首页> 美国卫生研究院文献>The Journal of Biophysical and Biochemical Cytology >Unconfined lateral diffusion and an estimate of pericellular matrix viscosity revealed by measuring the mobility of gold-tagged lipids
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Unconfined lateral diffusion and an estimate of pericellular matrix viscosity revealed by measuring the mobility of gold-tagged lipids

机译:通过测量带有金标记的脂质的迁移率可以发现无限制的横向扩散和对细胞周围基质粘度的估计

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摘要

Nanovid (video-enhanced) microscopy was used to determine whether lateral diffusion in the plasma membrane of colloidal gold-tagged lipid molecules is confined or is unrestricted. Confinement could be produced by domains within the plane of the plasma membrane or by filamentous barriers within the pericellular matrix. Fluorescein- phosphatidylethanolamine (F1-PE), incorporated into the plasma membranes of cultured fibroblasts, epithelial cells and keratocytes, was labeled with 30-nm colloidal gold conjugated to anti-fluorescein (anti-F1). The trajectories of the gold-labeled lipids were used to compute diffusion coefficients (DG) and to test for restricted motion. On the cell lamella, the gold-labeled lipids diffused freely in the plasma membrane. Since the gold must move through the pericellular matrix as the attached lipid diffuses in the plasma membrane, this result suggests that any extensive filamentous barriers in the pericellular matrix are at least 40 nm from the plasma membrane surface. The average diffusion coefficients ranged from 1.1 to 1.7 x 10(-9) cm2/s. These values were lower than the average diffusion coefficients (DF) (5.4 to 9.5 x 10(-9) cm2/s) obtained by FRAP. The lower DG is partially due to the pericellular matrix as demonstrated by the result that heparinase treatment of keratocytes significantly increased DG to 2.8 x 10(-9) cm2/s, but did not affect DF. Pericellular matrix viscosity was estimated from the frictional coefficients computed from DG and DF and ranged from 0.5 to 0.9 poise for untreated cells. Heparinase treatment of keratocytes decreased the apparent viscosity to approximately 0.1 poise. To evaluate the presence of domains or barriers, the trajectories and corresponding mean square displacement (MSD) plots of gold-labeled lipids were compared to the trajectories and MSD plots resulting from computer simulations of random walks within corrals. Based on these comparisons, we conclude that, if there are domains limiting the diffusion of F1-PE, most are larger than 5 microns in diameter.
机译:Nanovid(视频增强)显微镜用于确定胶体金标记脂质分子在质膜中的侧向扩散是受限制的还是不受限制的。限制可由质膜平面内的区域或细胞周围基质内的丝状屏障产生。掺入培养的成纤维细胞,上皮细胞和角质形成细胞质膜的荧光素-磷脂酰乙醇胺(F1-PE)用与抗荧光素偶联的30-nm胶体金标记(抗F1)。金标脂质的轨迹用于计算扩散系数(DG)并测试运动受限。在细胞层上,金标记的脂质在质膜中自由扩散。由于当附着的脂质在质膜中扩散时,金必须穿过细胞周质基质,因此该结果表明,细胞周质基质中任何广泛的丝状屏障距离质膜表面至少40 nm。平均扩散系数为1.1至1.7 x 10(-9)cm2 / s。这些值低于通过FRAP获得的平均扩散系数(DF)(5.4至9.5 x 10(-9)cm2 / s)。较低的DG部分是由于细胞周基质所致,结果表明,肝素酶处理角质形成细胞可将DG显着增加至2.8 x 10(-9)cm2 / s,但不影响DF。根据由DG和DF计算的摩擦系数估计细胞周基质粘度,对于未处理的细胞,其范围为0.5到0.9泊。肝素酶处理的角化细胞将表观粘度降低至约0.1泊。为了评估域或障碍的存在,将金标记脂质的轨迹和相应的均方位移(MSD)图与畜栏内随机游走的计算机模拟所得到的轨迹和MSD图进行了比较。基于这些比较,我们得出结论,如果存在限制F1-PE扩散的区域,则大多数直径大于5微米。

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