Literature DB >> 4017802

Automated analysis and survival selection of anchorage-dependent cells under normal growth conditions.

M Schindler, M L Allen, M R Olinger, J F Holland.   

Abstract

An instrument is described that can automatically analyze and select for a subpopulation of anchorage-dependent cells in tissue culture. Cells that label with fluorescently tagged antibodies or demonstrate structural variations are saved from exposure to a destructive high-intensity argon laser beam. The surviving population may then be cloned. The cell selection may occur in a tissue culture plate or in a microflow incubator which is designed to maintain a constant flow of media at 37 degrees C across cells growing on a glass coverslip. This incubator sits on an inverted microscope which focuses the laser beam to a diameter as small as 1 micron. A high-speed computer-controlled two-dimensional stage moves the cells past the beam for analysis, the results of which determine the fate of each cell: whether it is to be destroyed by radiant energy or selected for survival and subsequent proliferation. Another selection strategy performed by the instrument involves growing the cells on a thin, blackened polyester film which can be cut by the argon laser beam. Cells selected for cloning are then circumscribed. The heat of cutting welds the circumscribed film to a plastic coverslip surface or tissue culture chamber bottom. Nonselected cells may be removed by pulling the unattached polyester sheet from the attachment surface. The selected cells remain on polyester film disks welded to the plastic. Selections may be done automatically under computer control or manually by operator direction of stage movements. This instrument extends the art of automated cell selection and analysis to normal cell lines that must maintain cell-substratum contact (anchorage dependence) for differentiated cell function, e.g., neurons, fibroblasts, or kidney cells.

Entities:  

Mesh:

Year:  1985        PMID: 4017802     DOI: 10.1002/cyto.990060415

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


  9 in total

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Journal:  Stem Cell Rev Rep       Date:  2010-06       Impact factor: 5.739

4.  Contraction and intracellular calcium-ion elevation of cultured human aortic smooth muscle cells by endothelin-1, vasoactive intestinal contractor (VIC) and the derivatives.

Authors:  A Iwashima; M Kobayashi; K Saida; H Kagamu; S Ohashi; M Arakawa; Y Mitsui
Journal:  In Vitro Cell Dev Biol Anim       Date:  1997 Nov-Dec       Impact factor: 2.416

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Authors: 
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6.  Scanning laser cytometry: alterations induced by cholestatic agents in isolated rat hepatocyte couplets.

Authors:  N Thibault
Journal:  Cell Biol Toxicol       Date:  1994-12       Impact factor: 6.691

7.  Use of scanning cytometry in studying bradykinin binding in MRC-5 cells.

Authors:  M Maratrat; N Munoz; I Gravier; V Thybaud; A Crespo
Journal:  Cell Biol Toxicol       Date:  1994-12       Impact factor: 6.691

8.  Immunocytochemical identification and localization of the Mr 22,000 calcium-binding protein (sorcin) in an adriamycin-resistant myelogenous leukemia cell line.

Authors:  I Sugawara; K Mizumoto; E Ohkochi; H Hamada; T Tsuruo; S Mori
Journal:  Jpn J Cancer Res       Date:  1989-05

9.  Novel millimeter-wave-based method for in situ cell isolation and other applications.

Authors:  Barney Boyce; Natalia Samsonova
Journal:  Sci Rep       Date:  2018-10-03       Impact factor: 4.379

  9 in total

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