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1. An investigation of oxidative stress and antioxidant biomarkers during Greenshell mussel (Perna canaliculus) oocyte cryopreservation

Author

David J. Burritt, L.T. McGowan, H. Robin Tervit, Samantha L. Gale, and Serean L. Adams

Subjects
Male, Perna, Antioxidant, medicine.medical_treatment, Aquaculture, medicine.disease_cause, Antioxidants, Cryopreservation, Andrology, Superoxide dismutase, chemistry.chemical_compound, Food Animals, medicine, Animals, Small Animals, chemistry.chemical_classification, Reactive oxygen species, biology, Equine, Chemistry, Glutathione peroxidase, Glutathione, Spermatozoa, Oxidative Stress, Biochemistry, Catalase, Fertilization, Larva, Oocytes, biology.protein, Female, Animal Science and Zoology, Biomarkers, Oxidative stress
Abstract

Oxidative damage to proteins and lipids, the enzymatic and nonenzymatic antioxidants' response, and the fertilization and development capability of Perna canaliculus oocytes were investigated at critical treatment steps in a previously published controlled-rate cryopreservation protocol. The cryoprotectant (CPA) from this protocol comprises 10% ethylene glycol (v:v) and 0.2 M trehalose (wt/vol) final concentration. Critical treatment steps included (1) seawater control, (2) CPA addition, (3) CPA addition followed by cooling to −6 °C, (4) CPA addition and cooling to −10 °C, and (5) CPA addition and cooling to −35 °C and immersion in liquid nitrogen (LN). The percentage of fertilized oocytes was 53.8 ± 13.3% in the seawater control but was reduced to 26.0 ± 15.6% after −35 °C + LN treatment, whereas development to D-larvae was 21.0 ± 6.4% in the seawater control reduced to 4.8 ± 2.9% after cooling to −6 °C, and was zero at all the subsequent cooling steps. All oxidative damage biomarkers, protein carbonyls (PCs) and lipid hydroperoxides (LPs), and antioxidants, superoxide dismutase (SOD), catalase, glutathione peroxidase, percent reduced glutathione (%GSH), and total glutathione (defined as glutathione; reduced [GSH] plus glutathione disulphide; derived from two molecules of GSH [GSSG]) were measured over all treatments on unfertilized oocytes over a post-treatment recovery period of 0 to 240 minutes in seawater. An ANOVA showed that both treatment and post-treatment periods had significant effects on the concentrations of all biomarkers (P

Published
2014
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2. Multi-technique approach to characterise the effects of cryopreservation on larval development of the Pacific oyster (Crassostrea gigas)

Author

H.R. Tervit, L.T. McGowan, JR Morrish, S Suneja, Andrea C. Alfaro, Serean L. Adams, and Adam B. Rusk

Subjects
Larva, animal structures, Ecology, biology, Cryoprotectant, fungi, Aquatic Science, Pacific oyster, Larval morphology, biology.organism_classification, Trehalose, Cryopreservation, chemistry.chemical_compound, Horticulture, chemistry, Crassostrea, Ethylene glycol, Ecology, Evolution, Behavior and Systematics, Water Science and Technology
Abstract

Cryopreservation experiments were conducted on D-stage larvae of the Pacific oyster (Crassostrea gigas) to investigate the effects of two cryoprotectant solutions and three cooling rates on larval development from 1 to 22 days post-fertilisation. Cryoprotectant solutions were made up to final concentrations (after 1:1 dilution with larvae) of 10% ethylene glycol, 1% polyvinylpyrrolidone and either 0.2 or 0.4 M trehalose. Three cooling rates (0.5, 1 and 2 °C min−1 between −10 and −35 °C post-holding) were tested in an orthogonal design with the two cryoprotectants. Results indicate that control larvae out-performed all cryopreservation treatments for survival, feeding consumption and shell length parameters. However, larvae exposed to 0.4 M trehalose did considerably better than those exposed to 0.2 M trehalose, regardless of cooling rate conditions. Scanning electron and light microscopy observations were used to assess larval morphology and organogenesis, indicating that treatments with surviving larvae ...

Published
2014
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3. Cryopreservation of Greenshell™ mussel (Perna canaliculus) trochophore larvae

Author

Serean L. Adams, H.R. Tervit, John F. Smith, J.R. Morrish, L.T. McGowan, Ellie Watts, Samantha L. Gale, and Estefania Paredes

Subjects
Cryopreservation, Ethylene Glycol, Larva, Perna, biology, Cryoprotectant, Trehalose, Single step, General Medicine, Mussel, biology.organism_classification, General Biochemistry, Genetics and Molecular Biology, Fishery, Cryoprotective Agents, Animal science, Trochophore, Animals, General Agricultural and Biological Sciences, Perna canaliculus, Shellfish
Abstract

The Greenshell™ mussel (Perna canaliculus) is the main shellfish species farmed in New Zealand. The aim of this study was to evaluate the effects of cryoprotectant concentration, loading and unloading strategy as well as freezing and thawing method in order to develop a protocol for cryopreservation of trochophore larvae (16–20 h old). Toxicity tests showed that levels of 10–15% ethylene glycol (EG) were not toxic to larvae and could be loaded and unloaded in a single step. Through cryopreservation experiments, we designed a cryopreservation protocol that enabled 40–60% of trochophores to develop to D-larvae when normalized to controls. The protocol involved: holding at 0 °C for 5 min, then cooling at 1 °C min−1 to −10 °C, holding for a further 5 min, then cooling at 0.5 °C min−1 to −35 °C followed by a 5 min hold and then plunging into liquid nitrogen. A final larval rearing experiment of 18 days was conducted to assess the ability of these frozen larvae to develop further. Results showed that only 2.8% of the frozen trochophores were able to develop to competent pediveligers.

