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An efficient procedure for protein extraction from formalin-fixed, paraffin-embedded tissues for reverse phase protein arrays

机译:从福尔马林固定,石蜡包埋的组织中提取蛋白质的有效方法,用于反相蛋白质阵列

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Introduction Protein extraction from formalin-fixed paraffin-embedded (FFPE) tissues is challenging due to extensive molecular crosslinking that occurs upon formalin fixation. Reverse-phase protein array (RPPA) is a high-throughput technology, which can detect changes in protein levels and protein functionality in numerous tissue and cell sources. It has been used to evaluate protein expression mainly in frozen preparations or FFPE-based studies of limited scope. Reproducibility and reliability of the technique in FFPE samples has not yet been demonstrated extensively. We developed and optimized an efficient and reproducible procedure for extraction of proteins from FFPE cells and xenografts, and then applied the method to FFPE patient tissues and evaluated its performance on RPPA. Results Fresh frozen and FFPE preparations from cell lines, xenografts and breast cancer and renal tissues were included in the study. Serial FFPE cell or xenograft sections were deparaffinized and extracted by six different protein extraction protocols. The yield and level of protein degradation were evaluated by SDS-PAGE and Western Blots. The most efficient protocol was used to prepare protein lysates from breast cancer and renal tissues, which were subsequently subjected to RPPA. Reproducibility was evaluated and Spearman correlation was calculated between matching fresh frozen and FFPE samples. The most effective approach from six protein extraction protocols tested enabled efficient extraction of immunoreactive protein from cell line, breast cancer and renal tissue sample sets. 85% of the total of 169 markers tested on RPPA demonstrated significant correlation between FFPE and frozen preparations (p < 0.05) in at least one cell or tissue type, with only 23 markers common in all three sample sets. In addition, FFPE preparations yielded biologically meaningful observations related to pathway signaling status in cell lines, and classification of renal tissues. Conclusions With optimized protein extraction methods, FFPE tissues can be a valuable source in generating reproducible and biologically relevant proteomic profiles using RPPA, with specific marker performance varying according to tissue type.
机译:简介由于福尔马林固定后会发生广泛的分子交联,因此从福尔马林固定石蜡包埋(FFPE)组织中提取蛋白质具有挑战性。反相蛋白质阵列(RPPA)是一种高通量技术,可以检测多种组织和细胞来源中蛋白质水平和蛋白质功能的变化。它主要用于冷冻制剂或有限范围的基于FFPE的研究中,用于评估蛋白质表达。 FFPE样品中该技术的可重复性和可靠性尚未得到广泛证明。我们开发并优化了从FFPE细胞和异种移植物中提取蛋白质的有效且可重复的程序,然后将该方法应用于FFPE患者组织并评估了其在RPPA上的性能。结果本研究包括来自细胞系,异种移植物,乳腺癌和肾组织的新鲜冷冻和FFPE制剂。将连续的FFPE细胞或异种移植切片去石蜡并通过六种不同的蛋白质提取方案进行提取。蛋白质降解的产量和水平通过SDS-PAGE和Western Blots进行评估。最有效的方法用于从乳腺癌和肾组织中制备蛋白裂解物,然后将其进行RPPA处理。评估了可重复性,并在匹配的新鲜冷冻样品和FFPE样品之间计算了Spearman相关性。经过测试的六种蛋白质提取方案中最有效的方法是能够从细胞系,乳腺癌和肾组织样本集中有效提取免疫反应蛋白。在RPPA上测试的169种标记总数中,有85%证明FFPE与冷冻制剂在至少一种细胞或组织类型中具有显着相关性(p <0.05),在所有三个样品集中只有23种标记共有。此外,FFPE制剂产生了与细胞系中的信号通路状态以及肾组织分类有关的生物学意义的观察结果。结论通过优化的蛋白质提取方法,FFPE组织可以成为使用RPPA产生可再现的和生物学相关的蛋白质组学概况的有价值的来源,具体的标志物性能随组织类型而异。

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