Drosophila Maternal Hsp83 mRNA Destabilization Is Directed by Multiple SMAUG Recognition Elements in the Open Reading Frame

SMAUG (SMG) is an RNA-binding protein that functions as a keycomponent of a transcript degradation pathway that eliminatesmaternal mRNAs in the bulk cytoplasm of activated Drosophilamelanogaster eggs. We previously showed that SMG destabilizesmaternal Hsp83 mRNA by recruiting the CCR4-NOT deadenylase totrigger decay; however, the cis-acting elements through whichthis was accomplished were unknown. Here we show that Hsp83transcript degradation is regulated by a major element, theHsp83 mRNA instability element (HIE), which maps to a 615-nucleotideregion of the open reading frame (ORF). The HIE is sufficientfor association of a transgenic mRNA with SMG protein as wellas for SMG-dependent destabilization. Although the Hsp83 mRNAis translated in the early embryo, we show that translationof the mRNA is not necessary for destabilization; indeed, theHIE functions even when located in an mRNA's 3' untranslatedregion. The Hsp83 mRNA contains eight predicted SMG recognitionelements (SREs); all map to the ORF, and six reside within theHIE. Mutation of a single amino acid residue that is essentialfor SMG's interaction with SREs stabilizes endogenous Hsp83transcripts. Furthermore, simultaneous mutation of all eightpredicted SREs also results in transcript stabilization. A plausiblemodel is that the multiple, widely distributed SREs in the ORFenable some SMG molecules to remain bound to the mRNA despiteribosome transit through any individual SRE. Thus, SMG can recruitthe CCR4-NOT deadenylase to trigger Hsp83 mRNA degradation despitethe fact that it is being translated.

INTRODUCTION

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INTRODUCTION

During animal oogenesis and early embryogenesis, posttranscriptionalgene regulation represents an essential mechanism for the controlof gene expression. Mature oocytes and early embryos are transcriptionallyquiescent and rely upon maternally supplied mRNAs depositedduring oogenesis (5, 37). Often, multiple mechanisms of posttranscriptionalcontrol act coordinately to precisely regulate the spatial andtemporal expression of proteins derived from these maternalmRNAs (23, 25).

In Drosophila melanogaster, the first 2 hours of embryogenesisare programmed by maternal mRNAs (38). A surprisingly largefraction of the protein coding genome is present in this maternaltranscript pool, with between one-half and two-thirds of allmRNAs being represented (16, 21, 35). Between a quarter anda third of these maternal mRNAs are eliminated during the maternal-to-zygotictransition that occurs prior to cellularization 3 hours afterfertilization (16, 21, 35, 37). Two degradation pathways directelimination of these transcripts (3, 4). The first is termedthe "maternal degradation pathway" because it is comprised ofan exclusively maternally encoded machinery that is triggeredupon egg activation, prior to fertilization (4, 36). The second,termed the "zygotic degradation pathway" since it requires bothfertilization and zygotic transcription, initiates approximately2 hours into embryonic development (4). The identification ofthese two decay activities allows maternal mRNAs to be categorizedaccording to whether they are targeted exclusively by the maternaldegradation pathway (e.g., nanos and polar granule component),exclusively by the zygotic degradation pathway (e.g., hunchback),by both activities (e.g., Hsp83 and string), or by neither (e.g.,rpA1, rp49, and ${alpha}$ Tub84B) (4, 16, 30, 31, 35, 36).

A major regulator of transcript destabilization is the RNA-bindingprotein SMAUG (SMG), whose function is required for eliminationof two-thirds of the mRNAs attacked by the maternal pathway(35). Analyses of Hsp83 mRNA have shown that SMG acts as a specificityfactor, recruiting the CCR4-NOT deadenylase, thus initiatingdecay through deadenylation (30). SMG's sterile-alpha motif(SAM) domain binds to specific stem-loops termed SMG recognitionelements (SREs) (2, 11-13, 32, 33). However, mutation of fourcomputationally predicted SREs in the open reading frame (ORF)of Hsp83 had no effect on the kinetics of transcript decay (30),raising several possibilities: that additional SREs might residein the Hsp83 mRNA, that SMG recognizes a novel cis element inthe Hsp83 mRNA, or that SMG's interaction with Hsp83 mRNA isindirect. Subsequent to those analyses it was shown that VTS1,the Saccharomyces cerevisiae homolog of SMG, can bind to SREswith a loop up to 7 nucleotides (nt) long, CNGGN_0-3 (1). Inaddition, the crystal structure indicated that SRE binding involveslimited sequence specificity, through recognition of the G residueat position 3 of the loop, in combination with recognition ofthe tertiary structure of the SRE (1). Thus, sequences thatadopt a similar shape and contain a G residue in the correctcontext—but do not match the current SRE consensus—could,in principle, also be bound by VTS1/SMG (1).

Given the complexity of VTS1/SMG transcript recognition, herewe took an unbiased approach to mapping the cis elements inthe Hsp83 mRNA that are required for destabilization, usinghybrid transgenic mRNAs that fused parts of the Hsp83 mRNA toparts of a stable mRNA, rpA1. These hybrid mRNAs enabled usto test different parts of the Hsp83 transcript for a role inmRNA destabilization via the maternal degradation machinery(i.e., in unfertilized eggs) and via SMG (i.e., in smg mutants).Using this strategy, we mapped a major instability element—whichwe have termed the Hsp83 mRNA instability element (HIE)—withinthe ORF. The HIE is sufficient to strongly destabilize rpA1mRNA when inserted into its ORF. The presence of the HIE withinthe ORF suggested that translation of the Hsp83 mRNA might berequired for transcript destabilization. However, the HIE retainedits activity as an instability element even when inserted intoa 3' untranslated region (UTR), indicating that translationis not needed. We show that the HIE functions together withauxiliary elements in the more 5' part of the Hsp83 ORF as wellas in its 3' UTR to direct transcript destabilization. One ofthese auxiliary elements is the previously identified Hsp83degradation element (HDE), a 97-nt region within the Hsp83 3'UTR (4).