Published
2012
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4. Cryopreservation of Greenshell™ Mussel (Perna canaliculus) sperm. II. Effect of cryopreservation on fertility, motility, viability and chromatin integrity

Author

Robin M. McDonald, Serean L. Adams, Samantha L. Gale, John F. Smith, H. Robin Tervit, and L.T. McGowan

Subjects
endocrine system, urogenital system, media_common.quotation_subject, Motility, Fertility, Aquatic Science, Biology, Oocyte, biology.organism_classification, Sperm, Cryopreservation, Andrology, chemistry.chemical_compound, medicine.anatomical_structure, chemistry, Botany, medicine, Propidium iodide, Perna canaliculus, reproductive and urinary physiology, Fertilisation, media_common
Abstract

The effect of cryopreservation on aspects of sperm function was investigated for sperm of the Greenshell™ mussel ( Perna canaliculus ). Fertility, DNA integrity, viability and motility were measured before and after cryopreservation. Cryopreservation had a significant effect on fertility with many cryopreserved samples failing to achieve 50% oocyte fertilisation at the highest sperm concentration measured. Sperm DNA integrity, measured using the Sperm Chromatin Structure Assay, showed a small but significant increase in DNA damage as a result of cryopreservation. Sperm viability, measured using propidium iodide/SYBR-14 dual staining, decreased significantly following cryopreservation (69.9 ± 3.5% for fresh sperm versus 25.3 ± 2.9% for cryopreserved sperm). Aspects of motility were similarly affected. The number of sperm tracked, curvilinear velocity (VCL), average path velocity (VAP), variation of straight line velocity (PFT), mean angular displacement (MAD), beat cross frequency (BCF), amplitude of lateral head displacement (ALH) and dance mean (DMN) all decreased following cryopreservation. Correlation analyses between the various aspects of sperm function were carried out. However, no single aspect of sperm function was significantly correlated with sperm fertility following cryopreservation. In addition, the technique for fertility measurement is relatively quicker and less dependent on high tech equipment than the other parameters studied. Fertility therefore remains the most important and relevant end point to measure. Further optimisation of the cryopreservation protocol for Greenshell™ mussel sperm is needed to improve post-thaw fertility.

Published
2012
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5. Cryopreservation of Greenshell™ mussel (Perna canaliculus) sperm. I. Establishment of freezing protocol

Author

Samantha L. Gale, Rodney D. Roberts, Serean L. Adams, H. Robin Tervit, John F. Smith, and L.T. McGowan

Subjects
Animal science, Human fertilization, Cryoprotectant, Botany, Mussel, Aquatic Science, Biology, Liquid nitrogen, biology.organism_classification, Sperm, Perna canaliculus, Cryopreservation, Dilution
Abstract

A series of eight experiments was conducted to determine the most suitable cryoprotectants (CPAs), dilution rates and methods of CPA addition as well as freezing method for the cryopreservation of Greenshell™ mussel ( Perna canaliculus ) sperm. The experiments utilized a fertilization assay to determine the treatments that gave the highest post-thaw fertility. The assays revealed that dimethyl sulphoxide (DMSO) gave the best results of the seven CPAs tested. A concentration of DMSO of approximately 12% [volume: volume] in Milli-Q water provided the best results. A dilution rate of 1:1 (sperm: CPA solution) was superior to 1:3 indicating that more concentrated sperm had higher post-thaw fertility. The time that sperm were exposed to the CPA solution prior to freezing had no effect over the range tested which gives some flexibility in the amount of time sperm can be exposed to CPA prior to freezing. The addition of the CPA in either one step or in 4 equal volume steps over two min had no significant effect on fertility and the two different freezing methods (programmable freezer or rack floating above liquid nitrogen) produced similar results. The post-thaw fertility of mussel sperm using the final protocol developed (12% DMSO plus 0.2 M trehalose, sperm diluted 1:1, loaded into 0.5 mL straws and cooled on a rack 3 cm above liquid nitrogen followed by immersion in liquid nitrogen) was significantly reduced in comparison to fresh sperm. On average, approximately 363 x more sperm were required to achieve an equivalent level of fertilization as that of fresh sperm. The method is being used in mussel selective breeding, however, there is considerable between-animal variability. Further refinement to the method may help to improve post-thaw fertility.

Published
2012
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6. Cryopreservation of Greenshell™ Mussel (Perna canaliculus) Sperm

Author

L.T. McGowan, Jolene Taylor, H. Robin Tervit, Serean L. Adams, and John F. Smith

Subjects
endocrine system, biology, urogenital system, business.industry, fungi, Zoology, Mussel, biology.organism_classification, Selective breeding, Sperm, Cryopreservation, Aquaculture, business, Perna canaliculus, reproductive and urinary physiology
Abstract

Cryopreservation is a valuable technique for aquaculture as it enables a library or bank of genetically valuable animals to be maintained in a cost-effective manner. Here, we describe a method to cryopreserve the sperm of the Greenshell™ mussel (Perna canaliculus) and how to use the sperm post-thawing to maximize larval production from thawed sperm in selective breeding.

