Measuring apoptosis by microscopy and flow cytometry. Sep 21, 2000 techniques designed to identify, quantitate and characterize apoptosis are numerous, but flow cytometry fcm remains the methodology of choice to study the apoptotic cascade in relation to cell type, trigger and time. Apoptosis detection by flow cytometry springerlink. In a multicellular organism, quantification of apcd is more problematic due to the complex nature of the tissue. The software used to deconvolute the dna content frequency histograms, to estimate the proportions of cells. These distinctive typical forms of morphological changes in apoptotic cells are widely used for the identification and quantification of apoptosis. Normal top row and apoptotic hl60 human promyelocytic cell line cells, stained with pi and viewed by confocal microscopy. To quantify these fluorescence microscopy observations, apoptotic cells were examined by flow cytometry to measure the levels of exposure of myhiia in apoptotic cells. V fitc apoptosis detection kit provides a set of reagents for the detection of apoptosis using flow cytometry. Pdf detection of dna strand breaks in apoptotic cells by. Pdf analysis of cell cycle by flow cytometry methods. Both annexin v and ethidium homodimer iii rely upon the presence of intact membranes in healthy cells to accurately distinguish healthy cells from apoptotic or necrotic cells. Flow cytometry analysis showing a onestage electronic gating strategy used to identify viable cells, early apoptotic cells a5.
Measurement of apoptosis by scan, a system for counting and. Furthermore, the approach appears to underestimate the rate of apoptosis by 2fold to 3fold. Flow cytometry is the technical process that allows for the individual measurements of cell fluorescence and light scattering. The annexin vlabeling method can be improved by the staining with the vital dye 7aminoactinomycin d 7aad 11 to identify early and late apoptotic cells and necrotic ones. Flow cytometry of apoptotic cell death sciencedirect. Apoptotic cells displayed typical common features such as cell shrinkage, nuclear condensation, membrane blebbing, chromatin cleavage, and formation of pyknotic bodies of condensed chromatin. Ultrastructural features of apoptotic cells in den2 virusinfected monocytes. This information can be used to individually sort or separate subpopulations of cells.
Lackof chronic immune activation in hivinfected chimpanzees correlates with the resistance of t cells to fasapo1 cd95induced apoptosis and preservation of a th1 phenotype. Z darzynkiewicz, s bruno, g del bino, w gorczyca, m a hotz, p lassota, f traganos. Annexin v flow cytometry antibodies the aim was to study the role of various factors in bcell survival in vitro. Darzynkiewicz z, bruno s, del bino g, gorczyca w, hotz ma, lassota p, traganos f. Continued clearance of apoptotic cells critically depends on the phagocyte ucp2 protein. The first two are based on univariate analysis of cellular dna content following cell staining with either. Pdf overcoming limitations of microparticle measurement. Using flow cytometry to follow the apoptotic cascade.
Depending on the kind of sample to be analyzed and equipment available, a decision tree for selecting appropriate tools for the detection of apoptosis is listed on pages 89. These dna fragments can be extracted from apoptotic cells and result in the appearance of dna laddering when the dna is analyzed by agarose gel electrophoresis. Cell death, however, may be atypical, lacking the single measured attribute, or hav. Annexin v staining was used to detect apoptotic cells. Mitochondrial fission promotes the continued clearance of apoptotic cells by macrophages.
Measurement of caspase 3 activity with phiphilux g1d2 in both populations shows a caspase 3high cell populaton in the supposedly viable cell. Thapsigargin increases apoptotic cell death in human. Flow cytometry kit for apoptosis apobrdu datasheet. Detection of apoptosis using the bd annexin v fitc assay. Since then, a series of biochemical changes have been described. Apoptosis is a highly regulated process and involves a significant number of signaling pathways. Flow cytometry in analysis of cell cycle and apoptosis. M in control cells, apoptotic cells without stabilization, stabilized apoptotic cells and. To determine the percentage of early and late apoptotic cells in rtexposed cultures, conventional flow cytometry was performed using annexin vfitc and pi. Features of apoptotic cells measured by flow cytometry. Recently, we established a cell staining and flow cytometry approach that can identify apobds from viable, apoptotic and necrotic cells based on relative size and granularity, in addition to. Label one group as the control cells and the other as the treated cells. Estimation of cell viability by flow cytometry springerlink.
