CN113373166B - Application of tobacco NtAAP3 gene in tobacco - Google Patents
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Abstract
The invention belongs to the technical field of gene function analysis of tobacco genomes, and particularly relates to tobaccoNtAAP3The gene is applied to tobacco. TobaccoNtAAP3In connection with amino acid transport, after the amino acid transport is silenced, the tyrosine content, the proline content and the asparagine content in tobacco are obviously reduced, and the total protein content is obviously reduced; in another aspect, tobaccoNtAAP3The gene is related to the regulation of the content of pigment substances in the tobacco, and the content of the pigment substances such as chlorophyll a/b, total chlorophyll, carotenoid and the like in the tobacco leaves is obviously increased after the gene is silenced. The application is rightNtAAP3The relationship between gene and amino acid regulation, protein content regulation and pigment content regulation is primarily determined, and the explanation is providedNtAAP3The gene lays a theoretical foundation for the functions of amino acid absorption, transport, nitrogen utilization, plant stress resistance regulation and control and the like.
Description
Technical Field
The invention belongs to the technical field of gene function analysis of tobacco genomes, and particularly relates to tobaccoNtAAP3The gene is applied to tobacco.
Background
Amino acids, which are basic constituent units of enzymes and proteins, not only are carriers of organic nitrogen and precursors of important secondary metabolites in plants, but also play an important role in the growth and development of plants. Plants can assimilate inorganic nitrogen present in the form of ammonium salts and nitrates from the soil through the roots to produce amino acids, or can assimilate amino acids directly from the soil, or can autonomously synthesize amino acids in the leaves. The absorption and transport of amino acids in plants depends on amino acid transporters, which are located on biological membranes and are classified according to sequence homology and function as: APC super family (Amino acid, polyamine and Choline transporters super family) and ATF super family (Amino acid transporter family); the ATF superfamily is divided into 6 subfamilies, namely AAPs (amino acid catalysts), LHTs (lysine histone transporters), ProTs (proline transporters), gamma-GATs (gamma-aminobutyric transporters), ANTs (aromatic and neutral amino acid transporters) and AUX (antibiotic-resistant family), wherein the subfamilies of AAPs (amino acid catalysts) are relatively deeply studied.
Amino Acid Permeases (AAPs) were first discovered and isolated in Arabidopsis thalianaAAPs8 members of the Gene family: (AtAAP1~8) Mainly responsible for the transport of acidic and neutral amino acids, among themAtAAP1The gene is highly expressed in endosperm and cotyledon, is closely related to the transportation of glutamate and neutral amino acid at root, and can also influence the weight and quantity of plant seeds;AtAAP2andAtAAP3the expression level of the gene in the phloem of the stem and the root is higher, and the gene is responsible for the transportation of phloem amino acid;AtAAP5the gene is highly expressed mainly in the root cortex, and mediates the transportation of arginine and lysine;AtAAP6the gene has high expression level at the root and is responsible for adjusting the components and the content of amino acid in the sieve tube molecules;AtAAP8the gene regulates the transport of amino acids into endosperm at the early stage of seed development.
For crops, the research on AAPs has been mainly focused on rice, but there are reports on crops such as corn and potato. Rice (Oryza sativa L.) with improved resistance to stressAAPsUp to 19 members of a gene family, whereinOsAAP3The gene is related to the transport of lysine and arginine, and the inhibition of the gene expression can increase the spike number and tiller number of riceThereby improving the utilization rate of the nitrogen of the rice and increasing the yield;OsAAP6the gene participates in regulating and controlling the nutrition quality and protein content of rice. Pan et al discovered corn by yeast function complementation experimentZmAAP4The gene can regulate and control the transport of various amino acids, and particularly has strong affinity to glutamic acid and proline. Koch et al discovered potatoes by RNAi techniqueStAAP1The gene plays an important role in the transport of amino acids from leaves to rhizomes.
In the prior art, against tobaccoNtAAPThe family gene research shows that the tobacco amino acid permeaseNtAAP2Gene (tobacco amino acid permease)NtAAP2Gene and application thereof, CN 201711351625.2) has important influence on the regulation of the content of part types of amino acids in tobacco leaves. However, whether other genes in the family have similar functions in tobacco needs to be further researched to be further determined.
Disclosure of Invention
In the tobaccoNtAAP2On the basis of preliminary gene research, to further define the content of tobaccoNtAAPFamily of other genes, the present application aims to further define the tobaccoNtAAP3、NtAAP6The gene function, thereby laying a certain technical foundation for analyzing the genome function of the tobacco and cultivating new varieties of the tobacco.
The technical scheme adopted by the application is detailed as follows.
TobaccoNtAAP3Application of gene in tobacco, tobaccoNtAAP3In connection with amino acid transport, after the amino acid transport is silenced, the tyrosine content, the proline content and the asparagine content in tobacco are obviously reduced, and the total protein content is obviously reduced;
in another aspect, tobaccoNtAAP3The gene is related to the regulation of the content of pigment substances in the tobacco, and after the gene is silenced, the content of pigment substances such as chlorophyll a/b, total chlorophyll, carotenoid and the like in the tobacco leaves is obviously increased;