Published
2014
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7. Cryopreservation of in vitro-produced bovine embryos: Effects of protein type and concentration during freezing or of liposomes during culture on post-thaw survival

Author

P.A. Pugh, L.T. McGowan, A.E.L. Ankersmit, and H.R. Tervit

Subjects
Fertilization in Vitro, Biology, Morula, Cryopreservation, Andrology, Embryonic and Fetal Development, chemistry.chemical_compound, Food Animals, Animals, Bovine embryo, Small Animals, Liposome, Fetus, Equine, Hatching, Embryo, Embryo, Mammalian, In vitro, Sphingomyelins, Blastocyst, Cholesterol, Biochemistry, chemistry, Liposomes, embryonic structures, Cattle, Female, Animal Science and Zoology, Ethylene glycol
Abstract

Two experiments were conducted to examine the effect of membrane stabilization through the modification of in vitro culture medium or freezing medium on post-thaw survival of in vitro-produced bovine embryos. In Experiment 1, Day 7 (Day 0 = day of IVF) late morulae and blastocysts that developed following culture in SOF/aa/BSA (IVC medium) were frozen slowly to -35 degrees C in the presence of 1.5 M ethylene glycol prepared in ovum culture medium (OCM) or in OCM supplemented with 10, 25 or 50% fetal calf serum (FCS) or 5, 10 or 25 mg/mL BSA. Post-thaw survival was assessed by re-expansion and/or hatching following 48 h of culture in IVC medium + 10% FCS. Overall, survival was significantly (P0.01) affected by embryo stage, with more hatched blastocysts surviving (71%) than blastocysts (59%) or late morulae (51%). Addition of FCS significantly (P0.01) reduced survival compared with control embryos or those frozen in BSA-supplemented medium (50.48 vs 68.01 vs 63.53%, respectively). There was also a significant interaction between embryo stage and protein type (P0.05). The survival of late morulae/early blastocysts following freezing was improved in the presence of additional BSA but not FCS. In Experiment 2, the IVC medium was supplemented with liposomes containing lecithin, sphingomyelin and cholesterol. Sphingomyelin and cholesterol at ratios of 1:1, 1:4 and 4:1 were added to 50, 100 or 150 micrograms/mL lecithin to yield a final lipid concentration of 200 micrograms/mL. A further group contained 200 micrograms/mL lecithin only. Blastocysts were frozen in 1.5 M ethylene glycol in OCM, then thawed and assessed as in Experiment 1. The presence of liposomes during IVC did not affect the proportion of cleaved embryos that developed to blastocysts or survival following freezing. However, the survival of blastocysts that developed in the presence of 200 micrograms/mL lecithin only was significantly lower than in any other treatment (6%; P0.03). These studies demonstrate that the protein composition of the freezing medium can significantly affect survival after thawing and that the survival of late morulae can be improved with additional BSA. The presence of lecithin only in the liposome preparation did not affect embryo development, but significantly reduced survival after freezing, suggesting it can affect post-thaw embryo survival, perhaps by altering embryonic membrane composition.

Published
1998
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8. Total protein content and protein synthesis within pre-elongation stage bovine embryos

Author

Jeremy G. Thompson, L.T. McGowan, N.W. Allen, H.R. Tervit, and A.N.M. Sherman

Subjects
biology, Embryo culture, Cell Biology, Protein degradation, In vitro maturation, Andrology, medicine.anatomical_structure, Biochemistry, embryonic structures, Genetics, biology.protein, medicine, Oviduct, Blastocyst, Bovine serum albumin, Incubation, Fertilisation, Developmental Biology
Abstract

Protein content was measured in zona-free bovine oocytes and pre-elongation stage embryos, following in vitro maturation, fertilisation, and then culture in Synthetic Oviduct Fluid medium supplemented with amino acids and 8 mg ml-1 bovine serum albumin (BSA). Values (ng embryo-1) of 122 ± 7.8, 137 ± 8.6, 111 ± 8.8, 115 ± 10.4, 139 ± 9.0 and 152 ± 10.1 were obtained for zona-free mature oocytes, 2-cell (day 2), 8-cell (day 3), compact morula (day 6), blastocyst (day 7), and expanded blastocyst (day 8) stage embryos, respectively. The protein content of day 7 zona-enclosed blastocysts was 337 ± 58.0 ng embryo-1. These values suggest that prior to compaction and blastulation, the early cleavage stage bovine embryo has a higher rate of protein degradation than that of synthesis. Net growth is observed only after initiation of compaction. The protein content of day 7 blastocysts was measured in embryos following in vitro production and culture in the same media supplemented with either 0.5% w/v polyvinyl alcohol (PVA), 8 mg ml-1 BSA, 8 mg ml-1 BSA and further supplemented with 10% fetal calf serum (FCS) from the beginning of culture (FCS-D1), 8 mg ml-1 BSA and 10% FCS from the fourth day of culture (day 5 of development) or from in vivo-derived day 7 blastocysts. Protein content was significantly (P< 0.05) lower in PVA-cultured embryos than other treatments. To determine if this difference in PVA-cultured embryos was due to a difference in the rate of protein synthesis, comparisons were made between day 7 embryos derived from BSA-culture and either PVA-culture, FCS-D1 culture or in vivo-derived embryos. Despite differences in diameter, no significant difference was observed in the incorporation of L-[2,3,4,5,6-3H]-phenylalanine into the TCA-precipitable fraction in any of the three comparisons made. However, incubation in the presence of FITC-labelled BSA or β-casein and examination under either fluorescence or confocal microscopy revealed that protein in the extra-embryonic environment was actively taken up by the trophectoderm of day 7 blastocysts, most likely by endocytosis. These results suggest that exogenous protein is an important nutritive source, probably maintaining intracellular amino acid pools. Results obtained from the production of embryos in protein-free medium should be viewed with the knowledge that such embryos differ metabolically from those embryos grown in the presence of protein, including in vivo-derived embryos. Mol. Reprod. Dev. 50:139–145, 1998. © 1998 Wiley-Liss, Inc.

