从福尔马林固定、石蜡包埋的组织中提取蛋白质,能够通过质谱分析获得可靠的蛋白质组图谱。
Protein extraction of formalin-fixed, paraffin-embedded tissue enables robust proteomic profiles by mass spectrometry.
作者信息
Scicchitano Marshall S, Dalmas Deidre A, Boyce Rogely W, Thomas Heath C, Frazier Kendall S
机构信息
Department of Safety Assessment, 709 Swedeland Road, Mail Stop UE0364, King of Prussia, PA 19406, USA.
出版信息
J Histochem Cytochem. 2009 Sep;57(9):849-60. doi: 10.1369/jhc.2009.953497. Epub 2009 May 26.
Global mass spectrometry (MS) profiling and spectral count quantitation are used to identify unique or differentially expressed proteins and can help identify potential biomarkers. MS has rarely been conducted in retrospective studies, because historically, available samples for protein analyses were limited to formalin-fixed, paraffin-embedded (FFPE) archived tissue specimens. Reliable methods for obtaining proteomic profiles from FFPE samples are needed. Proteomic analysis of these samples has been confounded by formalin-induced protein cross-linking. The performance of extracted proteins in a liquid chromatography tandem MS format from FFPE samples and extracts from whole and laser capture microdissected (LCM) FFPE and frozen/optimal cutting temperature (OCT)-embedded matched control rat liver samples were compared. Extracts from FFPE and frozen/OCT-embedded livers from atorvastatin-treated rats were further compared to assess the performance of FFPE samples in identifying atorvastatin-regulated proteins. Comparable molecular mass representation was found in extracts from FFPE and OCT-frozen tissue sections, whereas protein yields were slightly less for the FFPE sample. The numbers of shared proteins identified indicated that robust proteomic representation from FFPE tissue and LCM did not negatively affect the number of identified proteins from either OCT-frozen or FFPE samples. Subcellular representation in FFPE samples was similar to OCT-frozen, with predominantly cytoplasmic proteins identified. Biologically relevant protein changes were detected in atorvastatin-treated FFPE liver samples, and selected atorvastatin-related proteins identified by MS were confirmed by Western blot analysis. These findings demonstrate that formalin fixation, paraffin processing, and LCM do not negatively impact protein quality and quantity as determined by MS and that FFPE samples are amenable to global proteomic analysis.
全球质谱(MS)分析和光谱计数定量用于鉴定独特的或差异表达的蛋白质,并有助于识别潜在的生物标志物。MS很少用于回顾性研究,因为从历史上看,用于蛋白质分析的可用样本仅限于福尔马林固定、石蜡包埋(FFPE)的存档组织标本。需要可靠的方法从FFPE样本中获取蛋白质组学图谱。这些样本的蛋白质组学分析因福尔马林诱导的蛋白质交联而受到干扰。比较了从FFPE样本以及全组织和激光捕获显微切割(LCM)的FFPE和冷冻/最佳切割温度(OCT)包埋的匹配对照大鼠肝脏样本中提取的蛋白质在液相色谱串联质谱格式中的性能。进一步比较了阿托伐他汀治疗大鼠的FFPE和冷冻/OCT包埋肝脏的提取物,以评估FFPE样本在鉴定阿托伐他汀调节蛋白方面的性能。在FFPE和OCT冷冻组织切片的提取物中发现了可比的分子量表现,而FFPE样本的蛋白质产量略低。鉴定出的共享蛋白质数量表明,FFPE组织和LCM的强大蛋白质组学表现不会对从OCT冷冻或FFPE样本中鉴定出的蛋白质数量产生负面影响。FFPE样本中的亚细胞表现与OCT冷冻样本相似,主要鉴定出细胞质蛋白。在阿托伐他汀治疗的FFPE肝脏样本中检测到生物学相关的蛋白质变化,并且通过蛋白质印迹分析证实了通过MS鉴定的选定的阿托伐他汀相关蛋白。这些发现表明,福尔马林固定、石蜡处理和LCM不会对MS测定的蛋白质质量和数量产生负面影响,并且FFPE样本适用于全球蛋白质组学分析。
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