Detection in situ of foreign DNA in eukaryotic cells

A simple technique is described that allows mixed populations of eukaryotic cells to be screened for clones containing multiple copies of a particular DNA. Essentially, eukaryotic cells are transferred to either nitrocellulose of Whatman 541 filters, and their DNA is immobilised in situ. Exposure of the filters to a 32P-labeled DNA "probe" results in detectable hybridisation only at the positions of clones containing multiple copies of the DNA. Using Whatman 541 paper, a portion of the cells, evenly distributed throughout the mixed population is retained on the culture dish, and can be propagated further for subsequent cell cloning. The technique has allowed rapid distinction of clones of transformed rat cells that contain a single or only a few copies per cell of polyoma viral DNA from clones maintaining multiple copies. The technique has also been used to distinguish between clones of mouse L-cells containing multiple and only a few copies of 0X174 DNA. In this manner the technique allows rapid detection of cells amplifying a particular species of DNA. Finally, the method can be used to detect cells assimilating many copies of a foreign DNA, even in the absence of a co-transfected selectable marker.     

Some observations on the ecology,metal uptake and nickel tolerance of Alyssum serpyllifolium subspecies from the Iberian peninsula

Experiments were carried out on the tolerance to, and uptake of, nickel by three iberian subspecies of Alyssum serpylliforium Desf. Two of these subspecies, the serpentine-endemic ssp. lusitanicum from Bragança, Portugal and ssp. malacitanum from Málaga, Spain, are hyperaccumulators (> 1000 g/g in dried material) of nickel. Their possible ancestor, ssp. serpyllifolium (from Granada, Spain) was a non-accumulator of this element. Seeds of the two serpentine-endemics germinated extensively in nickel concentrations up to 12 000 g/g (1.2%) whereas ssp. serpyllifolium only germinated in nickel concentrations below 60 g/ml. Tolerance tests involving measurement of new root lengths of excised seedlings placed in varying nickel concentrations, again showed much greater tolerance of the two serpentinophytes. In both series of experiments, the order of tolerance was: ssp. lusitanicum > ssp. malacitanum > ssp. serpyllifolium. In pot trials involving seedlings of ssp. malacitanum grown in mixtures containing varying amounts of calcium, magnesium, and nickel, the most important finding was that plants will tolerate higher nickel contents in the soil when excess calcium is added. This is achieved by lowering the uptake of nickel. There appeared to be some concomitant reduction in calcium uptake in the presence of nickel, and some increase in uptake of magnesium. The resultant lower calcium/magnesium ratio in the plant, though not symptomatic of a favourable condition for colonization of serpentine soils, probably results from a mechanism which renders nickel innocuous to the plant at the expense of calcium uptake. It is suggested that the physiological characters of ssp. lusitanicum and ssp malacitanum are sufficiently different to support arguments for promoting the latter to full specific rank as has now been done for ssp. lusitanicum.     

Accumulation of exogenous catecholamines in the neural tube and non-neural tissues of the early fowl embryo

Summary Catecholamines (CA) were localized in stage 11–34 domestic fowl embryos by the formaldehyde-induced fluorescence (FIF) method after exposure in vivo or in vitro to CA (noradrenaline or -methylnoradrenaline), or the CA precursorl-DOPA. The effects of drugs known to alter CA metabolism in the adult were also investigated.Negligible FIF was observed in embryos which had not been exposed to CA. After CA loading, FIF could be seen in the neural tube and in non-neural tissues such as the notochord and gut mesenchyme and to a lesser degree in suprarenal area tissue, liver endothelium, sclerotome, and myotome. This FIF was inhibited by desmethylimipramine, a blocker of adult neuronal CA uptake (Uptake₁), but not by corticosterone, a blocker of adult extraneuronal CA uptake (Uptake₂). The notochord, dorsal pancreas and some blood cells were fluorescent afterl-DOPA loading, and this FIF could be greatly diminished by the DOPA decarboxylase inhibitor RO4-4602.The pattern of FIF in the axial structures (neural tube and notochord) correlated with axial flexure in both position and time, and the intensity of fluorescence was strongest cranially and caudally, where flexure is most pronounced. The FIF in gut mesenchyme cells was closely related to the movement of the intestinal protals during early gut tube formation, and to the regions of the developing intestine that undergo intense morphogenesis during their early formation.     

