INTELLIGENT GENETIC BREEDING AND SEED PRODUCTION SYSTEM FOR CROP CROSS BREEDING AND HYBRID SEED PRODUCTION, AND APPLICATION THEREOF
20230332173 · 2023-10-19
Assignee
Inventors
- Baoguang AN (Hainan, CN)
- Tuan LONG (Hainan, CN)
- Xinpeng LI (Hainan, CN)
- Xiang ZENG (Hainan, CN)
- Yongzhong WU (Hainan, CN)
- Peijin HUANG (Hainan, CN)
Cpc classification
C12N15/8218
CHEMISTRY; METALLURGY
C12N15/8212
CHEMISTRY; METALLURGY
International classification
Abstract
An intelligent genetic breeding and seed production system for crop cross breeding and hybrid seed production are disclosed. The system comprises a GAT system carrier. The carrier comprises five functional element expression cassettes: a plant male fertility restoration genetic element expression cassette, used for restoring the male fertility of a recessive genic male sterile mutant; a plant pollen abortion genetic element expression cassette, used for clearing GAT-containing pollen and maintaining a heterozygous state or a hemizygous state of a GAT maintainer line; a chemical herbicide positive selection expression cassette, used for gene transformation and impurity removal and purification for the GAT maintainer line; a chemical herbicide negative selection expression cassette, used for clearing pollen and seed escape of a herbicide-sensitive GAT maintainer line and impurity removal and purification for a GAT sterile line; and a seed screening element expression cassette, used for mechanical sorting of seeds.
Claims
1. An intelligent genetic breeding and seed production system for crop cross breeding and seed production, called GAT system, characterized by comprising three lines of a plant recessive genic male sterile line, i.e., GAT sterile line, a recessive genic male sterile maintainer line, i.e., GAT maintainer line, and a common restorer line; wherein the GAT maintainer line contains a GAT vector which comprises five functional element expression cassettes: (1) a plant male fertility restoration genetic element expression cassette, used for restoring the male fertility of a recessive genic male sterile mutant; (2) a plant pollen abortion genetic element expression cassette, used for clearing GAT-containing pollen and maintaining a heterozygous state or a hemizygous state of the GAT maintainer line; (3) a gene transformation and maintainer line screening element expression cassette, used for gene transformation and impurity removal and purification for the GAT maintainer line; (4) a herbicide-sensitive element expression cassette, used for clearing pollen and seed escape of a herbicide-sensitive GAT maintainer line and impurity removal and purification for a GAT sterile line; (5) a seed screening element expression cassette, used for mechanical sorting of seeds; the five functional element expression cassettes are constructed on a final vector to obtain a GAT system vector.
2. The intelligent genetic breeding and seed production system according to claim 1, wherein the GAT vector is introduced into the GAT sterile line to create the GAT maintainer line, and the GAT vector exists in the genome of the GAT maintainer line in a single copy form; the GAT sterile line is a sterile line controlled by a single recessive nuclear gene, and is male sterile when a gene locus is in a recessive homozygous state; and is male fertile when a gene locus is in a heterozygous state and a dominant homozygous state; the GAT maintainer line is self-fertilized and fructified, and the obtained seeds are separated to obtain the GAT maintainer line and the GAT sterile line in a ratio of 1:1; the two seeds are separated by seed screening elements to realize self-propagation of GAT maintainer line; the GAT maintainer line pollinate GAT sterile line to make GAT sterile line bear and maintain male sterility in their progeny, thus realizing the propagation of recessive male genetic sterile line.
3. A vector for intelligent genetic breeding and seed production of the crop, called GAT vector, which is obtained by constructing five functional element expression cassettes on the final vector by linking them by a linker, the five functional element expression cassettes are respectively: (1) a plant male fertility restoration genetic element expression cassette, used for restoring the male fertility of a recessive genic male sterile mutant; (2) a plant pollen abortion genetic element expression cassette, used for clearing GAT-containing pollen and maintaining a heterozygous state or a hemizygous state of the GAT maintainer line; (3) a gene transformation and maintainer line screening element expression cassette, used for gene transformation and impurity removal and purification for the GAT maintainer line; (4) a herbicide-sensitive element expression cassette, used for clearing pollen and seed escape of a herbicide-sensitive GAT maintainer line and impurity removal and purification for a GAT sterile line; (5) a screening element expression cassette, used for mechanical sorting of seeds; the five functional element expression cassettes are constructed by linking the linker to obtain the GAT system vector.
4. The vector according to claim 3, wherein said (1) a plant male fertility restoration genetic element expression cassette is sequentially and functionally linked by a promoter, a male fertility restoration gene coding region and a terminator; the male fertility restoration genes are MS1, MS2, MS3, MS5, MS7, MS8, MS9, MS10, MS11, MS12, MS13, MS14, MS17, MS20, MS22, MS23, MS24, MS25, OsCYP704B2, MS27, MS28, MS29, MS30, MS31, MS32, MS33, MS34, MS36, MS37, MS38, MS43, MS45, MS48, MS50, or a wild-type gene of the OsCYP704B2 gene, the promoter and the terminator are promoters and terminators, respectively, of respective genes, preferably the OsCYP704B2 gene; preferably, the sequence of said (1) a plant male fertility restoration genetic element expression cassette is represented by SEQ ID NO. 6.
5. The vector according to claim 3, wherein said (2) a plant pollen abortion genetic element expression cassette is sequentially and functionally linked by a plant pollen specific promoter, a signal peptide, an abortion gene coding region and a terminator; preferably the promoters are corn PG47 promoter, rice PCHF15, OsPC32 promoters, preferably the abortion genes are rice α-amylase gene OsAA, corn α-amylase gene Zm-AA1, barley α-amylase gene HvAA1, millet α-amylase gene SiAA, cytokinin oxidase, cysteine protease and gibberellin oxidase, and the terminator is corn IN2-1 or NosT terminator; preferably, the sequence of said (2) a plant pollen abortion genetic element expression cassette is represented by SEQ ID NO. 7, or represented by SEQ ID NO. 8, or represented by SEQ ID NO. 9.
6. The vector according to claim 3, wherein said (3) a gene transformation and maintainer line screening element expression cassette is sequentially and functionally linked by a promoter, a screening marker gene coding region and a terminator; preferably the promoter is any one of Actin promoter or a 2180 bp sequence upstream of OsALS gene initiation codon ATG, preferably the screening marker gene coding region is any one of OsALSm1, OsALSm2, OsALSm3 sequence, glyphosate resistant gene EPSPSm sequence, glyphosate N-acetyltransferase sequence or glufosinate resistant gene Bar sequence; the terminator is an OsUbiT terminator or a NosT terminator; and preferably, the sequence of the gene transformation and maintainer line screening element expression cassette is represented by SEQ ID NO. 10; or represented by SEQ ID NO. 11, or represented by SEQ ID NO. 12, or represented by SEQ ID NO. 13.
7. The vector according to claim 3, wherein said (4) a herbicide-sensitive element expression cassette is sequentially and functionally linked by a promoter, a herbicide-dominant sensitive element and a terminator, preferably the promoter is a ZmUbi promoter, the herbicide-dominant sensitive element is an RNAi structural sequence P450i of cytochrome p450 gene CYP81A6, and the terminator is a PinII terminator and a NosT terminator; preferably, said (4) herbicide sensitive element expression cassette is P450i-1, P450i-2 or P450i-3, and the sequences thereof are represented by SEQ ID NO. 14, SEQ ID NO. 15 and SEQ ID NO. 16, respectively.
8. The vector according to claim 3, wherein said (5) seed screening element expression cassette is sequentially and functionally linked by a promoter, a seed coat chromogenic gene and a terminator, preferably, the promoter is a seed specific promoter ZZ1 promoter, the seed coat chromogenic gene is crimson fluorescent protein FP635, red fluorescent protein RFP or green fluorescent protein GFP, and the terminator is OS-T28 terminator and NosT terminator; preferably, the sequence of the seed screening element expression cassette is represented by SEQ ID NO. 17.
9. The vector according to claim 3, wherein the linker comprises a multiple cloning site MCSI, the sequence thereof is represented by SEQ ID NO. 18; a multiple cloning site MCSII, the sequence thereof is represented by SEQ ID NO. 19; a multiple cloning site MCSIII, the sequence thereof is represented by SEQ ID NO. 20; a multiple cloning site MCSIV, the sequence thereof is represented by SEQ ID NO. 21; or a multiple cloning site MCSV, and the sequence thereof is represented by SEQ ID NO. 22.
10. The vector according to claim 3, wherein the final vector is pC0307, the sequence thereof is represented by SEQ ID NO. 25, or the final vector is pC0308, the sequence thereof is represented by SEQ ID NO. 26, or the final vector is pC0309, and the sequence thereof is represented by SEQ ID NO. 27.
11. A vector according to claim 3, wherein the GAT vector is pC0308-MMMaauCK5400, pC0308-KhvMMaauMCK5400, pC0308-KhvMaauMCMK5400, pC0309-KhvMaauMCMK5400 and pC0307-KhvMaauMCMK5400; and the nucleotide sequences thereof are respectively represented by SEQ ID NOs. 1-5.
