OPTIMIZATION OF DROPLET VITRIFICATION PROTOCOL FOR CRYOPRESERVATION OF IN VITRO GROWN BLACKBERRY SHOOT TIPS

The study focused on an economically-important ornamental outdoor shrub, Nandina domestica, with the aims to (i) optimize an effective in vitro conservation method, and (ii) develop a cryopreservation protocol for shoot tips by the PVS2 vitrification and droplet-vitrification techniques. For in vitro conservation of shoot cultures, the tested parameters were sucrose content in the storage medium (30, 45, 60 g/L) and storage temperature (4 Â°C or 8 Â°C). Cryopreservation was performed by applying the PVS2 vitrification solution, in 2-ml cryovials or in drops over aluminum foil strips, for 15, 30, 60 or 90 min at 0 Â°C, followed by the direct immersion in liquid nitrogen of shoot tips. Results show that N. domestica shoots can be conserved successfully for 6 months at both the temperatures tested, especially when 60 g/L sucrose is used in the storage medium. However, conservation at 4 Â°C showed to be more appropriate, as hyperhydricity was observed in post-conservation of shoots coming from storage at 8 Â°C. As for cryopreservation, a daily gradual increase of sucrose concentration (from 0.25 to 1.0 M) produced better protection to the samples that were stored in liquid nitrogen. Indeed, with this sucrose treatment method, a 30-min PVS2 incubation time was enough to produce, 60 days after thawing, the best recovery (47% and 50%) of shoot tips, cryopreserved with PVS2 vitrification and droplet-vitrification, respectively.

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A COMPARISON OF VITRIFICATION AND DROPLET VITRIFICATION PROCEDURES FOR THE CRYOPRESERVATION OF IN VITRO GROWN BLACK CHOKEBERRY SHOOT TIPS

Acta Horticulturae ◽

10.17660/actahortic.2011.908.43 ◽

2011 ◽

pp. 325-330 ◽

Cited By ~ 5

Author(s):

D. Tanaka ◽

A. Nishiuchi ◽

T. Niino ◽

T. Matsumoto

Keyword(s):

Shoot Tips ◽

Droplet Vitrification ◽

Black Chokeberry

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Cryopreservation of 12 Vitis Species Using Apical Shoot Tips Derived from Plants Grown In Vitro

HortScience ◽

10.21273/hortsci13958-19 ◽

2019 ◽

Vol 54 (6) ◽

pp. 976-981 ◽

Cited By ~ 4

Author(s):

Jean Carlos Bettoni ◽

Aike Anneliese Kretzschmar ◽

Remi Bonnart ◽

Ashley Shepherd ◽

Gayle M. Volk

Keyword(s):

Cost Effective ◽

Shoot Tips ◽

Easy Access ◽

Biotic And Abiotic Stresses ◽

Breeding Programs ◽

Vitis Species ◽

Droplet Vitrification ◽

Effective Manner ◽

Ideal Method

The availability of and easy access to diverse Vitis species are prerequisites for advances in breeding programs. Plant genebanks usually maintain collections of Vitis taxa as field collections that are vulnerable to biotic and abiotic stresses. Cryopreservation has been considered an ideal method of preserving these collections as safety back-ups in a cost-effective manner. We report a droplet vitrification method used to cryopreserve 12 Vitis species (Vitis vinifera cvs. Chardonnay and ‘Riesling, V. actinifolia, V. aestivalis, V. jacquemontii, V. flexuosa, V. palmata, V. riparia, V. rupestris, V. sylvestris, V. ficifolia, V. treleasi, and V. ×novae angeliae) using shoot tips excised from plants grown in vitro. Our results demonstrated wide applicability of this technique, with regrowth levels at least 43% for 13 genotypes representing 12 Vitis species. We demonstrated that the droplet vitrification procedure can be successfully replicated by technical staff, thus suggesting that this method is ready for implementation.

