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Gene expression profiling of di-n-butyl phthalate in normal human mammary epithelial cells.

Journal of environmental pathology, toxicology and oncology : official organ of the International Society for Environmental Toxicology and Cancer 2007 Vol.26(1) p. 51-61

Gwinn MR, Whipkey DL, Tennant LB, Weston A

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Studies show that female workers in the personal-care industry have an increased risk of developing cancer believed to be the result of increased exposure to toxic and/or carcinogenic chemicals found

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APA Gwinn MR, Whipkey DL, et al. (2007). Gene expression profiling of di-n-butyl phthalate in normal human mammary epithelial cells.. Journal of environmental pathology, toxicology and oncology : official organ of the International Society for Environmental Toxicology and Cancer, 26(1), 51-61. https://doi.org/10.1615/jenvironpatholtoxicoloncol.v26.i1.60
MLA Gwinn MR, et al.. "Gene expression profiling of di-n-butyl phthalate in normal human mammary epithelial cells.." Journal of environmental pathology, toxicology and oncology : official organ of the International Society for Environmental Toxicology and Cancer, vol. 26, no. 1, 2007, pp. 51-61.
PMID 17725530

Abstract

Studies show that female workers in the personal-care industry have an increased risk of developing cancer believed to be the result of increased exposure to toxic and/or carcinogenic chemicals found in cosmetics, hair dyes, and nail polish. One chemical found in multiple personal-care products, di-n-butyl phthalate (DBP), is a known endocrine disruptor and has been found in increased levels in women of childbearing age. The goal of this study was to elucidate mechanisms of phthalate toxicity in normal human cells to provide information concerning interindividual variation and gene-environment interactions. Normal human mammary epithelial cell strains were obtained from discarded tissues following reduction mammoplasty [Cooperative Human Tissue Network (sponsors: NCI/NDRI)]. Gene transcription in each cell strain was analyzed using high-density oligonucleotide DNA microarrays (U133A, Affymetrix) and changes in the expression of selected genes were verified by real-time polymerase chain reaction (PCR) (ABI). DNA microarrays were hybridized with total RNA that was collected after DBP treatment for 5 hr and 10 hr. RNA was harvested from the vehicle control (acetone) at 10 hr. Data Mining Tool software (Affymetrix) was used to separate genes in clusters based on their expression patterns over time. Only 57 genes were found to be altered in all four cell strains following exposure to DBP. These included genes involved in fertility (inhibin, placental growth factor), immune response (tumor necrosis factor induced protein), and antioxidant status (glutathione peroxidase). Data from this study will help clarify the role of DBP in reproductive toxicity, and yield biomarkers of exposure for future epidemiology studies.

추출된 의학 개체 (NER)

유형영어 표현한국어 / 풀이UMLS CUI출처등장
해부 mammary 유방 dict 2
시술 reduction mammoplasty 유방성형술 dict 1
해부 tissues scispacy 1
해부 cell scispacy 1
해부 DNA scispacy 1
해부 DBP → di-n-butyl phthalate scispacy 1
합병증 necrosis 괴사 dict 1
합병증 nail scispacy 1
합병증 U133A scispacy 1
약물 di-n-butyl phthalate C0012052
dibutyl phthalate
scispacy 1
약물 phthalate toxicity scispacy 1
약물 acetone C0001002
acetone
scispacy 1
약물 glutathione C0017817
glutathione
scispacy 1
약물 DBP → di-n-butyl phthalate scispacy 1
약물 phthalate scispacy 1
질환 cancer C0006826
Malignant Neoplasms
scispacy 1
질환 toxic and/or carcinogenic chemicals scispacy 1
질환 high-density oligonucleotide scispacy 1
질환 tumor necrosis C0333516
Tumor necrosis
scispacy 1
질환 toxicity C0040539
Toxicity aspects
scispacy 1
기타 human mammary epithelial cells scispacy 1
기타 female scispacy 1
기타 hair scispacy 1
기타 women scispacy 1
기타 human cells scispacy 1
기타 human mammary epithelial cell strains scispacy 1
기타 Human Tissue Network scispacy 1
기타 inhibin scispacy 1
기타 tumor necrosis factor induced protein) scispacy 1
기타 glutathione peroxidase scispacy 1

MeSH Terms

Cells, Cultured; Dibutyl Phthalate; Female; Gene Expression Profiling; Gene Expression Regulation; Glutathione; Humans; Inhibins; Mammary Glands, Human; Oligonucleotide Array Sequence Analysis; Placenta Growth Factor; Plasticizers; Pregnancy Proteins; RNA; Tumor Necrosis Factor-alpha

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