12. The method for constructing a vector according to claim 3, wherein the vector is obtained by constructing five functional element expression cassettes on the final vector by linking them by a linker, the five functional element expression cassettes are respectively: (1) a plant male fertility restoration genetic element expression cassette, used for restoring the male fertility of a recessive genic male sterile mutant; the expression cassette is sequentially and functionally linked by a promoter, a male fertility restoration gene coding region and a terminator; (2) a plant pollen abortion genetic element expression cassette, used for clearing GAT-containing pollen and maintaining a heterozygous state or a hemizygous state of the GAT maintainer line; the expression cassette is sequentially and functionally linked by a plant pollen specific promoter, an abortion gene coding region and a terminator; (3) a gene transformation and maintainer line screening element expression cassette, used for gene transformation and impurity removal and purification for the GAT maintainer line; the expression cassette is sequentially and functionally linked by a promoter, a screening marker gene coding region and a terminator; (4) a herbicide-sensitive element expression cassette, used for clearing pollen and seed escape of a herbicide-sensitive GAT maintainer line and impurity removal and purification for a GAT sterile line; the expression cassette is sequentially and functionally linked by a promoter, a herbicide-dominant sensitive element and a terminator; (5) a seed screening element expression cassette, used for mechanical sorting of seeds; the five functional element expression cassettes are constructed by linking the linker to obtain the GAT system vector; the expression cassette is sequentially and functionally linked by a promoter, a seed coat chromogenic gene and a terminator.
13. A method for maintaining the genotypic state of a plant recessive genic male sterile plant, wherein the intelligent genetic breeding and seed production system according to claim 1 is adopted to introduce a GAT vector into a GAT sterile line with a recessive homozygous genotype to create a GAT transformant or a GAT maintainer line containing only a single copy of the GAT vector, and the genotype of the GAT transformant or the GAT maintainer line is recessive homozygous/GAT−, the GAT transformant or the GAT maintainer line is pollinated to the GAT sterile line, and the genotype of the obtained seed remains a recessive homozygous status, thereby maintaining male sterility in the progeny of the GAT sterile line and successfully propagating the GAT sterile line.
14. A method for maintaining a heterozygous state or a hemizygous state of the GAT locus in a GAT transformant or a GAT maintainer line, wherein the intelligent genetic breeding and seed production system according to claim 1 is adopted to introduce a GAT vector into a GAT sterile line with recessive homozygous genotype to create a GAT transformant or a GAT maintainer line containing only a single copy of the GAT vector, and the genotype of the GAT transformant or the GAT maintainer line is recessive homozygous/GAT−; the GAT transformant or the GAT maintainer line self-fertilizes and produces two genotypes of seeds, one genotypic seed is recessive homozygous/GAT−, which is a GAT maintainer line, and the other genotypic seed is recessive homozygous/−−, which is a GAT sterile line; according to the law of inheritance, the two are separated in 1:1, that is to say, the GAT locus with a genotype of recessive homozygous/GAT− in the self-progeny of a GAT transformant or a GAT maintainer line remained in the heterozygous state or the hemizygous state.
15. A method for screening or distinguishing seeds and plants obtained by self-breeding of a GAT transformant, the GAT transformant is a GAT transformant containing only a single copy of the GAT vector created by introducing a GAT vector into a GAT sterile line with a recessive homozygous genotype adopting the intelligent genetic breeding and seed production system according to claim 1, the genotype of the GAT transformant is recessive homozygous/GAT−, wherein the seeds obtained by self-breeding and fruiting of the GAT transformant are separated in a ratio of 1:1, wherein 50% of the seeds are seeds containing a GAT vector, the genotype is recessive homozygous/GAT−, and fluorescence is observed under excitation light; and 50% of the seeds are seeds without GAT vector, and the genotype was recessive homozygous, without GAT element, and no fluorescence is observed under excitation light; at the seed or plant level, with high resistance to all types of herbicides directed against acetolactate synthase or EPSPS or Bar genes, including but not limited to bispyribac-sodium, imazethapyr, methomyl, glyphosate, glufosinate or glufosinate ammonium when the genotype is recessive homozygous/GAT−; and 50% of the seeds are seeds without GAT vector and the genotype is recessive homozygous without GAT element and do not have this high resistance.
16. A method for preventing pollen drift of GAT plants, wherein the vector of claim 3 is transferred into a plant, so that when the pollen of the GAT vector-containing plant material is mature, the GAT vector-containing pollen abortion specifically due to the presence of pollen abortion gene element, while ensuring normal development of GAT carrier-free pollen and dispersing pollen, thus reducing the probability of the GAT vector-containing pollen escaping.
17. A method for preventing drift or intermixing of GAT-containing seeds or plants, wherein subjecting the seeds or plants containing the vector of claim 3, and the material containing the GAT-containing seeds or plants can be killed in a specific period by applying a specific concentration of a herbicide, including bentazone or bensulfuron-methyl or nicosulfuron, by coating at seed time or from a seedling stage to a flowering stage to prevent intermixing of GAT seeds or plants into other common materials.
18. A method for producing sterile line seeds using plant recessive genic male sterile line, wherein the intelligent genetic breeding and seed production system of claim 1 is adopted, the GAT maintainer line and the GAT sterile line are mixed and sowed in a certain ratio, the GAT maintainer line is used to pollinate to the GAT sterile line, and after the pollination is completed, herbicides including bentazone or bensulfuron or nicosulfuron are applied to specifically kill the GAT maintainer line and only the GAT sterile line is reserved for seeds harvesting.
19. A method for purifying a plant recessive genic male sterile line, wherein the intelligent genetic breeding and seed production system of claim 1 is adopted, and the purity of GAT sterile line can be ensured by seed coating or applying a specific concentration of herbicides including bentazone or bensulfuron or nicosulfuron from the seedling stage to the flowering stage.
20. A method for hybrid seed production using a plant recessive genic male sterile line, wherein the intelligent genetic breeding and seed production system of claim 1 is adopted to produce GAT maintainer line seeds and GAT sterile line seeds by self-crossing of the GAT maintainer line; GAT sterile line seeds are produced using GAT maintainer lines pollinated to GAT sterile lines; common commercial hybrids are produced using crosses between GAT sterile lines and conventional material.
21. A method for cross breeding using a plant recessive genic male sterile line, wherein the intelligent genetic breeding and seed production system of claim 1 is adopted, and GAT maintainer line and common materials are used for cross breeding, GAT maintainer lines and sterile lines breeding is by either conventional backcross breeding, or by genealogical breeding, and the breeding process is supplemented by various molecular markers of GAT, herbicide screening, seed color selection, etc. to accelerate selection.
22. A method for preparing a commercial hybrid without GAT element by using the intelligent genetic breeding and seed production system of claim 1, wherein GAT maintainer line is crossed with conventional material A to obtain F1 hybrid, and subsequently F2 can be obtained by self-fertilization, in F2 generation, GAT molecular markers, herbicide screening, seed color selection, etc. are supplemented to select materials containing homozygous recessive genic male sterile sites and GAT elements, high-generation stable materials are obtained through continuous self-fertilization, from which new GAT maintainer lines and GAT sterile lines are obtained, the newly bred GAT sterile lines can be crossed with common restorer lines to breed common commercial hybrids, which do not contain GAT elements and are conventional commercial hybrids.
23. A method for detecting transgenic positive plants containing GAT vector, wherein performing PCR detection on the genome of a sample to be detected using any of the following pairs of primers, the primer sequences for detecting the plant male fertility restoration genetic element expression cassette represented by are represented by SEQ ID NO. 28-29; or the primer sequences for detecting the plant pollen abortion genetic element expression cassette represented by are represented by SEQ ID NO. 30-31; or the molecular primer sequences for detecting the gene transformation and maintainer line screening element expression cassette represented by are represented by SEQ ID NO. 32-33; or the primer sequences for detecting the herbicide-sensitive element expression cassette represented by are represented by SEQ ID NO. 34-35; the molecular primer sequences for detecting the seed screening element expression cassette represented by are represented by SEQ ID NO. 36-37; if SEQ ID NO. 28-29 are used as the primers for amplification, the amplification product is electrophoresed after digestion with HaeIII, and three band types might appear in the final product: 86 bp is the wild-type band type of OsCYP704B2 gene in the original genome, 84 bp is the band type of oscyp704b2-3 mutant, and 66 bp is the band type of GAT vector; if 84 bp and 66 bp band types appear but no 88 bp band type, it indicates that the plant is in a male sterile mutant background and the plant male fertility restoration genetic element expression cassette is present; if primers SEQ ID NO. 30-31 are used for amplification, if a 914 bp band can be amplified, it indicates that the plant pollen abortion genetic element expression cassette is present; if primers SEQ ID NO. 32-33 are used for amplification, if a 831 bp band can be amplified, it indicates that the gene transformation and maintainer line screening element expression cassette is present; if primers SEQ ID NO. 34-35 are used for amplification, if a 923 bp band can be amplified, it indicates that the herbicide-sensitive element expression cassette is present; if primers SEQ ID NO. 36-37 are used for amplification, if a 1412 bp band can be amplified, it indicates that the seed screening element expression cassette is present.
