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Improved in situ hybridization and G-banding by pretreatment with Denhardt's solution and gelatin-chrome alum
Authors:Greta M Lee  Ellen M Rasch and Phillip R Musich
Institution:(1) Departments of Cellular Biophysics Quillen-Dischner College of Medicine, East Tennessee State University, 37614 Johnson City, Tennessee, USA;(2) Department of Biochemistry, Quillen-Dischner College of Medicine, East Tennessee State University, 37614 Johnson City, Tennessee, USA;(3) Present address: Department of Zoology, Duke University, 27706 Durham, North Carolina, USA
Abstract:Summary Various pretreatments of metaphase spreads were examined to obtain optimal DNA labelling patterns while maintaining chromosome integrity duringin situ hybridization procedures. Preparations of African green monkey (AGM) chromosomes fixed in methanol-acetic acid (CV-1 cell line) were treated by coating with Denhardt's solution, dilute gelatin-chrome alum, nonfat instant dry milk dissolved in saline—citrate solution (SSC) and/or acetylation prior to denaturation of chromosomal DNA in 70% formamide-2 x SSC for 2 min at 70° C. A3H-labelled, cloned DNA fragment of the highly, repetitive AGM component agrDNA was hybridized to the chromosomes by incubation at 45° C for 16 h. Treatment with gelatinchrome alum prior to denaturation greatly improved chromosome morphology and decreased background, but reduced pericentromeric labelling. Sequential treatment with 5 x Denhardt's solution followed by gelatin-chrome alum resulted in enhanced specificity of labelling and excellent chromosome morphology, as well as reduced levels of background. Acetylation had little effect after pretreatment with gelatin-chrome alum, but reduced background levels after pretreatment with Denhardt's solution. Chromosomes treated with Denhardt's solution plus gelatin-chrome alum can be routinely G-banded using trypsin afterin situ hybridization.
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