1990
DOI: 10.1159/000132913
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Rapid subchromosomal localization of cosmids by nonradioactive in situ hybridization

Abstract: A rapid method for localizing large numbers of complete cosmids by nonradioactive in situ hybridization is described. The cosmids are nick translated in the presence of biotin-16-dUTP, incubated with an excess of sonicated human DNA, and used as a probe for in situ hybridization. Sites of hybridization are detected by successive treatments with FITC-labeled avidin and biotinylated anti-avidin antibody. Fifty-two cosmids were localized on chromosome 16 in 5 d relative to translocation breakpoints contained in t… Show more

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Cited by 142 publications
(68 citation statements)
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“…Regionally localised BACs were labelled by nick-translation with biotin-14-dUTP (Gibco BRL) or digoxigenin-16-dUTP (Roche Diagnostics) as described by Kievits et al 15 In situ hybridisation using the labelled BACs as probes was performed according to Dauwerse et al 16 Slides containing Epstein Barr virus-transformed cells were processed for Fiber-FISH as described by Datson et al 17 For Fiber-FISH, pairs of BACs labelled in red and green were used as probes.…”
Section: Fluorescent In Situ Hybridisation (Fish) Analysismentioning
confidence: 99%
“…Regionally localised BACs were labelled by nick-translation with biotin-14-dUTP (Gibco BRL) or digoxigenin-16-dUTP (Roche Diagnostics) as described by Kievits et al 15 In situ hybridisation using the labelled BACs as probes was performed according to Dauwerse et al 16 Slides containing Epstein Barr virus-transformed cells were processed for Fiber-FISH as described by Datson et al 17 For Fiber-FISH, pairs of BACs labelled in red and green were used as probes.…”
Section: Fluorescent In Situ Hybridisation (Fish) Analysismentioning
confidence: 99%
“…All tumors were successfully karyotyped and included lesions with 6p21 (n ϭ 17) or 12q15 alterations (n ϭ 33), karyotypic alterations not involving 6p21 or 12q15 (n ϭ 13), or a normal karyotype (n ϭ 32). FISH was performed after GTG banding of the same metaphase spreads according to previously published procedures (Kievits et al, 1992). Metaphases were hybridized with a pool of different cosmids spanning over the breakpoint region 12q15 and flanking the third intron of HMGI-C Kazmierczak et al, 1996b) and with PAC clones containing the HMGI(Y) gene mapped at 6p21.2 (Kazmierczak et al, 1996c).…”
Section: Cytogenetic and Molecular Cytogenetic Analysismentioning
confidence: 99%
“…[30][31][32] FISH results were observed through a Leitz DM-RBE microscope (Leica, Rijswijk, The Netherlands) equipped for fluorescence microscopy and mounted with a Photometric Series 200, KAF1400 charged coupled device camera. Image acquisition and processing was performed on a Power Macintosh 7100, using the IP Lab Spectrum Multiprobe software (Photometrics, Munich, Germany).…”
Section: Fluorescence In Situ Hybridization (Fish)mentioning
confidence: 99%