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Developing new optical imaging techniques for single particle and molecule tracking in live cells

机译:开发新的光学成像技术以追踪活细胞中的单个粒子和分子

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摘要

Differential interference contrast (DIC) microscopy is a far-field as well as wide-field optical imaging technique. Since it is non-invasive and requires no sample staining, DIC microscopy is suitable for tracking the motion of target molecules in live cells without interfering their functions. In addition, high numerical aperture objectives and condensers can be used in DIC microscopy. The depth of focus of DIC is shallow, which gives DIC much better optical sectioning ability than those of phase contrast and dark field microscopies. In this work, DIC was utilized to study dynamic biological processes including endocytosis and intracellular transport in live cells.The suitability of DIC microscopy for single particle tracking in live cells was first demonstrated by using DIC to monitor the entire endocytosis process of one mesoporous silica nanoparticle (MSN) into a live mammalian cell. By taking advantage of the optical sectioning ability of DIC, we recorded the depth profile of the MSN during the endocytosis process. The shape change around the nanoparticle due to the formation of a vesicle was also captured.DIC microscopy was further modified that the sample can be illuminated and imaged at two wavelengths simultaneously. By using the new technique, noble metal nanoparticles with different shapes and sizes were selectively imaged. Among all the examined metal nanoparticles, gold nanoparticles in rod shapes were found to be especially useful. Due to their anisotropic optical properties, gold nanorods showed as diffraction-limited spots with disproportionate bright and dark parts that are strongly dependent on their orientation in the 3D space. Gold nanorods were developed as orientation nanoprobes and were successfully used to report the self-rotation of gliding microtubules on kinesin coated substrates. Gold nanorods were further used to study the rotational motions of cargoes during the endocytosis and intracellular transport processes in live mammalian cells. New rotational information was obtained: (1) during endocytosis, cargoes lost their rotation freedom at the late stage of internalization; (2) cargoes performed train-like motion when they were transported along the microtubule network by motor proteins inside live cells; (3) During the pause stage of fast axonal transport, cargoes were still bound to the microtubule tracks by motor proteins.Total internal reflection fluorescence microscopy (TIRFM) is another non-invasive and far-field optical imaging technique. Because of its near-field illumination mechanism, TIRFM has better axial resolution than epi-fluorescence microscopy and confocal microscopy. In this work, an auto-calibrated, prism type, angle-scanning TIRFM instrument was built. The incident angle can range from subcritical angles to nearly 90y, with an angle interval less than 0.2y. The angle precision of the new instrument was demonstrated through the finding of the surface plasmon resonance (SPR) angle of metal film coated glass slide. The new instrument improved significantly the precision in determining the axial position. As a result, the best obtained axial resolution was ~ 8 nm, which is better than current existing instruments similar in function.The instrument was further modified to function as a pseudo TIRF microscope. The illumination depth can be controlled by changing the incident angle of the excitation laser beam or adjusting the horizontal position of the illumination laser spot on the prism top surface. With the new technique, i.e., variable-illumination-depth pseudo TIRF microscopy, the whole cell body from bottom to top was scanned.
机译:差分干涉对比(DIC)显微镜是一种远场和广域光学成像技术。由于DIC显微镜是非侵入性的并且不需要样品染色,因此适合于追踪活细胞中目标分子的运动而不会干扰它们的功能。另外,高数值孔径的物镜和聚光镜可用于DIC显微镜。 DIC的聚焦深度较浅,这使DIC的光学切片能力比相衬对比度和暗场显微技术更好。在这项工作中,DIC用于研究动态生物学过程,包括活细胞的内吞作用和细胞内转运.DIC显微镜首先通过使用DIC监测一个介孔二氧化硅纳米颗粒的整个内吞作用过程证明了其对活细胞中单颗粒追踪的适用性。 (MSN)进入活的哺乳动物细胞。通过利用DIC的光学切片能力,我们记录了内吞过程中MSN的深度分布。还捕获了由于囊泡形成而导致的纳米颗粒周围的形状变化。进一步修改了DIC显微镜,可以同时在两个波长下对样品进行照明和成像。通过使用新技术,可以选择性地成像具有不同形状和大小的贵金属纳米粒子。在所有检查过的金属纳米颗粒中,发现棒状的金纳米颗粒特别有用。由于其各向异性的光学特性,金纳米棒显示为衍射受限的斑点,其亮和暗部分不成比例,强烈依赖于它们在3D空间中的方向。金纳米棒被开发为定向纳米探针,并成功地用于报道在驱动蛋白包被的基底上滑动微管的自转。金纳米棒还被用于研究哺乳动物活细胞内吞和细胞内运输过程中货物的旋转运动。获得了新的旋转信息:(1)在胞吞过程中,货物在内化后期失去了旋转自由度; (2)货物通过活细胞内的运动蛋白沿微管网络运输时呈火车状运动; (3)在快速轴突运输的暂停阶段,货物仍被运动蛋白束缚在微管轨道上。全内反射荧光显微镜(TIRFM)是另一种无创且远场光学成像技术。由于其近场照明机制,TIRFM具有比落射荧光显微镜和共聚焦显微镜更好的轴向分辨率。在这项工作中,制造了一种自动校准的棱镜型角度扫描TIRFM仪器。入射角的范围可以从亚临界角到近90y,且角度间隔小于0.2y。通过发现涂有金属膜的玻璃载玻片的表面等离振子共振(SPR)角,证明了新仪器的角度精度。新仪器大大提高了确定轴向位置的精度。结果,获得的最佳轴向分辨率为〜8 nm,这比当前功能相似的现有仪器要好。该仪器经过了进一步修改,可以用作伪TIRF显微镜。照明深度可以通过改变激发激光束的入射角或调节照明光斑在棱镜顶面上的水平位置来控制。利用新技术,即可变照明深度的伪TIRF显微镜,从下到上扫描了整个细胞体。

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    Sun, Wei;

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  • 年度 2010
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  • 正文语种 en
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