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Cryoprotectant agents and cooling effect on embryos of Macrobrachium amazonicum

There are few reports of cryopreservation and injuries in Macrobrachium amazonicum embryos. Thus, the aim of this study was to analyze the effects of cryoprotectants agents and cooling on stage VIII of this species. Fertilized eggs from ovigerous females were removed from the incubation chamber, the...

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Published in:Zygote (Cambridge) 2018-04, Vol.26 (2), p.111-118
Main Authors: Lucas, Caroline Costa, Melo, Luana Rolim, de Sousa, Míriam Luzia Nogueira Martins, de Morais, Glayciane Bezerra, Martins, Moisés Fernandes, Xavier, Francisco Antônio Félix, Evangelista, Janaina Serra Azul Monteiro, de Souza Sampaio, Célia Maria
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container_end_page 118
container_issue 2
container_start_page 111
container_title Zygote (Cambridge)
container_volume 26
creator Lucas, Caroline Costa
Melo, Luana Rolim
de Sousa, Míriam Luzia Nogueira Martins
de Morais, Glayciane Bezerra
Martins, Moisés Fernandes
Xavier, Francisco Antônio Félix
Evangelista, Janaina Serra Azul Monteiro
de Souza Sampaio, Célia Maria
description There are few reports of cryopreservation and injuries in Macrobrachium amazonicum embryos. Thus, the aim of this study was to analyze the effects of cryoprotectants agents and cooling on stage VIII of this species. Fertilized eggs from ovigerous females were removed from the incubation chamber, then placed in 10 ml Falcon tubes with a cryoprotectant solution and saline-free calcium solution. Thus, the embryos underwent a cooling curve of 1°C per min until reaching 5°C, and then were stored for 2 h. The tubes containing the embryos were washed to remove the cryoprotectant, acclimated for 5 min and then transferred to 50 ml incubators. At the end of the 24-h period, living embryos from each tube were counted and tabulated. A pool of embryos was fixed with 4% formaldehyde and then subjected to histology using 3-mm thick sections and stained with haematoxylin/eosin. Another pool was used for biometric analysis in which length, width and volume were analyzed. The cryoprotectants agents used were: dimethylsulfoxide (DMSO), methyl alcohol, ethylene glycol at 1, 5 and 10% and sucrose (0.5 M). Variance analysis was performed followed by Tukey's honest significant difference (HSD) test at 5% significance level. DMSO cryoprotectant affected embryo survival the least with rates of 71.8, 36.2 and 0% for concentrations of 1, 5 and 10%, respectively. Ethylene glycol caused 100% mortality at all the concentrations used. It was not possible to observe the interference of cooling and cryoprotectants on embryonic structures in this study.
doi_str_mv 10.1017/S0967199417000661
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ispartof Zygote (Cambridge), 2018-04, Vol.26 (2), p.111-118
issn 0967-1994
1469-8730
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source Cambridge University Press
subjects Alcohol
Alcohols
Animals
Calcium
Cooling
Cooling curves
Cooling effects
Cryopreservation
Cryoprotectants
Cryoprotectors
Eggs
Embryos
Ethylene glycol
Females
Histology
Incubation
Incubators
Macrobrachium amazonicum
Methanol
Polyethylene terephthalate
Sucrose
Sugar
Temperature
Variance analysis
title Cryoprotectant agents and cooling effect on embryos of Macrobrachium amazonicum
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