Methods for distinguishing apoptotic from necrotic necroptotic cells. The following cell features were found useful to characterize the mode of cell death. One approach relies on extraction of highly degraded, low molecular weight dna prior to, or at the time of, cell staining. By their ability to exclude pi, apoptotic cells can be erroneously classified by flow cytometry as viable cells. Determination of any one or a combination of these changes by flow cytometry. The difference in fluorescence intensity between apoptotic and nonapoptotic cells stained by our fluorescent annexin v conjugates, as measured by flow cytometry, is typically about 100fold figure 15.
Multiparametric analysis of apoptosis by flow and image cytometry. Determining the contents and cell origins of apoptotic bodies. Clear resolution of live apoptotic and nonapoptotic cells. Measure of dna fragmentation during apoptosis by flow cytometry. Flow cytometry and fluorescence microscopy are alternative techniques for investigating heterogeneous cell populations. Traganos the cancer research institute, new york medical college, valhalla, new york 10595 received for publication march 27, 1992. Apoptotic cells display a range of common characteristics that include cell shrinkage, plasma membrane blebbing, cell detachment, nuclear condensation, dna fragmentation, externalization of phosphatidylserine ps and activation of caspases. The apoptosis, dna damage, and cell proliferation kit contains key markers for the simultaneous determination of these important cellular states by flow cytometry saving time and samples, and improving results.
The flow cytometric data acquisition was conducted by using facs calibur becton dickinson, san jose, ca, usa. This process is performed at rates of thousands of cells per second. Morphological recognition of apoptotic cells apoptotic cells. In vivo, except possibly in necrotic centres in large tumours, necrotic and apoptotic cells will be removed from the body by phagocytosis. In nearly all these studies, decreased dna stainability with different f luorochromes has been pro posed as a marker of apoptotic cells. The apoptosis, dna damage, and cell proliferation kit contains key markers for the simultaneous determination of these important cellular states by flow cytometry. One of the most easily measured features of apoptotic cells is the breakup of the genomic dna by cellular nucleases. Ultrastructural features of apoptotic cells in den2 vir openi. Divide the cell suspension into two equal volumes and place each in a tissue culture flask.
Current flow cytometry methods for the quantification of apoptosis identify apoptotic cells and allow the calculation of the apoptotic index ai, i. In contrast, apoptotic cells have an intact plasma membrane. The apoptotic cells with degraded dna appear as cells with hypo diploid dna content and are represented in socalled subg1 peaks on dna histograms. Using flow cytometry, immunofluorescence, or immunohistochemistry, researchers can quickly and accurately determine the cell cycle status or tissue localization of individual cells. This is in contrast to necrotic cells, in which one of the earliest changes is the loss of membrane function and its structural integrity.
These include cell plasma membrane changes, changes in plasma membrane permeability, changes in mitochondrial membrane permeability, caspase activation, and dna cleavage. Methods for using flow cytometry to investigate the relationship between the induction of apoptosis and the cell cycle are discussed. Viable and apoptotic el4 cells can be distinguished based on their scatter properties, the apoptotic cells showing reduced forward scatter and increased side scatter. In addition, we determined myhiia exposure during early andor late apoptosis by staining with avpe and 7aad, which separates live cells avpe. This assay can be adapted to both current and older flow. In single cell organisms, it is possible to quantify levels of apcd by scoring the number of apoptotic cells using flow cytometry instruments. Isolation of cell typespecific apoptotic bodies by. D 7aad which will be subsequently used for measuring apoptotic cell permeability and. Flow cytometry analysis was performed before and after 24 h of culture. Cell death stages in single apoptotic and necrotic cells monitored by.
