Characterization of viability and proliferation of alginate‐poly‐<scp>L</scp>‐lysine–alginate encapsulated myoblasts using flow cytometry

Thakur, Ajit; Sengupta, Ruchira; Matsui, Hideto; Lillicrap, David; Jones, Kim S.; Hortelano, Gonzalo

doi:10.1002/jbm.b.31648

Cited by 18 publications

(17 citation statements)

References 32 publications

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“…Almost all the encapsulated cells (93-98%) were viable after encapsulation, which was similar to the other groups ( Figure 3A). The results were consistent with previous studies (Maguire et al, 2006;Thakur et al, 2010). There were no significant differences among all groups during the progressive stages of apoptosis ( Figure 3B and C).…”

Section: The Effect Of the Encapsulation Process On Cell Apoptosissupporting

confidence: 83%

“…In combination with the annexin V assay, our results indicated that stimuli from encapsulation process did not destroy ER homeostasis. Moreover, not only tumour cells but also normal cells (Thakur et al, 2010), even stem cells (Maguire et al, 2006), maintained viability when cultured within microencapsulate by electrostatic droplet technology. Overall, encapsulation process might be universal and friendly to the mammalian cells.…”

Section: Discussionmentioning

confidence: 99%

“…It is clear that several key non-physiological factors, including suspension status, nutrition-free condition, the high-voltage electrostatic field and shear forces, exist in the electrostatic microencapsulation process. Although previous studies have proven that most of the encapsulated cells are alive and retain their proliferation ability after the electrostatic microencapsulation process (Maguire et al, 2006;Thakur et al, 2010), it is still unknown whether the microencapsulated process influences the biological properties of tumour cells because tumour cells undergo significant environmental changes during this process. Studying the change in cellular biological properties during this process will help us to optimise the preparation conditions of microencapsulation.…”

Section: Introductionmentioning

confidence: 99%

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The effect of electrostatic microencapsulation process on biological properties of tumour cells

Sun

et al. 2013

Journal of Microencapsulation

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Microencapsulation is one of the promising strategies to develop a three-dimensional in vivo tumour-mimic model in cancer research. Although previous studies have shown that tumour cells grow well during the microencapsulated culture, it is still not clear whether the electrostatic encapsulation process has an important effect on cellular characteristics. In this study, we investigated cellular response against non-physiological stress factors existing in the electrostatic microencapsulation process, such as the high-voltage electrostatic field, suspension and nutrition-free status. Our results showed that these non-physiological stress factors did not significantly induce cellular apoptosis, and did not affect cellular adhesion and viability. Furthermore, no change was found about invasion and drug resistance of the tumour cells. The normal endoplasmic reticulum function might play a role in maintaining biological properties during the electrostatic microencapsulation process.

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Section: The Effect Of the Encapsulation Process On Cell Apoptosissupporting

confidence: 83%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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The effect of electrostatic microencapsulation process on biological properties of tumour cells

Sun

et al. 2013

Journal of Microencapsulation

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“…Our method of analysis defines dead cells as those which have a compromised cell membrane. An apoptotic/ necrotic dead cell with a compromised cell membrane is measured by the loss calcein intracellular staining and the change in its size and granularity, while (Bertho et al 2000;Thakur et al 2010). This is inherently more sensitive than relying on the ability of a second dye such as 7-AAD or ethidium bromide to label cells with a damaged cell membrane.…”

Section: Discussionmentioning

confidence: 99%

Single-colour flow cytometric assay to determine NK cell-mediated cytotoxicity and viability against non-adherent human tumor cells

et al. 2011

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A flow cytometry-based cytotoxicity (FCC) assay was developed using a single fluorophore, calcein-acetoxymethyl diacetylester (calcein-AM), to measure NK cell-mediated cytotoxicity. Non-adherent human K562 and U937 target cells were individually labelled with calcein-AM and co-incubated with effector NK cells to measure calcein loss, and therefore calculate target cell cytotoxicity. This FCC assay also provided a measure of sample viability. Notably, cell viability measured by traditional calcein/7-amino-actinomycin D (7-AAD) double labelling and Trypan Blue methods were comparable to the viability calculated using calcein-loss FCC. This FCC assay may also be used with various effector and target cell types and as a multi-parameter tool to measure viability and immunophenotype cells for tissue engineering purposes.

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“…[27] The most widely studied alginate-based formulations involve complexation with polycations, poly-L-lysine and chitosan in particular, to control permeability and increase strength and stability. [28][29][30] Nevertheless, other, different alginate-based formulations have been examined over the years to further improve the effectiveness of cell encapsulation, including cross-linked alginate-gelatine, [31] alginate-poly(ethylene glycol), [32] or alginate and hyaluronic acid stabilized with polyethyleneimine. [33] Together with alginate, different biopolymers capable of gelling under mild conditions have attracted attention as cell carriers.…”

Section: Introductionmentioning

confidence: 98%

Programmed cell delivery from biodegradable microcapsules for tissue repair

Draghi

Brunelli

Farè

et al. 2015

Journal of Biomaterials Science, Polymer Edition

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Injectable and resorbable hydrogels are an extremely attractive class of biomaterials. They make it possible to fill tissue defects accurately with an undoubtedly minimally invasive approach and to locally deliver cells that support repair or regeneration processes. However, their use as a cell carrier is often hindered by inadequate diffusion in bulk. A possible strategy for overcoming this transport limitation might be represented by injection of rapidly degradable cell-loaded microcapsules, so that maximum material thickness is limited by sphere radius. Here, the possibility of achieving programmable release of viable cells from alginate-based microcapsules was explored in vitro, by evaluating variations in material stability resulting from changes in hydrogel composition and assessing cell viability after encapsulation and in vitro release from microcapsules. Degradation of pure alginate microspheres was varied from a few days to several weeks by varying sodium alginate and calcium chloride concentrations. The addition of poloxamer was also found to accelerate degradation significantly, with capsule breakdown almost complete by two weeks, while chitosan was confirmed to strengthen alginate cross-linking. The presence of viable cells inside microspheres was revealed after encapsulation, and released cells were observed for all the formulations tested after a time interval dependent on bead degradation speed. These findings suggest that it may be possible to fine tune capsule breakdown by means of simple changes in material formulation and regulate, and eventually optimize, cell release for tissue repair.

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Characterization of viability and proliferation of alginate‐poly‐L‐lysine–alginate encapsulated myoblasts using flow cytometry

Cited by 18 publications

References 32 publications

The effect of electrostatic microencapsulation process on biological properties of tumour cells

The effect of electrostatic microencapsulation process on biological properties of tumour cells

Single-colour flow cytometric assay to determine NK cell-mediated cytotoxicity and viability against non-adherent human tumor cells

Programmed cell delivery from biodegradable microcapsules for tissue repair

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