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一种用于测量细胞内钙离子的紫外激光扫描共聚焦显微镜。

A UV laser-scanning confocal microscope for the measurement of intracellular Ca2+.

作者信息

Kuba K, Hua S Y, Hayashi T

机构信息

Department of Physiology, Saga Medical School, Japan.

出版信息

Cell Calcium. 1994 Sep;16(3):205-18. doi: 10.1016/0143-4160(94)90023-x.

Abstract

Modifications to the optics of a conventional confocal laser-scanning microscope were made to allow imaging intracellular Ca(2+)-dependent fluorescence with a UV laser (351 or 364 nm). Modifications included: (1) a chromatic compensation lens in the laser path; (2) the design of a practically achromatic relay lens; (3) a longer tube length for the objective; and (4) highly reflective mirrors maximizing fluorescence measurement. This UV laser-scanning confocal microscope (UV-CLSM) yielded a lateral resolution of < 0.3 micron and an axial resolution of < 1.5 microns and a relevant field size of 100 microns in diameter for a 40X objective). The effects of varying the focal length of a compensation lens, the degree of the correction for the coverglass thickness of objective and the detector aperture size on the quality of image formation were examined. Finally, UV-CLSM revealed optical sections of fine and complex structures of bullfrog sympathetic neurones loaded with a Ca(2+)-sensitive fluorescent probe. Changes in intracellular free Ca2+ distribution in response to high [K+] or caffeine were demonstrated. In addition, an increase in the intracellular concentration of caffeine applied externally was clearly imaged in space and time and distinguished from a resultant rise in [Ca2+]i. Thus, the UV-CLSM developed is suitable for ratiometric intracellular Ca2+ measurements and other biological studies.

摘要

对传统共聚焦激光扫描显微镜的光学系统进行了改进,以便使用紫外激光(351或364纳米)对细胞内钙依赖性荧光进行成像。改进措施包括:(1)在激光路径中设置一个色差补偿透镜;(2)设计一个实际消色差的中继透镜;(3)增加物镜的镜筒长度;(4)使用高反射镜以最大化荧光测量。这种紫外激光扫描共聚焦显微镜(UV-CLSM)的横向分辨率小于0.3微米,轴向分辨率小于1.5微米,对于40倍物镜,相关视场直径为100微米。研究了补偿透镜焦距变化、物镜盖玻片厚度校正程度和探测器孔径大小对成像质量的影响。最后,UV-CLSM显示了加载钙敏感荧光探针的牛蛙交感神经元精细和复杂结构的光学切片。证明了细胞内游离钙分布对高钾或咖啡因的响应变化。此外,外部施加的咖啡因细胞内浓度的增加在空间和时间上都能清晰成像,并与由此导致的细胞内钙浓度升高区分开来。因此,所开发的UV-CLSM适用于细胞内钙的比率测量和其他生物学研究。

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