Nuclear organization and dynamics of transcription sites in rat sensory ganglia neurons detected by incorporation of 5′-fluorouridine into nascent RNA

In this study we have used the transcription assay with 5′-fluorouridine incorporation into nascent RNA to analyze the nuclear organization and dynamics of transcription sites in rat trigeminal ganglia neurons. The 5′-FU administrated by i.p. injection was successfully incorporated into nuclear doma...

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Bibliographic Details
Published in:Neuroscience 2006-01, Vol.140 (2), p.453-462
Main Authors: Casafont, I., Navascués, J., Pena, E., Lafarga, M., Berciano, M.T.
Format: Article
Language:English
Subjects:
actinomycin D
Animals
Biological and medical sciences
Biological Assay - methods
Cajal bodies
Cell Nucleolus - genetics
Cell Nucleolus - metabolism
Cell Nucleolus - ultrastructure
Cell Nucleus - genetics
Cell Nucleus - metabolism
Cell Nucleus - ultrastructure
Dactinomycin - pharmacology
DNA repair
DNA Repair - physiology
Euchromatin - genetics
Euchromatin - metabolism
Euchromatin - ultrastructure
Fundamental and applied biological sciences. Psychology
Gene Expression - physiology
Gene Silencing - physiology
Histones - metabolism
Immunohistochemistry
Male
Microscopy, Electron, Transmission
Neurons, Afferent - metabolism
Neurons, Afferent - ultrastructure
nuclear speckles
nucleolus
Rats
Rats, Sprague-Dawley
RNA, Messenger - biosynthesis
RNA, Messenger - genetics
Staining and Labeling - methods
transcription foci
Transcription, Genetic - physiology
Transcriptional Activation - physiology
Trigeminal Ganglion - metabolism
Trigeminal Ganglion - ultrastructure
Uridine - analogs & derivatives
Uridine - metabolism
Vertebrates: nervous system and sense organs
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Summary:In this study we have used the transcription assay with 5′-fluorouridine incorporation into nascent RNA to analyze the nuclear organization and dynamics of transcription sites in rat trigeminal ganglia neurons. The 5′-FU administrated by i.p. injection was successfully incorporated into nuclear domains containing actively transcribing genes of trigeminal neurons. 5′-Fluorouridine RNA-labeling was detected with immunocytochemistry at light and electron microscopy levels. The 5′-fluorouridine incorporation sites were detected in the nucleolus, particularly on the dense fibrillar component, and in numerous transcription foci spread throughout the euchromatin regions, without preferential positioning at the nuclear periphery or in the nuclear interior. Double labeling experiments to combine 5′-fluorouridine incorporation with molecular markers of nuclear compartments showed the absence of transcription sites in Cajal bodies and nuclear speckles of splicing factors. Similarly, no 5′-fluorouridine labeling was detected in well-characterized chromatin silencing domain, the telomeric heterochromatin. The specificity and sensitivity of the run-on transcription assay in trigeminal ganglia neurons was verified by the i.p. administration of the transcription inhibitor actinomycin D. The dramatic reduction in RNA synthesis upon actinomycin D treatment was associated with two important cellular events, heterochromatin silencing and formation of DNA damage/repair nuclear foci, demonstrated by the expression of tri-methylated histone H4 and phosphorylated H2AX, respectively. 5′-Fluorouridine incorporation in animal models provides a useful tool to investigate the organization of gene expression in mammalian neurons in both normal physiology and experimental pathology systems.
ISSN:0306-4522
1873-7544
DOI:10.1016/j.neuroscience.2006.02.030