Seedling Development and Evaluation of Genetic Stability of Cryopreserved Dendrobium Hybrid Mature Seeds

Galdiano, Renato Fernandes; Lemos, Eliana Gertrudes de Macedo; Faria, Ricardo Tadeu de; Vendrame, Wagner A.

doi:10.1007/s12010-013-0699-8

Cited by 18 publications

(6 citation statements)

References 20 publications

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“…By determining the best dehydration time of explants at 0 °C, the toxicity of the vitrification solution can be reduced and, consequently, the exposure time to PVS2 solution can be increased for a successful cryopreservation protocol (Johari et al 2009, Vendrame et al 2008. Vendrame et al (2008) showed that pre-cooling treatment (ice) combined with PVS2 treatment for a period of time between 1 and 3 h was essential to allow proper germination of cryopreserved seeds of four commercial Dendrobium hybrids genotypes (Galdiano et al 2014). Likewise, in this study, the dehydration period was similar and 1 h in PVS2 can be recommended.…”

Section: IImentioning

confidence: 64%

Cryopreservation of banana’s cv Grand Naine in vitro rhizomes

Londe

Vendrame

Sanaei

et al. 2017

An. Acad. Bras. Ciênc.

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The preservation of banana genetic material is usually performed through seedlings. However, most banana cultivars do not produce seed and are propagated vegetatively. Therefore, cryopreservation is a feasible technique that allows the preservation of banana genotypes indefinitely. For the success of cryopreservation protocols, the selection of cryoprotectants and pre-freezing techniques are important factor. Therefore, the objective of this study was to verify the effects of different cryoprotectants with and without 1% phloroglucinol and pre-cooling periods on the development of a protocol for cryopreservation of in vitro rhizomes of Musa accuminata (AAA) cv Grand Naine banana. The addition of 1% phloroglucinol to the cryoprotective solutions, such as PVS2 enhanced recovery of cryopreserved banana rhizomes. In addition, pre-cooling of explants in ice for 3 hours in PVS2 + 1% of phloroglucinol allowed efficient cryopreservation of banana rhizomes, followed by successful recovery and regeneration of in vitro shoots of banana cv Grand Naine.

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Section: IImentioning

confidence: 64%

Cryopreservation of banana’s cv Grand Naine in vitro rhizomes

Londe

Vendrame

Sanaei

et al. 2017

An. Acad. Bras. Ciênc.

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“…For example, mature seeds of Oncidium flexuosum (11% WC) and a Dendrobium hybrid (13% WC) were unable to germinate or exhibited a low germination percentage after direct immersion in LN [28,29]. The seeds of these species should be cryopreserved through a vitrification method combined with rapid cooling and rewarming [28][29][30].…”

Section: Vitrification Methodsmentioning

confidence: 99%

Cryopreservation of Orchid Genetic Resources by Desiccation: A Case Study of Bletilla formosana

RungYi¹,

Chang²,

Hsieh³

et al. 2016

Cryopreservation in Eukaryotes

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Many native orchid populations declined yearly due to economic development and climate change. This resulted in some wild orchids being threatened. In order to maintain the orchid genetic resources, development of proper methods for the long-term preservation is urgent. Low temperature or dry storage methods for the preservation of orchid genetic resources have been implemented but are not effective in maintaining high viability of certain orchids for long periods. Cryopreservation is one of the most acceptable methods for long-term conservation of plant germplasm. Orchid seeds and pollens are ideal materials for long-term preservation (seed banking) in liquid nitrogen (LN) as the seeds and pollens are minute, enabling the storage of many hundreds of thousands of seeds or pollens in a small vial, and as most species germinate readily, making the technique very economical. This article describes cryopreservation of orchid genetic resources by desiccation and a case study of Bletilla formosana. We hope to provide a more practical potential cryopreservation method for future research needs.

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“…Freshly collected mature seeds were cleaned and dried over LiCl for 2 weeks and stored at 4 °C until used for the study (approximately 1 year). Lithium chloride-mediated drying is a commonly used method (Galdiano et al 2014 ). A pinch of seeds (ranging from 300 to 2000 seeds depending on the species) were transferred to hardened filter paper (Whatman, UK) and stapled.…”

Section: Plant Speciesmentioning

confidence: 99%

“…Seed and protocorm cryopreservation utilises a range of different available methods including: direct freezing, encapsulation-vitrification and droplet-freezing, each tested in several taxa (Sakai and Engelmann 2007 ; Sopalun et al 2010 ; Jitsopakul et al 2012 ; Hu et al 2013 ; Galdiano et al 2014 ; Teixeira da Silva et al 2014 ; Popova et al 2016 ). However, protocorms, a widely used propagule for cryopreservation, are prone to cryopreservation injury due to their cellular structure and high-water content.…”

Section: Introductionmentioning

confidence: 99%

Cryopreservation without vitrification suitable for large scale cryopreservation of orchid seeds

2018

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BackgroundOrchids are under threat from human activities and climate change, with populations limited to small geographic hotspots. This makes them ideal candidates for ex situ conservation. Orchid seeds are desiccation tolerant, but often have poor longevity in seed banks and cryopreservation of orchid protocorms is complex and expensive. Therefore, simple methods for large-scale storage programs are essential to store orchid seeds of different life forms. Seeds of five species representing epiphytic, lithophytic and terrestrial orchids from the Central Highlands of Madagascar were studied to find a simple and effective system of cryopreservation. The use of a vitrification solution prior to cryopreservation to improve survival was investigated, as well as the use of symbiotic and asymbiotic germination media to maximise germination after cryopreservation. Using the filter paper packet method, dried seeds were stored in vapour phase above liquid nitrogen and recovered after thawing with both symbiotic and asymbiotic media.ResultsThe study revealed that cryoprotection is not essential for the species in this study, which represented a range of lifeforms. Vitrification generally led to a decrease in germination post cryopreservation. The use of a symbiotic germination medium post cryopreservation was found to be successful in the species in which it was tested. However, the use of an asymbiotic medium was successful for all the species in this study.ConclusionsVitrification was not essential for the species in this study as the orchid seeds were already ultralow temperature and desiccation tolerant. However, further studies using more species are required to validate this approach. This may be an ecophysiological or genetic trait of these species. Therefore, this form of dry seed cryopreservation could form part of ex situ orchid seed conservation using a standard method. The methods developed here will store greater genetic diversity compared to what can be achieved with protocorms and are suitable for both asymbiotic and symbiotic recovery after cryopreservation. This will help reduce the time and cost of ex situ conservation, and help develop universal protocols for large genera, compared to custom protocols required for protocorm cryopreservation.Electronic supplementary materialThe online version of this article (10.1186/s40529-018-0229-7) contains supplementary material, which is available to authorized users.

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Seedling Development and Evaluation of Genetic Stability of Cryopreserved Dendrobium Hybrid Mature Seeds

Cited by 18 publications

References 20 publications

Cryopreservation of banana’s cv Grand Naine in vitro rhizomes

Cryopreservation of banana’s cv Grand Naine in vitro rhizomes

Cryopreservation of Orchid Genetic Resources by Desiccation: A Case Study of Bletilla formosana

Cryopreservation without vitrification suitable for large scale cryopreservation of orchid seeds

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