Plant constitutive promoter osubipro and its application
A constitutive promoter and promoter technology, applied in the field of agricultural biology, can solve problems such as transgene silencing
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Embodiment 1
[0056] The acquisition of embodiment 1 promoter OsUbipro
[0057] The bioinformatic analysis of the upstream sequence of OsUbi gene (SEQ ID NO.1) about 1756bp sequence (SEQ ID NO.1) by the promoter function prediction software PlantCARE and PlantPAN found that the sequence is rich in various promoter-related cis-acting elements such as CAAT-box , TATA-box, etc., indicated that the sequence of SEQ ID NO.1 has the structural characteristics of a plant cell promoter. And by PlantPAN analysis, its 375-1256bp sequence is rich in CpG islands, and CpG islands are also one of the sequence characteristics of eukaryotic promoters, so it is speculated that this sequence should have promoter activity, and its core sequence is 375-1256bp region .
[0058] The upstream sequences of the OsUbi gene of different lengths were intercepted to identify the promoter activity. After continuous screening and comparison, the sequence shown in SEQ ID NO.1 was finally determined as the promoter sequenc...
Embodiment 2
[0062] Expression analysis of embodiment 2 promoter OsUbipro
[0063] Using qPCR (fluorescent quantitative PCR) to identify the expression pattern of OsUbipro downstream genes, the specific method is as follows:
[0064] The roots, leaves, young panicles, seedlings and calluses of ZH11 were taken respectively, total RNA was extracted, and cDNA was obtained by reverse transcription. In the Thermo PikoReal96 real-time fluorescent quantitative PCR system, the expression of the OsUbi gene downstream of OsUbipro was detected using the Actin gene as an internal reference.
[0065] RT-PCR primer sequences:
[0066] OsUbi-qRtF2: GGCCGCACCTTGGCTGACTA (SEQ ID NO. 6)
[0067] OsUbi-qRtR2: GATCTGCATCCCACCCCTGA (SEQ ID NO. 7)
[0068] Actin-F: AGCATGAAGATCAAGGTGGTC (SEQ ID NO. 8)
[0069] Actin-R: GCCTTGGCAATCCACATC (SEQ ID NO. 9)
[0070] Fluorescent quantitative PCR reaction system and procedures are as follows:
[0071] Program: pre-denaturation at 94°C for 7 minutes, denaturation...
Embodiment 3
[0076] Embodiment 3 constructs the plant transgenic expression cassette and vector containing promoter OsUbipro
[0077] 1. Preparation of plant transgenic expression cassette containing promoter OsUbipro
[0078] The construction method of the plant transgenic expression cassette OsUbip-ALSm-OsUbiT (sequence such as SEQ ID NO.4) of the present invention is as follows:
[0079] Primers 0310-UAU-F / 0310-UAU-Rv1 were designed to amplify the promoter OsUbip fragment from the rice genome; The target gene ALSm1 fragment was amplified; the terminator OsUbiT fragment was amplified from the rice genome using primers 0310-UAU-F3 / 0310-UAU-Rv. Among them, the 5' ends of primers 0310-UAU-F and 0310-UAU-Rv have about 15 nucleotide sequences repeated with the corresponding connection positions of the vector; the 5' ends of the upstream and downstream primers of adjacent fragments also have 15 bp repeats (0310- UAU-Rv1 and 0310-UAU-F2, 0310-UAU-Rv2 and 0310-UAU-F3) for subsequent recombinat...
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