Ribozyme-Mediated Repair of Sickle Beta-Globin RNA and DNA

核酶介导的镰状 β-珠蛋白 RNA 和 DNA 修复

基本信息

  • 批准号:
    7407405
  • 负责人:
  • 金额:
    $ 29.6万
  • 依托单位:
  • 依托单位国家:
    美国
  • 项目类别:
  • 财政年份:
    2007
  • 资助国家:
    美国
  • 起止时间:
    2007-04-01 至 2008-03-31
  • 项目状态:
    已结题

项目摘要

The overall goal of this proposal is to explore the ability of group I and group II introns to repair mutant beta-globin genes and transcripts and assess the potential utility of these molecules in human cells. These introns have been of great scientific interest because they are able to perform catalysis and because a subclass of these RNA enzymes can act as mobile genetic elements. Moreover, their ability to modify RNA and DNA sequences through forward and reverse-splicing reactions makes these introns of particular interest to translational researchers. Previously, we demonstrated that trans-splicing group I ribozymes can convert sickle beta-globin encoding mRNAs into gamma-globin encoding transcripts following transient transfection of the ribozyme into erythrocyte precursors derived from patients with sickle cell disease. In addition, we have demonstrated that such RNA repair can proceed with low to moderate efficiency (up to 50% repair) in 293 cells cotransfected with ribozyme and sickle beta-globin expression cassettes. More recently, we have demonstrated that the Lactococcus lactis group II intron can reverse-splice and site specificallv insert itself into desired DNA target sequences in transfected human cells. These proof of concept studies suggest that such catalytic RNAs may represent molecules that can be employed to modify genetic instructions for therapeutic ends to treat sickle cell disease and other genetic disorders. These studies also underscore the necessity for further evaluation and optimization of these catalytic RNAs if they are to become therapeutically useful. Here we propose to perform more detailed analyses of group I and group II intron activity in human ceils focusing upon repair of mutant beta-globin transcripts and genes. The completion of these studies will establish the needed experimental foundation from which the logical development of therapeutic group I and group II ribozymes for the treatment of sickle cell disease and other genetic disorders can proceed.
本提案的总体目标是探索I族和II族内含子的修复能力

项目成果

期刊论文数量(0)
专著数量(0)
科研奖励数量(0)
会议论文数量(0)
专利数量(0)

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BRUCE ALAN SULLENGER其他文献

BRUCE ALAN SULLENGER的其他文献

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{{ truncateString('BRUCE ALAN SULLENGER', 18)}}的其他基金

Direct Detection and Characterization of Thrombosis In Vivo
体内血栓形成的直接检测和表征
  • 批准号:
    10438599
  • 财政年份:
    2019
  • 资助金额:
    $ 29.6万
  • 项目类别:
Direct Detection and Characterization of Thrombosis In Vivo
体内血栓形成的直接检测和表征
  • 批准号:
    10201739
  • 财政年份:
    2019
  • 资助金额:
    $ 29.6万
  • 项目类别:
Direct Detection and Characterization of Thrombosis In Vivo
体内血栓形成的直接检测和表征
  • 批准号:
    9980489
  • 财政年份:
    2019
  • 资助金额:
    $ 29.6万
  • 项目类别:
Nucleic Acid Binding Polymers as Anti-Inflammatory Agents
作为抗炎剂的核酸结合聚合物
  • 批准号:
    8309507
  • 财政年份:
    2011
  • 资助金额:
    $ 29.6万
  • 项目类别:
RNA aptamers as cell surface receptor agonists and siRNA delivery agents
RNA适体作为细胞表面受体激动剂和siRNA递送剂
  • 批准号:
    7847451
  • 财政年份:
    2009
  • 资助金额:
    $ 29.6万
  • 项目类别:
RNA aptamers as cell surface receptor agonists and siRNA delivery agents
RNA适体作为细胞表面受体激动剂和siRNA递送剂
  • 批准号:
    8333428
  • 财政年份:
    2009
  • 资助金额:
    $ 29.6万
  • 项目类别:
RNA aptamers as cell surface receptor agonists and siRNA delivery agents
RNA适体作为细胞表面受体激动剂和siRNA递送剂
  • 批准号:
    7737559
  • 财政年份:
    2009
  • 资助金额:
    $ 29.6万
  • 项目类别:
RNA aptamers as cell surface receptor agonists and siRNA delivery agents
RNA适体作为细胞表面受体激动剂和siRNA递送剂
  • 批准号:
    8326373
  • 财政年份:
    2009
  • 资助金额:
    $ 29.6万
  • 项目类别:
E2F, INTIMAL HYPERPLASIA
E2F,内膜增生
  • 批准号:
    6954604
  • 财政年份:
    2005
  • 资助金额:
    $ 29.6万
  • 项目类别:
E2F-mediated Control of Vascular Growth and Remodeling
E2F 介导的血管生长和重塑控制
  • 批准号:
    6856580
  • 财政年份:
    2003
  • 资助金额:
    $ 29.6万
  • 项目类别:

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  • 财政年份:
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