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从cDNA表达文库中对细胞毒性T淋巴细胞识别的肿瘤抗原进行ELISPOT克隆。

ELISPOT cloning of tumor antigens recognized by cytotoxic T-lymphocytes from a cDNA expression library.

作者信息

Uenaka A, Hata H, Win S, Ono T, Wada H, Nakayama E

机构信息

Department of Immunology, Okayama University Graduate School of Medicine and Dentistry, 2-5-1 Shikata-cho, Okayama 700-8558, Japan.

出版信息

Cancer Immun. 2001 Jul 13;1:8.

Abstract

The methodology of cloning genes coding for antigens recognized by T-cells from cDNA expression libraries was improved technically by using enzyme-linked immunospot (ELISPOT) assays instead of enzyme-linked immunosorbent assays (ELISA) or bioassays to detect cytokines produced by T-cells in response to antigens. Combining large and small scale ELISPOT assays for expression cloning has the following advantages compared to conventional cDNA expression cloning: i) the number of recombinant plasmids which can be screened is greater than 10,000 per well in a 24-well plate in a large scale ELISPOT assay compared to fewer than 100 per well in a 96-well plate in an IFN-gamma ELISA or a TNF-alpha bioassay; ii) the total number of recombinant plasmids which can be screened in a routine assay is 2 x 10 (5) in only one 24-well plate in a large scale ELISPOT assay compared to 1 x 10 (5) in ten 96-well plates in an IFN-gamma ELISA or a TNF-alpha bioassay. Thus the screening efficiency of large scale ELISPOT cloning is approximately 200 times that of conventional expression cloning approaches. The efficiency of the method was confirmed by detecting the model gene RLakt from a cDNA library of a murine leukemia RL male 1.

摘要

通过使用酶联免疫斑点(ELISPOT)分析而非酶联免疫吸附分析(ELISA)或生物分析来检测T细胞响应抗原产生的细胞因子,从cDNA表达文库中克隆编码T细胞识别抗原的基因的方法在技术上得到了改进。与传统的cDNA表达克隆相比,将大规模和小规模ELISPOT分析结合用于表达克隆具有以下优点:i)在大规模ELISPOT分析中,在24孔板中每孔可筛选的重组质粒数量大于10,000个,而在IFN-γ ELISA或TNF-α生物分析中,在96孔板中每孔少于100个;ii)在常规分析中,在大规模ELISPOT分析中仅一个24孔板中可筛选的重组质粒总数为2×10⁵,而在IFN-γ ELISA或TNF-α生物分析中,在十个96孔板中为1×10⁵。因此,大规模ELISPOT克隆的筛选效率约为传统表达克隆方法的200倍。通过从小鼠白血病RL雄性1的cDNA文库中检测模型基因RLakt证实了该方法的效率。

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