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Efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in E. coli DH10B using an inducible homologous recombination system

Gene therapy studies require techniques that allow alter- adapted an inducible homologous recombination system ation of human genomic DNA sequences. Bacterial arti- for use in E. coli DH10B cells, the host strain for BACs ficial chromosome cloning systems (BACs/PACs) bridge and PACs. Using this sy...

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Main Authors: Narayanan, Kulathuramaiyer, Williamson, R., Zhang, Y., Stewart, AF, Ioannou, PA
Format: Article
Language:English
Published: Stockton Press 1999
Subjects:
Q Science (General)
Online Access:http://ir.unimas.my/id/eprint/16746/1/Efficient.pdf
http://ir.unimas.my/id/eprint/16746/
http://www.nature.com/gt/journal/v6/n3/full/3300901a.html
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spelling my.unimas.ir.167462022-01-19T01:30:17Z http://ir.unimas.my/id/eprint/16746/ Efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in E. coli DH10B using an inducible homologous recombination system Narayanan, Kulathuramaiyer Williamson, R. Zhang, Y. Stewart, AF Ioannou, PA Q Science (General) Gene therapy studies require techniques that allow alter- adapted an inducible homologous recombination system ation of human genomic DNA sequences. Bacterial arti- for use in E. coli DH10B cells, the host strain for BACs ficial chromosome cloning systems (BACs/PACs) bridge and PACs. Using this system, we have introduced PCR the gap between vectors with small inserts and yeast arti- fragments carrying a selectable marker and a reporter ficial chromosomes (YACs). We report the use of a second gene downstream of the IVS I-110 splicing mutation into a generation BAC vector, pEBAC, containing eukaryotic sel- specific site within the b-globin gene sequence. The use ectable markers and combining some of the best features of this inducible system minimises the risk of unwanted of the BAC, PAC and HAEC systems, into which a 185 kb rearrangements by recombination between repetitive sequence containing the human b-globin gene cluster was elements and allows the introduction of relevant modifiretrofitted. To permit the introduction of mutations corre- cations or reporters at any specific sequence within sponding to those causing human pathology, we have BACs/PACs in E. coli DH10B cells. Stockton Press 1999 Article PeerReviewed text en http://ir.unimas.my/id/eprint/16746/1/Efficient.pdf Narayanan, Kulathuramaiyer and Williamson, R. and Zhang, Y. and Stewart, AF and Ioannou, PA (1999) Efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in E. coli DH10B using an inducible homologous recombination system. Gene Therapy, 6 (3). pp. 442-447. ISSN 0969-7128 http://www.nature.com/gt/journal/v6/n3/full/3300901a.html
institution Universiti Malaysia Sarawak
building Centre for Academic Information Services (CAIS)
collection Institutional Repository
continent Asia
country Malaysia
content_provider Universiti Malaysia Sarawak
content_source UNIMAS Institutional Repository
url_provider http://ir.unimas.my/
language English
topic Q Science (General)
spellingShingle Q Science (General)
Narayanan, Kulathuramaiyer
Williamson, R.
Zhang, Y.
Stewart, AF
Ioannou, PA
Efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in E. coli DH10B using an inducible homologous recombination system
description Gene therapy studies require techniques that allow alter- adapted an inducible homologous recombination system ation of human genomic DNA sequences. Bacterial arti- for use in E. coli DH10B cells, the host strain for BACs ficial chromosome cloning systems (BACs/PACs) bridge and PACs. Using this system, we have introduced PCR the gap between vectors with small inserts and yeast arti- fragments carrying a selectable marker and a reporter ficial chromosomes (YACs). We report the use of a second gene downstream of the IVS I-110 splicing mutation into a generation BAC vector, pEBAC, containing eukaryotic sel- specific site within the b-globin gene sequence. The use ectable markers and combining some of the best features of this inducible system minimises the risk of unwanted of the BAC, PAC and HAEC systems, into which a 185 kb rearrangements by recombination between repetitive sequence containing the human b-globin gene cluster was elements and allows the introduction of relevant modifiretrofitted. To permit the introduction of mutations corre- cations or reporters at any specific sequence within sponding to those causing human pathology, we have BACs/PACs in E. coli DH10B cells.
format Article
author Narayanan, Kulathuramaiyer
Williamson, R.
Zhang, Y.
Stewart, AF
Ioannou, PA
author_facet Narayanan, Kulathuramaiyer
Williamson, R.
Zhang, Y.
Stewart, AF
Ioannou, PA
author_sort Narayanan, Kulathuramaiyer
title Efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in E. coli DH10B using an inducible homologous recombination system
title_short Efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in E. coli DH10B using an inducible homologous recombination system
title_full Efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in E. coli DH10B using an inducible homologous recombination system
title_fullStr Efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in E. coli DH10B using an inducible homologous recombination system
title_full_unstemmed Efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in E. coli DH10B using an inducible homologous recombination system
title_sort efficient and precise engineering of a 200 kb b-globin human/bacterial artificial chromosome in e. coli dh10b using an inducible homologous recombination system
publisher Stockton Press
publishDate 1999
url http://ir.unimas.my/id/eprint/16746/1/Efficient.pdf
http://ir.unimas.my/id/eprint/16746/
http://www.nature.com/gt/journal/v6/n3/full/3300901a.html
_version_ 1724078495260213248
score 13.214268

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