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Cryopreservation of cherry rootstock Gisela 5 (Prunus cerasus × Prunus canescens) shoot tips by droplet-vitrification technique

Journal of Horticultural Research ◽

10.2478/johr-2013-0025 ◽

2013 ◽

Vol 21 (2) ◽

pp. 79-85 ◽

Cited By ~ 4

Author(s):

Djurdjina Ružić ◽

Tatjana Vujović ◽

Radosav Cerović

Keyword(s):

Liquid Medium ◽

Room Temperature ◽

Sucrose Concentration ◽

Shoot Multiplication ◽

Shoot Tips ◽

Prunus Cerasus ◽

Droplet Vitrification ◽

Vitrification Solution ◽

Gisela 5

ABSTRACT The droplet-vitrification technique was applied to in vitro shoot tips of cherry rootstock Gisela 5 (Prunus cerasus × Prunus canescens). Explants were precultured in the dark at 23 °C, in liquid MS medium with a progressively increasing sucrose concentration (0.3 M for 15 h, then 0.7 M for 5 h). Loading involved a 30 min incubation of explants in a solution comprising 1.9 M glycerol and 0.5 M sucrose. Explants were dehydrated at room temperature using a solution PVS A3 [Murashige and Skoog (MS) liquid medium, 22.5% (w/v) sucrose, 37.5% (w/v) glycerol, 15% (w/v) ethylene glycol and 15% (w/v) dimethylsulfoxide] for 30, 40 and 50 min and the PVS3 solution [MS liquid medium, 50% (w/v) sucrose, 50% (w/v) glycerol] for 60, 90 and 120 min. Explants were cooled by direct immersion in liquid nitrogen (LN) in 10 μl droplets of vitrification solution placed on aluminum foil strips. The foil strips were retrieved from LN and immersed in preheated (37 °C) unloading solution (0.8 M sucrose) for 30 s, and an equal volume of unloading solution at room temperature was added for further incubation for 30 min. Shoot tips were transferred onto the regrowth medium, cultivated in the dark for 7 days before being incubated under standard conditions. Three weeks after transferring the shoot tips onto the regrowth medium, the survival rate of control and cryopreserved explants of Gisela 5 dehydrated with PVS A3 was 100%, regardless of the treatment duration. After dehydration with solution PVS3, the survival varied between 70 and 100% for control explants and 78 and 95% for cryopreserved shoot tips. Gisela 5 shoot tips dehydrated for 40 min with PVS A3 vitrification solution demonstrated the best regrowth (38%). When using the PVS3 solution, survival of cryopreserved shoot tips was the highest (95%) after 60 min treatment followed by 40% regrowth. After three successive subcultures on shoot multiplication, medium shoots recovered viability, multiplication ability and morphology equal of that prior to cryopreservation.

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Cryopreservation of Grapevine Shoot Tips from In Vitro Plants Using Droplet Vitrification and V Cryo-plate Techniques

Synthetic Seeds ◽

10.1007/978-3-030-24631-0_22 ◽

2019 ◽

pp. 469-482

Author(s):

Jean Carlos Bettoni ◽

Ranjith Pathirana ◽

Remi Bonnart ◽

Ashley Shepherd ◽

Gayle Volk

Keyword(s):

Shoot Tips ◽

Droplet Vitrification ◽

In Vitro Plants

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Effect of the Duration of Liquid Nitrogen Storage on the Regrowth of Blackberry Cryopreserved by Droplet Vitrification

Contemporary Agriculture ◽

10.1515/contagri-2017-0008 ◽

2017 ◽

Vol 66 (1-2) ◽

pp. 44-50

Author(s):

Tatjana Vujović ◽

Đurđina Ružić ◽

Radosav Cerović

Keyword(s):

