CN106480047A - Recombinant nucleic acid fragment RecCR020325 and its detection method - Google Patents
Recombinant nucleic acid fragment RecCR020325 and its detection method Download PDFInfo
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Abstract
This application provides recombinant nucleic acid fragment and its detection method.The selection of the rice plant containing recombinant nucleic acid fragment that the application provides, carries out foreground selection and Foreground selection using molecular marker to restructuring plant, obtains the rice plant containing recombinant nucleic acid fragment.
Description
Technical field
The application is related to full-length genome selection and use technology.Specifically, the application relates to the use of
Full-length genome selection and use technology selection-breeding contains the rice plant of recombinant nucleic acid fragment, and thus
And the recombinant nucleic acid fragment obtaining and its detection method.
Background technology
Brown paddy plant hopper, scientific name Nilaparvata lugens (), belong to Homoptera, Delphacidae.Brown
Plant hopper is monophagy insect, only takes food Oryza sativa L., has happiness temperature, cold tolerance is weak, growth cycle
Short, migrate at a distance, the feature such as fulminant and wildness.Brown paddy plant hopper is typical pierce-suck type evil
Worm, is made a living with taking food phloem and xylem sap, and food ingestion is big, breeding is fast, once producing shockingly
Send out, No kernels or seeds are gathered, as in a year of scarcity can to cause damage area.Further, it is also possible to propagate Virus Diseases of Rice (such as:
Grass-like bushy stunt and tingia dwarf wilt), serious harm is also resulted in Rice Production.
Since the eighties in 20th century, from wild rice and cultivated rice identified more than 30
Individual brown planthopper resistant site.Due to the complexity of brown paddy plant hopper phenotypic evaluation, lead to just clone in recent years
The Individual genes such as Bph14, Bph26 and Bph3 (Du etc., PNAS.2009,106 (52):
22163-22168;Tamura etc., Sci Rep.2014,4:5872;Liu etc., Nature
Biotechnology.2015,33:301-305).In addition, producing with brown planthopper resistant kind
In continuous utilization, brown paddy plant hopper gradually strengthens to the adaptability of kind.Some are wide on producing
The resistant variety of general utilization is just gradually losing (Deen etc., the Rice Genet of the resistance to brown paddy plant hopper
Newsl.2010,25:70-72).At present, brown paddy plant hopper preventing and treating still relies upon chemical pesticide, not only increases
Plus production cost, pollute environment, and promote brown paddy plant hopper Drug resistance to strengthen.
As can be seen here, the cultivation demand of brown planthopper resistant new varieties is very urgent.
Content of the invention
On the one hand, this application provides recombinant nucleic acid fragment, it is selected from:I) comprise SEQ ID
NO:The sequence of the nucleotide of sequence 216-663 position shown in 1 or its fragment or its variant or its complementary sequence
Row;Ii) comprise SEQ ID NO:The sequence of sequence shown in 1 or its fragment or its variant or it is mutual
Complementary series;Iii) comprise SEQ ID NO:The sequence of the nucleotide of sequence 636-888 position shown in 2 or
Its fragment or its variant or its complementary series;Or iv) comprise SEQ ID NO:Sequence shown in 2
Sequence or its fragment or its variant or its complementary series;And the combination of above fragment.Real one
Apply in scheme, described recombinant nucleic acid fragment is genome recombination nucleic acid fragment.
Additionally, this application provides detecting the primer of described recombinant nucleic acid fragment, it is selected from:(I) special
Opposite sex identification SEQ ID NO:The forward primer of sequence of the nucleotide of sequence 1-216 position shown in 1 and
Specific recognition SEQ ID NO:Reversely the drawing of the sequence of the nucleotide of sequence 663-854 position shown in 1
Thing;(II) the combining of first group of primer pair and second group of primer pair below, it comprises first group of (a)
Primer pair:Specific recognition SEQ ID NO:The sequence of the nucleotide of sequence 1-216 position shown in 1
Forward primer and specific recognition SEQ ID NO:The nucleotide of sequence 217-662 position shown in 1
Sequence reverse primer;(b) second group of primer pair:Specific recognition SEQ ID NO:1
The forward primer of sequence of shown sequence 217-662 position nucleotide and specific recognition SEQ ID
NO:The reverse primer of the sequence of the nucleotide of sequence 663-854 position shown in 1;(III) specificity
Identification comprises SEQ ID NO:The forward direction of the sequence of the nucleotide of sequence 216-217 position shown in 1 is drawn
Thing and specific recognition comprise SEQ ID NO:The sequence of the nucleotide of sequence 662-663 position shown in 1
The reverse primer of row;(IV) specific recognition comprises SEQ ID NO:Sequence shown in 1
The forward primer of sequence of 216-217 position nucleotide and specific recognition SEQ ID NO:Shown in 1
The reverse primer of the sequence of sequence 663-854 position nucleotide;(V) specific recognition SEQ ID
NO:The forward primer of sequence of the nucleotide of sequence 1-216 position shown in 1 and specific recognition bag
The NO of ID containing SEQ:The reverse primer of the sequence of the nucleotide of sequence 662-663 position shown in 1;With
/ or optionally, (VI) specific recognition SEQ ID NO:The nucleotide of sequence 1-636 position shown in 2
The forward primer of sequence and specific recognition SEQ ID NO:Sequence 888-1050 position shown in 2
The reverse primer of the sequence of nucleotide;(VII) the 3rd group of primer pair and the 4th group of primer pair below
Combination, it comprises (c) the 3rd group of primer pair:Specific recognition SEQ ID NO:Sequence shown in 2
Arrange the forward primer of sequence and the specific recognition SEQ ID NO of 1-636 position nucleotide:2 institutes
Show the reverse primer of the sequence of sequence 637-887 position nucleotide;(d) the 4th group of primer pair:
Specific recognition SEQ ID NO:The forward direction of the sequence of the nucleotide of sequence 637-887 position shown in 2
Primer and specific recognition SEQ ID NO:The sequence of the nucleotide of sequence 888-1050 position shown in 2
The reverse primer of row;(VIII) specific recognition comprises SEQ ID NO:Sequence shown in 2
The forward primer of sequence of 636-637 position nucleotide and specific recognition comprise SEQ ID NO:2
The reverse primer of the sequence of shown sequence 887-888 position nucleotide;(IX) specific recognition bag
The NO of ID containing SEQ:The forward primer of sequence of the nucleotide of sequence 636-637 position shown in 2 and spy
Opposite sex identification SEQ ID NO:The sequence of the nucleotide of sequence 888-1050 position shown in 2 reverse
Primer;(X) specific recognition SEQ ID NO:The sequence of the nucleotide of sequence 1-636 position shown in 2
The forward primer of row and specific recognition comprise SEQ ID NO:Sequence 887-888 position shown in 2
The reverse primer of the sequence of nucleotide.
