Shi S R, Cote R J, Hawes D, Thu S, Shi Y, Young L L, Taylor C R
Department of Pathology, University of Southern California School of Medicine, Los Angeles, California 90033, USA.
J Histochem Cytochem. 1999 Apr;47(4):463-70. doi: 10.1177/002215549904700404.
A recent study by Morgan et al. on the mechanism of the heating antigen retrieval (AR) has raised an interesting issue concerning calcium-induced modification of protein conformation demonstrated by immunohistochemistry (IHC). The current study is based on calcium-induced modification of thrombospondin (TSP) and Ki-67, as demonstrated by IHC using seven monoclonal antibodies (MAbs) to TSP and an MAb MIB1. Experiments were carried out on frozen tissue sections of bladder carcinoma and lymph node. Frozen sections were incubated with solutions of 50 mM CaCl2 and/or 10 mM EDTA at 4C overnight before formalin or acetone fixation for TSP and Ki-67, respectively. Sections were then fixed in 10% neutral buffered formalin or acetone before immunostaining. Seven MAbs to TSP, named Ab1 to 7 representing clone numbers of A4.1, D4.6, C6.7, A6.1, B5.2, A2.5, and HB8432, respectively, and MIB1 were utilized as primary antibodies. ABC was used as the detection system and AEC as the chromogen for immunohistochemical staining. An extracellular immunostaining pattern represented a positive result for TSP, and nuclear staining for MIB1. Frozen sections preincubated in 50 mM CaCl2 overnight at 4C showed significant loss of staining and/or altered staining pattern for six of the seven antibodies to TSP and MIB1 compared to positive controls not exposed to CaCl2. Lack of immunostaining of TSP and MIB1 attributable to exposure to CaCl2 could be partially recovered by incubating the frozen sections in EDTA. Calcium-induced modification of protein structure was demonstrated more than 10 years ago on the basis of immunochemical techniques. In this study, similar calcium-induced modification of protein was detectable by IHC in frozen tissue sections, suggesting that calcium-induced modification of protein structure may occur independently of fixation-induced modification. The fact that calcium binding may affect IHC staining is not surprising in view of the fact that antibody/antigen interactions are protein structure-dependent. However, in this experiment the change occurred before and independent of formalin fixation and does not necessarily imply a role for calcium in AR. There may be a valuable role for the use of chemical modification in visualization of protein structure changes in tissue sections by IHC. (J Histochem Cytochem 47:463-469, 1999)
摩根等人最近进行的一项关于加热抗原修复(AR)机制的研究,提出了一个有趣的问题,即免疫组织化学(IHC)所证实的钙诱导蛋白质构象改变。当前的研究基于免疫组织化学使用七种针对血小板反应蛋白(TSP)的单克隆抗体(MAb)和一种单克隆抗体MIB1所证实的钙诱导血小板反应蛋白(TSP)和Ki-67的构象改变。实验在膀胱癌和淋巴结的冰冻组织切片上进行。在分别用福尔马林或丙酮固定TSP和Ki-67之前,将冰冻切片在4℃下用50 mM氯化钙和/或10 mM乙二胺四乙酸(EDTA)溶液孵育过夜。然后将切片用10%中性缓冲福尔马林或丙酮固定,再进行免疫染色。七种针对TSP的单克隆抗体,分别命名为Ab1至7,代表克隆编号A4.1、D4.6、C6.7、A6.1、B5.2、A2.5和HB8432,以及MIB1被用作一抗。ABC用作检测系统,AEC用作免疫组织化学染色的显色剂。细胞外免疫染色模式代表TSP的阳性结果,MIB1为核染色。与未暴露于氯化钙的阳性对照相比,在4℃下用50 mM氯化钙预孵育过夜的冰冻切片显示,七种针对TSP的抗体和MIB1中的六种染色明显缺失和/或染色模式改变。通过将冰冻切片在EDTA中孵育,可部分恢复因暴露于氯化钙而导致的TSP和MIB1免疫染色缺失。基于免疫化学技术,十多年前就已证实钙诱导蛋白质结构改变。在本研究中,通过免疫组织化学在冰冻组织切片中可检测到类似的钙诱导蛋白质改变,表明钙诱导蛋白质结构改变可能独立于固定诱导的改变而发生。鉴于抗体/抗原相互作用依赖于蛋白质结构,钙结合可能影响免疫组织化学染色这一事实并不令人惊讶。然而,在本实验中,这种变化发生在福尔马林固定之前且与之无关,并不一定意味着钙在抗原修复中起作用。在通过免疫组织化学观察组织切片中蛋白质结构变化时,化学修饰的应用可能具有重要作用。(《组织化学与细胞化学杂志》47:463 - 469,1999)
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