Their electron microscopic study of prednisoloneinduced cell death in the kidney defined the term apoptosis and provided the standard reference for the key morphological features associated with this form of cell death. Various methods available for detection of apoptotic cells a. Methods apoptosis and secondary necrosis of human lymphoid cells was induced by both uv irradiation and serum starvation. Detection of apoptosis using the bd annexin v fitc assay on the bd facsverse system. The hypodiploid cells were identified as apoptotic. This material was originally published in the purdue cytometry cdrom series,volume 3. Jurkat cells were treated with 200 ngml antifas ch11.
Many chronic lymphocytic leukemia antibodies recognize. Thermo fisher scientific offers a wide range of primary antibodies, elisa kits, multiplexed immunoassays, peptides and recombinant proteins as well as genomic assays targeted to specific proteins. Pdf flow cytometrybased apoptosis detection researchgate. Cytotoxic and apoptotic effects of boron compounds on. Darzynkiewicz z1, bruno s, del bino g, gorczyca w, hotz ma, lassota p, traganos f. The major advantages of flow cytometry include the possibility of multiparameter measurements correlation of different cellular events at a time, single cell analysis. The aim of the present study was to explore whether in situ dna fragmentation during apoptosis is discontinuous or. The methods are illustrated using a specific example of the effect of withdrawing an essential growth factor from a cell. Chapter 1 a brief history of flow cytometry and sorting. Features of apoptotic cells measured by flow cytometry 2. Digestion of chromatin in apoptotic cell microparticles. Detection of dna strand breaks in apoptotic cells by flow and imagecytometry article pdf available in methods in molecular biology clifton, n.
Staining methods for flow cytometry use either fixed cells or treat cells with a hypotonic solution to permit dna staining by nonvital dyes. Apoptosis is a biologically important form of cell death and therefore detection and measurement of apoptosis have become imperative. Many of the above features of apoptosis such as cell detachment and membrane blebbing, as well as nuclear condensation and fragmentation can be observed under the microscope. Flow cytometry approach used to discriminate whole cells from apoptotic bodies by gating in 7aminoactinomycin d 7aadfsc bivariate dotplots. Flow cytometry ploidy determination, cell cycle analysis. Pdf apoptosis detection by flow cytometry researchgate. Apoptosis, dna damage, and cell proliferation kit subject. Pdf an apoptosing cell demonstrates multitude of characteristic. Apoptotic cells were originally recognized by their characteristic morphology. Discontinuous fragmentation of nuclear dna during apoptosis. Cells undergoing apoptosis display typical changes in their morphological and physical properties cell shrinkage, condensation of chromatin and cytoplasm which are well measurable by flow cytometry. Determining the contents and cell origins of apoptotic. Several attempts to distinguish apoptotic cells by flow cytometry were reported 1,10,11,26,44,49,51,52, 56,58.
Apoptotic, necrotic, and healthy cells quantification kit. Analysis of cell cycle by flow cytometry 303 cytometers are becton dickinson immunocytometry systems, beckmancoulter inc. Hl60 cells untreated left or treated right with camptothecin for 3 hours were stained with jc1 and their orange and green fluorescence measured by flow cytometry pozarowski et al. Being a characteristic feature of apoptosis, dna fragmentation provided a basis for the development of two types of flow cytometric assays to identify apoptotic cells. Cell biology a dense, eosinophilic, pyknotic cell surrounded by a thin clear space, often lying within epithelium, which is due to apoptosis. Cells that are in late apoptosis or are already dead are positive for both annexin v and 7aad. Apoptotic cells, thus, exclude viability assay dyes such as trypan blue or pi. Cell sorting was added to the early flow cytometers for two purposes. For the identification of apoptotic cells and discrimination between apoptosis and necrosis, flow cytometry techniques are applied to evaluate for changes in cell morphology, the presence of. Multiparametric analysis of apoptosis by flow and image. Another molecular feature of apoptosis is the activation of caspases, which are inactive enzymes. Apoptotic cells have many characteristics that can be measured by flow cytometry. Flow cytometric measurement of apoptosis and necrosis in cryopreserved pbpc concentrates from patients with malignant diseases.