Eight computationally predicted SREs are present in the Hsp83mRNA; all reside in its ORF, and six map to the HIE. We showthat the HIE is sufficient to direct association with SMG proteinas well as to confer SMG-dependent transcript instability. Asingle-amino-acid substitution that abrogates SMG's abilityto bind SREs prevents Hsp83 transcript destabilization. Furthermore,simultaneous mutation of all eight predicted SREs (without substantiallyaltering the coding capacity of the ORF) stabilizes the transcript.We conclude that SMG binds directly to the Hsp83 mRNA's ORF,thus recruiting the CCR4-NOT deadenylase and triggering transcriptelimination despite the fact that Hsp83 transcripts are activelytranslated.

MATERIALS AND METHODS

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MATERIALS AND METHODS

Fly stocks. Drosophila melanogaster wild-type stocks included y w¹¹¹⁸ andw¹¹¹⁸. Both of these genetic backgrounds were used for the generationof transgenic lines. Expression of pUASP constructs was inducedusing P[GAL4::VP16-nos.UTR] (41). Due to the presence of a recessivelethal mutation(s) on the smg¹ chromosome, smg mutants weresmg¹/Df(3L)Scf^R6 (12). In some cases, a transgenic P elementinsertion and the smg¹ allele were recombined onto the samechromosome, which resulted in the loss of the recessive lethalmutation, and thus, smg mutants were smg¹/smg¹. These geneticbackgrounds are noted in the text.

Construction of transgenes. (i) H-H-H. The construct H-H-H was designed by Arash Bashirullah and containsthe full-length Hsp83 transcript with a p53 epitope tag inserted3' to the start codon. This transgene was constructed by Ventpolymerase PCR of three fragments. The first Hsp83 fragment,H**, contained the 5' genomic region (876 nt), the 5' UTR (149nt), the intron (1,129 nt), and start codon, flanked with a5' BamHI site and a 3' ApaI site. The second Hsp83 fragment,*H*, was designed to contain the entire ORF with no start codonbut with the stop codon (2,151 nt) and the first 6 nt of the3' UTR. This fragment was flanked with a 5' ApaI site whiletwo nucleotides, GC, were introduced between the +2 and +3 positionsof the 3' UTR to generate a 3' AatII site. The third Hsp83 fragment,**H, was designed to contain the 3' UTR (407 nt) and downstreamgenomic DNA (1,281 nt total) flanked by 5' AatII and 3' KpnIsites. These three PCR fragments were subcloned into pBAAK,which is a modified pBluescript-SK vector that contained ApaIand AatII sites between the BamHI and KpnI sites, by digestionwith HindIII/KpnI and insertion of annealed oligonucleotidesApa-Aat-F and Aat-Apa-R (all oligonucleotide sequences are listedin Table S1 in the supplemented material). The 5' fragment wasfirst cloned into pBAAK at the BamHI/ApaI sites, generatingpBAAK-H**, and the 3' fragment was subsequently cloned at AatII/KpnIsites to generate pBAAK-H*H. The final fragment, the ORF, wasthen cloned into pBAAK-H*H at ApaI/AatII sites to generate pBAAK-H-H-H.An N-terminal p53 tag was introduced at the ApaI site usingannealed oligonucleotides p53-F and p53-R, thus generating an8-amino-acid insertion immediately downstream of the start codon(the p53 epitope contains five residues). The insertion of thisoligonucleotide duplex destroyed the first ApaI site and maintainedthe second site.

(ii) R-R-R. The construct R-R-R was designed with a strategy similar tothat for H-H-H and used a full-length 2.7-kb genomic BamHI-BamHIrpA1 fragment (gift of Marcello Jacobs-Lorena) which was subclonedinto pBluescript-SK (collapsed at SalI/XhoI sites) and subsequentlyused as a PCR template for the following fragments. The firstrpA1 fragment, R**, was generated to contain the 5' BamHI site,5' flanking genomic DNA ( $~$ 1 kb), the 5' UTR (89 nt), the startcodon, the p53 tag, and an ApaI site. This fragment was PCRgenerated by Accuprime Pfx polymerase (Invitrogen) using primersR5-Bam-5gen-F and R5-Apa-p53-R and subsequently cloned intopBAAK at BamHI/ApaI sites to generate pBAAK-R**. The secondrpA1 fragment, *R*, contained the entire ORF, minus the startcodon but including the stop codon (339 nt), and was flankedby a 5' ApaI site and a 3' AatII site. This second fragmentwas PCR generated via Elongase (Invitrogen) utilizing the primersRO-Apa-F and RO-Aat-R and was cloned into pBAAK at ApaI/AatIIsites to generate pBAAK-*R*. The third rpA1 fragment,**R, containedthe entire 3' UTR (168 nt) and 3' flanking genomic DNA ( $~$ 1 kb)flanked by 5' AatII and 3' KpnI sites and was PCR generatedusing Accuprime Pfx polymerase (Invitrogen) and primers R3-Aat-Fand R3-Bam-R. This third fragment contained a BamHI site atthe 3' end just upstream of the flanking KpnI site. The thirdfragment was cloned into pBAAK at ApaI/KpnI sites to generatepBAAK-**R. Once all three fragments were individually clonedinto pBAAK, the vector pBAAK-R-R-R was constructed via sequentialdigestion and ligation of ApaI-AatII-digested pBAAK-*R* andAatII-KpnI digested pBAAK-**R fragments into the ApaI-KpnI-digestedpBAAK-R** backbone.

(iii) H/R hybrid constructs. The following constructs were generated from the appropriatedigestions and ligations of the BamHI-ApaI 5' fragment, theBamHI-AatII 5'+ ORF fragment, the ApaI-AatII ORF fragment, theApaI-KpnI ORF +3' fragment, or the AatII-KpnI 3' fragment fromthe vectors pBAAK-H-H-H and pBAAK-R-R-R: pBAAK-H-H-R, pBAAK-H-R-R,pBAAK-H-R-H, pBAAK-R-R-H, pBAAK-R-H-R, and pBAAK-R-H-H.

