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针对 I 型胶原合成的抗纤维化药物的发现进展。

Progress towards discovery of antifibrotic drugs targeting synthesis of type I collagen.

机构信息

King Abdullah University of Science and Technology (KAUST), Bldg 16, Rm 3124, Saudi Arabia.

出版信息

Curr Med Chem. 2011;18(22):3410-6. doi: 10.2174/092986711796504691.

DOI:10.2174/092986711796504691
PMID:21728959
Abstract

Type I collagen is the most abundant protein in human body. Fibrosis is characterized by excessive synthesis of type I collagen in parenchymal organs. It is a leading cause of morbidity and mortality worldwide, about 45% of all natural deaths are attributable to some fibroproliferative disease. There is no cure for fibrosis. To find specific antifibrotic therapy targeting type I collagen, critical molecular interactions regulating its synthesis must be elucidated. Type I and type III collagen mRNAs have a unique sequence element at the 5' end, the 5' stem-loop. This stem-loop is not found in any other mRNA. We cloned LARP6 as the protein which binds collagen 5' stem-loop with high affinity and specificity. Mutation of the 5' stem-loop or knock down of LARP6 greatly diminishes collagen expression. Mice with mutation of the 5' stem-loop are resistant to development of liver fibrosis. LARP6 associates collagen mRNAs with filaments composed of nonmuscle myosin; disruption of these filaments abolishes synthesis of type I collagen. Thus, LARP6 dependent collagen synthesis is the specific mechanism of high collagen expression seen in fibrosis. We developed fluorescence polarization (FP) method to screen for drugs that can inhibit binding of LARP6 to 5' stem-loop RNA. FP is high when LARP6 is bound, but decreases to low levels when the binding is competed out. Thus, by measuring decrease in FP it is possible to identify chemical compounds that can dissociate LARP6 from the 5' stem-loop. The method is simple, fast and suitable for high throughput screening.

摘要

I 型胶原蛋白是人体中最丰富的蛋白质。纤维化的特征是实质器官中 I 型胶原蛋白的过度合成。它是全世界发病率和死亡率的主要原因,大约 45%的自然死亡归因于某些纤维增生性疾病。纤维化目前无法治愈。为了找到针对 I 型胶原蛋白的特异性抗纤维化治疗方法,必须阐明调节其合成的关键分子相互作用。I 型和 III 型胶原蛋白的 mRNA 在 5'端具有独特的序列元件,即 5'茎环。这个茎环在任何其他 mRNA 中都找不到。我们克隆了 LARP6 作为与胶原蛋白 5'茎环具有高亲和力和特异性结合的蛋白质。5'茎环的突变或 LARP6 的敲低大大减少了胶原蛋白的表达。5'茎环突变的小鼠对肝纤维化的发展具有抗性。LARP6 将胶原蛋白 mRNAs 与由非肌肉肌球蛋白组成的细丝相关联;这些细丝的破坏会阻止 I 型胶原蛋白的合成。因此,LARP6 依赖的胶原蛋白合成是纤维化中高胶原蛋白表达的特异性机制。我们开发了荧光偏振 (FP) 方法来筛选可以抑制 LARP6 与 5'茎环 RNA 结合的药物。当 LARP6 结合时,FP 很高,但当结合被竞争掉时,FP 会降低到低水平。因此,通过测量 FP 的降低,可以识别出可以将 LARP6 从 5'茎环上解离的化学化合物。该方法简单、快速,适用于高通量筛选。

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