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dc.contributor.authorMangus, David A.
dc.contributor.authorAmrani, Nadia
dc.contributor.authorJacobson, Allan
dc.date2022-08-11T08:09:33.000
dc.date.accessioned2022-08-23T16:35:32Z
dc.date.available2022-08-23T16:35:32Z
dc.date.issued1998-11-20
dc.date.submitted2009-03-24
dc.identifier.citationMol Cell Biol. 1998 Dec;18(12):7383-96.
dc.identifier.issn0270-7306 (Print)
dc.identifier.pmid9819425
dc.identifier.urihttp://hdl.handle.net/20.500.14038/38580
dc.description.abstractThe poly(A) tail of an mRNA is believed to influence the initiation of translation, and the rate at which the poly(A) tail is removed is thought to determine how fast an mRNA is degraded. One key factor associated with this 3'-end structure is the poly(A)-binding protein (Pab1p) encoded by the PAB1 gene in Saccharomyces cerevisiae. In an effort to learn more about the functional role of this protein, we used a two-hybrid screen to determine the factor(s) with which it interacts. We identified five genes encoding factors that specifically interact with the carboxy terminus of Pab1p. Of a total of 44 specific clones identified, PBP1 (for Pab1p-binding protein) was isolated 38 times. Of the putative interacting genes examined, PBP1 promoted the highest level of resistance to 3-aminotriazole (>100 mM) in constructs in which HIS3 was used as a reporter. We determined that a fraction of Pbp1p cosediments with polysomes in sucrose gradients and that its distribution is very similar to that of Pab1p. Disruption of PBP1 showed that it is not essential for viability but can suppress the lethality associated with a PAB1 deletion. The suppression of pab1Delta by pbp1Delta appears to be different from that mediated by other pab1 suppressors, since disruption of PBP1 does not alter translation rates, affect accumulation of ribosomal subunits, change mRNA poly(A) tail lengths, or result in a defect in mRNA decay. Rather, Pbp1p appears to function in the nucleus to promote proper polyadenylation. In the absence of Pbp1p, 3' termini of pre-mRNAs are properly cleaved but lack full-length poly(A) tails. These effects suggest that Pbp1p may act to repress the ability of Pab1p to negatively regulate polyadenylation.
dc.language.isoen_US
dc.relation<a href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=pubmed&cmd=Retrieve&list_uids=9819425&dopt=Abstract">Link to Article in PubMed</a>
dc.subjectAmino Acid Sequence
dc.subjectCarrier Proteins
dc.subjectCloning, Molecular
dc.subjectFungal Proteins
dc.subjectGene Deletion
dc.subjectGene Expression Regulation, Fungal
dc.subjectGenes, Fungal
dc.subjectGenes, Reporter
dc.subjectMolecular Sequence Data
dc.subjectNuclear Proteins
dc.subjectOligonucleotides
dc.subjectPoly A
dc.subjectPoly(A)-Binding Proteins
dc.subjectPolyribosomes
dc.subjectProtein Biosynthesis
dc.subjectRNA, Messenger
dc.subjectRNA-Binding Proteins
dc.subjectSaccharomyces cerevisiae
dc.subject*Saccharomyces cerevisiae Proteins
dc.subjectSequence Alignment
dc.subjectSequence Analysis, DNA
dc.subjectLife Sciences
dc.subjectMedicine and Health Sciences
dc.titlePbp1p, a factor interacting with Saccharomyces cerevisiae poly(A)-binding protein, regulates polyadenylation
dc.typeJournal Article
dc.source.journaltitleMolecular and cellular biology
dc.source.volume18
dc.source.issue12
dc.identifier.legacyfulltexthttps://escholarship.umassmed.edu/cgi/viewcontent.cgi?article=2445&amp;context=oapubs&amp;unstamped=1
dc.identifier.legacycoverpagehttps://escholarship.umassmed.edu/oapubs/1446
dc.identifier.contextkey794943
refterms.dateFOA2022-08-23T16:35:32Z
html.description.abstract<p>The poly(A) tail of an mRNA is believed to influence the initiation of translation, and the rate at which the poly(A) tail is removed is thought to determine how fast an mRNA is degraded. One key factor associated with this 3'-end structure is the poly(A)-binding protein (Pab1p) encoded by the PAB1 gene in Saccharomyces cerevisiae. In an effort to learn more about the functional role of this protein, we used a two-hybrid screen to determine the factor(s) with which it interacts. We identified five genes encoding factors that specifically interact with the carboxy terminus of Pab1p. Of a total of 44 specific clones identified, PBP1 (for Pab1p-binding protein) was isolated 38 times. Of the putative interacting genes examined, PBP1 promoted the highest level of resistance to 3-aminotriazole (>100 mM) in constructs in which HIS3 was used as a reporter. We determined that a fraction of Pbp1p cosediments with polysomes in sucrose gradients and that its distribution is very similar to that of Pab1p. Disruption of PBP1 showed that it is not essential for viability but can suppress the lethality associated with a PAB1 deletion. The suppression of pab1Delta by pbp1Delta appears to be different from that mediated by other pab1 suppressors, since disruption of PBP1 does not alter translation rates, affect accumulation of ribosomal subunits, change mRNA poly(A) tail lengths, or result in a defect in mRNA decay. Rather, Pbp1p appears to function in the nucleus to promote proper polyadenylation. In the absence of Pbp1p, 3' termini of pre-mRNAs are properly cleaved but lack full-length poly(A) tails. These effects suggest that Pbp1p may act to repress the ability of Pab1p to negatively regulate polyadenylation.</p>
dc.identifier.submissionpathoapubs/1446
dc.contributor.departmentDepartment of Molecular Genetics and Microbiology
dc.source.pages7383-96


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