(iv) H-H-H^HDE and H-H^HORF4-H^HDE. The AatII-KpnI fragment of pBAAK-H-H-H and that of pBAAK-H-H^HORF4-H(see below), respectively, each containing the full-length Hsp833' UTR, were replaced by a corresponding AatII-KpnI fragmentfrom pBluescript- ${Delta}$ HDE vector. This fragment contained the 97-ntdeletion of the HDE, and its construction has been describedpreviously (4). For R-R^lacZ-R, a 621-nt fragment of the lacZcoding sequence was PCR generated with flanking SalI sites andinserted in frame into the unique SalI site of the rpA1 ORFwithin the full-length 2.7-kb genomic BamHI-BamHI rpA1 fragmentin pBluescript-SK (collapsed at SalI/XhoI sites) as describedabove. For R-R^lacZ-R^HDE, the BamHI-BamHI fragment of R-R^lacZ-Rwas subcloned into pUC18. In this vector backbone, a polylinkerwas inserted into the rpA1 3' UTR at the NgoMI site, which introducedAvrII and BglII sites using the annealed oligonucleotides AvrII-BglII-Fand BglII-AvrII-R. The HDE was PCR generated with flanking 5'AvrII and 3' BglII sites and subcloned into the same sites inpUC18-R-R^lacZ-R to generate pUC18-rpA1-lacZ+HDE.

(v) R-R^HORF-R. Four overlapping fragments of the Hsp83 ORF (named HORF1 throughHORF4 shifting 5' to 3') were PCR generated using Elongase (Invitrogen)and were flanked with XhoI sites. The vector pCSR4-H-H-H wasused as the template (see below for construction of pCSR4 vectors).Each fragment contained 612 nt of Hsp83 ORF sequence with theexception of HORF4, which contained 615 nt of the 3'-most regionof coding sequence. The primers Xho-HORF1-F and Xho-HORF1-Rwere used for generating HORF1, the primers Xho-HORF2-F andXho-HORF2-R were used for generating HORF2, the primers Xho-HORF3-Fand Xho-HORF3-R were used for generating HORF3, and the primersXho-HORF4-F and Xho-HORF4-R were used for generating HORF4.Each XhoI-digested PCR fragment was cloned into the unique SalIsite contained within the rpA1 ORF of pBAAK-R-R-R to generatethe following constructs: pBAAK-R-R^HORF1-R, pBAAK-R-R^HORF2-R,pBAAK-R-R^HORF3-R, and pBAAK-R-R^HORF4-R. The use of flankingXhoI sites in the primer sequences introduced amino acids VEat the 5' junction between rpA1 and Hsp83 coding sequences (i.e.,at the 5' collapsed SalI site) and amino acids LD at the 3'junction between Hsp83 and rpA1 coding sequences (i.e., at thepreserved SalI site). These insertions maintained both the rpA1and Hsp83 reading frames.

(vi) R-R^HORF4-X-R. Six overlapping subfragments ( $~$ 120 nt each) of the HORF4 codingregion were PCR generated using Taq polymerase (Amersham) andflanked with XhoI sites (fragment 4-7 was synthesized usingElongase [Invitrogen]). The vector pCSR4-H-H-H was used as thetemplate (see "P-element transformation" below for constructionof pCSR4 vectors). These six fragments overlap by $~$ 20 nt withone another and were named HORF4-1 through HORF4-6 shifting5' to 3' along the HORF4 region. The primers Xho-HORF4-F andXho-HORF4-1-R were used for generating HORF4-1. The primersXho-HORF4-n-F and Xho-HORF4-n-R were used to generate HORF4-n,where 2 $≤$ n $≤$ 5. The primers Xho-HORF4-6-F and Xho-HORF4-R wereused for generating HORF4-6. The HORF4 coding region was alsosubdivided into two larger overlapping fragments that were $~$ 320nt each and contained a $~$ 20-nt overlap. These subfragments werenamed HORF4-7 and HORF4-8 (with the former representing the5'-most fragment of the HORF4 region), were also PCR generatedvia Taq polymerase (Amersham), and were flanked with XhoI sites.The primers Xho-HORF4-F and Xho-HORF4-3-R were used for generatingHORF4-7, and the primers Xho-HORF4-4-F and Xho-HORF4-R wereused for generating HORF4-8. Each XhoI-digested PCR fragmentwas cloned into the unique SalI site contained within the rpA1ORF of pBAAK-R-R-R to generate the following constructs: pBAAK-R-R^HORF4-1-R,pBAAK-R-R^HORF4-2-R, pBAAK-R-R^HORF4-3-R, pBAAK-R-R^HORF4-4-R,pBAAK-R-R^HORF4-5-R, pBAAK-R-R^HORF4-6-R, pBAAK-R-R^HORF4-7-R,and pBAAK-R-R^HORF4-8-R. The use of flanking XhoI sites in theprimer sequences introduced amino acids VE at the 5' junctionbetween rpA1 and Hsp83 coding sequences (i.e., at the 5' collapsedSalI site) and amino acids LD at the 3' junction between Hsp83and rpA1 coding sequences (i.e., at the preserved SalI site).These insertions maintained both the rpA1 and Hsp83 readingframes.

(vii) R-R-R^HORF4. The HORF4 fragment was inserted in both sense and antisenseorientations at two different unique restriction sites withinthe rpA1 3' UTR in the vector pBAAK-R-R-R. The HORF4 fragmentwas generated by Elongase PCR (Invitrogen) and was flanked eitherwith AatII sites using primers Aat-HORF4-F and Aat-HORF4-R orwith FseI sites using primers Fse-HORF4-F and Fse-HORF4-R. Thevector pCSR4-H-H-H was used as the PCR template (see below forconstruction of pCSR4 vectors). These two fragments were digestedwith their appropriate restriction enzymes, i.e., either digestedwith AatII and subsequently ligated into the AatII site in pBAAK-R-R-R(which is immediately following the stop codon) or digestedwith FseI and subsequently ligated into the FseI site just upstreamof the poly(A) signal in the rpA1 3' UTR in pBAAK-R-R-R. Thisresulted in the construction of pBAAK-R-R-R^sHORF4(Aat), pBAAK-R-R-R^asHORF4(Aat),pBAAK-R-R-R^sHORF4(Fse), and pBAAK-R-R-R^asHORF4(Fse).

