CONTROL OF CELL ELASTICITY BY THE ACTIN CORTEX
肌动蛋白皮层对细胞弹性的控制
基本信息
- 批准号:6164030
- 负责人:
- 金额:$ 9.59万
- 依托单位:
- 依托单位国家:美国
- 项目类别:
- 财政年份:1999
- 资助国家:美国
- 起止时间:1999-03-18 至 2004-02-29
- 项目状态:已结题
- 来源:
- 关键词:
项目摘要
Eukaryotic cells reversibly assemble the actin protein into filaments
which are then arrayed by accessory proteins into the actin cytoskeleton
(AC). Disruption of the AC is associated with significant cell
softening and in the case of migrating cells it also results in loss of
motility. The exact role of the AC in the mechanical strength of cells
is not fully understood. The AC can be roughly divided into two
superimposing elastic elements: a homogeneous network of protein
filaments predominantly underlying the plasma membrane and stress fibers
which span the cell interior. This proposal will focus on the
homogeneous cortical part of the AC. The proposed research takes two
novel approaches: (1) in vitro measurements will investigate how the
elastic response of actin networks is generated on the microscopic level
of a single actin filament in a network and (2) in vivo measurements of
the specific elasticity of the cortical AC will determine the role of
actin networks for whole cell elasticity.
Simultaneous measurements of the elastic properties of F-actin
solutions/gels and fluorescence microscopy of individual constituent
actin filaments under shear will provide detailed characterization of
the interactions between actin filaments which cause the elastic
behavior. These data will distinguish between recently suggested models
and lead to quantitative predictions of the strength of the AC as a
function of its composition. This knowledge will improve the
understanding of cell motility. A particular focus will be on how
transient crosslinkers and molecular motors modulate the strength of
these networks. Preliminary results indicate that inactive myosin II
acts as a crosslinker, whereas active myosin liquefies F-actin networks
in the absence of other crosslinking proteins. The dependence of the
mechanical strength on filament stiffness will be investigated as an
additional possibility in modulating the strength of actin networks.
To accurately measure cell elasticity of large, statistically
significant numbers of cells, an optical tool has been developed to non-
destructively stretch single cells between two beams of a laser.
Measurements of cells in suspension, which show a peripheral AC but no
stress fibers, will allow the PI to quantify the contribution of actin
networks to cell elasticity. The contribution of these networks to the
overall mechanical strength of cells will be determined by measuring the
elasticity of cells with varying ACs. This also allows determination
of the relevance of in vitro research on homogeneous actin networks for
the cell cytoskeleton. A primary focus will be the extent to which
malignant transformation of cells by oncogenic vectors -which is
correlated with changes of the AC - can be monitored by cell elasticity
measurements.
真核细胞可逆地将肌动蛋白组装成细丝
项目成果
期刊论文数量(0)
专著数量(0)
科研奖励数量(0)
会议论文数量(0)
专利数量(0)
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JOSEF A KAS其他文献
JOSEF A KAS的其他文献
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肌动蛋白和肌动蛋白结合蛋白的结构/相互作用
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$ 9.59万 - 项目类别:














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