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通过跳过mdx营养不良小鼠中的突变外显子产生功能性肌营养不良蛋白的量。

Functional amounts of dystrophin produced by skipping the mutated exon in the mdx dystrophic mouse.

作者信息

Lu Qi Long, Mann Christopher J, Lou Fang, Bou-Gharios George, Morris Glenn E, Xue Shao-an, Fletcher Sue, Partridge Terence A, Wilton Stephen D

机构信息

Muscle Cell Biology, MRC Clinical Science Centre, Hammersmith Hospital, Du Cane Road, London, W12 0NN, UK.

出版信息

Nat Med. 2003 Aug;9(8):1009-14. doi: 10.1038/nm897. Epub 2003 Jul 6.

Abstract

As a target for gene therapy, Duchenne muscular dystrophy (DMD) presents many obstacles but also an unparalleled prospect for correction by alternative splicing. The majority of mutations in the dystrophin gene occur in the region encoding the spectrin-like central rod domain, which is largely dispensable. Thus, splicing around mutations can generate a shortened but in-frame transcript, permitting translation of a partially functional dystrophin protein. We have tested this idea in vivo in the mdx dystrophic mouse (carrying a mutation in exon 23 of the dystrophin gene) by combining a potent transfection protocol with a 2-O-methylated phosphorothioated antisense oligoribonucleotide (2OMeAO) designed to promote skipping of the mutated exon*. The treated mice show persistent production of dystrophin at normal levels in large numbers of muscle fibers and show functional improvement of the treated muscle. Repeated administration enhances dystrophin expression without eliciting immune responses. Our data establishes the realistic practicality of an approach that is applicable, in principle, to a majority of cases of severe dystrophinopathy.

摘要

作为基因治疗的靶点,杜氏肌营养不良症(DMD)存在诸多障碍,但通过可变剪接进行矫正也有着无与伦比的前景。肌营养不良蛋白基因中的大多数突变发生在编码血影蛋白样中央杆状结构域的区域,该区域在很大程度上是可有可无的。因此,围绕突变进行剪接可以产生一个缩短但读框内的转录本,从而允许翻译出部分功能性的肌营养不良蛋白。我们通过将一种高效转染方案与一种设计用于促进突变外显子跳跃的2'-O-甲基硫代磷酸化反义寡核糖核苷酸(2OMeAO)相结合,在mdx营养不良小鼠(其肌营养不良蛋白基因外显子23存在突变)体内对这一想法进行了测试*。经治疗的小鼠在大量肌纤维中持续产生正常水平的肌营养不良蛋白,且治疗后的肌肉功能得到改善。重复给药可增强肌营养不良蛋白的表达,而不会引发免疫反应。我们的数据证实了一种方法在现实中的可行性,该方法原则上适用于大多数严重肌营养不良症病例。

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