In one embodiment, for expanding SEQ ID NO:The primer pair of sequence shown in 1 is,
For example, 5 '-ATGATTATGTTCGTCTGCCTGATG-3 ', and 5 '-TCAACGTACC
GCGTAGACACTACA-3’.For detecting SEQ ID NO:The sequencing of sequence shown in 1 is drawn
Thing is, for example, 5 '-CGAGGGCGTATGAGGAGGAA-3 ';With 5 '-TCAACGTA
CCGCGTAGACACTACA-3’.
In another embodiment, for expanding SEQ ID NO:The primer pair of sequence shown in 2
For, for example, 5 '-GCCATCAGCCTGTCCAATAC-3 ', and 5 '-CAAGGCCAA
CGGAACTAACT-3’.For detecting SEQ ID NO:The sequencing primer of sequence shown in 2 is,
For example, 5 '-GCCATCAGCCTGTCCAATAC-3 ';5’-GAGATGCCGACATG
AGTGGT-3’;With 5 '-CACTACTAAGGTCCCGTTCT-3 '.
On the other hand, this application provides selection-breeding contains the side of the rice plant of recombinant nucleic acid fragment
Method, it includes using the Oryza sativa L. recipient plant parent without genes of interest group fragment as recurrent parent,
It is hybridized with the Oryza sativa L. donor plant containing genes of interest group fragment, then will be obtained
Cenospecies be returned with recurrent parent, then the step that obtained backcrossing kind is carried out selfing,
Wherein using molecular marker, foreground selection and Foreground selection are carried out to restructuring plant.For example, described
Recombinant nucleic acid fragment is as previously mentioned.
In the above-mentioned methods, for described foreground selection molecular marker be selected from BphC04ID06,
One or more of RM6659 and BphC04S08;And/or utilize Oryza sativa L. full-length genome breeding
Chip carries out described Foreground selection.
In one embodiment, the selection-breeding that the application provides contains brown planthopper resistant gene group recombinant nuclear
The method of the rice plant of acid fragment, it comprises the following steps:1) recurrent parent is planted with donor
Thing is hybridized, and obtained cenospecies and recurrent parent are returned, and obtains first backcross generation,
Using favorable selection labelling BphC04ID06 and negative itemsets labelling RM6659, BphC04S08
It is carried out with the unilateral homologous recombination fragment screening of brown planthopper resistant gene group fragment, and utilizes Oryza sativa L.
Full-length genome breeding chip, such as RICE6K, Foreground selection is carried out to it;2) background is selected to return
Multiple preferably restructuring individual plant (this generation background recovery value is more than 75%) is carried out again with recurrent parent
Backcrossing, is obtained second backcross generation, using favorable selection labelling BphC04ID06, it is detected,
Select the restructuring individual plant containing brown planthopper resistant gene group fragment, then educated using Oryza sativa L. full-length genome
Plant chip, such as RICE6K, Foreground selection is carried out to it;3) select the restructuring that background is replied
Individual plant (this generation background recovery value is more than 87.5%) is returned again with recurrent parent, obtains
Third backcross generation, using favorable selection labelling BphC04ID06 and negative itemsets labelling RM6659,
BphC04S08 carries out the opposite side homologous recombination fragment sieve of brown planthopper resistant gene group fragment to it
Choosing, and utilize Oryza sativa L. full-length genome breeding chip, such as RICE60K, background choosing is carried out to it
Select;And 4) select introgressed segment little, and restructuring individual plant that background is replied (background recovery value surpasses
Cross 93.75%), by the restructuring chosen individual plant selfing once, obtain selfed seed, using positive choosing
Select labelling BphC04ID06 it is detected, and utilize Oryza sativa L. full-length genome breeding chip,
Such as RICE60K, carries out Foreground selection to it, the final acquisition group of brown planthopper resistant gene containing homozygosis
Recombinant nucleic acid fragment and the rice plant of background reply (background recovery value is more than 99%).
In another embodiment, using molecular marker, restructuring plant is carried out adopting during foreground selection
Amplimer, including:For the primer pair of amplifier molecule labelling BphC04ID06, its
Middle forward primer is 5 '-CCTAGCCGTCAGGTTAATAGATCAT-3 ', reverse primer
For 5 '-ACCAGGTCTACTAGCTTTTACGGAG-3 ';For amplifier molecule labelling
The primer pair of RM6659, wherein forward primer are 5 '-TGTGGAGGCTTAGGAAATT
CTGG-3 ', reverse primer is 5 '-TGTGAAACATGCCACGATACTGC-3 ';With
In the primer pair of amplifier molecule labelling BphC04S08, wherein forward primer is 5 '-GAGCGAT
CCATTAGCACGTGACT-3 ', reverse primer is 5 '-GTTTCTAGGTGTTCCCA
ACTCTCCC-3’.
Another aspect, this application provides the method for detection recombinant nucleic acid fragment, it includes basis
Foregoing recombinant nucleic acid fragment design specific primer, is carried out with testing gene group for template
PCR reacts, and the step analyzing pcr amplification product.Specifically, for example, described primer is such as
Front described.Selectively, analyze pcr amplification product using Sanger sequencing.
