Williams Wes, Nix Paola, Bastiani Michael
Department of Biology, University of Utah, USA.
J Vis Exp. 2011 Nov 15(57):3331. doi: 10.3791/3331.
Laser axotomy followed by time-lapse microscopy is a sensitive assay for axon regeneration phenotypes in C. elegans(1). The main difficulty of this assay is the perceived cost ($25-100K) and technical expertise required for implementing a laser ablation system(2,3). However, solid-state pulse lasers of modest costs (<$10K) can provide robust performance for laser ablation in transparent preparations where target axons are "close" to the tissue surface. Construction and alignment of a system can be accomplished in a day. The optical path provided by light from the focused condenser to the ablation laser provides a convenient alignment guide. An intermediate module with all optics removed can be dedicated to the ablation laser and assures that no optical elements need be moved during a laser ablation session. A dichroic in the intermediate module allows simultaneous imaging and laser ablation. Centering the laser beam to the outgoing beam from the focused microscope condenser lens guides the initial alignment of the system. A variety of lenses are used to condition and expand the laser beam to fill the back aperture of the chosen objective lens. Final alignment and testing is performed with a front surface mirrored glass slide target. Laser power is adjusted to give a minimum size ablation spot (<1 um). The ablation spot is centered with fine adjustments of the last kinematically mounted mirror to cross hairs fixed in the imaging window. Laser power for axotomy will be approximately 10X higher than needed for the minimum ablation spot on the target slide (this may vary with the target you use). Worms can be immobilized for laser axotomy and time-lapse imaging by mounting on agarose pads (or in microfluidic chambers(4)). Agarose pads are easily made with 10% agarose in balanced saline melted in a microwave. A drop of molten agarose is placed on a glass slide and flattened with another glass slide into a pad approximately 200 um thick (a single layer of time tape on adjacent slides is used as a spacer). A "Sharpie" cap is used to cut out a uniformed diameter circular pad of 13 mm. Anesthetic (1 ul Muscimol 20mM) and Microspheres (Chris Fang-Yen personal communication) (1 ul 2.65% Polystyrene 0.1 um in water) are added to the center of the pad followed by 3-5 worms oriented so they are lying on their left sides. A glass coverslip is applied and then Vaseline is used to seal the coverslip and prevent evaporation of the sample.
激光切断术结合延时显微镜技术是一种用于检测秀丽隐杆线虫轴突再生表型的灵敏方法(1)。该方法的主要难点在于人们认为实施激光消融系统成本高昂(2.5万至10万美元)且需要专业技术(2,3)。然而,成本适中(低于1万美元)的固态脉冲激光器在目标轴突“靠近”组织表面的透明样本中进行激光消融时能提供强大的性能。系统的搭建和校准一天内即可完成。从聚焦聚光镜到消融激光的光路提供了便捷的校准指南。一个移除了所有光学元件的中间模块可专门用于消融激光,并确保在激光消融过程中无需移动任何光学元件。中间模块中的一个二向色镜可实现同时成像和激光消融。将激光束与聚焦显微镜聚光镜射出的光束对中可引导系统的初始校准。使用各种透镜来调节和扩展激光束,以填充所选物镜的后孔径。最终校准和测试使用前表面镀有反射膜的载玻片靶标进行。调整激光功率以产生最小尺寸的消融光斑(<1微米)。通过对最后一个以运动学方式安装的镜子进行微调,使消融光斑与固定在成像窗口中的十字线对中。用于轴突切断术的激光功率将比在靶标载玻片上产生最小消融光斑所需的功率高约10倍(这可能因所用靶标而异)。可通过将线虫安装在琼脂糖垫上(或微流控腔室中(4))来固定线虫以进行激光轴突切断术和延时成像。琼脂糖垫很容易用平衡盐溶液中10%的琼脂糖在微波炉中熔化制成。将一滴熔化的琼脂糖放在载玻片上,用另一载玻片将其压平成约200微米厚的垫(相邻载玻片上的单层时间胶带用作间隔物)。用“Sharpie”笔帽切出直径为13毫米的均匀圆形垫。在垫的中心加入麻醉剂(1微升20毫摩尔的蝇蕈醇)和微球(克里斯·方 - 严个人交流)(1微升水中2.65%的0.1微米聚苯乙烯),然后放入3 - 5条线虫,使它们左侧朝上。盖上盖玻片,然后用凡士林密封盖玻片以防止样品蒸发。
