Two Advanced Cryogenic Procedures for Improving Stevia rebaudiana (Bertoni) Cryopreservation

Benelli̇, C.; Carvalho, Lara Siqueira Oliveira; Merzougui, Soumaya El; Petruccelli, R.

doi:10.3390/plants10020277

Cited by 10 publications

(5 citation statements)

References 48 publications

(52 reference statements)

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“…In the case of the present study, shoot tip regrowth rates were higher and plantlet regeneration and growth was faster than when the vitrification procedure was used [17]. The droplet-vitrification been developed for many other plant species [7,8,12,13,14,15,16,21,22,23,24,25,26,27]. It is a practical, user-friendly technique and is now routinely applied for the cryopreservation of shoot tips of a wide range of plant species and genotypes and could be an alternative for implementing long-term storage of germplasm.…”

Section: Resultsmentioning

confidence: 98%

“…In other studies, it was reported that the best exposure times to PVS2 were 60 min for Stevia. [8], 20 min. for Rosa hybrida L. [14], 60 min for Malus domestica Borkh.…”

Section: Resultsmentioning

confidence: 99%

“…Therefore, one of the key factors in the design of a cryopreservation protocol is to select and optimize a dehydration strategy for the explants prior to freezing them in liquid nitrogen, to avoid the formation of ice crystals inside the cells and tissues Treatment of explants with vitrification solutions containing combinations of different cryoprotectants, such as DMSO (dimethyl sulfoxide), ethylene glycol, glycerol, and sucrose, added in specific concentrations has become a common strategy in the design of cryopreservation protocols. nt solutions must be used with caution since they might have a toxic effect or cause osmotic stress to cells of some plant species, compromising viability of the cells in the explant, resulting in cell death, especially if immersion in them occurs at temperatures above 0 °C or for prolonged periods of time [8,31]. Toxic effects can be prevented by selecting adequate cryoprotectants, adjusting the concentration of cryoprotectants in the solution, and the temperature and duration of the The aim of this study to develop a cryopreservation procedure based on the vitrification technique for shoot tips of (Spreng.)…”

Section: Discussionmentioning

confidence: 99%

“…is a cryopreservation technique that has been successfully applied to many plant species [7,8]. This technique consists of dripping vitrification solution containing one single explant on aluminum foil strips, which are immersed quickly in liquid nitrogen (LN) -196°C.…”

Section: Droplet-vitrificationmentioning

confidence: 99%

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Comparative Study of Three Vitrification Solutions for an Effective Droplet-vitrification Cryopreservation Procedure for Pfaffia Glomerata (Spreng.) Pedersen

Oliveira¹,

Salomão

Martins³

et al. 2021

EJMP

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Aims: The objective of this research was to establish a cryopreservation protocol for shoot tips (ST) of in vitro P. glomerata using the droplet-vitrification technique. Study Design: The experimental design was a factorial, with four factors, arranged in a completely randomized design. Three vitrification solutions (PVS2, PVS3, PVS4), three times (20, 40, 60 min) and two temperatures (25 ± 2 °C and 0 °C) of treatment with the solutions, followed by freezing (LN+) or not (LN-) with liquid nitrogen (LN) were tested. All tests were performed using six replicates and the results analysed using Two-way ANOVA and Tukey’s tests and expressed as the mean ± the standard error of the means (SEM) deviation. Place and Duration of Study: Laboratory of Plant Cryobiology, Embrapa Genetic Resources and Biotechnology, over a two-year period. Methodology: ST excised from in vitro plantlets were pre-cultured overnight (19h), treated with a loading solution (LS) and three different vitrification solutions (PVS2, PVS3, PVS4) prior to freezing in LN. Treatment with the vitrification solutions was carried out at 0 or 25°C, for 20, 40 or 60 min. For freezing, drops of the vitrification solutions containing a single ST were dispensed on aluminum foil strips and the strips were submerged in LN (-196°C). For thawing, foil strips were submerged into unloading solution (US) at 40 ± 2°C, for three min. Thawed ST were transferred to regeneration medium and cultured in vitro. Results: Highest regeneration percentages after cryopreservation were 82% for ST treated with PVS3, at 0°C, for 60 min; 32% for ST treated with PVS4 at 25°C for 60 min or 0°C for 40 min and 22% for those treated with PVS2 at 0°C for 60 min. Conclusion: Droplet-vitrification is a suitable technique to ensure survival of P. glomerata ST after cryopreservation. This procedure can be applied to establish germplasm collections of this medicinal species in gene banks.

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Section: Resultsmentioning

confidence: 98%

“…In other studies, it was reported that the best exposure times to PVS2 were 60 min for Stevia. [8], 20 min. for Rosa hybrida L. [14], 60 min for Malus domestica Borkh.…”

Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Droplet-vitrificationmentioning

confidence: 99%

See 2 more Smart Citations

Comparative Study of Three Vitrification Solutions for an Effective Droplet-vitrification Cryopreservation Procedure for Pfaffia Glomerata (Spreng.) Pedersen

Oliveira¹,

Salomão

Martins³

et al. 2021

EJMP

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“…The temperature during the incubation of plants in PVSs is important for both toxicity and dehydration. The temperature close to 0 • C for plants treated in PVS2 is crucial and had significantly lower lethality than at 22 • C [65,[141][142][143]. When the temperature is subsequently lowered, the penetrating components of PVS2 cryoprotect the cells by restricting the molecular mobility of water molecules and preventing them from nucleating ice crystals [11].…”

Section: Vitrification Solution and Cryopreservation Methodsmentioning

confidence: 99%

Vitrification Solutions for Plant Cryopreservation: Modification and Properties

Zámečnı́k

Faltus

Bilavčík

2021

Plants

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Many plants cannot vitrify themselves because they lack glassy state-inducing substances and/or have high water content. Therefore, cryoprotectants are used to induce vitrification. A cryoprotectant must have at least the following primary abilities: high glass-forming property, dehydration strength on a colligative basis to dehydrate plant cells to induce the vitrification state, and must not be toxic for plants. This review introduces the compounds used for vitrification solutions (VSs), their properties indicating a modification of different plant vitrification solutions, their modifications in the compounds, and/or their concentration. An experimental comparison is listed based on the survival or regeneration rate of one particular species after using more than three different VSs or their modifications. A brief overview of various cryopreservation methods using the Plant Vitrification Solution (PVS) is also included. This review can help in alert researchers to newly introduced PVSs for plant vitrification cryoprotocols, their properties, and the choice of their modifications in the compounds and/or their concentration.

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