| Literature DB >> 26779908 |
Inês Júlia Ribas Wajsenzon1,2, Litia Alves de Carvalho3,2,4, Adriano Biancalana5, Wagner Antönio Barbosa da Silva3,2, Claudia Dos Santos Mermelstein6, Elizabeth Giestal de Araujo7, Silvana Allodi8,9,10.
Abstract
Although there is a considerable demand for cell culture protocols from invertebrates for both basic and applied research, few attempts have been made to culture neural cells of crustaceans. We describe an in vitro method that permits the proliferation, growth and characterization of neural cells from the visual system of an adult decapod crustacean. We explain the coating of the culture plates with different adhesive substrates, and the adaptation of the medium to maintain viable neural cells for up to 7 days. Scanning electron microscopy allowed us to monitor the conditioned culture medium to assess cell morphology and cell damage. We quantified cells in the different substrates and performed statistical analyses. Of the most commonly used substrates, poly-L-ornithine was found to be the best for maintaining neural cells for 7 days. We characterized glial cells and neurons, and observed cell proliferation using immunocytochemical reactions with specific markers. This protocol was designed to aid in conducting investigations of adult crustacean neural cells in culture. We believe that an advantage of this method is the potential for adaptation to neural cells from other arthropods and even other groups of invertebrates.Entities:
Keywords: Cell culture; Glia; Immunocytochemistry; Invertebrates; Neurons; Visual system
Year: 2016 PMID: 26779908 PMCID: PMC5023563 DOI: 10.1007/s10616-015-9942-1
Source DB: PubMed Journal: Cytotechnology ISSN: 0920-9069 Impact factor: 2.058