4.5 Article

Cone and rod photoreceptor transplantation in models of the childhood retinopathy Leber congenital amaurosis using flow-sorted Crx-positive donor cells

期刊

HUMAN MOLECULAR GENETICS
卷 19, 期 23, 页码 4545-4559

出版社

OXFORD UNIV PRESS
DOI: 10.1093/hmg/ddq378

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资金

  1. Medical Research Council UK [G03000341, G0901550]
  2. Macula Vision Research Foundation
  3. Fight for Sight
  4. Wellcome Trust [082217]
  5. Ulverscroft Foundation
  6. NIHR Biomedical Research Centre for Ophthalmology at Moorfields Eye Hospital and UCL Institute of Ophthalmology
  7. NIHR Biomedical Research Centre for Paediatric Research at Great Ormond Street Hospital for Children and UCL Institute of Child Health
  8. Royal Society
  9. MRC [G0901550, G0700438] Funding Source: UKRI
  10. Great Ormond Street Hospital Childrens Charity [V1221] Funding Source: researchfish
  11. Medical Research Council [G0700438, G0901550] Funding Source: researchfish
  12. National Institute for Health Research [NF-SI-0508-10130] Funding Source: researchfish

向作者/读者索取更多资源

Retinal degenerative disease causing loss of photoreceptor cells is the leading cause of untreatable blindness in the developed world, with inherited degeneration affecting 1 in 3000 people. Visual acuity deteriorates rapidly once the cone photoreceptors die, as these cells provide daylight and colour vision. Here, in proof-of-principle experiments, we demonstrate the feasibility of cone photoreceptor transplantation into the wild-type and degenerating retina of two genetic models of Leber congenital amaurosis, the Crb1(rd8/rd8) and Gucy2e(-/-) mouse. Crx-expressing cells were flow-sorted from the developing retina of CrxGFP transgenic mice and transplanted into adult recipient retinae; CrxGFP is a marker of cone and rod photoreceptor commitment. Only the embryonic-stage Crx-positive donor cells integrated within the outer nuclear layer of the recipient and differentiated into new cones, whereas postnatal cells generated a 10-fold higher number of rods compared with embryonic-stage donors. New cone photoreceptors displayed unambiguous morphological cone features and expressed mature cone markers. Importantly, we found that the adult environment influences the number of integrating cones and favours rod integration. New cones and rods were observed in ratios similar to that of the host retina (1: 35) even when the transplanted population consisted primarily of cone precursors. Cone integration efficiency was highest in the cone-deficient Gucy2e(-/-) retina suggesting that cone depletion creates a more optimal environment for cone transplantation. This is the first comprehensive study demonstrating the feasibility of cone transplantation into the adult retina. We conclude that flow-sorted embryonic-stage Crx-positive donor cells have the potential to replace lost cones, as well as rods, an important requirement for retinal disease therapy.

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