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甲醇浸泡可降低多光子激光扫描显微镜中使用的长波长水浸透镜的球差。

Methanol immersion reduces spherical aberration of water dipping lenses at long wavelengths used in multi-photon laser scanning microscopy.

作者信息

Norris Greg, Gebril Ayman, Ferro Valerie A, McConnell Gail

机构信息

Centre for Biophotonics, Strathclyde Institute for Pharmaceutical and Biomedical Sciences, University of Strathclyde, 161 Cathedral Street, Glasgow, G4 0RE, UK.

出版信息

Biomed Opt Express. 2012 Dec 1;3(12):3314-24. doi: 10.1364/BOE.3.003314. Epub 2012 Nov 21.

Abstract

Dipping objectives were tested for multi-photon laser scanning microscopy, since their large working distances are advantageous for thick specimens and the absence of a coverslip facilitates examination of living material. Images of fluorescent bead specimens, particularly at wavelengths greater than 850 nm showed defects consistent with spherical aberration. Substituting methanol for water as the immersion medium surrounding the beads corrected these defects and produced an increase in fluorescence signal intensity. The same immersion method was applied to two representative biological samples of fixed tissue: mouse brain labeled with FITC for tubulin and mouse gut in which the Peyer's patches were labeled with Texas Red bilosomes. Tissue morphology was well preserved by methanol immersion of both tissues; the two-photon-excited fluorescence signal was six times higher than in water and the depth of penetration of useful imaging was doubled. No modification of the microscope was needed except the provision of a ring to retain a sufficient depth of methanol for imaging.

摘要

浸液物镜已针对多光子激光扫描显微镜进行了测试,因为其较大的工作距离对厚标本有利,且无需盖玻片便于对活体材料进行检查。荧光珠标本的图像,特别是在波长大于850 nm时,显示出与球差一致的缺陷。用甲醇代替水作为珠子周围的浸没介质纠正了这些缺陷,并使荧光信号强度增加。相同的浸没方法应用于两个固定组织的代表性生物样本:用异硫氰酸荧光素(FITC)标记微管蛋白的小鼠脑和其中派伊尔氏淋巴集结用德克萨斯红双脂质体标记的小鼠肠道。两种组织经甲醇浸没后,组织形态均得到良好保存;双光子激发荧光信号比在水中高六倍,有用成像的穿透深度增加了一倍。除了提供一个环以保留足够深度的甲醇用于成像外,无需对显微镜进行任何修改。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/984b/3521300/fb6e18fad711/boe-3-12-3314-g001.jpg

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