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Direct Manipulation and Observation of the Rotational Motion of Single Optically Trapped Microparticles and Biological Cells in Microvortices

机译:直接操纵和观察微旋涡中单个光学陷阱微粒和生物细胞的旋转运动

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This paper describes a method for manipulating and monitoring the rotational motion of single, optically trapped microparticles and living cells in a microvortex. To induce rotation, we placed the microparticle at the center of rotation of the vortex and used the recirculating fluid flow to drive rotation. We have monitored the rotation of single beads (which ranged in diameter from a few micrometers to tens of micrometers) and living cells in a microvortex. To follow the rotation of a smooth and symmetrically shaped bead, we first ablated a small region (~1 μm) on the bead. An Ar~(+) laser was then tightly focused (~0.5-μm spot size) onto the bead, and rotation was tracked by recording changes in the level of backscattered laser light as the ablated region repeatedly transited the laser focus. Using this method, we have followed bead rotation that varied in frequency from 0.15 to 100 Hz and have studied the effect of bead diameter on the rate of rotation at a given fluid flow rate. To monitor the rotation of single living cells, we selectively stained portions of B-lymphocytes with the fluorescent dye DiOC_(6). We observed rotation by following changes in the fluorescence signal as the dye-stained region transited the laser focal volume. This technique provides a simple and sensitive method for controlling and monitoring the rotational motion of microparticles in a microfluidic environment.
机译:本文介绍了一种用于操纵和监视微旋涡中单个被光学捕获的微粒和活细胞的旋转运动的方法。为了诱导旋转,我们将微粒置于涡旋的旋转中心,并使用再循环流体驱动旋转。我们已经监测了单个微珠(直径范围从几微米到几十微米)和活细胞在微涡旋中的旋转。为了跟随光滑且对称形状的珠子的旋转,我们首先烧蚀了珠子上的一个小区域(〜1μm)。然后将Ar〜(+)激光紧密聚焦(光斑尺寸约0.5μm),并通过记录消融区域重复转变激光聚焦时反向散射激光水平的变化来跟踪旋转。使用此方法,我们跟踪了从0.15到100 Hz的频率变化的磁珠旋转,并研究了在给定的流体流速下,磁珠直径对旋转速度的影响。为了监测单个活细胞的旋转,我们用荧光染料DiOC_(6)选择性地染色了B淋巴细胞的一部分。当染料染色的区域通过激光焦距时,我们通过跟踪荧光信号的变化观察到旋转。该技术提供了一种简单而灵敏的方法,用于控制和监视微流体环境中微粒的旋转运动。

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