NMR resonance assignments of RNase P protein from Thermotoga maritima

被引:0
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作者
Danyun Zeng
Benjamin P. Brown
Markus W. Voehler
Sheng Cai
Nicholas J. Reiter
机构
[1] Marquette University,Department of Chemistry
[2] Vanderbilt University,Chemical and Physical Biology Program
[3] Vanderbilt University,Center for Structural Biology
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NMR resonance assignment; RNase P; Protein–tRNA binding; Ribonucleoprotein; TALOS-N prediction;
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摘要
Ribonuclase P (RNase P) is an essential metallo-endonuclease that catalyzes 5′ precursor-tRNA (ptRNA) processing and exists as an RNA-based enzyme in bacteria, archaea, and eukaryotes. In bacteria, a large catalytic RNA and a small protein component assemble to recognize and accurately cleave ptRNA and tRNA-like molecular scaffolds. Substrate recognition of ptRNA by bacterial RNase P requires RNA–RNA shape complementarity, intermolecular base pairing, and a dynamic protein–ptRNA binding interface. To gain insight into the binding specificity and dynamics of the bacterial protein–ptRNA interface, we report the backbone and side chain 1H, 13C, and 15N resonance assignments of the hyperthermophilic Thermatoga maritima RNase P protein in solution at 318 K. Our data confirm the formation of a stable RNA recognition motif (RRM) with intrinsic heterogeneity at both the N- and C-terminus of the protein, consistent with available structural information. Comprehensive resonance assignments of the bacterial RNase P protein serve as an important first step in understanding how coupled RNA binding and protein–RNA conformational changes give rise to ribonucleoprotein function.
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页码:183 / 187
页数:4
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