Detection and Quantification of Histone H4 Citrullination in Early NETosis With Image Flow Cytometry Version 4

Detection and Quantification of Histone H4 Citrullination in Early NETosis With Image Flow Cytometry Version 4

Neutrophil extracellular traps (NETs) formation has been implicated in an increasing number of infectious and non-infectious pathologies. NETosis is a tightly regulated process; the end-stage and read-out is the formation of DNA strands extruded from the nuclei, and traditionally assessed by fluores...

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Main Authors: Emilia A. Barbu, Venina M. Dominical, Laurel Mendelsohn, Swee Lay Thein
Format: Article
Language:English
Published: Frontiers Media S.A. 2020-07-01
Series:Frontiers in Immunology
Subjects:
PMN
NETs
H4cit3
imaging flow cytometry
stimulus-dependent
Online Access:https://www.frontiersin.org/article/10.3389/fimmu.2020.01335/full
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spelling doaj-cacd4d3a7bf44e308b14678300b47f7d2020-11-25T03:02:43ZengFrontiers Media S.A.Frontiers in Immunology1664-32242020-07-011110.3389/fimmu.2020.01335479108Detection and Quantification of Histone H4 Citrullination in Early NETosis With Image Flow Cytometry Version 4Emilia A. Barbu0Venina M. Dominical1Laurel Mendelsohn2Swee Lay Thein3Sickle Cell Branch, National Heart, Lung, and Blood Institute, NIH, Bethesda, MD, United StatesFlow Cytometry Core Facility, National Heart, Lung, and Blood Institute, NIH, Bethesda, MD, United StatesSickle Cell Branch, National Heart, Lung, and Blood Institute, NIH, Bethesda, MD, United StatesSickle Cell Branch, National Heart, Lung, and Blood Institute, NIH, Bethesda, MD, United StatesNeutrophil extracellular traps (NETs) formation has been implicated in an increasing number of infectious and non-infectious pathologies. NETosis is a tightly regulated process; the end-stage and read-out is the formation of DNA strands extruded from the nuclei, and traditionally assessed by fluorescence microscopy. Since NETosis has emerged as a possible biomarker of the inflammatory process, there is a need for less time-consuming, consistent, and quantitative approaches to improve its application in clinical assessment of pro-inflammatory conditions. Imaging Flow Cytometry (IFC) combines features of conventional flow cytometry with qualitative power of fluorescence microscopy and has an added advantage of the capability of assessing the early processes leading up to extrusion of the DNA-scaffolded strands. We explored the optimal imaging-based tools that can be used to measure citrullination of H4 in early NETosis. IFC identified and quantified histone 4 citrullination (H4cit3) induced with several known NETosis stimuli (Ionophore, PMA, LPS, Hemin, and IL-8) following treatment periods ranging from 2 to 60 min. Its relationship with other alterations at nuclear and cellular level, such as nuclear decondensation and super-condensation, multi-lobulated nuclei vs. 1-lobe nuclei and cell membrane damage, were also quantified. We show that the early progress of the H4cit3 response in NETosis depends on the stimulus. Our method identifies fast (Ionophore and Hemin), intermediate and slow (PMA) inducers and shows that H4cit3 appears to have a limited contribution to both early LPS- and IL-8-induced NETosis. While this method is rapid and of a higher throughput compared to fluorescence microscopy, detection and quantification is limited to H4cit3-mediated nuclear events and is likely to be stimulus- and signaling pathway dependent.https://www.frontiersin.org/article/10.3389/fimmu.2020.01335/fullPMNNETsH4cit3imaging flow cytometrystimulus-dependent
collection DOAJ
language English
format Article
sources DOAJ
author Emilia A. Barbu
Venina M. Dominical
Laurel Mendelsohn
Swee Lay Thein
spellingShingle Emilia A. Barbu
Venina M. Dominical
Laurel Mendelsohn
Swee Lay Thein
Detection and Quantification of Histone H4 Citrullination in Early NETosis With Image Flow Cytometry Version 4
Frontiers in Immunology
PMN
NETs
H4cit3
imaging flow cytometry
stimulus-dependent
author_facet Emilia A. Barbu
Venina M. Dominical
Laurel Mendelsohn
Swee Lay Thein
author_sort Emilia A. Barbu
title Detection and Quantification of Histone H4 Citrullination in Early NETosis With Image Flow Cytometry Version 4
title_short Detection and Quantification of Histone H4 Citrullination in Early NETosis With Image Flow Cytometry Version 4
title_full Detection and Quantification of Histone H4 Citrullination in Early NETosis With Image Flow Cytometry Version 4
title_fullStr Detection and Quantification of Histone H4 Citrullination in Early NETosis With Image Flow Cytometry Version 4
title_full_unstemmed Detection and Quantification of Histone H4 Citrullination in Early NETosis With Image Flow Cytometry Version 4
title_sort detection and quantification of histone h4 citrullination in early netosis with image flow cytometry version 4
publisher Frontiers Media S.A.
series Frontiers in Immunology
issn 1664-3224
publishDate 2020-07-01
description Neutrophil extracellular traps (NETs) formation has been implicated in an increasing number of infectious and non-infectious pathologies. NETosis is a tightly regulated process; the end-stage and read-out is the formation of DNA strands extruded from the nuclei, and traditionally assessed by fluorescence microscopy. Since NETosis has emerged as a possible biomarker of the inflammatory process, there is a need for less time-consuming, consistent, and quantitative approaches to improve its application in clinical assessment of pro-inflammatory conditions. Imaging Flow Cytometry (IFC) combines features of conventional flow cytometry with qualitative power of fluorescence microscopy and has an added advantage of the capability of assessing the early processes leading up to extrusion of the DNA-scaffolded strands. We explored the optimal imaging-based tools that can be used to measure citrullination of H4 in early NETosis. IFC identified and quantified histone 4 citrullination (H4cit3) induced with several known NETosis stimuli (Ionophore, PMA, LPS, Hemin, and IL-8) following treatment periods ranging from 2 to 60 min. Its relationship with other alterations at nuclear and cellular level, such as nuclear decondensation and super-condensation, multi-lobulated nuclei vs. 1-lobe nuclei and cell membrane damage, were also quantified. We show that the early progress of the H4cit3 response in NETosis depends on the stimulus. Our method identifies fast (Ionophore and Hemin), intermediate and slow (PMA) inducers and shows that H4cit3 appears to have a limited contribution to both early LPS- and IL-8-induced NETosis. While this method is rapid and of a higher throughput compared to fluorescence microscopy, detection and quantification is limited to H4cit3-mediated nuclear events and is likely to be stimulus- and signaling pathway dependent.
topic PMN
NETs
H4cit3
imaging flow cytometry
stimulus-dependent
url https://www.frontiersin.org/article/10.3389/fimmu.2020.01335/full
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AT laurelmendelsohn detectionandquantificationofhistoneh4citrullinationinearlynetosiswithimageflowcytometryversion4
AT sweelaythein detectionandquantificationofhistoneh4citrullinationinearlynetosiswithimageflowcytometryversion4
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