Molecular marker for paddy recessive genic male sterility gene cyp704b2 and application thereof
A molecular marker, nuclear male technology, applied in the field of plant biology, can solve problems such as unfavorable large-scale and batch breeding practice, and achieve the effect of improving the efficiency of trait selection, accurate results and strong specificity
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Embodiment 1
[0034] Example 1 Primer Design and Amplified Fragment Analysis of the Rice Recessive Genic Sterile Gene cyp704b2
[0035] 1. Primer design
[0036] Referring to the difference between wild-type CYP704B2 and mutant cyp704b2 gene sequences, a three-primer combination capable of distinguishing recessive nuclear male sterility phenotype and normal fertility phenotype was designed:
[0037] M1907-F 1 : TGTCGGGTTTGGGGTTGAGATAGGG (SEQ ID NO. 1), M1907-F 2 : GGGTTTGGGGTTGAGATCTAAGCT (SEQ ID NO. 2), and M1907-R: AGCGTGACGATGATGTTGGCAGC (SEQ ID NO. 3) (see figure 1 ).
[0038] 2. Analysis of amplified fragments
[0039] Using the above primer combination to amplify the rice recessive male sterility gene cyp704b2, only a 90bp band can be amplified in the sterile material, and a 96bp band can be amplified in the fertile material, or a 96bp and a 96bp band can be amplified at the same time 90bp band. The nucleotide sequences of the 90bp and 96bp bands are shown in SEQ ID NO.4 and SEQ...
Embodiment 2
[0040] Example 2 Identifying the cyp704b2 genotype of rice varieties / lines with molecular markers of the present invention
[0041] 1. Experimental materials
[0042] 1907, Wufeng B, Huazhan, Zhongxiang Huangzhan, R51084, Qingfeng No. 1 B, South H197, Fufenghui 1658, S-127, 9311, Yue 4B, H28B
[0043] 2. Extraction of rice genomic DNA
[0044] Using the CTAB method to extract rice genomic DNA, the specific steps are as follows: take 3 cm long rice leaves at the seedling stage, and extract them in 800 μL of extraction buffer [1.5% (w / v) CTAB, 1.05mol / L NaCl, 75mmol / L Tris-HCl (pH 8.0), 15mmol / L EDTA (pH 8.0)] and collected in a 1.5mL centrifuge tube. Water bath at 65°C for 30 minutes, and mix by inverting occasionally. Add 800 μL of chloroform:isoamyl alcohol (volume ratio 24:1), and mix by inverting for 15 minutes. Centrifuge at 12000r / min for 10min at room temperature. Aspirate 450 μL of the supernatant, transfer to a new 1.5 mL centrifuge tube, add 2 times the volume of...
Embodiment 3
[0051] Embodiment 3 carries out assisted selection breeding with molecular marker of the present invention
[0052] 1. Experimental materials
[0053] 1907 Homozygous / 1907 Heterozygous Hybrid F 1 Generation 18 single plants, 1907 / 9311 hybrid F 2 Generation segregation population 12 individual plants.
[0054] 2. Extraction of rice genomic DNA
[0055] See Example 2.
[0056] 3. PCR amplification and detection
[0057] Participate in Example 2.
[0058] 4. Results and analysis
[0059] Using the molecular marker of Example 1 of the present invention (specific primer combination M1907-F 1 , M1907-F 2 and M1907-R obtained by PCR amplification) detect the cyp704b2 genotype of 30 individual plants in the present embodiment at the seedling stage, the results are shown in image 3 . 1907 Homozygous / 1907 Heterozygous Hybrid F 1 Of the 18 individual plants in the generation, 6 individual plants only amplified 90bp bands, and 12 individual plants simultaneously amplified 90bp...
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