Cho W K, Ebihara S, Nalbantoglu J, Gilbert R, Massie B, Holland P, Karpati G, Petrof B J
Respiratory Division and Meakins-Christie Laboratories, McGill University Health Centre, Montreal, Quebec, Canada.
Hum Gene Ther. 2000 Mar 20;11(5):701-14. doi: 10.1089/10430340050015608.
Duchenne muscular dystrophy (DMD) and other inherited myopathies lead to progressive destruction of most skeletal muscles in the body, including those responsible for maintaining respiration. DMD is a fatal disorder caused by defects in the dystrophin gene. Recombinant adenovirus vectors (AdV) are considered a promising means for therapeutic delivery of a functional dystrophin gene to DMD muscles. If AdV-mediated dystrophin gene replacement in DMD is to be successful, development of a systemic delivery method for targeting the large number of diseased muscles will be required. In this study we investigated two major factors preventing efficient AdV-mediated gene transfer to skeletal muscles of adult animals after intravascular AdV administration: (1) an inability of AdV particles to breach the endothelial barrier and enter into contact with myofibers, and (2) a relatively nonpermissive myofiber population for AdV infection due at least in part to insufficient levels of the coxsackie/adenovirus attachment receptor (CAR). On the basis of established principles governing the transendothelial flux of macromolecules, we further hypothesized that an alteration in Starling forces (increased hydrostatic and decreased osmotic pressures) within the intravascular compartment would facilitate AdV transendothelial flux via convective transport. In addition, experimental muscle regeneration was employed to increase the prevalence of immature myofibers in which CAR expression is upregulated. Here we report that by employing the above-described strategy, high-level heterologous reporter gene expression was achievable in hindlimb muscles of normal rats as well as dystrophic (mdx) mice (genetic homolog of DMD) after a single intraarterial injection of AdV. Microsphere studies confirmed enhanced transport into muscle of fluorescent tracer particles in the size range of AdV, and there was a high concordance between CAR upregulation and myofiber transduction after intraarterial AdV delivery. Furthermore, in mdx mice examined 10 days after intraarterial AdV delivery, the aforementioned procedures had no adverse effects on the force-generating capacity of targeted muscles. These findings have implications for eventual AdV-mediated gene therapy of generalized skeletal muscle diseases such as DMD using a systemic intraarterial delivery approach.
杜兴氏肌营养不良症(DMD)和其他遗传性肌病会导致身体大部分骨骼肌进行性破坏,包括那些负责维持呼吸的肌肉。DMD是一种由肌营养不良蛋白基因缺陷引起的致命疾病。重组腺病毒载体(AdV)被认为是将功能性肌营养不良蛋白基因治疗性递送至DMD肌肉的一种有前景的手段。如果要使AdV介导的DMD肌营养不良蛋白基因替代成功,就需要开发一种系统性递送方法来靶向大量患病肌肉。在本研究中,我们调查了血管内注射AdV后阻碍其有效介导基因转移至成年动物骨骼肌的两个主要因素:(1)AdV颗粒无法突破内皮屏障并与肌纤维接触;(2)肌纤维群体对AdV感染相对不敏感,这至少部分归因于柯萨奇病毒/腺病毒附着受体(CAR)水平不足。基于关于大分子跨内皮通量的既定原则,我们进一步假设血管内隔室中Starling力的改变(静水压力增加和渗透压降低)将通过对流运输促进AdV跨内皮通量。此外,采用实验性肌肉再生来增加未成熟肌纤维的比例,其中CAR表达上调。在此我们报告,通过采用上述策略,在单次动脉内注射AdV后,正常大鼠以及营养不良(mdx)小鼠(DMD的基因同源物)的后肢肌肉中可实现高水平的异源报告基因表达。微球研究证实了荧光示踪颗粒在AdV大小范围内向肌肉的转运增强,并且动脉内注射AdV后CAR上调与肌纤维转导之间存在高度一致性。此外,在动脉内注射AdV 10天后检查的mdx小鼠中,上述程序对靶向肌肉的力产生能力没有不良影响。这些发现对最终使用系统性动脉内递送方法对DMD等全身性骨骼肌疾病进行AdV介导的基因治疗具有重要意义。
