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1ST4

Structure of DcpS bound to m7GpppA

Summary for 1ST4
Entry DOI10.2210/pdb1st4/pdb
Related1ST0
DescriptormRNA decapping enzyme, P1-7-METHYLGUANOSINE-P3-ADENOSINE-5',5'-TRIPHOSPHATE, YTTRIUM (III) ION, ... (4 entities in total)
Functional Keywordsrna decay, exosome, decapping, hit protein, messenger rna, mrna, cap, rna binding protein
Biological sourceHomo sapiens (human)
Cellular locationCytoplasm: Q96C86
Total number of polymer chains2
Total formula weight79119.00
Authors
Gu, M.,Fabrega, C.,Liu, S.W.,Liu, H.,Kiledjian, M.,Lima, C.D. (deposition date: 2004-03-24, release date: 2004-04-13, Last modification date: 2023-08-23)
Primary citationGu, M.,Fabrega, C.,Liu, S.W.,Liu, H.,Kiledjian, M.,Lima, C.D.
Insights into the structure, mechanism, and regulation of scavenger mRNA decapping activity
Mol.Cell, 14:67-80, 2004
Cited by
PubMed Abstract: Complete removal of residual N-7 guanine cap from degraded messenger RNA is necessary to prevent accumulation of intermediates that might interfere with RNA processing, export, and translation. The human scavenger decapping enzyme, DcpS, catalyzes residual cap hydrolysis following mRNA degradation, releasing N-7 methyl guanosine monophosphate and 5'-diphosphate terminated cap or mRNA products. DcpS structures bound to m(7)GpppG or m(7)GpppA reveal an asymmetric DcpS dimer that simultaneously creates an open nonproductive DcpS-cap complex and a closed productive DcpS-cap complex that alternate via 30 A domain movements. Structural and biochemical analysis suggests an autoregulatory mechanism whereby premature decapping mRNA is prevented by blocking the conformational changes that are required to form a closed productive active site capable of cap hydrolysis.
PubMed: 15068804
DOI: 10.1016/S1097-2765(04)00180-7
PDB entries with the same primary citation
Experimental method
X-RAY DIFFRACTION (2.02 Å)
Structure validation

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數據於2024-11-13公開中

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