Affiliation:
1. Erfelijkheidsleer en Microbiologie, Vrije Universiteit Brussel
2. Laboratoire de Microbiologie, Université Libre de Bruxelles and Institut de Recherches Microbiologiques J.-M. Wiame, B-1070 Brussels, Belgium
Abstract
ABSTRACT
Sequencing a 8,519-bp segment of the
Sulfolobus acidocaldarius
genome revealed the existence of a tightly packed bipolar pyrimidine gene cluster encoding the enzymes of de novo UMP synthesis. The G+C content of 35.3% is comparable to that of the entire genome, but intergenic regions exhibit a considerably lower percentage of strong base pairs. Coding regions harbor the classical excess of purines on the coding strand, whereas intergenic regions do not show this bias. Reverse transcription-PCR and primer extension experiments demonstrated the existence of two polycistronic messengers,
pyrEF-orf8
and
pyrBI-orf1-pyrCD-orf2-orf3-orf4
, initiated from a pair of divergent and partially overlapping promoters. The gene order and the grouping in two wings of a bipolar operon constitute a novel organization of
pyr
genes that also occurs in the recently determined genome sequences of
Sulfolobus solfataricus
P2 and
Sulfolobus tokodaii
strain 7; the configuration appears therefore characteristic of
Sulfolobus
. The quasi-leaderless
pyrE
and
pyrB
genes do not bear a Shine-Dalgarno sequence, whereas the initiation codon of promoter-distal genes is preceded at an appropriate distance by a sequence complementary to the 3′ end of 16S rRNA. The polycistronic nature of the
pyr
messengers and the existence of numerous overlaps between contiguous open reading frames suggests the existence of translational coupling.
pyrB
transcription was shown to be approximately twofold repressed in the presence of uracil. The mechanism underlying this modulation is as yet unknown, but it appears to be of a type different from the various attenuation-like mechanisms that regulate
pyrB
transcription in bacteria. In contrast, the
pyrE-pyrB
promoter/control region harbors direct repeats and imperfect palindromes reminiscent of target sites for the binding of a hypothetical regulatory protein(s).
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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