Fig. 1: In vitro studies of mdx4cv mutation correction using ABE-NG. From: Efficient precise in vivo base editing in adult dystrophic mice a Genomic DNA, encoded amino acids and guide RNA with PAM (highlighted in blue) sequences at the stop codon mutation site (red). b The reporter construct contains a puromycin resistance cassette fused with E2A peptide, mdx4cv target sequence and ATG-removed EGFP. Correction of the stop codon within the target sequence would allow EGFP expression. c Fluorescence microscopy images of HEK293 cells transfected with reporter alone, or reporter, gRNA and one of the base editors (ABEmax, ABE-x, and ABE-NG). Scale bar: 500 µm. d–e Flow cytometry analysis of EGFP expression in HEK293 cells transfected as described in (c). n = 3 wells/group; one-way ANOVA with Turkey’s multiple comparisons test. Data are mean ± SD.

A novel gene editing technique developed by researchers at The Ohio State University Wexner Medical Center and College of Medicine is showing promise in correcting genetic mutations in Duchenne muscular dystrophy (DMD) and some cardiovascular diseases.

DMD is a deadly genetic disease caused by mutations to the dystrophin gene. Without dystrophin, muscle cells are damaged, resulting in progressive muscle weakness and wasting, which ultimately leads to respiratory impairment and . DMD is the most common form of and primarily affects boys. It occurs in about one out of every 5,000 male infants worldwide. The first symptoms usually start at age three and worsen over time, with many patients living only into their 20s.

CRISPR genome editing has shown promise in correcting disease-causing mutations but can cut DNA, endangering human health. Ohio State researchers were successful in modifying a —a technology built upon CRISPR—to safely and precisely edit a DMD mutation without cutting DNA in adult mice. Systemic delivery of an adeno-associated virus carrying the editor resulted in dystrophin restoration and functional improvement in the mice. The study's results were published in Nature Communications.

"Our technique shows systemic in vivo base editing can be achieved with high efficiency in a preclinical relevant animal model of DMD," said lead author Renzhi Han, a professor in the Division of Cardiac Surgery at the College of Medicine. "It has significant implications for clinical translation. This type of base editing does not require repeated treatment since it directly modifies the genetic code and produces a long-lasting therapeutic effect. Since it also doesn't cut the genomic DNA, which happens with CRISPR, there are no large DNA deletions and chromosomal rearrangements."

By modifying an adenine base editor to overcome various challenges, Han and his team were successful in restoring dystrophin expression in the muscle and hearts of mice with DMD. With a single intravenous injection of the improved at five weeks of age, over 95 percent of heart at 10 months of age were restored to re-express dystrophin naturally. Researchers didn't observe detectable adverse events in the treated animals.

"The editing efficiency in the heart was exceptionally high in the treated mice," Han said. "Our base editing technique has tremendous potential because it could be used for targeting many other genetic diseases."

The next step of the research is a larger animal trial for preclinical testing. Han and his team have been developing therapeutic strategies for muscular dystrophies for years and were part of a group that demonstrated for the first time in 2015 that in vivo genome editing can be used to correct DMD mutations in postnatal animals.

More information: Li Xu et al, Efficient precise in vivo base editing in adult dystrophic mice, Nature Communications (2021). DOI: 10.1038/s41467-021-23996-y

Journal information: Nature Communications