Specifically, in the method for detection recombinant nucleic acid fragment that the application provides, for expanding
And detection SEQ ID NO:The primer combination of sequence shown in 1 is as follows:Amplimer, including positive
Primer:5 '-ATGATTATGTTCGTCTGCCTGATG-3 ', and reverse primer:
5’-TCAACGTACCGCGTAGACACTACA-3’;Sequencing primer, including forward primer:
5 '-CGAGGGCGTATGAGGAGGAA-3 ', and reverse primer:5’-TCAACGTAC
CGCGTAGACACTACA-3’.Methods described with testing sample genomic DNA as template,
Enter performing PCR amplification using above-mentioned amplimer, then utilize above-mentioned sequencing primer to the expansion obtaining
Volume increase thing is sequenced, if sequencing result and SEQ ID NO:1 sequence is consistent or complementary, then treat
SEQ ID NO is contained in test sample product:Homologous recombination fragment shown in 1.
In addition, the application provide detection recombinant nucleic acid fragment method in, for amplification and
Detection SEQ ID NO:The primer combination of sequence shown in 2 is as follows:Amplimer, draws including forward direction
Thing:5 '-GCCATCAGCCTGTCCAATAC-3 ', and reverse primer:5’-CAAGGCC
AACGGAACTAACT-3’;Sequencing primer, including forward primer:5’-GCCATCAGCCT
GTCCAATAC-3 ', reverse primer:5 '-GAGATGCCGACATGAGTGGT-3 ',
And reverse primer:5’-CACTACTAAGGTCCCGTTCT-3’.Methods described is to treat test sample
Product genomic DNA is template, enters performing PCR amplification using above-mentioned amplimer, then utilizes
Above-mentioned sequencing primer is sequenced to the amplified production obtaining, if sequencing result and SEQ ID
NO:2 sequences are consistent or complementary, then contain SEQ ID NO in testing sample:Homology weight shown in 2
Group fragment.
Determined by detection and in testing sample, contain SEQ ID NO:1 and/or SEQ ID NO:2
The recombinant nucleic acid fragment of shown sequence, you can determine and comprise the restructuring of resistant gene group in testing sample
Nucleic acid fragment.
Additionally, present invention also provides the test kit of detection recombinant nucleic acid fragment, it includes as front
The primer stated.
Further, present invention also provides screening the rice plant containing recombinant nucleic acid fragment or
The method of seed, whether it includes containing as previously mentioned in the genome detect rice plant to be measured
Recombinant nucleic acid fragment step.In one embodiment, to be examined using foregoing primer
Survey and in the genome of rice plant to be measured, whether contain foregoing recombinant nucleic acid fragment.Another
In one embodiment, to be detected to be measured using the method for foregoing detection recombinant nucleic acid fragment
Foregoing recombinant nucleic acid fragment whether is contained in the genome of rice plant.In another enforcement
In scheme, whether to be detected in the genome of rice plant to be measured using foregoing test kit
Containing foregoing recombinant nucleic acid fragment.
It yet still another aspect, this application provides containing the application by what methods described screening obtained
The rice plant of disclosed recombinant nucleic acid fragment or its seed.
What the application provided contains brown planthopper resistant gene based on full-length genome selection and use technology selection-breeding
Group recombinant nucleic acid fragment rice plant method, have quick, accurate, stablize three big features.
Only pass through the transformation of five generations, you can only target gene group fragment is imported acceptor material, and simultaneously
Realize the reply of background.The acceptor material of the application improvement is restorer ' high mountain for widely used three
Extensive 9113 '.Using said method, ' the premise of extensive 9113 ' the original features in high mountain can retained
Under, import resistance gene of brown planthopper group fragment.Further, cenospecies are realized by combo brown
The increasing substantially of plant hopper resistance.The recombinant nucleic acid fragment that the application provides is tight with Brown Planthopper Resistance
Close correlation, can be applied to the cultivation of other kinds as Resistance resource.
Brief description
Fig. 1 is CR020325 Oryza sativa L. RICE60K full-length genome breeding in the embodiment of the present application 1
Chip detection result;Wherein, square frame indicated by abscissa numeral represents 12 dyeing of Oryza sativa L. successively
Body, vertical coordinate numeral is the physical location [with megabasse (Mb) as unit] on rice genome,
Lycoperdon polymorphum Vitt lines represent receptor parent, and ' the extensive 9113 ' genotype in high mountain, black lines represent donor parents
' magnificent 3418B ' genotype, white line represents the consistent i.e. no polymorphic region of two parent genotypes
Section.At in figure rice chromosome black round dot, lines display block is the brown planthopper resistant importing
Genome recombination nucleic acid fragment RecCR020325.
Fig. 2 is RecCR020325 upstream homologous recombination sequencing fragment ratio in the embodiment of the present application 2
To result;Asterisk shown in figure represents identical base in comparison result, and in figure CR020325 is
The new lines obtaining, T005 is that ' high mountain extensive 9113 ', R002 is donor parents ' China to receptor parent
3418B’.
Fig. 3 is RecCR020325 downstream homologous recombination sequencing fragment ratio in the embodiment of the present application 2
To result.
Fig. 4 is the structure of RecCR020325 both sides homologous recombination fragment in the embodiment of the present application 2
Figure;Wherein, (A) is upstream homologous recombination fragment structure figure;(B) it is downstream homologous recombination fragment
Structure chart, top base is donor ' SNP the or InDel labelling of magnificent 3418B ', lower section alkali
Base is receptor ' SNP the or InDel labelling on high mountain extensive 9113 '.Lycoperdon polymorphum Vitt section is from ' high mountain
Extensive 9113 ' genomic segment, black section be from ' magnificent 3418B ' genomic segment,
White section is homologous recombination section, and abscissa is fragment length, with base pairs (bp) is
Unit.