24. A method for sorting plants and progeny with different functions, wherein the GAT vector according to claim 3 is transferred into a plant, and (3) a gene transformation and maintainer line screening element expression cassette, (4) a herbicide-sensitive element expression cassette and (5) a seed screening element expression cassette in the GAT vector are used to sort the plants and progeny with different functions based on a combination of positive and negative bi-directional selection with chemical herbicides and mechanical color selection; the positive and negative bi-directional selection with chemical herbicides being the same plant showing resistance to one herbicide and sensitivity to another herbicide; preferably, the chemical herbicide for positive selection is resistant to bispyribac-sodium, imazethapyr, methomyl, resistant to glyphosate, resistant to glufosinate or glufosinate ammonium, and the chemical herbicide for negative selection is sensitive to bendazone, bensulfuron or nicosulfuron; the mechanical color selection is performed to screen and separate GAT vector-containing seeds or GAT vector-free seeds by different fluorescence of the seeds.
Description
BRIEF DESCRIPTION OF THE DRAWINGS
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DETAILED DESCRIPTION
[0108] The present invention is described in detail below in connection with specific embodiments.
[0109] The following Examples are used to illustrate the present invention, but are not intended to limit the scope of the invention. If not specifically indicated, the technical means used in the Examples are conventional means known to a person skilled in the art, and the raw materials used are commercially available commodities.
Example 1. GAT Vector Construction and Validation
I. Construction of GAT Vector
[0110] The GAT vector was constructed in segments with the expression cassette as the unit, and the unit was assembled. The expression cassette was first constructed on the transition vector pC1300 (
[0111] 1. MCS pC0307 fragment (SEQ ID NO. 38) was synthesized, and Sac II and Pme I were linked into pC1300 to obtain pC0307 (
[0112] 2. MCS pC0308 fragment (SEQ ID NO. 39) was synthesized, and Sac II and Sph I were linked into pC1300 to obtain pC0308 (
[0113] 3. MCS pC0309 fragment (SEQ ID NO. 40) was synthesized, and Sac II and Pme I were linked into pC1300 to obtain pC0309 (
[0114] 4. DNA fragment NSPT-Construct V1.81-Marker 1 was synthesized, and Kpn I+Hind III double digestion were linked into pC1300 to obtain pC1300-Marker 1. The sequence of NSPT-Construct V1.81-Marker 1 consists of Kpn I digestion site ggtacc, MCSI (sequence is represented by SEQ ID NO. 18), herbicide-sensitive element expression cassette Marker 1 (SEQ ID NO. 14), MCSII (SEQ ID NO. 19), the spacer sequence tgcagggacccttgccaac, and the Hind III enzyme cut site aagctt linked in sequence. The sequence of MCSI consists of Pst I, Srf I, Afe I, and Xmn I enzymatic sites linked in sequence. The sequence of herbicide-sensitive element expression cassette Marker 1 consists of NosT terminator, an RNAi stem-loop structural sequence of cytochrome P450 gene CYP81A6, and ZmUbiP promoter linked in sequence. The RNAi stem-loop structural sequence of cytochrome P450 gene CYP81A6 consists of a reverse stem sequence composed of a CYP81A6 coding region, a loop sequence composed of a rice intron, and a forward stem sequence complementary to the CYP81A6 coding region linked in sequence. The sequence of MCSII consists of Hpa I, PshA I, BspE I, Pac I enzyme cleavage sites linked in sequence.
[0115] 5. The DNA fragment NSPT-Construct V1.9-Marker 2 was synthesized, and EcoR I+Hind III double digestion was linked into pC1300 to obtain pC1300-Marker 2. The sequence of NSPT-Construct V1.9-Marker 2 consisted of EcoR I enzyme cut site gaattc, Pst I digest site ctgcag, spacer sequence ggacccttgccaaca, polyclonal site MCSII (sequence is represented by SEQ ID NO. 19), gene transformation and maintainer line screening element expression cassette Marker 2 (SEQ ID NO. 10), MCSIII (SEQ ID NO. 20), spacer sequence tgcagtcccaaggcttccg, and the Hind III digestion site aagctt linked in sequence. The sequence of MCSII consists of Hpa I, PshA I, BspE I, Pac I enzymatic sites linked in sequence, the sequence of gene transformation and maintainer line screening element expression cassette Marker 2 consists of NosT terminator, ALS gene coding region sequence OsALSm1, ActinP promoter linked in sequence, and the sequence of MCSIII consists of BsrG I, Bae I, AsiS I, and FspAI enzyme cut sites linked in sequence.
[0116] 6. DNA fragment NSPT-Construct V1.81-Complementation was synthesized, and Sac I+Hind III double digestion was linked into pC1300 to obatin pC1300-Complementation. The sequence of NSPT-Construct V1.81-Complementation consists of Sac I digest site gagctc, Pst I digest site ctgcag, spacer sequence tcccaaggcttccga, polyclonal site MCSIII (SEQ ID NO. 20), plant male fertility restoration genetic element expression cassette Complementation (SEQ ID NO. 6), MCSIV (SEQ ID NO. 21), spacer sequence tgcagcctgttgccaggga, and Hind III enzyme cleavage site aagctt linked in sequence. The sequence of MCSIII consists of BsrG I, Bae I, AsiS I, and FspA I enzymatic cut sites linked in sequence. The plant male fertility restoration gene element expression cassette Complementation consisted of the 1112 bp sequence upstream of the rice OsCYP704B2 gene start codon ATG, the codon optimized OsCYP704B2 gene coding region, and the 274 bp sequence downstream of the OsCYP704B2 gene stop codon TGA. The sequence of MCSIV consists of Swa I, BstB I, Mlu I, and Rsr II enzyme cleavage sites linked in sequence.
[0117] 7. DNA fragment NSPT-Construct V1.81-Killer was synthesized, and Nde I+EcoR V double digestion was linked into pUC57-Simple to obtain pUC57-Simple. The sequence of NSPT-Construct V1.81-Killer consists of Nde I enzyme cut site catatg, spacer sequence cagggacccttgccaaca, Nru I digest site tcgcga, Pac I digest site ttaattaa, Pst I digest site ctgcag, spacer sequence cctgttgccagggaa, polyclonal site MCSIV (SEQ ID NO. 21), plant pollen abortive genetic element expression cassette Killer (SEQ ID NO. 7), spacer sequence tcgacgcggccgatcccccgg, Stu I digest site aggcct, Sac I digest site gagctc, polyclonal site MCSV (SEQ ID NO. 22), spacer sequence tggcactggccgtcgtttt, Hind III enzyme cut site aagctt, EcoR I enzyme cut site gaattc, and the spacer sequence gggcgcgccccca linked in sequence. The sequence of MCSIV consists of Swa I, BstB I, Mlu I, and Rsr II enzymatic sites linked in sequence. The plant pollen abortion genetic element expression cassette Killer consists of promoter PG47, Zm-AA1 coding region and terminator IN2-1 sequence. The sequence of MCSV consists of Avr II, Pml I, SnaB I, Alo I enzyme cleavage sites linked in sequence.
[0118] 8. pC1300-Marker 1 and pUC57-Simple-Killer were digested with Pac I+Hind III, and the expression cassette Killer was linked into pC1300-Marker 1 to generate pC1300-Marker 1-Killer.
[0119] 9. pC1300-Marker 2 and pC1300-Complementation were digested with BsrG I+Hind III, and the expression cassette Complementation was linked into pC1300-Marker 2 to generate pC1300-Marker 2-Complementation.
[0120] 10. pC1300-Marker 1-Killer and pC1300-Marker 2-Complementation were digested with Pac I+Swa I, and two linked expression cassette Marker 2-Complementation were linked into pC1300-Marker 1-Killer to generate GAT vector pC1300-Marker 1-Marker 2-Complementation-Killer (pC1300-MMCK,
[0121] 11. pC1300-MMCK, pC0308, pC0309 were digested with Pst I+Hind III, and the four linked expression cassette Marker 1-Marker 2-Complementation-Killer were ligated into pC0308 and pC0309 to generate GAT vector pC0308-MMCK (
[0122] 12. DNA fragment Killer 5400 was synthesized, BstB I+Avr II double digestion was linked into pUC57-Simple-Killer, Killer was replaced with expression cassette Killer 5400 to generate pUC57-Simple-Killer 5400. Killer 5400 consists of polyclonal site MCSIV (SEQ ID NO. 21), plant pollen abortion genetic element expression cassetteKiller 5400 (SEQ ID NO. 8), and polyclonal site MCSV (SEQ ID NO. 22) linked in sequence. The plant pollen septic gene component expression cassette Killer 5400 includes PG47 promoter, coding region of rice α-amylase gene OsAA (i.e. 5400) and NosT terminator.
[0123] 13. pUC57-Simple-Killer 5400 and pC0308-MMCK were double digested with Swa I+SnaB I. The expression cassette Killer 5400 and the digested product pC0308-MMC were recovered, and Killer 5400 was linked into pC0308-MMC to generate pC0308-Marker 1-Marker 2-Complementation-Killer5400 (pC0308-MMCK5400).