said tobaccoNtAAP3The specific CDS sequence of the gene is shown as SEQ ID No.1, and the corresponding edited amino acid sequence of the tobacco NtAAP3 protein is shown as SEQ ID No.2, or specifically as follows:
NtAAP3gene CDS sequence (1440 bp):
ATGGGAGAAAACAACAACGTTGCTTCAAAACACCAAGTGTTCGATGTTTCCATTAATGTGACTGAATCCAAGTGCTTTGACGATGATGGCCGTCTCAAAAGAACCGGGAGCGTTTGGACGGCAAGTGCTCATATCATAACAGCTGTGATTGGTTCGGGAGTTTTGTCTTTAGCATGGGCAGTAGCTCAACTTGGTTGGATTGCTGGTCCTATTGTTATGATTTTGTTCTCTTTTGTTACTTATTACACTTCCGCTCTTCTTGCCGATTGTTACCGCTCCGGCGACTCTGTTTCCGGCAAGAGAAACTATACTTACATGGATGCTGTCCAAGCCAATCTTGGTGGGCTCCAAGTCAAGATTTGTGGATGGATTCAGTATGCGAATCTTTTTGGAGTTGCTATCGGATACACCATTGCATCTTCAATTAGCATGATAGCTATTAAAAGGTCTAATTGTTTCCACAAACATGGTGATCAAGCTCCTTGTCAAGTATCCAGCACTCCATACATGATCATGTTTGGAATAATAGAAATCATCTTCTCCCAAATTCCAGATTTTGATCAGATTTGGTGGCTTTCAATTGTGGCTGCCGTTATGTCTTTCACTTACTCTACTATTGGACTAGGATTAGGAGTTGCTAAAGTGGCAGAAACTGGAAAAATCGGAGGAAGTCTCACTGGAATTAGCATCGGAACTGTGACTGAAATGCAAAAGATTTGGAAAAGCTTCCAAGCCCTTGGAGCTATCGCTTTTGCCTATTCTTACTCTCTCATCCTTATTGAGATTCAGGATACACTCAAATCTCCACCGTCAGAATCCAAGACAATGAAAAATGCAACTCTAATTAGTGTAGCAGTAACAACAGTTTTCTACATGCTCTGTGGCTGCTTTGGCTATGCAGCATTTGGAGATCTTGCTCCTGGAAACTTACTAACTGGTTTTGGATTCTACAATCCTTATTGGCTACTCGATATAGCGAACATAGCCATTGTCGTCCACCTTGTTGGTGCATACCAGGTTTACTGCCAGCCCCTTTTCGCCTTCATTGAAAAAACAGCAGCAGAATGGTACCCCGAGAGTAAATTCATTGCCAAAGAGATTAGTGTCCCGATTATAGGCTATAAATCCTTTAAACTCAACCTTTTCCGCATAATTTGGAGGACTATTTTCGTCATCATCACCACGGTCATATCTATGCTATTGCCATTCTTCAATGACATAGTTGGAATTCTTGGAGCCTTTGGGTTTTGGCCGCTAACAGTCTATTTCCCGGTGGAAATGTACATTGTGCAAAAGAAGATAACAAAATGGAGCACAAAATGGATTTGCCTTCAAATGCTTAGTGTTGCTTGCCTTATTATCTCAATTGCTGCAGCTGCTGGTTCTTTTGCTGGCGTTGTATCTGATCTACAAGTTTACAAGCCTTTTAAGACGACTTGA;
NtAAP3 protein sequence (479 AA):
MGENNNVASKHQVFDVSINVTESKCFDDDGRLKRTGSVWTASAHIITAVIGSGVLSLAWAVAQLGWIAGPIVMILFSFVTYYTSALLADCYRSGDSVSGKRNYTYMDAVQANLGGLQVKICGWIQYANLFGVAIGYTIASSISMIAIKRSNCFHKHGDQAPCQVSSTPYMIMFGIIEIIFSQIPDFDQIWWLSIVAAVMSFTYSTIGLGLGVAKVAETGKIGGSLTGISIGTVTEMQKIWKSFQALGAIAFAYSYSLILIEIQDTLKSPPSESKTMKNATLISVAVTTVFYMLCGCFGYAAFGDLAPGNLLTGFGFYNPYWLLDIANIAIVVHLVGAYQVYCQPLFAFIEKTAAEWYPESKFIAKEISVPIIGYKSFKLNLFRIIWRTIFVIITTVISMLLPFFNDIVGILGAFGFWPLTVYFPVEMYIVQKKITKWSTKWICLQMLSVACLIISIAAAAGSFAGVVSDLQVYKPFKTT*。
tobaccoNtAAP6Application of gene in tobacco, tobaccoNtAAP6In connection with amino acid transport, after the amino acid transport is silenced, the tyrosine content, the proline content and the asparagine content in tobacco are obviously reduced, and the total protein content is obviously reduced;
in another aspect, tobaccoNtAAP6The gene is related to the regulation of the content of pigment substances in the tobacco, and after the gene is silenced, the content of pigment substances such as chlorophyll a/b, total chlorophyll, carotenoid and the like in the tobacco leaves is obviously increased;
said tobaccoNtAAP6The specific CDS sequence of the gene is shown as SEQ ID No.3, and the corresponding edited amino acid sequence of the tobacco NtAAP6 protein is shown as SEQ ID No.4, or specifically as follows:
NtAAP6gene CDS sequence (1506 bp):
ATGGCACCCGAATTTCAGAAGAACACTATGTACGTATCAACAGAACTCGAAAGAGGAGATGTTCAAAAAAACTTTGATGATGATGGGCGTGAGAAAAGAACTGGGACGTTACTAACGGCAAGTGCACATATTATCACTGCTGTAATTGGTTCAGGAGTGCTTTCTTTAGCATGGGCTATAGCTCAGTTAGGATGGGTGGCTGGTCCTGCTGTTCTCTTTGCTTTTTCTTTCATTACATACTTCACTTCTACACTTCTTGCCGACTGTTACCGTTCTCCCGGCCCCATCTCCGGCAAGAGAAACTACACTTACATGGACGTTGTTCGTTCTCACTTAGGAGGTGTGAAGGTAACACTGTGTGGACTTGCACAATATGCTAACCTCGTCGGAGTTACCATTGGATACACTATTACAGCATCTATCAGTATGGTCGCAGTAAAGAGATCAAATTGTTTTCACAAACATGGCCACGAAGCCAGCTGCTCAATATCGAGCTACCCATATATGATCATATTTGCAGTCATTCAAGTAGTTCTAAGCCAAATACCAAATTTCCACAAGCTCTCATGGCTATCAATTCTTGCTGCTGTTATGTCTTTTACTTACGCTTCTATTGGTCTTGGACTCTCTATTGCCAAAGCTGCTGGGGTAGGGCACCATGTAAAGACAAGCCTAACAGGGACGACAGTAGGAGTTGATGTGTCTGGATCAGAGAAAATATGGAAAAGCTTCCAAGCCATAGGAGATATTGCATTTGCTTATGCTTATTCCACCGTTCTCATCGAAATACAGGCAAGCACACTGTCATTGATTCTGATTCTGATCTTTTCTAAGATTTTATTACGTCGTAGGGATACATTGAGGTCACAACCTCCAGAAAGCAAGGTTATGAAGAGAGCCTCATTAGCTGGAGTTTCCACCACAACTTTATTCTATATACTATGTGGTACCATTGGTTATGCAGCCTTTGGAAATGATGCTCCTGGAAATTTCCTTACTGGTTTTGGTTTCTATGAACCATTTTGGCTAATTGACTTTGCCAACGTTTGCATTGCCGTCCACCTTGTTGGAGCTTACCAGGTTTTCTGCCAACCTTTATATGGGTTCGTGGAGGCTCGTTGCAACGAGCGATGGTCAGACAGCAAATTCATCACCTCCGAGTACGCTGTGCAAGTTCCATGCTGTGGCGTTTACAACGTCAACTTGTTCAGGTTGGTGTGGAGAACAGCATATGTTGTAGTGACAGCCGTGATTGCCATGATATTCCCCTTCTTCAATGACTTCTTGGGTTTGATCGGGGCAGCATCGTTCTATCCATTAACTGTCTACTTCCCAATAGAGATGCACATTGCCCAGAGAAAGATACCAAAGTATTCTTTCACATGGGTATGGCTGAAAATTTTGAGCTGGACTTGCCTGGTTGTATCACTTGTTGCAGCTGCTGGATCTATCCAGGGTCTTGTCACTTCTCTCAAGCATTACAAGCCTTTCTCAACTCAACAATAA;
NtAAP6 protein sequence (501 AA):
MAPEFQKNTMYVSTELERGDVQKNFDDDGREKRTGTLLTASAHIITAVIGSGVLSLAWAIAQLGWVAGPAVLFAFSFITYFTSTLLADCYRSPGPISGKRNYTYMDVVRSHLGGVKVTLCGLAQYANLVGVTIGYTITASISMVAVKRSNCFHKHGHEASCSISSYPYMIIFAVIQVVLSQIPNFHKLSWLSILAAVMSFTYASIGLGLSIAKAAGVGHHVKTSLTGTTVGVDVSGSEKIWKSFQAIGDIAFAYAYSTVLIEIQASTLSLILILIFSKILLRRRDTLRSQPPESKVMKRASLAGVSTTTLFYILCGTIGYAAFGNDAPGNFLTGFGFYEPFWLIDFANVCIAVHLVGAYQVFCQPLYGFVEARCNERWSDSKFITSEYAVQVPCCGVYNVNLFRLVWRTAYVVVTAVIAMIFPFFNDFLGLIGAASFYPLTVYFPIEMHIAQRKIPKYSFTWVWLKILSWTCLVVSLVAAAGSIQGLVTSLKHYKPFSTQQ*。
obtaining tobacco by PCR amplificationNtAAP3The primer pair for the gene comprises the following specific steps:
the upstream primer NtAAP 3-F: 5'-ATGGGAGAAAACAACAACGTTGC-3' the flow of the air in the air conditioner,
downstream primer NtAAP 3-R: 5'-TCAAGTCGTCTTAAAAGGCTTG-3' are provided.
A method for preparing tobaccoNtAAP3The PCR amplification method of the gene takes safflower large gold element cDNA as a template and utilizes a primer pair NtAAP3-F, NtAAP3-R to carry out PCR amplification.
Obtaining tobacco by PCR amplificationNtAAP6The primer pair for the gene comprises the following specific steps:
the upstream primer NtAAP 6-F: 5'-ATGGCACCCGAATTTCAGAAGAA-3' the flow of the air in the air conditioner,
the downstream primer NtAAP 6-R: 5'-TTATTGTTGAGTTGAGAAAGGC-3' are provided.
A method for preparing tobaccoNtAAP6The PCR amplification method of the gene takes safflower large gold element cDNA as a template and utilizes a primer pair NtAAP6-F, NtAAP6-R to carry out PCR amplification.
