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使用微纹理表面降低癌细胞粘附

Reducing Cancer Cell Adhesion using Microtextured Surfaces.

作者信息

McCue Caroline, Atari Adel, Parks Sean, Tseng Yuen-Yi, Varanasi Kripa K

机构信息

Department of Mechanical Engineering, Massachusetts Institute of Technology, 77 Massachusetts Ave, Cambridge, MA, 02139, USA.

Cancer Program, Broad Institute of Harvard and MIT, 415 Main St, Cambridge, MA, 02142, USA.

出版信息

Small. 2023 Dec;19(49):e2302401. doi: 10.1002/smll.202302401. Epub 2023 Aug 9.

Abstract

For the past century, trypsin has been the primary method of cell dissociation, largely without any major changes to the process. Enzymatic cell detachment strategies for large-scale cell culturing processes are popular but can be labor-intensive, potentially lead to the accumulation of genetic mutations, and produce large quantities of liquid waste. Therefore, engineering surfaces to lower cell adhesion strength could enable the next generation of cell culture surfaces for delicate primary cells and automated, high-throughput workflows. In this study, a process for creating microtextured polystyrene (PS) surfaces to measure the impact of microposts on the adhesion strength of cells is developed. Cell viability and proliferation assays show comparable results in two cancer cell lines between micropost surfaces and standard cell culture vessels. However, cell image analysis on microposts reveals that cell area decreases by half, and leads to an average twofold increase in cell length per area. Using a microfluidic-based method up to a seven times greater percentage of cells are removed from micropost surfaces than the flat control surfaces. These results show that micropost surfaces enable decreased cell adhesion strength while maintaining similar cell viabilities and proliferation as compared to flat PS surfaces.

摘要

在过去的一个世纪里,胰蛋白酶一直是细胞解离的主要方法,在很大程度上该过程没有任何重大变化。用于大规模细胞培养过程的酶促细胞脱离策略很受欢迎,但可能需要大量人力,有导致基因突变积累的潜在风险,并且会产生大量液体废物。因此,设计具有较低细胞粘附强度的表面能够为培养脆弱的原代细胞以及实现自动化、高通量工作流程打造新一代细胞培养表面。在本研究中,开发了一种制造微纹理聚苯乙烯(PS)表面的方法,以测量微柱对细胞粘附强度的影响。细胞活力和增殖分析表明,在两种癌细胞系中,微柱表面和标准细胞培养容器的结果相当。然而,对微柱上的细胞进行图像分析发现,细胞面积减少了一半,导致单位面积内细胞长度平均增加了两倍。使用基于微流控的方法,从微柱表面去除的细胞百分比比平坦对照表面高出多达七倍。这些结果表明,与平坦的PS表面相比,微柱表面能够降低细胞粘附强度,同时保持相似的细胞活力和增殖能力。

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