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一种使用细胞外基质凝胶进行小型化三维细胞培养的概念。

A concept for miniaturized 3-D cell culture using an extracellular matrix gel.

作者信息

Frisk Thomas, Rydholm Susanna, Andersson Helene, Stemme Göran, Brismar Hjalmar

机构信息

Microsystems Laboratory, School of Electrical Engineering, Royal Institute of Technology, Stockholm, Sweden.

出版信息

Electrophoresis. 2005 Dec;26(24):4751-8. doi: 10.1002/elps.200500478.

Abstract

This paper presents a novel method to embed, anchor, and cultivate cells in a controlled 3-D flow-through microenvironment. This is realized using an etched silicon pillar flow chamber filled with extracellular matrix (ECM) gel mixed with cells. At 4 degrees C, while in liquid form, ECM gel is mixed with cells and injected into the chamber. Raising the temperature to 37 degrees C results in a gel, with cells embedded. The silicon pillars both stabilize and increase the surface to volume ratio of the gel. During polymerization the gel shrinks, thus creating channels, which enables perfusion through the chip. The pillars increase the mechanical stability of the gel permitting high surface flow rates without surface modifications. Within the structure cells were still viable and proliferating after 6 days of cultivation. Our method thus makes it possible to perform medium- to long-term cultivation of cells in a controlled 3-D environment. This concept opens possibilities to perform studies of cells in a more physiological environment compared to traditional 2-D cultures on flat substrates.

摘要

本文提出了一种在可控的三维流通微环境中嵌入、固定和培养细胞的新方法。这是通过一个蚀刻硅柱流动腔来实现的,该流动腔中填充有与细胞混合的细胞外基质(ECM)凝胶。在4摄氏度时,处于液态的ECM凝胶与细胞混合并注入腔室。将温度升至37摄氏度会使凝胶形成,细胞被嵌入其中。硅柱既能稳定凝胶,又能增加凝胶的表面积与体积比。在聚合过程中,凝胶会收缩,从而形成通道,使灌注能够通过芯片。这些柱子提高了凝胶的机械稳定性,允许在不进行表面修饰的情况下实现高表面流速。在培养6天后,结构内的细胞仍然存活并增殖。因此,我们的方法使得在可控的三维环境中进行细胞的中长期培养成为可能。与传统的在平面基质上的二维培养相比,这一概念为在更接近生理环境的条件下进行细胞研究开辟了可能性。

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