Spelling suggestions: "subject:"boxicity testing - In vitro"" "subject:"bioxicity testing - In vitro""
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Development of in vitro toxicity methods for fire combustion productsLestari, Fatma, Safety Science, Faculty of Science, UNSW January 2006 (has links)
A large range of polymers are used in building and mass transport interiors which released more toxic products during combustion. This work explores the cytotoxicity of selected chemicals and smoke derived from materials combustion. A selection of polymers and fiberglass reinforced polymer (FRP) composites used in building and railway carriage interiors including: polyethylene (PE), polypropylene (PP), polycarbonate (PC), polymethyl methacrylate (PMMA), polyvinyl chloride (PVC), melamine plywood, and two FRPs were studied. A small scale laboratory fire test using a vertical tube furnace was designed for the generation of combustion products. The volatile organic compounds were identified using ATD-GCMS (Automatic Thermal Desorption-Gas Chromatography Mass Spectrometry). The in vitro techniques were developed for human cells exposure to fire effluents including the indirect (impinger) and direct (air/liquid interface using Harvard Navicyte Chamber) exposure. Cytotoxic effects were assessed based on cell viability using a range of in vitro assays. Human skin tissue was also used as preliminary study to assess the toxic effects at the tissue level. A minor change in the cellular function of the skin from the exposure of PMMA combustion products was observed. The combustion study was conducted under different burning stage of fire: non-flaming and flaming combustion. Results suggested that PVC was the most toxic material for both non-flaming (IC50 1.24 mg/L) and flaming combustion (IC50 1.99 mg/L). The degree of toxicity generated depends on the fire stage: non-flaming or flaming combustion. Some materials revealed to be more toxic under flaming combustion (PP, PC, FRPs), whilst others (PVC, PMMA, PE, and melamine plywood) appear to be more toxic under non-flaming combustion. A strong correlation was shown between the change in toxicity as measured by IC50 and TLC and the change in concentration of volatile organic compounds (VOCs) and particulates. A comparison between in vitro data versus published in vivo combustion data indicated the in vitro results to be more sensitive than animal toxicity data. The outcome of this study has the potential for an alternative method to current fire toxicity standard, whilst providing more accurate toxicity information for fire safety professionals, materials manufacturer, building designers and consumer safety data.
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Development of a novel, rapid, in vitro assay for the detection of Clostridium botulinum neurotoxin type ECadieux, Brigitte. January 2001 (has links)
Botulism is a foodborne intoxication caused by ingestion of Clostridium botulinum neurotoxin (BoNT). Preliminary studies focussed on the production of polyclonal antisera against BoNT/E by immunizing a rabbit with botulinal toxoid type E. The antiserum was subsequently used to detect BoNT/E using the slot blot immunoassay where samples were applied to a slot blot filtration manifold and drawn by vacuum through a membrane. The membrane was then immunologically processed before chemiluminescent detection. However, the antisera lacked specificity and cross-reacted with closely related clostridia strains. / The specificity of the antisera was increased by adsorbing cross-reactive antibodies from whole antisera with affinity columns made with total proteins from culture supernatants of closely related clostridia. Alternatively, specific antibodies were isolated with an affinity column prepared with C. botulinum type E toxoid. / Different methods of concentrating BoNT/E in each sample prior to testing them were evaluated to increase the sensitivity of the assay. / The slot blot immunoassay was then evaluated for detection of BoNT/E in mixed cultures and in food samples. (Abstract shortened by UMI.)
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Development of a novel, rapid, in vitro assay for the detection of Clostridium botulinum neurotoxin type ECadieux, Brigitte. January 2001 (has links)
No description available.
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In vitro toxicity testing of phthalocyanines on different cell lines using a continuous laser sourceMaduray, Kaminee January 2010 (has links)
Submitted in fulfilment of the requirements of the Degree of Master of Technology: Biotechnology, Durban University of Technology, 2010. / Photodynamic therapy is a promising treatment for cancer. It involves the
combination of a photosensitizer and light of an appropriate wavelength (laser source)
to cause the destruction of cancer cells. Phthalocynanines are second–generation
photosensitizers with enhanced photophysical and photochemical properties.
In this in vitro study the effect of aluminium (AlTSPc) or zinc (ZnTSPc)
tetrasulfophthalocyanines in its inactive and active state (laser induced) on melanoma
(skin cancer cells), fibroblast (healthy normal skin cells) and keratinocyte (healthy
normal skin cells) cells was evaluated. For each of the cell lines approximately
3 x 104 cells/ml were seeded onto 24-well cell culture plates and allowed to attach
overnight, after which cells were treated with different concentrations of AlTSPc or
ZnTSPc. The photosensitizers were synthesized at Rhodes University. After 2 hrs,
cells were irradiated with a diode laser at a wavelength of 672 nm and a beam
diameter of 1 cm. The laser power varied between 20-30 mW and the irradiation time
was calculated to deliver a light dose of 4.5 J/cm2. Post-irradiated cells were
incubated for 24 hrs before cell viability was measured using the CellTiter-BlueTM
Viability Assay.
