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剪接抑制素A作用于剪接因子3b(SF3b),并抑制前体信使核糖核酸(pre-mRNA)的剪接和核滞留。

Spliceostatin A targets SF3b and inhibits both splicing and nuclear retention of pre-mRNA.

作者信息

Kaida Daisuke, Motoyoshi Hajime, Tashiro Etsu, Nojima Takayuki, Hagiwara Masatoshi, Ishigami Ken, Watanabe Hidenori, Kitahara Takeshi, Yoshida Tatsuhiko, Nakajima Hidenori, Tani Tokio, Horinouchi Sueharu, Yoshida Minoru

机构信息

Chemical Genetics Laboratory, RIKEN, 2-1 Hirosawa, Wako, Saitama 351-0198, Japan.

出版信息

Nat Chem Biol. 2007 Sep;3(9):576-83. doi: 10.1038/nchembio.2007.18. Epub 2007 Jul 22.

Abstract

The removal of intervening sequences from transcripts is catalyzed by the spliceosome, a multicomponent complex that assembles on the newly synthesized pre-mRNA. Pre-mRNA translation in the cytoplasm leads to the generation of aberrant proteins that are potentially harmful. Therefore, tight control to prevent undesired pre-mRNA export from the nucleus and its subsequent translation is an essential requirement for reliable gene expression. Here, we show that the natural product FR901464 (1) and its methylated derivative, spliceostatin A (2), inhibit in vitro splicing and promote pre-mRNA accumulation by binding to SF3b, a subcomplex of the U2 small nuclear ribonucleoprotein in the spliceosome. Importantly, treatment of cells with these compounds resulted in leakage of pre-mRNA to the cytoplasm, where it was translated. Knockdown of SF3b by small interfering RNA induced phenotypes similar to those seen with spliceostatin A treatment. Thus, the inhibition of pre-mRNA splicing during early steps involving SF3b allows unspliced mRNA leakage and translation.

摘要

转录本中内含序列的去除由剪接体催化,剪接体是一种多组分复合物,它在新合成的前体mRNA上组装。前体mRNA在细胞质中的翻译会导致产生潜在有害的异常蛋白质。因此,严格控制以防止不需要的前体mRNA从细胞核输出及其后续翻译是可靠基因表达的基本要求。在此,我们表明天然产物FR901464(1)及其甲基化衍生物剪接抑制素A(2)通过与SF3b结合来抑制体外剪接并促进前体mRNA积累,SF3b是剪接体中U2小核核糖核蛋白的一个亚复合物。重要的是,用这些化合物处理细胞会导致前体mRNA泄漏到细胞质中并在那里进行翻译。用小干扰RNA敲低SF3b会诱导出与剪接抑制素A处理相似的表型。因此,在涉及SF3b的早期步骤中对前体mRNA剪接的抑制会导致未剪接的mRNA泄漏和翻译。

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