2018
DOI: 10.1186/s12575-018-0072-y
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DNA Area and NETosis Analysis (DANA): a High-Throughput Method to Quantify Neutrophil Extracellular Traps in Fluorescent Microscope Images

Abstract: BackgroundNeutrophil extracellular traps (NETs), extracellular structures composed of decondensed chromatin and antimicrobial molecules, are released in a process called NETosis. NETs, which are part of normal host defense, have also been implicated in multiple human diseases. Unfortunately, methods for quantifying NETs have limitations which constrain the study of NETs in disease. Establishing optimal methods for NET quantification holds the potential to further elucidate the role of NETs in normal and pathol… Show more

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Cited by 50 publications
(63 citation statements)
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“…For automatic analysis, we used ImageJ software with the DANA plug-in to quantify the area, raw integrated density, aspect ratio, roundness, maximum and minimum brightness, and solidity of each region of interest of 49,6-diamidino-2phenylindole dihydrochloride-labeled neutrophils, as previously described. 30…”
Section: Analysis Of Netsmentioning
confidence: 99%
“…For automatic analysis, we used ImageJ software with the DANA plug-in to quantify the area, raw integrated density, aspect ratio, roundness, maximum and minimum brightness, and solidity of each region of interest of 49,6-diamidino-2phenylindole dihydrochloride-labeled neutrophils, as previously described. 30…”
Section: Analysis Of Netsmentioning
confidence: 99%
“…Furthermore, there are multiple methodologies used to quantitatively assess the process of NETs formation-some of them relying on the measurement of the extracellular DNA using DNA-intercalating dyes, some of them using ELISA measurements of DNA complexed with neutrophil-derived proteins, and others are based on the analysis of microscopical images with manual or automated counting [10,[54][55][56]. Even though a number of automated or semi-automated methodologies to quantify NETs based on microscopy images have been proposed [11,14,20], some of them relatively easy to implement on a large scale [12,13,17], still very few of them have been widely adopted by other researchers. Recently, an imaging flow cytometry has been proposed as a method for automatic determination of NETosis [21,57].…”
Section: Discussionmentioning
confidence: 99%
“…What is more, simple immune processing of the samples would not allow to differentiate, whether changes in the nucleus morphology coincide with the disruption of plasma membrane. Live imaging of cells appears to be a good alternative to immune labelling, since it requires less processing and entails much lower risk of introducing artifacts [13,17,19]. However, immune-histological staining may be necessary to confirm the presence of NETs if uncommon inducers are used or in samples consisting of mixed cell populations (not solely isolated granulocytes).…”
Section: Discussionmentioning
confidence: 99%
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