Also, the efficacy of the light dose and laser source used for the killing of
approximately 50% of the melanoma cancer cells were investigated. AlTSPc and
ZnTSPc decreased cell viability of melanoma cancer cells to approximately 50% with
photosensitizer concentrations of 40 μg/ml and 50 μg/ml respectively. These
photosensitizer concentrations caused a slight decrease in the percentage cell viability
of fibroblast and keratinocyte cells. Results for the dark toxicity assay showed that
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both photosensitizers in the presence of high concentrations (60 μg/ml – 100 μg/ml)
showed cytotoxicity effects on melanoma cancer cells in their inactive state. This was
not observed in fibroblast and keratinocyte cells treated under the same experimental
conditions. The optimal AlTSPc and ZnTSPc concentrations in combination with the
light dose of 4.5 J/cm2 was the most efficient in killing the melanoma cancer cells
with reduced killing effects on healthy normal fibroblast and keratinocyte cells when
compared to other light doses (2.5 J/cm2, 7.5 J/cm2 and 10 J/cm2).
The irradiation of cells photosensitized with the optimal photosensitizer
concentrations with a femtosecond laser using similar laser parameters to continuous
wave laser experiments resulted in a reduction in the cell viability of healthy normal
fibroblast and keratinocyte cells compared to melanoma cancer cells. The presence of
DNA degradation on agarose gel, morphological changes like blebbing and
ultrastructural changes like nucleus condensation indicated that photodynamic therapy
treated melanoma cancer cells with the optimal concentrations of AlTSPc and
ZnTSPc induced cell death via apoptosis. This concludes that low concentrations of
AlTSPc and ZnTSPc activated with an appropriate laser source can be used to induce
cell death in melanoma cancer cells. Both AlTSPc and ZnTSPc exhibit the potential to
be used as a photosensitizer in photodynamic therapy for the treatment of melanoma
cancer with the occurrence of minimal damage to surrounding healthy tissue.
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Investigations into mechanisms of paracetamol-induced toxicity using ìn vitro' systemsBruschi, Sam A. (Sam Anthony) January 1987 (has links) (PDF)
Bibliography: leaves 116-138.
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Development of comparitive methods for chemical analysis and in vitro cytotoxicity testing of contaminated sitesManglik, Aparna, Safety Science, Faculty of Science, UNSW January 2006 (has links)
This project developed methodology for in vitro toxicity assessment of contaminated sites using the Promega?? MTS [3-(4,5-dimethylthiazol-2-yl)-5-(3-carboxy-methoxyphenyl)-2-(4-sulfophenyl)-2H-tetrazolium] assay performed on human cells (HepG2 and Skin fibroblasts). The project included the development of a method for extracting contaminants from soil based on leaching and centrifugation. A number of solvents and surfactants were assessed for their suitability as extracting agents. The Zwitterionic surfactant CHAPS ({3[(3-Cholamidopropyl) dimethylammonio] propanesulphonic acid}), which is an irritant in vivo, was found suitable for in vitro toxicity assessment applications. CHAPS was found to be the least toxic surfactant in vitro when tested on skin fibroblasts (NOEC: 1800??577 ppm, IC50: 4000??577 ppm) and HepG2 cells (NOEC: 833??289 ppm, IC50: 5300??287 ppm). The chosen surfactant was used in three different methods for extraction of Toluene and Xylene spiked in 2 g and 10g soil. The combination comprising of 0.1% (s/w) CHAPS and cosolvent 1% (w/w) Isopropanol, at their respective NOEC (No Observed Effective Concentration) toxicity values, showed good recovery of the nonpolar organic compounds in comparison to the recovery by 0.1% CHAPS and 0.5% CHAPS. The study found additive interactions to be the most common form of toxicity for 16 concentration combinations of Formaldehyde (polar), Toluene and Xylene (nonpolar) when compared to predicted toxicity (R2=0.943, P<0.0001). When assessing the in vitro toxicity of unknown (blind) contaminated soil samples, the Hazard Index (HI) predicted from the chemical analyses results showed a relatively good correlation (R2>0.7062, n=26) when compared to the experimental toxicity results on HepG2 cells. Furthermore, the comparison of Australian Health Investigation Levels (HIL) with in vitro toxicity testing gave similar correlation (R2>0.6882, n=26) on HepG2 cells. The overall project suggests the potential application of the zwitterionic surfactant (CHAPS) in sampling contaminants from soils in an in vitro toxicity assessment. This study demonstrates the application of in vitro toxicity assessment using human cells for the prediction of toxic risk as a sentinel to human toxicity from a contaminated site.