[0124] 14. DNA fragment Marker 3 ZFN was synthesized, and Pst I+Xma I double digestion was linked into pC0308-MMCK5400 to generate pC0308-Marker 3-Marker 1-Marker 2-Complementation-Killer5400 (pC0308-MMMCK). The sequence of the Marker 3 ZFN fragment consists of Pst I digest site ctgcag, seed screening element expression cassette Marker 3 ZFN (SEQ ID NO. 17), spacer sequence g, and Xma I digest site cccggg linked in sequence. The seed screening element expression cassette Marker 3 ZFN sequentially includes NosT terminator, coding region of the deep red fluorescent protein FP635 gene, and ZZ1P promoter.
[0125] 15. OsALSP fragment (SEQ ID NO. 23) was synthesized, Nco I+BsrG I double digestion was linked into pC1300-NSPT-Construct V1.9-Marker 2 to generate pC1300-Marker 2 AAN. DNA fragment OsUbiT (SEQ ID NO. 24) was synthesized, Pac I+Kpn I double digestion was linked into pC1300-Marker 2 AAN to generate another gene transformation and maintainer line screening element expression cassette Marker 2 AAU (SEQ ID NO. 11) (i.e. the gene transformation and maintainer line screening element expression cassette of the present application), the corresponding vector was pC1300-Marker 2 AAU. Marker 2 AAU expression cassette includes OsUbiT terminator, ALS gene coding region sequence OsALSm1, and OsALSP promoter.
[0126] 16. pC1300-Marker 2 AAU was double digested with Pac I+BsrG I, and Marker 2 AAU expression cassette was recovered. pC0308-MMMCK5400 was double digested with Pac I+BsrG I, and the larger fragment was recovered and linked with Marker 2 AAU to generate GAT vector pC0308-Marker 3-Marker 1-Marker 2aau-Complementation-Killer5400 (pC0308-MMMaauCK5400,
[0127] 17. Vector pC0308-MMaauCK5400 generated in step 16 was double digested with Xma I+BspE I to obtain a smaller fragment Marker 1 and a larger fragment pC0308-M_MaauCK5400. The ends of the above fragments were flattened with high fidelity Taq enzyme and recovered separately. The pC0308-M_MaauCK5400 was self-associated, and then digested with AsiSA I, and the ends were then flattened with high-fidelity Taq enzyme, and then linked with the flat end of the flattened Marker 1 to obtain the transition vector pC0308-Marker 3-Marker 2aau-Marker 1-Complementation-Killer5400 (pC0308-MMaauMCK5400). Marker 1 transcription direction was kept unchanged.
[0128] 18. Killer Hv fragment was synthesized, and the transition vector pC0308-MMaauMCK5400 generated in step 19 was linked with Pst I single digestion to obtain GAT vector pC0308-Killer Hv-Marker 3-Marker 2aau-Marker 1-Complementation-Killer5400 (pC0308-KhvMMaauMCK5400,
[0129] 19. The Killer Hv fragment synthesized in step 20 was double digested with Pst I+Pac I, and Pst I+Pac I were recovered. The transition vector pC0308-MMaauMCK5400 generated in step 19 was double digested with Pst I+Pac I, and the largest fragment of the digested product pC0308-_MaauMCK5400 were recovered. The digested Killer Hv was linked into pC0308-_MaauMCK5400 to obtain the transition vector pC0308-Killer Hv-Marker 2aau-Marker 1-Complementation-Killer5400 (pC0308-KhvMaauMCK5400).
[0130] 20. The transition vector pC0308-MMaauMCK5400 generated in step 19 was double digested with Pst I+Pac I. The smaller fragment Marker 3 ZFN in the digested product was revovered, and flattened with high fidelity Taq enzyme. The transition vector pC0308-KhvMaauMCK5400 obtained in step 21 was digested with Swa I, and linked with the flattened Marker 3 ZFN to obtain the GAT vector pC0308-Killer Hv-Marker 2aau-Marker 1-Complementation-Marker 3-Killer5400 (pC0308-KhvMaauMCMK5400,
[0131] 21. GAT vector pC0308-KhvMaauMCMK5400 obtained in step 22 was double digested with Pst I+SnaB I, and the largest fragment KhvMaauMCMK5400 in the digested product was revovered. pC0309 and pC0307 was double digested with Pst I+SnaB I, respectively, and the linearized pC0309 and pC0307 was revovered. KhvMaauMCMK5400 was linked into pC0309 and pC0307 respectively, to obtain GAT vector pC0309-Killer Hv-Marker 2aau-Marker 1-Complementation-Marker 3-Killer5400 (pC0309-KhvMaauMCMK5400,
II. Validation of the GAT Vector
[0132] The above constructed GAT vectors pC0308-MMMaauCK5400, pC0308-KhvMMaauMCK5400, pC0308-KhvMaauMCMK5400, pC0309-KhvMaauMCMK5400 and pC0307-KhvMaauMCMK5400 were subjected to enzyme digestion and Sequencing verification.
[0133] 1 μl of the above plasmids were mixed with 50 μl of E. coli competent cells, respectively, and transformed by 1.8 KV electroshock. The transformation products were coated on LA plates containing kanamycin and incubated at 37° C. for about 16 h. Single colonies were picked and PCR detection of the bacterial broth was performed using specific primers (
[0142] Kpn I, Hind III and Sma I, Hind III and Pst I, Hind III and Kpn I were selected for enzymatic validation of pC0308-MMaauCK5400, Kpn I, Pst I and Sma I were selected for enzymatic validation of pC0308-KhvMMaauMCK5400, Kpn I, BamH I, Sac I, Sma I, and Bgl II were selected for enzymatic validation of pC0308-KhvMaauMCMK5400, Sac I, Sph I, Kpn I, BamH I, Xho I were selected for enzymatic validation of pC0309-KhvMaauMCMK5400, and Sac I, BamH I, Kpn I were selected for enzymatic validation of pC0307-KhvMaauMCMK5400. The digestion system was 10×Buffer 1 μl, plasmid DNA 3 μl, DNA restriction endonuclease 0.21, and 10 μl was made up with ddH.sub.2O. the digestion conditions were as follows: incubation at 37° C. for 10-15 min, then inactivation at 70° C. for 5 min. The digested products were detected by electrophoresis in 1% agarose gel.
[0143] As shown in
[0144] As shown in
[0145] As shown in
[0146] As shown in
[0147] As shown in
Example 2. Agrobacterium-Mediated Genetic Transformation of Rice with GAT Vector
[0148] 1. Transformation of Agrobacterium tumefaciens with the GAT Vector Constructed in Example 1 and Validation.
[0149] Agrobacterium tumefaciens EHA105 stored at −80° C. was taken and subjected to plate streaking in YEP containing rifampicin (25 μg/ml)+streptomycin (50 μg/ml) at 28° C. A single colony was picked and inoculated in 5 ml of YEP liquid medium containing the above antibiotics, and incubated at 220 rpm for 12 to 16 h at 28° C. 2 ml of bacterial broth were transferred to 100 ml of YEP liquid medium containing the above antibiotics, and incubated at 28° C. and 220 rpm until OD.sub.600=0.5. The resultant was pre-cooled on ice for 10 min, and centrifuged at 4° C., 5000 rpm for 10 min (pre-cooled to 4° C. by frozen centrifuge). The resultant was washed 2 times with sterile deionized water (10 ml each time), 1 time with 10% sterile glycerol, 4° C., centrifuge at 5000 rpm for 10 min, and the bacteria were resuspended in 3 ml of 10% sterile glycerol. 1 μl of the correctly sequenced GAT plasmid pC0308-MMMaauCK5400 obtained in Example 1 were taken and added with 50 μl of Agrobacterium tumefaciens competent cells, the resultant was subjected to 1.8 KV electric shock transformation. The cells were coated on YEP plates containing kanamycin, rifampicin and streptomycin, incubated at 28° C. for about 48 h, and single colonies were picked and shaken overnight.
[0150] Colony PCR validation of pC0308-MMMaauCK5400 transformed Agrobacterium monoclonal was performed using specific primers SEQ ID NO. 30-31 and SEQ ID NO. 34-35 (as in
[0151] 2. Agrobacterium-Mediated Genetic Transformation
[0152] Induction: Seeds from the Zhonghua 11 (ZH11) background and carrying the pure recessive male sterility gene Oscyp704b2-3 were sterilized by sodium hypochlorite and placed on induction medium (N.sub.6+2.4-D 3 mg/L+CH 0.6 g/L+Pro0.5 g/L+Sucrose 30 g/L+Phytagel 3 g/L) and incubated at 28° C. in the dark at room temperature for 30-40d, the obtained induced healing wounds was subjected to secondary culture for 30-40d.
[0153] Screening: The engineered Agrobacterium obtained in the present Example was transformed into the above healing tissue by Agrobacterium-mediated genetic transformation method, and after a total of 3 d of culture, the resultant was washed 5 to 6 times and transferred to a screening medium containing bispyribac-sodium resistance (N.sub.6+2.4-D 2 mg/L+CH 0.6 g/L+Pro0.5 g/L+sucrose 30 g/L+Phytagel 3 g/L+Cn 500 mg/L+bispyribac-sodium 0.3-0.6 μm/L or hygromycin 50 mg/L), and cultured in the dark at 30° C. for 30-50 d to screen for resistant healing.
