An additional ribosome-binding site on mRNA of highly expressed genes and a bifunctional site on the colicin fragment of 16S rRNA from Escherichia coli: important determinants of the efficiency of translation-initiation

doi:10.1093/nar/17.8.2973

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Nucleic Acids Research, 1989, Vol. 17, No. 8 2973-2985
© 1989

MOLECULAR BIOLOGY

An additional ribosome-binding site on mRNA of highly expressed genes and a bifunctional site on the colicin fragment of 16S rRNA from Escherichia coli: important determinants of the efficiency of translation-initiation

T.A. Thanaraj and M.W. Pandit^*

Centre for Cellular and Molecular Biology Hyderabad 500 007, India

^*To whom correspondence should be addressed

Received February 1, 1989. Revised March 23, 1989. Accepted March 23, 1989.

For various genes of E.coli, three regions (–55 to –1;–35 to –1; –21 to –1)5' to AUG codonon mRNA were searched for sites of interaction with colicinfragment of 16S rRNA. The detailed sequence comparison pointsout that apart from Shine-Dalgarno base pairing, an additionalribosome binding site, a subsequence of 5'-UGAUCC-3' invariablyexists in mRNA for highly expressed genes. Poorly expressedgenes appear to be controlled by only Shine-Dalgarno base pairing.The analysis indicates that in the initiator region, the –55to –1 region contains the signal which decides the efficiencyof the translation-initiation. The site on 16S rRNA, 5'-GGAUCA-3'at position 1529, that can base pair to the above site, hasa recognition site on 23S rRNA at position 2390. In the lightof the conserved nature and accessibility of these sites, itis proposed that the site on 16S rRNA plays a bifunctional role-initiallyit binds to mRNA from highly expressed genes to form a stable30S initiation complex, and upon association with 505 subunitit exchanges base pairing with 23S rRNA, thus leaving the siteon mRNA free.

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