Fig. 5 is CR020325 Brown Planthopper Resistance interior qualification result in the embodiment of the present application 3;
Shown in figure, blade is followed successively by:(A) high sense brown paddy plant hopper kind ' coming No. 1 in platform ';(B) original
Plant ' high mountain extensive 9113 ';(C) new lines CR020325 are improved;(D) donor parents ' magnificent 3418B '.
Specific embodiment
There is provided defined below and method in order to preferably to define the application and to put into practice middle finger in the application
Lead those of ordinary skill in the art.Unless otherwise mentioned, term is according to association area ordinary skill people
The common usage of member understands.
As used herein, " nucleotide sequence " includes being related to the deoxyribose of single-stranded or double-stranded form
Nucleotide or ribonucleotide polymer, and unless otherwise restriction, nucleotide sequence is with 5 ' extremely
3 ' directions are write from left to right, including the known analog (example with natural nucleotide fundamental property
As peptide nucleic acid(PNA)), described analog with naturally occurring nucleotide similar mode and single-stranded core
Acid hybridization.
In some embodiments, the nucleotide sequence of the application can be changed, to enter
Row conserved amino acid replacement.In certain embodiments, can be according to unifacial leaf codon preference
Property is not changed the replacement of aminoacid sequence to the nucleotide sequence of the application, for example, can use
The codon with amino acid sequence for the coding replaced by the codon of monocotyledon preference, and do not change
Become the aminoacid sequence coded by this nucleotide sequence.
Specifically, the application is related to SEQ ID NO:1 or SEQ ID NO:2 is excellent further
Change the nucleotide sequence of gained.The more details of the method are described in Murray etc. (1989)
Nucleic Acids Res.17:477-498.Optimize nucleotide sequence to can be used for improving brown planthopper resistant base
Because organizing expression in Oryza sativa L. for the recombinant nucleic acid fragment.
In some embodiments, the application further relates to SEQ ID NO:1 or SEQ ID NO:2
The variant of shown sequence.In general, the variant of specific nucleotide sequence will be with this specific nucleoside
Acid sequence has at least about 70%, 75%, 80%, 85%, 86%, 87%, 88%, 89%,
90%th, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, 99.5%
Or 99.9% or higher sequence iden, or more complementary seriess.Such variant sequence thereof
Including the interpolation of one or more nucleic acid, disappearance or replacement, corresponding such that it is able to lead to
The interpolation of amino acid residue, remove or replace.By alignment programs known in the art
Determine sequence iden including hybridization technique.The nucleotide sequence variants of embodiment and the application
The difference of sequence may be as few as 1-15 nucleotide, as little as 1-10 (such as 6-10),
As little as 5, as little as 4,3,2 or even 1 nucleotide.
The application further relates to comprise SEQ ID NO:1 or SEQ ID NO:Specific in sequence shown in 2
The sequence in site or its fragment or its variant or its complementary series, for example, comprise SEQ ID NO:1
The sequence of 216-663 position nucleotide of shown sequence or fragment or its variant or its complementary series,
Or comprise SEQ ID NO:The sequence of 636-888 position nucleotide of sequence shown in 2 or fragment or
Its variant or its complementary series.According to the fragment comprising above-mentioned specific site, can be specifically
Identify corresponding SEQ ID NO:1 or SEQ ID NO:Sequence shown in 2.Further, lead to
Cross and identify containing SEQ ID NO:1 or SEQ ID NO:The recombinant nucleic acid piece of sequence shown in 2
Section, you can determine and comprise resistant gene group recombinant nucleic acid fragment in testing sample.
As used herein, " Oryza sativa L. " is any rice plant include can be all with rice breeding
Plant variety.As used herein, " plant " or " plant ", including whole plant, plant cell,
Plant cell tissue cultures that plant organ, plant protoplast, plant can therefrom regenerate,
Complete plant cell in plant callus, vegetation bed and plant or plant part, described plant
Part for example embryo, pollen, ovule, seed, leaf, flower, branch, fruit, cane, root, the tip of a root,
Flower pesticide etc..
Go for any rice varieties needing selection-breeding in the present processes.That is,
Can (i.e. Comprehensive Traits be preferably sent out it is contemplated that having by any improved seeds lacking certain beneficial traits
The kind of exhibition future) it is used as recurrent parent.With another, there are beneficial traits lacking in this receptor
Kind is as donor parents.In the embodiment of the application, using Oryza sativa L. ' high mountain extensive 9113 '
As recurrent parent, using the Oryza sativa L. ' magnificent 3418B ' conduct with good Brown Planthopper Resistance
Donor.
In the selection of restructuring plant provided herein, using molecular marker to restructuring
Plant carries out foreground selection.The reliability of foreground selection depends primarily on labelling and target gene group
The intersegmental chain tightness degree of piece, for improving the accuracy rate of selection, typically uses both sides adjacent simultaneously
Two labellings target gene group fragment is tracked select.
In the embodiment of the application, the foreground selection labelling of employing includes favorable selection labelling
With negative itemsets labelling, wherein, favorable selection labelling is (brown containing resisting away from target gene group fragment
Plant hopper gene) screening in the range of upstream and downstream 50kb (in Oryza sativa L. its genetic distance be 0.2cM)
Pleiomorphism molecular marker.Negative itemsets labelling is away from target gene group fragment upstream and downstream
The pleiomorphism molecular marker of screening in the range of 500kb (its genetic distance is 2cM in Oryza sativa L.).?
In specific embodiments, the favorable selection labelling of optimized Select to use is and target gene pack
The labelling BphC04ID06 of section close linkage, negative itemsets labelling is away from target fragment upstream about
The molecular marker RM6659 of 220kb, and the molecular marker away from target fragment downstream about 360kb
BphC04S08.
