SBIR-STTR Award

The long-term objective of this project is to develop a laboratory test for monitoring low-level toxicity from chemical exposure at levels that do not produce acute symptoms such as cytotoxicity, butproduce detectable damage later. The specific aims for this Phase I investigations are to:(1)determine the subcytotoxic levels of three enviromental agents-a myotoxin, a polycyclic hydrocarbon, and an aromatic amine;(2) set up a fairly long-term(3 to 4 months) bioassay using a well-characterized rat liver epithelial cell line, exposed chronically to the above subcytotoxic doses of carcinogens; and(3)monitor the emergence of a population of cells containing mutated ras oncogene using molecular biological endpoints.The technical innovations in these studies include polymerase chain reaction amplification of low levels of chemically induced mutations in an oncogene from mammalian cells and their measurement and detection with a liquid hybridization/gel retardation assay.Awardee's statement of the potential commercial applications of the research:The direct outcome of this project is the development of an in vitro assay for genotoxic chemicals that activate oncogenes at very low doses. A by-product of this study could be the monitoring of populations at risk of developing cancer by the ultrasensitive assay of DNA isolated from peripheral blood lymphocytes.National Institute of Environmental Health Sciences (NIEHS)

The long-term objective is to establish screening systems for chemicals that produce mutations in important regulatory DNA sequences of mammalian cells at low levels of exposure. During the Phase I study, we will demonstrate the ability of different classes of toxic chemicals to induce mutations in ras proto-oncogenes in rat liver epithelial cell cultures, a well-established model for carcinogenesis was documented. The specific objectives for Phase 11 include 1) adaptation of the liver cell model for quantitative measurement of mutated ras proto-oncogenes, and refinement of the PCR technology for error-free amplification of the oncogene, 2) determination of the temporal relationship between mutations of ras gene in rat liver epithelial cells exposed to genotoxic chemicals and the emergence of an altered tumor suppressor gene, p53, 3) extension of new system to include direct-acting and non-genotoxic chemicals as additional positive controls for the large-scale screening, and 4) classification of many diverse chemicals based on their mutagenic action on the ras proto-oncogene and the p53 tumor suppressor gene. The salient technical innovation in these studies is the use of PCR amplification of the very few mutations induced in a oncogenes and suppressor genes in an in vitro liver cell model of chemical carcinogenesis that simulate human exposure in vivo.Awardee's statement of the potential commercial applications of the research: The direct outcome will be the availability of a commercial service to identify a class of chemicals that activate oncogenes or inactivate suppressor genes when exposed to very low doses. A by-product could be the monitoring of human population at risk of developing cancer by the ultrasensitive assay of DNA isolated from peripheral blood lymphocytes.National Institute of Environmental Health Sciences (NIEHS)