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Development of comparitive methods for chemical analysis and in vitro cytotoxicity testing of contaminated sitesManglik, Aparna, Safety Science, Faculty of Science, UNSW January 2006 (has links)
This project developed methodology for in vitro toxicity assessment of contaminated sites using the Promega?? MTS [3-(4,5-dimethylthiazol-2-yl)-5-(3-carboxy-methoxyphenyl)-2-(4-sulfophenyl)-2H-tetrazolium] assay performed on human cells (HepG2 and Skin fibroblasts). The project included the development of a method for extracting contaminants from soil based on leaching and centrifugation. A number of solvents and surfactants were assessed for their suitability as extracting agents. The Zwitterionic surfactant CHAPS ({3[(3-Cholamidopropyl) dimethylammonio] propanesulphonic acid}), which is an irritant in vivo, was found suitable for in vitro toxicity assessment applications. CHAPS was found to be the least toxic surfactant in vitro when tested on skin fibroblasts (NOEC: 1800??577 ppm, IC50: 4000??577 ppm) and HepG2 cells (NOEC: 833??289 ppm, IC50: 5300??287 ppm). The chosen surfactant was used in three different methods for extraction of Toluene and Xylene spiked in 2 g and 10g soil. The combination comprising of 0.1% (s/w) CHAPS and cosolvent 1% (w/w) Isopropanol, at their respective NOEC (No Observed Effective Concentration) toxicity values, showed good recovery of the nonpolar organic compounds in comparison to the recovery by 0.1% CHAPS and 0.5% CHAPS. The study found additive interactions to be the most common form of toxicity for 16 concentration combinations of Formaldehyde (polar), Toluene and Xylene (nonpolar) when compared to predicted toxicity (R2=0.943, P<0.0001). When assessing the in vitro toxicity of unknown (blind) contaminated soil samples, the Hazard Index (HI) predicted from the chemical analyses results showed a relatively good correlation (R2>0.7062, n=26) when compared to the experimental toxicity results on HepG2 cells. Furthermore, the comparison of Australian Health Investigation Levels (HIL) with in vitro toxicity testing gave similar correlation (R2>0.6882, n=26) on HepG2 cells. The overall project suggests the potential application of the zwitterionic surfactant (CHAPS) in sampling contaminants from soils in an in vitro toxicity assessment. This study demonstrates the application of in vitro toxicity assessment using human cells for the prediction of toxic risk as a sentinel to human toxicity from a contaminated site.
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The effect of short-term pretreatment with peroxisome proliferators on the acute toxicity of various toxicants, including paracetamol / Felicity April Nicholls-Grzemski.Nicholls-Grzemski, Felicity April January 1998 (has links)
Erratum tipped in before chapter 1. / Bibliography: leaves 226-248. / xv, 248 leaves : ill. (chiefly col.) ; 30 cm. / Title page, contents and abstract only. The complete thesis in print form is available from the University Library. / Shows that pretreatment with peroxisome proliferators protects mice against the acute hepatotoxicity of paracetamol, in addition to a number of other toxicants. / Thesis (Ph.D.)--University of Adelaide, Dept. of Clinical and Experimental Pharmacology, 1999
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A pharmacological characterisation of death adder (Acanthophis Spp.) venoms and toxinsWickramaratna, Janith C. January 2003 (has links)
Abstract not available
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Development of in vitro methods for toxicity assessment of workplace air contaminantsBakand, Shahnaz, Safety Science, Faculty of Science, UNSW January 2006 (has links)
Exposure to air contaminants is significantly associated with both short-term and long-term health effects. However, the precise mechanisms that derive such effects are not always understood. While an extensive background database from in vivo toxicological studies have been developed, most toxicity data is from oral and dermal chemical exposures rather than inhalation exposure. There is a need to explore new alternative approaches to provide toxicity information particularly on this technically demanding area. This research explores the potential of in vitro methods for toxicity assessment of workplace air contaminants. A tiered approach for in vitro toxicity testing of workplace contaminants was designed in which appropriate air sampling and exposure techniques were developed. A diversified battery of in vitro assays including the MTS (tetrazolium salt, Promega), NRU (neutral red uptake, Sigma) and ATP (adenosine triphosphate, Promega) and a multiple human cell system including: A549- lung derived cells; HepG2-liver derived cells, and skin fibroblasts were used. Primarily the application and merits of in vitro methods for prediction of toxicity of selected workplace contaminants including Ammonium hydroxide, Cadmium chloride, Cobalt chloride, Formaldehyde, Glutaraldehyde, Manganese chloride, Mercuric chloride, Sodium dichromate, Sulphureous acid and Zinc chloride was confirmed. To study the toxicity of airborne contaminants an indirect exposure method was established using air sampling techniques followed by static and dynamic direct exposure methods by culturing cells on porous membranes to reveal representative data relating to human airborne exposures. The static method enabled the measurement of an airborne IC50 (50% inhibitory concentration) value for selected volatile organic compounds (VOCs) including: Xylene (IC50 = 5,350-8,200 ppm) and Toluene (IC50 = 10,500- 16,600 ppm) after 1 hr exposure. By implementing the dynamic method, airborne IC50 values were calculated for gaseous contaminants including: NO2 (IC50 = 11 ?? 3.54 ppm; NRU), SO2 (IC50 = 48 ?? 2.83 ppm; ATP) and NH3 (IC50 = 199 ?? 1.41 ppm; MTS). A higher sensitivity of in vitro methods was observed compared to in vivo published data. A range of in vitro bioassays in conjunction with exposure techniques developed in this thesis may provide an advanced technology for a comprehensive risk assessment of workplace air contaminants.
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