(viii) H-H^HORF4-H. The construct pBAAK-H-H-H was digested at unique Bsu36I andAatII sites, which deleted a 528-nt fragment of the Hsp83 codingregion containing the majority of HORF4 (615 nt). The oligonucleotidesH4-Bsu-Aat-F and H4-Aat-Bsu-R were annealed and ligated intothe digested pBAAK-H-H-H vector to generate pBAAK-H-H^HORF4-H.A stop codon in the oligonucleotide duplex truncated the Hsp83ORF after codon 541 of the 717-amino-acid HSP83 protein. ForR-H^HORF4-R, the ApaI-AatII fragment of pBAAK-H-H^HORF4-H wasligated into ApaI/AatII-digested pBAAK-R-R-R to generate pBAAK-R-H^HORF4-R.For H-H^HORF4+lacZ-H, a 528-nt lacZ ORF fragment that containedflanking 5' Bsu36I and 3' AatII sites was PCR generated usingTaq polymerase (Amersham) and primers LacZ-Bsu-F and LacZ-Aat-R.This PCR lacZ fragment and the vector pBAAK-H-H-H were bothdigested with Bsu36I and AatII and ligated together to generatepBAAK-H-H^HORF4+lacZ-H. The lacZ PCR fragment was partially digestedwith Bsu36I, as it also contains a Bsu36I site internal to theprimer sequences, and thus, the full-length lacZ fragment wasmaintained. The construct Hsp83-lacZ (H-H^1.8kb+lacZ-H) has beenpreviously described (4, 10). Briefly, the Hsp83 5' genomicregion, 5' UTR, intron, and first 333 nt were fused to a 603-nttruncated fragment of the lacZ ORF. The 3' end of the lacZ ORFwas flanked with AatII and KpnI sites in which the same AatII-KpnIfragment described for the generation of H-H-H was used to insertthe full-length Hsp83 3' UTR and downstream genomic region.Thus, this construct created a $~$ 1.8-kb deletion of the Hsp83ORF which was replaced with a lacZ fragment. The lacZ fragmentdid not, however, contain a stop codon and thus allowed translationto proceed into the Hsp83 3' UTR.

Translation constructs. Oligonucleotide pairs were annealed and inserted at the uniqueBsiWI site within the Hsp83 5' UTR of pCSR4-H-H-H. All oligonucleotideduplexes maintained the 5' BsiWI site but eliminated the 3'BsiWI site when inserted into BsiWI-digested pCSR4-H-H-H. Forthe generation of the H^hairpin-H-H construct, the 75-nt oligonucleotidesHsp83-5'HP-F and Hsp83-5'HP-R were designed to include the stronghp7 hairpin sequence (20, 29) and annealed according to thePromega protocol for cloning a hairpin insert into pGeneClipvectors (Promega). These oligonucleotides contained NotI sitesimmediately internal to the BsiWI sites and also introduceda unique SacII site into the vector. H^random-H-H was producedby inserting the BsiWI-digested product of an Elongase PCR-amplifiedfragment of pCSR4 using the oligonucleotides Bsi-CSR-F and Bsi-CSR-Rinto the BsiWI site of pCSR-H-H-H. The 75-nt random sequencefrom the pCSR4 vector introduced an additional HindIII sitewhich aided detection of positive transformants.

pUASP-SMG rescue constructs. The generation of the SMG^RBD point mutation A642H has been previouslydescribed (2). Both wild-type and point-mutated (A642H) smgcDNA fragments containing the ORF and 3' UTR were cloned intothe pUASP vector (27).

H-H^8xSRE(-)-H. Four overlapping fragments of the Hsp83 ORF were PCR generatedusing Accuprime Pfx (Invitrogen). The vector 4xSRE^– pCSR4-H-H-H(30) was used as the template. The primers Apa-HORF1-F and H-SRE3&4-R were used to generate 1.1614, H-SRE 3&4-F andH-SRE 6-R were used for 1567.1953, H-SRE 6-F and H-SRE 8-R wereused for 1929.2100, and H-SRE 8-F and Hsp83 3U100-3H were usedfor 2095.3U-100. Accuprime Pfx, primer Apa-HORF1-F, Hsp83 3U100-3H,and 1 µl of each gel-purified fragment were used to PCRgenerate 8xSRE(-) Hsp83 ORF+3U-100. Gel-purified PCR fragmentwas cloned into the pCR21.TOPO vector. ApaI- and AatII-digested8xSRE(-) HORF fragment was subcloned into the same site in pBAAK-H-H-Hto replace the wild-type HORF and generate the 8xSRE(-) pBAAK-H-H-H,the mRNA from which is referred to in the text as H-H^8xSRE(-)-H.

P-element transformation. All NotI-KpnI inserts from the pBAAK vectors described above(i.e., containing the 5', p53 tag, ORF, and 3' fragments) werethen subcloned into pCSR4 (39) at NotI/KpnI sites. All insertswere sequenced in pBAAK and/or pCSR4 vectors (except for thefull-length p53-tagged Hsp83 construct, H-H-H, which was testedfor its ability to rescue an Hsp83 RNA null mutation and forwild-type mRNA decay kinetics [30]). The BamHI fragment fromrpA1-lacZ in pBluescript-SK was subcloned into pCSR2 (39) atthe BamHI site, while the BamHI fragment of rpA1-lacZ+HDE (R-R^lacZ-R^HDE)in pUC18 was subcloned into pCSR4 at its BamHI site. Germ linetransformants were recovered using standard methods (28).

Northern, RNA dot blot, and real-time RT-PCR analysis. Fertilized embryo and unfertilized egg collections were performedat 25°C as previously described (4). Unfertilized eggs werederived from adult virgin females mated to T(Y,2) sterile males.RNase H cleavage assays, Northern blotting, and RNA dot blottingtechniques were performed as previously described (4, 30). Briefly,total RNA was extracted from eggs/embryos collected at varioustime periods after egg lay (AEL) by homogenizing it in Trizol(Invitrogen) containing 250 µg/ml glycogen and followingstandard reagent protocols. For Northern blot analyses, samplescontaining either an equivalent number of eggs/embryos or anequivalent amount of total RNA were electrophoresed using 1%agarose-formaldehyde gels in 1x morpholinepropanesulfonic acid(MOPS) buffer and transferred overnight onto Hybond-N nylonmembranes. For RNase H cleavage assays, samples containing 10µg of total RNA were incubated with the oligonucleotideHsp83ORF.3 (for detection of H-H-H^HDE mRNA) or the oligonucleotidep53-Apa24.3 (for detection of R-R-R mRNA) in the presence ofRNase H according to standard methods (15). Cleaved RNA samplescontaining H-H-H^HDE mRNA were run on a 4% denaturing urea-polyacrylamidegel and electrotransferred overnight using the Trans-blot cell(Bio-Rad Laboratories) at 30 V while R-R-R mRNA samples wereresolved using a 1.2% agarose-formaldehyde gel and transferredas described above. For RNA dot blots, total RNA was extractedfrom single embryos and blotted directly onto Hybond-N membranein SSC (1x SSC is 0.15 M NaCl plus 0.015 M sodium citrate) bufferusing the Schleicher & Schuell Minifold-I dot blot systemaccording to the manufacturer's protocol (Schleicher & Schuell).All blots were UV cross-linked, hybridized overnight with random-primedradiolabeled probes, and exposed to a storage phosphor screen,which was then scanned using the STORM860 (Molecular Dynamics)phosphorimager. Quantification was performed using Imagequantsoftware (Molecular Dynamics) and Excel (Microsoft Office).Real-time reverse transcription-PCR (RT-PCR) was performed asdescribed previously (30).

