Literature DB >> 2419056

Flow cytometric discrimination of mitotic cells: resolution of M, as well as G1, S, and G2 phase nuclei with mithramycin, propidium iodide, and ethidium bromide after fixation with formaldehyde.

J K Larsen, B Munch-Petersen, J Christiansen, K Jørgensen.   

Abstract

Cells in mitosis can be flow cytometrically discriminated from G1, S, and G2 cells by analysis of a nuclear suspension prepared with nonionic detergent, fixed with formaldehyde, and stained with mithramycin, propidium iodide, or ethidium bromide. With these DNA-fluorochromes, the fluorescence is quenched by formaldehyde less in mitotic nuclei than in interphase nuclei. Mitotic nuclei have a 20-40% increased mithramycin fluorescence and 30-60% decreased light scatter in comparison to those of G2 nuclei. There is a high correlation (r = 0.95; P less than 0.001) between microscope counts of mitotic figures in smear preparations of the initial cell suspension and the flow cytometrically estimated fraction of nuclei with increased mithramycin fluorescence. Flow sorting (FACS) demonstrates that the mitotic nuclei are confined to the peak of increased mithramycin fluorescence and decreased light scatter. The method has been applied to cultures of Yoshida ascites tumor cells, JB-1 reticulosarcoma cells, and PHA-stimulated human lymphocytes, incubated in the presence or absence of vinblastine for mitotic arrest. In a heteroploid mixture of fixed Yoshida (near-diploid) and JB-1 (hypotetraploid) nuclei, the mitotic fractions of the two cell lines could be estimated separately when analyzed with mithramycin fluorescence versus light scatter or with mithramycin fluorescence versus propidium iodide fluorescence.

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Year:  1986        PMID: 2419056     DOI: 10.1002/cyto.990070108

Source DB:  PubMed          Journal:  Cytometry        ISSN: 0196-4763


  15 in total

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2.  Cytometric sorting based on the fluorescence lifetime of spectrally overlapping signals.

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3.  Proliferation of germ cells and somatic cells in first trimester human embryonic gonads as indicated by S and S+G2+M phase fractions.

Authors:  K P Sørensen; M C Lutterodt; L S Mamsen; A G Byskov; J K Larsen
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4.  Use of flow cytometry to study growth of human airway smooth muscle cells.

Authors:  Z D Zhang; G Cox
Journal:  In Vitro Cell Dev Biol Anim       Date:  1998-04       Impact factor: 2.416

5.  Genome-wide analysis of replication timing in mammalian cells: troubleshooting problems encountered when comparing different cell types.

Authors:  Vishnu Dileep; Ruth Didier; David M Gilbert
Journal:  Methods       Date:  2012-06-06       Impact factor: 3.608

6.  Metaphase Cells Enrichment for Efficient Use in the Dicentric Chromosome Assay.

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7.  Flow cytometric DNA analysis of lesions from 18 children with langerhans cell histiocytosis (histiocytosis x).

Authors:  K Ornvold; H Carstensen; J K Larsen; I J Christensen; E Ralfkiaer
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8.  Human microvascular endothelial cell-extracellular matrix interaction in cellular growth state determination.

Authors:  S R Mallery; L E Lantry; M C Toms; L C Titterington; B L Hout; G P Brierley; R E Stephens
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9.  DNA ploidy and S-phase fraction in medullary carcinoma of the breast--a flow cytometric analysis using archival material.

Authors:  L Pedersen; J K Larsen; I J Christensen; A Lykkesfeldt; S Holck; T Schiødt
Journal:  Breast Cancer Res Treat       Date:  1994       Impact factor: 4.872

10.  Cellular response to 5-fluorouracil (5-FU) in 5-FU-resistant colon cancer cell lines during treatment and recovery.

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