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Establishment of in vitro shoot tips regeneration system of foxtail millet and obtainment of transgenic plants of SiSERK1

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Abstract Foxtail millet (Setaria italica) would be suitable as a model plant of C4 plants given its small genome (about 490 MB) and diploid self-pollination. However, the study of foxtail millet faces the problem of low efficiency of explant regeneration and genetic transformation. In this study, a new genetic transformation system of Yugu1 foxtail millet was established with in vitro shoot tips as the explant, and, the concentrations of 6-BA and kanamycin were optimized. Thus, 0.5 mg•L-1 6-BA and 25 mg•L-1 kanamycin were the most suitable in terms of the differentiation rate of shoot tips and survival rate of differentiated seedlings. In addition, 12 transgenic foxtail millets of SiSERK1 were identified by resistance screening and PCR and identified the insertion site of one of the transgenic plants. The results of qRT-PCR showed that the expression of SiSERK1 gene in plants transformed was significantly higher than that in wild-type plants. A new method of generation of material for further study of SiSERKs is provided for foxtail millet genetics and breeding.
Title: Establishment of in vitro shoot tips regeneration system of foxtail millet and obtainment of transgenic plants of SiSERK1
Description:
Abstract Foxtail millet (Setaria italica) would be suitable as a model plant of C4 plants given its small genome (about 490 MB) and diploid self-pollination.
However, the study of foxtail millet faces the problem of low efficiency of explant regeneration and genetic transformation.
In this study, a new genetic transformation system of Yugu1 foxtail millet was established with in vitro shoot tips as the explant, and, the concentrations of 6-BA and kanamycin were optimized.
Thus, 0.
5 mg•L-1 6-BA and 25 mg•L-1 kanamycin were the most suitable in terms of the differentiation rate of shoot tips and survival rate of differentiated seedlings.
In addition, 12 transgenic foxtail millets of SiSERK1 were identified by resistance screening and PCR and identified the insertion site of one of the transgenic plants.
The results of qRT-PCR showed that the expression of SiSERK1 gene in plants transformed was significantly higher than that in wild-type plants.
A new method of generation of material for further study of SiSERKs is provided for foxtail millet genetics and breeding.

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