-
Something wrong with this record ?
Introduction of macarpine as a novel cell-permeant DNA dye for live cell imaging and flow cytometry sorting
I. Slaninová, N. López-Sánchez, K. Šebrlová, O. Vymazal, JM. Frade, E. Táborská,
Language English Country England, Great Britain
Document type Journal Article, Research Support, Non-U.S. Gov't
PubMed
26482322
DOI
10.1111/boc.201500047
Knihovny.cz E-resources
- MeSH
- Benzophenanthridines analysis MeSH
- Cell Culture Techniques MeSH
- Cell Cycle physiology MeSH
- DNA analysis MeSH
- Fluorescent Dyes analysis MeSH
- Microscopy, Fluorescence methods MeSH
- Humans MeSH
- Flow Cytometry * methods MeSH
- Cell Separation methods MeSH
- Cell Survival MeSH
- Green Fluorescent Proteins metabolism MeSH
- Check Tag
- Humans MeSH
- Publication type
- Journal Article MeSH
- Research Support, Non-U.S. Gov't MeSH
BACKGROUND INFORMATION: Macarpine (MA) is a quaternary benzophenanthridine plant alkaloid isolated from Macleaya microcarpa or Stylophorum lasiocarpum. Benzophenanthridine alkaloids are interesting natural products that display antiproliferative, antimicrobial, antifungal and anti-inflammatory activities, and also fluorescence properties. In a previous study, we demonstrated that thanks to its ability to interact with DNA and its spectral properties MA could be used as a supravital DNA probe for fluorescence microscopy and flow cytometry including analyses of the cell cycle. In this study, we evaluated the suitability of MA as a DNA dye for time-lapse microscopy and flow-cytometric cell sorting. RESULTS: Living A-375 and MEF cells stained with MA were monitored by time-lapse microscopy for 24 h. Mitoses were observed at MA concentrations up to 0.5 μg/ml during the first 2-3 h. After this period of time, cells treated with MA at concentrations of 0.75 and 0.5 μg/ml underwent apoptosis. Cells cultivated with MA at concentration of 0.25 μg/ml or lower survived throughout the 24 h period. Toxicity of MA was dependent on light wavelength and frequency of image capturing. The intensity of MA fluorescence decreased during the incubation. MA concentration of 0.1 μg/ml was identified as the most suitable for live cell imaging with respect to fluorescence intensity and toxicity. MA at the concentration 10 μg/ml was used for sorting of enhanced green fluorescent protein (EGFP)-labelled neurons and fibroblasts yielding profiles similar to those obtained with DRAQ5. Contrary to DRAQ5, MA-stained cells survived in culture, and the sorted cells lost the MA signal suggesting reversible binding of the dye to the DNA. CONCLUSION: The results proved that MA may readily be used for chromosomes depicting and mitosis monitoring by time-lapse microscopy. In addition, MA has shown to be a suitable probe for sorting of EGFP-labelled cells, including neurons, that survived the labelling process. SIGNIFICANCE: In consideration of the results, we highly anticipate an onward use of MA in a broad range of applications based on live cell sorting and imaging, for example, cell synchronisation and monitoring of proliferation as an important experimental and/or diagnostic utility.
Cajal Institute IC CSIC Avda Doctor Arce 37 Madrid E 28002 Spain
Department of Biochemistry Faculty of Medicine Masaryk University Brno 62500 Czech Republic
Department of Biology Faculty of Medicine Masaryk University Brno 62500 Czech Republic
References provided by Crossref.org
- 000
- 00000naa a2200000 a 4500
- 001
- bmc17000943
- 003
- CZ-PrNML
- 005
- 20170113094429.0
- 007
- ta
- 008
- 170103s2016 enk f 000 0|eng||
- 009
- AR
- 024 7_
- $a 10.1111/boc.201500047 $2 doi
- 024 7_
- $a 10.1111/boc.201500047 $2 doi
- 035 __
- $a (PubMed)26482322
- 040 __
- $a ABA008 $b cze $d ABA008 $e AACR2
- 041 0_
- $a eng
- 044 __
- $a enk
- 100 1_
- $a Slaninová, Iva $u Department of Biology, Faculty of Medicine, Masaryk University, Brno, 62500, Czech Republic.