Tobacco for silencingNtAAP3The gene editing vector of the gene is specifically constructed by the following steps:
(1) first of all, the first step is to,to is directed atNtAAP3The gene (target site specific sequence: GTGACTGAATCCAAGTGCTTTG), the design and editing primer sequence is as follows:
NtAAP3-K-F:5’-GATTGTGACTGAATCCAAGTGCTTTG-3’,
NtAAP3-K-R:5’-AAACCAAAGCACTTGGATTCAGTCAC-3’;
(2) then, obtaining double-stranded DNA of a target site in an annealing operation mode;
(3) next, the CRISPR/Cas9 vector pORE-Cas9/gRNA was usedBsaI, enzyme digestion is carried out, and a digestion product is connected with the annealing product;
(4) and finally, transforming the ligation product into an escherichia coli competent cell, and screening and identifying to ensure correct recombination.
Tobacco for silencingNtAAP3The gene editing vector of the gene is specifically constructed by the following steps:
(1) first, toNtAAP6The gene (target site specific sequence: GTATCAACAGAACTCGAAAG), the design and editing primer sequence is as follows:
NtAAP6-K-F:5’-GATTGTATCAACAGAACTCGAAAG-3’,
NtAAP6-K-R:5’-AAACCTTTCGAGTTCTGTTGATAC-3’。
(2) then, obtaining double-stranded DNA of a target site in an annealing operation mode;
(3) next, the CRISPR/Cas9 vector pORE-Cas9/gRNA was usedBsaI, enzyme digestion is carried out, and a digestion product is connected with the annealing product;
(4) and finally, transforming the ligation product into an escherichia coli competent cell, and screening and identifying to ensure correct recombination.
An obtainingNtAAP3A method for cultivating new variety of gene-silenced tobaccoNtAAP3Transforming agrobacterium into infection liquid with gene editing vector, transforming tobacco, screening and identifying to obtainNtAAP3A new gene-silenced tobacco variety.
An obtainingNtAAP6Method for breeding new variety of gene-silenced tobaccoNtAAP6Gene editing vector transformation of genesAgrobacterium is used as an infection liquid, then tobacco is transformed, and finally, the tobacco is obtained by screening and identifyingNtAAP6A new gene-silenced tobacco variety.
In the prior art, aiming at tobaccoNtAAP2Although there have been preliminary studies on gene functions, further studies have been made on gene functionsNtAAP3、NtAAP6It was found that all three genes belong toAAPsMembers of the gene family, but their actual functions are still clearly distinct. Specifically, the method comprises the following steps:NtAAP2the gene is highly expressed in the roots and stems of the tobacco in the full-bloom stage, particularly the expression level in the stems is higher, andNtAAP3the expression level of the gene in the leaves in the vigorous growth stage and the topping stage is obviously higher than that of other organs,NtAAP6the result that the expression level of the gene in roots and leaves, especially in leaves, is significantly higher than that in other organs indicatesNtAAP3、NtAAP6The functions of the two genes in different growth and development stages and different tissues of tobacco are different. On the other hand, from the construction aspect of new gene mutant varieties, as the RNAi silencing technology has the defects of high off-target rate, poor silencing effect, low conversion rate and the like, the application designs a new gene mutant conversion technology by adopting the CRISPR/Cas9 gene editing technology, thereby laying a certain technical foundation for new variety cultivation.
Generally, the method detects and analyzes the physiological characters such as protein content change, photosynthetic index change, pigment content change and the likeNtAAP3Gene, gene,NtAAP6The relationship between gene and amino acid regulation, protein content regulation and pigment content regulation is preliminarily determined. Based on these studies, for elucidationNtAAP3The gene,NtAAP6The gene lays a theoretical foundation for the functions of amino acid absorption, transport, nitrogen utilization, plant stress resistance regulation and control and the like, and also lays a certain technical foundation for improving the high-efficiency utilization of nitrogen by tobacco and further for breeding new tobacco varieties.
Drawings
FIG. 1 shows the results of total RNA electrophoresis, in which: m: trans2K DNA Marker; 1-2 are directed toNtAAP3The electrophoresis results of total RNA extracted during gene cloning (28S, 18S and 5S bands in the figure, wherein 1-2 are total RNA results of different samples), and 3-4 are specificNtAAP6The electrophoresis result of total RNA extracted during gene cloning (28S, 18S and 5S bands in the figure, wherein 3-4 are the total RNA result of different samples);
FIG. 2 shows the result of electrophoresis of PCR products, in which: m: trans2K DNA Marker, left handNtAAP3Electrophoresis results after gene PCR amplification, right panelNtAAP6Electrophoresis results after gene PCR amplification;
FIG. 3NtAAP3Relative expression quantity of the gene in different periods and tissues of the common tobacco Honghuadajinyuan;
FIG. 4NtAAP6Relative expression quantity of the gene in different periods and tissues of the common tobacco Honghuadajinyuan;
FIG. 5 shows the first round of PCR electrophoresis results in the process of identifying the gene-editing mutant, wherein: m: DL5000 DNA Marker; the upper drawing is a partNtAAP3Identifying results of the gene editing mutants (1-8 are numbers of tobacco plant samples to be identified); the lower drawing is a partNtAAP6Identifying results of the gene editing mutants (1-5 are numbers of tobacco plant samples to be identified);
FIG. 6 shows the results of a second round of PCR electrophoresis of a sample of partial gene editing mutants, wherein: m: DL5000 DNA Marker; the upper diagram isNtAAP3Performing second round PCR electrophoresis on the gene editing mutant (1-8 in the figure are tobacco seedling samples to be identified, and correspond to the samples in the figure 5); the lower diagram isNtAAP6Second round PCR electrophoresis result of gene editing mutant (in the figure, 1-5 are to be identified tobacco seedling samples, corresponding to the sample in figure 5)
FIG. 7 is a drawing showingNtAAP3Statistical results of agronomic traits for Gene editing mutants (legend from top to bottom in each set of histograms from left to right)
FIG. 8 is a drawing showingNtAAP6The agronomic character statistical result of the gene editing mutant;
FIG. 9 shows the change of total protein content of tobacco leaves after gene mutant baking, wherein: the upper diagram isNtAAP3The total protein content of the tobacco leaves is changed after the gene mutant is roasted; the lower diagram isNtAAP6The total protein content of the tobacco leaves is changed after the gene mutant is roasted;
FIG. 10 shows the amino acid content change of the tobacco leaves after gene mutants are baked, wherein: the upper diagram isNtAAP3Gene mutant roastThe amino acid content of the tobacco leaves is changed; the lower diagram isNtAAP6The amino acid content of the tobacco leaves after the gene mutants are baked is changed (each group of column charts correspond to tyrosine, proline and asparagine from left to right respectively);
FIG. 11 is a schematic view ofNtAAP3Fv/Fm values (upper panel), NPQ values (lower panel) of the gene mutants under normal conditions;
FIG. 12 is a schematic view ofNtAAP6Fv/Fm values (upper panel), NPQ values (lower panel) of the gene mutants under normal conditions;
FIG. 13 is a drawing showingNtAAP3Fv/Fm value (upper graph) and NPQ value (lower graph) of the gene mutant under strong light stress;
FIG. 14 is a schematic view ofNtAAP6Fv/Fm value (upper graph) and NPQ value (lower graph) of the gene mutant under strong light stress;
FIG. 15 is a drawing showingNtAAP3The chlorophyll a content (upper graph) and the chlorophyll b content (lower graph) of the gene mutants;
FIG. 16 is a drawing showingNtAAP6The chlorophyll a content (upper graph) and the chlorophyll b content (lower graph) of the gene mutants;
FIG. 17 is a schematic view ofNtAAP3Total chlorophyll content (upper panel) and carotene content (lower panel) of the gene mutant;
FIG. 18 is a drawing showingNtAAP6Total chlorophyll content (upper panel) and carotenoid content (lower panel) of the gene mutants.
Detailed Description
The present application is further illustrated by the following examples. Before describing the specific embodiments, a brief description will be given of some experimental background cases in the following embodiments.
