TY - JOUR
T1 - Structure, backbone dynamics and interactions with RNA of the C-terminal RNA-binding domain of a mouse neural RNA-binding protein, Musashi1
AU - Nagata, Takashi
AU - Kanno, Reisuke
AU - Kurihara, Yasuyuki
AU - Uesugi, Seiichi
AU - Imai, Takao
AU - Sakakibara, Shin ichi
AU - Okano, Hideyuki
AU - Katahira, Masato
N1 - Funding Information:
We thank Mr A. Hiwatashi, Mr M. Miyauchi and Mr M. Ohtsu for their contributions in an early stage of this study, and Mr H. Kobayashi for the measurement in the chemical shift perturbation experiments. This work was supported by Grants-in-Aid from the Ministry of Education, Science, Sports and Culture of Japan to M.K. (numbers 10129205, 10179101, 09680648 and 06276103) and to H.O. (no. 08260101). T.I. is a research fellow of Japan Society for Promotion of Science and was supported by a grant from the Ministry of Education, Science, Sports and Culture of Japan.
PY - 1999/3/26
Y1 - 1999/3/26
N2 - Musashi1 is an RNA-binding protein abundantly expressed in the developing mouse central nervous system. Its restricted expression in neural precursor cells suggests that it is involved in the regulation of asymmetric cell division. Musashi1 contains two ribonucleoprotein (RNP)-type RNA-binding domains (RBDs), RBD1 and RBD2. Our previous studies showed that RBD1 alone binds to RNA, while the binding of RBD2 is not detected under the same conditions. Joining of RBD2 to RBD1, however, increases the affinity to greater than that of RBD1 alone, indicating that RBD2 contributes to RNA-binding. We have determined the three-dimensional solution structure of the C-terminal RBD (RBD2) of Musashi1 by NMR. It folds into a compact up structure comprising a four-stranded antiparallel β-sheet packed against two α-helices, which is characteristic of RNP-type RBDs. Special structural features of RBD2 include a β-bulge in β2 and a shallow twist of the β-sheet. The smaller 1H-15N nuclear Overhauser enhancement values for the residues of loop 3 between β2 and β3 suggest that this loop is flexible in the time-scale of nano- to picosecond order. The smaller 15N T2 values for the residues around the border between α2 and the following loop (loop 5) suggest this region undergoes conformational exchange in the milli- to microsecond time-scale. Chemical shift perturbation analysis indicated that RBD2 binds to an RNA oligomer obtained by in vitro selection under the conditions for NMR measurements, and thus the nature of the weak RNA-binding of RBD2 was successfully characterized by NMR, which is otherwise difficult to assess. Mainly the residues of the surface composed of the four-stranded β-sheet, loops and C-terminal region are involved in the interaction. The appearance of side-chain NH proton resonances of arginine residues of loop 3 and imino proton resonances of RNA bases upon complex formation suggests the formation of intermolecular hydrogen bonds. The structural arrangement of the rings of the conserved aromatic residues of β2 and β3 is suitable for stacking interaction with RNA bases, known to be one of the major protein-RNA interactions, but a survey of the perturbation data suggested that the stacking interaction is not ideally achieved in the complex, which may be related to the weaker RNA-binding of RBD2.
AB - Musashi1 is an RNA-binding protein abundantly expressed in the developing mouse central nervous system. Its restricted expression in neural precursor cells suggests that it is involved in the regulation of asymmetric cell division. Musashi1 contains two ribonucleoprotein (RNP)-type RNA-binding domains (RBDs), RBD1 and RBD2. Our previous studies showed that RBD1 alone binds to RNA, while the binding of RBD2 is not detected under the same conditions. Joining of RBD2 to RBD1, however, increases the affinity to greater than that of RBD1 alone, indicating that RBD2 contributes to RNA-binding. We have determined the three-dimensional solution structure of the C-terminal RBD (RBD2) of Musashi1 by NMR. It folds into a compact up structure comprising a four-stranded antiparallel β-sheet packed against two α-helices, which is characteristic of RNP-type RBDs. Special structural features of RBD2 include a β-bulge in β2 and a shallow twist of the β-sheet. The smaller 1H-15N nuclear Overhauser enhancement values for the residues of loop 3 between β2 and β3 suggest that this loop is flexible in the time-scale of nano- to picosecond order. The smaller 15N T2 values for the residues around the border between α2 and the following loop (loop 5) suggest this region undergoes conformational exchange in the milli- to microsecond time-scale. Chemical shift perturbation analysis indicated that RBD2 binds to an RNA oligomer obtained by in vitro selection under the conditions for NMR measurements, and thus the nature of the weak RNA-binding of RBD2 was successfully characterized by NMR, which is otherwise difficult to assess. Mainly the residues of the surface composed of the four-stranded β-sheet, loops and C-terminal region are involved in the interaction. The appearance of side-chain NH proton resonances of arginine residues of loop 3 and imino proton resonances of RNA bases upon complex formation suggests the formation of intermolecular hydrogen bonds. The structural arrangement of the rings of the conserved aromatic residues of β2 and β3 is suitable for stacking interaction with RNA bases, known to be one of the major protein-RNA interactions, but a survey of the perturbation data suggested that the stacking interaction is not ideally achieved in the complex, which may be related to the weaker RNA-binding of RBD2.
KW - Dynamics
KW - Musashi
KW - NMR
KW - RNA-binding protein
KW - RNA-protein interaction
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U2 - 10.1006/jmbi.1999.2596
DO - 10.1006/jmbi.1999.2596
M3 - Article
C2 - 10080895
AN - SCOPUS:0033605940
SN - 0022-2836
VL - 287
SP - 315
EP - 330
JO - Journal of Molecular Biology
JF - Journal of Molecular Biology
IS - 2
ER -