A Novel Rapid Method of Red Blood Cell and Platelet Permeabilization and Staining for Flow Cytometry Analysis

Fauré, Sixtine; Agthoven, Andreas van; Bernot, Denis; Altié, Alexandre; Grino, Michel; Alessi, Marie‐Christine; Malergue, Fabrice; Canault, Matthias

doi:10.1002/cyto.b.21839

Cited by 5 publications

(4 citation statements)

References 28 publications

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“…It was reported that different buffer systems and pH of different staining methods had different effects on cell morphology, integrity, and contents, 23,24 which would lead to a change in cell size. During the process of staining, the hypotonic or hypertonic extracellular environment could change cell size 25,26 .…”

Section: Discussionmentioning

confidence: 99%

“…13 Previous studies showed that protamine-deficient sperm could significantly change the size and shape of sperm heads. 22 So as to determine whether the size of the sperm head is normal or not, a CASMA It was reported that different buffer systems and pH of different staining methods had different effects on cell morphology, integrity, and contents, 23,24 which would lead to a change in cell size. During the process of staining, the hypotonic or hypertonic extracellular environment could change cell size.…”

Section: Discussionmentioning

confidence: 99%

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Effects of six kinds of sperm staining methods on human sperm size and evaluation of their staining effects

Lü

Tang

2022

Clinical Laboratory Analysis

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Background Large‐ and small‐headed sperm are common morphological abnormalities. If different sperm staining methods affect sperm size, they will make a difference in the accuracy of sperm morphological analysis results. In this case, the normal reference values of sperm head parameters for different staining methods should be established. Methods Six sperm staining methods, including Papanicolaou, Diff‐Quik, Shorr, Hematoxylin–eosin (HE), Wright, and Wright‐Giemsa staining, were used to stain the sperm smears of 25 semen samples, respectively. Sperm head parameter's length (L), width (W), area (A), perimeter, acrosomal area (Ac), and the derived values L/W and Ac/A of 2500 sperm (100 for each specimen) per staining method were measured by a computer‐aided sperm morphological analysis system. Results The highest sperm head length and width were observed with the Wright‐Giemsa and Wright staining, followed by the Diff‐Quik. The lowest sperm head length and width were observed with the Papanicolaou staining, and the sperm head length and width of HE and Shorr staining were between those of Papanicolaou and Diff‐Quik staining. There was the same trend in changes in sperm head area and perimeter. Diff‐Quik and Shorr staining could clearly distinguish acrosome and nucleus, followed by HE staining, whereas the boundary between acrosome and nucleus was not evident in Papanicolaou, Wright, and Wright‐Giemsa staining. Conclusion Different staining methods influence sperm size, and the normal reference values of sperm head parameters of each staining method should be established. Diff‐Quik and Shorr staining may be suitable methods for routine sperm morphological analysis.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Effects of six kinds of sperm staining methods on human sperm size and evaluation of their staining effects

Lü

Tang

2022

Clinical Laboratory Analysis

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“…New FCM‐based controls are always paving the way to new avenues of investigating platelet degranulation or red blood cell (RBC) subpopulation, for instance. In 2019, a new and rapid method was developed to stain platelets and RBCs directly from whole blood without washing or toxic fixation with formaldehyde (Fauré et al., 2019). Another study revealed a method to detect intracellular signaling proteins and B‐cell transcription factors at a single‐cell resolution (Marsman, Jorritsma, Ten Brinke, & van Ham, 2020).…”

Section: Discussionmentioning

confidence: 99%

A Guide to Flow Cytometry: Components, Basic Principles, Experimental Design, and Cancer Research Applications

2023

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Flow cytometry (FCM) is a state-of-the-art technique for the qualitative and quantitative assessment of cells and other particles' physical and biological properties. These cells are suspended within a high-velocity fluid stream and pass through a laser beam in single file. The main principle of the FCM instrument is the light scattering and fluorescence emission upon the interaction of the fluorescent particle with the laser beam. It also allows for the physical sorting of particles depending on different parameters. A flow cytometer comprises different components, including fluidic, optics, and electronics systems. This article briefly explains the mechanism of all components of a flow cytometer to clarify the FCM technique's general principles, provides some useful guidelines for the proper design of FCM panels, and highlights some general applications and important applications in cancer research.

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“…Following TX100 treatment, oval biconcave-shaped erythrocytes remain, while cell membrane permeability significantly increases, allowing intake of bovine serum albumin [87]. Recently, the use of the ionic detergent N-lauryl sarcosine increased the permeability of erythrocytes and enabled intracellular binding of antibodies for flow cytometric assays; however, a significant decrease in cell size was also observed [88]. Overall, fluorochrome permeation into the erythrocyte membrane could be enhanced using ionic or nonionic detergents such as Nonidet P-40.…”

Section: Enhancement Of Erythrocyte Membrane Permeability To Fluorochromesmentioning

confidence: 99%

Progress and challenges in the use of fluorescence‐based flow cytometric assays for anti‐malarial drug susceptibility tests

Kulkeaw

2021

Malar J

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Drug-resistant Plasmodium is a frequent global threat in malaria eradication programmes, highlighting the need for new anti-malarial drugs and efficient detection of treatment failure. Plasmodium falciparum culture is essential in drug discovery and resistance surveillance. Microscopy of Giemsa-stained erythrocytes is common for determining anti-malarial effects on the intraerythrocytic development of cultured Plasmodium parasites. Giemsa-based microscopy use is conventional but laborious, and its accuracy depends largely on examiner skill. Given the availability of nucleic acid-binding fluorescent dyes and advances in flow cytometry, the use of various fluorochromes has been frequently attempted for the enumeration of parasitaemia and discrimination of P. falciparum growth in drug susceptibility assays. However, fluorochromes do not meet the requirements of being fast, simple, reliable and sensitive. Thus, this review revisits the utility of fluorochromes, notes previously reported hindrances, and highlights the challenges and opportunities for using fluorochromes in flow cytometer-based drug susceptibility tests. It aims to improve drug discovery and support a resistance surveillance system, an essential feature in combatting malaria.

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A Novel Rapid Method of Red Blood Cell and Platelet Permeabilization and Staining for Flow Cytometry Analysis

Cited by 5 publications

References 28 publications

Effects of six kinds of sperm staining methods on human sperm size and evaluation of their staining effects

Effects of six kinds of sperm staining methods on human sperm size and evaluation of their staining effects

A Guide to Flow Cytometry: Components, Basic Principles, Experimental Design, and Cancer Research Applications

Progress and challenges in the use of fluorescence‐based flow cytometric assays for anti‐malarial drug susceptibility tests

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