To detect H-H^8xSRE(-)-H transcripts, a 19-base locked nucleicacid (LNA) probe specific to the sequence encoding the p53 tagwas synthesized (5'-CCA CCA CGG AGT GGC GGC C-3', where underlinesindicate locked bases; the 3' end was modified with digoxigenin).Gel running and transfer steps for RNA were performed as describedabove. Hybridization followed the Exiqon microRNA LNA probeNorthern protocol. Briefly, the membrane was prehybridized inRNA hybridization buffer (50% formamide, 0.5% sodium dodecylsulfate [SDS], 5x SSPE [1x SSPE is 0.18 M NaCl, 10 mM NaH₂PO₄,and 1 mM EDTA (pH 7.7)], 5x Denhardt's solution, and 20 µg/mlsheared, denatured, salmon sperm DNA) for 30 to 60 min. Forty-eightpicomoles of p53-LNA probe was heated for 1 minute at 95°Cbefore being added to 7 ml hybridization buffer. The membranewas hybridized overnight with the LNA probe at 45°C in thesame solution. After hybridization, membranes were washed with2x SSC-0.1% SDS at 45°C twice for 5 minutes, then with 0.1xSSC-0.1% SDS at 59°C twice for 10 minutes. The digoxigeninluminescent detection kit (Roche 1363514) was used followingRoche's protocol. Briefly, the membranes were blocked and incubatedwith antidigoxigenin-alkaline phosphatase antibody and thendeveloped with CSPD. Membranes were exposed to an imaging deviceor to X-ray film. Quantification was performed using Imagequantsoftware and Excel (Microsoft Office).

Real-time RT-PCR was performed as described previously (30).Embryos were disrupted in a minimal volume of buffer A (150mM KCl, 20 mM HEPES, pH 7.4, 1 mM MgCl₂, 1 mM dithiothreitol[DTT], 1 mM aminoethylbenzenesulfonyl fluoride, 2 µg/mlleupeptin, 2 µg/ml pepstatin, 2 mM benzamidine). Aftercentrifugation the supernatant was supplemented with glycerolto a final concentration of 10%, and 9 M urea (supplementedwith 1 mM DTT, 1 mM aminoethylbenzenesulfonyl fluoride, 2 µg/mlleupeptin, 2 µg/ml pepstatin, 2 µM benzamidine)was added to 75 µl of extract to a 2 M final concentration.The extract was recentrifuged and added to 5 µl of proteinG beads carrying either rat anti-SMG antibody or normal ratserum. Beads were incubated for 2 h at 4°C and washed severaltimes in buffer A supplemented with urea. RNA was then purifiedfrom the beads using Trizol reagent (Invitrogen) and reversetranscribed using random primers and Superscript II (Invitrogen).Samples were subjected to real-time PCR using Sybr green mastermix and the ABI Prism 7900 sequence detection system (AppliedBiosystems).

Western blot analysis. Western blot analyses were carried out as previously described(30). Briefly, eggs/embryos were dechorionated in 50% bleach,rinsed and homogenized in lysis buffer (150 mM NaCl, 50 mM Tris,pH 7.5, 1% NP-40, 1 mM DTT, 1x EDTA-free protease inhibitorcocktail [Roche]), incubated on ice for 5 min, and then centrifugedfor 5 min at 12,000 x g at 4°C. The supernatant was combinedwith 2x SDS loading dye, loaded, and subjected to SDS-polyacrylamidegel electrophoresis (7.5% acrylamide). The Bio-Rad Trans-blotSD semidry transfer cell was used to transfer proteins to apolyvinylidene difluoride membrane (Invitrogen). Blots wereblocked in 1% skim milk powder before incubations with primaryand secondary antibodies. Primary antibodies used were mousemonoclonal anti-p53 at 1:1,000 (Santa Cruz Biotechnology; SC-99),guinea pig polyclonal anti-SMG at 1:10,000 (35), and guineapig polyclonal anti-DDP1 at 1:10,000 (24, 35). Secondary horseradishperoxidase-conjugated antibodies were used at 1:5,000 (JacksonImmunoResearch Laboratories, Inc.). Chemiluminescence was detectedusing Pierce enhanced chemiluminescence Western blotting reagentand standard X-ray film.

RESULTS

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RESULTS

The Hsp83 ORF functions as a transcript instability element. To map cis-acting instability elements in the Hsp83 mRNA, chimerictransgenes were constructed, each containing combinations ofthe 5' UTR, ORF, and 3' UTR of Hsp83 and rpA1, a highly stablemRNA. The constructs are listed in Table 1; these, and additionalones used in subsequent experiments, encoded a five-residuep53 epitope tag immediately after the amino-terminal methionineunless otherwise noted. The stability profiles of the hybridmRNAs were examined using Northern blot assays of total RNAextracted from staged unfertilized eggs laid by transgenic femalesat 0 to 2, 2 to 4, and 4 to 6 h AEL, thus enabling us to assessthe role of the cis elements in the maternally encoded transcriptdegradation pathway.

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TABLE 1. The Hsp83 ORF acts as a strong instability element

The control rpA1 transgenic transcript, R-R-R (where the firstletter denotes the source of the 5' UTR, the second the sourceof the ORF, and the third the source of the 3' UTR), was highlystable, although less so than endogenous rpA1 mRNA (Table 1)(for endogenous rpA1, 95% ± 21% of the transcripts remainedat 4 to 6 h AEL, while for R-R-R 74% ± 5% remained).The R-H-R and R-R-H constructs were used to assess whether theHsp83 ORF or Hsp83 3' UTR, respectively, was sufficient to destabilizerpA1 mRNA while R-H-H and H-H-R were used to ask whether thecorresponding regions were necessary for Hsp83 mRNA decay. Fortechnical reasons, the sufficiency of the Hsp83 5' UTR couldnot be assayed in these experiments (see footnotes to Table1); however, our subsequent experiments showed definitivelythat the 5' UTR is not required for destabilization. Since 26%± 5% of R-R-R mRNA was degraded by 4 to 6 h AEL, throughoutthis study we have used the following terminology to describethe results: instability was defined as "strong" if >50%of the mRNA was eliminated by 4 to 6 h AEL, "weak" if 30 to50% was eliminated, and "none" if <30% was eliminated.

