Current status of the cryopreservation of embryogenic material of woody species

Daniel Ballesteros; María Teresa Martínez; Carolina Sánchez-Romero; Itziar Aurora Montalbán; Ester Sales; Paloma Moncaleán; Isabel Arrillaga; Elena Corredoira

doi:10.3389/fpls.2023.1337152

Current status of the cryopreservation of embryogenic material of woody species

Front Plant Sci. 2024 Jan 17:14:1337152. doi: 10.3389/fpls.2023.1337152. eCollection 2023.

Authors

Daniel Ballesteros^{1

2}, María Teresa Martínez³, Carolina Sánchez-Romero⁴, Itziar Aurora Montalbán⁵, Ester Sales⁶, Paloma Moncaleán⁵, Isabel Arrillaga⁷, Elena Corredoira³

Affiliations

¹ Departamento de Botánica y Geología, Facultad de Farmacia, Universitat de València, Burjassot, Valencia, Spain.
² Royal Botanic Gardens, Kew, Wakehurst Place, Haywards Heath, United Kingdom.
³ Misión Biológica de Galicia (MBG-CSIC), Sede Santiago de Compostela, Santiago de Compostela, Spain.
⁴ Dpto. de Botánica y Fisiología Vegetal, Universidad de Málaga, Málaga, Spain.
⁵ Depto. Ciencias Forestales, Neiker-BRTA, Vitoria, Spain.
⁶ Dpto. Ciencias Agrarias y del Medio natural, Instituto Universitario de Investigación en Ciencias Ambientales (IUCA), Universidad de Zaragoza, Escuela Politécnica Superior, Huesca, Spain.
⁷ Institut Biotec/Med, Dpto Biología Vegetal, Facultad de Farmacia, Universitat de València, Burjassot, Valencia, Spain.

Abstract

Cryopreservation, or the storage at liquid nitrogen temperatures (-196°C), of embryogenic cells or somatic embryos allows their long-term conservation without loss of their embryogenic capacity. During the last decade, protocols for cryopreservation of embryogenic material of woody species have been increasing in number and importance. However, despite the large experimental evidence proved in thousands of embryogenic lines, the application for the large-scale conservation of embryogenic material in cryobanks is still limited. Cryopreservation facilitates the management of embryogenic lines, reducing costs and time spent on their maintenance, thus limiting the risk of the appearance of somaclonal variation or contamination. Somatic embryogenesis in combination with cryopreservation is especially useful to preserve the juvenility of lines while the corresponding clones are being field-tested. Hence, when tree performance has been evaluated, selected varieties can be propagated from the cryostock. The traditional method of slow cooling or techniques based on vitrification are mostly applied procedures. For example, slow cooling methods are widely applied to conserve embryogenic lines of conifers. Desiccation based procedures, although simpler, have been applied in a smaller number of species. Genetic stability of the cryopreserved material is supported by multiloci PCR-derived markers in most of the assayed species, whereas DNA methylation status assays showed that cryopreservation might induce some changes that were also observed after prolonged subculture of the embryogenic lines. This article reviews the cryopreservation of embryogenic cultures in conifers, fruit species, deciduous forest species and palms, including a description of the different cryopreservation procedures and the analysis of their genetic stability after storage in liquid nitrogen.

Keywords: conifers; deciduous forest species; fruit species; genetic stability; liquid nitrogen; slow cooling; somatic embryos; vitrification.

Publication types

Review

Grants and funding

The author(s) declare financial support was received for the research, authorship, and/or publication of this article. This review was partly funded by the MICINN (Spain) through the projects PID2020-112627RB-C31, PID2020-112627RB-C32 and PID2020-112627RB-C33 and the COST Action CA21157 “European Network for Innovative Woody Plant Cloning”, www.copytree.eu, supported by COST (European Cooperation in Science and Technology) www.cost.eu.