Published
1998
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9. Effects of culture duration and time of gonadotropin addition on in vitro maturation and fertilization of red deer () oocytes

Author

H.R. Tervit, G.W. Asher, L.T. McGowan, Yutaka Fukui, and R.W. James

Subjects
medicine.medical_specialty, Equine, medicine.drug_class, Semen, Embryo, Biology, Oocyte, Electroejaculation, In vitro, In vitro maturation, Endocrinology, medicine.anatomical_structure, Human fertilization, Food Animals, Internal medicine, medicine, Animal Science and Zoology, Gonadotropin, Small Animals
Abstract

Immature red deer (Cervus elaphus) oocytes (n = 1208) were collected from 1 to 4 - mm diameter follicles on ovaries and then cultured for 16, 20, 24 or 28 h (Groups I to IV) in TCM 199 supplemented with 10% FCS, 1 x 10(6) granulosa cells/ml and 1 microg/ml estradiol at 39 degrees C under 5% CO(2) in air. Gonadotropins (10 microg/ml, FSH and LH) were added to the culture medium at the start of culture (0 h) or after 6 h. Approximately one-third of the oocytes were examined for maturation, and the remainder were fertilized in vitro with frozen-thawed semen collected from a stag by electroejaculation. In vitro fertilized oocytes (n = 309) from four of the maturation treatment (Groups II and III in both gonadotropin treatments) were cultured for 7 d and examined for cleavage. Oocytes cultured for 16 h (Group I) had lower (P < 0.001) maturation rates (4.7%) than those in the longer culture durations (Groups II to IV: 68.9%). Culture for 20 (Group II) and 24 h (Group III) resulted in higher (P

Published
1991
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10. Towards cryopreservation of Greenshell mussel (Perna canaliculus) oocytes

Author

John F. Smith, Samantha L. Gale, Liliana Salinas-Flores, L.T. McGowan, Serean L. Adams, Rodney D. Roberts, Stephen C. Webb, H. Robin Tervit, Steven F. Mullen, and John K. Critser

Subjects
Perna, Cryoprotectant, Aquaculture, Biology, General Biochemistry, Genetics and Molecular Biology, Cryopreservation, chemistry.chemical_compound, Animal science, Human fertilization, Cryoprotective Agents, Botany, Glycerol, Animals, Perna canaliculus, General Medicine, biology.organism_classification, Trehalose, Sperm, chemistry, Fertilization, Larva, Oocytes, Female, General Agricultural and Biological Sciences, Ethylene glycol, New Zealand
Abstract

Cryopreservation is a powerful tool for selective breeding in aquaculture as it enables genetic material from selected stock to be stored and crossed at will. The aim of this study was to develop a method for cryopreserving oocytes of the Greenshelltrade mark mussel (Perna canaliculus), New Zealand's main aquaculture species. The ability of oocytes to be fertilized post-thawing was used as the criterion for success in initial experiments and then subsequently, the ability of frozen oocytes to develop further to D-stage larvae was assessed. Ethylene glycol, propylene glycol, dimethyl sulphoxide and glycerol were evaluated at a range of concentrations with and without the addition of 0.2M trehalose using post-thaw fertilization as the endpoint. Ethylene glycol was most effective, particularly when used in combination with trehalose. A more detailed investigation revealed that ethylene glycol at 9% or 10% in the presence of 0.2-0.4M trehalose afforded the best protection. In experiments varying sperm to egg ratio and egg density in post-thaw fertilization procedures, D-larval yield averaged less than 1%. Following these results, a detailed experiment was conducted to determine the damaging steps in the cryopreservation process. Fertilization losses occurred at each step whereas D-larval yield approximately halved following CPA addition and was almost zero following cooling to -10 degrees C. Cryomicroscopy studies and fertilization results suggest that the inability of oocytes to develop to D-larvae stage after cooling to -10 degrees C and beyond are most likely related to some form of chilling injury rather than extracellular ice triggering intracellular ice formation. Further research is needed to determine the causes of this injury and to reduce CPA toxicity and/or osmotic effects.

Published
2008

11. Effect of 2,4-dinitrophenol on the energy metabolism of cattle embryos produced by in vitro fertilization and culture

Author

L.T. McGowan, Jeremy G. Thompson, S.F. Cox, D Rieger, and P.A. Pugh

Subjects
medicine.medical_specialty, Reproductive technology, Oxidative phosphorylation, Fertilization in Vitro, Carbohydrate metabolism, Biology, Tritium, 2,4-Dinitrophenol, chemistry.chemical_compound, Endocrinology, Adenosine Triphosphate, Internal medicine, Culture Techniques, Pyruvic Acid, Genetics, medicine, Animals, Glycolysis, Carbon Radioisotopes, Molecular Biology, Uncoupling Agents, Metabolism, Embryo, Mammalian, Citric acid cycle, Blastocyst, Glucose, Reproductive Medicine, chemistry, Animal Science and Zoology, Cattle, Pyruvic acid, Energy Metabolism, Developmental Biology, Biotechnology
Abstract

In cattle embryos, the proportion of ATP produced by glycolysis increases following the major activation of the embryonic genome, and development to the blastocyst stage is improved in the presence of 10 µM 2,4-dinitrophenol (DNP), an uncoupler of oxidative phosphorylation, from Day 5 to Day 7 of culture. In Experiment 1 of the present study, culture of cattle embryos in the presence of 10 µM DNP from Day 5 to Day 7 stimulated development to the blastocyst stage, but had no significant effects on oxygen, pyruvate or glucose uptake, or on lactate production. In Experiment 2, culture of cattle embryos in the presence of 10 µM DNP from Day 5 to Day 7, stimulated the metabolism of [2-14C]pyruvate (a measure of Krebs cycle activity) on all of Days 5, 6 and 7, and stimulated metabolism of [5-3H]glucose (a measure of glycolysis) on Day 7 only. The results show that 10 µM DNP stimulates oxidative and glycolytic metabolism in Day-5 to Day-7 cattle embryos, but this does not fully explain the observed increase in developmental competence. We propose that partial inhibition or uncoupling of oxidative phosphorylation may reduce the level of intracellular reactive oxygen species production, thereby facilitating development.

