The response of living cells to electric field (EF) has been observed for more than a hundred years, but the mechanism of how cells interact with EF is not entirely ascertained. Although many efforts have been devoted to the application of EF stimulation in tissue engineering and regeneration, the fundamental scientific principle of such practice remains unveiled and keeps drawing attention during the pursuit of consistent outcomes. In this regard, my research focuses on the underlying mechanism by which EF stimulation evokes cellular responses and the EF modulation of cell signaling pathways to physiological behaviors. The first part of my research focuses on developing the platform for controlled EF stimulation and real-time imaging/analysis. High-k dielectric passivated microelectrodes are fabricated to send capacitively coupled alternating current electric field (AC EF) stimulation to cells. I have developed two generations of EF stimulation devices with environmental control chambers: the first one is used to study cell signaling pathway dynamics; the second one is upgraded with long-term culture capability to study cell physiological behaviors. The second part of my research focuses on the quantification and mechanistic study of AC EF perturbation of the extracellular signal-related kinase (ERK) signaling pathway. I demonstrate that AC EF stimulation can induce both inhibition and activation of the ERK pathway, with different AC EF amplitude thresholds and time and magnitude scales. The mechanistic study shows that the ERK activation is initiated by AC EF-induced epidermal growth factor receptor (EGFR) phosphorylation, and the ERK inhibition is related to AC EF-induced change of Ras activities. In addition, these ERK responses show high sensitivity to AC EF waveform and timing, indicating electrostatic coupling mechanism and providing new parameter spaces for further investigation on the modulation of the ERK signaling pathway via AC EF stimulation. The last part of my research steers to cell physiological behaviors under prolonged AC EF stimulation. I report that AC EF stimulation can clearly inhibit cell proliferation and migration, and the inhibition in cell proliferation is sensitive to AC EF amplitude, stimulation pattern, and pulse rising time. These findings can benefit the AC EF application in medical treatment.

This dissertation features a compilation of studies concerning the biophysics of multicellular systems. I explore eukaryotic systems across length scales of the cell cytoskeleton to macroscopic scales of tissues. I begin with a general overview of the natural phenomena of life and a philosophy of investigating developmental systems in biology. The topics covered throughout this dissertation require a background in eukaryotic cell physiology, viscoelasticity, and processes of embryonic tissue morphogenesis. Following a brief background on these topics, I present an overview of the Subcellular Element Model (ScEM). This is a modeling framework which allows one to compute the dynamics of large numbers of three-dimensional deformable cells in multi-cellular systems. A primary focus of the work presented here is implementing cellular function within the framework of this model to produce biologically meaningful phenotypes. In this way, it is hoped that this modeling may inform biological understanding of the underlying mechanisms which manifest into a given cell or tissue scale phenomenon. Thus, all theoretical investigations presented here are motivated by and compared to experimental observations. With the ScEM modeling framework I first explore the passive properties of viscoelastic networks. Then as a direct extension of this work, I consider the active properties of cells, which result in biological behavior and the emergence of non-trivial biological phenotypes in cells and tissues. I then explore the possible role of chemotaxis as a mechanism of orchestrating large scale tissue morphogenesis in the early embryonic stages of amniotes. Finally I discuss the cross-sectional topology of proliferating epithelial tissues. I show how the Subcellular Element Model (ScEM) is a phenomenological model of finite elements whose interactions can be calibrated to describe the viscoelastic properties of biological materials. I further show that implementing mechanisms of cytoskeletal remodeling yields cellular and tissue phenotypes that are more and more biologically realistic. Particularly I show that structural remodeling of the cell cytoskeleton is crucial for large scale cell deformations. I provide supporting evidence that a chemotactic dipole mechanism is able to orchestrate the type of large scale collective cell movement observed in the chick epiblast during gastrulation and primitive streak formation. Finally, I show that cell neighbor histograms provide a potentially unique signature measurement of tissue topology; such measurements may find use in identifying cellular level phenotypes from a single snapshot micrograph.