Literature DB >> 3132355

Flow cytometric discrimination of mitotic nuclei by right-angle light scatter.

R M Zucker1, K H Elstein, R E Easterling, E J Massaro.   

Abstract

Flow cytometry has been used to demonstrate alterations in protein, RNA, and DNA content of cells as they traverse the cell cycle. Employing fluorescein isothiocyanate (FITC) to stain protein and propidium iodide (PI) to stain nucleic acids, multiple regions within the G1 and G2 phases of the cell cycle, in addition to the M phase, can be distinguished. In this study, cytograms of the 90 degree light scatter signal vs. PI fluorescence were remarkably similar to those of FITC fluorescence vs. PI fluorescence, suggesting a relationship between 90 degree light scatter and protein content. M-phase nuclei can be distinguished from G2-phase nuclei on cytograms of 90 degree light scatter vs. PI fluorescence. However, the percentage of mitotic nuclei obtained by this technique is less than that found by light microscopic analysis. Flow cytometric parameters of nuclei prepared by nonionic detergent (NP40) lysis in Dulbecco's PBS, Vindelov's buffer, or Pollack's hypotonic EDTA/Tris buffer were compared. The best resolution of mitotic nuclei was obtained in Pollack's buffer. However, the stainability of the M-phase nuclei is reduced, and the nuclei are located in the late S/G2 region of the single-parameter histogram.

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Year:  1988        PMID: 3132355     DOI: 10.1002/cyto.990090307

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


  10 in total

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2.  Flow cytometric analysis of the mechanism of methylmercury cytotoxicity.

Authors:  R M Zucker; K H Elstein; R E Easterling; E J Massaro
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3.  Improved bromodeoxyuridine/DNA analysis by anti-BudR monoclonal antibody versus right angle light scatter.

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5.  An efficient multiple-exposure analysis of the toxicity of crisnatol, a DNA intercalator in phase II clinical trials.

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7.  Increase in total protein following infection of CV-1 cells with SV40 virus as assayed by flow cytometry.

Authors:  J M Lehman; E Dickerson; T Friedrich; J Laffin
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8.  Ki-67 staining for determination of rhesus macaque T cell proliferative responses ex vivo.

Authors:  Devon J Shedlock; Kendra T Talbott; Matthew P Morrow; Bernadette Ferraro; David A Hokey; Karuppiah Muthumani; David B Weiner
Journal:  Cytometry A       Date:  2010-03       Impact factor: 4.355

9.  Discrimination of mitotic cells using anti-p105 monoclonal antibody to analyze the mode of action of etoposide and podophyllotoxin in human gastric cancer cells.

Authors:  S Ohyama; Y Yonemura; K Tsugawa; I Miyazaki; M Tanaka; T Sasaki
Journal:  Jpn J Cancer Res       Date:  1991-11

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  10 in total

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