Published
2002

12. Effect of sperm number and oxygenation state of the storage media on in vitro fertility of bovine sperm stored at ambient temperature

Author

Jacek Krzyzosiak, L.T. McGowan, R Vishwanath, and Peter C. Molan

Subjects
Male, endocrine system, Time Factors, media_common.quotation_subject, medicine.medical_treatment, Motility, Semen, Fertility, Fertilization in Vitro, Biology, Andrology, Food Animals, medicine, Animals, Blastocyst, Small Animals, Sperm competition, reproductive and urinary physiology, media_common, In vitro fertilisation, Sperm Count, urogenital system, Equine, Temperature, Sperm, Spermatozoa, Oxygen, Female sperm storage, medicine.anatomical_structure, Oocytes, Sperm Motility, Animal Science and Zoology, Cattle, Semen Preservation
Abstract

The effects of storage time and the oxygenation state of the storage medium motility, viability, and in vitro fertility of stored diluted sperm were investigated. Oocytes collected from abattoir material were matured and fertilized in vitro on defined days with sperm stored for up to 11 days in a citrate-based commercial diluent. The proportions of oocytes fertilized and developing to the blastocyst stage were used to assess the quality of the stored semen. In vitro fertility of sperm declined with storage time. There was no significant effect of the oxygenation state of the medium on in vitro fertility of stored sperm. Increased sperm-to-oocyte ratios resulted in a significant elevation of the proportion of oocytes fertilized on day 0 of storage and the proportion of fertilized oocytes developing to the blastocyst stage on days 0 and 3 of storage, suggesting some form of sperm competition or egg selection of sperm based on the ability of sperm to induce normal development.

Published
2001

13. Effect of delayed supplementation of fetal calf serum to culture medium on bovine embryo development in vitro and following transfer

Author

L.T. McGowan, Jeremy G. Thompson, M.G Lambert, N.W. Allen, A.C.S. Bell, and H.R. Tervit

Subjects
Male, animal structures, Plasma Substitutes, Pilot Projects, Fertilization in Vitro, Biology, Andrology, Embryonic and Fetal Development, Random Allocation, Food Animals, Pregnancy, medicine, Animals, Birth Weight, Blastocyst, Bovine serum albumin, Small Animals, Fetus, Equine, Embryogenesis, Embryo, Dextrans, medicine.disease, Embryo Transfer, Fetal Blood, In vitro, Culture Media, medicine.anatomical_structure, Biochemistry, Charcoal, embryonic structures, biology.protein, Oviduct, lipids (amino acids, peptides, and proteins), Animal Science and Zoology, Cattle, Female
Abstract

Supplementation of synthetic oviduct fluid (SOF) medium plus amino acids and bovine serum albumin (BSA) with either fetal calf serum (FCS) or charcoal-treated FCS (CT-FCS) from Day 5 of development was investigated to determine if either in vitro or post-transfer development was altered. Development to the compact morula stage or beyond was similar for all 3 treatments. However, blastocyst development at Day 7 was accelerated when serum was added to the medium (21.6, 40.1 and 39.4% blastocysts from cleaved embryos for BSA, FCS and CT-FCS, respectively; P < 0.01), but cell number of the resulting embryos was unaffected. Furthermore, addition of CT-FCS decreased the between replicate variation in embryo development and produced more Grade 1 and 2 quality embryos (25.8%) than BSA supplementation (18.1%; P < 0.05). The transfer of Grade 1 and 2 embryos at Day 7 following culture resulted in similar pregnancy and embryo survival rates for the 3 treatments, with a tendency for lower embryo survival of embryos cultured in FCS (embryo survival at Day 50 = 37.7% vs 53.3% and 57.6% for FCS, BSA and CT-FCS, respectively; P = 0.1). Significant fetal loss from Day 50 to term occurred within all 3 treatments. There were no birth weight differences for calves amongst the 3 culture treatments; however, one of the sires produced calves that were significantly heavier than expected, suggesting a possible sire-by-embryo interaction. These results demonstrate that addition of FCS may promote blastocyst development; however, there was also a tendency for lower embryo survival. Thus charcoal treatment of FCS is recommended, because it decreases variability in embryo development between runs and results in embryo survival rates to term similar to that BSA-supplemented media.

