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Protein Chemical Modification Inside Living Cells Using Split Inteins

Methods Mol. Biol.. 2017-01; 
BorraRadhika, CamareroJul
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Recombinant Proteins … Genomic DNA from Nostoc punctiforme strain ATCC 29133/PCC 73102 (obtained from ATCC). 3. DNA encoding human YY1 proteins (cDNA clone IMAGE: 5261384) (can be obtained from many sources, eg, Genscript, USA). 4. TE buffer: 10 mM Tris–HCl, 1 mM EDTA, pH 8.0 … Get A Quote

摘要

Methods to visualize, track, measure, and perturb or activate proteins in living cells are central to biomedical efforts to characterize and understand the spatial and temporal underpinnings of life inside cells. Although fluorescent proteins have proven to be extremely useful for in vivo studies of protein function, their utility is inherently limited because their spectral and structural characteristics are interdependent. These limitations have spurred the creation of alternative approaches for the chemical labeling of proteins. We describe in this protocol the use of fluorescence resonance emission transfer (FRET)-quenched DnaE split-inteins for the site-specific labeling and concomitant fluorescenc... More

关键词

Fluorescence,Npu intein,Protein labeling,Protein trans-splicing,Split-in
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