Collection of gametes from live axolotl, Ambystoma mexicanum, and standardization of in vitro fertilization

This study established the first protocol for collection of gametes from live axolotl, Ambystoma mexicanum, by gentle abdominal massage and in vitro fertilization. To stimulate spermiation and ovulation, human chorionic gonadotrophin (hCG) and Ovopel pellets, which are commercially used to stimulate...

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Bibliographic Details
Published in:Theriogenology 2011-01, Vol.75 (2), p.354-361
Main Authors: Mansour, N., Lahnsteiner, F., Patzner, R.A.
Format: Article
Language:English
Subjects:
abdominal massage semen collection technique
Ambystoma
Ambystoma mexicanum
Ambystoma mexicanum - physiology
Amphibians
Animals
Axolotl
Cell Separation
embryogenesis
Female
Fertilization
Fertilization in Vitro - methods
Fertilization in Vitro - standards
Fertilization in Vitro - veterinary
germ cells
Germ Cells - cytology
Handling (Psychology)
human chorionic gonadotropin
in vitro fertilization
Male
Oocyte Retrieval - methods
Oocyte Retrieval - standards
Oocyte Retrieval - veterinary
osmolality
ovulation
Quality Control
Reference Standards
salamanders and newts
Semen
simulation models
spawning
Sperm Retrieval - standards
Sperm Retrieval - veterinary
Urodele
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Summary:This study established the first protocol for collection of gametes from live axolotl, Ambystoma mexicanum, by gentle abdominal massage and in vitro fertilization. To stimulate spermiation and ovulation, human chorionic gonadotrophin (hCG) and Ovopel pellets, which are commercially used to stimulate spawning in fish, were tested. The hCG was more effective than Ovopel pellets and yielded a higher semen volume in the injected males and a shorter response time in the females. Collected semen by this method was already motile and fertile. Fertile eggs could be collected in 3–4 successive collection times after the female has started the typical spawning behaviour. The fertilization condition that yielded the highest hatching rate was mixing semen with eggs before the addition of a fertilization saline solution (20 mmol/l NaCl, 1 mmol/l KCl, 1 mmol/l Mg 2SO 4, 1 mmol Ca 2Cl, 3 mmol NaHCO 3, 10 mmol/l Tris, pH 8.5 – Osmolality = 65 mosmol/kg). When the pH of the fertilization solution was increased to ≥ 10, the hatching rate was significantly increased. The use of fertilization solutions with osmolalities of ≥ 150 and ≥ 182 were accompanied with a significant decrease in hatching rates and the appearance of deformed larvae, respectively. In conclusion, a reliable protocol for gamete collection from live axolotl is established as a laboratory model of in vitro fertilization for urodele amphibians. This protocol may be transferable to endangered urodeles.
ISSN:0093-691X
1879-3231
DOI:10.1016/j.theriogenology.2010.09.006