Biological material:
indoor culture of common tobacco Honghua Dajinyuan is carried out in the greenhouse of the national tobacco gene research center (Zhengzhou), and the culture conditions are as follows: the temperature is 23 +/-1) DEG C, the relative humidity is 60 +/-2 percent, and the illumination/darkness is 16 h/8 h; planting and culturing in field;
the synthesis and sequencing of related primers are completed by the Biotechnology Limited company of the New industry of Beijing Optingkok;
experimental reagent:
EasyPure Plant RNA Kit、EasyPure Plant Genomic DNA Kit、TransStartGreen qPCR SuperMix、TransScript Reverse Transcriptase、2×TransTaq High Fidelity (HiFi) PCR SuperMix、pEASY-T1 Cloning Kit、Trans5α Chemically Competent Cell、Trans2K DNA Marker was purchased from Beijing Quanjin Biotechnology Ltd;
DL5000 DNA Marker was purchased from Biotechnology, Inc., of New industry, Kyork, Beijing.
Example 1
The embodiment first of allNtAAP3Gene, gene,NtAAP6The process for obtaining the gene is briefly described below.
(I) designing primers for PCR amplification
Based on the existing tobacco genome sequence and aiming at the target geneNtAAP3、NtAAP6The primer sequences for PCR amplification were designed as follows:
the upstream primer NtAAP 3-F: 5'-ATGGGAGAAAACAACAACGTTGC-3', and the adhesive tape is used for adhering the film to a substrate,
downstream primer NtAAP 3-R: 5'-TCAAGTCGTCTTAAAAGGCTTG-3', respectively;
an upstream primer NtAAP 6-F: 5'-ATGGCACCCGAATTTCAGAAGAA-3', and the adhesive tape is used for adhering the film to a substrate,
downstream primer NtAAP 6-R: 5'-TTATTGTTGAGTTGAGAAAGGC-3' are provided.
(II) preparation of template for PCR amplification
Taking tobacco leaves of Honghuadajinyuan as sample source, freezing with liquid nitrogen, grinding, and referringEasyPurePlant RNA Kit instruction, extracting total RNA, detecting the concentration and purity of the RNA by using a NanoDrop 2000 ultramicro spectrophotometer, and referring to the obtained product after ensuring that the use requirement is metTransScriptReverse Transcriptase, further Reverse transcribing the extracted total RNA into cDNA for later use as a template for subsequent PCR amplification.
The electrophoresis results of total RNA extracted from different samples are shown in FIG. 1, and it can be seen that: the 18S and 28S bands of the total RNA of the extracted tobacco leaves are clear and have no obvious degradation. Further, the RNA concentration determined by an ultramicro spectrophotometer NanoDrop 2000 is 900-1000 ng/muL,OD260/OD280The range of 1.8-2.0, and the requirements of subsequent experiments are met.
(III) PCR amplification
Reference 2TransTaqIn the specification of High Fidelity (High fi) PCR Supermix, the cDNA prepared in the step (two) is used as a template, the primers designed in the step (one) are used for PCR amplification, and a 50-microliter amplification system is designed as follows:
cDNA template, 2. mu.L;
upstream primer, (10. mu. mol/L) 1. mu.L;
downstream primer, (10. mu. mol/L) 1. mu.L;
2×TransTaq HiFi PCR SuperMix ,25 μL;
ultrapure water, added to 50 μ L;
the PCR reaction conditions are as follows: pre-denaturation at 94 ℃ for 2 min; denaturation at 94 ℃ for 30 s, annealing at 56 ℃ for 30 s, extension at 72 ℃ for 90 s, and 35 cycles; extension at 72 ℃ for 5 min.
And detecting the PCR amplification product by 1% agarose gel electrophoresis. The electrophoresis results are shown in fig. 2, and it can be seen that: there is a clear band around 1500 bp.
Then, the target fragment is recovered from the gel, and is connected and transformed according to the description of pEASY-T1 Cloning Kit, and is sent to Beijing Optimalaceae Biotech limited company for sequencing identification (the specific sequence information is shown as SEQ ID No. 1-4, and is expected to be connected with the sequence information of the target fragment) after further screening and colony PCR identificationNtAAP31440 bp gene sequence length,NtAAP6The 1506 bp length of the gene results in agreement).
On the basis of the sequencing result, the inventors further developed the sequence by using the Real-time PCR technologyNtAAP3The gene,NtAAP6The expression pattern of the gene was specifically analyzed, and the specific procedures are briefly described below.
First, based on sequencingNtAAP3、NtAAP6CDS sequence of gene, designing primer sequence for Real-time PCR primer as follows:
upstream primer NtAAP 3-qF: 5'-AGTGTGGTCCATTGAACTCAGAA-3' the flow of the air in the air conditioner,
the downstream primer NtAAP 3-qR: 5'-TATGATATGAGCACTTGCCGTC-3';
the upstream primer NtAAP 6-qF: 5'-ACACACACGCGCGCTAAA-3' the flow of the air in the air conditioner,
the downstream primer NtAAP 6-qR: 5'-GACCAGCCACCCATCCTAAC-3';
at the same time, aiming at the reference geneL25The gene, the primer sequence for PCR amplification is designed as follows:
L25-F:5’-CCCCTCACCACAGAGTCTGC-3’,
L25-R:5’-AAGGGTGTTGTTGTCCTCAATCTT-3’
then, inL25The gene is used as an internal reference gene, cDNA is used as a template, and reference is carried outTransStartGreen qPCR SuperMix instructions, a 20 μ L amplification system was designed as follows:
cDNA template, 1. mu.L;
upstream primer, (10. mu. mol/L) 0.4. mu.L;
downstream primer, (10. mu. mol/L) 0.4. mu.L;
2×TransStart Green qPCR SuperMix,10 μL;
supplementing the nucleic-free Water to 20 mu L;
the reaction conditions are as follows: 94 ℃ for 30 s; 94 ℃, 5 s, 60 ℃, 30 s, 45 cycles; storing at 4 ℃. Each sample was tested in triplicate, averaged, and 2 applied C-△△ T And calculating the result by the method.
The result analysis of the expression pattern shows that:NtAAP3the expression level of the gene in the leaf is obviously higher than that of other organs (P< 0.05), especially in the vigorous and apical stages (see FIG. 3 for specific results); in a similar manner to this, the first and second,NtAAP6the expression level of the gene in roots and leaves, especially in leaves, is also significantly higher than that in other organs (see FIG. 4 for specific results).
Example 2
On the basis of example 1, to determineNtAAP3、NtAAP6The specific functions of the genes, namely the CRISPR/Cas9 technology, are utilized, and the inventor further constructs a gene editing vector and carries out gene silencing so as to specifically determine the functions of the two genes. This example is specifically summarized below with respect to the relevant experimental conditions.
(I) construction of Gene editing vector
(1) First, toNtAAP3The gene (target site specific sequence: GTGACTGAATCCAAGTGCTTTG), the design and editing primer sequence is as follows:
NtAAP3-K-F:5’-GATTGTGACTGAATCCAAGTGCTTTG-3’,
NtAAP3-K-R:5’-AAACCAAAGCACTTGGATTCAGTCAC-3’;
to is directed atNtAAP6The gene (target site specific sequence: GTATCAACAGAACTCGAAAG), the design and editing primer sequence is as follows:
NtAAP6-K-F:5’-GATTGTATCAACAGAACTCGAAAG-3’,
NtAAP6-K-R:5’-AAACCTTTCGAGTTCTGTTGATAC-3’。
(2) subsequently, with reference to the Annealing Buffer for DNA oligonucleotides (5 ×) kit instructions, target site double-stranded DNA was obtained by Annealing operation; in a specific reaction, a 20. mu.L reaction system was designed as follows:
upstream primer, 4. mu.L (50. mu. mol/L);
downstream primer, 4. mu.L (50. mu. mol/L);
Annealing Buffer for DNA Oligos (5×), 4 μL;
nuclear-free Water, to 20 μ L;
the specific annealing reaction conditions are as follows: reducing the temperature of 95 ℃ for 5 min to 25 ℃ every 8 s, wherein the temperature is reduced by 0.1 ℃; the reaction product is directly applied or stored at 4 ℃ for later use.
