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在细胞毒性T细胞检测中,BLT酯酶活性作为铬释放法的替代方法。

BLT esterase activity as an alternative to chromium release in cytotoxic T cell assays.

作者信息

Suhrbier A, Fernan A, Burrows S R, Saul A, Moss D J

机构信息

Queensland Institute of Medical Research, Brisbane, Australia.

出版信息

J Immunol Methods. 1991 Dec 15;145(1-2):43-53. doi: 10.1016/0022-1759(91)90309-4.

Abstract

Granules released by cytotoxic T cells (CTL), during recognition and killing of target cells, contain granule enzyme A. This serine protease has an esterase activity, which is easily measured using the substrate benzyloxycarbonyl-L-lysine thiobenzyl ester (BLT). BLT activity, routinely used as an assay for granule release, provides an alternative to the standard chromium release assay as a measure of CTL-mediated killing. The two methods were highly comparable when either exogenous synthetic peptide or endogenously produced epitopes were used as targets and human CTL clones acted as effectors. The advantages of the BLT assay are that it uses inexpensive non-radioactive reagents, the assay can be run over any period between 4 and 30 h and can be performed with as few as 10(4) CTLs if synthetic peptide epitopes are used.

摘要

细胞毒性T细胞(CTL)在识别和杀伤靶细胞过程中释放的颗粒含有颗粒酶A。这种丝氨酸蛋白酶具有酯酶活性,使用底物苄氧羰基-L-赖氨酸硫代苄酯(BLT)可轻松测定该活性。BLT活性通常用作颗粒释放的检测方法,作为衡量CTL介导杀伤作用的一种手段,它可替代标准的铬释放检测法。当使用外源性合成肽或内源性产生的表位作为靶标且人CTL克隆作为效应细胞时,这两种方法具有高度可比性。BLT检测法的优点在于它使用价格低廉的非放射性试剂,该检测可在4至30小时的任何时间段内进行,并且如果使用合成肽表位,仅用10⁴个CTL即可完成检测。

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