Abstract

Efficient flow of red blood cells (RBCs) and white blood cells (WBCs) through the microcirculation is necessary for oxygen and nutrient delivery as well as immune cell function. Because blood is a dense particulate suspension, consisting of 40% RBCs by volume, it is difficult to analyze the physical mechanisms by which individual blood cells contribute to the bulk flow properties of blood. Both experimental and computational approaches are hindered by these non-Newtonian properties, and predicting macroscopic blood flow characteristics such as viscosity has historically been an empirical process. In order to examine the effect of the individual cells on macroscopic blood rheology, we developed a lattice-Boltzmann model that considers the blood as a suspension of particles in plasma, accounting explicitly for cell–cell and cell–wall interactions. Previous studies have concluded that the abundance of leukocyte rolling in postcapillary venules is due to the interactions between red blood cells and leukocytes as they enter postcapillary expansions. Similar fluid dynamics may be involved in the initiation of rolling at branch points, a phenomenon linked to atherosclerosis. The lattice-Boltzmann approach is used to analyze the interactions of red and white blood cells as they flow through vascular networks digitized from normal and tumor tissue. A major advantage of the lattice-Boltzmann method is the ability to simulate particulate flow dynamically and in any geometry. Using this approach, we can accurately determine RBC–WBC forces, particle trajectories, the pressure changes in each segment that accompany cellular traffic in the network, and the forces felt by the vessel wall at any location. In this technique, intravital imaging using vascular contrast agents produces the network outline that is fed to the lattice-Boltzmann model. This powerful and flexible model can be used to predict blood flow properties in any vessel geometry and with any blood composition.

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