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在 3D 培养中解耦信号传导的扩散控制和尺寸控制揭示了肌球蛋白在管状形成中的作用。

Decoupling diffusional from dimensional control of signaling in 3D culture reveals a role for myosin in tubulogenesis.

机构信息

Department of Biomedical Engineering, Johns Hopkins University School of Medicine, Baltimore, MD 21205, USA.

出版信息

J Cell Sci. 2010 Sep 1;123(Pt 17):2877-83. doi: 10.1242/jcs.055079. Epub 2010 Aug 3.

Abstract

We present a novel microfabricated platform to culture cells within arrays of micrometer-scale three-dimensional (3D) extracellular matrix scaffolds (microgels). These microscale cultures eliminate diffusion barriers that are intrinsic to traditional 3D culture systems (macrogels) and enable uniform cytokine stimulation of the entire culture population, as well as allow immunolabeling, imaging and population-based biochemical assays across the relatively coplanar microgels. Examining early signaling associated with hepatocyte growth factor (HGF)-mediated scattering and tubulogenesis of MDCK cells revealed that 3D culture modulates cellular responses both through dimensionality and altered stimulation rates. Comparing responses in 2D culture, microgels and macrogels demonstrated that HGF-induced ERK signaling was driven by the dynamics of stimulation and not by whether cells were in a 2D or 3D environment, and that this ERK signaling was equally important for HGF-induced cell scattering on 2D substrates and tubulogenesis in 3D. By contrast, we discovered a specific HGF-induced increase in myosin expression leading to sustained downregulation of myosin activity that occurred only within 3D contexts and was required for 3D tubulogenesis but not 2D scattering. Interestingly, although absent in cells on collagen-coated plates, downregulation of myosin activity also occurred for cells on collagen gels, but was transient and mediated by a combination of myosin dephosphorylation and enhanced myosin expression. Furthermore, upregulating myosin activity via siRNA targeted to a myosin phosphatase did not attenuate scattering in 2D but did inhibit tubulogenesis in 3D. Together, these results demonstrate that cellular responses to soluble cues in 3D culture are regulated by both rates of stimulation and by matrix dimensionality, and highlight the importance of decoupling these effects to identify early signals relevant to cellular function in 3D environments.

摘要

我们提出了一种新颖的微制造平台,用于在微米级三维(3D)细胞外基质支架(微凝胶)阵列中培养细胞。这些微尺度培养物消除了传统 3D 培养系统(大凝胶)中固有的扩散障碍,能够均匀地刺激整个培养物群体,并且允许在相对共面的微凝胶上进行免疫标记、成像和基于群体的生化分析。研究与肝细胞生长因子(HGF)介导的 MDCK 细胞散射和小管形成相关的早期信号表明,3D 培养通过维度和改变的刺激率来调节细胞反应。在 2D 培养、微凝胶和大凝胶中比较反应表明,HGF 诱导的 ERK 信号是由刺激的动力学驱动的,而不是由细胞是否处于 2D 或 3D 环境驱动的,并且这种 ERK 信号对于 HGF 诱导的 2D 底物上的细胞散射和 3D 中的小管形成同样重要。相比之下,我们发现 HGF 诱导的肌球蛋白表达增加导致肌球蛋白活性的持续下调,这种下调仅发生在 3D 环境中,并且是 3D 小管形成所必需的,但不是 2D 散射所必需的。有趣的是,尽管在胶原包被板上的细胞中不存在,但肌球蛋白活性的下调也发生在胶原凝胶上,但却是短暂的,并通过肌球蛋白去磷酸化和增强肌球蛋白表达的组合介导的。此外,通过针对肌球蛋白磷酸酶的 siRNA 上调肌球蛋白活性不会抑制 2D 中的散射,但会抑制 3D 中的小管形成。总之,这些结果表明,3D 培养中细胞对可溶性信号的反应受到刺激速率和基质维度的调节,并强调了解耦这些效应以识别与 3D 环境中细胞功能相关的早期信号的重要性。

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