[0154] Differentiation: resistant healings obtained by screening were transferred to a resistant differentiation medium containing bispyribac-sodium (MS+KT 2 mg/L+NAA 0.5-2 mg/L+sorbitol 20-30 g/L+sucrose 30 g/L+Phytagel 3 g/L+bispyribac-sodium 0.1-0.3 μm/L), and positive seedlings were obtained by differentiation for 25-30 d.
[0155] Rooting: positive seedlings obtained by differentiation were transferred to a rooting medium containing bispyribac-sodium resistance (½ MS+sucrose 20 g/L+paclobutrazol 0.5-1 mg/L+Phytagel 3 g/L+bispyribac-sodium 0.15-0.5 μm/L), and rooted for 7-15 d to finally obtain positive transgenic plants.
[0156] Hardening-seedling and transplanting: the sealing film of the bottle for the transformed strains with vigorous root growth was opened, sterile water was added to cover the medium 1-2 cm high, the resultant was placed in contact with air at room temperature for 2-3 d for hardening-seedling, and then transplanted to the greenhouse for cultivation. A total of 574 GAT transformed lines were obtained from the screening, and 563 plants survived 7-14 days after transplanting. At the time of transplanting GAT transformed lines, a certain number of ZH11 at the period of two leaves and a centre was transplanted as a control.
Example 3. Molecular Identification of GAT T0 Generation Transformed Material
[0157] The leaves of the transgenic plants obtained in Example 2 were taken at the period of five leaves to extract total genomic DNA by CTAB method as follows: 2-4 cm leaves were taken into a mortar, and 800-900 ul of 1.5% CTAB solution were added for grinding, then the ground liquid was transferred into a 1.5 ml centrifuge tube, and placed on ice or in a low-temperature refrigerator to be used. Sample was placed at water bath at 65° C. for 30 min, during which the resultant was inverted several times for mixing well. In a fume hood, chloroform and isoamyl alcohol solution were added with a glass pipette (chloroform:isoamyl alcohol=24:1, i.e., 500 ml chloroform vs 22 ml isoamyl alcohol, the resultant was mixed gently) 650 ul, after mixing well, and the resultant was shaken on a shaker for 30 min or hand shaken for about 10 min, and then obvious stratification can be seen. The shaken sample was centrifuged at 8000-10000 rpm for 8 min; about 400 ul of supernatant was sucked, and transferred to a new centrifuge tube, −20° C. pre-cooled 95% ethanol 800 ul were added and, gently inverted and mixed, the resultant was placed into −20° C. refrigerator for 30 min. The frozen sample at −20° C. was taken, and centrifuged at 12000 rpm for 10 min, the supernatant was removed; 75% ethanol was added, the resultant was stood for about 1 min, and the supernatant was removed, then subjected to air dry; 200-300 ul of sterilized water (ddH.sub.2O) were added, the air-dried sample DNA was dissolved to be used.
[0158] The total DNA of T0 transgenic plants of pC0308-MMMaauCK5400 was subjected to positive assay by PCR using specific primers SEQ ID NO. 30-31 (
[0159] The DNA of T0 transgenic positive plants of pC0308-MMMaauCK540 screened by PCR positive assay above was firstly amplified by PCR with specific primers SEQ ID NO. 28 and SEQ ID NO. 29, and then the amplified products were digested with HaeIII enzyme, and finally detected by 6% SDS-PAGE gel. As shown in
[0160] The amplified regions of the specific primers SEQ ID NO. 28 and SEQ ID NO. 29 contain the cyp704b2-3 mutant variant site, and the presence of a 2-base deletion mutation in cyp704b2-3 mutant background plants can be observed in polyacrylamide gel electrophoresis. The amplified regions of the primers also contain an A.fwdarw.C SNP introduced in the coding region (CDS position 660) of CYP704B2 in the plant male fertility restoration genetic element expression cassette during vector construction. The SNP introduces a HaeIII cleavage site that allows the plant male fertility restoration genetic element expression cassette to be digested by HaeIII, whereas wild-type CYP704B2 cannot be digested by HaeIII. After amplifying the DNA of the trans-GAT vector plants with the above primer pair and subjecting to digestion with HaeIII, there are three possible fragments: 86 bp for the wild-type genotype of rice's own genome, 84 bp for the cyp704b2-3 mutant genotype, and 66 bp for the genotype of the transformed fragment. Plants with a genetic background of cyp704b2-3 pure mutant and containing the GAT vector were identified using the above method.
Example 4 Phenotype Identification of Transformation Materials of GAT T0 Generation
[0161] Herbicide Screening-Phenotype Identification of Bispyribac-Sodium Resistance
[0162] In order to test the working efficiency of screening marker elements in the GAT system, a 600 mg/L bispyribac-sodium solution was prepared with 10% bispyribac-sodium (Nominee, Japan), and 563 GATT0 generation obtained in example 2 and wild-type control ZH11 3 to 5 leaf stage seedlings were sprayed. After spraying, continuous observation was carried out. The leaves of the control ZH11 appeared withered and yellow on the third day after spraying. The control ZH11 appeared withered and yellow and was dying on the seventh day after spraying. Most of the GAT transformants grew normally, and some of them showed yellowing or their growth was inhibited. the control ZH11 had completely died on the 14th day after spraying, but the GAT transformants showed three types of normal growth, growth inhibition and near death or irreversible death. Among them, the normal growth strains were highly resistant to bispyribac-sodium with 184 strains in total, indicating that the working efficiency of screening marker elements in these strains was high; the growth inhibited strains were mediumly resistant to bispyribac-sodium with 163 strains in total, indicating that the working efficiency of screening marker elements in these strains was average; the irreversible death strains or the near-death strains were non-resistant or low resistant to bispyribac-sodium with 216 strains in total, indicating that the working efficiency of screening marker elements in these strains was poor (
[0163] In this experiment, the bispyribac-sodium resistance strains were screened for later screening and differentiation of maintainer and sterile lines, as well as impurity removal and purity maintenance of the maintainer line. In this process, it can be seen that the more functional elements are integrated on a vector, the less likely to have a transformation event where all the corresponding phenotypes of functional elements can be shown, which also confirms the consensus reached in the field at present, that is, the more elements integrated on the same vector, the more difficult to achieve simultaneously consistent traits, that is, the more functional elements, the less likely the expected phenotype occurred in the transformation event. However, in the process of screening the working efficiency of marker elements in the GAT system constructed by the present invention, the inventors screened on each phenotype, and found that the probability of the GAT transformants showing normal growth strains highly resistant to bispyribac-sodium was 32.68%, which was much more than the success rate of transformation events currently integrated with three functional elements or four functional elements in the art. Because in actual transgenic events, the success rate of single trait phenotype is 30% to 50%. Theoretically, for the transformation event integrated with multi-functional element, the probability that all elements meet the expectation should be between 30% to 50% of the N power, and N is the number of functional elements.
[0164] 2. Herbicide Screening—Identification of Bentazon Sensitive Phenotype
[0165] In order to test the working efficiency of herbicide sensitive elements in the GAT system, after the identification of bispyribac-sodium resistance phenotype, a 3 g/L bentazone solution was prepared with 48% bentazone mother liquor (Changzhou Precision Biotechnology Co., Ltd.). The scribed area of plant leaves of surviving GAT T0 generation (347 strains) in the last spraying experiment with bispyribac-sodium and the wild-type control ZH11 were sprayed with the resultant solution, and were continuously observed after spraying. Some GAT transformants T0 had curly and yellow leaf tips on the third day after spraying. From the 7th day to the 14th day after spraying, 144 strains showed irreversible leaf wilt, belonging to highly sensitive strains, indicating that the working efficiency of herbicide sensitive elements in these strains was high; the leaves of 81 strains withered severely at the early stage but gradually recovered, belonging to moderately sensitive strains, indicating that the working efficiency of herbicide sensitive elements in these strains was average; 122 strains had obvious changes before and after being sprayed with bentazone, belonging to low sensitive or non-phenotypic strains, indicating that the working efficiency of herbicide sensitive elements in these strains was poor (
[0166] After spraying the herbicide such as bispyribac-sodium and bentazone, it was observed that there was no significant morphological difference between these GAT transformed strains and the control ZH11, and they continued to grow until flowering for the next experiment.
[0167] 3. Identification of Pollen Fertility
[0168] In order to identify the working efficiency of restoring gene elements and pollen abortion gene elements, the pollen of GAT transformants was tested by iodine staining during flowering to detect pollen fertility of the transformed strains. Because the GAT vector contains the restoring gene element, if the restoring gene elements work normally, the male fertility can be restored. There are two types of pollen (ms/GAT) and (ms/−) produced. Because the (ms/GAT) type of pollen contains the pollen abortion gene element in the GAT vector, if it works normally, the pollen will be aborted, thus only (ms/−) type of pollen will survive. Therefore, if the GAT transformants contains only one copy of the GAT vector, and the restoring gene elements and the pollen abortion gene elements work normally, its pollens were separated that fertile pollen:sterile pollen=1:1.
