2001
DOI: 10.1038/sj.bmt.1702809
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Large populations of non-clonogenic early apoptotic CD34-positive cells are present in frozen-thawed peripheral blood stem cell transplants

Abstract: Summary:Apoptosis is the common cell death pathway which is initiated by a variety of different stimuli. The recognition of early apoptotic events would markedly improve reliability and convenience of apoptosis assays. In the present study the vital stain Syto R 16 in combination with the permeability marker 7-amino actinomycin D, (7-AAD) has been used to identify an early stage of apoptosis, not detected with trypan blue or 7-AAD alone or with conventional apoptosis tests and not consistently and only partly … Show more

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Cited by 77 publications
(113 citation statements)
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“…For multiparametric (two-color and tri-color stainings) logarithmic fluorescence signals were collected using following filters: SYTO dyes (FL1 530/30 BP), TMRM (FL2 585/42 BP), PI (FL2 585/42 BP), 7-AAD (FL3 650 LP). As described by others (14) due to the strong spectral overlap of SYTO16 (in FL2 and FL3) special attention has been made to compensate both channels. For evaluation of fractional DNA content propidium iodide fluorescence was collected using linear amplification scale and 585/42 BP filter.…”
Section: Flow Cytometry and Cell Sortingmentioning
confidence: 99%
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“…For multiparametric (two-color and tri-color stainings) logarithmic fluorescence signals were collected using following filters: SYTO dyes (FL1 530/30 BP), TMRM (FL2 585/42 BP), PI (FL2 585/42 BP), 7-AAD (FL3 650 LP). As described by others (14) due to the strong spectral overlap of SYTO16 (in FL2 and FL3) special attention has been made to compensate both channels. For evaluation of fractional DNA content propidium iodide fluorescence was collected using linear amplification scale and 585/42 BP filter.…”
Section: Flow Cytometry and Cell Sortingmentioning
confidence: 99%
“…It has been previously tested by others that loss of SYTO16 fluorescence can be considered as a truly apoptotic feature (12)(13)(14)23,24), but to the best of our knowledge there is very limited data available to show SYTO behavior in cells exposed to oncotic stimuli. We observed that in the presence of relatively harsh oncotic stimuli (4 h-incubation with 1% NaN 3 , or 5 min at 56°C) the majority of cells was SYTO low /PI 1 , representative of cells with a compromised plasma membrane, whereas the number of SYTO dim /PI 2 events did not significantly increase above background levels ( Fig.…”
Section: Apoptotic Vs Oncotic Syto Staining Profilementioning
confidence: 99%
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