Evaluation of different media for cell proliferation in mantle tissue culture of the green mussel, Perna viridis (Linnaeus, 1758)

Suja, C P; Raghavan, Srinivasa; Jayasankar, Vidya; Divipala, Indira; Mohamed, M Bareen; Mary, B Koncies; Vijayan, K.

doi:10.21077/ijf.2017.64.special-issue.76285-34

Cited by 6 publications

(7 citation statements)

References 18 publications

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“…On the contrary, cells cultured in Leibovitz's L-15 demonstrated a lower cell growth. The current finding is in contrast to previous studies which suggested L-15 as a suitable media for molluscan cell culture of various tissues (Van Der Merwe et al 2010;Dessai 2012;Daugavet and Blinova 2015;Suja et al 2017;Barrick et al 2018). An earlier study by Suja et al (2007) on Haliotis varia mantle tissue demonstrated that L-15 promotes cell proliferation while M199 enhances cell adherence.…”

Section: Discussioncontrasting

confidence: 99%

“…The effectiveness of lipid supplementation was previously demonstrated on oyster's heart cell (Cecil 1969;Domart-Coulon et al 1994;Cornet 1995). On the other hand, fetal bovine serum were shown to enhance mollusc cell culture (Dessai 2012;Suja et al 2017;Barrick et al 2018). High concentration of FBS, however, may cause a detrimental effect to some cells (Kusumoto et al 1997), whilst, batch to batch variations may also have an impact on cell growth.…”

Section: Discussionmentioning

confidence: 99%

“…The difficulty is due to the lack of vital information regarding the cell requirements and their physiology (Rinkevich 2005(Rinkevich , 2011. Several studies had attempted to establish a marine invertebrate primary culture with limited success (Lebel et al 1996;Giard et al 1998;Sera et al 2000;Suja et al 2017). The lack of knowledge on rhogocyte cell physiology has been attributed to the difficulty of isolating and sorting out rhogocyte cells and the poor understanding of optimal culture conditions.…”

Section: Introductionmentioning

confidence: 99%

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Lipoprotein-induced cell growth and hemocyanin biosynthesis in rhogocytes

et al. 2022

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Rhogocyte is a unique molluscan cell that synthesises a supramolecular respiratory protein known as hemocyanin. Its ability to synthesise the protein has eluded the scientists despite hemocyanin’s importance as a carrier protein and complex molecule with anti-viral activity. Although a hypothetical model of hemocyanin release from the rhogocytes lacunae was proposed based on colloid-osmotic pressure mechanism, lack of in vitro studies limits further validation of this model. In this study, we aim to investigate the impact of cell culture conditions and nature of hemocyanin biosynthesis of rhogocyte cells dissociated from Haliotis laevigata mantle tissue. Population of cells with different hemocyanin expression levels was profiled using flow cytometry, while hemocyanin concentrations in the media were elucidated by ELISA assay. We demonstrated that addition of lipoprotein supplement into the media resulted in a burst secretion of hemocyanin into the culture media. Over 7 days of culture, the population of cells tagged with hemocyanin antibody increased steadily while hemocyanin release in the media decreased significantly. Variation of culture medium, temperature, growth supplement type and concentration also impacted the cell growth and hemocyanin biosynthesis. These results indicated the possibility of an active process triggered by the addition of supplement to synthesise the protein at the highest amount during the first hour. The current study provides a glimpse of the hemocyanin biosynthesis by rhogocyte that may be significant to understand the cell ability to synthesise supramolecular protein and secretion through lacunae.

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Section: Discussioncontrasting

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Lipoprotein-induced cell growth and hemocyanin biosynthesis in rhogocytes

et al. 2022

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“…The addition of BCS was essential to sustain proliferation, and yeast extract provided stability to the culture media, reducing the variability between cultures. Yeast extract was previously used in culture media as a source of vitamins and other supplements [30]. It is thus reasonable to presume that its addition complements the L-15 formulation and provides unknown useful components for mussel cell maintenance [31].…”

Section: Discussionmentioning

confidence: 99%

In vitroproliferation ofMytilus edulismale germ cell progenitors

Khorami,

Breton,

Angers

2023

Preprint

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Our understanding of basic cellular processes has mostly been provided by mammalian cell culture, and by some non-mammalian vertebrate and few invertebrate cell culture models. Developing reliable culture conditions for non-model organisms is essential to allow investigation of more unusual cellular processes. Here, we investigate how cells isolated from different tissues of the marine musselMytilus edulisthrive and survivein vitroin the hope of establishing a suitable laboratory model for the investigation of cellular mechanisms specific to these bivalve mollusks. We found that cells dissociated from male mantle tissue attached to the culture vessels and proliferated wellin vitro, whereas all other cell types, although remaining viable, did not maintain divisions over three to four weeks in culture. We used antibodies against the germ-line marker DEAD-box helicase 4 (DDX4), also known as VASA, and the epithelial cell marker cytokeratin to distinguish different cell types in culture. DDX4-positive cells were the only cells that significantly proliferated in culture, and only from male tissue samples. Overall, the culture conditions described here allow an efficient selection of male germ cells that could be used to study specific cellular mechanismsin vitro.