In the embodiment of the application, carry out homologous recombination using above-mentioned foreground selection labelling
During detection, the criterion of side or unilateral homologous recombination is BphC04ID06 detection and ' China
The identical banding pattern of 3418B ', and RM6659 or BphC04S08 detection and the ' extensive 9113 ' phases in high mountain
Same banding pattern;The criterion of both sides or bilateral homologous recombination is BphC04ID06 detection and ' China
The identical banding pattern of 3418B ', and RM6659 and BphC04S08 detection and the ' extensive 9113 ' phases in high mountain
Same banding pattern.
In this application, it is possible to use any available chip carries out provided herein
Breeding method in Foreground selection.In preferred embodiments, the applicant can be adopted
Oryza sativa L. full-length genome breeding chip disclosed in Chinese patent application CN102747138A
RICE6K, or the Oryza sativa L. full genome disclosed in PCT international application WO/2014/121419
Group breeding chip RICE60K.Full content in this two parts of application documents is integrally incorporated to be made herein
It is reference.
Following examples are merely to illustrate and the purpose of unrestricted the application scope.If not referring in particular to
Bright, embodiment all according to conventional laboratory conditions, such as Sambrook equimolecular Cloning: A Laboratory Manual
(Sambrook J&Russell DW,Molecular cloning:a laboratory manual,
2001) condition, or according to manufacturer's description suggestion.
Rice plant material information used in this application all can be found in rice in China kind and its
Pedigree data base (http://www.ricedata.cn/variety/index.htm).
The rice genome physical location being previously mentioned in the application is all with reference to the fine genome of Oryza sativa L. Japan
MSU/TIGR annotates the 6.1st edition (http://rice.plantbiology.msu.edu/).
The open SSR molecular marker that the application is previously mentioned can be found in website
http://www.gramene.org/.
Embodiment 1Selection-breeding imports the restructuring plant of brown planthopper resistant gene group fragment
Used in the present embodiment, material is Oryza sativa L. ' high mountain extensive 9113 ' and Oryza sativa L. ' magnificent 3418B '.
' magnificent 3418B ' has good Brown Planthopper Resistance thus it is speculated that possibly No. 4 contaminates for Oryza sativa L.
Colour solid Bph3 (Liu etc., Nature Biotechnology.2015,33:301-305)、QBph4
(Hu etc., Molecular Breeding.2015,35:3) and Bph15 (Yang etc.,
Theoretical and Applied Genetics.2004,110:Gene cluster area 182-191) being located
Pivotal role has been played to the Brown Planthopper Resistance of this material in domain.
In the Breeding Process of restructuring plant, using molecular marker, prospect choosing is carried out to restructuring plant
Select, the foreground selection molecular marker being adopted is screened.The molecular marker portion being used
Divide and derive from website http://www.gramene.org/, partially self designs.Method for designing is,
Annotate the 6.1st edition with reference to the fine genome MSU/TIGR of Oryza sativa L. Japan, download aforementioned zones segment DNA
Sequence.Using SSRLocator software, the SSR site in above-mentioned sequence is scanned.Profit
With Primer Premier 3.0 software to the SSR site design primer searching out, design primer altogether
106 pairs.By the method for PCR, screen above-mentioned primer pair in ' magnificent 3418B ' and ' high mountain is extensive
Polymorphism in 9113 ', finally picks out and has polymorphism, amplification efficiency in two parts of materials
High foreground selection molecular marker, is favorable selection labelling BphC04ID06 and negative sense choosing respectively
Select labelling RM6659, BphC04S08.Expand specifically drawing of above-mentioned molecular marker for PCR
Thing information is shown in Table 1.
Table 1 foreground selection molecular labeling primer information
By ' genomic fragment that in magnificent 3418B ', forementioned gene cluster is located imports to ' high mountain extensive 9113 '
In, detailed process is as follows:
With ' high mountain extensive 9113 ' as recurrent parent, ', magnificent 3418B ' is hybridized for donor parents,
By obtained cenospecies, ' high mountain extensive 9113 ' is returned, and obtains BC with recurrent parent again1F1
Seed, utilizes favorable selection labelling BphC04ID06 and negative itemsets labelling after nursery
RM6659, BphC04S08 carry out Single-plant selection of recombinating, and filter out 13 in target gene group
The individual plant of fragment side homologous recombination, that is, BphC04ID06 detection is with ' magnificent 3418B ' is identical
Banding pattern, and RM6659 or BphC04S08 detection with ' extensive 9113 ' the identical banding patterns in high mountain, and
Using Oryza sativa L. full-length genome breeding chip RICE6K (CN102747138A), background choosing is carried out to it
Select (Yu etc., Plant Biotechnology Journal.2014,12:28-37).
Comparable chip result in the unilateral homologous recombination individual plant of 13 filtering out, selects background to return
Multiple best restructuring individual plant (this generation background recovery value is more than 75%) so as to recurrent parent ' high mountain
Extensive 9113 ' are returned again, obtain BC2F1Seed, utilizes favorable selection labelling after nursery
BphC04ID06 detects to it, selects the restructuring individual plant containing target gene group fragment,
I.e. BphC04ID06 detection is with ' the identical banding pattern of magnificent 3418B ', is educated using Oryza sativa L. full-length genome
Plant chip RICE6K and Foreground selection is carried out to it.
Select background reply preferable individual plant (this generation background recovery value is more than 87.5%) so as to
' high mountain extensive 9113 ' is returned again recurrent parent, obtains BC3F1Seed, profit after nursery
With favorable selection labelling BphC04ID06 and negative indicia RM6659, BphC04S08 to receipts
The seed obtaining carries out the screening of target gene group fragment opposite side homologous recombination fragment, obtains 9
In the individual plant of target fragment both sides restructuring, i.e. BphC04ID06 detection and ' magnificent 3418B ' phase
Same banding pattern, and RM6659 with BphC04S08 detection and ' extensive 9113 ' the identical banding patterns in high mountain.
Using Oryza sativa L. full-length genome breeding chip RICE60K (WO/2014/121419) to above-mentioned 9
Individual bilateral exchanges individual plant and carries out background and target fragment selection (Chen etc., Molecular Plant.
