Increased variability in nuclear DNA content of testis cells and spermatozoa from mice with irregular meiotic segregation. |
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Authors: | M L Meistrich S Lake L L Steinmetz B L Gledhill |
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Affiliation: | 1. Biomedical Sciences Division, Lawrence Livermore Laboratory, University of California, Livermore, Calif. 94550, USA;2. Section of Experimental Radiotherapy, The University of Texas System Cancer Center, M.D. Anderson Hospital and Tumor Institute, Houston, Texas 77030, U.S.A. |
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Abstract: | Variability in DNA content to testis cells and sperm from F1 hybrids between the laboratory mouse (M. muscullus) and the tobacco mouse (M. poschiavinus), has been determined by flow cytometry (FMC). The F1 hybrid mouse is known to be heterozygous for seven metacentric chromosomes produced by Robertsonian fusion. Enriched populations of nuclei from late pachytene spermatocytes and round spermatids were obtained by velocity sedimentation. These nuclei, as well as epididymal sperm nuclei and spleen cells, were stained by the acriflavin-Feulgen technique for DNA and measured by FCM. Peaks in the fluorescence intensity frequency distributions resulting from these measurements were analyzed to determine their mean fluorescence intensities and their widths (coefficients of variation). Because mean intensities of corresponding cell types from M. musculus and the F1 hybrids were identical, the average DNA contents were taken to be the same. The average coefficients of variation of the peaks to fluorescence from the pachytene, spermatid, and sperm nuclei and spleen cells from M. muscullus animals were about 5%. While the peaks of fluorescence from spleen cells and pachytene nuclei from f1 hybrids also had average coefficients of variation of 5%, post-meiotic nuclei from spermatids and spermatozoa had coefficients of variationof 8%. From these results we conclude that, in these F1 hybrids, abnormal meiotic segregation causes an increased variability of 6% in the amount of DNA in the spermatozoa. |
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Keywords: | CV, coefficient of variation FMC, flow cytometry |
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