas high carbohydrate content decreased the conversion rates. Formula 3, with 12.0% protein, 23.9% fat, and only 0.2% carbohydrates, simulated values found in bears' milk and produced the best growth rates. Formula 6 (bread, fruits, and meat) was used from ages 7 to 35 months, and over this period, the efficiency of gross energy conversion decreased gradually, by an eventual factor of 3.8. Hand-reared cubs ranged from 1.3 to 2.7 times heavier than 17 wild cubs measured at matching ages. Wild mass is probably limited by maternal hibernation, and by the largely herbivorous nature of the diet. © 1993 Wiley-Liss, Inc.     

Quaternary structure,Mg2+ interactions,and some kinetic properties of the (β-galactosidase fromThermoanaerobacterium thermosulfurigenes EM1

Theβ-galactosidase fromThermoanaerobacterium thermosulfurigenes EM1 was found to be a dimer with a monomer molecular weight of about 85,000. It lacks theα-peptide and an importantα-helix that are both needed for dimer-dimer interaction and there is no homology in other important dimer-dimer interaction areas. These differences in structure probably account for the dimeric (rather than tetrameric) structure. Only 0.19 Mg²⁺ bound per monomer and Mg²⁺ had only small effects on the activity and heat stability. The absence of residues equivalent to Glu-416 and His-418 (two of the three ligands to Mg²⁺ in theβ-galactosidase fromEscherichia coli) probably accounts for the low level of Mg²⁺ binding and the consequent lack of response to Mg²⁺. Both Na⁺ and K⁺ also had no effect on the activity. The enzyme activity witho-nitrophenyl-β-D-galactopyanoside (ONPG) was very similar to that withp-nitrophenyl-β-D-β-D-galactopyranoside (PNPG) and the ONPG pH profile was very similar to the PNPG pH profile. These differences are in contrast to theE. coli β-galactosidase, which dramatically discriminates between these two substrates. The lack of discrimination by theT. thermosulfurigenes β-galactosidase could be due to the absence of the sequence equivalent to residues 910-1023 of theE. coli β-galactosidase. Trp-999 is probably of the most importance. Trp-999 of theE. coli β-galactosidase is important for aglycone binding and ONPG and PNPG differ only in their aglycones. The suggestion that the aglycone site of theT. thermosulfurigenes β-galactosidase is different was strengthened by competitive inhibition studies. Compared toE. coli β-galactosidase, D-galactonolactone was a very good inhibitor of theT. thermosulfurigenes enzyme, while L-ribose inhibited poorly. These are transition-state analogs and the results indicate thatT. thermosulfurigenes β-galactosidase binds the transition state differently than doesE. coli β-galactosidase. Methanol and glucose were good acceptors of galactose, and allolactose was formed when glucose was the acceptor. Allolactose could not, however, be detected by TLC when lactose was the substrate. The differences noted may be due to the thermophilic nature ofT. thermosulfurigenes.     

Identification of Ser-543 as the major regulatory phosphorylation site in spinach leaf nitrate reductase.

Spinach leaf NADH:nitrate reductase (NR) responds to light/dark signals and photosynthetic activity in part as a result of rapid regulation by reversible protein phosphorylation. We have identified the major regulatory phosphorylation site as Ser-543, which is located in the hinge 1 region connecting the cytochrome b domain with the molybdenum-pterin cofactor binding domain of NR, using recombinant NR fragments containing or lacking the phosphorylation site sequence. Studies with NR partial reactions indicated that the block in electron flow caused by phosphorylation also could be localized to the hinge 1 region. A synthetic peptide (NR6) based on the phosphorylation site sequence was phosphorylated readily by NR kinase (NRk) in vitro. NR6 kinase activity tracked the ATP-dependent inactivation of NR during several chromatographic steps and completely inhibited inactivation/phosphorylation of native NR in vitro. Two forms of NRk were resolved by using anion exchange chromatography. Studies with synthetic peptide analogs indicated that both forms of NRk had similar specificity determinants, requiring a basic residue at P-3 (i.e., three amino acids N-terminal to the phosphorylated serine) and a hydrophobic residue at P-5. Both forms are strictly calcium dependent but belong to distinct families of protein kinases because they are distinct immunochemically.     

Characterization of a 100-kilodalton binding protein for the six serotypes of coxsackie B viruses.

Viral infection of host cells primarily depends on binding of the virus to a specific cell surface protein. In order to characterize the binding protein for group B coxsackieviruses (CVB), detergent-solubilized membrane proteins of different cell lines were tested in virus overlay protein-binding assays. A prominent virus-binding protein with a molecular mass of 100 kDa was detected in various CVB-permissive human and monkey cell lines but was not detected in nonpermissive cell lines. The specificity of CVB binding to the 100-kDa protein on permissive human cells was substantiated by binding of all six serotypes of CVB and by competition experiments. In contrast, poliovirus and Sendai virus did not bind to the 100-kDa CVB-specific protein. A fraction of HeLa membrane proteins enriched in the range of 100 kDa showed functional activity by transforming infectious CVB (160S) into A-particles (135S). In order to purify this CVB-binding protein, solubilized membrane proteins from HeLa cells were separated by preparative sodium dodecyl sulfate-polyacrylamide gel electrophoresis followed by elution of the 100-kDa protein. Amino acid sequence analysis of tryptic fragments of the CVB-binding protein indicated that this 100-kDa CVB-specific protein is a cell surface protein related to nucleolin. These results were confirmed by immunoprecipitations of the CVB-binding protein with nucleolin-specific antibodies, suggesting that a nucleolin-related membrane protein acts as a specific binding protein for the six serotypes of CVB.