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Unfolding and Extraction of a Transmembrane α-Helical Peptide: Dynamic Force Spectroscopy and Molecular Dynamics Simulations

机译:跨膜α-螺旋肽的展开和提取:动态力谱和分子动力学模拟。

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摘要

An atomic force microscope (AFM) was used to visualize CWALP1923 peptides (+H3N-ACAGAWWLALALALALALALWWA-COO) inserted in gel-phase DPPC and DSPC bilayers. The peptides assemble in stable linear structures and domains. A model for the organization of the peptides is given from AFM images and a 20 ns molecular dynamics (MD) simulation. Gold-coated AFM cantilevers were used to extract single peptides from the bilayer through covalent bonding to the cystein residue. Experimental and simulated force curves show two distinct force maxima. In the simulations these two maxima correspond to the extraction of the two pairs of tryptophan residues from the membrane. Unfolding of the peptide precedes extraction of the second distal set of tryptophans. To probe the energies involved, AFM force curves were obtained from 10 to 104 nm/s and MD force curves were simulated with 108–1011 nm/s pulling velocities (V). The velocity relationship with the force, F, was fitted to two fluctuation adhesive potential models. The first assumes the pulling produces a constant bias in the potential and predicts an F ∼ ln (V) relationship. The second takes into account the ramped bias that the linker feels as it is being driven out of the adhesion complex and scales as F ∼ (ln V)2/3.
机译:使用原子力显微镜(AFM)观察凝胶相中插入的CWALP 19 23个肽段DPPC和DSPC双层。肽以稳定的线性结构和结构域组装。从AFM图像和20 ns分子动力学(MD)模拟中给出了肽组织的模型。镀金的AFM悬臂用于通过与半胱氨酸残基的共价键合从双层中提取单个肽。实验和模拟力曲线显示了两个不同的力最大值。在模拟中,这两个最大值对应于从膜中提取两对色氨酸残基。肽的解折叠先于第二组远端色氨酸的提取。为了探测所涉及的能量,获得了10至10 4 nm / s的AFM力曲线,并使用10 8 –10 11 模拟了MD力曲线。 sup> nm / s拉动速度(V)。将速度与力F的关系拟合到两个波动的粘合电位模型。第一个假设拉力在电势中产生恒定的偏差,并预测F〜ln(V)关系。第二个因素考虑了接头被赶出粘附复合体时所感觉到的倾斜偏斜,并按F〜(ln V) 2/3 缩放。

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