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(Received for publication, December 7, 1994; and in revised form, January
23, 1995) RNA editing in Trypanosoma brucei results in the
addition and deletion of uridine residues within several mitochondrial
mRNAs. Editing is thought to be directed by guide RNAs and may proceed
via a chimeric guide RNA/mRNA intermediate. We have previously shown
that chimera-forming activity sediments with 19 S and 35-40 S
mitochondrial ribonucleoprotein particles (RNPs). In this report we
examine the involvement of RNA ligase in the production of chimeric
molecules in vitro. Two adenylylated proteins of 50 and 57 kDa
cosediment on glycerol gradients with RNA ligase activity as components
of the ribonucleoprotein particles. The two adenylylated proteins
differ in sequence and contain AMP linked via a phosphoamide bond. Both
proteins are deadenylylated by the addition of ligatable RNA substrate
with the concomitant release of AMP and by the addition of
pyrophosphate to yield ATP. Incubation with nonligatable RNA substrate
results in an accumulation of the adenylylated RNA intermediate. These
experiments identify the adenylylated proteins as RNA ligases. AMP
release from the mitochondrial RNA ligase is also concomitant with
chimera formation. Inhibition by nonhydrolyzable analogs indicates that
both RNA ligase and chimera-forming activities require
Volume 270,
Number 13,
Issue of March 31, 1995 pp. 7233-7240
©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
EVIDENCE FOR A CLEAVAGE-LIGATION MECHANISM OF TRYPANOSOMA
BRUCEI mRNA EDITING
-
bond
hydrolysis of ATP. Deadenylylation of the ligase inhibits chimera
formation. These results strongly suggest the involvement of RNA ligase
in in vitro chimera formation and support the
cleavage-ligation mechanism for kinetoplastid RNA editing.
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