2014,7:541-553), screen importing target fragment less, and the target list that background is replied
One (this generation background recovery value is more than 93.75%) of strain.
By the individual plant selfing chosen once, obtain BC3F2, after nursery, utilize favorable selection labelling
BphC04ID06 detects to it, selects the individual plant containing target gene group fragment, that is,
BphC04ID06 detection is with ' the identical banding pattern of magnificent 3418B ', using Oryza sativa L. full-length genome breeding core
Piece RICE60K carries out Foreground selection to it.
Final acquisition target fragment homozygosis, and background replys the strain of (background recovery value is more than 99%)
It is one, be named as CR020325.Chip detection result is shown in Fig. 1.
Embodiment 2The determination of homologous recombination fragment after importing resistance gene of brown planthopper group fragment
In order to determine the brown planthopper resistant gene group clip size of importing, to ' high mountain extensive 9113 ' is led
The homozygosis individual plant entering brown planthopper resistant gene group fragment has carried out target gene group fragment both sides homology weight
The sequencing of group fragment.By the brown planthopper resistant gene group recombinant nucleic acid fragment life contained by CR020325
Entitled RecCR020325.
Primarily determined that by Oryza sativa L. full-length genome breeding chip RICE60K testing result,
RecCR020325 is located at two SNP marker R0406475020AG and F0406988115GA
Between.
Meanwhile, using Miseq sequencing technologies to ' high mountain extensive 9113 ', ' magnificent 3418B ' and
Tri- samples of CR020325 carry out genome sequencing.Using TruSeq Nano DNA LT Kit
(illumina) test kit carries out library foundation, using Library Quantification Kit
Universal (KAPA Biosystems) test kit carries out quantitation, using MiSeq V2Reagent
Kit (illumina) test kit carries out sequencing reaction.Using the desk-top sequenator of Miseq (illumina)
Detected.Concrete steps and method are referring to each test kit and sequenator operation instructions.
According to aforementioned SNP chip and Miseq sequencing result, by CR020325 brown planthopper resistant base
Because the 6499948bp that group recombinant fragment upstream homologous recombination fragment is positioned at the 4th chromosome arrives
6500808bp is interval, and downstream homologous recombination fragment is positioned 6986399bp to 6987430bp
Interval.
On this basis, annotate the 6.1st edition with reference to the fine genome MSU/TIGR of Oryza sativa L. Japan,
Download respective segments DNA sequence.Using the amplification of Primer Premier 5.0 software design and survey
Sequence primer, design requirement be the long 22nt of primer about, G/C content 40-60% and do not have mispairing.
With receptor parent, ' ' magnificent 3418B ' is for comparison, right for high mountain extensive 9113 ' and donor parents
The upstream and downstream homologous recombination fragment of CR020325 separately designs amplimer, using high-fidelity
Enzyme KOD FX Neo (TOYOBO) is expanded, and is found optimal using two-step method or three-step approach
Amplification condition is it is ensured that amplified production is shown as single bright bar in agarose gel electrophoresiies detection
Band.The upstream homologous recombination fragment amplification primer reaction condition of wherein determination is:94℃2min;
98 DEG C of 10sec, 61 DEG C of 30sec, 68 DEG C of 150sec, 37 circulations;20℃1min.Under
Swimming homologous recombination fragment amplification primer reaction condition is:94℃2min;98 DEG C of 10sec, 60 DEG C
30sec, 68 DEG C of 90sec, 37 circulations;20℃1min.Thus, two are finally filtered out right
Amplimer is respectively used to the amplification of upstream and downstream homologous recombination fragment.
In addition, with amplified production as template, being sequenced using Sanger sequencing, according to reality
Border sequencing effect, finally filters out 2 and 3 sequencing primers are respectively used to upstream and downstream together
The sequencing of source recombinant fragment.
Specific amplimer and sequencing primer sequence are shown in Table 2, and sequencing result is shown in Fig. 2 and Fig. 3.
RecCR020325 upstream homologous recombination sequencing fragment length is 854bp (SEQ ID
NO:1).1-216bp is that ' genomic segment on high mountain extensive 9113 ', with donor ' magnificent 3418B ' for receptor
Relatively, there is 1 SNP, 2 InDel.This 446bp section of 217-662bp is homology
Restructuring section.663-854bp is that ' magnificent 3418B ' genomic fragment, with ' high mountain extensive 9113 ' for donor
Relatively, there are 6 SNP, 1 InDel.
RecCR020325 downstream homologous recombination sequencing fragment length is 1050bp (SEQ ID
NO:2).1-636bp is that ' genomic segment of magnificent 3418B ', with ' high mountain extensive 9113 ' for donor
Relatively, there are 3 SNP, 2 Indel.This 251bp section of 637-887bp is homology
Restructuring section.888-1050bp is that ' genomic segment on high mountain extensive 9113 ', with donor ' China for receptor
3418B ' compares, and there are 7 SNP, 1 Indel.
Fig. 4 is the structure chart of RecCR020325 both sides homologous recombination fragment.Wherein, (A)
For upstream homologous recombination fragment structure figure;(B) it is downstream homologous recombination fragment structure figure.Top alkali
Base is that ' SNP the or InDel labelling of magnificent 3418B ', lower section base is that ' high mountain is extensive for receptor to donor
9113 ' SNP or InDel labelling.Lycoperdon polymorphum Vitt section is from ' extensive 9113 ' the genomes in high mountain
Section, black section is from ' magnificent 3418B ' genomic segment, white section is homology
Restructuring section.Abscissa is fragment length, with base pairs (bp) as unit.
Table 2 brown planthopper resistant gene group recombinant nucleic acid fragment amplification and sequencing primer information
Embodiment 3' high mountain extensive 9113 ' imports the Resistance Identification after brown planthopper resistant gene group fragment
In order to identify the Brown Planthopper Resistance of the plant of fragment containing recombinant nucleic acid selecting, to the application
' high mountain is extensive 9113 ', donor parents ' magnificent 3418B ' for new lines CR020325 of selection-breeding, receptor parent
(as positive control), and high sense brown paddy plant hopper kind ' coming No. 1 in platform ' is (right as feminine gender
According to) carrying out brown paddy plant hopper interior Resistance Identification, authentication method is as follows.
