Theiler's murine encephalomyelitis virus group includes two distinct genetic subgroups that differ pathologically and biologically.

The intracellular development and RNA composition of Theiler's murine encephalomyelitis virus (TMEV) isolates were determined by electron microscopy, sucrose gradient centrifugation, and RNase T1 fingerprinting. Replication of FA virus, a virulent strain of TMEV, was characterized by the appearance of viral crystalline arrays in the cytoplasm of infected cells. In contrast, cells infected with the less virulent isolates (WW, TO4, BeAn 8386, and Yale) showed no crystalline arrays; instead, virions were found to be arranged between two layers of membranes in the cytoplasm of infected cells. Analysis of the RNAs of TMEV isolates showed that the RNAs were single-stranded molecules having sedimentation coefficients of 35S. RNase T1 fingerprinting of TMEV RNA revealed that striking differences between the virulent and less virulent TMEV isolates existed. Moreover, base composition analysis of RNase T1-resistant oligonucleotides of two TMEV isolates which represented the two subgroups indicated that there were no substantial oligonucleotides common to both subgroups. Based on these findings and the known difference in virulence, we suggest that the TMEV group contains two genetically district subgroups of viruses.     

Elevated recombination and pairing structures during meiotic arrest in yeast of the nuclear division mutant cdc5

Summary A diploid strain of yeast, homozygous for the mutation cdc5-1, undergoes a normal meiosis at 25° C. At the nonpermissive temperature of 34° C, meiosis is arrested at the first meiotic division, after premeiotic DNA replication and recombination commitment have taken place. Haploidisation commitment does not occur at 34° C. Electron microscopy reveals that synaptons (synaptonemal complexes) are formed and the stage of arrest is characterised by a prevalence of modified synaptons, which consist of paired lateral elements lacking the central elements. Prolonged incubation at this stage of arrest results in unusually high recombination levels, perhaps related to the synaptonal structures observed.Temperature shift-up experiments (transfers of cells from 25° C to 34° C at various times during meiosis) reveal that the CDC5 function is required for both the first and the second divisions of meiosis.     

Concepts and strategies for human gene therapy.

Methods of modern molecular genetics have been developed that allow stable transfer and expression of foreign DNA sequences in human and other mammalian somatic cells. It is therefore no surprise that the methods have been applied in attempts to complement genetic defects and correct disease phenotypes. Two decades of research have now led to the first clinically applicable attempts to introduce genetically modified cells into human beings to cure diseases caused at least partially by genetic defects. We discuss here some of the strategies being followed for both in vitro and in vivo application of therapeutic gene transfer and summarize some of the technical and conceptual difficulties associated with somatic-cell gene therapy.     

Pseudotype formation of murine leukemia virus with the G protein of vesicular stomatitis virus.

Mixed infection of a cell by vesicular stomatitis virus (VSV) and retroviruses results in the production of progeny virions bearing the genome of one virus encapsidated by the envelope proteins of the other. The mechanism for the phenomenon of pseudotype formation is not clear, although specific recognition of a viral envelope protein by the nucleocapsid of an unrelated virus is presumably involved. In this study, we used Moloney murine leukemia virus (MoMLV)-based retroviral vectors encoding the gene for neomycin phosphotransferase to investigate the interaction between the VSV G protein and the retroviral nucleocapsid during the formation of MoMLV(VSV) pseudotypes. Our results show that VSV G protein can be incorporated into the virions of retrovirus in the absence of other VSV-encoded proteins or of retroviral envelope protein. Infection of hamster cells by MoMLV(VSV) pseudotypes gave rise to neomycin phosphotransferase-resistant colonies, and addition of anti-VSV serum to the virus preparations completely abolished the infectivity of MoMLV(VSV) pseudotypes. It should be possible to use existing mutants of VSV G protein in the system described here to identify the signals that are important for the formation of MoMLV(VSV) pseudotypes.     

The cryptoendolithic microbial environment in the Ross Desert of Antarctica: Satellite-transmitted continuous nanoclimate data, 1984 to 1986

Summary A satellite mediated station for monitoring nanoclimate (climate in the millimeter range) data, suitable for use in polar regions is described. The station, located in the Ross desert of Antarctica, has been in operation for more than 3 years, measuring rock temperatures, air temperature, light, snow, wind, and moisture. The data indicate that biological activity in the cryptoendolithic microbial ecosystem is limited to the period from mid November to mid February. The total number of hours of biological activity, based on assumptions of the minimum light, temperature and moisture requirements of the community, is less than 1000 h/year. The time above 0°C, representing more nearly optimal conditions, is between 50 and 550 h/year, depending on the orientation of the surface.Ross desert is an unofficial name for the ice-free region between 160° and 164°E and 76°30 and 78°30S. This area is more generally referred to as the dry valleys     

Die Balz vonSemioptera wallacei halmaherae in Gefangenschaft

Ohne ZusammenfassungAus dem englischen Manuskript übersetzt vonJ. Plathner.     

Reverse-phase purification and silica gel thin-layer chromatography of porphyrin carboxylic acids

Thin-layer chromatography on silica gel 60 plates in the solvent N,N-dimethylformamide/methanol/ethylene glycol/glacial acetic acid/1-chlorobutane/chloroform (4/35/6/0.4/18/20 by volume) separates porphyrin carboxylic acids by the number of free carboxyl groups. Coproporphyrins I and III and isocoproporphyrin are separated in 30 min, other porphyrins in 15 min. The N,N-dimethylformamide and acetic acid in the solvent strongly increase porphyrin fluorescence on the plates. Fading and diffusion of the fluorescent patterns is prevented by storage of the plates in the cold and dark without oxygen and with desiccant. In a preliminary step, porphyrins are purified in high yields, concentrated, and deacidified rapidly (2 min) by reversephase chromatography on cartridges containing a C₁₈ spacer or on Amberlite XAD-2 columns. The methods are applied to urines of porphyria patients and for following porphyrin ester hydrolysis.