Ultraweak and induced photon emission after wounding of plants.

The ultraweak and induced photon emission were measured by a single photon counting equipment (Photomultiplier Hamamatsu R562) on Cucurbita pepo variaca styriacae after wounding. Wounding significantly changes the emission from a stationary to a nonstationary state and the shape of the decay curve obtained after light illumination. The rise in the ultraweak photon emission depends on the kind of wounding and its localization on the plant. The decay curves obtained after wounding could be better fit by an exponential function than by a hyperbolic one. So the biophoton emission correlates with physiological and bioelectrical changes like membrane depolarizations as they also depend on the kind of injury.

Treatment of the budding yeast Saccharomyces cerevisiae with the lipid peroxidation product 4-HNE provokes a temporary cell cycle arrest in G1 phase.

The effects of 4-hydroxy-2-nonenal (HNE) on the cell division cycle were investigated in the yeast Saccharomyces cerevisiae. A short treatment with HNE at a concentration in the range of the IC50 value in S. cerevisiae SP-4 cells induced a significant increase in the proportion of G0/G1 cells at the expense of S-phase cells. A similar delay in cell cycle progression upon treatment with HNE has recently been shown for HL-60 neoplastic cells. Long-term exposure in a synchronized yeast culture resulted in a pronounced dose-dependent block between G0G1- and S-phase, probably at or close to a point in the cell cycle that has been designated as "START." Incorporation of radioactively labeled precursors of macromolecules revealed that DNA synthesis was most susceptible to HNE in comparison to RNA and protein synthesis. Production of glutathione appeared to be required for the continuation of the cell cycle. HNE-treated yeast cells reentered the cell cycle when their glutathione content exceeded about twice the level of control cells. The release from the cell division cycle delay was followed by an enhanced growth to an extent that HNE-treated cells exceeded the number of control cells. These results indicate that HNE causes a biphasic modulation of cell proliferation. It was concluded that this effect was conserved during evolution from yeast to mammalian cells, emphasizing once more the usefulness of this unicellular organism as a model system for the investigation of the effects of free radical-derived products on the proliferation of eukaryotes.

Human low density lipoprotein as a target of hypochlorite generated by myeloperoxidase.

The aim of this study was to further clarify which part of human low density lipoprotein (LDL) is attacked by the MPO/H2O2/Cl- -system and which reactive oxygen species is responsible for the attack. Therefore the influence of this system on the modification of the lipid and protein moiety of LDL was studied in vitro. Using the monochlorodimedone assay it was found that HOCl is produced in micromolar quantities in the absence of LDL and is rapidly consumed by LDL in a concentration dependent manner. The consumption of HOCl was reflected in the formation of HOCl-specific epitopes on apo B-100 as determined by an antibody raised against HOCl-modified LDL. The absorbency at 234 nm was applied to measure continuously the extent of modification of LDL. The general kinetic pattern of the absorbency measurement consisted of a lag phase where no LDL modification was observed, followed by a rapid increase of absorbency and a plateau phase. Finally the absorbency decreased due to LDL precipitation. Time dependent absorption spectra indicated that this kinetic pattern is mainly caused by light scattering due to particle aggregation rather than by a specific absorption at 234 nm due to conjugated diene formation. In agreement with this finding a low rate of thiobarbituric acid reactive substances (TBArS) formation was observed after a lag phase. The aggregation of LDL occurs most likely by modification of apo B-100, which was determined fluorimetrically in terms of LDL-tryptophan destruction in presence of the MPO/H2O2/Cl(-)-system. The kinetic course of tryptophan fluorescence generally consisted of a rapid decrease leveling off into a low plateau phase. Gas chromatographic determinations of linoleic acid in LDL in presence of the MPO system showed that this polyunsaturated fatty acid (PUFA) is easily attacked by HOCl. Consistent with this finding NMR spectra of HOCl modified LDL indicated a complete disappearance of bis-allylic methylene groups. Since lipid peroxidation products only partially account for this loss of PUFAs, other reactions of HOCl with unsaturated lipids--probably chlorohydrin formation--must be involved. Summarizing, although the rate of lipid peroxidation is low, both the lipid and the protein moiety of LDL are readily modified by the MPO system. It appears that the immediate consequence of apo B-100 modification is its aggregation. It is concluded that MPO, which has been detected in atherosclerotic lesions, is able to contribute to the modification of LDL into a form recognizable for uncontrolled uptake by macrophages.

Physiology of young Norway spruce.

In the Hohenheim experiment young spruce (Picea abies L. Karst.) were exposed to low levels of SO(2) and/or O(3) and acid precipitation. At the end of a five-year experimental period (1983-88) the following physiological parameters were examined: water soluble thiols, ascorbic acid, glutathionereductase activity and pigment content. Exposure to SO(2), leads to an increase in thiol content, to a slight decrease of ascorbic acid and to a pronounced decrease of pigments. O(3) exposure increases the content of ascorbic acid and decreases the thiols and the glutathione-reductase activity with no change in the pigment content. The combined exposure to SO(2), and O(3) results in the most distinct deviations compared to the control chamber response. These needles show the highest increase of ascorbic acid and thiols, the dry weight is decreased as is the glutathione-reductase activity and the pigment content is reduced. Consequences of these physiological alterations for the plant's health are discussed.

A perfusion chamber with temperature regulation.

When investigating microscopic preparations perfusion chambers allow exchange and regulation of different solutions and ensure their constant flow in the sample chamber. Temperature deviations, however, may be problematic. We describe a new chamber that contains an additional circulation system which regulates the inside temperature using an external thermostat. An integrated thermometer probe records the sample temperature, which appears on a monitor. The glass chamber, measuring 75 x 35 x 3 mm, provides good optical quality and is compatible with every type of microscope.