Each part material is soaked seed indoors, accelerating germination, subsequently sowing pulling the plastic cover of grid line
In basin, every part of material divides 3 row to sow 45 plants altogether, when two one heart stages of leaf, often capable reservation 10
Totally 30 plants of consistent plant of healthy growing way are used for connecing worm for strain.Worm sources come since field collect brown
Plant hopper, and captive breeding indoors.Take 2-3 age nymph to plant to be identified, every plant has
5-10 head nymph.When ' coming No. 1 in platform ' dead seedling 95%, start recording respectively identifies Seedling
Resistance class, take the meansigma methodss of the resistance class of 30 young plants, as the resistance class of this material,
Its resistance level is evaluated according to resistance class.Wherein, resistance class is divided into 10 grades:0 or 1 grade,
Blade is not aggrieved or first piece leaf blade tip turns to be yellow;2 grades, first piece leaf 1/2 turns to be yellow or blade tip wrinkle
Contracting;3 grades, first piece leaf turns to be yellow or withered;4 grades, second leaf portion distributes yellow or lobus cardiacus leaf
Point jaundice;5 grades, the jaundice of second leaf, shrinkage or withered, the blue or green volume of lobus cardiacus;6 grades, lobus cardiacus
Curling, lobus cardiacus tip burn on leaf;7 grades, lobus cardiacus curling is withered, and plant is not dead;8 grades, lobus cardiacus
Withered, somewhat lodge;9 grades, whole strain lodging.According to above-mentioned resistance class, 0-0.9 level judges
Resist for high, 1.0-2.9 level is anti-, 3.0-5.9 level is anti-in being, 6.0-6.9 level is middle sense, 7.0-7.9
Level is sense, and 8.0-9.0 level is high sense.
Brown paddy plant hopper interior Resistance Identification result is shown in Fig. 5, wherein ' is coming No. 1 in platform ' and is feeling for high,
' high mountain extensive 9113 ' is sense to original kind, and improvement new lines CR020325 are anti-, donor parents ' China
3418B ' is high anti-.
Although, above with a general description of the specific embodiments the application has been made in detail
Most description, but on the basis of the application, it can be made some modifications or improvements, this is to this
It is obvious for skilled person.Therefore, on the basis without departing from the application spirit
Upper these modifications or improvements, belong to this application claims scope.
Claims (10)
1. recombinant nucleic acid fragment, it is selected from:
I) comprise SEQ ID NO:The sequence of the nucleotide of sequence 216-663 position shown in 1 or its fragment
Or its variant or its complementary series;
Ii) comprise SEQ ID NO:The sequence of sequence shown in 1 or its fragment or its variant or it is mutual
Complementary series;
Iii) comprise SEQ ID NO:The sequence of the nucleotide of sequence 636-888 position shown in 2 or its piece
Section or its variant or its complementary series;
Iv) comprise SEQ ID NO:The sequence of sequence shown in 2 or its fragment or its variant or it is mutual
Complementary series;And
The combination of above fragment.
2. test right requires the primer of fragment described in 1, and wherein said primer is selected from:
(I) specific recognition SEQ ID NO:The sequence of the nucleotide of sequence 1-216 position shown in 1
Forward primer and specific recognition SEQ ID NO:The sequence of the nucleotide of sequence 663-854 position shown in 1
The reverse primer of row;
(II) the combining of first group of primer pair and second group of primer pair below, it comprises
(a) first group of primer pair:Specific recognition SEQ ID NO:Sequence shown in 1
The forward primer of sequence of 1-216 position nucleotide and specific recognition SEQ ID NO:Sequence shown in 1
Arrange the reverse primer of the sequence of 217-662 position nucleotide;With
(b) second group of primer pair:Specific recognition SEQ ID NO:Sequence shown in 1
The forward primer of sequence of 217-662 position nucleotide and specific recognition SEQ ID NO:Shown in 1
The reverse primer of the sequence of sequence 663-854 position nucleotide;
(III) specific recognition comprises SEQ ID NO:The nucleotide of sequence 216-217 position shown in 1
The forward primer of sequence and specific recognition comprise SEQ ID NO:Sequence shown in 1
The reverse primer of the sequence of 662-663 position nucleotide;
(IV) specific recognition comprises SEQ ID NO:The nucleotide of sequence 216-217 position shown in 1
The forward primer of sequence and specific recognition SEQ ID NO:Sequence 663-854 position shown in 1
The reverse primer of the sequence of nucleotide;
(V) specific recognition SEQ ID NO:The sequence of the nucleotide of sequence 1-216 position shown in 1
Forward primer and specific recognition comprise SEQ ID NO:The core of sequence 662-663 position shown in 1
The reverse primer of the sequence of thuja acid;And/or optionally,
(VI) specific recognition SEQ ID NO:The sequence of the nucleotide of sequence 1-636 position shown in 2
Forward primer and specific recognition SEQ ID NO:The nucleotide of sequence 888-1050 position shown in 2
The reverse primer of sequence;
(VII) the combining of the 3rd group of primer pair and the 4th group of primer pair below, it comprises
(c) the 3rd group of primer pair:Specific recognition SEQ ID NO:Sequence shown in 2
The forward primer of sequence of 1-636 position nucleotide and specific recognition SEQ ID NO:Sequence shown in 2
Arrange the reverse primer of the sequence of 637-887 position nucleotide;With
(d) the 4th group of primer pair:Specific recognition SEQ ID NO:Sequence shown in 2
The forward primer of sequence of 637-887 position nucleotide and specific recognition SEQ ID NO:Shown in 2
The reverse primer of the sequence of sequence 888-1050 position nucleotide;
(VIII) specific recognition comprises SEQ ID NO:The nucleoside of sequence 636-637 position shown in 2
The forward primer of sequence of acid and specific recognition comprise SEQ ID NO:Sequence shown in 2
The reverse primer of the sequence of 887-888 position nucleotide;
(IX) specific recognition comprises SEQ ID NO:The nucleotide of sequence 636-637 position shown in 2
The forward primer of sequence and specific recognition SEQ ID NO:Sequence 888-1050 shown in 2
The reverse primer of the sequence of position nucleotide;
(X) specific recognition SEQ ID NO:The sequence of the nucleotide of sequence 1-636 position shown in 2
Forward primer and specific recognition comprise SEQ ID NO:The core of sequence 887-888 position shown in 2
The reverse primer of the sequence of thuja acid.
