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含有在三磷酸链中用 BH3、Se 和 NH 取代帽结构的 mRNAs 的翻译、稳定性和抗脱帽。

Translation, stability, and resistance to decapping of mRNAs containing caps substituted in the triphosphate chain with BH3, Se, and NH.

机构信息

Department of Biochemistry and Molecular Biology, Louisiana State University Health Sciences Center, Shreveport, Louisiana 71130-3932, USA.

出版信息

RNA. 2011 May;17(5):978-88. doi: 10.1261/rna.2430711. Epub 2011 Mar 29.

Abstract

Decapping is an essential step in multiple pathways of mRNA degradation. Previously, we synthesized mRNAs containing caps that were resistant to decapping, both to dissect the various pathways for mRNA degradation and to stabilize mRNA for more sustained protein expression. mRNAs containing an α-β CH(2) group are resistant to in vitro cleavage by the decapping enzyme hDcp2 but poorly translated. mRNAs containing an S substitution at the β-phosphate are well translated but only partially resistant to hDcp2. We now describe seven new cap analogs substituted at the β-phosphate with BH(3) or Se, or substituted at either the α-β or β-γ O with NH. The analogs differ in affinity for eIF4E and efficiency of in vitro incorporation into mRNA by T7 RNA polymerase. Luciferase mRNAs capped with these analogs differ in resistance to hDcp2 hydrolysis in vitro, translational efficiency in rabbit reticulocyte lysate and in HeLa cells, and stability in HeLa cells. Whereas mRNAs capped with m(2)(7,2'-O)Gpp(S)pG were previously found to have the most favorable properties of translational efficiency and stability in mammalian cells, mRNAs capped with m(7)Gpp(BH3)pm(7)G are translated with the same efficiency but are more stable. Interestingly, some mRNAs exhibit a lag of up to 60 min before undergoing first-order decay (t(1/2) ≅ 25 min). Only mRNAs that are efficiently capped, resistant to decapping in vitro, and actively translated have long lag phases.

摘要

脱帽是 mRNA 降解多条途径中的一个基本步骤。以前,我们合成了对脱帽具有抗性的含有帽的 mRNAs,以分别剖析各种 mRNA 降解途径,并稳定 mRNA 以实现更持续的蛋白质表达。含有 α-β CH(2) 基团的 mRNAs 对脱帽酶 hDcp2 的体外切割具有抗性,但翻译效率较低。含有 β-磷酸上 S 取代的 mRNAs 翻译效率较好,但仅部分抵抗 hDcp2。我们现在描述了七个新的帽类似物,它们在 β-磷酸上被 BH(3)或 Se 取代,或者在 α-β 或 β-γ O 上被 NH 取代。这些类似物在与 eIF4E 的亲和力和 T7 RNA 聚合酶体外掺入 mRNA 的效率上有所不同。用这些类似物加帽的荧光素酶 mRNAs 在体外对 hDcp2 水解的抗性、在兔网织红细胞裂解物和 HeLa 细胞中的翻译效率以及在 HeLa 细胞中的稳定性不同。虽然之前发现用 m(2)(7,2'-O)Gpp(S)pG 加帽的 mRNAs 具有在哺乳动物细胞中翻译效率和稳定性的最佳特性,但用 m(7)Gpp(BH3)pm(7)G 加帽的 mRNAs 具有相同的翻译效率但更稳定。有趣的是,一些 mRNAs 在经历一级衰减(t(1/2) ≅ 25 min)之前有长达 60 分钟的滞后。只有那些被高效加帽、对体外脱帽具有抗性和被积极翻译的 mRNAs 才有长的滞后期。

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