Isolation of recombinant proteins from milk.

Milk is a complex bio-colloid which presents some unique problems for the protein isolation chemist, but the majority of the processing criteria for purifying recombinant proteins are the same as with any complex biological mixture. The casein micelles and fat globules behave as separate phases; they prevent filtration of the milk and interfere with the usual separation methods. The usual first step is to centrifuge the milk to remove the fat and precipitate the casein micelles with low pH or precipitating agents. Some recombinant proteins may associate to some degree with the micelles which may necessitate solubilizing them with chelating agents. If the majority of the product protein associates with either the fat or micelles, this can be used to advantage. Once the casein micelles have been removed or disrupted, the clarified milk can be processed by the usual separation methods. There also are proteases in milk which can degrade recombinant proteins. The greatest advantage of producing recombinant proteins in milk is the high concentration which can be obtained. The high levels of product protein can alleviate many problems associated with the application of classical purification strategies to transgenic milk proteins.     

Biosynthesis and metabolic roles of cadystins (γ-EC)nG and their precursors in Datura innoxia

Metal-tolerant Datura innoxia cells synthesize large amounts of cadystin, [poly(-glutamylcysteinyl) glycines, (-EC)_nG, n=2–5], a class of metal-binding polypeptides, when exposed to Cd. These polypeptides have a high affinity for Cd (II) and certain other metal ions and are thought to play a role in metal tolerance in higher plants. Cells rapidly synthesize these metal-binding polypeptides when exposed to Cd and cellular concentrations of glutathione and cysteine, precursors for the synthesis of these compounds, are initially depleted then rapidly replenished. The time-frame of de novo polypeptide, glutathione and cysteine biosynthesis suggests that this pathway is, at least initially, regulated at the enzyme level. Significant amounts of Fe are associated with Cd: polypeptide complexes isolated from D. innoxia. Exposure of cultures to Cd results in an increased Fe accumulation by the cells. All the additional Fe found in the soluble portion of cell extracts is associated with the Cd: polypeptide complexes. The physiological significance of the synthesis of these polypeptides and their precursors and its relevance to Cd tolerance and metal homeostasis are discussed.     

Soil solute concentration and water uptake by single lupin and radish plant roots

Application of computer assisted tomography to gamma and X-ray attenuation measurements and Na⁺-LIX microelectrodes were used to determine the spatial distributions of soil water content and Na⁺ concentrations respectively near single roots of eighteen day old lupin and radish plants. These quantities were monitored at root depths of 3, 6 and 9 cm and at zero, 2, 4, 6, and 8 hour intervals from the diurnal commencement of transpiration. The plants were subjected to two levels of transpirational demand and five Na⁺ soil solution concentration levels. Water extraction rates for the lupin and radish roots increased continuously with time but were substantially reduced with increasing Na⁺ concentration in the treatment. Water uptake was uniform along the length of the essentially constant diameter lupin roots but decreased along the tapering radish roots as the diameter and hence the surface area per unit length of the roots decreased. The accumulation of Na⁺ at the root surfaces of both plants increased gradually with time in a near linear fashion and was slightly higher under the higher transpiration demand. These increases were not exponential as would be expected with non-absorption by the roots and this is considered to be due to back diffusion at the relatively high water contents used. At these water contents matric potentials had a much smaller influence on transpiration than osmotic potentials. The relationships between leaf water potentials (Ψ₁) and osmotic potentials at the root surfaces were linear with the decreases in Ψ₁ almost exactly reflecting the decreases in Ψ_π indicating rapid plant adjustment. Leaf water potentials decreased progressively with time and the relationships between leaf water potential and the transpiration rate were also linear supporting the suggestion of constant plant resistances at any given concentration.     

