8 ± 1 4 au, Fig 4E), compared to controls (21 1 ± 0 6 au, Fig 4

8 ± 1.4 au, Fig. 4E), compared to controls (21.1 ± 0.6 au, Fig. 4A). The lower intensity of green fluorescence in controls (high green, Fig. 4A), is due to the lack of JC-1 monomers present in cells, as under control conditions monomers form aggregates in mitochondria and fluoresce red, lowering the overall intensity of green fluorescence, indicating healthy living cells [42]. The higher peak of fluorescent intensity (high green, Fig. 4E) shows damaged cells with depolarized mitochondria.

Fig. 4A and B along with Fig. 4E and F show that intact and damaged mitochondria are accurately distinguished from debris with a fluorescence threshold. The mitochondrial membrane potential of events identified as cells (from Fig. 4) were also assessed using a one parameter histogram of the intensity of red fluorescence. Fluorouracil supplier The red fluorescence intensity of J-aggregates from the mitochondrial

DNA/RNA Synthesis inhibitor polarization assay JC-1 and the corresponding light scatter properties of HUVEC are presented in Fig. 5. The forward and side light scatter properties of control (Fig. 5A), and plunged (Fig. 5B), samples are presented with a corresponding histogram of JC-1 red fluorescence (Fig. 5C). The high red fluorescence in control cells (red peak, Fig. 5C), is from the formation of J-aggregates present in cells with polarized mitochondria, whereas the low red fluorescence of plunged cells (blue peak, Fig. 5C), occurs when mitochondria are depolarized. Cells with high red fluorescence and corresponding high forward and high side scatter properties indicate cells with intact mitochondria (red) and cells with low red fluorescence and low forward scatter properties indicate cells with damaged mitochondria (blue). JC-1 not only discriminates cells from debris but also reflects the functional capacity of HUVEC based on the polarized state of their mitochondria O-methylated flavonoid indicated by the presence of red fluorescent

J-aggregates. Light scatter is used as a key parameter in flow cytometry to reveal information about cell size and morphological characteristics that can aid in the identification of cell types and subpopulations; however the relationship between light and particle properties is complex. Since Mullaney et al. demonstrated a relationship between forward light scatter and cell volume under the assumption that cells were homogenous spheres with a uniform refractive index [27] a common generalization has emerged that light scatter in the forward direction gives an estimation of cell size. Though volume does play a major role, there are limitations to this generalization, and it has been shown that with polystyrene latex microspheres forward scattered light increases with diameter in a non-linear manner [39], indicating that other factors are also involved.

Leave a Reply

Your email address will not be published. Required fields are marked *

*

You may use these HTML tags and attributes: <a href="" title=""> <abbr title=""> <acronym title=""> <b> <blockquote cite=""> <cite> <code> <del datetime=""> <em> <i> <q cite=""> <strike> <strong>