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Bridging the resolution gap: Imaging the same transcription factories in cryosections by light and electron microscopy.

Abstract:
The resolution of conventional light microscopy is limited to approximately 200 nm in the x- and y-axes and >500 nm in the z-axis. A simple way of improving z-axis resolution is to analyze thin sections of 100-200 nm. The utility of such an approach is illustrated by reference to transcription sites imaged in cryosections of human nuclei. Cells are permeabilized, allowed to extend nascent transcripts in Br-UTP, fixed, cryosectioned, and Br-RNA-immunolabeled with fluorochromes and gold particles. As expected, physical sectioning improves resolution and brings other advantages. First, sections allow improved antibody access and better immunolabeling. Second, more sites (with a more representative range of intensities) can now be resolved against lower backgrounds, facilitating quantitative analysis. Third, problems associated with chromatic aberration when two differently colored images of the same objects are collected can be sidestepped by refocusing between image collection. Fourth, exactly the same sites can be imaged by light and electron microscopy, allowing direct comparison between the two techniques. Immunogold labeling and electron microscopy provided the most accurate counts of site number. The results confirm that nascent transcripts in the nucleoplasm are confined to several thousand sites, or "factories," with diameters of approximately 40 nm. (J Histochem Cytochem 47:471-480, 1999)
Publication status:
Published

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Publisher copy:
10.1177/002215549904700405

Authors

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Institution:
University of Oxford
Division:
MSD
Department:
Pathology Dunn School
Role:
Author


Journal:
journal of histochemistry and cytochemistry : official journal of the Histochemistry Society More from this journal
Volume:
47
Issue:
4
Pages:
471-480
Publication date:
1999-04-01
DOI:
EISSN:
1551-5044
ISSN:
0022-1554


Language:
English
Keywords:
Pubs id:
pubs:28877
UUID:
uuid:f2560f8a-5865-4887-a3db-7b80a041e943
Local pid:
pubs:28877
Source identifiers:
28877
Deposit date:
2012-12-19
ARK identifier:

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