(3) Next, the CRISPR/Cas9 vector pORE-Cas9/gRNA was usedBsaI, enzyme digestion is carried out, and a digestion product is connected with the annealing product;
during specific enzyme digestion, a 20-mu-L enzyme digestion system is designed as follows:
pORE-Cas9/gRNA vector, 3. mu.L;
10× Buffer,2 μL;
Bsaenzyme I, 1 μ L;
supplementing sterile water to 20 μ L;
the enzyme was cleaved at 37 ℃ for 1 h.
In the specific connection, a 20 μ L connection system is designed as follows:
3 mu L of carrier enzyme digestion product;
annealed product, 6 μ L;
10× T4 DNA Ligase Buffer,2 μL;
T4 DNA Ligase,1 μL;
supplementing sterile water to 20 μ L;
ligation was carried out at 16 ℃ for 30 min.
(4) Finally, the ligation product is convertedTrans5 α chemical Complex Cell (E.coli Competent Cell), and screening and colony PCR identification (forNtAAP3The gene editing vector of (1), when identifying, a primer pair U26-jiance-F, NtAAP3-K-R is adopted; to is directed atNtAAP6The gene editing vector of (1), when identifying, a primer pair U26-jiance-F, NtAAP6-K-R is adopted; U26-jiance-F: 5'-TTAGGTTTACCCGCCAATA-3'); and (3) further sequencing and identifying the positive clone plasmid with correct identification to ensure that the recombination is correct.
(II) preparation of transfection solution
And (3) further amplifying the positive clone (the gene editing vector with correct recombination) which is sequenced and identified in the step (I), transferring the gene editing vector into agrobacterium GV3101 by using an electric transfer method, and further screening and carrying out colony PCR identification to ensure that the transformation is correct. For identification of the correct transformants, Kan was used+And Rif+Further expanding and culturing the two resistant LB liquid culture media, when OD value is 0.6-0.8, centrifugally collecting thalli, and then using MS to perform MS0Liquid Medium (MS)0Liquid culture medium: 4.4 g/L MS inorganic salt, pH value of 5.8-5.9) to OD value of 0.2-0.3, and using the suspension as transfection solution for standby.
(III) transformation and screening
And (5) further transforming the tobacco by using the transfection solution prepared in the step (II) by adopting a leaf disc transformation method, and screening and identifying positive transformation materials.
Specific transformation operations can be referred to as follows:
cutting the leaves of the tobacco aseptic seedlings into 0.5-1 cm2Immersing the square leaf disc into the transfection solution for 7-9 min, taking out the leaf disc, absorbing residual bacteria liquid on the leaf disc by using sterile absorbent paper, and transferring the leaf disc to a transfer stationMS solid culture medium;
dark culture at 22-25 deg.c for 2 days and transferring to MS (Kan)+) Differentiating the culture medium, culturing under the conditions of illumination at 28 ℃ for 16 h, darkness at 25 ℃ for 8 h and relative humidity of 60%, and replacing the fresh culture medium every 8-10 days until adventitious buds grow out;
when the adventitious bud grows to about 1 cm, cutting the adventitious bud, transferring the adventitious bud into an elongation culture medium for culture, and transferring the adventitious bud into a rooting culture medium for continuous culture after two weeks; after the root system grows well, transferring the root system from the culture medium to a seedling culture medium for culture.
The specific culture medium formula can be referred to as follows:
MS culture medium: 4.4 g/L of MS inorganic salt, 30 g/L of cane sugar and 2.5 g/L of plant gel, wherein the pH value is 5.8-5.9;
MS(Kan+) Differentiation medium: 4.4 g/L of MS inorganic salt, 30 g/L of cane sugar, 1 mg/L of 6-BA, 0.1 mg/L of NAA, 150 mg/L of kanamycin, 250 mg/L of cefotaxime sodium, 2.5 g/L of plant gel and the pH value is 5.8-5.9;
an elongation culture medium: 4.4 g/L of MS inorganic salt, 30 g/L of cane sugar, 0.1 mg/L of 6-BA, 150 mg/L of kanamycin, 250 mg/L of cefotaxime sodium, 2.5 g/L of plant gel and the pH value of 5.8-5.9;
rooting culture medium: 4.4 g/L of MS inorganic salt, 30 g/L of cane sugar, 0.002 mg/L of NAA, 150 mg/L of kanamycin, 250 mg/L of cefotaxime sodium, 2.5 g/L of plant gel and the pH value of the plant gel is 5.8-5.9.
When the specific screening and identification are carried out:
firstly, extracting the DNA of tobacco leaves to be identified, and taking the DNA as a template for PCR amplification;
subsequently, respectively utilizing primer pairs NtAAP3-K-F/NtAAP3-K-R, NtAAP6-K-F/NtAAP6-K-R to carry out first round PCR amplification, carrying out electrophoresis detection on PCR amplification products, and carrying out gel recovery on the amplification products;
finally, the first round PCR amplification product recovered by the gel is used as a template, a second round PCR amplification is respectively carried out on NtAAP3-JD-F/NtAAP3-K-R (NtAAP 3-JD-F: 5'-ATAACAGCTGTGATTGGTT-3') and NtAAP6-JD-F/NtAAP6-K-R (NtAAP 6-JD-F: 5'-ACTAACGGCAAGTGCACAT-3') by using a target specific primer, and the electrophoresis detection is carried out on the PCR amplification product.
Based on the second round amplification product results, if the product is little or no, the mutant is a potential homozygous mutant, and then the corresponding first round PCR product is clonally transformed and subjected to sequencing analysis to determine whether the mutant is a homozygous mutant.
The electrophoresis results of the first round PCR amplification products are shown in FIG. 5. It can be seen that the samples of the related gene editing mutants were amplified to obtain specific target bands.
The electrophoresis results of the second round PCR amplification products are shown in FIG. 6. It can be seen that the partially edited mutant samples had fewer PCR products and could be potential homozygous mutants for further characterization.
Further sequencing identification results show that the DNA aims atNtAAP3The result that a base substitution G → A occurred at the target site in the partially mutant sample of gene editing and the base substitution caused a change in the original amino acid sequence, resulting in loss of function of the NtAAP3 protein, indicates that a positive result was successfully obtainedNtAAP3Editing mutant tobacco seedlings by using genes; to aim atNtAAP6The results of gene sequencing showed that base substitution G → T occurred at a part of the target site, and the base substitution caused a change in the original amino acid sequence, resulting in loss of function of the NtAAP6 protein, indicating that a positive result was successfully obtainedNtAAP6And (3) editing mutant tobacco seedlings by genes.
(IV) tobacco trait Change after Gene editing
Based on the homozygous mutant obtained by screening, field planting is carried out on Yuxi Yu Yunnan, and agronomic characters such as plant height, leaf number, stem circumference, pitch, maximum waist leaf length/width and the like are subjected to statistical analysis before and after the topping period.
In the planting process, the contents of the protein, the amino acid and the pigment of the tobacco leaves of the editing mutant are synchronously detected (the total protein of the tobacco leaves is respectively detected by a continuous flow method according to the determination of the protein of YC/T249-2008 tobacco and tobacco products of tobacco products by the method for detecting the total protein of the tobacco leaves, the content of the protein of the fresh tobacco leaves and the baked tobacco leaves is detected by the content of the amino acid according to the determination of the free amino acid of YCT 282-2009 tobacco leaves by the method for detecting the content of various amino acids, and the content of chlorophyll and carotenoid in the tobacco is detected by a high performance liquid chromatography method for determining the plastid pigment of YC/T382-2010 tobacco and tobacco products).
Meanwhile, in the planting process, an Imaging-PAM (polyacrylamide) -full-leaf fluorescence Imaging system is used for monitoring various photosynthetic physiological indexes of the gene editing mutant subjected to topping.
The following is a brief introduction of specific experimental results.