Published
2000

15. 069 Advances in shellfish germplasm cryopreservation: Current status and future directions

Author

Zoë Hilton, Adam B. Rusk, Serean L. Adams, L.T. McGowan, H. Robin Tervit, David J. Burritt, Andrea C. Alfaro, Samantha L. Gale, and John F. Smith

Subjects
animal structures, Cryoprotectant, biology, fungi, Zoology, General Medicine, Mussel, Pacific oyster, biology.organism_classification, Sperm, General Biochemistry, Genetics and Molecular Biology, Cryopreservation, Panopea zelandica, Botany, General Agricultural and Biological Sciences, Perna canaliculus, Shellfish
Abstract

Cryopreservation can be a powerful tool in shellfish aquaculture for selective breeding programmes and hatchery production. Most species that are commercially farmed are broadcast spawners, releasing sperm and eggs into the environment where they fertilize and develop. However, some species are brooders (e.g. flat oysters (Ostrea chilensis) ), which retain and rear embryos until they reach later developmental stages. Sperm cryopreservation has been successfully achieved for several farmed species including the Pacific oyster ( Crassostrea gigas ), greenshell™ mussel ( Perna canaliculus ) and abalone ( Haliotis iris ). In general, dimethyl sulphoxide and trehalose are the preferred cryoprotectants (CPAs) and simple methods to control cooling rate (e.g. floating rack on liquid nitrogen; methanol/dry ice bath) have worked well for our main species of interest (Pacific oyster, greenshell™ mussel and abalone). Interestingly, sperm perform better in CPAs that are prepared in Milli-Q water as opposed to seawater, indicating that a lower salt concentration during freezing is beneficial. Recent studies with flat oysters and geoducks ( Panopea zelandica ) have also resulted in successful sperm cryopreservation. Shellfish oocyte and larvae cryopreservation has proven more challenging, however, successful cryopreservation of Pacific oyster oocytes has been achieved. Pacific oyster oocytes are able to be fertilized and develop to normal spat post-thawing. However, for other species (e.g. greenshell™ mussel) and for larvae, cryo-injuries are not always immediately apparent post-thawing but manifest during development and are often lethal. greenshell™ mussel oocytes are irretrievably damaged when they reach -6 to -8°C and attempts to overcome this sub-zero chilling injury by vitrification have been unsuccessful. Towards understanding these injuries and their effects, we investigated the effect of cryopreservation on the meiotic spindle of greenshell™ mussel oocytes. Results show that the meiotic spindle undergoes major changes during both CPA addition and cooling. However, the spindle is able to re-form normally in most instances given sufficient time post thawing. For a proportion of oocytes, cryopreservation appears to trigger oocyte activation. The effect of cryopreservation on oxidative stress in greenshell™ mussel oocytes has also been investigated. Although, there are changes in oxidative stress parameters as a result of cryopreservation and strong correlations between fertilization, development and oxidative stress parameters (lipid hydroperoxides, superoxide dismutase, protein carbonyls, total glutathione and glutathione state), preliminary attempts to mitigate oxidative stress using antioxidants have so far failed to enable normal development following cooling, suggesting that oxidative stress may be a secondary rather than primary stress event. Research on shellfish larval cryopreservation utilizing SEM and confocal microscopy has also been carried out for greenshell™ mussel. Later larval stages (D-larvae) appear more resilient to cryopreservation than trochophore larvae, but abnormalities are still apparent (e.g.shell abnormalities and delayed organogenesis). Future studies are aimed toward elucidating mechanisms of injury using new tools such as proteomics and then targeting susceptible cellular processes for protection during cryopreservation. Source of funding: This research was funded by the New Zealand Ministry of Business Innovation and Employment (CAWX0802). Conflict of interest: None declared. serean.adams@cawthron.org.nz

Published
2013
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16. 118. Cryopreservation of Pacific oyster (Crassostrea gigas) trochophore larvae

Author

Samantha L. Gale, Serean L. Adams, Estefania Paredes, H.R. Tervit, L.T. McGowan, and John F. Smith

Subjects
Fishery, Larva, biology, Trochophore, Crassostrea, General Medicine, Pacific oyster, General Agricultural and Biological Sciences, biology.organism_classification, General Biochemistry, Genetics and Molecular Biology, Cryopreservation
Published
2011
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19. 161. Effect of cryoprotectants and chilling on the metaphase I spindle of Greenshell™ mussel Perna canaliculus oocytes

Author

Samantha L. Gale, Steven F. Mullen, Robin H. Tervit, Serean L. Adams, L.T. McGowan, and John F. Smith

Subjects
Andrology, Cryoprotectant, biology, Metaphase i, General Medicine, Mussel, General Agricultural and Biological Sciences, biology.organism_classification, Perna canaliculus, General Biochemistry, Genetics and Molecular Biology
Published
2009
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20. 101. Cryopreservation of Greenshell™ mussel (Perna cancaliculus) sperm and post-thaw improvement using sperm motility stimulants

Author

Stephen C. Webb, Serean L. Adams, Samantha L. Gale, H. Robin Tervit, Rodney D. Roberts, John F. Smith, and L.T. McGowan

Subjects
Andrology, General Medicine, Mussel, Anatomy, Biology, General Agricultural and Biological Sciences, Sperm, General Biochemistry, Genetics and Molecular Biology, Sperm motility, Cryopreservation
Published
2009
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21. 158. Improving cryopreservation of Greenshell mussel Perna canaliculus oocytes to produce higher D-larvae yield

Author

Steven F. Mullen, Samantha L. Gale, Rodney D. Roberts, H. Robin Tervit, L.T. McGowan, Serean L. Adams, and John F. Smith

Subjects
Fishery, Larva, Animal science, Yield (engineering), biology, General Medicine, Mussel, General Agricultural and Biological Sciences, biology.organism_classification, Perna canaliculus, General Biochemistry, Genetics and Molecular Biology, Cryopreservation
Published
2009
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22. Factors affecting the in-vitro development to blastocysts of bovine oocytes matured and fertilized in vitro

