Mitchell Aaron C, Alford Spencer C, Hunter Sean A, Kannan Deepti, Parra Sperberg R Andres, Chang Cheryl H, Cochran Jennifer R
Department of Bioengineering, Stanford University , Stanford, California 94305, United States.
Cancer Biology Program, Stanford University , Stanford, California 94305, United States.
ACS Chem Biol. 2018 Jan 19;13(1):66-72. doi: 10.1021/acschembio.7b00715. Epub 2017 Dec 12.
Dysregulated activity of the protease matriptase is a key contributor to aggressive tumor growth, cancer metastasis, and osteoarthritis. Methods for the detection and quantification of matriptase activity and inhibition would be useful tools. To address this need, we developed a matriptase-sensitive protein biosensor based on a dimerization-dependent red fluorescent protein (ddRFP) reporter system. In this platform, two adjoining protein domains, connected by a protease-labile linker, produce fluorescence when assembled and are nonfluorescent when the linker is cleaved by matriptase. A panel of ddRFP-based matriptase biosensor designs was created that contained different linker lengths between the protein domains. These constructs were characterized for linker-specific cleavage, matriptase activity, and matriptase selectivity; a biosensor containing a RSKLRVGGH linker (termed B4) was expressed at high yields and displayed both high catalytic efficiency and matriptase specificity. This biosensor detects matriptase inhibition by soluble and yeast cell surface expressed inhibitor domains with up to a 5-fold dynamic range and also detects matriptase activity expressed by human cancer cell lines. In addition to matriptase, we highlight a strategy that can be used to create effective biosensors for quantifying activity and inhibition of other proteases of interest.
蛋白酶matriptase的活性失调是侵袭性肿瘤生长、癌症转移和骨关节炎的关键因素。检测和定量matriptase活性及抑制作用的方法将是有用的工具。为满足这一需求,我们基于二聚化依赖性红色荧光蛋白(ddRFP)报告系统开发了一种matriptase敏感的蛋白质生物传感器。在这个平台中,两个相邻的蛋白质结构域通过一个蛋白酶敏感的连接子相连,连接子完整时组装后产生荧光,而当连接子被matriptase切割时则无荧光。我们构建了一组基于ddRFP的matriptase生物传感器设计,其中蛋白质结构域之间包含不同长度的连接子。对这些构建体进行了连接子特异性切割、matriptase活性和matriptase选择性的表征;含有RSKLRVGGH连接子(称为B4)的生物传感器以高产率表达,并且具有高催化效率和matriptase特异性。该生物传感器可检测可溶性和酵母细胞表面表达的抑制剂结构域对matriptase的抑制作用,动态范围高达5倍,还可检测人癌细胞系表达的matriptase活性。除了matriptase,我们还重点介绍了一种可用于创建有效生物传感器以定量感兴趣的其他蛋白酶活性和抑制作用的策略。