AUUUA is not sufficient to promote poly(A) shortening and degradation of an mRNA: the functional sequence within AU-rich elements may be UUAUUUA(U/A)(U/A).

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Mol Cell Biol. 1994 December; 14(12): 7984-7995

AUUUA is not sufficient to promote poly(A) shortening and degradation of an mRNA: the functional sequence within AU-rich elements may be UUAUUUA(U/A)(U/A).

C A Lagnado, C Y Brown and G J Goodall

Hanson Centre for Cancer Research, Division of Human Immunology, Adelaide, South Australia.

ABSTRACT

AU-rich elements (AREs) in the 3' untranslated regions of severalcytokine and oncogene mRNAs have been shown to function as signalsfor rapid mRNA degradation, and it is assumed that the manyother cytokine and oncogene mRNAs that contain AU-rich sequencesin the 3' untranslated region are similarly targeted for rapidturnover. We have used a chimeric gene composed mostly of growthhormone sequences with expression driven by the c-fos promoterto investigate the minimal sequence required to act as a functionaldestabilizing element and to monitor the effect of these sequenceson early steps in the degradation pathway. We find that neitherAUUUA, UAUUUA, nor AUUUAU can function as a destabilizing element.However, the sequence UAUUUAU, when present in three copies,is sufficient to destabilize a chimeric mRNA. We propose thatthis sequence functions by virtue of being a sufficient portionof the larger sequence, UUAUUUA(U/A)(U/A), that we propose formsthe optimal binding site for a destabilizing factor. The destabilizingeffect depends on the number of copies of this proposed bindingsite and their degree of mismatch in the first two and lasttwo positions, with mismatches in the AUUUA sequence not beingtolerated. We found a strict correlation between the effectof an ARE on degradation rate and the effect on the rate ofpoly(A) shortening, consistent with deadenylation being thefirst and rate-limiting step in degradation, and the step stimulatedby destabilizing AREs. Deadenylation was observed to occur inat least two phases, with an oligo(A) intermediate transientlyaccumulating, consistent with the suggestion that the degradationprocesses may be similar in yeast and mammalian cells. AREsthat are especially U rich and contain no UUAUUUA(U/A)(U/A)motifs failed to influence the degradation rate or the deadenylationrate, either when downstream of suboptimal destabilizing AREsor when alone.

Mol Cell Biol. 1994 December; 14(12): 7984-7995

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