INFORMATION:
This work was supported by the National Institutes of Health (R01DA036865, U01HG007900, DP2OD008586, P30AR066527) and the National Science Foundation (CBET-1151035).
"Epigenome editing by a CRISPR-Cas9-based acetyltransferase activates genes from promoters and enhancers," Isaac B Hilton, Anthony M D'Ippolito, Christopher M Vockley, Pratiksha I. Thakore, Gregory E Crawford, Timothy E Reddy, Charles A Gersbach. Nature Biotechnology, April 6, 2015. DOI: 10.1038/nbt.3199 END
Pulling the strings of our genetic puppetmasters
Engineers gain control of gene activity; new therapies may be ahead
2015-04-06
(Press-News.org) DURHAM, N.C. -- Duke researchers have developed a new method to precisely control when genes are turned on and active.
The new technology allows researchers to turn on specific gene promoters and enhancers -- pieces of the genome that control gene activity -- by chemically manipulating proteins that package DNA. This web of biomolecules that supports and controls gene activity is known as the epigenome.
The researchers say having the ability to steer the epigenome will help them explore the roles that particular promoters and enhancers play in cell fate or the risk for genetic disease and it could provide a new avenue for gene therapies and guiding stem cell differentiation.
The study appears online April 6 in Nature Biotechnology.
"The epigenome is everything associated with the genome other than the actual genetic sequence, and is just as important as our DNA in determining cell function in healthy and diseased conditions," said Charles Gersbach, assistant professor of biomedical engineering at Duke. "That becomes immediately obvious when you consider that we have over 200 cell types, and yet the DNA in each is virtually the same. The epigenome determines which genes each cell activates and to what degree."
This genetic puppetmaster consists of DNA packaging proteins called histones and a host of chemical modifications -- either to these histones or the DNA itself -- that help determine whether a gene is on or off.
But Gersbach's team didn't have to modify the genes themselves to gain some control.
"Next to every gene is a DNA sequence called a promoter that controls its activity," explained Gersbach. "But there's also many other pieces of the genome called enhancers that aren't next to any genes at all, and yet they play a critical role in influencing gene activity too."
Timothy Reddy, assistant professor of biostatistics and bioinformatics at Duke, has spent the better part of a decade mapping millions of these enhancers across the human genome. There has not, however, been a good way to find out exactly what each one does. An enhancer might affect a gene next door or several genes across the genome -- or maybe none at all.
To activate these enhancers and see what they do, Reddy thought perhaps he could chemically alter the histones at the enhancers to turn them on.
"There are already drugs that will affect enhancers across the whole genome, but that's like scorching the earth," said Reddy. "I wanted to develop tools to go in and modify very specific epigenetic marks in very specific places to find out what individual enhancers are doing."
Reddy found that specificity by teaming up with Gersbach, his neighbor within Duke's Center for Genomic and Computational Biology, who specializes in a gene-targeting system called CRISPR. Originally discovered as a natural antiviral system in bacteria, researchers have hijacked the system over the past few years and are now using it to cut and paste DNA sequences in the human genome.
For this epigenome editing application, Gersbach silenced the DNA-cutting mechanism of CRISPR and used it solely as a targeting system to deliver an enzyme (acetyltransferase) to specific promoters and enhancers.
"It's like we use CRISPR to find a genetic address so that we can alter the DNA's packaging at that specific site," said Reddy.
Gersbach and Reddy put their artificial epigenetic agent to the test by targeting a few well-studied gene promoters and enhancers. While these histone modifications have long been associated with gene activity, it wasn't clear if they were enough to turn genes on. And though Gersbach and Reddy had previously used other technologies to activate gene promoters, they had not successfully activated enhancers.
To the duo's great surprise, not only did the agent activate the gene promoters, it turned on the adjacent genes better than their previous methods. Equally surprising was that it worked on enhancers as well: they could turn on a gene -- or even families of genes -- by targeting enhancers at distant locations in the genome -- something that their previous gene activators could not do.
But the real excitement from their results is an emerging ability to probe millions of potential enhancers in a way never before possible.
"Some genetic diseases are straightforward -- if you have a mutation within a particular gene, then you have the disease," said Isaac Hilton, postdoctoral fellow in the Gersbach Lab and first author of the study. "But many diseases, like cancer, cardiovascular disease or neurodegenerative conditions, have a much more complex genetic component. Many different variations in the genome sequence can affect your risk of disease, and this genetic variation can occur in these enhancers that Tim has identified, where they can change the levels of gene expression. With this technology, we can explore what exactly it is that they're doing and how it relates to disease or response to drug therapies."
Gersbach added, "Not only can you start to answer those questions, but you might be able to use this technique for gene therapy to activate genes that have been abnormally silenced or to control the paths that stem cells take toward becoming different types of cells. These are all directions we will be pursuing in the future."
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[Press-News.org] Pulling the strings of our genetic puppetmastersEngineers gain control of gene activity; new therapies may be ahead