[0169] Therefore, about 50% of iodine stained fertile pollens are blue black and 50% are sterile pollens without staining. The specific methods of iodine staining microscopy are as follows: [0170] (1) Preparing potassium iodide dye solution (2 g KI was taken and dissolved in 5-10 mL of distilled water, then 1 g I.sub.2 (dissolved with an appropriate amount of absolute ethanol) was added, and after completely dissolving, the distilled water was added to the volume of 300 mL. The resultant was stored in a brown bottle for standby, and was diluted to iodine dye working solution according to the ratio of potassium iodide:deionized water=1:1 during use). [0171] (2) Pollen collection: the fully mature anthers to be scattered was taken and peeled off with the glume, and the anthers were taken out and placed on the slide. [0172] (3) Microscopic examination: about 70 μl iodine dye working solution was dropped on the anther, and the anther was fully crushed with tweezers to release the pollen grains. The cover glass was covered and the pollen grains were observed under a low power microscope. The pollen grains dyed to blue black are fertile pollen grains, while those in light yellow are sterile pollen grains.
[0173] Iodine staining microscopy examination showed that the cyp704b2-3 mutant on the background of Zhonghua 11 had no pollen (Ain
[0174] 4. Fluorescence Identification of Seeds
[0175] There are 26 strains with excellent herbicide phenotype and pollen staining phenotype, as shown in Table 1. The seeds of T0 generation (T1 generation) were harvested by self pollination of the above strains. According to the results of the identification of pollen fertility, if the GAT transformants contains only one copy of the GAT vector, and the restoring gene elements and the pollen abortion gene elements work normally, its self-pollinated seeds will also show 1:1 separation, that is, wherein 50% of the seeds containing the GAT vector (genotype is ms ms/GAT−) will show dark red fluorescence under 560 nm to 595 nm excitation light; 50% of the seeds without GAT vector (genotype: ms ms) showed no fluorescence under 560 nm to 595 nm excitation light. The results showed that the control ZH11 seed had no fluorescence (WT in
TABLE-US-00001 TABLE 1 Summary of fluorescence of T0 generation seed of GAT transformants Total Non- Fluorescence number of Fluorescent fluorescent Theoretical Whether No. Strains intensity seeds seeds seeds value X.sup.2c P 1:1 is met 1 2-1 Weak/none 643 162 481 321.5 158.26 P < 0.05 No 2 2-2 Weak 38 24 14 19 2.66 P > 0.05 Yes 3 11-1 Medium 269 120 149 134.5 3.13 P > 0.05 Yes 4 23-2 Strong 143 74 69 71.5 0.18 P > 0.05 Yes 5 53-3 Strong 70 29 41 35 2.07 P > 0.05 Yes 6 77-2 Strong 428 193 235 214 4.12 P < 0.05 About 7 82-1 None 361 29 332 180.5 254.32 P < 0.05 No 8 83-1 None 511 34 477 255.5 384.05 P < 0.05 No 9 88-4 Strong 582 285 297 291 0.25 P > 0.05 Yes 10 93-2 Strong 339 155 184 169.5 2.48 P > 0.05 Yes 11 95-2 Strong 193 85 108 96.5 2.75 P > 0.05 Yes 12 140-3 None 8 0 8 4 8.13 P < 0.05 No 13 147-3 Strong 15 4 11 7.5 3.33 P > 0.05 Yes 14 150-2 Strong 5 3 2 2.5 0.40 P > 0.05 Yes 15 174-3 Strong 122 58 64 61 0.30 P > 0.05 Yes 16 175-2 Strong 30 15 15 15 0.03 P > 0.05 Yes 17 175-4 Strong 52 24 28 26 0.33 P > 0.05 Yes 18 179-1 Strong 2 2 0 1 2.50 P > 0.05 Yes 19 180-2 None 43 0 43 21.5 43.02 P < 0.05 No 20 180-3 None 33 0 33 16.5 33.03 P < 0.05 No 21 2 Weak/none 286 20 266 143 211.60 P < 0.05 No 22 4 Strong 99 53 46 49.5 0.51 P > 0.05 Yes 23 7 Strong 86 42 44 43 0.06 P > 0.05 Yes 24 20 Strong 181 86 95 90.5 0.45 P > 0.05 Yes 25 23 Strong 225 114 111 112.5 0.04 P > 0.05 Yes 26 28 Strong 177 80 97 88.5 1.64 P > 0.05 Yes
[0176] 5. Identification of Fertility and Screening and Separation of Recessive Nuclear Male Sterile Line and Maintainer Line
[0177] The fertility of two kinds of seeds (fluorescent seeds and non-fluorescent seeds) of excellent strains obtained in step 4 were observed from germination and transplanting to seedling stage, as shown in
Example 5 Phenotype Identification of Transformation Materials of GAT T1 Generation
[0178] In order to identify the stability and working efficiency of the GAT system in different generations, the following experiments were conducted on 14 strains with more seeds among the 18 excellent strains obtained in T0 generation:
[0179] 1. Herbicide Screening—Validation of Tissue Culture Screening of Bispyribac-Sodium
[0180] In order to identify the working efficiency of screening marker elements in the GAT T1 generation, tissue culture germination was used to screen the T1 generation of key strains and candidate strains. If the GAT vector exists in the genome in the form of a single copy and the pollen abortion gene element works normally, the T1 generation of the strains will show 1:1 separation, that is, 50% of the strains contains the GAT vector, which is resistant to bispyribac-sodium and can germinate normally under the screening pressure of bispyribac-sodium; 50% of them do not contain GAT vector, which was not resistant to bispyribac-sodium, and cannot germinate under the screening pressure of bispyribac-sodium.
[0181] Therefore, ½MS medium+3 μm bispyribac-sodium was prepared for screening the key strains and the candidate strains of GAT, and the germination results were shown in Table 2. Among them, 10 strains accorded with the germination ratio of 1:1; the germination ratio of one strain was close to 1:1, which indicated that the working efficiency of screening marker elements in these 11 strains was normal and the heredity between generations was relatively stable. It also indicated that screening marker elements could effectively distinguish two different types of seeds or seedlings (i.e., GAT sterile lines and GAT maintainer lines) isolated from the inbred progeny of the GAT transformants; the germination ratio of other strains was not consistent, indicating that there might be abnormal working efficiency of elements or unstable heredity between generations.
TABLE-US-00002 TABLE 2 Summary of screening results of BS medium of T0 generation seeds of GAT Key strains The number Non- Theoretical Whether No. Strains of seeds Germination germination value X.sup.2c P 1:1 is met CK ZH11 40 0 40 1 11-1 58 26 32 29 0.64 P > 0.05 Yes 2 23-2 30 19 11 15 2.17 P > 0.05 Yes 3 53-3 19 7 12 9.5 1.37 P > 0.05 Yes 4 77-2 46 29 17 23 3.15 P > 0.05 Yes 5 88-4 62 30 32 31 0.08 P > 0.05 Yes 6 93-2 34 15 19 17 0.50 P > 0.05 Yes 7 95-2 35 10 25 17.5 6.46 P < 0.05 About 8 174-3 15.2 12 3.2 7.6 5.16 P < 0.05 No 9 175-4 27.3 14 13.3 13.65 0.05 P > 0.05 Yes 10 4 45 24 21 22.5 0.22 P > 0.05 Yes 11 7 29 11 18 14.5 1.72 P > 0.05 Yes 12 20 40 10 30 20 10.03 P < 0.05 No 13 23 110 61 49 55 1.32 P > 0.05 Yes 14 28 59 16 43 29.5 12.37 P < 0.05 No
[0182] 2. Herbicide Screening—Identification of Bentazone Phenotype
[0183] In order to identify the working efficiency of herbicide sensitive elements in the T1 generation of the GAT transformants, a 3 g/L bentazone solution was prepared with 48% bentazone mother liquor (Changzhou Precision Biotechnology Co., Ltd.). Some plants in the positive strains screened by bispyribac-sodium in Example 5-1 were sprayed, and continuously observed after spraying. Among them, 6 strains of the bispyribac-sodium resistance strains were highly susceptible to wilt and death on the 14th day after spraying, and showed highly sensitive; in 5 strains, individual plants showed slightly less sensitive, but eventually the individual plants died after a long time; more than half of the two strains have poor individual sensitivity and segregation, indicating that there might be abnormal working efficiency of elements or unstable heredity between generations. See Table 3 and
TABLE-US-00003 TABLE 3 Summary of screening results of bentazone in T1 generation seedlings of GAT key plants Total number of Highly Highly Medium Low No No. Strains plants sprayed sensitive(dead) sensitive ratio sensitivity sensitivity phenotype 1 ZH11 4 0 0/4 0 0 4 2 CK + (P450i2-30) 4 4 4/4 0 0 0 3 11-1 8 8 8/8 0 0 0 4 23-2 12 11 11/12 1 0 0 5 53-3 8 8 8/8 0 0 0 6 77-2 2 2 2/2 0 0 0 7 88-4 13 12 12/13 1 0 0 8 93-2 9 8 8/9 0 1 0 9 95-2 2 2 2/2 0 0 0 10 174-3 10 4 4/10 0 6 0 11 175-4 7 5 5/7 2 0 0 12 4 2 1 1/2 1 0 0 13 7 15 2 2/15 0 13 0 14 20 3 2 2/3 1 0 0 15 23 14 14 14/14 0 0 0 16 28 7 7 7/7 0 0 0
[0184] ZH11 is Resistance Control, CK+(P450i2-30) is the Sensitive Positive Control
[0185] 3. Identification of Pollen Fertility
