In essence, apoptosis is a containment program preparing the cell corpse for engulfment by efferocytosis. When the phagocytic capacity is insufficient, apoptotic cells undergo disintegration accompanied by the release of cellular content, coined secondary necrosis. As secondary necrotic cells can elicit an inflammatory response [1], insights into the underlying mechanisms or molecules driving secondary necrosis are of major importance for therapeutic targeting. Rogers et al. reported that gasdermin E (GSDME), a member of the pore-forming gasdermin protein family and a substrate of the apoptotic caspase-3, drives secondary necrosis [2]. Indeed, Gsdme−/− macrophages displayed lower plasma membrane permeabilization upon the stimulation with etoposide, an apoptosis inducer, as assessed by propidium iodide (PI) [2]. However, other reports showed that the loss of GSDME did not result in differential kinetics in plasma membrane permeabilization measured by TO-PRO-3 fluorescent DNA dye in UV irradiated THP-1 and Jurkat T cells [3]. Similarly, the absence of GSDME did not affect membrane permeabilization measured by YOYO-1 fluorescent DNA dye in macrophages upon anti-Fas treatment [4].
In theory, impermeant DNA-binding dyes seem ideal for assessing the membrane permeabilizing function of GSDME. These dyes enter and bind to nuclear DNA and allow detection of cells that lose membrane integrity. Most of them demonstrate little to no solution fluorescence and greatly increased quantum yield when bound to DNA [5,6,7]. However, most of these dyes were initially designed to stain DNA before being repurposed to stain cells with compromised membranes. Although their binding and membrane passing characteristics are largely unknown, all of these cell impermeant nuclear dyes are used to measure plasma membrane permeabilization. Importantly, some of these small cationic nuclear dyes were shown to enter cells by pannexin channels mediated mechanisms (YO-PRO-1, and TO-PRO-3) [8, 9], allowing for labeling early apoptotic cells [10, 11] associated with the activation of pannexin-1 and making their applicability in measuring plasma membrane permeabilization problematic.
In that respect, the contradicting results concerning the role of GSDME during apoptosis-driven secondary necrosis might be attributed to the choice of nucleic acid stain to measure plasma membrane permeabilization rather than to differences in cellular context or GSDME expression levels. Next to PI and 7-AAD, SYTOX dyes are commonly used as dead-cell markers as they provide some advantages to other dyes, such as a good signal-to-noise ratio at low concentrations and a low photobleaching rate [6, 12]. Despite the small size of SYTOX cyanine nuclear DNA dyes (<0.6 kDa) they are not associated with pannexin-mediated mechanisms nor known to label early apoptotic cells.
In the light of these conflicting findings, we decided to investigate GSDME function in the murine fibrosarcoma cell line L929sAhFas, susceptible to apoptosis when stimulated with human Fas antibody [13], and generated L929sAhFas GSDME KO cell lines (Fig. 1A). Surprisingly, using 7-AAD and SYTOX blue (SB) dyes combined, we came across a differential staining pattern in the absence of GSDME expression in L929sAhFas during apoptosis-driven secondary necrosis. Upon anti-Fas treatment, L929sAhFas wild-type clones proceeded from a double negative (7-AAD−/SB−) population toward a double positive population (7-AAD+/SB+) (Fig. 1B, C), while in L929sAhFas Gsdme-deficient clones, a clear 7-AAD single positive stage (7-AAD+/SB−) (Fig. 1B) and a decrease in SB uptake (Fig. 1D) was observed. Doxycycline-inducible mGSDME reconstitution and anti-Fas stimulation in one L929sAhFas Gsdme-deficient clone (Fig. 1E) rescued the reduced SB staining (Fig. 1F, G) in absence of GSDME expression into the simultaneous 7-AAD and SB staining (Fig. 1F, H) initially observed in L929sAhFas wild type (Fig. 1B, C). This suggests that the observed distinct uptake patterns were due to the presence and absence of GSDME. Live cell imaging confirmed a delay in nuclear staining by SB compared to 7-AAD in cells lacking GSDME (Fig. 1J, K, Supplementary videos). Interestingly, GSDME expression had no effect on the uptake of 7-AAD in our analysis, suggesting that other, GSDME independent, cell membrane permeabilization mechanisms could operate in L929sAhFas allowing uptake 7-AAD upon anti-Fas treatment and excluding SB uptake. As reconstitution of GSDME expression resulted in the simultaneous uptake of 7-AAD and SB upon anti-Fas treatment (Fig. 1I, L), our results suggest that GSDME favors cell membrane permeabilization mechanisms allowing nuclear staining by SB, while 7-AAD is entering the cell by another mechanism.
Thus, our results based on SB staining are consistent with the findings of Rogers et al. reporting that GSDME is responsible for membrane permeabilization during apoptosis-driven secondary necrosis [2]. On the opposite, our results based on 7-AAD staining support the findings of Tixeira et al. and Lee et al. stating that GSDME does not affect cell membrane permeabilization during apoptosis-driven secondary necrosis [3, 4]. Therefore, caution is needed when drawing conclusions from different studies using various cell death markers. Additional studies using markers of late apoptotic cells could clarify the current contradicting findings and assess the importance of the choice of marker to investigate cell membrane permeabilization mechanisms. Altogether, it seems that next to pannexin channels mediated mechanism, different GSDME dependent and independent mechanisms leading to membrane permeabilization take place during apoptosis-driven secondary necrosis, allowing the selective uptake of different nuclear dyes. Although the use of cell impermeant dyes might not be suitable to study membrane permeabilization processes itself, the double staining with SB and 7-AAD may allow functionality studies of GSDME and maybe other GSDMs.
