Intraspecific variation in the lens proteins

A review of the literature indicates that intraspecific variation among the lens proteins (crystallins) is almost invariably quantitative rather than qualitative. Lens extracts were examined from inbred strains of the laboratory mouse, rat, and guinea pig and from domestic breeds of sheep. Differences in the mobilities of protein bands after electrophoresis in polyacrylamide gels were never found to be greater than the variation observed when a sample was repeatedly subjected to electrophoresis. Differences, however, were observed between widely separated populations of the bank vole (Clethrionomys glareolus). In bank voles and mice, there were variations in the intensities of bands. Electrophoresis of extracts in the presence of 6 m urea indicated that there were no major differences between six mouse strains in the subunits constituting their - and -crystallins. More detailed examination of -crystallins from two mouse strains by isoelectric focusing and amino acid analysis supported this conclusion.This work was carried out while one of the authors (T.H.D.) was supported by a Medical Research Council Research Studentship and a European Molecular Biology Organisation Fellowship. A grant from the Edinburgh University Weir Memorial Fund allowed the collection of some of the Yugoslavian bank voles.     

Recovery of Colony-Forming Ability and Genetic Marker Activity by UV-Damaged Hemophilus influenzae

The rate of recovery of UV-irradiated Hemophilus influenzae from acriflavine-sensitized loss of colony-forming ability was studied at various acriflavine concentrations, UV doses, and temperatures. This rate (as calculated from an equation based upon certain assumptions) was on the order of 0.07 per minute per cell at 37°C. This did not vary greatly with UV dose or acriflavine concentration, but did with temperature, giving a ΔH‡ of about 16 kcal/mole. In another set of experiments, cells bearing two genetic markers (resistance to 2000 μg/ml streptomycin and to 2.5 μg/ml novobiocin) were irradiated and then incubated without acriflavine. DNA extracts made from samples taken after various periods of incubation time were assayed on antibiotic-sensitive cells using acriflavine to inhibit repair during and following transformation. It was found that both in vivo irradiated markers were reactivated in the donor to approximately the same extent (with a rate constant of 0.04 per minute). This result was in contrast to the results obtained when extracted DNA bearing the same markers was irradiated in vitro and used to transform cells. In this latter case the streptomycin marker was much more sensitive than the novobiocin marker. This difference is interpreted as being due to the mechanics of the transformation system.     

Identification of hair and feather remains in the gut and faeces of stoats and weasels

Qualitative analysis of the gut and faeces contents of stoates and weasels is complicated by the lack of readily identifiable bone fragments, teeth, feathers, etc., of mammalian or avian prey. Often the only evidence of such prey was hair or feather fragments. Since the bulk of food taken by stoats and weasels was from these two food classes, the problem of qualitative analysis resolved itself into that of identifying these hair and feather fragments.
By using the scale pattern, cross-section and medulla type, it was possible to construct a key which would identify guard hairs of small mammals of the generic level. Feather identification was based on the structural variations to the down barbules of coverts. Using such criteria a key to the main bird orders was devised.