Diamonds are a cryosectioner's best friend

Michel, Martin; Gnägi, Helmut; Müller, Martin

doi:10.1111/j.1365-2818.1992.tb01506.x

Cited by 56 publications

(35 citation statements)

References 32 publications

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“…Cryosectioning was performed as described previously (Michel et al, 1992;Buchanan et al, 1993). In brief, cryosections were cut en face from the well frozen surface (Ͻ20 m deep) of previously marked regions of CA3 st. lucidum, trimmed to a 0.25 ϫ 0.25 mm block face.…”

Section: Methodsmentioning

confidence: 99%

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Activity-Dependent Calcium Sequestration in Dendrites of Hippocampal Neurons in Brain Slices

Leapman

et al. 1997

J. Neurosci.

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Synaptic activity-dependent changes in the spatio-temporal distribution of calcium ions regulate important neuronal functions such as dendritic integration and synaptic plasticity, but the processes that terminate the free Ca 2ϩ transients associated with these changes remain unclear. We have characterized at the electron microscopic level the intracellular compartments involved in buffering free Ca 2ϩ transients in dendritic cytoplasm of CA3 neurons by measuring the larger changes in the concentrations of total Ca that persist for several minutes after neuronal activity. Quantitative energy-dispersive x-ray microanalysis of cryosections from hippocampal slice cultures rapidly frozen 3 min after afferent synaptic activity identified a subset of dendritic endoplasmic reticulum (ER) as a highcapacity Ca 2ϩ buffer. Calcium sequestration by cisterns of this subset of ER was graded, reversible, and dependent on a thapsigargin-sensitive Ca 2ϩ -ATPase. Sequestration was so robust that after repetitive high-frequency stimulation the Ca content of responsive ER cisterns increased as much as 20-fold. These results demonstrate that a subpopulation of ER is the major dendritic Ca sequestration compartment in the minutes after neuronal activity.

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Section: Methodsmentioning

confidence: 99%

“…These slice cultures are also well suited for en face cryosectioning, which, using newer sectioning techniques (Michel et al, 1992;Buchanan et al, 1993) produces uniform, truly ultrathin cryosections in which even small organelles such as cisterns of ER are unambiguously recognizable (Fig. 2).…”

Section: Methodological Considerationsmentioning

confidence: 99%

Activity-Dependent Calcium Sequestration in Dendrites of Hippocampal Neurons in Brain Slices

Leapman

et al. 1997

J. Neurosci.

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“…Over the last decade, however, several major problems have been largely ameliorated by significant advances in instrumentation and techniques. Among the most important of these are: (1) the ability to prepare high-quality truly ultrathin cryosections of unfixed, rapidly frozen tissues that have structural detail comparable to conventional preparations Michel et al, 1992), while still retaining native distributions of diffusible elements; and (2) improved detectors and analytical microscopes (e.g., Leapman et al, 1993) that can achieve, in a clean environment, the high sensitivity and resolution necessary to characterize biologically relevant changes in cellular [Ca].…”

Section: Introductionmentioning

confidence: 99%

Correlated measurements of free and total intracellular calcium concentration in central nervous system neurons

Pozzo-Miller

Pivovarova

Connor

et al. 1999

Microsc. Res. Tech.

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“…The observation by cryo-electron microscopy of thin cryosections of vitrified specimens makes it possible to observe samples in their native hydrated state without the usual artefacts of chemical fixation, dehydration and staining (Dubochet et al, 1988;Michel et al, 1991Michel et al, , 1992Sartori & Salamin Michel, 1994). The basic requirement for this method is that the specimen must be vitrified, i.e.…”

Section: Introductionmentioning

confidence: 99%

Electron‐beam‐induced amorphization of ice III or IX obtained by high‐pressure freezing

Sartori

Bednář

Dubochet

1996

Journal of Microscopy

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SummaryCryo-electron microscopy of vitrified specimens makes it possible to observe fully hydrated biological samples unimpaired by chemical fixation, staining and dehydration. Highpressure freezing represents important progress since it allows a 10-fold increase in the vitrification depth. Highpressure freezing can also induce the formation of undesirable high-pressure forms of ice. We show that ice III or IX is amorphized under the electron beam at a dose of about 2400 electrons nm ÿ 2 and that the resulting amorphous ice is similar to the vitreous water obtained by high-pressure freezing.

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Diamonds are a cryosectioner's best friend

Cited by 56 publications

References 32 publications

Activity-Dependent Calcium Sequestration in Dendrites of Hippocampal Neurons in Brain Slices

Activity-Dependent Calcium Sequestration in Dendrites of Hippocampal Neurons in Brain Slices

Correlated measurements of free and total intracellular calcium concentration in central nervous system neurons

Electron‐beam‐induced amorphization of ice III or IX obtained by high‐pressure freezing

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