2010
DOI: 10.1007/s00424-010-0869-2
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Measurement of the thickness and volume of adherent cells using transmission-through-dye microscopy

Abstract: Cell volume is one of the basic characteristics of a cell and is being extensively studied in relationship to a variety of processes, such as proliferation, apoptosis, fertility, or locomotion. At the same time, its measurement under a microscope has not been well developed. The method we propose uses negative transmission contrast rendered to cells by a strongly absorbing dye present in the extracellular medium. Cells are placed in a shallow compartment, and a nontoxic and cell-impermeant dye, such as acid bl… Show more

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Cited by 34 publications
(38 citation statements)
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References 52 publications
(56 reference statements)
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“…7). This observation is consistent with significant reduction of mean volume in staurosporine-treated HeLa, U937 and NG108-15 cells measured by Coulter-type cell size analyzer [14,28] as well as decrease of single cell volume estimated from the cross-sectional area of cerebellar granule neurones [29] and by recently developed 3D reconstruction technique using negative transmission contrast rendered to T24 cells by strongly colored membrane-impermeable dye [30]. Third, decreased cell volume detected in cells undergoing apoptosis can be at least partially explained by secondary events, such as plasma membrane budding and the formation of apoptotic bodies rather than by primary shrinkage triggered by outwardly directed movements of intracellular osmolytes and osmotically obliged water.…”
Section: Discussionsupporting
confidence: 88%
“…7). This observation is consistent with significant reduction of mean volume in staurosporine-treated HeLa, U937 and NG108-15 cells measured by Coulter-type cell size analyzer [14,28] as well as decrease of single cell volume estimated from the cross-sectional area of cerebellar granule neurones [29] and by recently developed 3D reconstruction technique using negative transmission contrast rendered to T24 cells by strongly colored membrane-impermeable dye [30]. Third, decreased cell volume detected in cells undergoing apoptosis can be at least partially explained by secondary events, such as plasma membrane budding and the formation of apoptotic bodies rather than by primary shrinkage triggered by outwardly directed movements of intracellular osmolytes and osmotically obliged water.…”
Section: Discussionsupporting
confidence: 88%
“…6 A fast and resistant to instability of the light source technique is developed to obtain the volume and thickness of the adherent cells. 7 It is an essential need to have access to a comprehensive model of the mechanical probe to study the dynamic behavior of the AFM system and having a precise control scheme for acquiring high-resolution image of the ultra-small materials. For this aim, there are various research works studying different models for the AFM system.…”
Section: Introductionmentioning
confidence: 99%
“…While we have evidence (11) that AB9 does not enter living cells other than by endocytosis (which can be a slow process), the question becomes critical for chemically fixed samples. Indeed, cells treated with cross-linking fixatives paraformaldehyde (PFA) and glutaraldehyde become partially leaky, and the extent of membrane damage may be sensitive to fixation conditions (14).…”
mentioning
confidence: 98%
“…When the absorption is too strong, parts of cells lying deep inside the dye may become too dark to be imaged. For imaging of live cells, food colorants Acid Blue 9 (AB9) or Patent Blue V at 510 mg/mL appear to be compatible with normal cell functioning (11); at these concentrations, the absorption at 630 nm is 0.10.2 m 1 , allowing sufficiently deep light penetration to obtain complete images of cell monolayers while keeping the vertical resolution below the diffraction limit (about 0.1 m/pixel).…”
mentioning
confidence: 99%
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