The extent of mRNA destabilization produced by the necessityconstructs, R-H-H (78% ± 7% degraded by 4 to 6 h AEL)and H-H-R (88% ± 4% degraded), was strong and comparableto that observed for endogenous Hsp83 mRNA (92% ± 6%)(Table 1). With respect to sufficiency, the Hsp83 ORF insertedinto R-H-R was sufficient to strongly destabilize the hybridtranscripts, eliminating 72% ± 7% of the transcriptsby 4 to 6 h AEL. In contrast, the effects of the Hsp83 3' UTRon R-R-H were weak, eliminating 36% ± 15% of transcriptsby the same stage. The region common to all of the hybrid transcriptsthat exhibited strong destabilization is the Hsp83 ORF, consistentwith the hypothesis that the ORF contains one or more transcriptinstability elements. The data are also consistent with thepossibility that the 3' UTR contains a weak instability element.

We note that an alternative to the "instability element" interpretationpresented here is that the rpA1 mRNA houses stabilization elements.For example, the R-H-R transcript could be unstable due to lossof such elements. rpA1 has been used previously as a backbonewith which to map instability elements within the bicoid andfushi tarazu mRNAs (17, 19, 26, 34). Since the bicoid and fushitarazu instability elements function in the presence of therpA1 5' UTR and/or ORF, we favor—and subsequent experimentspresented below support—the interpretation that the Hsp83mRNA contains instability elements.

A 615-nt HIE resides within the ORF. To refine the mapping of the strong instability element(s) withinthe Hsp83 ORF, four overlapping fragments that together spannedthe entire 2,154 nt were inserted in frame into the ORF of R-R-R(Fig. 1A). These fragments were each $~$ 615 nt long and overlappedby $~$ 100 nt. The stability of the resulting hybrid mRNAs was assayedin unfertilized eggs as described above. The fourth fragment,HORF4, was sufficient to strongly destabilize R-R-R mRNA, eliminating68% ± 1% of transcripts by 4 to 6 h AEL, while the otherfragments—HORF1 (12% ± 14%), HORF2 (25% ±6%), and HORF3 (15% ± 9%)—had no significant destabilizingactivity (Fig. 1B and C). That all four fragments of the Hsp83ORF were inserted at the same site within the R-R-R ORF andyet only HORF4 destabilized the hybrid mRNA supports the hypothesisthat the instability of R-R^HORF4-R transgenic mRNA is due tothe presence of the HORF4 sequence and not to an effect of theinsertion site. Consistent with this conclusion, insertion ofa piece of the lacZ ORF into this same site did not significantlydestabilize the mRNA (see R-R^lacZ-R below and Fig. 4I and J).

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FIG. 1. A strong instability element—the HIE—maps within the Hsp83 ORF. (A) Schematic representation of the Hsp83 ORF sufficiency constructs. Four overlapping fragments ( $~$ 615 nt each with 100-nt overlap) of the Hsp83 coding sequence (HORF1 to HORF4) were independently inserted in frame into the transgenic R-R-R construct at a unique SalI restriction site within the rpA1 coding sequence. Constructs are drawn to scale. (B) Northern blot analysis of the Hsp83 ORF sufficiency constructs in unfertilized eggs. Blots were probed with the rpA1 3' UTR to detect mRNA from both the transgene and the loading control, rpA1. (C) Quantification of Northern blot data in panel B. Average normalized transgenic mRNA levels between two or more independently derived transgenic fly lines are shown. Transgenic mRNA levels were normalized to loading controls. Error bars represent standard deviations calculated from at least two independent experiments. All experiments were performed using unfertilized eggs from transgenic mothers, collected at 0 to 2 h, 2 to 4 h, and 4 to 6 h AEL. Transcript levels at 2 to 4 h and 4 to 6 h AEL are represented as a percentage of the initial amount detected at 0 to 2 h (i.e., % mRNA remaining).

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FIG. 4. Mapping of auxiliary ORF elements and the role of the HDE. (A and B) Test of the necessity of the HDE to mediate Hsp83 mRNA decay via the maternal degradation pathway. (A) RNase H cleavage and Northern blot analysis of H-H-H^HDE transgenic mRNA. Hsp83 mRNA and H-H-H^HDE mRNA were cleaved with RNase H in the presence of an oligonucleotide that anneals to the 3' end of the ORF and oligo(dT), thus generating 407-nt and 307-nt 3' UTR fragments without their poly(A) tails, respectively. The blot was probed with full-length Hsp83 3' UTR. (B) Quantification of Northern blot data in panel B revealed similar degradation rates for Hsp83 and H-H-H^HDE transcripts. H-H-H^HDE females were heterozygous for the H-H-H transgene, thus accounting for the differences in initial levels relative to Hsp83 mRNA. Raw mRNA levels are shown. Experiments were performed in duplicate. (C and D) Deletion of the both the HIE and HDE does not stabilize Hsp83 transcripts. Northern blots were probed with Hsp83 probe, thus detecting both endogenous Hsp83 transcripts and the transgenic RNA (C). Quantification (D) included normalization relative to rpA1 transcripts. Experiments were performed in duplicate, and the averages ± standard deviations are shown. For H-H^HORF4-H, 22% ± 13% of transcripts remained at 4 to 6 h AEL while, for H-H^HORF4-H^HDE, 21% ± 0% remained at 4 to 6 h AEL compared with <10% of endogenous mRNA. (E and F) Deletion of a $~$ 1.8-kb 3' region of the Hsp83 ORF weakly stabilizes the transcript. The H-H^1.8kb+lacZ-H transgene contains a $~$ 1.8-kb 3' deletion of the Hsp83 coding sequence (including deletion of the entire HIE) along with a 603-nt lacZ ORF substitution. No p53 tag was present. For the Northern blot analysis of H-H^1.8kb+lacZ-H mRNA in unfertilized eggs, both endogenous Hsp83 and H-H^1.8kb+lacZ-H mRNAs were detected by probing for Hsp83. rpA1 mRNA was used as a loading control. Quantification values are the averages of three independent replicates for H-H^1.8kb+lacZ-H. (G and H) Role of the HDE is revealed in a sensitized background. Northern blots were probed with Hsp83 probe, thus detecting both endogenous Hsp83 transcripts and the transgenic RNA. Quantification (H) included normalization relative to rpA1 transcripts. Experiments were performed in duplicate, and the averages ± standard deviations are shown. For H-H^1.8kb+lacZ-H, 31% ± 3% of transcripts remained at 4 to 6 h AEL (F) while, for H-H^1.8kb+lacZ-H^HDE, 66% ± 3.7% remained at 4 to 6 h AEL (H). (I and J) Sufficiency of the HDE. R-R^lacZ-R and R-R^lacZ-R^HDE were derived from the same genomic rpA1 DNA as R-R-R but lacked the p53 epitope tag and restriction sites at the 5'-UTR/ORF and ORF/3'-UTR junctions. Instead, these constructs contained a lacZ tag within their coding sequence. For Northern blot analysis of transgenic R-R^lacZ-R and R-R^lacZ-R^HDE mRNA, blots were probed with full-length rpA1 to detect both endogenous and transgenic mRNAs. For quantification of Northern blot data of R-R^lacZ-R and R-R^lacZ-R^HDE, experiments were replicated two and five times, respectively, and the averages of those experiments ± standard deviations are shown. Constructs are drawn to scale.

