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识别细胞表面蛋白酶的蛋白质抑制剂的亲和制备。

Affinity preparation of a protein inhibitor recognising a cell surface protease.

作者信息

Steven F S, Griffin M M, Bell J, Talbot I C

机构信息

Department of Biochemistry and Molecular Biology, School of Biological Sciences, University of Manchester, UK.

出版信息

J Enzyme Inhib. 1993;7(1):65-76. doi: 10.3109/14756369309020190.

DOI:10.3109/14756369309020190
PMID:7510796
Abstract

Epithelial cell surfaces possess a trypsin-like protease, referred to as guanidinobenzoatase (GB). The cytoplasm of these cells contains an extractable protein (I) which recognises the cell surface GB by forming an enzyme-inhibitor complex (GB-I). Rhodamine-agmatine (Rh-Agm) was designed as a red fluorescent probe, directed to the active centre of GB, which can be used to locate cells with GB, employing fluorescence microscopy. Rh-Agm has a high affinity for GB and will displace I from GB-I on the surfaces of cells in frozen sections. Rh-Agm has been used to displace I from immobilised GB-I complexes on the surface of cultured colonic carcinoma cells in an affinity procedure aimed at purifying the inhibitors of GB obtained from cultured carcinoma cells. These inhibitors have been tested on protected frozen sections of normal colon and carcinoma of the colon, the formation of GB-I complexes being followed by a second yellow fluorescent probe which competes for the active centre of GB. The study of the protein-protein interactions to form GB-I has been facilitated by employing two synthetic fluorescent inhibitors of GB with differing affinities for GB and different fluorescent properties. The use of sections of tissue in this study has enabled a sequence of reactions to be carried out on the same cell surface GB, such that reversible inhibition reactions can be quickly demonstrated and recorded by fluorescence microscopy.

摘要

上皮细胞表面有一种类似胰蛋白酶的蛋白酶,称为胍基苯甲酸酶(GB)。这些细胞的细胞质中含有一种可提取的蛋白质(I),它通过形成酶 - 抑制剂复合物(GB - I)来识别细胞表面的GB。罗丹明 - 胍丁胺(Rh - Agm)被设计为一种红色荧光探针,指向GB的活性中心,可用于通过荧光显微镜定位含有GB的细胞。Rh - Agm对GB具有高亲和力,并且会在冷冻切片的细胞表面将I从GB - I中置换出来。在旨在纯化从培养的癌细胞中获得的GB抑制剂的亲和程序中,Rh - Agm已被用于从培养的结肠癌细胞表面的固定化GB - I复合物中置换I。这些抑制剂已在正常结肠和结肠癌的冷冻保护切片上进行了测试,GB - I复合物的形成通过第二种竞争GB活性中心的黄色荧光探针进行跟踪。通过使用两种对GB具有不同亲和力和不同荧光特性的GB合成荧光抑制剂,促进了对形成GB - I的蛋白质 - 蛋白质相互作用的研究。在本研究中使用组织切片能够在同一细胞表面GB上进行一系列反应,从而可以通过荧光显微镜快速证明和记录可逆抑制反应。

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