(1) Statistical results of agricultural characters of field
The statistical results of the agronomic traits of part of the fields are shown in fig. 7 and 8. As can be seen,NtAAP3a gene-editing mutant,NtAAP6The phenotype of the related traits of the gene editing mutants is similar, namely: the natural plant height and the knockout plant height of the gene-editing mutant were reduced compared with those of the control group (HD), presumably because ofNtAAP3Gene, gene,NtAAP6The mutation of the gene affects the amino acid transport and nitrogen metabolism, thereby reducing the total biological yield, but the length/width of the maximum waist leaf has no obvious change, and the total tobacco yield is not affected. In general, the agronomic characters of the gene editing mutant are more in line with the requirements of high-quality flue-cured tobacco.
(2) Tobacco leaf protein and amino acid content change
The results of measuring the total protein content and the amino acid content of the tobacco leaves after the gene editing mutants are baked are shown in fig. 9 and fig. 10. Analysis can see that: compared with the control group of safflower Honghuadajinyuan (HD),NtAAP3gene, gene,NtAAP6The total protein content of the tobacco leaves after the gene editing mutant is baked is reduced,NtAAP3the total protein content of the mutant was reduced by 19.8%,NtAAP6the total protein content of the mutant was reduced by 8.4%; the contents of tyrosine, proline and asparagine are lower than those of the control, wherein the reduction of proline and asparagine is particularly remarkable,NtAAP3the proline of the mutant is reduced by 19.0 percent, the asparagine is reduced by 68.1 percent,NtAAP6proline of the mutant is reduced by 36.3%, and asparagine is reduced by 62.9%; show thatNtAAP3Gene, gene,NtAAP6Mutation of the gene reduces the transport efficiency of amino acids and proteins to some extentIs accumulated.
It should be explained that, in view of the manufacturing of cigarette end products, obtaining cigarette raw materials with low phenol release amount during smoking is a main technical objective of related variety improvement, and therefore, when the content of the amino acid is measured, the content of part of typical amino acids in the flue-cured tobacco used as a direct raw material for preparing the cigarette end products is measured, so that the technical effect of the application can be reflected more directly.
(3) Physiological changes of photosynthesis
The results of the photo-biological analysis (the results are shown in FIG. 11, FIG. 12, FIG. 13 and FIG. 14),NtAAP3a gene-editing mutant,NtAAP6The related change trends of the gene editing mutants are consistent, and specifically: compared with the HD of the control group,NtAAP3a gene-editing mutant,NtAAP6The Fv/Fm values of the gene editing mutants under normal conditions are not obviously different, while the NPQ values are increased, which indicates thatNtAAP3Gene, gene,NtAAP6After the gene is edited, the photosynthetic efficiency of the plant is not greatly influenced, and the photoprotective capacity of the plant is improved.
Further, the measurement result under the strong light condition (60000-70000 Lux) shows that compared with the HD of the control group,NtAAP3a gene-editing mutant,NtAAP6The Fv/Fm and NPQ values of the gene editing mutant are obviously reduced under the strong stress condition. The photosynthetic efficiency of the plant should be improved when the illumination is enhanced, and the plant also starts the heat dissipation, namely the photoprotection mechanism, at the same timeNtAAP3A mutant,NtAAP6The Fv/Fm and NPQ values of the gene editing mutant do not rise or fall, which indicates that the gene is edited, the transport rate of amino acid is influenced, the photosynthetic efficiency of the plant is possibly reduced, and the photoprotective ability of the plant is weakened.
(4) Change of pigment content
The measurement results of different types of pigment contents (fresh tobacco leaves at harvest time) are shown in fig. 15, fig. 16, fig. 17 and fig. 18.NtAAP3A gene-editing mutant,NtAAP6The related change trends of the gene editing mutants are consistent, and specifically:NtAAP3a gene editing mutant,NtAAP6Leaves of Gene-editing mutantsThe contents of chlorophyll a/b, total chlorophyll and carotenoid are all increased, whereinNtAAP3The chlorophyll a of the mutant is increased by 10.5 percent, the chlorophyll b is increased by 17.5 percent, the total chlorophyll is increased by 12.6 percent, the carotenoid is increased by 6.4 percent,NtAAP6the chlorophyll a of the mutant is increased by 15.8%, the chlorophyll b is increased by 15.4%, the total chlorophyll is increased by 15.7%, and the carotenoid is increased by 21.4%. This indicates that the mutation of the gene, although affecting amino acid transport and protein accumulation, did not reduce the pigment content of tobacco. The appearance and the internal quality of the tobacco leaves can be influenced by the content of the carotenoid, degradation and thermal cracking products of the carotenoid contain a plurality of aroma substances and are closely related to the aroma of the tobacco leaves, and the mutant also ensures the internal and external excellent quality of the tobacco leaves on the basis of reducing the content of amino acid and protein.
Amino acids are very important nitrogen-containing compounds in plants, play a very important role in the processes of growth, development, metabolic regulation and the like of plants, and amino acid transporters play an indispensable role in the process of amino acid transport in plants. Amino Acid Permeases (AAPs), a subfamily of amino acid transporters, are widely involved in the transport and absorption of amino acids in various tissues and organs throughout plant growth and development.
In the present application, through the above-mentioned pairsNtAAP3The gene,NtAAP6The preliminary study of gene function can preliminarily confirm that:
NtAAP3the gene is highly expressed in leaves, and has direct influence on the transfer rate of amino acid after mutation, particularly obviously reduces the reduction of the content of amino acid such as proline, asparagine and the like, and further reduces the content of total protein; on the other hand, in the case of a liquid,NtAAP3the content of pigment substances such as chlorophyll a/b, total chlorophyll, carotenoid and the like in the mutant is obviously increased;
andNtAAP3the genes are similar to each other and can be used,NtAAP6the gene is highly expressed in roots and leaves, has direct influence on the transport rate of amino acid after being mutated, particularly obviously reduces the reduction of the content of amino acid such as proline, asparagine and the like, and further leads to the content of total proteinDecreasing; on the other hand, in the case of a liquid,NtAAP6the content of pigment substances such as chlorophyll a/b, total chlorophyll, carotenoid and the like in the mutant is obviously increased.
In combination with the results of the relevant assays, will furtherNtAAP3AndNtAAP6the statistics of the changes in some components in the gene editing mutants are shown in table 1 below.
In the context of Table 1, the following examples are,NtAAP3andNtAAP6statistics of changes in Components of Gene editing mutants
Note: the trends in the changes ↓and ↓ in the table relative to the control.
By combining the data in the table, the following can be seen visually:NtAAP3andNtAAP6in comparison between the gene-editing mutants,NtAAP3the reduction of total protein and asparagine of the mutant is larger than that of the mutantNtAAP6The mutant is a mutant of a microorganism,NtAAP3respectively isNtAAP62.36 times and 1.08 times of the total weight of the composition; chlorophyll b is increased more thanNtAAP6The mutant is a mutant of a microorganism,NtAAP3is amplified byNtAAP61.14 times of. WhileNtAAP6The proline of the mutant is reduced more thanNtAAP3The mutant is a mutant of a microorganism,NtAAP6is reduced in amplitudeNtAAP31.91 times of; the chlorophyll a, total chlorophyll and carotenoid are increased more thanNtAAP3The mutant is a mutant of a microorganism,NtAAP6respectively isNtAAP31.50 times, 1.25 times and 3.34 times of the total weight of the composition.
These data further show that it is possible to identify,NtAAP3andNtAAP6although genes perform similar functions in some respects, they are somewhat different.