These results demonstrate that the Hsp83 ORF houses a stronginstability element within its 3'-most region (viz., nucleotidepositions 1537 to 2154 in reference to the published DrosophilaHsp83 cDNA sequence [6]). Since there was a $~$ 100-nt overlap betweenHORF3 and HORF4, and HORF4 but not HORF3 could trigger strongdestabilization, the major instability element is likely toreside within the last 516 nt of the Hsp83 ORF. However, sincewe cannot rule out the possibility that the 3' limit of HORF3fragment disrupts an instability element that spans this boundary,we have called the entire 615-nt HORF4 fragment the HIE. Theidentification of the HIE is consistent with a conclusion reachedabove: that a major instability element resides within the Hsp83mRNA coding region. Furthermore, if there are stabilizationelements present within the rpA1 transcript, the HIE is ableto override their stabilizing functions.

To dissect the HIE further, six subfragments spanning the entireHIE were generated and named HORF4-1 through HORF4-6 (Fig. 2A).These subfragments were each $~$ 120 nt long with an $~$ 20-nt overlapand were inserted into R-R-R as described above. In addition,two larger subfragments of the HIE, which were each $~$ 320 nt longwith $~$ 20 nt of overlap, were inserted in frame into the R-R-RORF (HORF4-7 and HORF4-8) (Fig. 2A). None of the subfragmentsof the HIE was capable of recapitulating the strong destabilizationaccomplished by insertion of the entire HIE (Fig. 2B and C).A weak destabilizing effect was observed by 4 to 6 h upon insertionof HORF4-1 (50% ± 5% mRNA eliminated), HORF4-6 (39% ±20% eliminated), HORF4-7 (34% ± 5% eliminated), and HORF4-8(33% ± 9% eliminated). Transcripts carrying HORF4-2,HORF4-3, HORF4-4, and HORF4-5 were stable since only 16% ±7%, 13% ± 5%, 10% ± 4%, and 21% ± 11% ofthe respective transcripts were eliminated by 4 to 6 h AEL.

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FIG. 2. Several subfragments of the HIE confer moderate instability. (A) Schematic representation of the HORF4 subfragments utilized to study the HIE. Six overlapping fragments ( $~$ 100 nt each with 20-nt overlap) as well as two larger overlapping fragments ( $~$ 320 nt each with 20-nt overlap) of the HORF4 region (HORF4-1 to HORF4-8) were independently inserted into the transgenic R-R-R construct at a unique SalI restriction site within the rpA1 coding sequence. All HORF fragments were inserted in frame into R-R-R. Constructs are drawn to scale. (B) Northern blot analysis of the HORF4 subfragment sufficiency constructs in unfertilized eggs. Blots were probed with the HORF4 fragment of the Hsp83 ORF to detect transgenic mRNAs and with the loading control, rp49. (C) Quantification of Northern blot data in panel B. Average normalized transgenic mRNA levels between two independently derived transgenic fly lines are shown. Egg collection time points were the same as those for Fig. 1, and normalization was performed as described for Fig. 1. Light grey, 0 to 2 h AEL; dark grey, 2 to 4 h AEL; black, 4 to 6 h AEL. The red lines indicate the cutoffs defined in the text for lack of destabilizing ability (above the upper red line), weak destabilizing ability (between the red lines), and strong destabilizing ability (below the lower red line) at the 4- to 6-h time point.

The inability to uncover a single subfragment of the HIE thatproduced a strong decay profile resembling that of the entireHIE, along with the weak destabilizing effect of several subfragments,suggests that the HIE contains two or more subelements thatfunction in combination, possibly additively, to mediate strongtranscript degradation. The weak destabilizing activity of HORF4-1and HORF4-6 supports the notion that most of these subelementsreside toward the ends, rather than the central region, of theHIE. Consistent with this hypothesis, weak degradation was alsoinduced by each of the larger subfragments, HORF4-7 and HORF4-8,which include HORF4-1 and HORF4-6, respectively.

The HIE is not necessary for the destabilization of full-length Hsp83 mRNA. To assess the role of the HIE in the context of the Hsp83 mRNA,we constructed a transgene, H-H^HORF4-H, in which the majorityof the HIE was removed (i.e., the 3'-most 528 nt of the 615-ntHIE) (Fig. 3A). To ensure that any observed instability wasnot a consequence of shortening the length of the ORF, a "substitution"construct was also made, in which the deleted 528 nt were replacedwith 528 nt of the lacZ coding sequence fused in frame to theHsp83 ORF (H-H^HORF4+lacZ-H) (Fig. 3A). Both the H-H^HORF4-H andH-H^HORF4+lacZ-H transgenic mRNAs were strongly unstable: 78%± 13% of the H-H^HORF4-H transcripts were eliminated by4 to 6 h AEL while 78% ± 0% of H-H^HORF4+lacZ-H transcriptswere eliminated (Fig. 3B and C). Thus, the 528-nt fragment ofthe HIE is not necessary for H-H-H mRNA degradation, likelybecause of additional instability elements elsewhere in theHsp83 mRNA.

