DXO/Rai1 enzymes remove 5 '-end FAD and dephospho-CoA caps on RNAs

Doamekpor Selom K.; Grudzien-Nogalska Ewa; Mlynarska-Cieslak Agnieszka; Kowalska Joanna; Kiledjian Megerditch; Tong Liang

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DXO/Rai1 enzymes remove 5 '-end FAD and dephospho-CoA caps on RNAs

机译：DXO / RAI1酶在RNA上删除5' - 敦等FAD和Dephospho-CoA帽

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In eukaryotes, the DXO/Rai1 enzymes can eliminate most of the incomplete and non-canonical NAD caps through their decapping, deNADding and pyrophosphohydrolase activities. Here, we report that these enzymes can also remove FAD and dephospho-CoA (dpCoA) non-canonical caps from RNA, and we have named these activities deFADding and deCoAping. The crystal structures of mammalian DXO with 3'-FADP or CoA and fission yeast Rai1 with 3'-FADP provide elegant insight to these activities. FAD and CoA are accommodated in the DXO/Rai1 active site by adopting folded conformations. The flavin of FAD and the pantetheine group of CoA contact the same region at the bottom of the active site tunnel, which undergoes conformational changes to accommodate the different cap moieties. We have developed FAD-capQ to detect and quantify FAD-capped RNAs and determined that FAD caps are present on short RNAs (with less than similar to 200 nucleotides) in human cells and that these RNAs are stabilized in the absence of DXO.

机译：在真核生物中，DXO / RAI1酶可以通过拆下，溶解和焦磷酸酶活性消除大多数不完全和非典型的NAD帽。在这里，我们报告说，这些酶也可以从RNA中除去配对和脱磷 - COA（DPCOA）非规范帽，我们将这些活动命名为碎片和腐蚀。哺乳动物DXO的晶体结构与3'-FADP或COA和裂变酵母RAI1，3'-FADP为这些活动提供了优雅的见解。 FAD和COA通过采用折叠的构象，在DXO / RAI1活动站点中容纳在DXO / RAI1活动站点中。 FAD的黄素和粘连的COA组与活性部位隧道底部的相同区域接触，该区域经过一致性变化以适应不同的盖子部分。我们已经开发了FAD-CAPQ以检测和定量FAD封端的RNA，并确定在人体细胞中的短RNA（少于200个核苷酸）上存在FAD帽，并且这些RNA在没有DXO的情况下稳定。

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《Nucleic Acids Research》 |2020年第11期|共13页
作者
Doamekpor Selom K.; Grudzien-Nogalska Ewa; Mlynarska-Cieslak Agnieszka; Kowalska Joanna; Kiledjian Megerditch; Tong Liang;
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作者单位

Columbia Univ Dept Biol Sci New York NY 10027 USA;

Rutgers State Univ Dept Cell Biol &

Neurosci Piscataway NJ 08854 USA;

Univ Warsaw Fac Phys Inst Expt Phys Div Biophys PL-02093 Warsaw Poland;

Univ Warsaw Fac Phys Inst Expt Phys Div Biophys PL-02093 Warsaw Poland;

Rutgers State Univ Dept Cell Biol &

Neurosci Piscataway NJ 08854 USA;

Columbia Univ Dept Biol Sci New York NY 10027 USA;

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正文语种 eng
中图分类生物化学;
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1. DXO/Rai1 enzymes remove 5 '-end FAD and dephospho-CoA caps on RNAs [J] . Doamekpor Selom K., Grudzien-Nogalska Ewa, Mlynarska-Cieslak Agnieszka, Nucleic Acids Research . 2020,第11期

机译：DXO / RAI1酶在RNA上删除5' - 敦等FAD和Dephospho-CoA帽
2. DXO/Rai1 enzymes remove 5′-end FAD and dephospho-CoA caps on RNAs [J] . Selom K Doamekpor, Ewa Grudzien-Nogalska, Agnieszka Mlynarska-Cieslak, Nucleic acids research . 2020,第11期

机译：DXO / Rai1酶在RNA上移除5'-末端的使用和Dephospho-CoA帽
3. Judge, Jury, and Executioner: DXO Functions as a Decapping Enzyme and Exoribonuclease in Pre-mRNA Quality Control [J] . MugridgeJ.S., GrossJ.D. Molecular cell . 2013,第1期

机译：法官，陪审团和执行人：DXO在mRNA纯化前的质量控制中充当脱盖酶和外切核酸酶的功能
4. ENZYME ENGINEERING OF FUNGAL-DERIVED FAD-GDH BY CIRCULAR PERMUTATION [C] . Satoru Ishihara, Kyoichi Nishio, Satoshi Koikeda, Conference on biochemical and molecular engineering . 2019

机译：循环置换法制备真菌衍生的FAD-GDH的酶工程
5. Functional characterization of trypanosoma mRNA capping enzymes and archaeal RNA ligase [D] . Takagi, Yuko 2011

机译：锥虫瘤mRNA封端酶和古细菌RNA连接酶的功能表征
6. DXO/Rai1 enzymes remove 5′-end FAD and dephospho-CoA caps on RNAs [O] . Selom K Doamekpor, Ewa Grudzien-Nogalska, Agnieszka Mlynarska-Cieslak, 2020

机译：DXO / Rai1酶去除RNA上的5端FAD和去磷酸CoA帽
7. DXO/Rai1 enzymes remove 5′-end FAD and dephospho-CoA caps on RNAs [O] . Selom K Doamekpor, Ewa Grudzien-Nogalska, Agnieszka Mlynarska-Cieslak, 2020

机译：DXO / Rai1酶在RNA上移除5'-末端的使用和Dephospho-CoA帽

DXO/Rai1 enzymes remove 5 '-end FAD and dephospho-CoA caps on RNAs

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