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Please use this identifier to cite or link to this item: http://hdl.handle.net/1893/9934
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dc.contributor.authorAdam, Musa Men_UK
dc.contributor.authorRana, Kausiken_UK
dc.contributor.authorMcAndrew, Brendanen_UK
dc.date.accessioned2017-01-17T23:25:14Z-
dc.date.available2017-01-17T23:25:14Zen_UK
dc.date.issued1995-02en_UK
dc.identifier.urihttp://hdl.handle.net/1893/9934-
dc.description.abstractCryoprotectants, which are essential for minimizing cryoinjury during freezing, can be toxic to biological systems. Monohydric alcohols, dimethyl sulfoxide (Me2SO), and ethylene glycol (EG), are known to denature enzymes at room temperature. In this study, rosy barb (Puntius conchonius) and zebra fish (Brachydanio rerio) embryos at cleavage, epiboly, and closure of blastopore stages were exposed to Me2SO and EG at 1.0, 2.0, 3.0, and 4.0 M for 0.25. 0.5, 1.0, 2.0, and 3.0 at room temperature. The cryoprotectants were then removed and the activities of two glycolytic enzymes, lactate dehydrogenase (LDH) and glucose-6-phosphate dehydrogenase (G-6-PDH), were determined. Cryoprotectant concentration and equilibration period had a significant (P < 0.05) effect on the total activity of the two enzymes. In both species the decline in enzymatic activity was more pronounced for G-6-PDH, and EG was more toxic than Me2SO. Zebra fish embryos were more resistant to cryoprotectant enzymatic denaturation than rosy barb embryos. For both species the total LDH activity measured after 3.0 h equilibration in 4.0 M Me2SO and EG declifted sharply. In zebra fish cleavage, epiboly, and closure of blastopore embryos, the total LDH activity (or control value) when Me2SO and EG were used was reduced by 70.0 and 86.1, 79.2 and 83.0, and 57 and 75% for the three embryonic stages, respectively. Under similar conditions G-6-PDH activity was reduced by 100 and 100, 88.3 and 100, and 69.0 and 100%, respectively, for the same embryonic stages. Similarly for rosy barb embryos, the total LDH activity was reduced by 89.2 and 98.8, 85.0 and 87.1, and 80.6 and 95.4% when equilibrated in Me2SO and EG. In embryos at the closure of blastopore stage. G-6-PDH activity was reduced by 71.2% when equilibrated in 4 M Me2SO. The reduction in the total activity of these enzymes was probably due to the damage to the perivitelline membrane and blastoderm caused by the osmotic stress and partial denaturation of the leached enzymes within the perivitelline space.en_UK
dc.language.isoenen_UK
dc.publisherElsevieren_UK
dc.relationAdam MM, Rana K & McAndrew B (1995) Effect of cryoprotectants on activity of selected enzymes in fish embryos. Cryobiology, 32 (1), pp. 92-104. https://doi.org/10.1006/cryo.1995.1008en_UK
dc.rightsThe publisher does not allow this work to be made publicly available in this Repository. Please use the Request a Copy feature at the foot of the Repository record to request a copy directly from the author. You can only request a copy if you wish to use this work for your own research or private study.en_UK
dc.rights.urihttp://www.rioxx.net/licenses/under-embargo-all-rights-reserveden_UK
dc.subjectAquacultureen_UK
dc.subjectFishes Eggs Identificationen_UK
dc.subjectAquacultureen_UK
dc.titleEffect of cryoprotectants on activity of selected enzymes in fish embryosen_UK
dc.typeJournal Articleen_UK
dc.rights.embargodate2999-12-29en_UK
dc.rights.embargoreason[AdamEtal_Cryobiology_1995.pdf] The publisher does not allow this work to be made publicly available in this Repository therefore there is an embargo on the full text of the work.en_UK
dc.identifier.doi10.1006/cryo.1995.1008en_UK
dc.citation.jtitleCryobiologyen_UK
dc.citation.issn0011-2240en_UK
dc.citation.volume32en_UK
dc.citation.issue1en_UK
dc.citation.spage92en_UK
dc.citation.epage104en_UK
dc.citation.publicationstatusPublisheden_UK
dc.citation.peerreviewedRefereeden_UK
dc.type.statusVoR - Version of Recorden_UK
dc.author.emailb.j.mcandrew@stir.ac.uken_UK
dc.contributor.affiliationUniversity of Stirlingen_UK
dc.contributor.affiliationInstitute of Aquacultureen_UK
dc.contributor.affiliationInstitute of Aquacultureen_UK
dc.identifier.isiWOS:A1995QF43900008en_UK
dc.identifier.scopusid2-s2.0-0002829648en_UK
dc.identifier.wtid760058en_UK
dc.contributor.orcid0000-0001-7384-5133en_UK
dcterms.dateAccepted1995-02-28en_UK
dc.date.filedepositdate2012-11-09en_UK
rioxxterms.typeJournal Article/Reviewen_UK
rioxxterms.versionVoRen_UK
local.rioxx.authorAdam, Musa M|en_UK
local.rioxx.authorRana, Kausik|en_UK
local.rioxx.authorMcAndrew, Brendan|0000-0001-7384-5133en_UK
local.rioxx.projectInternal Project|University of Stirling|https://isni.org/isni/0000000122484331en_UK
local.rioxx.freetoreaddate2999-12-29en_UK
local.rioxx.licencehttp://www.rioxx.net/licenses/under-embargo-all-rights-reserved||en_UK
local.rioxx.filenameAdamEtal_Cryobiology_1995.pdfen_UK
local.rioxx.filecount1en_UK
local.rioxx.source0011-2240en_UK
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