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基于抗原修复技术的福尔马林固定石蜡包埋组织切片免疫组织化学标准化:从实验到假说

Standardization of immunohistochemistry for formalin-fixed, paraffin-embedded tissue sections based on the antigen-retrieval technique: from experiments to hypothesis.

作者信息

Shi Shan-Rong, Liu Cheng, Taylor Clive R

机构信息

Department of Pathology, University of Southern California School of Medicine HMR 204, 2011 Zonal Avenue, Los Angeles, CA 90033, USA.

出版信息

J Histochem Cytochem. 2007 Feb;55(2):105-9. doi: 10.1369/jhc.6P7080.2006. Epub 2006 Sep 18.

DOI:10.1369/jhc.6P7080.2006
PMID:16982846
Abstract

From a practical point of view, one of the most difficult issues in the standardization of IHC for FFPE tissue is the adverse influence of formalin upon antigenicity, as well as the great variation in fixation/processing procedures. Based on previous study, an additional study using four markers demonstrated the potential for obtaining equivalent IHC staining among FFPE tissue sections with periods of formalin fixation ranging from 6 hr to 30 days. On this basis, the following hypothesis is proposed. "The use of optimized AR protocols permits retrieval of specific proteins (antigens) from FFPE tissues to a defined and reproducible degree (expressed as R%), with reference to the amount of protein present in the original fresh/unfixed tissue". This hypothesis may also be presented mathematically: the protein amount in a fresh cell/tissue, expressed as Pf, produces an IHC signal in fresh tissue of integral(Pf). When the identical IHC staining plus AR treatment is applied to a FFPE tissue section, the IHC signal may be represented as integral (Pffpe). The degree of retrieval after AR (R%) is calculated as follows: R% = integral (Pffpe)/ integral (Pf) x 100%. The amount of protein in the FFPE tissue may then be derived as follows: Pffpe = Pf x R%. In a situation where optimized AR is 100% effective, the IHC signal would then be of equal strength in fresh tissue and FFPE tissue, and Pffpe= Pf. Further studies are designed to test the limitations of the proposed hypothesis.

摘要

从实际角度来看,福尔马林固定石蜡包埋(FFPE)组织免疫组化标准化过程中最困难的问题之一是福尔马林对抗原性的不利影响,以及固定/处理程序的巨大差异。基于先前的研究,另一项使用四种标志物的研究表明,在福尔马林固定时间从6小时到30天不等的FFPE组织切片中,获得等效免疫组化染色的可能性。在此基础上,提出了以下假设。“使用优化的抗原修复(AR)方案可以从FFPE组织中以确定且可重复的程度(表示为R%)检索特定蛋白质(抗原),以原始新鲜/未固定组织中存在的蛋白质数量为参考”。这个假设也可以用数学方式表示:新鲜细胞/组织中的蛋白质量,以Pf表示,在新鲜组织中产生积分(Pf)的免疫组化信号。当对FFPE组织切片应用相同的免疫组化染色加抗原修复处理时,免疫组化信号可以表示为积分(Pffpe)。抗原修复后的检索程度(R%)计算如下:R% = 积分(Pffpe)/积分(Pf)×100%。然后,FFPE组织中的蛋白质量可以如下推导:Pffpe = Pf×R%。在优化的抗原修复100%有效的情况下,新鲜组织和FFPE组织中的免疫组化信号强度将相等,且Pffpe = Pf。进一步的研究旨在测试所提出假设的局限性。

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