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A novel regeneration system for a wild passion fruit species (<Emphasis Type="Italic">Passiflora cincinnata</Emphasis> Mast.) based on somatic embryogenesis from mature zygotic embryos
Authors:Maurecilne Lemes da Silva  Daniela Lopes Paim Pinto  Miguel Pedro Guerra  Eny Iochevet Segal Floh  Cláudio Horst Bruckner  Wagner Campos Otoni
Institution:1.Biological Sciences Department, Botany Department,Mato Grosso State University (UNEMAT),Tangará da Serra,Brazil;2.Plant Tissue Culture Laboratory, Plant Biology Department/BIOAGRO,Federal University of Vi?osa,Vi?osa,Brazil;3.Plant Science Department, Developmental Physiology and Plant Genetics Laboratory,Federal University of Santa Catarina,Florianópolis,Brazil;4.Plant Cell Biology Laboratory (BIOCEL), Institute of Biological Sciences, Botany Department,University of S?o Paulo (USP),S?o Paulo,Brazil;5.Plant Science Department,Federal University of Vi?osa,Vi?osa,Brazil
Abstract:The objective of the present work was to induce somatic embryogenesis from zygotic embryos of Passiflora cincinnata Masters. Zygotic embryos formed calli on media with different concentrations of 2,4-dichlorophenoxyacetic acid (2,4-D) and 4.5 μM benzyladenine (BA) after 30 days of in vitro culture. A concentration of 18.1 μM 2,4-D resulted in the largest number of somatic embryos. Embryogenic calli were yellowish and friable, forming whitish proembryogenic masses. Morphologically, embryogenic cells were small and had large nuclei and dense cytoplasm, whereas non-embryogenic cells were elongated, with small nuclei and less dense cytoplasm. Calli cultured under white light on basal Murashige and Skoog’s medium with activated charcoal produced embryos in all developmental stages. There were differences among the treatments, with some leading to the production of calli with embryos and some only to callus formation. Some abnormalities were associated with somatic embryos, including fused axes, fused cotyledons and polycotyledonary embryos. Production of secondary somatic embryos occurred in the first cycle of primary embryo development. Secondary embryos differentiated from the surface of the protodermal layer of primary embryos with intense cell proliferation, successive mitotic divisions in the initial phase of embryoid development, and a vascular system formed with no connection to the parental tissue. This secondary embryogenic system of P. cincinnata is characterized by intense proliferation and maintenance of embryogenic competence after successive subcultures. This reproducible protocol opens new prospects for massive propagation and is an alternative to the current organogenesis-based transformation protocol.
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