Tropism of the Novel AAVBR1 Capsid Following Subretinal Delivery

被引:0
作者
Carroll, Lara [1 ]
Uehara, Hironori [2 ]
Zhang, Xiaohui [2 ]
Ambati, Balamurali [2 ]
机构
[1] Moran Eye Ctr, 65 Mario Capecchi Way, Salt Lake City, UT 84132 USA
[2] 6231 Univ Oregon, Phil & Penny Knight Campus Accelerating Sci Impac, Eugene, OR 97403 USA
基金
美国国家卫生研究院;
关键词
subretinal delivery; adeno-associated virus (AAV); gene therapy; transduction; binding motif; IMMUNE-RESPONSE; VIRAL VECTOR; INTRAVITREAL;
D O I
10.3390/ijms23147738
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
A serious limitation of current adeno-associated viral (AAV) capsids employed for subretinal delivery is achieving adequate lateral spread beyond the injection site, required for the efficient delivery of gene therapy to the outer retina and/or RPE. AAVBR1 is a unique AAV with exceptional tropism for CNS microvasculature following systemic delivery. Here, we used in vivo and ex vivo analysis to show that subretinal delivery of AAVBR1.GFP in mice achieves superior tropism to RPE and outer retina than either AAV2.GFP or AAV8.GFP, two of the most common capsids used for subretinal delivery. At a low (5 x 10(8) vg) subretinal dose, the AAVBR1.GFP signal was visible by 48 h and significantly surpassed peak fluorescence of other AAVs in retina and RPE. The co-injection of AAVBR1.GFP with the AAVBR1-specific heptapeptide, NRGTEWD, significantly blocked the AAVBR1.GFP signal, but had no effect on AAV2.GFP fluorescence, confirming that AAVBR1's enhanced tropism for RPE and outer retina derives from this 7AA modification within the capsid-binding motif. Enhanced dispersal and consequent transduction suggest that AAVBR1 can be employed at a lower dosage than the standard AAV2 capsid to achieve equivalent expression for gene therapy, warranting further evaluation of its utility as a therapeutic vehicle for subretinal delivery.
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页数:10
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