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首页> 外文期刊>Journal of Immunological Methods >Monoclonal antibodies raised to paraffin wax embedded archival tissue; feasibility study of their potential to detect novel antigenic markers.
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Monoclonal antibodies raised to paraffin wax embedded archival tissue; feasibility study of their potential to detect novel antigenic markers.

机译:产生针对石蜡包埋档案组织的单克隆抗体;它们检测新型抗原标记的潜力的可行性研究。

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摘要

A study to determine the feasibility of using archival paraffin wax embedded tissue to generate monoclonal antibodies is described. Specifically, monoclonal antibodies were raised to paraffin wax embedded normal human kidney tissue to test the possibility of producing antibodies to such tissue samples prior to attempting generation of antibodies to valuable archival tissue. Multiple sections (10 x 5 microm) were pooled and dewaxed as for immunohistochemical procedures and combined with Freund's adjuvant for immunization of BALB/c mice in vivo. Immunized spleen cells were fused with SP2 myeloma cells and subsequent clones screened on paraffin wax embedded normal human kidney sections, a range of cell lines and normal mouse tissue. Supernatants from 11 wells (from a total of 90 wells screened) showed different staining patterns on sections of paraffin wax embedded kidney. One clone, 1/11C, (isotype IgG1) which exhibited strong staining on all kidney tubules by immunohistochemical studies (glomeruli interstitium and vessels were unstained) and identified a band at 52 kDa on immunoblots of dewaxed kidney tissue (as used for immunogen) was chosen for further characterization. Immunoblotting of five mammalian cell lines showed differential expression of this 52 kDa band (distinct expression on 3/5, weak expression on 2/5 cell lines) whereas, all cell lines displayed a band at 44 kDa and a third band at 70 kDa was observed on 2/5 cell lines. In mouse tissue extracts, the 52 kDa band was identified in kidney tissue only (not in the lung, liver or spleen) with the 44 kDa and 70 kDa bands weakly expressed in all tissues. This preliminary investigation of a novel approach to identifying possible new antigenic markers or producing monoclonal antibodies which react better to known antigens on sections of paraffin wax embedded tissue showed that this method is feasible. The need to have a comprehensive screening system in place and the ability to identify potentially useful clones after the initial screening is paramount due to the relative scarcity of screening material (archival tissue sections) and the tedious nature of the screening method.
机译:描述了一项确定使用档案石蜡包埋组织产生单克隆抗体的可行性的研究。具体而言,在试图产生针对有价值的档案组织的抗体之前,将单克隆抗体引起石蜡包埋的正常人肾组织,以测试针对此类组织样品产生抗体的可能性。合并多个切片(10×5微米),并按照免疫组织化学方法脱蜡,并与弗氏佐剂组合用于体内BALB / c小鼠的免疫。将免疫的脾细胞与SP2骨髓瘤细胞融合,然后在石蜡包埋的正常人肾切片,一系列细胞系和正常小鼠组织中筛选随后的克隆。来自11个孔的上清液(总共筛选了90个孔)在石蜡包埋的肾脏切片上显示出不同的染色模式。通过免疫组织化学研究(所有肾小球间质和血管未染色)在所有肾小管上均显示强染色的克隆(1 / 11C)(同种型IgG1)(在脱蜡的肾脏组织的免疫印迹上鉴定出一条52 kDa的条带)(用于免疫原)。选择用于进一步表征。五个哺乳动物细胞系的免疫印迹显示该52 kDa条带差异表达(3/5处表达明显,2/5细胞系弱表达),而所有细胞系均显示44 kDa处的一条带和70 kDa处的第三条带。在2/5个细胞系中观察到。在小鼠组织提取物中,仅在肾脏组织中(而非肺,肝或脾脏)鉴定出52 kDa的条带,而在所有组织中均弱表达了44 kDa和70 kDa的条带。对鉴定可能的新抗原标记或产生对石蜡包埋组织切片上的已知抗原反应更好的单克隆抗体的新方法的初步研究表明,该方法是可行的。由于筛选材料(档案组织切片)的相对稀缺和筛选方法的乏味,因此需要有一套完善的筛选系统,并且在初次筛选后才能鉴定出潜在有用克隆的能力至关重要。

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