Institute for Clinical Chemistry, Medical Faculty Mannheim of University of Heidelberg, University Hospital Mannheim, Theodor-Kutzer-Ufer 1-3, 68167 Mannheim, Germany.
Int J Oncol. 2011 Jul;39(1):145-54. doi: 10.3892/ijo.2011.1009. Epub 2011 Apr 18.
The progression of many solid tumors is characterized by the release of tumor-associated proteases, such as cancer procoagulant, MMP2 and MMP7. Consequently, the detection of tumor-specific proteolytic activity in serum specimens has recently been proposed as a new diagnostic tool in oncology. However, tumor-associated proteases are highly diluted in serum specimens and it is challenging to identify substrates that are specifically cleaved. In this study, we describe the systematic optimization of a synthetic peptide substrate using a positional scanning synthetic combinatorial library (PS-SCL) approach. The initial reporter peptide (RP) comprises of the cleavage site, WKPYDAAD, that is part of the coagulation factor X, the natural substrate of the tumor-associated cysteine protease cancer procoagulant (EC 3.4.22.26). Specifically, the amino acid substitution of aspartatic acid (D) in position P1' against asparagine (N) improved the processing of respective RPs in serum specimens from patients with colorectal tumors compared to healthy controls. Proteolytic fragments of RPs accumulated during prolonged incubation with serum specimens and were quantified with matrix-assisted laser desorption/ionization time-of-flight mass spectrometry. Finally, the optimized RP with the cleaved motif WKPYNAAD was combined with the RPs, VPLSLTMG and IPVSLRSG, that were cleaved by the tumor-associated proteases, MMP2 and MMP7, respectively. The diagnostic accuracy of MS-based protease profiling was evaluated for this triplex RP mix in a cohort of 50 serum specimens equally divided into colorectal cancer patients and healthy control individuals. Multiparametric analysis showed an AUC value of 0.90 for the receiver operating characteristic curve and was superior to the classification accuracy of the single markers. Our results demonstrate that RPs for MS-based protease profiling can systematically be optimized with a PS-SCL. Furthermore, the combination of different RPs can additionally increase the classification accuracy of functional protease profiling, and this in turn could lead to improved diagnosis, monitoring and prognosis of malignant disease.
许多实体瘤的进展特征是释放肿瘤相关蛋白酶,如癌促凝血酶、MMP2 和 MMP7。因此,最近有人提出在肿瘤学中,检测血清标本中的肿瘤特异性蛋白水解活性是一种新的诊断工具。然而,肿瘤相关蛋白酶在血清标本中高度稀释,难以鉴定特异性切割的底物。在本研究中,我们描述了使用位置扫描合成组合文库(PS-SCL)方法对合成肽底物进行系统优化。初始报告肽(RP)包含凝血因子 X 的切割位点 WKPYDAAD,是肿瘤相关半胱氨酸蛋白酶癌促凝血酶(EC 3.4.22.26)的天然底物。具体来说,与健康对照组相比,位于 P1'位置的天冬氨酸(D)被天冬酰胺(N)取代,提高了各自 RP 在结直肠肿瘤患者血清标本中的加工效率。在与血清标本长时间孵育过程中,RP 积累了蛋白水解片段,并通过基质辅助激光解吸/电离飞行时间质谱进行定量。最后,将具有切割基序 WKPYNAAD 的优化 RP 与分别由肿瘤相关蛋白酶 MMP2 和 MMP7 切割的 RP(VPLSLTMG 和 IPVSLRSG)组合。基于 MS 的蛋白酶谱分析的诊断准确性在 50 个血清标本的队列中进行了评估,这些标本平均分为结直肠癌患者和健康对照组。多参数分析显示,用于三重 RP 混合物的接收器操作特征曲线的 AUC 值为 0.90,优于单个标志物的分类准确性。我们的结果表明,基于 MS 的蛋白酶谱分析的 RP 可以通过 PS-SCL 进行系统优化。此外,不同 RP 的组合还可以进一步提高功能蛋白酶谱分析的分类准确性,从而改善恶性疾病的诊断、监测和预后。
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