ABSTRACT
Bacteria are ubiquitous in complex three-dimensional (3D) porous environments, such as biological tissues and gels, and subsurface soils and sediments. However, the majority of previous work has focused on studies of cells in bulk liquids or at flat surfaces, which do not fully recapitulate the complexity of many natural bacterial habitats. Here, this gap in knowledge is addressed by describing the development of a method to 3D-print dense colonies of bacteria into jammed granular hydrogel matrices. These matrices have tunable pore sizes and mechanical properties; they physically confine the cells, thus supporting them in 3D. They are optically transparent, allowing for direct visualization of bacterial spreading through their surroundings using imaging. As a proof of this principle, here, the capability of this protocol is demonstrated by 3D printing and imaging non-motile and motile Vibro cholerae, as well as non-motile Escherichia coli, in jammed granular hydrogel matrices with varying interstitial pore sizes.
Subject(s)
Bacteria , Hydrogels , Porosity , Printing, Three-Dimensional , Escherichia coliABSTRACT
How do growing bacterial colonies get their shapes? While colony morphogenesis is well studied in two dimensions, many bacteria grow as large colonies in three-dimensional (3D) environments, such as gels and tissues in the body or subsurface soils and sediments. Here, we describe the morphodynamics of large colonies of bacteria growing in three dimensions. Using experiments in transparent 3D granular hydrogel matrices, we show that dense colonies of four different species of bacteria generically become morphologically unstable and roughen as they consume nutrients and grow beyond a critical size-eventually adopting a characteristic branched, broccoli-like morphology independent of variations in the cell type and environmental conditions. This behavior reflects a key difference between two-dimensional (2D) and 3D colonies; while a 2D colony may access the nutrients needed for growth from the third dimension, a 3D colony inevitably becomes nutrient limited in its interior, driving a transition to unstable growth at its surface. We elucidate the onset of the instability using linear stability analysis and numerical simulations of a continuum model that treats the colony as an "active fluid" whose dynamics are driven by nutrient-dependent cellular growth. We find that when all dimensions of the colony substantially exceed the nutrient penetration length, nutrient-limited growth drives a 3D morphological instability that recapitulates essential features of the experimental observations. Our work thus provides a framework to predict and control the organization of growing colonies-as well as other forms of growing active matter, such as tumors and engineered living materials-in 3D environments.
Subject(s)
Bacteria , Models, Biological , Morphogenesis , Hydrogels , SoilABSTRACT
The mechanical properties of ultrathin polystyrene (PS) films have been shown to change as the thickness approaches the average size of a polymer molecule. Previous measurements of the uniaxial stress-strain relationship for ultrathin polymer films have required the use of liquid-support layers. However, the influence of the liquid support layer, specifically water, on the mechanical properties of PS films has remained an open question. Here, we introduce a method for directly measuring the complete stress-strain response of ultrathin freestanding polymer films. For freestanding PS thin films, we observe a constant elastic modulus and maximum stress with decreasing thickness for film thicknesses as thin as 30 nm, consistent with the liquid supported measurement. From the freestanding measurements, we identify that the liquid supporting layer leads to enhanced craze stability for ultrathin PS films. We compare these results to the previous liquid-supported measurements and provide insights into how the liquid surface interactions can alter polymer behavior in thin polymer films.