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通过电子能量损失谱(EELS)对水合和脱水冷冻切片进行厚度测量。

Thickness measurement of hydrated and dehydrated cryosections by EELS.

作者信息

Shi S, Sun S, Andrews S B, Leapman R D

机构信息

Biomedical Engineering and Instrumentation Program, NCRR, National Institutes of Health, Bethesda, Maryland 20892, USA.

出版信息

Microsc Res Tech. 1996 Feb 15;33(3):241-50. doi: 10.1002/(SICI)1097-0029(19960215)33:3<241::AID-JEMT1>3.0.CO;2-T.

Abstract

Electron energy-loss spectroscopy (EELS) provides a useful method for determining the thickness of frozen-hydrated and dehydrated cryosections in terms of the inelastic mean free path. Cryosection thickness is an important parameter because plural inelastic scattering limits the sensitivity of elemental microanalysis based on core-loss EELS, and because overlapping structures can affect interpretation of microanalytical data as well as the quality of electron images. The purpose of this work was to establish the minimum practical thickness for cutting cryosections and to explain the measured values for hydrated and dehydrated specimens. Hydrated sections were typically found to be between 1.5-2.5 times thicker than expected from the nominal microtome setting; this difference can be largely explained by compression during cutting. Comparison of micrographs from hydrated and dehydrated cryosections of rapidly-frozen, vitrified liver revealed a lateral shrinkage of approximately 20% on drying. The measured compression and shrinkage factors are consistent with dark-field scanning transmission electron microscopy (STEM) mass measurements on freeze-dried sections. Freeze-dried cryosections, cut to a nominal thickness of 90 nm and supported on thin Formvar/carbon films, had a relative thickness t/lambda i in the range of 0.5 for cytoplasm to 0.9 for mitochondria when analyzed at 100 keV beam energy. Mass loss of approximately 30% occurring at high electron dose enabled useful core-loss spectra to be recorded even from high-mass compartments such as mitochondria without excessive plural scattering.

摘要

电子能量损失谱(EELS)提供了一种有用的方法,可根据非弹性平均自由程来确定冷冻水合和脱水冷冻切片的厚度。冷冻切片厚度是一个重要参数,这是因为多次非弹性散射会限制基于芯损EELS的元素微分析的灵敏度,还因为重叠结构会影响微分析数据的解释以及电子图像的质量。这项工作的目的是确定切割冷冻切片的最小实际厚度,并解释水合和脱水标本的测量值。通常发现水合切片比标称切片机设置预期的厚度厚1.5至2.5倍;这种差异在很大程度上可以通过切割过程中的压缩来解释。对快速冷冻、玻璃化肝脏的水合和脱水冷冻切片的显微照片进行比较,结果显示干燥后横向收缩约20%。测得的压缩和收缩因子与冷冻干燥切片的暗场扫描透射电子显微镜(STEM)质量测量结果一致。在100 keV束能量下分析时,标称厚度为90 nm并支撑在薄福尔马膜/碳膜上的冷冻干燥冷冻切片,其相对厚度t/λi在细胞质中为0.5至线粒体中为0.9的范围内。即使在高质量隔室(如线粒体)中,在高电子剂量下发生约30%的质量损失,也能记录有用的芯损谱,而不会出现过多的多次散射。

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