Method for obtaining Brassica oleracea var. acephala DC. small spore regenerated plants and special culture medium
A technology for regenerating plants and rooting medium, applied in botany equipment and methods, plant regeneration, horticultural methods, etc., can solve the problems of low efficiency, difficult to capture recessive traits, and long time, and achieve broad application prospects and adaptability wide, high embryonic rate
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Embodiment 1
[0028] Embodiment 1, the cultivation of kale microspore regeneration plant
[0029] The donor mother plants of ornamental kale (Brassica oleracea var. acephala) were grown in plastic greenhouses with insect-proof nets. The genotypes covered various types of ornamental kale, and the leaf types included whole round leaves, wavy leaves, crepe leaves, lobed leaves and deeply lobed leaves, etc., the leaf colors include white, light yellow, pink, bright red, purple red, etc., a total of 15 materials, in the first ten days of March to June (Note: During the entire collection season, remove in time Bloom and pod branch and weak branch, guarantee the exuberant growth of new inflorescence) collect microspore and carry out in vitro culture with the method of the present invention, concrete process comprises the following steps:
[0030] 1) Free microspore culture
[0031] DAPI fluorescent staining by nucleus (Colemen A W, Goff L J. Application offluorochrome to pollen biology I. Mithram...
Embodiment 2
[0039] Embodiment 2, the cultivation of kale microspore regeneration plant
[0040] The donor mother plants of ornamental kale (Brassica oleracea var. acephala) were grown in plastic greenhouses with insect-proof nets. The genotypes covered various types of ornamental kale, and the leaf types included whole round leaves, wavy Leaves, crepe leaves, lobed leaves and deeply lobed leaves, etc., leaf color includes white, pink, scarlet, purple red and light yellow, etc., a total of 16 parts of materials, collected microspores in the first ten days of March to June and carried out in vitro with the method of the present invention Cultivation, the specific process includes the following steps:
[0041] 1) Free microspore culture
[0042] Through the DAPI fluorescent staining of the nucleus, microscopic examination, determine the development period of the microspore, get the flower bud containing 80% mononuclear marginal stage microspore cell and 20% binucleate stage cell, the flower...
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