AI Article Synopsis

  • Functional defects in type VII collagen, linked to mutations in the COL7A1 gene, lead to severe skin blistering in recessive dystrophic epidermolysis bullosa (RDEB).
  • The large size of the COL7A1 gene makes it challenging to use traditional gene therapy methods, but trans-splicing techniques offer a solution by shortening the transcript.
  • By using trans-splicing to correct type VII collagen expression in RDEB skin cells, researchers observed improved cell function and structure, paving the way for potential gene therapy treatments.

Article Abstract

Functional defects in type VII collagen, caused by premature termination codons on both alleles of the COL7A1 gene, are responsible for the severe autosomal recessive types of the skin blistering disease, recessive dystrophic epidermolysis bullosa (RDEB). The full-length COL7A1 complementary DNA (cDNA) is about 9 kb, a size that is hardly accommodated by therapeutically used retroviral vectors. Although there have been successful attempts to produce functional type VII collagen protein in model systems of RDEB, the risk of genetic rearrangements of the large repetitive cDNA sequence may hamper the clinical application of full-length COL7A1 cDNA in the human system. Therefore, we used trans-splicing to reduce the size of the COL7A1 transcript. Retroviral transduction of RDEB keratinocytes with a 3' pre-trans-splicing molecule resulted in correction of full-length type VII collagen expression. Unlike parental RDEB keratinocytes, transduced cells displayed normal morphology and reduced invasive capacity. Moreover, transduced cells showed normal localization of type VII collagen at the basement membrane zone in skin equivalents, where it assembled into anchoring fibril-like structures. Thus, using trans-splicing we achieved correction of an RDEB phenotype in vitro, which marks an important step toward its application in gene therapy in vivo.

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Source
http://dx.doi.org/10.1038/jid.2010.249DOI Listing

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