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利用原子力显微镜通过纳米力学探测和粘附力测量分析LRP-1沉默对癌细胞侵袭潜能的影响。

Analysis of the effect of LRP-1 silencing on the invasive potential of cancer cells by nanomechanical probing and adhesion force measurements using atomic force microscopy.

作者信息

Le Cigne A, Chièze L, Beaussart A, El-Kirat-Chatel S, Dufrêne Y F, Dedieu S, Schneider C, Martiny L, Devy J, Molinari M

机构信息

Laboratoire de Recherche en Nanosciences LRN EA4682, Université de Reims Champagne-Ardenne, 21 rue Clément Ader, 51685 Reims Cedex 2, France.

Institute of Life Sciences, Université Catholique de Louvain, Croix du Sud 4-5, bte L7.07.06, 1348 Louvain-la-neuve, Belgique.

出版信息

Nanoscale. 2016 Apr 7;8(13):7144-54. doi: 10.1039/c5nr08649c.

DOI:10.1039/c5nr08649c
PMID:26965453
Abstract

Low-density lipoprotein receptor-related protein 1 (LRP-1) can internalize proteases involved in cancer progression and is thus considered a promising therapeutic target. However, it has been demonstrated that LRP-1 is also able to regulate the endocytosis of membrane-anchored proteins. Thus, strategies that target LRP-1 to modulate proteolysis could also affect adhesion and cytoskeleton dynamics. Here, we investigated the effect of LRP-1 silencing on parameters reflecting cancer cells' invasiveness by atomic force microscopy (AFM). The results show that LRP-1 silencing induces changes in the cells' adhesion behavior, particularly the dynamics of cell attachment. Clear alterations in morphology, such as more pronounced stress fibers and increased spreading, leading to increased area and circularity, were also observed. The determination of the cells' mechanical properties by AFM showed that these differences are correlated with an increase in Young's modulus. Moreover, the measurements show an overall decrease in cell motility and modifications of directional persistence. An overall increase in the adhesion force between the LRP-1-silenced cells and a gelatin-coated bead was also observed. Ultimately, our AFM-based force spectroscopy data, recorded using an antibody directed against the β1 integrin subunit, provide evidence that LRP-1 silencing modifies the rupture force distribution. Together, our results show that techniques traditionally used for the investigation of cancer cells can be coupled with AFM to gain access to complementary phenotypic parameters that can help discriminate between specific phenotypes associated with different degrees of invasiveness.

摘要

低密度脂蛋白受体相关蛋白1(LRP-1)可使参与癌症进展的蛋白酶内化,因此被视为一个有前景的治疗靶点。然而,已有研究表明LRP-1也能够调节膜锚定蛋白的内吞作用。因此,靶向LRP-1来调节蛋白水解的策略也可能影响黏附及细胞骨架动力学。在此,我们通过原子力显微镜(AFM)研究了LRP-1沉默对反映癌细胞侵袭性参数的影响。结果显示,LRP-1沉默会诱导细胞黏附行为发生变化,尤其是细胞附着的动力学。还观察到形态上有明显改变,如应力纤维更明显且铺展增加,导致面积和圆度增大。通过AFM测定细胞的力学性能表明,这些差异与杨氏模量的增加相关。此外,测量结果显示细胞运动性总体下降且方向持续性发生改变。还观察到LRP-1沉默细胞与明胶包被微珠之间的黏附力总体增加。最终,我们使用针对β1整合素亚基的抗体记录的基于AFM的力谱数据提供了证据,表明LRP-1沉默会改变破裂力分布。总之,我们的结果表明,传统上用于研究癌细胞的技术可与AFM相结合,以获取互补的表型参数,这些参数有助于区分与不同侵袭程度相关的特定表型。

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