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首页> 外文期刊>Endocrine >Relationships of ESR1 and XBP1 expression in human breast carcinoma and stromal cells isolated by laser capture microdissection compared to intact breast cancer tissue
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Relationships of ESR1 and XBP1 expression in human breast carcinoma and stromal cells isolated by laser capture microdissection compared to intact breast cancer tissue

机译:与完整乳腺癌组织相比,激光捕获显微切割法分离的人乳腺癌和基质细胞中ESR1和XBP1表达的关系

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摘要

Results from investigations of human genomics which utilize intact tissue biopsy specimens maybe compromised due to a host of uncontrolled variables including cellular heterogeneity of a sample collected under diverse conditions, then processed and stored using different protocols. To determine the cellular origin and assess relationships of mRNA expression of two genes reported to be co-expressed in human breast carcinoma (estrogen receptor-α, ESR1 and X-box binding protein 1, XBP1), gene expression analyses were performed with intact tissue sections and compared with those of laser capture microdissection (LCM)-procured carcinoma and stromal cells from serial sections of the same tissue. Frozen sections of human breast carcinomas were first evaluated for structural integrity and pathology after hematoxylin and eosin (H&E) staining. Total RNA preparations from intact tissue sections and LCM-procured carcinoma and stromal cells were reverse transcribed for measurements of ESR1 and XBP1 expression by quantitative PCR (qPCR). These results were compared with those obtained from microarray analyses of LCM-procured carcinoma cells. Levels of ESR1 and XBP1 were detected in the intact breast cancer tissue sections suggesting coordinate gene expression. Although coordinate expression of these genes was observed in the LCM-procured carcinoma cells, it was not discerned in LCM-procured stromal cells. The origin of coordinate expression of ESR1 and XBP1 observed in whole tissue sections of human breast cancer biopsies is due principally to their co-expression in carcinoma cells and not in the surrounding stromal cells as substantiated using LCM-procured cells. Collectively, a microgenomic process was established from human tissue preparation to RNA characterization and analysis to identify molecular signatures of specific cell types predicting clinical behavior.
机译:利用完整组织活检标本进行人类基因组学研究的结果可能会受到损害,原因是存在许多不受控制的变量,包括在不同条件下收集的样品的细胞异质性,然后使用不同的协议进行处理和存储。为了确定细胞起源并评估据报道在人类乳腺癌中共表达的两个基因(雌激素受体-α,ESR1和X-box结合蛋白1,XBP1)的mRNA表达之间的关系,对完整组织进行了基因表达分析并与激光捕获显微切割(LCM)所获得的癌和来自同一组织连续切片的基质细胞进行比较。在苏木精和曙红(H&E)染色后,首先评估人乳腺癌的冷冻切片的结构完整性和病理学。将来自完整组织切片以及LCM所致癌和基质细胞的总RNA制剂反转录,以通过定量PCR(qPCR)测量ESR1和XBP1的表达。将这些结果与从LCM采购的癌细胞的微阵列分析获得的结果进行比较。在完整的乳腺癌组织切片中检测到ESR1和XBP1的水平,暗示了协调基因的表达。尽管在LCM采购的癌细胞中观察到了这些基因的协调表达,但在LCM采购的基质细胞中却没有发现。在人类乳腺癌活组织检查的整个组织切片中观察到的ESR1和XBP1协调表达的起源主要是由于它们在癌细胞中的共表达,而不是在周围基质细胞中的共表达,这是使用LCM采购的细胞所证实的。集体地建立了从人类组织制备到RNA表征和分析的微基因组学过程,以识别预测临床行为的特定细胞类型的分子标记。

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  • 来源
    《Endocrine》 |2011年第2期|p.212-221|共10页
  • 作者

    Sarah A. Andres; James L. Wittliff;

  • 作者单位

    Hormone Receptor Laboratory, Department of Biochemistry &amp Molecular Biology, Brown Cancer Center and the Institute for Molecular Diversity &amp Drug Design, University of Louisville, Health Sciences Center A Bldg.—Room 604, Louisville, KY, 40292, USA;

    Hormone Receptor Laboratory, Department of Biochemistry &amp Molecular Biology, Brown Cancer Center and the Institute for Molecular Diversity &amp Drug Design, University of Louisville, Health Sciences Center A Bldg.—Room 604, Louisville, KY, 40292, USA;

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  • 关键词

    Gene expression; ESR1; XBP1; Laser capture microdissection; Carcinoma cells; Stromal cells;

    机译:基因表达;ESR1;XBP1;激光捕获显微切割;癌细胞;基质细胞;

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