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Title: Solution structure of loop A from the hairpin ribozyme from tobacco ringspot virus satellite

Journal Article · · Biochemistry (Eaton)
DOI:https://doi.org/10.1021/bi952985g· OSTI ID:494233
;  [1]
  1. Univ. of California, Berkeley, CA (United States)

The solution structure of loop A form the hairpin ribozyme fund in the minus strand of tobacco ringspot virus satellite has been determined by NMR spectroscopy. The ribozyme consists of two internal loops flanked by short helices: loop A and helices I and II include the substrate and substrate binding site; loop B and helices III and IV are the catalytic domain. Loop A is a symmetric internal loop of eight nucleotides that contains the cleavage site. The 2-amino group of the guanine immediately 3{prime} to the cleavage site is essential for catalysis. NMR results show that this guanine forms a sheared G{sm_bullet}A base pair. The cytosine residue immediately 5{prime} to the cleavage site forms an AH{sup +}{sm_bullet}C base pair with an adenine whose pK{sub a} is shifted to 6.2 to allow partial protonation near neutral pH. Although the residues flanking the cleavage site are stacked in an A-form pattern, the phosphodiester backbone next to the cleavage site on the 3{prime} side is splayed apart. This places the following base-a uracil-in the expanded major groove. The conformational flexibility and the lack of steric hindrance of the uracil as well as the unoccupied Watson-Crick positions on the sheared G{sm_bullet}A base pair can allow loop A to specifically interact with the catalytic domain (loop B) without drastically changing its own conformation. The three-dimensional structure of loop A provides explanations for previously published mutation and structural mapping results. 38 refs., 10 figs., 2 tabs.

DOE Contract Number:
FG03-86ER60406; FG05-86ER75281
OSTI ID:
494233
Journal Information:
Biochemistry (Eaton), Vol. 35, Issue 19; Other Information: PBD: 14 May 1996
Country of Publication:
United States
Language:
English

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