Weaver F E, Polster H, Febboriello P, Sheetz M P, Schmid-Schonbein H, Koppel D E
Department of Biochemistry, University of Connecticut Health Center, Farmington 06032.
Biophys J. 1990 Dec;58(6):1427-36. doi: 10.1016/S0006-3495(90)82488-7.
Normal nonnucleated erythrocytes subjected to continuous hydrodynamic shear exhibit membrane deformation or "tanktreading," a process important for reduction of the bulk viscosity of circulating blood. To characterize the effect of this unique process on the erythrocyte membrane we have measured the lateral diffusion of band 3 during tanktreading. Band 3 is normally constrained through interactions with the spectrin-actin cytoskeleton, therefore, any significant disruption of these interactions would result in alterations in band 3 dynamics. Band 3 of human erythrocytes was labeled with dichlorotriazinyl amino fluorescein. After laser photobleaching of an equatorial stripe, fluorescence images were recorded from cells in the presence or absence of shear. The amplitude of induced nonuniformity in the surface distribution of fluorescence was calculated directly from images of unsheared cells. In shear the bleached line rotated with the tanktreading motion of the cells. The surface integral of fluorescence oscillated with this motion. For this case, the amplitude of photobleaching-induced nonuniformity was defined as the amplitude at the fundamental frequency of fast Fourier transforms in time of the oscillations. Shear stress-induced membrane flow did not interrupt the linkage of band 3 with the erythrocyte cytoskeleton. Diffusion coefficient and mobile fraction (1.5 +/- 0.5 x 10(-10) cm2/s and 54 +/- 11%, respectively) were unaffected by shear. The rate of fluorescence recovery of cells in shear was also similar at the centers and at the edges, where in-plane shear forces are maximal.
正常无核红细胞在持续流体动力剪切作用下会发生膜变形或“罐体 tread”现象,这一过程对于降低循环血液的整体粘度很重要。为了表征这一独特过程对红细胞膜的影响,我们测量了罐体 tread 过程中带 3 的横向扩散。带 3 通常通过与血影蛋白 - 肌动蛋白细胞骨架的相互作用而受到限制,因此,这些相互作用的任何显著破坏都会导致带 3 动力学的改变。人红细胞的带 3 用二氯三嗪基氨基荧光素进行标记。在对赤道条纹进行激光光漂白后,在有或无剪切的情况下记录细胞的荧光图像。直接从未受剪切的细胞图像计算荧光表面分布中诱导不均匀性的幅度。在剪切作用下,漂白线随着细胞的罐体 tread 运动而旋转。荧光的表面积分随此运动而振荡。对于这种情况,光漂白诱导不均匀性的幅度定义为振荡时间的快速傅里叶变换基频处的幅度。剪切应力诱导的膜流动并未中断带 3 与红细胞细胞骨架的连接。扩散系数和可移动部分(分别为 1.5±0.5×10⁻¹⁰ cm²/s 和 54±11%)不受剪切影响。在剪切作用下,细胞中心和边缘的荧光恢复速率也相似,而边缘处的面内剪切力最大。