Methods and materials for high throughput testing of transgene combinations
원문보기
IPC분류정보
국가/구분
United States(US) Patent
등록
국제특허분류(IPC7판)
A01H-001/04
C12Q-001/68
C12N-015/82
출원번호
US-0327217
(2014-07-09)
등록번호
US-9101100
(2015-08-11)
발명자
/ 주소
Pennell, Roger I.
Hamilton, Richard
Portereiko, Michael F.
출원인 / 주소
Ceres, Inc.
대리인 / 주소
Fish & Richardson P.C.
인용정보
피인용 횟수 :
0인용 특허 :
61
초록▼
High throughput methods are described for identifying combinations of transgenes that can be used to improve a phenotypic feature in an organism. Large populations of organisms (e.g., plants) containing different combinations of transgenes as well as different promoter-coding sequence combinations c
High throughput methods are described for identifying combinations of transgenes that can be used to improve a phenotypic feature in an organism. Large populations of organisms (e.g., plants) containing different combinations of transgenes as well as different promoter-coding sequence combinations can be assessed using the methods.
대표청구항▼
1. A method for identifying a combination of genetic elements responsible for a desirable phenotype of a plant, wherein said method comprises: (a) selecting at least four target transgenes, wherein each target transgene of said at least four target transgenes comprises a regulatory region comprising
1. A method for identifying a combination of genetic elements responsible for a desirable phenotype of a plant, wherein said method comprises: (a) selecting at least four target transgenes, wherein each target transgene of said at least four target transgenes comprises a regulatory region comprising an upstream activating sequence operably linked to a nucleotide sequence to be expressed, whereby said upstream activating sequence of each of said at least four target transgenes is the same or different;(b) selecting at least two activator transgenes, wherein each activator transgene comprises a plant promoter operably linked to a sequence encoding a chimeric polypeptide comprising a DNA binding domain fused to a transcription activation domain, wherein each DNA binding domain of said at least two chimeric polypeptides binds to the upstream activating sequence comprised within said regulatory region of at least one of said at least four target transgenes;(c) obtaining a first parental plant and a second parental plant, wherein each of said at least four target transgenes and said at least two activator transgenes (i) is individually present in either said first parental plant or said second parental plant, (ii) is unlinked from each of the other of said at least four target transgenes and said at least two activator transgenes that are present within the same said first parental plant or said second parental plant, and (iii) is in a hemizygous state within said first parental plant or said second parental plant;(d) sexually crossing said first parental plant and said second parental plant to produce a population of progeny plants, whereby said population of progeny plants has different combinations of said at least four target transgenes and said at least two activator transgenes;(e) comparing different plants of said population of progeny plants to one another and selecting at least one progeny plant from said population as having said desirable phenotype to obtain a selected progeny plant; and(f) determining which target transgenes and activator transgenes are present within said selected progeny plant, thereby identifying a combination of genetic elements responsible for said desirable phenotype of a plant. 2. The method of claim 1, wherein at least one of said nucleotide sequences to be expressed is a nucleotide sequence encoding a dominant negative polypeptide. 3. The method of claim 1, wherein said first parental plant comprises said at least four target transgenes, and said second parental plant comprises said at least two activator transgenes. 4. The method of claim 1, wherein said chimeric polypeptide encoded by each of said at least two activator transgenes is the same. 5. The method of claim 1, wherein said upstream activating sequence of each of said at least four target transgenes is the same. 6. The method of claim 1, wherein said plant promoter of each of said at least two activator transgenes is different. 7. The method of claim 1, wherein said method further comprises, after said step (f): (a1) selecting at least four target transgenes, wherein each target transgene of said at least four target transgenes comprises a regulatory region comprising an upstream activating sequence operably linked to a nucleotide sequence to be expressed, and wherein said selected at least four target transgenes includes said target transgenes determined to be present within said selected progeny plant in step (f), and whereby said upstream activating sequence of each of said at least four target trans genes is the same or different;(b1) selecting at least two activator transgenes, wherein each activator transgene comprises a plant promoter operably linked to a sequence encoding a chimeric polypeptide comprising a DNA binding domain fused to a transcription activation domain, wherein each DNA binding domain of said at least two chimeric polypeptides binds to the upstream activating sequence comprised within said regulatory region of at least one of said at least four target transgenes, and wherein said selected at least two activator transgenes includes said activator transgenes determined to be present within said selected progeny plant in step (f);(c1) obtaining a third parental plant and a fourth parental plant, wherein each of said at least four target transgenes of said step (a1) and said at least two activator transgenes of said step (b1) (i) individually present in either said third parental plant or said fourth parental plant, (ii) is unlinked from each of the other of said at least four target trans genes and said at least two activator trans genes that are present within the same said third parental plant or said fourth parental plant, and (iii) is in a hemizygous state within said third parental plant or said fourth parental plant;(d1) sexually crossing said third parental plant and said fourth parental plant to produce a second population of progeny plants, whereby said second population of progeny plants has different combinations of said at least four target transgenes of step (a1) and said at least two activator transgenes of step (b1);(e1) comparing different plants of said second population of progeny plants to one another and selecting at least one progeny plant from said second population as having a desirable phenotype to obtain a second selected progeny plant; and(f1) determining which target transgenes and activator transgenes are present within said second selected progeny plant, thereby identifying a combination of genetic elements responsible for a desirable phenotype of a plant. 8. The method of claim 1, wherein said first parental plant and said second parental plant are selected from the group consisting of Zea mays, Sorghum bicolor, Triticum aestivum, and Oryza sativa. 