Author

H.R. Tervit, Yutaka Fukui, P.A. Pugh, R.W. James, and L.T. McGowan

Subjects
Embryology, Cell Count, Fertilization in Vitro, Biology, Cleavage (embryo), Andrology, Endocrinology, Human fertilization, Oxygen Consumption, medicine, Animals, Fallopian Tubes, Embryogenesis, Obstetrics and Gynecology, Cell Biology, Luteinizing Hormone, Oocyte, In vitro, Culture Media, medicine.anatomical_structure, Blastocyst, Reproductive Medicine, Immunology, Oocytes, Oviduct, Cattle, Female, Follicle Stimulating Hormone, Luteinizing hormone, Hormone
Abstract

The effects of media (TCM199 vs. synthetic oviduct fluid, SOF), sera (foetal calf serum, FCS vs. human serum, HS), gas atmosphere (5% CO2 in air vs. 5% CO2, 5% O2 and 90% N2) and coculture with bovine oviduct epithelial cells (cells vs. no cells) on the in-vitro development of in-vitro matured and fertilized bovine oocytes were examined. Immature oocytes surrounded with compacted cumulus cells were cultured for 24 h in TCM199 supplemented with 10% FCS, 10 micrograms follicle-stimulating hormone (FSH)/ml and 10 micrograms luteinizing hormone (LH)/ml, 1 microgram oestradiol/ml, and 1 x 10(6) granulosa cells at 39 degrees C under 5% CO2 in air. In-vitro fertilization was performed with frozen-thawed, heparin-treated (100 micrograms/ml, 15 min) spermatozoa from 2 bulls. Oocytes were incubated with 2.5 x 10(6) spermatozoa/ml for 24 h and then cultured in one of 16 treatments for 7 days. Cleavage (2-8-cell) and development to blastocysts were recorded on Days 2 and 7, respectively, after the start of culture. SOF was superior to TCM199 for cleavage (P less than 0.01), development to blastocysts (P less than 0.001) and for proportion of cultured ova resulting in blastocysts with at least 60 or at least 100 nuclei (P less than 0.001). FCS was superior to HS for development to blastocysts (P less than 0.001) and 5% oxygen was superior to air for the proportion of ova reaching at least 60 cells (P less than 0.01). For cleavage and development to blastocysts, there was an interaction between serum and cells (P less than 0.01). In the presence of cells, ova preferred FCS, in their absence, serum had little effect.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1991

23. 120. Determination of the cell volume, osmotically inactive volume, and osmotic tolerance limits for Greenshell mussel (Perna canaliculus) oocytes

Author

John F. Smith, Liliana Salinas Flores, S.F. Mullen, H. Robin Tervit, L.T. McGowan, Chongbei Zhao, John K. Critser, and Serean L. Adams

Subjects
Volume (thermodynamics), Cell volume, Botany, General Medicine, Mussel, Biology, General Agricultural and Biological Sciences, biology.organism_classification, Perna canaliculus, General Biochemistry, Genetics and Molecular Biology
Published
2006
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28. Prolongation of the oestrous cycle in cows and ewes after passive immunization with PGF antibodies

Author

R. J. Fairclough, L.T. McGowan, and J. F. Smith

Subjects
endocrine system, Embryology, medicine.medical_specialty, Prostaglandin, Antibodies, chemistry.chemical_compound, Endocrinology, Estrus, Corpus Luteum, Pregnancy, Internal medicine, medicine, Animals, Progesterone, Estrous cycle, Sheep, biology, Prostaglandins F, Immunization, Passive, Albumin, Obstetrics and Gynecology, Cell Biology, medicine.anatomical_structure, Reproductive Medicine, Immunization, chemistry, Ovariectomized rat, biology.protein, Cattle, Female, lipids (amino acids, peptides, and proteins), Arachidonic acid, Antibody, Corpus luteum
Abstract

Summary. Three cows and 2 sheep were passively immunized against prostaglandin (PG) F on Day 16 and Days 13\p=n-\15of the oestrous cycle respectively. The PGF antiplasma was raised in ovariectomized ewes against a PGF-2\g=a\\p=n-\bovineserum albumin complex and showed 100%, 12\m=.\5%,0\m=.\3%

Published
1981
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29. Effect of Exogenous Progestogens on Plasma Concentrations of the Oxytocin-Associated Neurophysin and 13,14-Dihydro-15-keto-prostaglandin F in Intact and Ovariectomized Ewes over the Time of Expected Luteal Regression

Author

L.T. McGowan, J F Smith, R J Fairclough, L G Moore, and Wayne B. Watkins

Subjects
Medroxyprogesterone, medicine.medical_specialty, Luteolysis, Medroxyprogesterone Acetate, Peptide hormone, Luteal phase, Biology, Dinoprost, Estrus, Pregnancy, Internal medicine, Blood plasma, medicine, Animals, Progesterone, Neurophysins, Estrous cycle, Sheep, Ovary, Prostaglandins F, Uterus, Radioimmunoassay, Cell Biology, General Medicine, Endocrinology, Reproductive Medicine, Oxytocin, Ovariectomized rat, Female, hormones, hormone substitutes, and hormone antagonists, medicine.drug
Abstract

Plasma concentrations of the prostaglandin F metabolite 13,14-dihydro-15-keto-prostaglandin F (PGFM), the oxytocin-associated neurophysin (OT-N) and progesterone were monitored by radioimmunoassay (RIA) in five ewes sampled from the jugular vein at hourly intervals between 0700-1900 h from Days 12-16 of the estrous cycle. These hormones were also determined in plasma samples collected at similar times from five intact and five ovariectomized ewes given twice daily injections of medroxyprogesterone acetate (MPA) over Days 10 to 20 after the last observed estrus. In both the control and intact MPA-treated ewes, coincident surges of OT-N and PGFM were observed in jugular plasma during the time of luteal regression. No significant differences were noted in the number and amplitude of OT-N and number of PGFM peaks between the control and intact MPA-treated animals, although in the latter the amplitude of the PGFM peaks was significantly reduced (P less than 0.01). No marked surges in the plasma concentrations of PGFM or OT-N were observed in the ovariectomized ewes given exogenous MPA. This latter finding is consistent with previous proposals, suggesting that the ovaries are a major source of oxytocin in the ewe. In addition, the observation that exogenous progestogens in the intact ewes did not influence the number and peak height of the OT-N surges, indicates that a fall in progesterone levels during the normal cycle is not obligatory for oxytocin release although it may facilitate the release of uterine PGF2 alpha.

