In situ hybridization using 32P labelled oligodeoxyribonucleotides for the cellular localisation of mRNA in neuronal and endocrine tissue |
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Authors: | J. V. Priestley M. A. Hynes V. K. M. Han M. Réthelyi E. R. Perl P. K. Lund |
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Affiliation: | (1) Department of Physiology, University of North Carolina at Chapel Hill, 27514 Chapel Hill, NC, USA;(2) Departments of Physiology and Biochemistry, United Medical and Dental Schools, St. Thomas's Campus, Lambeth Palace Road, SE1 7EH London, England;(3) 2nd Department of Anatomy, Semmelweis University, Medical School, Budapest, Hungary |
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Abstract: | Summary Methodological variables for in situ hybridization using 32P labelled oligodeoxyribonucleotides (oligomers) have been examined. Four different oligomers directed against proglucagon messenger RNA (mRNA) and two different oligomers against prosomatostatin mRNA have been used. Specific hybridization was obtained in adult rat brain, stomach and pancreas and in neonatal rat ileum. Tissue was perfusion fixed with 4% paraformaldehyde 0.2% glutaraldehyde and hybridization was carried out in 50% formamide for 72 h at 42° C. Using hybridization conditions of lower stringency (33% formamide) labelling was also obtained in guinea pig tissue. Other variables which affected hybridization signal intensity were the inclusion of a prehybridization dehydration stage, the probe concentration, the inclusion of ammonium acetate in the posthybridization dehydrating ethanols and in the autoradiographic emulsion, and the exposure time. The localisation of proglucagon mRNA in rat pancreas using a 20mer was used as a model tissue for testing these methodological variables and the results were found generally also to apply to the other probes and tissues tested. The methods described provide single cell resolution and show that 32P labelled oligomers may be used to localise neuropeptide and endocrine mRNAs in different types of tissue and in different mammalian species. |
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