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An Improved Breast Epithelial Sampling Method for Molecular Profiling and Biomarker Analysis in Women at Risk for Breast Cancer

机译:一种改进的乳腺癌上皮采样方法,用于有乳腺癌风险的女性的分子谱分析和生物标志物分析

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Background: There is a strong need to define the molecular changes in normal at-risk breast epithelium to identify biomarkers and new targets for breast cancer prevention and to develop a molecular signature for risk assessment. Improved methods of breast epithelial sampling are needed to promote whole-genome molecular profiling, increase ductal epithelial cell yield, and reduce sample cell heterogeneity.Methods: We developed an improved method of breast ductal sampling with ductal lavage through a 22-gauge catheter and collection of ductal samples with a microaspirator. Women at normal risk or increased risk for breast cancer were studied. Ductal epithelial samples were analyzed for cytopathologic changes, cellular yield, epithelial cell purity, quality and quantity of DNA and RNA, and use in multiple downstream molecular applications.Results: We studied 50 subjects, including 40 subjects at normal risk for breast cancer and 37 subjects with non-nipple aspirate fluid-yielding ducts. This method provided multiple 1.0 mL samples of high ductal epithelial cell content (median ≥8 samples per subject of ≥5,000 cells per sample) with 80%–100% epithelial cell purity. Extraction of a single intact ductal sample (fluid and cells) or the separate frozen cellular component provided DNA and RNA for multiple downstream studies, including quantitative reverse transcription- polymerase chain reaction (PCR) for microRNA, quantitative PCR for the human telomerase reverse transcriptase gene, whole-genome DNA amplification, and array comparative genomic hybridization analysis.Conclusion: An improved breast epithelial sampling method has been developed, which should significantly expand the acquisition and biomarker analysis of breast ductal epithelium in women at risk for breast cancer.
机译:背景:迫切需要定义正常高危乳腺上皮的分子变化,以识别生物标志物和预防乳腺癌的新靶标,并开发出用于风险评估的分子标记。需要改进的乳腺上皮采样方法以促进全基因组分子图谱分析,增加导管上皮细胞产量并减少样品细胞异质性。方法:我们开发了一种通过22口径导管进行导管灌洗的乳腺导管采样方法,并进行了收集用微量抽吸器采集导管样品。研究了处于正常风险或罹患乳腺癌风险增加的女性。分析了导管上皮样品的细胞病理学变化,细胞产量,上皮细胞纯度,DNA和RNA的质量和数量,并将其用于多种下游分子应用。结果:我们研究了50名受试者,包括40名处于正常乳腺癌风险的受试者和37名受试者非乳头抽吸输液管的受试者。该方法提供了多个1.0 mL高导管上皮细胞含量的样品(每个受试者中位≥8个样品,每个样品≥5,000个细胞),上皮细胞纯度为80%–100%。提取单个完整的导管样品(流体和细胞)或分离的冷冻细胞成分可为多种下游研究提供DNA和RNA,包括用于microRNA的定量逆转录-聚合酶链反应(PCR),用于人类端粒酶逆转录酶基因的定量PCR结论,全基因组DNA扩增和阵列比较基因组杂交分析。结论:已开发出一种改良的乳腺上皮采样方法,该方法应显着扩大有乳腺癌风险的女性乳腺导管上皮的获取和生物标志物分析。

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