- 245 10
- $a Introduction of macarpine as a novel cell-permeant DNA dye for live cell imaging and flow cytometry sorting / $c I. Slaninová, N. López-Sánchez, K. Šebrlová, O. Vymazal, JM. Frade, E. Táborská,
- 520 9_
- $a BACKGROUND INFORMATION: Macarpine (MA) is a quaternary benzophenanthridine plant alkaloid isolated from Macleaya microcarpa or Stylophorum lasiocarpum. Benzophenanthridine alkaloids are interesting natural products that display antiproliferative, antimicrobial, antifungal and anti-inflammatory activities, and also fluorescence properties. In a previous study, we demonstrated that thanks to its ability to interact with DNA and its spectral properties MA could be used as a supravital DNA probe for fluorescence microscopy and flow cytometry including analyses of the cell cycle. In this study, we evaluated the suitability of MA as a DNA dye for time-lapse microscopy and flow-cytometric cell sorting. RESULTS: Living A-375 and MEF cells stained with MA were monitored by time-lapse microscopy for 24 h. Mitoses were observed at MA concentrations up to 0.5 μg/ml during the first 2-3 h. After this period of time, cells treated with MA at concentrations of 0.75 and 0.5 μg/ml underwent apoptosis. Cells cultivated with MA at concentration of 0.25 μg/ml or lower survived throughout the 24 h period. Toxicity of MA was dependent on light wavelength and frequency of image capturing. The intensity of MA fluorescence decreased during the incubation. MA concentration of 0.1 μg/ml was identified as the most suitable for live cell imaging with respect to fluorescence intensity and toxicity. MA at the concentration 10 μg/ml was used for sorting of enhanced green fluorescent protein (EGFP)-labelled neurons and fibroblasts yielding profiles similar to those obtained with DRAQ5. Contrary to DRAQ5, MA-stained cells survived in culture, and the sorted cells lost the MA signal suggesting reversible binding of the dye to the DNA. CONCLUSION: The results proved that MA may readily be used for chromosomes depicting and mitosis monitoring by time-lapse microscopy. In addition, MA has shown to be a suitable probe for sorting of EGFP-labelled cells, including neurons, that survived the labelling process. SIGNIFICANCE: In consideration of the results, we highly anticipate an onward use of MA in a broad range of applications based on live cell sorting and imaging, for example, cell synchronisation and monitoring of proliferation as an important experimental and/or diagnostic utility.
- 650 _2
- $a benzofenantridiny $x analýza $7 D053119
- 650 _2
- $a buněčné kultury $7 D018929
- 650 _2
- $a buněčný cyklus $x fyziologie $7 D002453
- 650 _2
- $a separace buněk $x metody $7 D002469
- 650 _2
- $a viabilita buněk $7 D002470
- 650 _2
- $a DNA $x analýza $7 D004247
- 650 12
- $a průtoková cytometrie $x metody $7 D005434
- 650 _2
- $a fluorescenční barviva $x analýza $7 D005456
- 650 _2
- $a zelené fluorescenční proteiny $x metabolismus $7 D049452
- 650 _2
- $a lidé $7 D006801
- 650 _2
- $a fluorescenční mikroskopie $x metody $7 D008856
- 655 _2
- $a časopisecké články $7 D016428
- 655 _2
- $a práce podpořená grantem $7 D013485
- 700 1_
- $a López-Sánchez, Noelia $u Cajal Institute, IC-CSIC, Avda. Doctor Arce 37, Madrid, E-28002, Spain.
- 700 1_
- $a Šebrlová, Kristýna $u Department of Biochemistry, Faculty of Medicine, Masaryk University, Brno, 62500, Czech Republic.
- 700 1_
- $a Vymazal, Ondřej $u Department of Biology, Faculty of Medicine, Masaryk University, Brno, 62500, Czech Republic.
- 700 1_
- $a Frade, José María $u Cajal Institute, IC-CSIC, Avda. Doctor Arce 37, Madrid, E-28002, Spain.
- 700 1_
- $a Táborská, Eva $u Department of Biochemistry, Faculty of Medicine, Masaryk University, Brno, 62500, Czech Republic.
- 773 0_
- $w MED00000749 $t Biology of the cell $x 1768-322X $g Roč. 108, č. 1 (2016), s. 1-18
- 856 41
- $u https://pubmed.ncbi.nlm.nih.gov/26482322 $y Pubmed
- 910 __
- $a ABA008 $b sig $c sign $y a $z 0
- 990 __
- $a 20170103 $b ABA008
- 991 __
- $a 20170113094530 $b ABA008
- 999 __
- $a ok $b bmc $g 1180083 $s 961510
- BAS __
- $a 3
- BAS __
- $a PreBMC
- BMC __
- $a 2016 $b 108 $c 1 $d 1-18 $e 20151118 $i 1768-322X $m Biology of the cell $n Biol Cell $x MED00000749
- LZP __
- $a Pubmed-20170103
