Ricci Francesco, Bonham Andrew J, Mason Aaron C, Reich Norbert O, Plaxco Kevin W
Dipartimento di Scienze e Tecnologie Chimiche, Universita di Roma Tor Vergata, Via della Ricerca Scientifica, 00133, Rome, Italy.
Anal Chem. 2009 Feb 15;81(4):1608-14. doi: 10.1021/ac802365x.
Here we demonstrate a reagentless, electrochemical platform for the specific detection of proteins that bind to single- or double-stranded DNA. The sensor is composed of a double- or single-stranded, redox-tagged DNA probe which is covalently attached to an interrogating electrode. Upon protein binding the current arising from the redox tag is suppressed, indicating the presence of the target. Using this approach we have fabricated sensors against the double-stranded DNA binding proteins TATA-box binding protein and M.HhaI methyltransferase, and against the single-strand binding proteins Escherichia coli SSBP and replication protein A. All four targets are detected at nanomolar concentrations, in minutes, and in a convenient, general, readily reusable, electrochemical format. The approach is specific; we observed no significant cross-reactivity between the sensors. Likewise the approach is selective; it supports, for example, the detection of single strand binding protein directly in crude nuclear extracts. The generality of our approach (including its ability to detect both double- and single-strand binding proteins) and a strong, non-monotonic dependence of signal gain on probe density support a collisional signaling mechanism in which binding alters the collision efficiency, and thus electron transfer efficiency, of the attached redox tag. Given the ubiquity with which protein binding will alter the collisional dynamics of an oligonucleotide, we believe this approach may prove of general utility in the detection of DNA and RNA binding proteins.
在此,我们展示了一种用于特异性检测与单链或双链DNA结合的蛋白质的无试剂电化学平台。该传感器由共价连接到检测电极上的双链或单链、带有氧化还原标签的DNA探针组成。蛋白质结合后,氧化还原标签产生的电流被抑制,表明目标物的存在。利用这种方法,我们制备了针对双链DNA结合蛋白TATA盒结合蛋白和M.HhaI甲基转移酶以及单链结合蛋白大肠杆菌单链结合蛋白(SSBP)和复制蛋白A的传感器。所有这四种目标物都能在纳摩尔浓度下,在几分钟内以方便、通用、易于重复使用的电化学形式被检测到。该方法具有特异性;我们观察到传感器之间没有明显的交叉反应。同样,该方法具有选择性;例如,它支持直接在粗核提取物中检测单链结合蛋白。我们方法的通用性(包括其检测双链和单链结合蛋白的能力)以及信号增益对探针密度的强烈、非单调依赖性支持了一种碰撞信号机制,即结合改变了附着的氧化还原标签的碰撞效率,进而改变了电子转移效率。鉴于蛋白质结合会普遍改变寡核苷酸的碰撞动力学,我们相信这种方法可能在检测DNA和RNA结合蛋白方面具有普遍实用性。