Claims for Patent: 6,395,487
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Summary for Patent: 6,395,487
| Title: | Method chromosomal rearrangement by consecutive gene targeting of two recombination substrates to the deletion endpoints |
| Abstract: | The present invention involves the creation of defined chromosomal deficiencies, inversions and duplications using Cre recombinase in ES cells transmitted into the mouse germ line. These chromosomal reconstructions can extend up to 3-4 cM. Chromosomal rearrangements are the major cause of inherited human disease and fetal loss. Additionally, translocations and deletions are recognized as major genetic changes that are causally involved in neoplasia. Chromosomal variants such as deletions and inversions are exploited commonly as genetic tools in organisms such as Drosophila. Mice with defined regions of segmental haploidy are useful for genetic screening and allow accurate models of human chromosomal diseases to be generated. |
| Inventor(s): | Bradley; Allan (Houston, TX), Ramirez-Solis; Ramiro (Missouri City, TX), Liu; Pentao (Frederick, MD), Su; Hong (Houston, TX), Zheng; Binhai (Houston, TX) |
| Assignee: | Baylor College of Medicine (Houston, TX) |
| Application Number: | 09/552,219 |
| Patent Claims: | 1. A method for deleting, duplicating or inverting a selected region of genetic material in cells comprising the steps of:
inserting a first selection cassette at a 5' end of said selected region using gene targeting methods, said first selection cassette comprising a first selectable marker, a first lox recombination site, and a first portion of a second selectable marker; selecting cells expressing said first selectable marker; inserting a second selection cassette at a 3' end of said selected region using gene targeting methods, said second selection cassette comprising a third selectable marker, a second lox recombination site, and a remaining portion of said second selectable marker; selecting cells expressing said third selectable marker; expressing a recombinase to produce recombination between said first and second lox sites; and selecting cells expressing said second selectable marker. 2. A method of claim 1 wherein said lox sites are loxP. 3. A method of claim 1 wherein said recombinase is Cre recombinase. 4. A method for inverting a selected region of genetic material in cells comprising the steps of: inserting a first selection cassette at a 5' end of said selected region using gene targeting methods, said first selection cassette comprising a first selectable marker, a first loxP recombination site, and a first portion of a second selectable marker; selecting cells expressing said first selectable marker; inserting a second selection cassette at a 3' end of said selected region using gene targeting methods, said second selection cassette comprising a third selectable marker, a second loxP recombination site, and a remaining portion of said second selectable marker; selecting cells expressing said third selectable marker; expressing Cre recombinase to produce recombination between said first and second loxP sites; and selecting cells expressing said second selectable marker. 5. The method of claim 4 wherein said first selectable marker is a puromycin resistance gene, said second selectable marker is an Hprt gene, and said third selectable marker is a neomycin resistance gene. 6. The method of claim 4 wherein said first selectable marker is a puromycin resistance gene. 7. The method of claim 4 wherein said second selectable marker is a functional Hprt gene. 8. The method of claim 4 wherein said third selectable marker is a neomycin resistance gene. 9. The method of claim 4 wherein said cells are embryonic stem cells. 10. The method of claim 4 wherein said Cre is transiently expressed Cre. 11. The method of claim 4 wherein said Cre is inducibly expressed Cre. 12. The method of claim 4 wherein said Cre is constitutively expressed Cre. 13. A method of inverting a selected region of genetic material in cells comprising the steps of: inserting a gene selection cassette at a 5' end of said selected region using either a gene targeting vector or a first viral vector, said first selection cassette comprising a first selectable marker, a first loxP recombination site, and a first portion of a second selectable marker; selecting cells expressing said first selectable marker; inserting a second selection cassette at a 3' end of said selected region using a second gene targeting vector or a second viral vector, said second selection cassette comprising a third selectable marker, a second loxP recombination site, and a remaining portion of said second selectable marker; selecting cells expressing said third selectable marker; expressing transiently Cre recombinase to produce recombination between said first and second loxP sites; and selecting cells expressing said second selectable marker. 14. The method of claim 13 wherein at least one viral vector is a retrovirus. 15. The method of claim 13 wherein at least one viral vector has a provirus structure comprising a cassette in turn comprising an hprt5' cassette, a loxP site, and a puromycin resistance gene. 16. The method of claim 13 wherein at least one viral vector has a provirus structure comprising a cassette in turn comprising an hprt5' cassette, a loxP site, and a neomycin resistance gene. 17. The method of claim 13 wherein the first targeting vector is a first vector for inserting a first native sequence of DNA at said 5' end, comprising: said first native sequence of DNA cloned into the vector of about 7.5 kb; a tyrosinase mingene; a neomycin resistance gene; a 5' hprt fragment; and a loxP site in a hprt fragment intron; and said second targeting vector for inserting a second native sequence of DNA at said 3' end, comprising: said second native sequence of DNA cloned into the vector of about 7.5 kb; a K14-agouti gene; a puromycin resistance gene; a 3' hprt fragment; and a loxP site in a hprt fragment intron. 18. The method of claim 13 wherein the first viral vector is a first vector for inserting a first native sequence of DNA at said 5' end, comprising: sad first native sequence of DNA cloned into the vector of about 7.5 kb; a tyrosinase mingene; a neomycin resistance gene; a 5' hprt fragment; and a loxP site in a hprt fragment intron; and said second viral vector for inserting a second native sequence of DNA at said 3' end, comprising: said second native sequence of DNA cloned into the vector of about 7.5 kb; a K14-agouti gene; a puromycin resistance gene; a 3' hprt fragment; and a loxP site in a hprt fragment intron. 19. A method for creating a defined chromosomal inversion comprising the steps of: identifying a desired region of a chromosome of interest to be inverted; inserting two sequences which are native to the chromosome of interest at each endpoint of said region of said chromosome of interest using a first and a second targeting vector, wherein each targeting vector is comprised of one or more selectable markers and a loxP site and an hprt fragment; transiently expressing Cre recombinase to produce recombination between each of two said loxP sites; whereby upon chromosomal rearrangement induced by said Cre recombinase, a functional hprt expression cassette is reconstructed, wherein the defined chromosomal inversion is created. |
Details for Patent 6,395,487
| Applicant | Tradename | Biologic Ingredient | Dosage Form | BLA | Approval Date | Patent No. | Expiredate |
|---|---|---|---|---|---|---|---|
| Merck Sharp & Dohme Corp. | INTRON A | interferon alfa-2b | For Injection | 103132 | 06/04/1986 | ⤷ Try a Trial | 2016-06-26 |
| Merck Sharp & Dohme Corp. | INTRON A | interferon alfa-2b | For Injection | 103132 | ⤷ Try a Trial | 2016-06-26 | |
| Merck Sharp & Dohme Corp. | INTRON A | interferon alfa-2b | Injection | 103132 | ⤷ Try a Trial | 2016-06-26 | |
| >Applicant | >Tradename | >Biologic Ingredient | >Dosage Form | >BLA | >Approval Date | >Patent No. | >Expiredate |
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