X-Linked Female-Sterile Loci in DROSOPHILA MELANOGASTER

We have examined the number of X-linked loci specifically required only during oogenesis. Complementation analyses among female-sterile (fs) mutations obtained in two mutagenesis screens--GANS' and MOHLER's--indicate that any fs locus represented by two or more mutant alleles in GANS' collection are usually present in MOHLER's collection. However, when a locus is represented by a single allele in one collection, it is generally not present in the other collection. We propose that this discrepancy is due to the fact that most "fs loci" represented by less than two mutant alleles are, in fact, vital (zygotic lethal) genes, and that the fs alleles are hypomorphic mutations of such genes. In support of this hypothesis we have identified lethal alleles at 12 of these "fs loci." The present analysis has possibly identified all maternal-effect lethal loci detectable by mutations on the X chromosome and has allowed us to reevaluate the number of "ovary-specific fs" loci in the Drosophila genome. Finally, germline clone analysis of a large number of fs mutations was performed in order to estimate the relative contribution of germline and somatic cell derivatives to oogenesis and to embryonic development. All the maternal-effect lethal loci tested are germline-dependent.     

Nachweise von Zweitbruten beim Wei?sternigen Blaukehlchen (Luscinia svecica cyanecula)

Summary Close to the village Trieb in Upper Franconia (50° 09 N/11° 10 E) two cases of second breeding in the Bluethroat could be proved. The birds were colour-banded. Second broods are presumably rather common in the population along the upper River Main.     

Immunoelectron microscopic studies on the localization of peptidoglycan peptide subunit pentapeptides in bacterial cell walls

The peptide subunit pentapeptide H-L-Ala-D-Glu(L-Lys-D-Ala-D-Ala-OH)-NH₂ of peptidoglycan was localized in the cell walls of several Gram-positive bacteria employing the indirect immunoferritin technique. Specific antibodies to the D-alanyl-D-alanine moiety of non-crosslinked peptide subunit pentapeptide were raised in rabbits by immunization with synthetic immunogen albumin-(CH₂CO-Gly-L-Ala-L-Ala-D-Ala-D-Ala-OH)₃₉. Specificity of these antibodies for the peptide subunit pentapeptide and not for the peptide subunit tetrapeptide was corroborated in a Farr-type radio-active hapten binding assay. Specificity of labelling with ferritin was established by immunoelectron microscopic controls, and by the excellent correlation between specific labelling of cells with ferritin and the particular peptidoglycan primary structure of bacterial strains investigated. Cells of Lactobacillus gasseri, Streptococcus pyogenes and Staphylococcus aureus revealing non-crosslinked peptide subunit pentapeptides in their peptidoglycans could specifically be labelled. Lactobacillus acidophilus and Bacillus subtilis, on the contrary, missing such pentapeptides, failed in labelling.The implication of this method to possibly localize the points of attack of penicillin or cycloserine is discussed.Abbreviations used meso-A₂pm meso-diaminopimelic acid - DSM Deutsche Sammlung für Mikroorganismen, Göttingen, FRG This paper is dedicated to Professor Gerhart Drews on the occasion of his 60th birthday     

Covalent immobilization of the multienzyme enniatin synthetase

Summary The multienzyme enniatin synthetase was covalently immobilized to N-hydroxysuccinimide activated agarose. The stability of the immobilized enzyme at 25°C was enhanced compared to the soluble enzyme. Immobilization experiments also indicated that the enniatins are synthesized by a single molecule and thus do not require interactions of several enzyme molecules.     

Anaerobic degradation of 3,4,5-trimethoxybenzoate by a defined mixed culture of Acetobacterium woodii, Pelobacter acidigallici, and Desulfobacter postgatei

Abstract Acetobacterium woodii was continuously grown on 3,4,5-trimethoxybenzoate as pure culture or in commensalistic combination with Pelobacter acidigallici and Desulfobacter postgatei . Under pure culture conditions the following growth parameters were determined: μ _max= 0.112 h⁻¹, K _s= 1.07 mM, Y _max= 35 g/mol, and m = 0.22 mmol·g⁻¹·h⁻¹. In coculture with P. acidigallici the affinity for the substrate increased and the K _s value was found to be 135 μM. Under batch culture conditions mixed populations of A. woodii, P. acidigallici , and D. postgatei completely mineralized 3,4,5-trimethoxybenzoate to CO₂, whereas under continuous culture conditions more than 3 mM acetate remained unused.     

Langzeitkulturen von Süßwasserschwämmen (Porifera,Spongillidae) unter Laborbedingungen

Zusammenfassung Süßwasserschwämme (Spongilliden) lassen sich in 120-1-Aquarien mit Herkunftswasser der Schwämme kultivieren. Das gut durchlüftete Wasser soll nicht wärmer als 17°C sowie mit den Zusätzen Aquatonic und Schwarztorf versehen sein. Anstelle des Teichbzw. Flußwassers kann auch Leitungswasser oder eine Mischung von Leitungs- und vollentsalztem Wasser verwendet werden. Das Wasser der Aquarien ist alle vier Monate zu erneuern.Als Kulturgefäße eignen sich Glas- und Kunststoffschalen. Diese werden mittels spezieller Halter in die Aquarien eingebracht.Langzeitkulturen bieten beste Voraussetzungen für die Schwammforschung.

