Cryopreservation of potato cultivated varieties and wild species: critical factors in droplet vitrification

The applicability of cryopreservation protocols to a broad range of genotypes is a key issue for genebanks. We tried to identify the critical factors causing differences in survival of cryopreserved shoot tips using potato varieties coming from cultivated and wild species. The droplet-vitrification...

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Veröffentlicht in:	Cryo-Letters 2006-07, Vol.27 (4), p.223-234
Hauptverfasser:	Kim, Haeng-Hoon, Yoon, Ju-Won, Park, Young-Eun, Cho, Eun-Gi, Sohn, Jae-Keun, Kim, Tae-San, Engelmann, Florent
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Sprache:	eng
Schlagworte:	Cell Survival - drug effects Cell Survival - physiology Conservation of Natural Resources Cryopreservation - methods Cryoprotective Agents - pharmacology Culture Media - pharmacology Culture Techniques - methods Dose-Response Relationship, Drug DROPLET-VITRIFICATION Genotype Glycerol - pharmacology Plant Shoots - cytology Plant Shoots - drug effects Plant Shoots - physiology Pvs2/pvs3 Loading Shoot Tips Solanum - cytology Solanum - genetics Solanum - physiology Solanum Tuberosum L Sucrose - pharmacology Temperature Time Factors
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creator	Kim, Haeng-Hoon Yoon, Ju-Won Park, Young-Eun Cho, Eun-Gi Sohn, Jae-Keun Kim, Tae-San Engelmann, Florent
description	The applicability of cryopreservation protocols to a broad range of genotypes is a key issue for genebanks. We tried to identify the critical factors causing differences in survival of cryopreserved shoot tips using potato varieties coming from cultivated and wild species. The droplet-vitrification method, a combination of droplet-freezing and solution-based vitrification, was selected from several protocols. High survival after freezing was observed after dehydration with PVS2 for 20 min, cooling shoot tips placed in a droplet of PVS2 solution on aluminum foil strips by immersing the foil strips in liquid nitrogen, warming them by plunging the foil strips into a 0.8 M sucrose solution (at 40°C) for 30 s and unloading in 0.8 M sucrose for 30 min. This optimized protocol was successfully applied to 12 accessions with survival ranging between 64.0 and 94.4%.
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We tried to identify the critical factors causing differences in survival of cryopreserved shoot tips using potato varieties coming from cultivated and wild species. The droplet-vitrification method, a combination of droplet-freezing and solution-based vitrification, was selected from several protocols. High survival after freezing was observed after dehydration with PVS2 for 20 min, cooling shoot tips placed in a droplet of PVS2 solution on aluminum foil strips by immersing the foil strips in liquid nitrogen, warming them by plunging the foil strips into a 0.8 M sucrose solution (at 40°C) for 30 s and unloading in 0.8 M sucrose for 30 min. This optimized protocol was successfully applied to 12 accessions with survival ranging between 64.0 and 94.4%.</abstract><cop>England</cop><pub>Cryoletters</pub><pmid>16990950</pmid><tpages>12</tpages></addata></record>
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source	MEDLINE; Ingenta Connect; EZB-FREE-00999 freely available EZB journals
subjects	Cell Survival - drug effects Cell Survival - physiology Conservation of Natural Resources Cryopreservation - methods Cryoprotective Agents - pharmacology Culture Media - pharmacology Culture Techniques - methods Dose-Response Relationship, Drug DROPLET-VITRIFICATION Genotype Glycerol - pharmacology Plant Shoots - cytology Plant Shoots - drug effects Plant Shoots - physiology Pvs2/pvs3 Loading Shoot Tips Solanum - cytology Solanum - genetics Solanum - physiology Solanum Tuberosum L Sucrose - pharmacology Temperature Time Factors
title	Cryopreservation of potato cultivated varieties and wild species: critical factors in droplet vitrification
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