Localization of DNA in the fibrillar components of the nucleolus: a cytochemical and morphometric studyM Derenzini, F Farabegoli and D Trere Dipartimento di Patologia Sperimentale, Universita degli Studi di Bologna, Italia. We studied the distribution of DNA in human circulating lymphocyte nucleoli using three different cytochemical methods for selective visualization of DNA in thin sections: the Feulgen-like osmium-ammine reaction, the NAMA-Ur procedure, and the osmium-ammine staining in glycine buffer, pH 1.5. All three methods indicated the presence of uniformly distributed, highly decondensed DNA filaments forming a large solitary agglomerate in the central part of the nucleolar area, corresponding to the solitary large fibrillar center (FC) as revealed by uranium and lead staining. We also studied the relationship between DNA agglomerates and nucleolar fibrillar components in resting and phytohemagglutinin (PHA)-stimulated lymphocytes by morphometric analysis of the areas occupied by these structures. In resting lymphocytes the mean area of the DNA agglomerates was 0.479 micron 2 +/- 0.161 SD, whereas that of FCs was 0.380 micron 2 +/- 0.149 SD, with a ratio of 1.26. In PHA-stimulated lymphocytes the mean area of the DNA agglomerates was 0.116 micron 2 +/- 0.056 SD, whereas that of the FCs was 0.075 micron 2 +/- 0.032 SD, with a ratio of 1.55. In PHA- stimulated lymphocytes we also measured the area occupied by the FCs plus the closely associated dense fibrillar component (DFC). The mean value of these two fibrillar components was 0.206 micron 2 +/- 0.081 SD. These data demonstrate that decondensed DNA filaments are uniformly distributed in the FCs and that in transcriptionally active nucleoli they are also present in the proximal portion of the DFC surrounding the FCs.
Volume 41,
Issue 6,
pp. 829-836,
06/01/1993
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M. Derenzini, G. Pasquinelli, M.-F. O'Donohue, D. Ploton, and M. Thiry Structural and Functional Organization of Ribosomal Genes within the Mammalian Cell Nucleolus J. Histochem. Cytochem., February 1, 2006; 54(2): 131 - 145. [Abstract] [Full Text] [PDF] |
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T. Wei, H. Baiqu, L. Chunxiang, and Z. Zhonghe In situ visualization of rDNA arrangement and its relationship with subnucleolar structural regions in Allium sativum cell nucleolus J. Cell Sci., March 15, 2003; 116(6): 1117 - 1125. [Abstract] [Full Text] [PDF] |
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M. Biggiogera, M. Malatesta, S. Abolhassani-Dadras, F. Amalric, L. I. Rothblum, and S. Fakan Revealing the unseen: the organizer region of the nucleolus J. Cell Sci., January 9, 2001; 114(17): 3199 - 3205. [Abstract] [Full Text] [PDF] |
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O. Stoss, F.-W. Schwaiger, T. A. Cooper, and S. Stamm Alternative Splicing Determines the Intracellular Localization of the Novel Nuclear Protein Nop30 and Its Interaction with the Splicing Factor SRp30c J. Biol. Chem., April 16, 1999; 274(16): 10951 - 10962. [Abstract] [Full Text] [PDF] |
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A Olmedilla, P. Testillano, O Vicente, M Delseny, and M. Risueno Ultrastructural rRNA localization in plant cell nucleoli. RNA/RNA in situ hybridization, autoradiography and cytochemistry J. Cell Sci., January 12, 1993; 106(4): 1333 - 1346. [Abstract] [PDF] |
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