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“…However, in this study a relatively simple and cost effective culture medium composed of sterilized seawater supplemented with 0.1% yeast, developed by Jayasankar et al (2018) was used successfully for culture of P. margaritifera mantle explants. Sea water, with or without added factors has been used in earlier studies too as a culture medium for invertebrate cells (Cecil, 1969;Qiao et al, 2003;Suja et al, 2017;van der Merwe et al 2010).The close resemblance of these media to natural seawater, the habitat of marine molluscs, in terms of pH and osmolarity is what makes it an attractive _________________________________________________________________________________________________ Journal of Coastal Research, Special Issue No. 86, 2019 Figure 5.…”

Section: Discussionmentioning

confidence: 99%

Cell Culture and Gene Expression Studies in Relation to Biomineralization in the Black-lip Pearl Oyster, Pinctada margaritifera

Raghavan

Jayasankar

Suja

et al. 2019

Journal of Coastal Research

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Srinivasa Raghavan, V.; Jayasankar, V.; Suja, C.P., and Laxmilatha, P., 2019. Cell culture and gene expression studies in relation to biomineralization in the black-lip pearl oyster, Pinctada margaritifera. In: Jithendran, K.P.; Saraswathy, R.; Balasubramanian, C.P.; Kumaraguru Vasagam, K.P.; Jayasankar, V.; Raghavan, R.; Alavandi, S.Nacre is composed of aragonite platelets and organic material formed by molluscs as inner shell layer through biomineralization process, and mantle epithelial cells control nacre formation. A primary culture of granulated epithelial cells was established from mantle tissue of Pinctada margaritifera, through a process of continuous subculturing at 28°C in yeast supplemented sea water culture medium. Nuclear beads were placed in culture wells containing semi-solid agar medium and incubated in vitro with cultured granulated epithelial cells in order to evaluate the nacre secretion. On visual observation, a brown coloration was observed on the surface of the bead after 7-10 days. Evaluation of the surface of the nuclear beads by scanning electron microscopy (SEM) after 60 days of incubation revealed a good brick and mortar pattern, characteristic of nacreous layer formation. A lustrous hue was also seen to develop on bead surfaces after this stage. SEM images of a cross section of the nacre-coated bead showed a pattern of arrangement of aragonite tablets similar to that seen in cross sections of the nacre layer of shell of molluscs. The functional ability of cultured granulated epithelial cells was further confirmed by detecting gene expression of two matrix proteins, nacrein and amorphous calcium carbonate binding proteins (ACCBP), which play an important role in formation of the nacreous layer, in both cultured cells and in native mantle tissue. Amplification products for nacrein (480 bp) and ACCBP (500 bp) genes were obtained in both native mantle tissue and in vitro cultured mantle epithelial cells. There was good correlation between the expression patterns of the two genes in in vitro cultured cells and in native mantle tissue, signifying that cultured mantle epithelial cells retain their functional characteristics of biomineralization. ADDITIONAL INDEX WORDS: ACCBP, biomineralization, mantle, nacre, nacrein, pearl oyster. LITERATURE CITED Auzoux-Bordenave, S.; Fouchereau-Peron, M.; Helleouet, M.N., and Doumenc, D., 2007. CGRP regulates the activity of mantle cells and hemocytes in abalone primary cell cultures. Journal of Shellfish Research, 26, 887-894. Awaji, M. and Machii, A., 2011. Fundamental studies on in vivo and in vitro pearl formation: contribution of outer epithelial cells of pearl oyster mantle and pearl sacs. Aqua-BioScience Monographs, 4, 1-39. Awaji, M.; Yamamoto, T.; Kakinuma, M.; Nagai, K., and Watabe, S., 2014. Pearl formation by transplantation of outer epithelial cells isolated from the mantle of pearl oyster Pinctada fucata. Nippon Suisan Gakkaishi, 80, 578-588 (Japanese). Bellaaj-Zouari, A.; Dkhili, S.; Gharsalli, R.; Derbali, A., and Aloui-Bejaoui, N., 2011. ...

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Evaluation of different media for cell proliferation in mantle tissue culture of the green mussel, Perna viridis (Linnaeus, 1758)

Cited by 6 publications

References 18 publications

Lipoprotein-induced cell growth and hemocyanin biosynthesis in rhogocytes

Lipoprotein-induced cell growth and hemocyanin biosynthesis in rhogocytes

In vitroproliferation ofMytilus edulismale germ cell progenitors

Cell Culture and Gene Expression Studies in Relation to Biomineralization in the Black-lip Pearl Oyster, Pinctada margaritifera

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