class='kwd-title'>Keywords: Deparaffinization of'/> A novel xylene-free deparaffinization method for the extraction of proteins from human derived formalin-fixed paraffin embedded (FFPE) archival tissue blocks
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A novel xylene-free deparaffinization method for the extraction of proteins from human derived formalin-fixed paraffin embedded (FFPE) archival tissue blocks

机译:从人源福尔马林固定石蜡包埋(FFPE)档案组织块中提取蛋白质的新型无二甲苯脱蜡方法

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摘要

class="kwd-title">Keywords: Deparaffinization of paraffin embedded tissue blocks without the use of xylene class="kwd-title">Keywords: Pathology, Paraffin blocks, Protein extraction, Western blot, Xylene, Water class="head no_bottom_margin" id="idm140621834740240title">AbstractProtein detection methods in formalin-fixed paraffin embedded (FFPE) tissue blocks are widely used in research and clinical setting in order to diagnose or to confirm a diagnosis of various types of diseases. Therefore, multiple protein extraction methods from FFPE tissue sections have been developed in this regard. However, the yield and the quality of proteins extracted from FFPE tissues are significantly reduced in blocks stored for longer periods of time. Regardless the protein extraction method used, tissue sections must be first deparaffinized with xylene, and then washed in serial dilutions of ethanol in order to remove the toxic organic solvent “xylene” and rehydrate the tissue. The objective of this study was first to develop a method to deparaffinize FFPE blocks that excludes the use of toxic solvent “xylene”. Second minimize the time required to perform the extraction. Here we describe a method where: class="first-line-outdent">
  • • The entire paraffin embedded blocks are deparaffinized and rehydrated using only hot distilled water as a substitute for both xylene and ethanol
  • • The entire procedure takes about 15 min
  • • Deparaffinized blocks are immediately homogenized in lysis buffer, and the obtained lysate analyzed by Western blot.With this new modified technique, we were able to successfully detect actin and AKT proteins in lysates from blocks embedded in paraffin for up to 9 years.
  • 机译:<!-fig ft0-> <!-fig @ position =“ anchor” mode =文章f4-> <!-fig mode =“ anchred” f5-> <!-fig / graphic | fig / alternatives / graphic mode =“ anchored” m1-> class =“ kwd-title”>关键字:不使用二甲苯的石蜡包埋的组织块的去石蜡作用 class =“ kwd-title”>关键字:病理学,石蜡阻滞,蛋白质提取,蛋白质印迹,二甲苯,水 class =“ head no_bottom_margin” id =“ idm140621834740240title”>摘要福尔马林固定石蜡包埋(FFPE)中的蛋白质检测方法组织块广泛用于研究和临床环境中,以诊断或确认各种疾病的诊断。因此,在这方面已经开发了从FFPE组织切片提取多种蛋白质的方法。但是,从FFPE组织中提取的蛋白质的产量和质量在长时间存储的块中显着降低。无论采用哪种蛋白质提取方法,都必须先用二甲苯对组织切片进行脱蜡,然后用连续的乙醇稀释液洗涤,以去除有毒的有机溶剂“二甲苯”并使组织重新水化。这项研究的目的是首先开发一种将FFPE嵌段脱蜡的方法,该方法不使用有毒溶剂“二甲苯”。第二,最小化执行提取所需的时间。在这里,我们描述一种方法,其中: class =“ first-line-outdent”> <!-list-behavior =简单的前缀-word = mark-type = none max-label-size = 9->
  • •仅使用热蒸馏水作为二甲苯和乙醇的替代物,将整个石蜡包埋的块进行脱蜡和再水化
  • •整个过程大约需要15分钟
  • •将脱蜡的嵌段立即在裂解缓冲液中匀浆,并通过Western blot分析所得裂解物。 通过这种新的改良技术,我们能够成功检测肌动蛋白和AKT蛋白在裂解物中的溶解时间长达9年。
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