流式细胞术定量人肺肿瘤细胞系细胞内组织蛋白酶活性。

B Ulbricht, E Spiess, R Schwartz-Albiez, W Ebert
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引用次数: 13

摘要

半胱氨酸蛋白酶组织蛋白酶B和组织蛋白酶L很可能参与正常和恶性细胞的侵袭过程,它们与许多疾病有关,可能是人类肺癌结果的预后标志物。因此,我们分别用流式细胞术和分光光度法测定了不同组织蛋白酶组成的人肺癌细胞系细胞和细胞提取物中这些相关酶的活性。为此,我们将合成的二肽基底物苯氧羰基精氨酸-和苯氧羰基苯基精氨酸-偶联到4-甲氧基- β -萘酰胺、氨基甲基-coumarine或罗丹明R110。蛋白酶抑制剂,特别是E-64和CA-074,对表观酶活性有不同的定义。当4-甲氧基- β -萘酰胺或氨基甲基coumarine为离去基团时,超过99%的表观活性是由于组织蛋白酶B。用于检测细胞相关活性的4-甲氧基- β -萘酰胺沉淀物显示出对荧光的广谱激发,阻碍了其他可能的荧光标记的应用。因此,它的应用仅限于单参数荧光研究。与罗丹明R110偶联的两种二肽基都是混杂的:只有25 - 30%的表观活性是由组织蛋白酶B引起的;无论对细胞内或细胞提取物的活性进行分析,主要活性来自组织蛋白酶L。然而,罗丹明r110偶联底物为含有组织蛋白酶B和L的细胞的多参数荧光分析开辟了道路,如果额外应用适当的抑制剂来规范酶活性。4-甲氧基- β -萘酰胺会对细胞造成不可修复的损伤,与之相反,罗丹明底物允许对活细胞和活细胞分选进行研究。
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Quantification of intracellular cathepsin activities in human lung tumor cell lines by flow cytometry.

The cysteine proteases cathepsin B and cathepsin L are very likely involved in invasive processes of normal and malignant cells, they become relevant for a number of diseases and are possibly prognostic markers for the outcome of human lung cancer. Therefore, we have determined activities of these related enzymes in cells and in cell extracts of human lung carcinoma cell lines of different cathepsin composition by flow cytometry and by spectrophotometry, respectively. To this end we applied the synthetic dipeptidyl substrates benzoxycarbonyl-arginyl-arginine- and benzoxycarbonyl-phenyl-arginine- coupled to 4-methoxy-beta-naphthylamide, aminomethyl-coumarine or rhodamine R110. The apparent enzymatic activities were differentially defined by protease inhibitors, particularly E-64 and CA-074. Independent of the dipeptidyl-composition more than 99 per cent of the apparent activity was due to cathepsin B when 4-methoxy-beta-naphthylamide or aminomethylcoumarine were the leaving groups. The 4-methoxy-beta-naphthylamide precipitate used for detection of cell associated activities revealed a wide spectrum of excitation to fluorescence thwarting the application of other possible fluorescent tags. Therefore, its application is restricted to uniparametric fluorescence investigations. Both dipeptidylgroups coupled to rhodamine R110 were promiscuous: only 25 to 30% of the apparent activity were due to cathepsin B; the predominant activity came from cathepsin L, irrespective whether intracellular or activities of cellular extracts were analyzed. However, rhodamine R110-coupled substrates open the way for multiparametric fluorescent analysis of cathepsins B and L containing cells if appropriate inhibitors for specification of the enzymatic activities are additionally applied. In very contrast to 4-methoxy-beta-naphthylamide, which causes irreparable damage to the cells, the rhodamine substrates permit studies with living cells and live cell sorting.

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