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J Biol Chem, Vol. 274, Issue 30, 21342-21348, July 23, 1999
From the Department of Genetics, University of Washington,
Seattle, Washington 98195-7360
For 25 mutant alleles of ret1,
encoding the second largest subunit of yeast RNA polymerase III, we
have studied the polymerase III nuclease activity, measuring both the
total yield and dinucleotide product composition. Mutations affecting
amino acids 309-325 gave slightly elevated nuclease activity. In
region 367-376, two mutations gave 12-15-fold increased nuclease
activity. Our results do not support the catalytic role in nuclease
activity proposed for the conserved DDRD motif in this region (Shirai,
T., and Go, M. (1991) Proc. Natl. Acad. Sci. U. S. A. 88, 9056-9060). Mutations centered on a basic region from amino acids 480 to 490, which aligns with Escherichia coli
-subunit
sequences between Rifr clusters I and II, produce
changes in the relative yields of A- and G-containing dinucleotides.
Four such mutant polymerases pause during elongation at GPy sequences
and, in addition, have a reduced frequency of termination at
T5 terminator sequences. We propose that the side chains of
these mutationally altered amino acids are in direct contact with bases
in the RNA-DNA hybrid very near the growing 3'-end. Two mutations in
domain I near the C terminus produced very large increases in
exonuclease activity and strongly increased termination, suggesting
that this region also contacts the nascent RNA in the hybrid region.
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