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A complementary transposon tool kit for Drosophila melanogaster using P and piggyBac
Authors:Thibault Stephen T  Singer Matthew A  Miyazaki Wesley Y  Milash Brett  Dompe Nicholas A  Singh Carol M  Buchholz Ross  Demsky Madelyn  Fawcett Robert  Francis-Lang Helen L  Ryner Lisa  Cheung Lai Man  Chong Angela  Erickson Cathy  Fisher William W  Greer Kimberly  Hartouni Stephanie R  Howie Elizabeth  Jakkula Lakshmi  Joo Daniel  Killpack Keith  Laufer Alex  Mazzotta Julie  Smith Ronald D  Stevens Lynn M  Stuber Christiana  Tan Lory R  Ventura Richard  Woo Alesa  Zakrajsek Irena  Zhao Lora  Chen Feng  Swimmer Candace  Kopczynski Casey  Duyk Geoffrey  Winberg Margaret L  Margolis Jonathan
Affiliation:Exelixis, 170 Harbor Way, South San Francisco, California 94083-0511, USA. thibault@exelixis.com
Abstract:With the availability of complete genome sequence for Drosophila melanogaster, one of the next strategic goals for fly researchers is a complete gene knockout collection. The P-element transposon, the workhorse of D. melanogaster molecular genetics, has a pronounced nonrandom insertion spectrum. It has been estimated that 87% saturation of the approximately 13,500-gene complement of D. melanogaster might require generating and analyzing up to 150,000 insertions. We describe specific improvements to the lepidopteran transposon piggyBac and the P element that enabled us to tag and disrupt genes in D. melanogaster more efficiently. We generated over 29,000 inserts resulting in 53% gene saturation and a more diverse collection of phenotypically stronger insertional alleles. We found that piggyBac has distinct global and local gene-tagging behavior from that of P elements. Notably, piggyBac excisions from the germ line are nearly always precise, piggyBac does not share chromosomal hotspots associated with P and piggyBac is more effective at gene disruption because it lacks the P bias for insertion in 5' regulatory sequences.
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