SEQUENCE LISTING
<110> Zhengzhou tobacco institute of China tobacco general Co
<120> application of NtAAP3 gene of tobacco in tobacco
<130> none
<160> 4
<170> PatentIn version 3.5
<210> 1
<211> 1440
<212> DNA
<213> Nicotiana tabacum
<400> 1
atgggagaaa acaacaacgt tgcttcaaaa caccaagtgt tcgatgtttc cattaatgtg 60
actgaatcca agtgctttga cgatgatggc cgtctcaaaa gaaccgggag cgtttggacg 120
gcaagtgctc atatcataac agctgtgatt ggttcgggag ttttgtcttt agcatgggca 180
gtagctcaac ttggttggat tgctggtcct attgttatga ttttgttctc ttttgttact 240
tattacactt ccgctcttct tgccgattgt taccgctccg gcgactctgt ttccggcaag 300
agaaactata cttacatgga tgctgtccaa gccaatcttg gtgggctcca agtcaagatt 360
tgtggatgga ttcagtatgc gaatcttttt ggagttgcta tcggatacac cattgcatct 420
tcaattagca tgatagctat taaaaggtct aattgtttcc acaaacatgg tgatcaagct 480
ccttgtcaag tatccagcac tccatacatg atcatgtttg gaataataga aatcatcttc 540
tcccaaattc cagattttga tcagatttgg tggctttcaa ttgtggctgc cgttatgtct 600
ttcacttact ctactattgg actaggatta ggagttgcta aagtggcaga aactggaaaa 660
atcggaggaa gtctcactgg aattagcatc ggaactgtga ctgaaatgca aaagatttgg 720
aaaagcttcc aagcccttgg agctatcgct tttgcctatt cttactctct catccttatt 780
gagattcagg atacactcaa atctccaccg tcagaatcca agacaatgaa aaatgcaact 840
ctaattagtg tagcagtaac aacagttttc tacatgctct gtggctgctt tggctatgca 900
gcatttggag atcttgctcc tggaaactta ctaactggtt ttggattcta caatccttat 960
tggctactcg atatagcgaa catagccatt gtcgtccacc ttgttggtgc ataccaggtt 1020
tactgccagc cccttttcgc cttcattgaa aaaacagcag cagaatggta ccccgagagt 1080
aaattcattg ccaaagagat tagtgtcccg attataggct ataaatcctt taaactcaac 1140
cttttccgca taatttggag gactattttc gtcatcatca ccacggtcat atctatgcta 1200
ttgccattct tcaatgacat agttggaatt cttggagcct ttgggttttg gccgctaaca 1260
gtctatttcc cggtggaaat gtacattgtg caaaagaaga taacaaaatg gagcacaaaa 1320
tggatttgcc ttcaaatgct tagtgttgct tgccttatta tctcaattgc tgcagctgct 1380
ggttcttttg ctggcgttgt atctgatcta caagtttaca agccttttaa gacgacttga 1440
<210> 2
<211> 479
<212> PRT
<213> Nicotiana tabacum
<400> 2
Met Gly Glu Asn Asn Asn Val Ala Ser Lys His Gln Val Phe Asp Val
1 5 10 15
Ser Ile Asn Val Thr Glu Ser Lys Cys Phe Asp Asp Asp Gly Arg Leu
20 25 30
Lys Arg Thr Gly Ser Val Trp Thr Ala Ser Ala His Ile Ile Thr Ala
35 40 45
Val Ile Gly Ser Gly Val Leu Ser Leu Ala Trp Ala Val Ala Gln Leu
50 55 60
Gly Trp Ile Ala Gly Pro Ile Val Met Ile Leu Phe Ser Phe Val Thr
65 70 75 80
Tyr Tyr Thr Ser Ala Leu Leu Ala Asp Cys Tyr Arg Ser Gly Asp Ser
85 90 95
Val Ser Gly Lys Arg Asn Tyr Thr Tyr Met Asp Ala Val Gln Ala Asn
100 105 110
Leu Gly Gly Leu Gln Val Lys Ile Cys Gly Trp Ile Gln Tyr Ala Asn
115 120 125
Leu Phe Gly Val Ala Ile Gly Tyr Thr Ile Ala Ser Ser Ile Ser Met
130 135 140
Ile Ala Ile Lys Arg Ser Asn Cys Phe His Lys His Gly Asp Gln Ala
145 150 155 160
Pro Cys Gln Val Ser Ser Thr Pro Tyr Met Ile Met Phe Gly Ile Ile
165 170 175
Glu Ile Ile Phe Ser Gln Ile Pro Asp Phe Asp Gln Ile Trp Trp Leu
180 185 190
Ser Ile Val Ala Ala Val Met Ser Phe Thr Tyr Ser Thr Ile Gly Leu
195 200 205
Gly Leu Gly Val Ala Lys Val Ala Glu Thr Gly Lys Ile Gly Gly Ser
210 215 220
Leu Thr Gly Ile Ser Ile Gly Thr Val Thr Glu Met Gln Lys Ile Trp
225 230 235 240
Lys Ser Phe Gln Ala Leu Gly Ala Ile Ala Phe Ala Tyr Ser Tyr Ser
245 250 255
Leu Ile Leu Ile Glu Ile Gln Asp Thr Leu Lys Ser Pro Pro Ser Glu
260 265 270
Ser Lys Thr Met Lys Asn Ala Thr Leu Ile Ser Val Ala Val Thr Thr
275 280 285
Val Phe Tyr Met Leu Cys Gly Cys Phe Gly Tyr Ala Ala Phe Gly Asp
290 295 300
Leu Ala Pro Gly Asn Leu Leu Thr Gly Phe Gly Phe Tyr Asn Pro Tyr
305 310 315 320
Trp Leu Leu Asp Ile Ala Asn Ile Ala Ile Val Val His Leu Val Gly
325 330 335
Ala Tyr Gln Val Tyr Cys Gln Pro Leu Phe Ala Phe Ile Glu Lys Thr
340 345 350
Ala Ala Glu Trp Tyr Pro Glu Ser Lys Phe Ile Ala Lys Glu Ile Ser
355 360 365
Val Pro Ile Ile Gly Tyr Lys Ser Phe Lys Leu Asn Leu Phe Arg Ile
370 375 380
Ile Trp Arg Thr Ile Phe Val Ile Ile Thr Thr Val Ile Ser Met Leu
385 390 395 400
Leu Pro Phe Phe Asn Asp Ile Val Gly Ile Leu Gly Ala Phe Gly Phe
405 410 415
Trp Pro Leu Thr Val Tyr Phe Pro Val Glu Met Tyr Ile Val Gln Lys
420 425 430
Lys Ile Thr Lys Trp Ser Thr Lys Trp Ile Cys Leu Gln Met Leu Ser
435 440 445
Val Ala Cys Leu Ile Ile Ser Ile Ala Ala Ala Ala Gly Ser Phe Ala
450 455 460
Gly Val Val Ser Asp Leu Gln Val Tyr Lys Pro Phe Lys Thr Thr
465 470 475
<210> 3
<211> 1506
<212> DNA
<213> Nicotiana tabacum
<400> 3
atggcacccg aatttcagaa gaacactatg tacgtatcaa cagaactcga aagaggagat 60
gttcaaaaaa actttgatga tgatgggcgt gagaaaagaa ctgggacgtt actaacggca 120
agtgcacata ttatcactgc tgtaattggt tcaggagtgc tttctttagc atgggctata 180
gctcagttag gatgggtggc tggtcctgct gttctctttg ctttttcttt cattacatac 240
ttcacttcta cacttcttgc cgactgttac cgttctcccg gccccatctc cggcaagaga 300
aactacactt acatggacgt tgttcgttct cacttaggag gtgtgaaggt aacactgtgt 360
ggacttgcac aatatgctaa cctcgtcgga gttaccattg gatacactat tacagcatct 420
atcagtatgg tcgcagtaaa gagatcaaat tgttttcaca aacatggcca cgaagccagc 480
tgctcaatat cgagctaccc atatatgatc atatttgcag tcattcaagt agttctaagc 540
caaataccaa atttccacaa gctctcatgg ctatcaattc ttgctgctgt tatgtctttt 600
acttacgctt ctattggtct tggactctct attgccaaag ctgctggggt agggcaccat 660
gtaaagacaa gcctaacagg gacgacagta ggagttgatg tgtctggatc agagaaaata 720
tggaaaagct tccaagccat aggagatatt gcatttgctt atgcttattc caccgttctc 780
atcgaaatac aggcaagcac actgtcattg attctgattc tgatcttttc taagatttta 840
ttacgtcgta gggatacatt gaggtcacaa cctccagaaa gcaaggttat gaagagagcc 900
tcattagctg gagtttccac cacaacttta ttctatatac tatgtggtac cattggttat 960
gcagcctttg gaaatgatgc tcctggaaat ttccttactg gttttggttt ctatgaacca 1020
ttttggctaa ttgactttgc caacgtttgc attgccgtcc accttgttgg agcttaccag 1080
gttttctgcc aacctttata tgggttcgtg gaggctcgtt gcaacgagcg atggtcagac 1140
agcaaattca tcacctccga gtacgctgtg caagttccat gctgtggcgt ttacaacgtc 1200