E the expression of ifninducible marker sca1 on b cells from peripheral blood as measured by flow cytometry. A coefficient of 1 indicates strong correlation, whereas a coefficient of 0 indicates no correlation. This feature, probed by staining with ao at low ph, provided a sensitive and early assay to discriminate between live, apoptotic and necrotic cells, and to evaluate the cell cycle phase specificity of these processes. Darzynkiewicz z1, bruno s, del bino g, gorczyca w, hotz ma. Apoptotic cell definition of apoptotic cell by medical. As a result, apoptotic cells contain a fractional dna content relative to viable cells that can be readily distinguished by flow cytometry. Mitochondrial fission promotes the continued clearance of. Different phases of phagocytosis and digestion of apoptotic cells. C3c3bc3bi surface and intracellular expression on live and apoptotic human t and b primary cells as well as cell lines was monitored by flow cytometry facs, western blot and confocal microscopy. All of the different methods for evaluating viability are based on either direct leak detection or measurement. In nearly all these studies, decreased dna stainability with different f luorochromes has been pro. May 17, 2017 one detects only low numbers of apoptotic cells using such criteria. The major advantages of flow cytometry include the possibility of multiparameter measurements correlation of different cellular events at a time, single cell. Analysis and discrimination of necrosis and apoptosis programmed cell death by multiparameter flow cytometry.
In vitro morphological assessment of apoptosis induced by. Flow cytometric measurement of apoptosis and necrosis in. Because the low molecular weight dna fragments are extracted during cell staining in aqueous solutions, apoptotic cells can be identified on dna content frequency histograms as cells with fractional sub. Ildo nicoletti, roberta mannucci, graziella migliorati 1, carlo riccardi 1 and fausto grignani. Dive c, gregory cd, phipps dj, evans dl, milner ae, wyllie ah. Quantitative measurements of apoptotic cell properties using. The estimation of the viability of a cell population by flow cytometry is based on a simple yet powerful principle. Flow cytometry enumeration of apoptotic cancer cells by. Analysis of apoptosis by laser scanning cytometry bedner. Described are four widely used procedures to analyze the cell cycle by flow cytometry.
These include cell plasma membrane changes, changes in plasma. Measurement of apoptosis in cell culture springerlink. Suspend the cells in fresh cell culture media at a concentration of 1. A number of these can be exploited to discriminate vital and dying cells and to analyse the extent and the type of cell death apoptosis or necrosis. Measurement of apoptotic cells by flow cytometry tunnel. In order to perform analysis of apoptotic versus necrotic necroptotic cells, one can do analysis of morphology by timelapse microscopy, flow fluorocytometry, and transmission electron microscopy. Flow cytometry techniques that are widely used in studies of cell death, and particularly in the identification of apoptotic cells, generally rely on the measurement of a single characteristic biochemical or molecular attribute. Biochemical events lead to characteristic cell changes and death. Detecting cell apoptosis on tissue slides bitesize bio.
Analysis of apoptotic cells using the bd facsarraybioanalyzer. Necrotic cells are usually defined by the lack of integrity of the plasma membrane, which can be measured by the flow cytometer. Thus, a series of methods have been proposed for measuring apoptotic cell death through evaluation of light scattering parameters of cells. A second use of flow cytometry is for the analysis of the cell cycle in the nuclei and of the division frequency, expressed through the mitotic index mi, of the cell population studied. Dissociation of phagocyte recognition of cells undergoing. Fixation, freezing, sectioning, or dissociation of tissues can affect the ps on the outer leaflet and compromise membrane integrity. Apoptosis is characterised by a series of common morphological and biochemical features that include cell shrinkage, membrane blebbing, cell detachment, nuclear condensation, dna fragmentation, mitochondrial fragmentation, externalization of plasma membrane phosphatidylserine ps and activation of apoptotic caspases. Cell death stages in single apoptotic and necrotic cells. Use of flow cytometry for detection of apoptotic cell death. However, it has yet to be established whether any of these changes unequivocally identify an apoptotic cell. Since one of the recorded parameters is the time of cell measurement, the file merge feature allows determination of time resolved events such as enzyme kinetics or efflux reactions within individual cells. Using this method, a single observation is unable to distinguish cells that have undergone apoptotic death from those that have died as a result of a necrotic pathway. Cell state classification for imaging flow cytometry. Investigating the relationship between the cell cycle and.