Transposase enzymes can insert new pieces of DNA in a genome LAGUNA DESIGN/SCIENCE PHOTO LIBRARY
The CRISPR genome editing technology currently revolutionising biology may soon become even powerful. A new variant of the method based on 鈥渏umping genes鈥 could make it much easier to insert pieces of DNA into genomes.
鈥淚t鈥檚 still in the experimental phase,鈥 says geneticist Helen O鈥橬eill of University College London. 鈥淏ut it鈥檚 quite exciting.鈥
Biologists would love to edit genomes with the same ease we can change digital texts using the 鈥渇ind and replace鈥 command. What CRISPR聽currently excels at, however, is 鈥渇ind and delete鈥.
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The standard form of CRISPR involves adding a protein called Cas9 to a cell along with a piece of guide RNA. The protein searches through the genome until it finds DNA that matches the guide RNA sequence and then cuts the DNA at this point. Some DNA is lost when the cell sticks the ends back together, resulting in deletions that typically disable genes.
This is extremely useful. Many diseases could be treated by disabling genes. It is possible to dramatically lower cholesterol levels this way, for instance.
But in many cases it would be better to fix faulty genes rather than disable them. It is possible to do this by adding a corrected gene to a cell along with the CRISPR Cas9 protein and the RNA guide. Cells sometimes splice the corrected version into the genome when they repair the DNA.
Unfortunately, this typically works only 20 per cent of the time, and in many cell types it simply doesn鈥檛 work at all.
Lots of teams are working on improving . Feng Zhang of聽the Massachusetts Institute of Technology has now developed a whole new approach based on聽transposons, also known as jumping genes.
罢丑别蝉别听extremely selfish genes聽do nothing but copy and paste themselves from one part of the genome to another using enzymes called transposases. These genetic parasites are extremely common: more than half of our genome consists of now defunct jumping genes.
It was recently discovered that that bacteria use to defend against viruses. These Tn-7 jumping genes use a protein called Cas12k to find specific sequences. But these variants don鈥檛 cut the DNA at the target sequence; instead transposase enzymes insert the jumping genes into this site.
Read more: What is CRISPR?
Feng鈥檚 team have now shown the Cas12k protein and the Tn-7 transposes can be used to insert pieces of DNA several thousand letters long into specific sites in the genome of the E. coli bacterium. What鈥檚 more, it worked around 80 per cent of the time.
鈥淥verall, the results shown in the paper are remarkable,鈥 says Gaeten Burgio of the Australian National University, who studies CRISPR systems. But the team have yet to show this approach works in animal and plant cells, he cautions.
If this jumping gene CRISPR system can be made to work in complex cells, it would give biologists 鈥渇ind and add鈥 function. That鈥檚 not the 鈥渇ind and replace鈥 function of their dreams but it would be a powerful addition to our toolset that would be useful for everything from basic research to treating diseases.
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