Isolation and characterization of Df(2L)BSC106
Jennifer Deal and Kevin Cook
Bloomington Stock Center
Indiana University
Df(2L)BSC106 was isolated as a FLP recombinase-induced recombination event involving P{XP}d03548 and PBac{WH}f03258. The deletion was isolated as a chromosome lacking miniwhite markers in progeny of P{hsFLP}1, y1 w1118; P{XP}d03548/PBac{WH}f03258 males crossed to w1118; P{w+mC=hs-hid}2, wgSp-1/CyO females. These males were heat shocked as larvae as described in Parks et al., Nature Genetics 36: 288-292, 2004 (FBrf0175003). This cross and crosses in preceding and succeeding generations maintained the original genetic background of the Exelixis insertion stocks (Thibault et al, Nature Genetics 36: 283-287, 2004; FBrf0175002). The recombination event generated the genetic element P+PBac{XP5.WH5}BSC106 from the segment of P{XP}d03548 to the left of its FRT site and the segment of PBac{WH}f03258 to the right of its FRT site. Its presence was verified using the PCR methods and primers described in Parks et al. Exelixis, Inc. determined the insertion site of P{XP}d03548 to be at Release 3 genomic coordinate 291646 on chromosome arm 2L and the insertion site of PBac{WH}f03258 to be at Release 3 genomic coordinate 419212 on arm 2L. The Gene Disruption project determined the insertion site of P{XP}d03548 to be at Release 3 genomic coordinate 291729 on arm 2L and the insertion site of PBac{WH}f03258 to be at Release 3 genomic coordinate 419612 on arm 2L. The cytological breakpoints of Df(2L)BSC106 predicted from these coordinates are 21B8;21C4. It failed to complement P{lacW}U2af38k14504, al1 and P{lacW}RpI135k16513.