Isolation, in vitro culture, and characterization of black crappie, Pomoxis nigromaculatus and white crappie, P. annularis ovarian tissue primary cells

Investigations were conducted to develop a general protocol for the isolation and in vitro culture of ovary‐derived cells from black crappie, Pomoxis nigromaculatus, and white crappie, P. annularis. Five digestive enzymes: 500 U/mL collagenase type I, 500 U/mL collagenase type IV, 0.05% trypsin‐EDTA...

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Published inJournal of the World Aquaculture Society Vol. 54; no. 6; pp. 1534 - 1545
Main Authors Bhattarai, Sujan, Jones, Jacob H., Renukdas, Nilima N., Kelly, Anita M., Perera, Dayan A.
Format Journal Article
LanguageEnglish
Published Hoboken, USA Wiley Subscription Services, Inc 01.12.2023
John Wiley & Sons, Inc
Wiley
Subjects
Cell culture
Cell size
Cells
Collagen (type I)
Collagenase
crappie
Culture media
Digestive enzymes
Dissociation
Edetic acid
Ethylenediaminetetraacetic acids
Fetal calf serum
Flasks
Freshwater fishes
Growth media
Incubation
Incubation period
incubation temperature
Inoculation
ovarian cell isolation
Ovaries
Pomoxis annularis
Pomoxis nigromaculatus
primary cell culture
Serum
Substrates
TrypLE™ express
Trypsin
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Summary:Investigations were conducted to develop a general protocol for the isolation and in vitro culture of ovary‐derived cells from black crappie, Pomoxis nigromaculatus, and white crappie, P. annularis. Five digestive enzymes: 500 U/mL collagenase type I, 500 U/mL collagenase type IV, 0.05% trypsin‐EDTA, 0.25% trypsin‐EDTA, and 1X TrypLE™ Express were evaluated for live cell isolation. The isolated cells were cultured in 10 or 20% fetal bovine serum (FBS) in L‐15 growth media. In addition, four incubation temperatures (15°C, 20°C, 25°C, and 30°C) were also evaluated. The number of live cells obtained from the 0.25% trypsin and TrypLE™ Express treatments was significantly higher than other treatments. No difference in cell growth was observed between the two FBS treatments. Cells isolated using TrypLE™ Express and 0.25% trypsin reached 80% to 90% confluency in 12.5 cm2 cell culture flasks within 5 days of inoculation at 20 and 25°C. At 15°C, 10 days were required to reach 80%–90% confluency. Morphologically, cells incubated at 15°C, 20°C, and 25°C appeared healthier than cells incubated at 30°C, where irregular cell shape and substrate detachment were observed. We concluded TrypLE™ Express and 0.25% trypsin were optimal for cell dissociation and isolation of crappie ovarian cells. An incubation temperature of 20°C–25°C was favorable for cell culture in L‐15 media supplemented with either 10% or 20% FBS.
Bibliography:Sujan Bhattarai and Dayan A. Perera are the primary contributors and Co‐First Authors of this Manuscript.
ISSN:0893-8849
1749-7345
DOI:10.1111/jwas.12981