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人自然杀伤细胞裂解活性微细胞毒性测定的标准化

Standardization of a micro-cytotoxicity assay for human natural killer cell lytic activity.

作者信息

Mariani E, Monaco M C, Sgobbi S, de Zwart J F, Mariani A R, Facchini A

机构信息

Laboratorio di Immunologia e Genetica, Istituto di Ricerca Codivilla Putti I.O.R., Bologna, Italy.

出版信息

J Immunol Methods. 1994 Jun 24;172(2):173-8. doi: 10.1016/0022-1759(94)90104-x.

Abstract

Cytotoxicity assays are widely used to evaluate the functional activity of NK and T cells against tumour target cells and the release of radioactive sodium chromate from labelled target cells is still the most commonly used marker of target lysis in culture supernatants. We describe here the standardization of a micro-cytotoxicity test in which the number of cytolytic effector and tumour target cells have been decreased by a factor of 10. The release obtained by 500 tumour target cells was compared with the release obtained by 5000 target cells in the standard cytotoxicity assay for target:effector cell ratios from 1:1 to 1:100. Both gamma and beta emissions of the 51Cr isotope were evaluated to determine the assay release. The results obtained by the micro-cytotoxicity assay (500 target cells) were comparable to those of the standard assay (5000 target cells) and 51Cr release evaluation using the gamma counter was the most sensitive method of determining lytic activity using 500 tumour target cells. beta counter evaluation using solid phase scintillation was found to be a reproducible alternative method, even if the lytic curves cannot be compared with those obtained using the traditional method.

摘要

细胞毒性测定被广泛用于评估自然杀伤细胞(NK)和T细胞对肿瘤靶细胞的功能活性,并且从标记的靶细胞中释放放射性铬酸钠仍然是培养上清液中最常用的靶细胞裂解标记物。我们在此描述一种微量细胞毒性试验的标准化方法,其中溶细胞效应细胞和肿瘤靶细胞的数量减少了10倍。对于1:1至1:100的靶细胞与效应细胞比例,将500个肿瘤靶细胞所获得的释放量与标准细胞毒性试验中5000个靶细胞所获得的释放量进行比较。评估了51Cr同位素的γ和β发射以确定试验释放量。微量细胞毒性试验(500个靶细胞)所获得的结果与标准试验(5000个靶细胞)的结果相当,并且使用γ计数器进行51Cr释放评估是使用500个肿瘤靶细胞确定裂解活性的最灵敏方法。发现使用固相闪烁法进行β计数器评估是一种可重复的替代方法,即使裂解曲线无法与使用传统方法获得的曲线进行比较。

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