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the phagocytosis and toxicity of amorphous silica非晶硅的吞噬作用和毒性
The Phagocytosis and Toxicity of Amorphous Silica
¤ ´
Lindsey M. Costantini , Renee M. Gilberti, David A. Knecht*
Department of Molecular and Cell Biology, University of Connecticut, Storrs, Connecticut, United States of America
Abstract
Background: Inhalation of crystalline silica is known to cause an inflammatory reaction and chronic exposure leads to lung
fibrosis and can progress into the disease, silicosis. Cultured macrophages bind crystalline silica particles, phagocytose
them, and rapidly undergo apoptotic and necrotic death. The mechanism by which particles are bound and internalized and
the reason particles are toxic is unclear. Amorphous silica has been considered to be a less toxic form, but this view is
controversial. We compared the uptake and toxicity of amorphous silica to crystalline silica.
Methodology/Principal Findings: Amorphous silica particles are phagocytosed by macrophage cells and a single
internalized particle is capable of killing a cell. Fluorescent dextran is released from endo-lysosomes within two hours after
silica treatment and Caspase-3 activation occurs within 4 hours. Interestingly, toxicity is specific to macrophage cell lines.
Other cell types are resistant to silica particle toxicity even though they internalize the particles. The large and uniform size
of the spherical, amorphous silica particles allowed us to monitor them during the uptake process. In mCherry-actin
transfected macrophages, actin rings began to form 1-3 minutes after silica binding and the actin coat disassembled rapidly
following particle internalization. Pre-loading cells with fluorescent dextran allowed us to visualize the fusion of
phagosomes with endosomes during internalization. These
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