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Robust 3D DNA FISH Using Directly Labeled Probes
Authors:Daniel J Bolland  Michelle R King  Wolf Reik  Anne E Corcoran  Christel Krueger
Institution:1.Nuclear Dynamics Programme, The Babraham Institute;2.Epigenetics Programme, The Babraham Institute;3.Centre for Trophoblast Research, University of Cambridge
Abstract:3D DNA FISH has become a major tool for analyzing three-dimensional organization of the nucleus, and several variations of the technique have been published. In this article we describe a protocol which has been optimized for robustness, reproducibility, and ease of use. Brightly fluorescent directly labeled probes are generated by nick-translation with amino-allyldUTP followed by chemical coupling of the dye. 3D DNA FISH is performed using a freeze-thaw step for cell permeabilization and a heating step for simultaneous denaturation of probe and nuclear DNA. The protocol is applicable to a range of cell types and a variety of probes (BACs, plasmids, fosmids, or Whole Chromosome Paints) and allows for high-throughput automated imaging. With this method we routinely investigate nuclear localization of up to three chromosomal regions.
Keywords:Genetics  Issue 78  Molecular Biology  Biochemistry  Cellular Biology  Genomics  Epigenetics  Cell Nucleus  Fluorescence  In Situ Hybridization  FISH  3D DNA FISH  fluorescence in situ hybridization  nuclear structure  fluorescently labeled probes  visualization  imaging  DNA  chromosomes  sequencing  probes  assay
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