Methods for age determination and sorting of cells according to their age: Difference between revisions
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Revision as of 14:59, 24 November 2008
Note
- Technical description
- precision,
- limitations,
- results of experiments done with these techniques.
- Comprehensive bibliography
Yeast s. cerevisiae
- replicative life span:
first done by mortimer (1959): micromanipulation: throwing away the daugther cell
- Separation of Old and younger cells:
1/ centrifugation: egilmez,1989 young buds and cells are supernatant., synchro, then centri...etc
2/ biotin labelling of initial mothers:
Biotinylated surface proteins are retained in mothers but are not found in their daughters,because the daughters’ cell walls are newly synthesized.
Smeal et al, 1996 not very efficient toxic
3/chen and contreras used microbeads (50 nm diameter). Because of their small size, microbeads did not affect cell physiology and therefore bead detachment was not necessary. Then WGA to bind chitin, and FACS. Not so precise however.
3/ Then they all count bud scars to determine the average age of the isolated population. Not really sharp isolation, event with double purification.
Old phenotype: Bigger, scars with chitin, symetric cell division, cell cycle slows.
Mammalian cells
Primary cells, non immortal.mostly human fibroblasts. Hayflick limit (hayflick, 1961). in vitro, senescence due to a telomeres shortening.
Note the technical limitation allows only to separate youngvs senescent cells. No intermediates, no clear dimension of which gradual processes can happen..
- Methods
Actually, at a given time, a population of Human fibroblasts is highly heterogenous; It's a mix of senescent and non senescent cells, and the number of senescent cells increase with population doubling. Not all cells enter senescence at the same time. So how do people manage to obtain "pure populations" of senescent cells?
Senescent phenotype:: to be expanded and detailled with references.
cell and nuclear sizer (big),shape, production of ROS, Beta galactosidase activity, age pigment accumulation (lipofuscin), gene expression pattern, mitochondrial function.
Methods for Cell Sorting of Young and Senescent Cells:
João F. Passos and Thomas von Zglinicki (from Methods in Molecular Biology: Biological Aging: Methods and Protocols Edited by: T. O. Tollefsbol © Humana Press Inc., Totowa, NJ)
Fixed cells
staining and FACS for different markers:
- proteins upregulated in senescent cells: p16, p21, γ-H2AX.
- Failure to replicate: brdu incorporation, negative selection.
- staining for SA-β-galactosidase active at pH6 only in senescent cells (Dimri et al, 1995)