Liquid Nitrogen ◽

Room Temperature ◽

Shoot Tips ◽

Lower Survival Rate ◽

Droplet Vitrification ◽

Vitrification Solution ◽

Long Term Preservation ◽

Direct Immersion

SummaryIn vitro shoot tips of the blackberry cultivar ‘Čačanska Bestrna’ were cryopreserved using the droplet vitrification technique. Upon loading (30 min) in a solution of 1.9 M glycerol and 0.5 M sucrose, the explants were dehydrated for 40 min on ice with the PVS A3 vitrification solution (glycerol 37.5%, dimethyl sulfoxide 15%, ethylene glycol 15% and sucrose 22.5%) and for 40 min at room temperature with the PVS3 solution (glycerol 50% and sucrose 50%). They were subsequently frozen in individual microdroplets of vitrification solution, by direct immersion in liquid nitrogen (LN), and kept therein for 2, 4, 8 and 24 h. The explant rewarming was performed in an unloading solution (0.8 M sucrose) for 30 min at room temperature. The duration of LN exposure did not exert significant effects on the survival and regrowth of explants in both types of vitrification solutions. The survival and regrowth of cryopreserved shoot tips dehydrated with PVS3 solution ranged between 90–95% and 80–90%, respectively. However, dehydration with PVS A3 resulted in a lower survival rate (80–90%) and a considerably lower regrowth rate (55–65%) of explants. Monitoring the shoots regenerated in the in vitro culture revealed their normal capacity for multiplication and rooting in comparison with the controls, which fully confirms the purpose of cryopreservation in the long-term preservation of plant material.

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A modified droplet vitrification method for cryopreservation of shoot tips from in vitro potato plants

Vavilov Journal of Genetics and Breeding ◽

10.18699/vj19.505 ◽

2019 ◽

Vol 23 (4) ◽

pp. 422-429 ◽

Cited By ~ 2

Author(s):

T. A. Gavrilenko ◽

N. A. Shvachko ◽

N. N. Volkova ◽

Yu. V. Ukhatova

Keyword(s):

Plant Genetic Resources ◽

Original Method ◽

Shoot Tips ◽

Droplet Vitrification ◽

Modified Method ◽

Long Term Storage ◽

Common Potato ◽

The Impact

Collections of common potato maintained in the field genebanks suffer significant losses due to the impact of extreme environmental factors, diseases and pests. The solution of the problem of safe long-term preservation of common potato accessions is to create doublet in vitro and cryo-collections. Cryogenic collections are stored at ultra-low temperatures in cryobanks. Several methods of potato cryoconservation are known, of which the droplet vitrification method developed by B. Panis with colleagues in 2005 is the most widely used in genebanks. This paper provides a detailed description of the modified method of droplet vitrification, which is used for cryopreservation of apexes (shoot tips) of potato in vitro plants at the N.I. Vavilov All-Russian Institute of Plant Genetic Resources (VIR). The method modified at VIR includes the main steps of the original droplet-vitrification method developed by B. Panis and colleagues: 1) preparation of plant material, 2) isolation of shoot tips, 3) treatment of explants with cryoprotector solutions, 4) freezing/immersion in liquid nitrogen, 5) thawing, 6) post-cryogenic recovery and evaluation of viability and regeneration capacity. The modifications of stages 1, 2 and 6 proposed at VIR lead to a significant reduction in the duration of cryopreservation experiments in comparison with the original method of B. Panis. This paper presents the results of cryopreservation of modern potato cultivars and South American landraces which were obtained using the method of droplet vitrification as modified at VIR. The majority (76.7 %) of the studied accessions of cultivated potato were characterized by high rates of postcryogenic recovery (40–95 %) and 23.3 % of the samples had the values of postcryogenic regeneration from 20 to 39 %, which corresponds to the minimal permissible values for long-term storage in a cryobank. Currently the modified droplet-vitrification method is used for further expanding of the VIR potato cryocollection.

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Cryopreservation in vitro of apple shoot tips following droplet-vitrification

Acta Horticulturae ◽

10.17660/actahortic.2020.1289.1 ◽

2020 ◽

pp. 1-8

Author(s):

T. Vujović ◽

Đ. Ružić ◽

D. Vranić ◽

T. Marjanović

Keyword(s):

Shoot Tips ◽

Droplet Vitrification ◽

Apple Shoot

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Integration of Cryopreservation and Tissue Culture for Germplasm Conservation and Propagation of Rosa pomifera ‘Karpatia’

Notulae Botanicae Horti Agrobotanici Cluj-Napoca ◽

10.15835/nbha45110566 ◽

2017 ◽

Vol 45 (1) ◽

pp. 208-214 ◽

Cited By ~ 1

Author(s):

Ewelina KWAŚNIEWSKA ◽

Ewa DZIEDZIC ◽

Bożena PAWŁOWSKA

Keyword(s):