3. test right requires the primer of fragment described in 1, and wherein said primer is selected from:
(I) expand SEQ ID NO:The primer pair of sequence shown in 1
5 '-ATGATTATGTTCGTCTGCCTGATG-3 ',
5’-TCAACGTACCGCGTAGACACTACA-3’;And
(II) be sequenced SEQ ID NO:The primer of sequence shown in 1
5’-CGAGGGCGTATGAGGAGGAA-3’;
5’-TCAACGTACCGCGTAGACACTACA-3’;And/or optionally,
(III) expand SEQ ID NO:The primer pair of sequence shown in 2
5 '-GCCATCAGCCTGTCCAATAC-3 ',
5’-CAAGGCCAACGGAACTAACT-3’;
(IV) be sequenced SEQ ID NO:The primer of sequence shown in 2
5’-GCCATCAGCCTGTCCAATAC-3’;
5’-GAGATGCCGACATGAGTGGT-3’;
5’-CACTACTAAGGTCCCGTTCT-3’.
4. the method that selection-breeding contains the rice plant of recombinant nucleic acid fragment described in claim 1,
It includes using the Oryza sativa L. recipient plant parent without genes of interest group fragment as recurrent parent, will
It is hybridized with the Oryza sativa L. donor plant containing genes of interest group fragment, then will be obtained
Cenospecies are returned with recurrent parent, then the step that obtained backcrossing kind is carried out selfing,
Wherein using molecular marker, foreground selection and Foreground selection are carried out to restructuring plant.
5. method as claimed in claim 4, is wherein used for the molecular marker of described foreground selection
Selected from one or more of BphC04ID06, RM6659 and BphC04S08;And/or
Optionally, carry out described Foreground selection using Oryza sativa L. full-length genome breeding chip.
6. the method as described in claim 4 or 5, wherein said recombinant nucleic acid fragment contains anti-
Brown paddy plant hopper gene, and the method comprising the steps of:
1) recurrent parent is hybridized with donor plant, by obtained cenospecies and samsara parent
Originally it is returned, obtained first backcross generation, using favorable selection labelling BphC04ID06 and negative sense
Selected marker RM6659, BphC04S08 carries out the one side of brown planthopper resistant gene group fragment to it
Homologous recombination fragment is screened, and carries out Foreground selection using Oryza sativa L. full-length genome breeding chip to it;
2) select background to reply preferably restructuring individual plant to be returned again with recurrent parent, obtain
Second backcross generation, is detected to it using favorable selection labelling BphC04ID06, select containing
The restructuring individual plant of brown planthopper resistant gene group fragment, then utilizes Oryza sativa L. full-length genome breeding chip pair
It carries out Foreground selection;
3) select the restructuring individual plant that background is replied to be returned again with recurrent parent, obtain
Third backcross generation, using favorable selection labelling BphC04ID06 and negative itemsets labelling RM6659,
BphC04S08 carries out the opposite side homologous recombination fragment sieve of brown planthopper resistant gene group fragment to it
Choosing, and using Oryza sativa L. full-length genome breeding chip, Foreground selection is carried out to it;And
4) select introgressed segment little, and the restructuring individual plant that background is replied, by the restructuring chosen list
Strain selfing once, is obtained selfed seed, using favorable selection labelling BphC04ID06, it is carried out
Detection, and using Oryza sativa L. full-length genome breeding chip, Foreground selection is carried out to it, final acquisition contains
Homozygosis brown planthopper resistant gene group heavy nucleus acid fragment and the rice plant of background reply.
7. the method as any one of claim 4 to 6, wherein utilizes molecular marker pair
The amplimer that restructuring plant carries out employing during foreground selection is as follows:
The primer pair of amplifier molecule labelling BphC04ID06, it includes:
Forward primer:5 '-CCTAGCCGTCAGGTTAATAGATCAT-3 ',
Reverse primer:5’-ACCAGGTCTACTAGCTTTTACGGAG-3’;
The primer pair of amplifier molecule labelling RM6659, it includes:
Forward primer:5 '-TGTGGAGGCTTAGGAAATTCTGG-3 ',
Reverse primer:5’-TGTGAAACATGCCACGATACTGC-3’;And
The primer pair of amplifier molecule labelling BphC04S08, it includes:
Forward primer:5 '-GAGCGATCCATTAGCACGTGACT-3 ',
Reverse primer:5’-GTTTCTAGGTGTTCCCAACTCTCCC-3’.
8. the method that test right requires the recombinant nucleic acid fragment described in 1, it includes adopting right
Require the primer described in 2 or 3, performing PCR reaction is entered for template with testing gene group, and analyzes
The step of PCR primer.
9. test right requires the test kit of the recombinant nucleic acid fragment described in 1, and it includes right will
Seek the primer described in 2 or 3.
10. the rice plant containing the recombinant nucleic acid fragment described in claim 1 for the screening or seed
Method, whether it is included detecting in rice plant to be measured or the genome of seed containing has the right will
The step seeking the recombinant nucleic acid fragment described in 1;
Preferably, using the primer described in Claims 2 or 3, or adopt claim 8
Described method, or detected using the test kit described in claim 9.
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