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Permanent cultures of freshwater sponges (Porifera, Spongillidae) in the laboratory

Summary Freshwater sponges (Spongillidae) can be cultivated in 120-1 aquariums with water from the natural sponge habitats. The well-aired water should not be warmer than 17°C and should contain Aqua-tonic and black peat. Instead of habitat water, tap water or a mixture of tap and distilled water may be used. The water in the aquariums should be renewed every 4 months.For the culture we use glass or plastic vessels. These are mounted in the aquariums by special holders.Permanent cultures offer ideal conditions for sponge research.

     

Ultrastruktur und polysaccharidanteile der cuticula von Triops cancriformis Bosc. (Crustacea,Notostraca) während der Häutungsvorbereitung

Zusammenfassung Die Cuticula von Triops cancriformis besteht aus Endo-, Exo- und Epicuticula. Die Epicuticula ist aus vier Schichten aufgebaut, die Exocuticula aus 10 und die Endocuticula aus 60–80. Die Schichten der Endocuticula sind aus annähernd oberflächenparallel verlaufenden Mikrofibrillen, die zu Lamellulae zusammentreten, gebildet. Diese Lamellulae atehen senkrecht zur Oberfläche. Die Lamellulae der einzelnen Lagen verlaufen im rechten Winkel zu denen der Nachbarlagen. In Sinnesborsten verläuft so ein Teil der Fibrillen in Längsrichtung, der andere quer zur Längsachse.Polysaccharide finden sich in den Lamellulae, in zwei Schichten der Epicuticula, den Desmosomen und als Glykogengranula in Epidermiszellen.Die Häutung zeigt anscheinend keine Besonderheiten gegenüber anderen Arthropoden.

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Ultrastructure and polysaccharide content of the cuticle of Triops cancriformis Bosc. (Crustacea, Notostraca) during the Molting preparation

Summary The cuticle of Triops cancriformis consists of endo-, exo- and epicuticle. The epicuticle comprises 4 layers, the epocuticle 10 and the endocuticle 60–80 layers. The layers of the endocuticle consist of microfibrils. These microfibrils are almost parallel to the surface of the cuticle and merge into lamellulae. These lamellulae run vertical to the surface. The lamellulae in any one layer are at right angles to the lamellulae in the neighbouring layers. Thus, some of the fibrils in sensory setae are parallel to the longitudinal axis and others are perpendicular to it.Polysaccharides are found in the lamellulae, in two layers of the epicuticle, in the attachment regions and in the glycogen deposits in the epidermis cells.The molting process seems to be similar to the molting process of other arthropoda.

     

Human HepG2 and Rat Fao Hepatic-Derived Cell Lines Show Different Responses to Ciprofibrate, a Peroxisome Proliferator: Analysis by Flow Cytometry

Peroxisome proliferators, and especially hypolipidemic drugs such as ciprofibrate, are known to be hepatocarcinogens in rodents, but their effect in humans is controversial. In an attempt to investigate the effects of ciprofibrate at a cellular level, the analysis of individual whole cells was performed by flow cytometry on samples from two hepatic-derived cell lines: the rat Fao cell line and the human HepG2 cell line. The increase of light scatter signals in rat Fao cells treated for 3 days with ciprofibrate at 250 μMwas related to modifications of intrinsic cellular parameters, such as size and cytoplasmic granularity. Conversely, no variations appeared in human HepG2-treated cells. Moreover, the study of the cell cycle distribution of asynchronously growing cells showed an increase in the percentage of proliferative cells in Fao-treated cells, but not in HepG2-treated cells. In order to give a simultaneous assessment of changes in cellular parameters and cell metabolism, these flow cytometric experiments were completed with the measurements of the palmitoyl–CoA oxidase activity, used as a marker of peroxisome proliferation. The cellular modifications in the rat Fao cell line were accompanied by a great increase in this enzymatic activity, whereas the human HepG2 cell line, which failed to exhibit changes of cytometric data, presented no, or weak, increase in this oxidase activity. The cellular modifications observed in the rat Fao cell line may be related to the well-known hepatocarcinogenicity of ciprofibrate in rodents, whereas the absence of response of HepG2 cells is in favor of the noncarcinogenicity of this drug in humans. This report validates another methodological approach for the investigation of the safety of peroxisome proliferators in humans.     

Separation of the enantiomers of coumarinic anticoagulant drugs by capillary electrophoresis using maltodextrins as chiral modifiers

The separation and quantitation of coumarinic anticoagulant drug enantiomers were achieved by direct chiral capillary electrophoresis using complex maltooligosaccharide mixtures as stereoselective electrolyte modifiers. Chiral separations were characterized by a high selectivity and efficiency, enabling enantiomeric excess determinations. In addition, preliminary results indicate the applicability of the method for the determination of individual enantiomers in biological samples. So the method can be used to perform stereoselective pharmacokinetic studies. © 1994 Wiley-Liss, Inc.