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J. Biol. Chem., Vol. 261, Issue 27, 12633-12642, 09, 1986
GJ Wu and RE Cannon
Both VARNA genes in the adenovirus genome are transcribed by host DNA-
dependent RNA polymerase III. Nevertheless, late in infection the mass
ratio of VARNA2 to VARNA1 in adenovirus-infected human KB or HeLa cells is
about 1:40. This difference is most likely due to differences in promoter
strength which may be attributed to sequence differences in the control
regions of the two genes. To investigate this possibility, the two genes
were cloned into separate plasmid molecules and their transcription
efficiencies were compared in vitro. The VARNA2 gene was transcribed in
vitro at least 50 times less efficiently than the VARNA1 gene. The
competing strengths of the two genes were similar, which suggests that the
B block sequence in the VARNA2 gene may be fully functional for
sequestering factors. Therefore, the major difference must reside in the
region upstream of the B block. By analyzing the hybrid RNAs transcribed
from a hybrid gene and 27 fused genes in which only the control region of
the VARNA1 gene was fused to various lengths of the 5'-flanking and the
coding regions of the VARNA2 gene, one major and one minor termination
site, which caused premature termination, were revealed downstream of the A
block sequence and in the 5'-flanking region of the VARNA2 gene,
respectively. The presence of termination sequences, a suboptimal
interblock spacing, and an altered A block sequence in the control region
may result in a weaker promoter in the VARNA2 gene.
Termination sequences in the control region of the Ad2-specific VARNA2 gene
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