Literature DB >> 27167405

Spectral imaging to visualize higher-order genomic organization.

Iain A Sawyer1,2, Sergei P Shevtsov1, Miroslav Dundr1.   

Abstract

A concern in the field of genomics is the proper interpretation of large, high-throughput sequencing datasets. The use of DNA FISH followed by high-content microscopy is a valuable tool for validation and contextualization of frequently occurring gene pairing events at the single-cell level identified by deep sequencing. However, these techniques possess certain limitations. Firstly, they do not permit the study of colocalization of many gene loci simultaneously. Secondly, the direct assessment of the relative position of many clustered gene loci within their respective chromosome territories is impossible. Thus, methods are required to advance the study of higher-order nuclear and cellular organization. Here, we describe a multiplexed DNA FISH technique combined with indirect immunofluorescence to study the relative position of 6 distinct genomic or cellular structures. This can be achieved in a single hybridization step using spectral imaging during image acquisition and linear unmixing. Here, we detail the use of this method to quantify gene pairing between highly expressed spliceosomal genes and compare these data to randomly positioned in silico simulated gene clusters. This is a potentially universally applicable approach for the validation of 3C-based technologies, deep imaging of spatial organization within the nucleus and global cellular organization.

Keywords:  Cajal bodies; DNA FISH; chromosome territories; gene positioning; genome organization; nuclear bodies; spectral imaging; spliceosomal U snRNA genes

Mesh:

Substances:

Year:  2016        PMID: 27167405      PMCID: PMC4991238          DOI: 10.1080/19491034.2016.1187344

Source DB:  PubMed          Journal:  Nucleus        ISSN: 1949-1034            Impact factor:   4.197


  57 in total

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