aacttgttca ggttggtgtg gagaacagca tatgttgtag tgacagccgt gattgccatg 1260
atattcccct tcttcaatga cttcttgggt ttgatcgggg cagcatcgtt ctatccatta 1320
actgtctact tcccaataga gatgcacatt gcccagagaa agataccaaa gtattctttc 1380
acatgggtat ggctgaaaat tttgagctgg acttgcctgg ttgtatcact tgttgcagct 1440
gctggatcta tccagggtct tgtcacttct ctcaagcatt acaagccttt ctcaactcaa 1500
caataa 1506
<210> 4
<211> 501
<212> PRT
<213> Nicotiana tabacum
<400> 4
Met Ala Pro Glu Phe Gln Lys Asn Thr Met Tyr Val Ser Thr Glu Leu
1 5 10 15
Glu Arg Gly Asp Val Gln Lys Asn Phe Asp Asp Asp Gly Arg Glu Lys
20 25 30
Arg Thr Gly Thr Leu Leu Thr Ala Ser Ala His Ile Ile Thr Ala Val
35 40 45
Ile Gly Ser Gly Val Leu Ser Leu Ala Trp Ala Ile Ala Gln Leu Gly
50 55 60
Trp Val Ala Gly Pro Ala Val Leu Phe Ala Phe Ser Phe Ile Thr Tyr
65 70 75 80
Phe Thr Ser Thr Leu Leu Ala Asp Cys Tyr Arg Ser Pro Gly Pro Ile
85 90 95
Ser Gly Lys Arg Asn Tyr Thr Tyr Met Asp Val Val Arg Ser His Leu
100 105 110
Gly Gly Val Lys Val Thr Leu Cys Gly Leu Ala Gln Tyr Ala Asn Leu
115 120 125
Val Gly Val Thr Ile Gly Tyr Thr Ile Thr Ala Ser Ile Ser Met Val
130 135 140
Ala Val Lys Arg Ser Asn Cys Phe His Lys His Gly His Glu Ala Ser
145 150 155 160
Cys Ser Ile Ser Ser Tyr Pro Tyr Met Ile Ile Phe Ala Val Ile Gln
165 170 175
Val Val Leu Ser Gln Ile Pro Asn Phe His Lys Leu Ser Trp Leu Ser
180 185 190
Ile Leu Ala Ala Val Met Ser Phe Thr Tyr Ala Ser Ile Gly Leu Gly
195 200 205
Leu Ser Ile Ala Lys Ala Ala Gly Val Gly His His Val Lys Thr Ser
210 215 220
Leu Thr Gly Thr Thr Val Gly Val Asp Val Ser Gly Ser Glu Lys Ile
225 230 235 240
Trp Lys Ser Phe Gln Ala Ile Gly Asp Ile Ala Phe Ala Tyr Ala Tyr
245 250 255
Ser Thr Val Leu Ile Glu Ile Gln Ala Ser Thr Leu Ser Leu Ile Leu
260 265 270
Ile Leu Ile Phe Ser Lys Ile Leu Leu Arg Arg Arg Asp Thr Leu Arg
275 280 285
Ser Gln Pro Pro Glu Ser Lys Val Met Lys Arg Ala Ser Leu Ala Gly
290 295 300
Val Ser Thr Thr Thr Leu Phe Tyr Ile Leu Cys Gly Thr Ile Gly Tyr
305 310 315 320
Ala Ala Phe Gly Asn Asp Ala Pro Gly Asn Phe Leu Thr Gly Phe Gly
325 330 335
Phe Tyr Glu Pro Phe Trp Leu Ile Asp Phe Ala Asn Val Cys Ile Ala
340 345 350
Val His Leu Val Gly Ala Tyr Gln Val Phe Cys Gln Pro Leu Tyr Gly
355 360 365
Phe Val Glu Ala Arg Cys Asn Glu Arg Trp Ser Asp Ser Lys Phe Ile
370 375 380
Thr Ser Glu Tyr Ala Val Gln Val Pro Cys Cys Gly Val Tyr Asn Val
385 390 395 400
Asn Leu Phe Arg Leu Val Trp Arg Thr Ala Tyr Val Val Val Thr Ala
405 410 415
Val Ile Ala Met Ile Phe Pro Phe Phe Asn Asp Phe Leu Gly Leu Ile
420 425 430
Gly Ala Ala Ser Phe Tyr Pro Leu Thr Val Tyr Phe Pro Ile Glu Met
435 440 445
His Ile Ala Gln Arg Lys Ile Pro Lys Tyr Ser Phe Thr Trp Val Trp
450 455 460
Leu Lys Ile Leu Ser Trp Thr Cys Leu Val Val Ser Leu Val Ala Ala
465 470 475 480
Ala Gly Ser Ile Gln Gly Leu Val Thr Ser Leu Lys His Tyr Lys Pro
485 490 495
Phe Ser Thr Gln Gln
500
Claims (2)
1. TobaccoNtAAP3The application of the gene in the regulation and control of the amino acid content or the total protein content of the tobacco is characterized in that the tobaccoNtAAP3In relation to amino acid transport, the regulation is to silence the NtAAP3 gene, to down regulate the amino acid content in tobacco or the total protein content, the amino acids being tyrosine, proline and asparagine;
said tobaccoNtAAP3The gene and the specific CDS sequence are shown in SEQ ID No. 1.
2. TobaccoNtAAP3The application of the gene in the regulation and control of tobacco pigment substances is characterized in that the tobaccoNtAAP3The gene is related to the content of pigment substances in tobacco, the NtAAP3 gene is silenced, the content of the pigment substances in tobacco leaves is increased, and the pigment substances are chlorophyll a, chlorophyll b and carotenoid;
said tobaccoNtAAP3The gene and the specific CDS sequence are shown in SEQ ID No. 1.
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| CN202110736575.XA CN113373166B (en) | 2021-06-30 | 2021-06-30 | Application of tobacco NtAAP3 gene in tobacco |
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| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN202110736575.XA CN113373166B (en) | 2021-06-30 | 2021-06-30 | Application of tobacco NtAAP3 gene in tobacco |
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| Publication Number | Publication Date |
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| CN113373166A CN113373166A (en) | 2021-09-10 |
| CN113373166B true CN113373166B (en) | 2022-06-24 |
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| CN202110736575.XA Active CN113373166B (en) | 2021-06-30 | 2021-06-30 | Application of tobacco NtAAP3 gene in tobacco |
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Families Citing this family (2)
| Publication number | Priority date | Publication date | Assignee | Title |
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| CN114350685B (en) * | 2022-01-27 | 2023-10-24 | 中国烟草总公司郑州烟草研究院 | Application of tobacco NtTAC1 gene in leaf angle regulation and control |
| CN114990151B (en) * | 2022-04-18 | 2023-04-14 | 河北省农林科学院粮油作物研究所 | Crop nitrogen utilization efficiency and grain yield collaborative improvement method based on gene editing technology |
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| GB0510928D0 (en) * | 2005-05-27 | 2005-07-06 | Swetree Technologies Ab | Altered amino acid uptake in plants |
| CN104046638A (en) * | 2014-05-09 | 2014-09-17 | 吉林农业大学 | Arabidopis thaliana AAP1 gene cloning and plant expression vector construction method |
| CN108220305A (en) * | 2017-12-15 | 2018-06-29 | 中国烟草总公司郑州烟草研究院 | Tobacco amino acid permease NtAAP2 genes and its application |
| CN112342222A (en) * | 2019-08-09 | 2021-02-09 | 山东省农业科学院作物研究所 | Wheat salt-tolerant gene TaAAP3 and application thereof |
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