[0186] In order to identify the working efficiency of pollen abortion gene elements in the T1 generation of the GAT transformants, the pollen of the other half of the strains with good detection efficiency in examples 5-1 and 5-2 were iodine stained at the time of rice flowering to detect the pollen fertility of the GAT transformants. The fertility of T0 generation pollen is the same as that in Example 4. If the GAT vector in T1 generation exists as a single copy in the genome, and the pollen abortion gene elements works normally, the fertile pollen is 1:1 separated from the sterile pollen. For the specific method of iodine staining microscopic examination, refer to example 4-3. The results show that most of the pollens in the control ZH11 can be dyed blue black, which is completely fertile (as shown in B in
TABLE-US-00004 TABLE 4 Identification of pollen fertility of T1 generation plants of GAT transformants The checked number of The number of plants whether is stable No. Strains plants with 1:1 segregation inheritance 1 11-1 6 6 Yes 2 23-2 3 3 Yes 3 53-3 6 6 Yes 4 77-2 10 9 Separation 5 88-4 8 8 Yes 6 93-2 6 6 Yes 7 95-2 7 7 Yes 8 174-3 5 5 Yes 9 175-4 3 3 Yes 10 4 10 7 Separation 11 7 7 7 Yes 12 20 6 3 Separation 13 23 16 14 Separation 14 28 1 1 Yes
[0187] 4. Fluorescence Identification of Seeds
[0188] The fluorescence of the self-pollinated and harvested seeds of the above strains were further tested to test the working efficiency of seed screening elements in the T1 generation of the GAT transformants. The results showed that the seed coat of some seeds in the T1 generation of all strains showed strong dark red fluorescence (GAT in
TABLE-US-00005 TABLE 5 Fluorescence identification of T1 generation seeds of GAT transformants Total The number The number Fluorescence number of fluorescent of non-fluorescent Theoretical Whether No. strains intensity of seeds seeds seeds value X.sup.2c P 1:1 is met 1 11-1 Strong 260 112 148 130 4.99 P < 0.05 About 2 23-2 Strong 167 70 97 112.5 4.37 P < 0.05 About 3 53-3 Strong 310 154 156 155 0.02 P > 0.05 Yes 4 77-2 Strong 422 193 229 211 3.07 P > 0.05 Yes 5 88-4 Strong 409 202 207 204.5 0.06 P > 0.05 Yes 6 93-2 Strong 290 130 160 145 3.11 P > 0.05 Yes 7 95-2 Strong 240 87 153 120 18.15 P < 0.05 No 8 174-3 Strong 122 58 64 61 0.30 P > 0.05 Yes 9 175-4 Strong 52 24 28 26 0.33 P > 0.05 Yes 10 4 Strong 315 107 208 157.5 32.39 P < 0.05 No 11 7 Strong 514 202 312 257 23.54 P < 0.05 No 12 20 Strong 378 155 223 189 12.24 P < 0.05 No 13 23 Strong 525 240 285 262.5 3.86 P > 0.05 Yes 14 28 Strong 108 44 64 54 3.7 0.05 Yes
[0189] Based on the above results, all elements in the T1 generation of the GAT transformants worked normally and the strains with single copy of GAT vector include strains 11-1, 23-2, 53-3, 77-2, 88-4, 93-2, 23 and the like, and strains 95-2, 4, and 175-4 were selected as candidates. The above strains can meet all the requirements of GAT maintainer line and can be used as the excellent initial GAT maintainer line for variety breeding, sterile line and hybrid seed production.
[0190] 5. Identification of Pollen Drift
[0191] The pollen and seed in the excellent initial maintainer line of GAT conformed to the segregation ratio of 1:1, which preliminarily indicated that the working efficiency of the pollen abortion elements in GAT was normal. To further detect whether its pollen escapes, in this example, the rice material of common sterile line was pollinated through the strains of the excellent initial maintainer line of GAT, and it was checked whether the hybrid seed has the resistance to bispyribac-sodium (the method is the same as that in Example 5). If so, the pollen containing GAT escapes; If not, it indicated that the pollen abortion elements in GAT had a good working efficiency and could effectively prevent the transformed pollen containing GAT from escaping. GAT strains (23-2, 88-4) were selected as male parents to pollinate female sterile line 1907, and 221 and 373 hybrid seeds were obtained respectively. After 21 days of screening hybrid seeds with bispyribac-sodium, it was observed that under the medium without screening pressure (½MS), the hybrid seeds germinated normally, while under the medium with screening pressure (½MS+3 uM BS), the hybrid seeds were consistent with non-transgenic ZH11, 9311 and MH63, and could not germinate (see
TABLE-US-00006 TABLE 6 Detection of the escape rate of GAT pollen Survival Total Survival Culture medium Strains number number rate 1/2MS ZH11 190 200 95.00% 9311 188 200 94.00% MH63 193 200 96.50% 23-2(T2) 165 200 82.50% 1907 × 23-2(T1) 8 10 80.00% 88-4(T2) 169 200 84.50% 1907 × 88-4(T1) 9 10 90.00% ZH11 0 200 0.00% 9311 0 200 0.00% MH63 0 200 0.00% 1/2MS + 3uMBS 23-2(T2) 95 200 47.50% 1907 × 23-2(T1) 0 211 0.00% 88-4(T2) 83 200 41.50% 1907×88-4(T1) 0 363 0.00%
[0192] 6. Fertility Identification and Screening and Separation of Recessive Nuclear Male Sterile Line and Maintainer Line
[0193] The two kinds of seeds (fluorescent seeds and non-fluorescent seeds) of excellent strains obtained in step 4 were germinated, transplanted, and the fertility is observed in the seedling stage as shown in
[0194] In conclusion, the results of Examples 1-5 prove that the present application has successfully achieved the reproduction of recessive nuclear male sterile materials and the maintenance of the sterility of recessive nuclear male sterile materials by using the GAT system. In combination with the seed fluorescent color selection system and the functional organic combination of maintainer line screening elements and herbicide sensitive elements, the subsequent GAT maintainer line and sterile line can be used to remove impurities and maintain purity. In the seed stage, vegetative growth stage and reproductive growth stage, the recessive nuclear male sterile seeds/plants (GAT sterile line) and fertile seeds/plants (GAT retention) can be separated. The present application successfully solves the problem of large-scale reproduction and maintenance of recessive genic male sterile, so as to successfully realize the industrialization of recessive nuclear male sterile materials.
Example 6 GAT Sterile Line Transfer
[0195] This example is a recessive nuclear sterile transfer, that is, a GAT sterile line transfer, which replaces the dominant homozygous CYP704B2 in H28B with the mutant recessive homozygous cyp704B2-3, but still retains the remaining H28B traits through backcross transfer, so that the third line maintainer line H28B is finally transferred to GAT sterile line, which is called GAT sterile line transfer.
[0196] Cyp704b2-3 is a rice CYP704B2 gene mutant, which is obtained by replacing the GGG after the 794th base of rice CYP704B2 gene with a T, and the mutation site is located in the third exon (disclosed in Chinese patent CN 105002191 B). The mutant cyp704B2-3 was hybridized, backcrossed and self crossed with the normal fertility receptor, and the cyp704b2-3 gene and genetic background were selected with molecular markers in this process. Finally, the recessive nuclear sterile line with homozygous cyp704b2-3 gene in the background of the target receptor was obtained. H28B (H28B is an approved variety of traditional three line male sterile line, belonging to a three line maintainer line, which is a CYP704B2 locus that is dominant homozygous and does not contain GAT vector elements) was taken as an example, the specific steps of transfer are as follows: [0197] 1. F.sub.1 was obtained by crossing the recipient parent, such as H28B, as male parent with a homozygous mutant containing cyp704b2-3. [0198] 2. BC.sub.1F.sub.1 was obtained by backcrossing F1 as female parent and recipient parent, such as H28B. [0199] 3. BC.sub.1F.sub.1 was planted, cyp704b2-3 genotype was detected by using primer with sequence as SEQ ID NO. 28-29. The heterozygous genotype cyp704b2-3 was selected, that is, plants with 86 bp and 84 bp bands could be amplified at the same time. [0200] 4. a group of genotypes (such as 100, or 200, etc.) were used with polymorphism between the cyp704b2-3 mutant and the recurrent parent genome, and evenly distributed molecular markers (which can be but not limited to SSR, SNP, INDEL, EST, RFLP, AFLP, RAPD, SCAR and other types of markers), the genetic background of the single plant selected in step 3 was identified, plants with high similarity to the recurrent parent genotype (such as greater than 88% similarity, or 2% selection rate, etc.) were selected. [0201] 5. BC.sub.2F.sub.1 was obtained by backcrossing the plant selected in step 4 with the recipient parent, such as H28B. [0202] 6. BC.sub.2F.sub.1 was planted and steps 3 and 4 were repeated to select the plants with cyp704b2-3 genotype heterozygosity and high genetic background recovery rate (such as more than 98%, or 2% of the selection rate), and receive inbred BC.sub.2F.sub.2. [0203] 7. BC.sub.2F.sub.2 was planted and steps 3 and 4 were repeated to select the plant with cyp704b2-3 genotype heterozygosity and the highest homozygous rate of genetic background and receive inbred BC.sub.2F.sub.3.
