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Structure-Function Analysis of the Glioma Targeting NFL-TBS.40-63 Peptide Corresponding to the Tubulin-Binding Site on the Light Neurofilament Subunit

机译:瞄准NFL-TBs。40-63肽对应于圣光神经丝亚基的微管蛋白结合位点的脑胶质瘤结构 - 功能分析

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摘要

We previously reported that a 24 amino acid peptide (NFL-TBS.40-63) corresponding to the tubulin-binding site located on the light neurofilament subunit, selectively enters in glioblastoma cells where it disrupts their microtubule network and inhibits their proliferation. Here, we analyzed the structure-function relationships using an alanine-scanning strategy, in order to identify residues essential for these biological activities. We showed that the majority of modified peptides present a decreased or total loss to penetrate in these cells, or to alter microtubules. Correspondingly, circular dichroism measurements showed that this peptide forms either β-sheet or α-helix structures according to the solvent and that alanine substitution modified or destabilized the structure, in relation with changes in the biological activities. Moreover, substitution of serine residues by phosphoserine or aspartic acid concomitantly decreased the cell penetrating activity and the structure stability. These results indicate the importance of structure for the activities, including selectivity to glioblastoma cells of this peptide, and its regulation by phosphorylation.
机译:我们以前曾报道过,对应于位于轻神经丝亚基上的微管蛋白结合位点的24个氨基酸的肽段(NFL-TBS.40-63)选择性进入胶质母细胞瘤细胞中,从而破坏其微管网络并抑制其增殖。在这里,我们使用丙氨酸扫描策略分析了结构与功能的关系,以鉴定这些生物学活性必不可少的残基。我们表明,大多数修饰的肽呈现出减少或完全丧失的能力,无法穿透这些细胞或改变微管。相应地,圆二色性测量表明,该肽根据溶剂形成β-折叠或α-螺旋结构,并且丙氨酸取代与生物活性的变化有关而使结构改变或不稳定。此外,用磷酸丝氨酸或天冬氨酸取代丝氨酸残基会同时降低细胞穿透活性和结构稳定性。这些结果表明结构对于活性的重要性,包括对该肽对胶质母细胞瘤细胞的选择性及其通过磷酸化的调节。

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