Treatment Time ◽

Germplasm Conservation ◽

Shoot Multiplication ◽

Shoot Tips ◽

Ms Medium ◽

Droplet Vitrification ◽

Multiplication Cycle ◽

New Research

Cryopreservation is an useful technique for long-term conservation that requires minimal space and maintenance. Germplasm protection of Rosa is important to preserve genetic diversity, to store material for breeding and to expand new research. This study was conducted to develop a droplet vitrification cryopreservation and micropropagation of Rosa pomifera cv. ‘Karpatia’, whose large hypanthia are characterized by remarkable pro-health properties. Culture in vitro was stabilized and shoot tips collected from dormant buds served as initial explants. The multiplication of shoots was carried out on MS medium containing benzyladenine. For the droplet vitrification cryopreservation, shoot tips from in vitro cultures were used: small with exposed meristem, and large with a meristem covered with leaves, as well as shoot tips from in situ plants, which were collected in winter. Treatment time with plant vitrification solution (PVS2) was also tested (10-30 minutes). From in vitro culture, 32-41% small explants with exposed meristem survived, but they regenerated at a very low level. The best cryostorage results were obtained for shoot tips from dormant buds and a 20-minute PVS2 treatment: the survival was 84% and regeneration 72%. During the post-freezing regeneration multiplication index was 2.4 shoots per one multiplication cycle, after cryopreservation and in the control. On half MS medium without growth regulators, 97-99% of shoots rooted, and all rooted plants have adapted to ex vitro conditions and were planted into the soil. Biometric analyses during shoot multiplication, rooting and acclimatization stages did not reveal any changes compared to the non-cryopreserved samples.

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Investigation of the post-cryogenic regeneration ability of potato varieties under different cultivation conditions

Vavilov Journal of Genetics and Breeding ◽

10.18699/vj19.500 ◽

2019 ◽

Vol 23 (3) ◽

pp. 281-286 ◽

Cited By ~ 1

Author(s):

E. S. Bespalova ◽

Yu. V. Ukhatova ◽

N. N. Volkova ◽

E. V. Oves ◽

N. A. Gaitova ◽

...

Keyword(s):

Shoot Tips ◽

Axillary Buds ◽

Regeneration Ability ◽

Cultivation Conditions ◽

Regeneration Rate ◽

Dark Incubation ◽

Potato Varieties ◽

Droplet Vitrification ◽

In Vitro Plants

Cryopreservation provides long-term storage of the gene pool of potato varieties in cryobanks at extremely low temperatures. Currently, droplet vitrification is the most widely used method for cryopreservation of potato varieties, which is constantly improving to increase the regeneration rates of the stored plant material. Different modifications of this method are used in the world’s leading potato genebanks. This paper presents the results of studying the effect of cultivation conditions after plunging into liquid nitrogen and thawing of shoots tips and axillary buds of in vitro plants on their postcryogenic recovery. The droplet-vitrification method modified at VIR was used for cryopreservation. The factor “prolonged dark incubation of explants” did not have a significant effect on the frequency of post-cryogenic regeneration of the studied varieties except for one variety (Krepysh), for which a significant increase in the regeneration rate was observed for the shoot tips cultivated in the darkness compared to the cultivation under the photoperiod 16/8 hours (light/darkness). The frequency of post-cryogenic regeneration of shoot tips was higher than that of the axillary buds for all varieties; however, these differences were significant (p < 0.05) only in two cases: for the variety Udacha (a photoperiod of 16/8 hours) and for the variety Krepysh (the dark incubation). The results of two-factor analysis of variance indicate that there is no effect of interaction of factor 1 (prolonged dark incubation) and factor 2 (explant type) on the ability of varieties to post-cryogenic recovery. Taking into account the obtained results, the further cryopreservation of an extended subset of 9 varieties was carried out using shoot tips, which, after freezing-thawing, were cultivated under the photoperiod of 16/8 hours. The frequency of post-cryogenic regeneration of these varieties varied from 30 to 60 %. A significant effect of genotype on postcryogenic recovery has been established. The ability of varieties to regenerate shoots after freezing and thawing was not related to the values of morphogenic indices of in vitro plants. The age of the meriklons (2–4 years) did not significantly affect either the morphogenic indices or the frequency of post-cryogenic regeneration.

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