Department of Mechanical Engineering, Massachusetts Institute of Technology, Cambridge, MA, USA.
Integr Biol (Camb). 2013 Oct;5(10):1262-71. doi: 10.1039/c3ib40149a.
A deeper understanding of the mechanisms of tumor cell extravasation is essential in creating therapies that target this crucial step in cancer metastasis. Here, we use a microfluidic platform to study tumor cell extravasation from in vitro microvascular networks formed via vasculogenesis. We demonstrate tight endothelial cell-cell junctions, basement membrane deposition and physiological values of vessel permeability. Employing our assay, we demonstrate impaired endothelial barrier function and increased extravasation efficiency with inflammatory cytokine stimulation, as well as positive correlations between the metastatic potentials of MDA-MB-231, HT-1080, MCF-10A and their extravasation capabilities. High-resolution time-lapse microscopy reveals the highly dynamic nature of extravasation events, beginning with thin tumor cell protrusions across the endothelium followed by extrusion of the remainder of the cell body through the formation of small (1 μm) openings in the endothelial barrier which grows in size (8 μm) to allow for nuclear transmigration. No disruption to endothelial cell-cell junctions is discernible at 60×, or by changes in local barrier function after completion of transmigration. Tumor transendothelial migration efficiency is significantly higher in trapped cells compared to non-trapped adhered cells, and in cell clusters versus single tumor cells.
深入了解肿瘤细胞外渗的机制对于开发针对癌症转移这一关键步骤的治疗方法至关重要。在这里,我们使用微流控平台研究了通过血管生成形成的体外微血管网络中肿瘤细胞的外渗。我们证明了紧密的内皮细胞-细胞连接、基底膜沉积和血管通透性的生理值。通过我们的测定方法,我们证明了炎症细胞因子刺激会导致内皮屏障功能受损和外渗效率增加,以及 MDA-MB-231、HT-1080、MCF-10A 的转移潜力与其外渗能力之间存在正相关关系。高分辨率延时显微镜揭示了外渗事件的高度动态性质,首先是肿瘤细胞突起穿过内皮细胞,然后通过在内皮屏障形成小(约 1 μm)开口将剩余的细胞体挤出,该开口的大小会增大(至约 8 μm)以允许核穿过。在 60×下,或在穿过内皮细胞迁移完成后,内皮细胞-细胞连接没有明显的破坏,局部屏障功能也没有变化。与非被困贴壁细胞相比,被困细胞的肿瘤细胞穿过内皮的迁移效率明显更高,与单个肿瘤细胞相比,细胞簇的迁移效率更高。
