Evaluation of the information content of RNA structure mapping data for secondary structure prediction

被引:44
|
作者
Quarrier, Scott [2 ]
Martin, Joshua S. [2 ]
Davis-Neulander, Lauren [1 ]
Beauregard, Arthur [2 ]
Laederach, Alain [1 ,2 ]
机构
[1] Wadsworth Ctr, Albany, NY 12208 USA
[2] SUNY Albany, Program Biomed Sci, Albany, NY 12208 USA
关键词
RNA structure; chemical mapping; DMS; footprinting; secondary structure; CAPILLARY-ELECTROPHORESIS; FOOTPRINTING ANALYSIS; THERMOPHILA RIBOZYME; PARTITION-FUNCTION; TERTIARY STRUCTURE; CRYSTAL-STRUCTURE; BASE-PAIRS; MOLECULE; SHAPE; MINIMIZATION;
D O I
10.1261/rna.1988510
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Structure mapping experiments (using probes such as dimethyl sulfate [DMS], kethoxal, and T1 and V1 RNases) are used to determine the secondary structures of RNA molecules. The process is iterative, combining the results of several probes with constrained minimum free-energy calculations to produce a model of the structure. We aim to evaluate whether particular probes provide more structural information, and specifically, how noise in the data affects the predictions. Our approach involves generating "decoy" RNA structures (using the sFold Boltzmann sampling procedure) and evaluating whether we are able to identify the correct structure from this ensemble of structures. We show that with perfect information, we are always able to identify the optimal structure for five RNAs of known structure. We then collected orthogonal structure mapping data (DMS and RNase T1 digest) under several solution conditions using our high-throughput capillary automated footprinting analysis (CAFA) technique on two group I introns of known structure. Analysis of these data reveals the error rates in the data under optimal (low salt) and suboptimal solution conditions (high MgCl2). We show that despite these errors, our computational approach is less sensitive to experimental noise than traditional constraint-based structure prediction algorithms. Finally, we propose a novel approach for visualizing the interaction of chemical and enzymatic mapping data with RNA structure. We project the data onto the first two dimensions of a multidimensional scaling of the sFold-generated decoy structures. We are able to directly visualize the structural information content of structure mapping data and reconcile multiple data sets.
引用
收藏
页码:1108 / 1117
页数:10
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