Gel Electrophoresis: Proteins

S. Afford
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Abstract

a monoclonal antibody directed against Ki67, purchased from Dako, Glostrup, Denmark. The authors did not recommend the use of this antibody on paraffin wax sections. We have also tested the antibody on sections from routine blocks from human gingiva, tonsils and lymph nodes using different time schedules for microwave pretreatment and application of the primary antibody. Two crucial procedures for detecting Ki67 antigen successfully were identified. Firstly, slides should be pretreated in a microwave oven in citrate buffer (pH 6.0) for over 20 minutes (4 x 5 minutes).2 Secondly, Ki67 antibody (diluted 1 in 100-200) should be incubated overnight at 4°C to produce strong staining. Torp et al pretreated sections by microwaving for only 10 minutes (2 x 5 minutes) and incubated the Ki67 antibody for only one hour. Under these conditions, we could not achieve satisfactory staining on sections of the three tissues described above. Bankfalvi et ar have reported that almost identical results were found with the Ki67 and MIB 1 antibodies. In their method, microwave heating was carried out for 35 minutes (7 x 5 minutes) and the Ki67 monoclonal antibody
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凝胶电泳:蛋白质
一种针对Ki67的单克隆抗体,购自丹麦格洛斯特鲁普的Dako。作者不推荐在石蜡切片上使用该抗体。我们还对人牙龈、扁桃体和淋巴结的常规块切片进行了不同时间的微波预处理和一抗的应用测试。成功地确定了检测Ki67抗原的两个关键步骤。首先,载玻片应在微波炉中柠檬酸缓冲液(pH 6.0)中预处理超过20分钟(4 x 5分钟)其次,Ki67抗体(100-200稀释1)在4°C孵育过夜,以产生强染色。Torp等人通过微波预处理切片仅10分钟(2 x 5分钟),并孵育Ki67抗体仅1小时。在这些条件下,我们无法在上述三种组织的切片上获得令人满意的染色。Bankfalvi等人报道了Ki67和MIB 1抗体几乎相同的结果。在他们的方法中,微波加热35分钟(7 x 5分钟)和Ki67单克隆抗体
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