Published
1983
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30. Temporal relationship between plasma concentrations of 13,14-dihydro-15-keto-prostaglandin F and neurophysin I/II around luteolysis in sheep

Author

J. F. Smith, W.B. Watkins, H.R. Tervit, L.T. McGowan, L G Moore, A. J. Peterson, and R. J. Fairclough

Subjects
medicine.medical_specialty, Time Factors, Neurophysin I, Luteolysis, Uterus, Luteal phase, Dinoprost, Oxytocin, Biochemistry, Endocrinology, Estrus, Pregnancy, Internal medicine, medicine, Animals, Progesterone, Estrous cycle, Neurophysins, Sheep, Chemistry, Prostaglandins F, Radioimmunoassay, medicine.anatomical_structure, Hypothalamus, Female, medicine.drug
Abstract

Plasma concentrations of neurophysin I/II (N-I/II), 13,14-dihydro-15-keto-prostaglandin F (PGFM) and progesterone were measured by radioimmunoassay in plasma samples collected from four sheep at hourly intervals between 0700 and 1900 h from Days 12–17 of the estrous cycle. Plasma samples were also collected from a fifth sheep at 2-hourly intervals during Days 12–16 of the cycle. In all sheep, intermittent surges in the plasma concentrations of PGFM and N-I/II occurred during the period of luteal regression. On at least one occasion in each sheep a surge in the plasma concentration of N-I/II was observed coincident with a rise in PGFM concentrations. In general, the highest levels of N-I/II were observed early in luteolysis (Days 13–14 of the cycle) while the corresponding levels of PGFM in plasma were maximal around Day 15 when luteolysis was well advanced. It is suggested from this temporal data that oxytocin, which is considered to be released in association with N-I/II, may play an important role in ovine luteolysis by stimulating the secretion of prostaglandin F from the uterus during Days 13–15 of the estrous cycle.

Published
1980

31. Effect of inhibitors and uncouplers of oxidative phosphorylation during compaction and blastulation of bovine embryos cultured in vitro

Author

L.T. McGowan, Bianca Gasparrini, H.R. Tervit, C McNaughton, Jeremy G. Thompson, Thompson, J. G., Mcnaughton, C., Gasparrini, Bianca, Mcgowan, L. T., and Tervit, H. R.

Subjects
Embryology, Glucose uptake, Obstetrics and Gynecology, Embryo, Antimycin A, Oxidative phosphorylation, Metabolism, Cell Biology, Mitochondrion, Biology, Blastula, Andrology, chemistry.chemical_compound, Dose–response relationship, Endocrinology, chemistry, Biochemistry, Reproductive Medicine
Abstract

The effect of inhibiting ATP production via oxidative phosphorylation during pericompaction of in vitro produced bovine embryos was investigated. This was achieved by: (i) varying the atmospheric O2 concentration (0, 1, 2, 4 and 7%); (ii) addition of oxidative phosphorylation inhibitors, NaN3 and antimycin A; and (iii) addition of 2,4-dinitrophenol, an uncoupler of oxidative phosphorylation from electron transport. The development of embryos under various O2 concentrations from day 5 to day 7 of development indicated that an optimal concentration occurred at about 2%. Addition of NaN3 revealed that doses above 100 mumol l-1 were toxic to embryo development, but that concentrations of 5-10 mumol l-1 stimulated embryo development by 10-25%. A similar result was observed after addition of 2,4-dinitrophenol, whereas antimycin A was inhibitory at doses as low as 1 mumol l-1. At concentrations of NaN3 or 2,4-dinitrophenol that stimulated embryo development, the number of cells of the resulting blastocysts was also significantly increased. Addition of NaN3 from day 1 of development inhibited subsequent development. Metabolic data of NaN3-treated embryos revealed that O2 uptake was significantly lower at inhibitory doses (100 mumol l-1). A significant (P < 0.05) log linear increase in glucose uptake was measured between the three concentrations of NaN3 (0, 10 and 100 mumol l-1). These results demonstrate that ATP production via oxidative phosphorylation is essential for bovine embryo development in vitro. However, transient (subacute) inhibition appears to be beneficial to embryo development and the number of cells, perhaps by creating a more favourable intracellular environment.

32. Proceedings: Effect of oestradiol-17beta, progesterone and prostaglandin F-2alpha antiplasma on luteal function in the ewe

Author

J. F. Smith, L.T. McGowan, R. J. Fairclough, and A. J. Peterson

Subjects
Embryology, medicine.medical_specialty, Sheep, Estradiol, Prostaglandins F, Obstetrics and Gynecology, Cell Biology, Biology, Luteal phase, Endocrinology, Reproductive Medicine, Corpus Luteum, Internal medicine, medicine, Animals, Female, Progesterone, Function (biology), Prostaglandin f
Published
1976
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