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Fibroblast Activation Protein Peptide Substrates Identified from Human Collagen I Derived Gelatin Cleavage Sites

劈理(地质) 成纤维细胞活化蛋白 成纤维细胞 蛋白酶 化学 肽序列 间质细胞 分子生物学 金属蛋白酶 蛋白酵素 生物化学 基质金属蛋白酶 生物 体外 基因 癌症研究 古生物学 遗传学 癌症 断裂(地质)
作者
Saurabh Aggarwal,W. Nathaniel Brennen,Thomas P. Kole,Elizabeth Schneider,Özlem Topaloglu,Melinda S. Yates,Robert J. Cotter,Samuel R. Denmeade
出处
期刊:Biochemistry [American Chemical Society]
卷期号:47 (3): 1076-1086 被引量:82
标识
DOI:10.1021/bi701921b
摘要

A highly consistent trait of tumor stromal fibroblasts is the induction of the membrane-bound serine protease fibroblast activation protein-α (FAP), which is overexpressed on the surface of reactive stromal fibroblasts present within the stroma of the majority of human epithelial tumors. In contrast, FAP is not expressed by tumor epithelial cells or by fibroblasts or other cell types in normal tissues. The proteolytic activity of FAP, therefore, represents a potential pan-tumor target that can be exploited for the release of potent cytotoxins from inactive prodrugs consisting of an FAP peptide substrate coupled to a cytotoxin. To identify FAP peptide substrates, we used liquid chromatography tandem mass spectroscopy based sequencing to generate a complete map of the FAP cleavage sites within human collagen I derived gelatin. Positional analysis of the frequency of each amino acid at each position within the cleavage sites revealed FAP consensus sequences PPGP and (D/E)-(R/K)-G-(E/D)-(T/S)-G-P. These studies further demonstrated that ranking cleavage sites based on the magnitude of the LC/MS/MS extracted ion current predicted FAP substrates that were cleaved with highest efficiency. Fluorescence-quenched peptides were synthesized on the basis of the cleavage sites with the highest ion current rankings, and kinetic parameters for FAP hydrolysis were determined. The substrate DRGETGP, which corresponded to the consensus sequence, had the lowest Km of 21 μM. Overall the Km values were relatively similar for both high and low ranked substrates, whereas the kcat values differed by up to 100-fold. On the basis of these results, the FAP consensus sequences are currently being evaluated as FAP-selective peptide carriers for incorporation into FAP-activated prodrugs.

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