[0204] The homozygous plants of cyp704b2-3, namely, cyp704b2-3 recessive nuclear sterile line, were isolated from BC.sub.2F.sub.3 offspring. BC.sub.2F.sub.3 was used to preserve the germplasm resources of cyp704b2-3 recessive nuclear sterile line. The letter G is used to name the recessive nuclear sterile line, for example, the homozygous recessive nuclear sterile line cyp704b2-3 of H28B in this example is named H28G.
[0205] Only H28B was taken as an example of transfer above, but not limited to H28B, which can be any rice material.
Example 7 GAT Maintainer Line Transfer
[0206] This example reflects the acquisition of a GAT maintainer line, that is, cyp704B2-3 containing GAT vector elements is obtained, but other traits retain the original traits of the donor. For example, H28B (H28B itself is a CYP704B2 dominant homozygous genotype and does not contain GAT vector elements) was used, through continuous backcross breeding with H28B and molecular marker assisted selection, other traits obtained are the same as H28B, but cyp704B2-3 is recessively homozygous and contains GAT vector elements, the resultant was named H28T. The process is called GAT maintainer line transfer.
[0207] The homozygous mutation at CYP704B2 site was selected from the transgenic plants of the GAT large vector obtained in Example 4, and the detection of the GAT transgenic PCR positive was positive. The plants with phenotypes controlled by each GAT element were used as the donor parents for the transformation of the GAT maintainer line. Cyp704b2-3 heterozygous plants obtained in Example 6, such as H28G heterozygous plants, were selected as recipient parents. The donor plants and recipient plants were hybridized, backcrossed and self crossed, and the cyp704b2-3 gene, GAT elements and genetic background were selected with molecular markers in this process. Finally, the GAT maintainer line with homozygous cyp704b2-3 gene and GAT elements in H28B background was obtained. The specific implementation steps are as follows: [0208] 1. F.sub.1 was obtained by hybridization between donor parents and cyp704b2-3 heterozygous genotype receptor parents, such as H28G of cyp704b2-3 heterozygous genotype. [0209] 2. BC.sub.1F.sub.1 was obtained by backcrossing F.sub.1 with cyp704b2-3 heterozygous receptor parent, such as cyp704b2-3 heterozygous H28G. [0210] 3. BC.sub.1F.sub.1 was planted, PCR amplification of the genomic DNA of BC1F1 plant was conducted by using primer with sequence as SEQ ID NO. 28-29, and then the amplified product was digested with HaeIII enzyme, and the genotype of the plant was determined according to the bands of the enzyme digestion product. Plants with 84 bp and 66 bp bands, i.e., plants with cyp704b2-3 gene and GAT transgene were selected. [0211] 4. a group of genotypes (such as 100, or 200, etc.) were used with polymorphism between the cyp704b2-3 mutant and the recurrent parent genome, and evenly distributed molecular markers (which can be but not limited to SSR, SNP, INDEL, EST, RFLP, AFLP, RAPD, SCAR and other types of markers), the genetic background of the single plant selected in step 3 was identified, plants with high similarity to the recurrent parent genotype (such as greater than 88% similarity, or 2% selection rate, etc.) were selected. [0212] 5. BC.sub.2F.sub.1 was obtained by backcrossing the plants selected in step 4 with cyp704b2-3 heterozygous receptor parents, such as cyp704b2-3 heterozygous H28G. [0213] 6. BC.sub.2F.sub.1 was planted and steps 3 and 4 were repeated to select the plants with high genetic background recovery rate (such as more than 98%, or 2% selection rate, etc.), and receive inbred BC.sub.2F.sub.2. [0214] 7. BC.sub.2F.sub.2 was planted and steps 3 and 4 were repeated to select the plant with the highest homozygous rate of genetic background, and receive the inbred BC.sub.2F.sub.3, namely the GAT maintainer line. The letter T is used to name the GAT maintainer line, for example, the GAT maintainer line of H28G in this example is named H28T.
[0215] Only H28B was taken as an example of transfer above, but not limited to H28B, which can be any rice material.
Example 8 GAT Maintenance Line Production
[0216] The seeds of the GAT maintainer line were planted in the legal transgenic area, and the seeds were harvested by self pollination. The seeds with dark red fluorescence were obtained by screening with the fluorescent seed sorter, which were the seeds of the GAT maintainer line. Later, the seeds can be used for the self-reproduction of the GAT maintainer line or pollination to the GAT sterile line for the seed production of the sterile line.
Example 9 Impurity Removal and Purity Maintenance of GAT Maintainer Line
[0217] GAT maintainer line is sown, and 30 to 90 mg/m.sup.2 of bispyribac-sodiumor 50 to 100 mg/L of methomyl or 185 to 750 mg/L of imazethapyr was sprayed at seedling stage to remove impurities and maintain purity; 60-120 mg/m.sup.2 of bispyribac-sodium or 100 to 200 mg/L of methomyl or 500 to 1500 mg/L of imazethapyr was sprayed from tillering stage to booting stage to remove impurities and maintain purity; 120 to 300 mg/m.sup.2 of bispyribac-sodium or 200 to 750 mg/L of methomyl or 1000 to 3000 mg/L of imazethapyr at flowering stage to remove impurities and maintain purity; the herbicide mentioned above was sprayed, which can not only kill the non-GAT maintainer line materials, but also help to weed in the field. It plays an important role in the production of maintainer line and in impurity removal and purity maintenance, killing two birds with one stone.
Example 10 Production of GAT Sterile Line (1)
[0218] The seeds of the GAT maintainer line were planted in the legal transgenic area, and the seeds were harvested by self pollination. The seeds without fluorescence were obtained by screening with the fluorescent seed sorter, which were the seeds of the GAT sterile line. Later, the seeds can be used as the female parent for seed production with other varieties (male parents), and can also be used to reproduce the GAT male sterile line.
Example 11 Production of GAT Sterile Line (2)
[0219] The seeds of the GAT sterile line obtained from example 10 were mixed or interspersed with the seeds of the GAT maintainer line to the statutory transgenic area. When the flowering period came, the GAT maintainer line would disperse powder to seed the GAT sterile line. After the powder was dispersed, the GAT maintainer line was killed by spraying 1 to 3 g/m.sup.2 bentazone or 500 to 3000 mg/L bensulfuron, and all seeds were harvested. Fluorescent seed sorters were used to screen and obtain non-fluorescent seeds, that is, the seeds of the GAT sterile line. Later, it can be used for seed production with other varieties as male parent, and can also be used for breeding sterile line.
Example 12 Impurity Removal and Purity Maintenance of GAT Sterile Line
[0220] GAT sterile line was sown, and 0.1 to 1 g/m.sup.2 bentazone or 100 to 800 mg/L bensulfuron was sprayed at seedling stage to remove impurities and maintain purity; 0.5 to 1.5 g/m.sup.2 bentazone or 500 to 2000 mg/L bensulfuron was sprayed from tillering stage to booting stage to remove impurities and maintain purity; 1 to 3 g/m.sup.2 bentazone or 500 to 3000 mg/L bensulfuron was sprayed at flowering stage to remove impurities and maintain purity; the herbicide mentioned above was sprayed, which can not only kill the GAT maintainer line materials to maintain the purity of the GAT sterile line, but also help to weed in the field, killing two birds with one stone.
Example 13 GAT Hybrid Production
[0221] The GAT sterile line obtained in examples 10 and 11 was crossed with the male parent for seed production, and the seeds on the sterile line were harvested after pollination, all of which were non-transgenic hybrid seeds.
INDUSTRIAL APPLICABILITY
[0222] The present invention provides an intelligent genetic breeding and seed production system for crop cross breeding and hybrid seed production, and application thereof. The system of the present invention contains GAT system vector, which includes five functional element expression cassettes: a plant male fertility restoration genetic element expression cassette, used for restoring the male fertility of a recessive genic male sterile mutant; a plant pollen abortion genetic element expression cassette, used for clearing GAT containing pollen and maintaining a heterozygous state or a hemizygous state of a GAT maintainer line; a chemical herbicide positive selection expression cassette, used for gene transformation and impurity removal and purification for the GAT maintainer line; a chemical herbicide negative selection expression cassette, used for clearing pollen and seed escape of a herbicide-sensitive GAT maintainer line and impurity removal and purification for a GAT sterile line; and a seed screening element expression cassette, used for mechanical sorting of seeds. The method can be used for cross breeding and hybrid seed production of plant recessive genic male sterile materials, thereby obtaining new varieties of plants having high quality, high yield, wide adaptability and high resistance, and seeds thereof, and has good economic value and application prospects.