GAP-SCAN DELETION ANALYSIS OF BACILLUS-SUBTILIS RNASE P-RNA

被引:28
作者
WAUGH, DS
PACE, NR
机构
[1] INDIANA UNIV, DEPT BIOL, BLOOMINGTON, IN 47405 USA
[2] INDIANA UNIV, INST MOLEC & CELLULAR BIOL, BLOOMINGTON, IN 47405 USA
关键词
RNASE-P; RIBOZYME; TRANSFER RNA PROCESSING; DELETION ANALYSIS;
D O I
10.1096/fasebj.7.1.7678561
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
We carried out an exhaustive deletion analysis of Bacillus subtilis ribonuclease P (RNase P) RNA, seeking sequences that are essential for its catalytic activity. A collection of partially deleted RNase P RNA genes was used to construct templates for synthesis, by in vitro transcription, of circularly permuted RNA molecules that lack various wild-type sequences. The mutant RNAs were assayed for catalytic activity in vitro, using a precursor of B. subtilis tRNA(Asp) as a substrate. Gap-scan deletion analysis revealed that most of the RNase P RNA sequence is important for activity; only two substantive deletions did not dramatically inhibit pre-tRNA processing in vitro. One part of the molecule (nucleotides 225-270) seemed particularly sensitive to deletion, but considering a collection of mutants with overlapping deletion gaps, it was possible to remove every residue in the RNase P RNA without completely abolishing its catalytic activity. Thus, the catalytic mechanism of RNase P does not depend absolutely on a single, particular nucleotide or local sequence for activity.
引用
收藏
页码:188 / 195
页数:8
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