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Affinity and Structural Analysis of the U1A RNA Recognition Motif with Engineered Methionines to Improve Experimental Phasing

Crystals (Basel). 2021-03; 
Yoshita Srivastava , Rachel Bonn-Breach , Sai Shashank Chavali , Geoffrey M Lippa , Jermaine L Jenkins , Joseph E Wedekind
Products/Services Used Details Operation
Gene Synthesis Synthetic genes for dmU1A, dmU1A(F37M/F77M), and TBP6.9(F34M/F37M/F77M) were produced by DNA synthesis and subcloned into pET28a (GenScript Inc., Piscataway, NJ, USA). Get A Quote
PCR Cloning and Subcloning Get A Quote

摘要

RNA plays a central role in all organisms and can fold into complex structures to orchestrate function. Visualization of such structures often requires crystallization, which can be a bottleneck in the structure-determination process. To promote crystallization, an RNA-recognition motif (RRM) of the U1A spliceosomal protein has been co-opted as a crystallization module. Specifically, the U1-snRNA hairpin II (hpII) single-stranded loop recognized by U1A can be transplanted into an RNA target to promote crystal contacts and to attain phase information via molecular replacement or anomalous diffraction methods using selenomethionine. Herein, we produced the F37M/F77M mutant of U1A to augment the phasing capability... More

關鍵詞

RNA crystallization; RNA-protein interactions; S–π interaction; U1A RRM; X-ray crystallography; anomalous diffraction; isothermal titration calorimetry; selenomethionine.
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