Expression vector changing distribution of rice storage protein as well as preparation and use thereof
An expression vector and storage protein technology, which is applied in the field of expression vectors for changing the distribution of rice storage proteins, and can solve problems such as reducing and changing the expression sites of rice storage proteins.
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Embodiment 1
[0048] This embodiment is to illustrate the method for constructing a rice glutenin gene expression vector that contains a resistance marker gene and is guided by a waxy gene promoter and the structure of the obtained vector. The construction process is as follows:
[0049] a) In pCAMBIA1301 (referred to as p1301, from researcher Wang Zongyang, Shanghai Institute of Plant Physiology and Ecology, Chinese Academy of Sciences) plasmid vector (see figure 2 Shown) PCR primers were designed at both ends of the NOS terminator, and HindIII restriction sites were introduced upstream and downstream; the PCR product was connected to the T vector to obtain the T-1 vector, and transformed into Escherichia coli competent cells; then HindIII was used for T- 1 The plasmid was digested, and the small fragment was recovered by electrophoresis, and the small fragment was connected with the pCAMBIA1301 plasmid HindIII digestion product to obtain the pCAMBIA1301-NOS vector (abbreviated as p1301-NO...
Embodiment 2
[0057] This embodiment is to illustrate the method for constructing a vector that does not contain a resistance marker gene and is guided by a waxy gene promoter and the structure of the obtained vector. The construction process is as follows:
[0058] According to the same method of embodiment 1, from the publication number is that CN129802IA patent specification is searched for 232 indica type rice waxy gene promoter nucleotide sequence, with reference to this sequence, design upstream primer at about 2.6kb place before translation initiation point ATG, in primer A KpnI restriction site was introduced at one end; using the same method as in Example 1, a downstream primer was designed at the 3' UTR behind the Gt1 gene coding region, and an XhoI restriction site was introduced at one end; a pair of new primers designed as above were used for the embodiment 1 The constructed p1301-Wx-Gt1 was subjected to PCR amplification reaction to obtain the DNA sequence of the rice glutelin ...
Embodiment 3
[0060] This example is to illustrate the method for constructing a glycinin gene expression vector that does not contain a resistance marker gene and is guided by a waxy gene promoter and the structure of the obtained vector. The construction process is as follows:
[0061] a) Extract total RNA from the cotyledon of soybean (Glycine max) at the mid-mature stage, use a reverse transcription kit to obtain the first strand of cDNA, and then design a pair of specific PCR primers according to the glycinin Gy7 mRNA sequence published by Genbank AF319777, the upstream primer No enzyme cleavage site is introduced, the downstream primer introduces XhoI site and adds protective bases, using a high-fidelity DNA polymerase that does not contain A at the end of the PCR product, and using the first strand of cDNA as a template, PCR amplification obtains glycinin The cDNA sequence after the signal peptide of Gy7 gene;
[0062] b) According to the same method as in Example 1, search for the n...
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