References
Sachet M, Liang YY, Oehler R. The immune response to secondary necrotic cells. Apoptosis. 2017;22:1189–204.
Rogers C, Fernandes-Alnemri T, Mayes L, Alnemri D, Cingolani G, Alnemri ES. Cleavage of DFNA5 by caspase-3 during apoptosis mediates progression to secondary necrotic/pyroptotic cell death. Nat Commun. 2017;8:14128.
Tixeira R, Shi B, Parkes MAF, Hodge AL, Caruso S, Hulett MD, et al. Gasdermin E does not limit apoptotic cell disassembly by promoting early onset of secondary necrosis in Jurkat T cells and THP-1 monocytes. Front Immunol. 2018;9:2842.
Lee BL, Mirrashidi KM, Stowe IB, Kummerfeld SK, Watanabe C, Haley B, et al. ASC- and caspase-8-dependent apoptotic pathway diverges from the NLRC4 inflammasome in macrophages. Sci Rep. 2018;8:3788.
Gill JE, Jotz MM, Young SG, Modest EJ, Sengupta SK. 7 Amino actinomycin D as a cytochemical probe. I. Spectral properties. J Histochem Cytochem. 1975;23:793–9.
Thakur S, Cattoni DI, Nöllmann M. The fluorescence properties and binding mechanism of SYTOX green, a bright, low photo-damage DNA intercalating agent. Eur Biophys J. 2015;44:337–48.
Fürstenberg A, Deligeorgiev TG, Gadjev NI, Vasilev AA, Vauthey E. Structure–fluorescence contrast relationship in cyanine DNA intercalators: toward rational dye design. Chem A Eur J. 2007;13:8600–9.
Chekeni FB, Elliott MR, Sandilos JK, Walk SF, Kinchen JM, Lazarowski ER, et al. Pannexin 1 channels mediate ‘find-me’ signal release and membrane permeability during apoptosis. Nature. 2010;467:863–7.
Qu Y, Misaghi S, Newton K, Gilmour LL, Louie S, Cupp JE, et al. Pannexin-1 is required for ATP release during apoptosis but not for inflammasome activation. J Immunol. 2011;186:6553–61.
Glisic-Milosavljevic S, Waukau J, Jana S, Jailwala P, Rovensky J, Ghosh S. Comparison of apoptosis and mortality measurements in peripheral blood mononuclear cells (PBMCs) using multiple methods. Cell Prolif. 2005;38:301–11.
Jiang L, Tixeira R, Caruso S, Atkin-Smith GK, Baxter AA, Paone S, et al. Monitoring the progression of cell death and the disassembly of dying cells by flow cytometry. Nat Protoc. 2016;11:655–63.
Chiaraviglio L, Kirby JE. Evaluation of impermeant, DNA-binding dye fluorescence as a real-time readout of eukaryotic cell toxicity in a high throughput screening format. Assay Drug Dev Technol. 2014;12:219–28.
Vercammen D, Beyaert R, Denecker G, Goossens V, Van Loo G, Declercq W, et al. Inhibition of caspases increases the sensitivity of L929 cells to necrosis mediated by tumor necrosis factor. J Exp Med. 1998;187:1477–85.
Acknowledgements
Research in the Vandenabeele group is supported by Flemish grants (EOS MODEL-IDI, FWO Grant 30826052), FWO research grants (G.0E04.16N, G.0C76.18N, G.0B71.18N, G.0B96.20N), Methusalem (BOF16/MET_V/007), iBOF20/IBF/039 ATLANTIS, Foundation against Cancer (FAF-F/2016/865, F/2020/1505), CRIG and GIGG consortia, and VIB. We thank the VIB-UGent BioImaging Core for assistance.
Author information
Authors and Affiliations
Corresponding authors
Ethics declarations
Competing interests
The authors declare no competing interests.
Additional information
Publisher’s note Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
Supplementary Information
Rights and permissions
Open Access This article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made. The images or other third party material in this article are included in the article’s Creative Commons license, unless indicated otherwise in a credit line to the material. If material is not included in the article’s Creative Commons license and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this license, visit http://creativecommons.org/licenses/by/4.0/.
About this article
Cite this article
De Schutter, E., Cappe, B., Wiernicki, B. et al. Plasma membrane permeabilization following cell death: many ways to dye!. Cell Death Discov. 7, 183 (2021). https://doi.org/10.1038/s41420-021-00545-6
Received:
Accepted:
Published:
DOI: https://doi.org/10.1038/s41420-021-00545-6
This article is cited by
-
Plasma membrane perforation by GSDME during apoptosis-driven secondary necrosis
Cellular and Molecular Life Sciences (2022)