9. The method of claim 1, wherein said first parental plant or said second parental plant is cytoplasmically male sterile. 10. The method of claim 1, wherein said selecting of step (e) is based at least in part on results under field testing conditions. 11. The method of claim 1, wherein said first parental plant and said second parental plant belong to distinct heterotic groups. 12. A method for making a collection of seeds, wherein said method comprises: (a) selecting at least four target transgenes, wherein each target transgene of said at least four target transgenes comprises a regulatory region comprising an upstream activating sequence operably linked to a nucleotide sequence to be expressed, whereby said upstream activating sequence of each of said at least four target transgenes is the same or different;(b) selecting at least two activator transgenes, wherein each activator transgene comprises a plant promoter operably linked to a sequence encoding a chimeric polypeptide comprising a DNA binding domain fused to a transcription activation domain, wherein each DNA binding domain of said at least two chimeric polypeptides binds to the upstream activating sequence comprised within said regulatory region of at least one of said at least four target transgenes;(c) obtaining a first parental plant and a second parental plant, wherein each of said at least four target transgenes and said at least two activator transgenes (i) is individually present in either said first parental plant or said second parental plant, (ii) is unlinked from each of the other of said at least four target transgenes and said at least two activator transgenes that are present within the same said first parental plant or said second parental plant, and (iii) is in a hemizygous state within said first parental plant or said second parental plant;(d) sexually crossing said first parental plant and said second parental plant to produce a population of progeny plants, whereby said population of progeny plants has different combinations of said at least four target transgenes and said at least two activator transgenes;(e) comparing different plants of said population of progeny plants to one another and selecting at least one progeny plant from said population as having said desirable phenotype to obtain a selected progeny plant;(f) determining which target transgenes and activator transgenes are present within said selected progeny plant, thereby identifying a combination of genetic elements responsible for said desirable phenotype of a plant; and(g) making a collection of seeds, wherein the cells of said seeds comprise said combination of genetic elements. 13. The method of claim 12, wherein at least one of said nucleotide sequences to be expressed is a nucleotide sequence encoding a dominant negative polypeptide. 14. The method of claim 12, wherein said first parental plant comprises said at least four target transgenes, and said second parental plant comprises said at least two activator transgenes. 15. The method of claim 12, wherein said chimeric polypeptide encoded by each of said at least two activator transgenes is the same. 16. The method of claim 12, wherein said upstream activating sequence of each of said at least four target transgenes is the same. 17. The method of claim 12, wherein said plant promoter of each of said at least two activator transgenes is different. 18. The method of claim 12, wherein said method further comprises, after said step (f): (a1) selecting at least four target transgenes, wherein each target transgene of said at least four target transgenes comprises a regulatory region comprising an upstream activating sequence operably linked to a nucleotide sequence to be expressed, whereby said upstream activating sequence of each of said at least four target transgenes is the same or different, and wherein said selected at least four target transgenes includes said target transgenes determined to be present within said selected progeny plant in step (f);(b1) selecting at least two activator transgenes, wherein each activator transgene comprises a plant promoter operably linked to a sequence encoding a chimeric polypeptide comprising a DNA binding domain fused to a transcription activation domain, wherein each DNA binding domain of said at least two chimeric polypeptides binds to the upstream activating sequence comprised within said regulatory region of at least one of said at least four target transgenes, and wherein said selected at least two activator transgenes includes said activator transgenes determined to be present within said selected progeny plant in step (f);(c1) obtaining a third parental plant and a fourth parental plant, wherein each of said at least four target transgenes of said step (a1) and said at least two activator transgenes of said step (b1) (i) is individually present in either said third parental plant or said fourth parental plant, (ii) is unlinked from each of the other of said at least four target transgenes and said at least two activator transgenes that are present within the same said third parental plant or said fourth parental plant, and (iii) is in a hemizygous state within said third parental plant or said fourth parental plant;(d1) sexually crossing said third parental plant and said fourth parental plant to produce a second population of progeny plants, whereby said second population of progeny plants has different combinations of said at least four target transgenes of step (a1) and said at least two activator transgenes of step (b1);(e1) comparing different plants of said second population of progeny plants to one another and selecting at least one progeny plant from said second population as having a desirable phenotype to obtain a second selected progeny plant; and(f1) determining which target transgenes and activator transgenes are present within said second selected progeny plant, thereby identifying a combination of genetic elements responsible for a desirable phenotype of a plant. 19. The method of claim 12, wherein said first parental plant and said second parental plant are selected from the group consisting of Zea mays, Sorghum bicolor, Triticum aestivum, and Oryza sativa. 20. The method of claim 12, wherein said first parental plant or said second parental plant is cytoplasmically male sterile. 21. The method of claim 12, wherein said selecting of step (e) is based at least in part on results under field testing conditions. 22. The method of claim 12, wherein said first parental plant and said second parental plant belong to distinct heterotic groups. 23. The method of claim 1, wherein said DNA binding domain is of non-plant origin. 24. The method of claim 23, wherein said DNA binding domain is a yeast or bacterial DNA binding domain. 25. The method of claim 12, wherein said DNA binding domain is of non-plant origin. 26. The method of claim 25, wherein said DNA binding domain is a yeast or bacterial DNA binding domain.
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