Lead-210 dating of sediments compared with accumulation rates estimated by natural markers and measured with sediment traps

Methods to provide accurate accumulation rates for lake models are discussed. Cores were taken in 1979 in two basins of Lake Lucerne, Switzerland, and accumulation rates were calculated by using Pb-210 dating and by a natural landslide marker of 1795 in one basin (Weggis). In the other basin (Horw Bay) the sediment accumulation rates based on the lead method were compared with yearly sedimentation rates measured by sediment traps in 1969/70. At the Weggis station, the core dating yielded sediment accumulation rates of about 400 g dry wt. m^–2 y^–1 with the lead method, averaged over a sediment depth of 4–20 cm; accumulation was about 700 g dry wt. m^–2 y^–1 with the marker method, averaged over 0–33 cm. In Horw Bay, the trap method yielded about 1300 g dry wt. M^–2 y^–1 compared with 400–1000 g dry wt. m^–2 y^–1 obtained with the lead method and related to various depth intervals. The characteristic sources of error of the three methods as well as several hypotheses for these discrepancies are discussed.     

Conditioning prepulses and kinetics of potassium conductance in the frog node

Summary The kinetics of potassium conductance were analyzed in response to voltage-clamp steps with holding potential (–75 mV) as initial condition and after a positive prepulse to-wards +45 mV of 10-msec duration. As the potassium reversal potentialE _K altered during potassium current flow, a method to obtain the conductance independent ofE _K was used. Conductance kinetics at 15°C were analyzed according to the Hodgkin-Huxley (HH) model. The time constant of potassium activation, with holding potential as initial condition, is a monotonous decreasing function of membrane potential. Its value ofca. 9 msec at –50 mV decreases to 1 msec at +30 mV. Changes inE _K did not affect the voltage dependency of this time constant. The time constant of potassium deactivation, i.e. the off-response following a 10-msec prepulse towards +45 mV, shows a completely different voltage dependency. At a membrane potential of –90 mV it is approximately 2 msec and gradually increases for more positive voltages towards a maximum value of about 6 msec, that is reached between –5 and 0 mV. At still larger values of membrane voltage this time constant starts to fall again. It is concluded that a HH-model, as applied for a single population of potassium channels, has to be rejected. Computer simulations indicate that an extension to two populations of independent potassium channels, each with HH-kinetics, is also inconsistent with the observed results.     

Effect of 2-chloroethylphosphonic acid on capsule formation and alkaloid content in Papaver somniferum

Application of different concentrations of ethephon (2-chloroethylphosphonic acid) to Papaver somniferum L. at the times of stem elongation, bud, and capsule formation produced different effects. Ethephon (10^-2 M ) retarded growth of the plant and inhibited capsule formation during stem elongation, significantly reduced capsule size during the flowering period, but did not alter capsule development during capsule formation. When applied during the period of stem elongation, ethephon (10^-3 M and 10^-4 M ) reduced capsule size; alkaloid accumulation was reduced by ethephon at a concentration of 10^-3 M , but slightly increased by 10^-4 M . Ethephon (10^-3 M and 10^-4 M ) did not alter capsule development or alkaloid content significantly when applied during bud formation, but stimulated capsule size and alkaloid content when applied during capsule formation. Pretreating the plants with Ag⁺ (silver nitrate) did not reverse the ethephon effect. The results suggest that capsule maturation and alkaloid accumulation in P. somniferum are modified by ethylene, which is produced as a result of exogenous ethephon treatment.     

Effects of accumulation of 3-O-methylglucose on growth and osmotic regulation in Chlorella emersonii

Abstract. The effect of accumulation of 3- O -methylglucose (MG) on growth and steady-stale concentrations of the endogenous osmotic solutes proline and sucrose was studied in Chlorella emersonii grown at external osmotic pressure (II) of 0.08-1.64 MPa. NaCL was used as osmoticum. The total solute content of the cells was manipulated by supplying 2 mol m⁻³ MG for 4 and 48 h. MG accumulated to 50–230 mol m⁻³ within 4h and was not metabolized. Uptake of MG resulted in decreases in concentrations of proline and sucrose, the two solutes mainly responsible for osmotic adaptation of C. emersonii to high II. After 4 or 48 h growth in the presence of MG, the decreases in concentration of proline and sucrose were as predicted from the contribution of MG to the total solute content of the cell.