Effect of Cryoprotectant and Pre-Freezing on the Sperm Motility, Viability and Fertility of Goldfish Carassius Auratus (Pisces: Cyprinidae) Post Short-Term Cryopreservation

Author:

Nurlaili Nurlaili1,Eriani Kartini1,Salma Itsnatani1,Maulida Siti2,Riska Rahayu Sri2,Syafrida Handayani Luvi2,Kocabas Filiz Kutluyer3,Siti-Azizah Mohd Nor4,Wilkes Martin5,Muchlisin Zainal Abidin2

Affiliation:

1. Master Program in Biology, Faculty of Matemathics and Natural Sciences, Syiah Kuala University, Banda Aceh, 23111, Indonesia

2. Department of Aquaculture, Faculty of Marine and Fisheries, Syiah Kuala University, Banda Aceh, 23111 Indonesia

3. Faculty of Fisheries, Munzur University, Turkey

4. Universiti Malaysia Terengganu, Kuala Terengganu, Malaysia

5. University of Essex, Essex, England

Abstract

BACKGRUND: Goldfish Carassius auratus is a popular ornamental fish extensively cultured worldwide. Sperm cryopreservation is a common fish breeding method that ensures sperm availability around the year. Studies on cryopreservation of goldfish sperm, especially on the suitability of cryoprotectant types and pre-freezing time, are scarcely available. OBJECTIVE: To determine the most suitable type of cryoprotectant and pre-freezing for the successful cryopreservation of goldfish sperm. MATERIALS AND METHODS: A completely randomized design with two factors was utilized in this study. The first factor is the type of cryoprotectants, which included methanol, ethanol, ethylene glycol, glycerol, and DMSO. The second is pre-freezing times of 10, 20, 30, and 40 min at each of the pre- freezing temperatures of 4°C, −10°C, and −79°C, meaning that the total times for the ramping down of temperature were 30, 60, 90 and 120 min, respectively. The Ringer solution and 10% egg yolk were used as extender and extracellular cryoprotectant. The sperm was stored at −179°C for 7 days. RESULTS: The ANOVA test showed that cryoprotectants and pre-freezing significantly affected the motility, viability, and fertility of goldfish sperm after freezing in liquid nitrogen for 7 days (ρ<0.05). Furthermore, 10% DMSO combined with 15% egg yolk with an pre-freezing time of 20 min can maintain sperm motility, viability, and fertility higher than other treatments, by 79%, 80%, and 33%, respectively. The agarose gel electrophoresis showed no DNA fragmentation in all samples, including fresh sperm. CONCLUSION: We conclude that 10% DMSO combined with 15% egg yolk and 20 min pre-freezing is the best treatment for goldfish sperm cryopreservation.

Publisher

CryoLetters Limited Liability Partnership

Subject

General Medicine

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