Flow cytometric measurement of pollutant stresses on algal cells

Flow cytometric measurement of pollutant stresses on algal cells

The lichen Usnea fulvoreagens (Räs.) Räs. was treated with four pH levels (5.5, 4.5, 3.5, and 2.5) of simulated acid rain (sulfuric acid, nitric acid, and a 1:1 combination of both) and automobile exhaust. The samples were dissociated and analyzed by a Becton‐Dickin‐son FACS 440 flow cytometer. Anal...

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Veröffentlicht in:Cytometry (Baltimore); (United States) 1988-03, Vol.9 (2), p.150-155
Hauptverfasser: Berglund, Deborah L., Eversman, Sharon
Format: Artikel
Sprache:eng
Schlagworte:
560300 - Chemicals Metabolism & Toxicology
ACID RAIN
AIR POLLUTION
ALGAE
Animal, plant and microbial ecology
Applied ecology
ATMOSPHERIC PRECIPITATIONS
AUTOMOBILES
Biological and medical sciences
BIOLOGICAL INDICATORS
BIOLOGICAL STRESS
calcofluor white M2R
CELL CONSTITUENTS
CELL FLOW SYSTEMS
CELL MEMBRANES
Cell Separation
Chemical Precipitation
Ecotoxicology, biological effects of pollution
Environmental Pollutants - adverse effects
ENZYME ACTIVITY
ENZYMES
ESTERASES
Eukaryota - cytology
EXHAUST GASES
Flow cytometry
Flow Cytometry - methods
FLUIDS
fluorescein diacetate
Fluoresceins
FLUORESCENCE
Fundamental and applied biological sciences. Psychology
FUNGI
GASEOUS WASTES
GASES
HYDROLASES
lichen
LICHENS
Lichens - cytology
LUMINESCENCE
MEMBRANES
PERMEABILITY
PLANTS
pollutants
POLLUTION
RADIATION, THERMAL, AND OTHER ENVIRON. POLLUTANT EFFECTS ON LIVING ORGS. AND BIOL. MAT
RAIN
SIMULATION
Staining and Labeling - methods
Terrestrial environment, soil, air
TOXICITY
Usnea fulvoreagens
Vehicle Emissions - adverse effects
VEHICLES
WASTES
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Zusammenfassung:The lichen Usnea fulvoreagens (Räs.) Räs. was treated with four pH levels (5.5, 4.5, 3.5, and 2.5) of simulated acid rain (sulfuric acid, nitric acid, and a 1:1 combination of both) and automobile exhaust. The samples were dissociated and analyzed by a Becton‐Dickin‐son FACS 440 flow cytometer. Analyses included measurement of chlorophyll autofluorescence and fluorescence due to uptake of fluorescein diacetate (FDA) and calcofluor white M2R (CFW). Cell parameters measured were esterase activity (FDA), membrane permeability (FDA, CFW), and intracellular pH (FDA). Mean fluorescence intensity from FDA staining and numbers of events were incorporated with autofluorescence information to produce a “stress index” of relative cell stress. Results indicated that highly stressed samples (lower pH treatments and greater exposure to exhaust) exhibited a low “stress index” of FDA fluorescence.
ISSN:0196-4763
1097-0320
DOI:10.1002/cyto.990090209