Krasnoslobodtsev Alexey V, Zhang Yuliang, Viazovkina Ekaterina, Gall Alexander, Bertagni Chad, Lyubchenko Yuri L
Department of Pharmaceutical Sciences, University of Nebraska Medical Center, Nebraska Medical Center, Omaha, Nebraska; Department of Physics, University of Nebraska Omaha, Omaha, Nebraska.
Department of Pharmaceutical Sciences, University of Nebraska Medical Center, Nebraska Medical Center, Omaha, Nebraska.
Biophys J. 2015 May 5;108(9):2333-9. doi: 10.1016/j.bpj.2015.03.040.
Immobilization is a key step involved in probing molecular interactions using single-molecule force spectroscopy methods, including atomic force microscopy (AFM). To our knowledge, we describe a novel approach termed flexible nanoarray (FNA) in which the interaction between the two internally immobilized amyloid β peptides is measured by pulling of the tether. The FNA tether was synthesized with nonnucleotide phosphoramidite monomers using the DNA synthesis chemistry. The two anchoring points for immobilization of the peptides inside the tether were incorporated at defined distances between them and from the ends of the polymer. Decamers of amyloid β peptide capable of dimer formation were selected as a test system. The formation of the peptide dimers was verified by AFM force spectroscopy by pulling the tether at the ends. In these experiments, the thiolated end of the FNA tether was covalently immobilized on the AFM substrate functionalized with maleimide. The other end of the FNA tether was functionalized with biotin to form a noncovalent link with the streptavidin functionalized AFM tip during the approach stage. The dimers' rupture fingerprint was unambiguously identified on the force curves by its position and the force value. The FNA design allowed reversible experiments in which the monomers were allowed to associate after the rupture of the dimers by performing the approach stage before the rupture of the biotin-streptavidin link. This suggests that the FNA technique is capable of analyzing multiple intermolecular interactions in the same molecular complex. The computational analysis showed that the tethered peptides assemble into the same dimer structure as that formed by nontethered peptides, suggesting that the FNA tether has the necessary flexibility to enable assembly of the dimer even during the course of the force spectroscopy experiment.
固定化是使用单分子力谱方法(包括原子力显微镜(AFM))探测分子相互作用所涉及的关键步骤。据我们所知,我们描述了一种称为柔性纳米阵列(FNA)的新方法,其中通过拉伸系链来测量两个内部固定的淀粉样β肽之间的相互作用。FNA系链是使用DNA合成化学方法用非核苷酸亚磷酰胺单体合成的。在系链内部固定肽的两个锚定点被并入它们之间以及与聚合物末端的特定距离处。能够形成二聚体的淀粉样β肽十聚体被选作测试系统。通过在末端拉伸系链,利用AFM力谱验证了肽二聚体的形成。在这些实验中,FNA系链的硫醇化末端共价固定在用马来酰亚胺功能化的AFM基底上。FNA系链的另一端用生物素功能化,以便在接近阶段与用链霉亲和素功能化的AFM探针形成非共价连接。二聚体的断裂指纹通过其在力曲线上的位置和力值被明确识别。FNA设计允许进行可逆实验,即在生物素 - 链霉亲和素连接断裂之前执行接近阶段,使二聚体断裂后单体能够重新缔合。这表明FNA技术能够分析同一分子复合物中的多种分子间相互作用。计算分析表明,系链肽组装成与非系链肽形成的相同二聚体结构,这表明FNA系链具有必要的灵活性,即使在力谱实验过程中也能使二聚体组装。