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FIG. 3. The HIE is not necessary for destabilization of full-length Hsp83 transgenic mRNA but is required for the destabilization of R-H-R transgenic mRNA. (A) Schematic representation of necessity constructs. These constructs all contained a deletion within the Hsp83 coding sequence that removes the majority of the HIE (the 5'-most 87 nt of HIE are still present). This 3'-most 528-nt region of the Hsp83 coding sequence was deleted within full-length H-H-H (top), was replaced with 528-nt lacZ coding sequence within full-length H-H-H (middle), and was deleted within the transgenic construct R-H-R (bottom). (B) Northern blot analysis of H-H^HORF4-H, H-H^HORF4+lacZ-H, and R-H^HORF4-R mRNAs in unfertilized eggs. H-H^HORF4-H and H-H^HORF4+lacZ-H mRNAs were detected by probing for the p53 sequence, and rpA1 mRNA was used as a loading control. For R-H^HORF4-R, probing was with the rpA1 3' UTR, which detected both the transgenic mRNA and the loading control, rpA1. (C) Quantification of Northern blot data in panel B. Average normalized transgenic mRNA levels between two independently derived transgenic fly lines are shown.

To assess the necessity of the HIE in the absence of additionalHsp83 mRNA instability elements, we next examined the 528-ntdeletion of the HIE within the context of the R-H-R transgene,which lacks the Hsp83 5' UTR and 3' UTR (Fig. 3A). TransgenicR-H^HORF4-R transcripts were substantially stabilized relativeto R-H-R but did remain weakly unstable (39% ± 3% eliminatedversus 72% ± 7%, respectively) (Fig. 3B and C).

Together, our results support the hypothesis that the HIE isa major instability element that can function to strongly destabilizean otherwise stable mRNA (R-R-R). The weak instability of R-H^HORF4-RmRNA is consistent with additional, minor instability elementsresiding in the undeleted part of the Hsp83 ORF. Furthermore,the fact that the HIE is necessary to mediate strong degradationin the R-H-R context but not in the full-length H-H-H contextis consistent with additional instability elements mapping outsidethe ORF, possibly in the 3' UTR, which exerts weak destabilizingactivity (Table 1).

A large deletion in the Hsp83 ORF substantially stabilizes the mRNA. Given the inference that weak instability elements might residein the Hsp83 ORF upstream of the HIE, we next assessed whethera large deletion within the ORF would stabilize the mRNA toa greater extent than deletion of the HIE alone. We previouslyreported that an Hsp83-lacZ hybrid mRNA containing the Hsp835' UTR, the first 333 nt of the ORF (fused in frame to a fragmentof the lacZ ORF), and the full-length Hsp83 3' UTR is unstablein early embryos (4). To assess whether this 1,821-nt deletion,which removes more than 80% of the ORF, affects transcript stabilityvia the maternal decay pathway, we examined the Hsp83-lacZ reportermRNA—here renamed H-H^1.8kb+lacZ-H to be consistent withthe nomenclature used in the present study—in unfertilizedeggs and found that it was partially stabilized (Fig. 4 E and F):at 2 to 4 h AEL, 79% ± 10% of H-H^1.8kb+lacZ-H mRNA remainedcompared to 14% ± 3% of endogenous Hsp83 transcriptswhile, by 4 to 6 h, 31% ± 3% of H-H^1.8kb+lacZ-H transcriptsremained compared with only 2% ± 1% of endogenous transcripts.Thus, deletion of most of the Hsp83 ORF, including the HIE,substantially (but incompletely) abrogates mRNA degradationvia the maternal decay pathway.

The fact that H-H^1.8kb+lacZ-H transcripts were partially stabilizedrelative to H-H^HORF4-H and H-H^HORF4+lacZ-H transcripts is consistentwith the hypothesis that instability elements additional tothe HIE reside in the more-5' region of the Hsp83 ORF. The factthat the H-H^1.8kb+lacZ-H transcript was only weakly stabilizedis consistent with additional instability elements mapping inthe 3' UTR.

An auxiliary instability element—the previously identified HDE—resides in the Hsp83 3' UTR. We previously reported that deletion of a 97-nt region withinthe 407-nt 3' UTR of Hsp83—the HDE—within the contextof the H-H^1.8kb+lacZ-H reporter mRNA (i.e., H-H^1.8kb+lacZ-H^HDE)resulted in strong stabilization of this mRNA in unfertilizedeggs (4). The HDE is, however, not necessary for degradationof Hsp83 transcripts: deletion of the HDE in the context ofa full-length Hsp83 transgene (H-H-H^HDE) had no effect on transcriptdestabilization (Fig. 4A and B). That the HDE is not requiredfor the decay of the Hsp83 transcripts is consistent with ourfinding that H-H-R transcripts, in which the entire Hsp83 3'UTR was replaced, remained highly unstable (Table 1).

We next assayed whether simultaneous deletion of the HIE andHDE (H-H^HORF4-H^HDE) had an effect on stability. Our resultsclearly indicated that there is no difference between the decaykinetics of H-H^HORF4-H and those of H-H^HORF4-H^HDE transcripts:in the case of H-H^HORF4-H, 22% ± 13% of transcripts remainedwhile, for H-H^HORF4-H^HDE, 21% ± 0% remained at 4 to 6h AEL compared with <10% of endogenous mRNA (Fig. 4C and D).

As described in the previous section, transcripts carrying thelarge, 1.8-kb ORF deletion, H-H^1.8kb+lacZ-H, are weakly stabilized,with 31% ± 3% remaining 4 to 6 h AEL (Fig. 4E and F).However, together with the HDE deletion (H-H^1.8kb+lacZ-H^HDE),these were strongly stabilized with 66% ± 4% remainingat 4 to 6 h AEL (Fig. 4G and H).

Together, these data support the hypothesis that several instabilityelements for Hsp83 mRNA—including a major element, theHIE—reside in its ORF and that the 3'-UTR-located HDEfunctions as an auxiliary instability element whose role isrevealed only in the context of a sensitized transcript in whichmost, but not all, of the ORF-located elements are deleted.

The sufficiency experiments documented above are consistentwith the hypothesis that the HDE is an auxiliary instabilityelement, since weak destabilization was observed for R-R-H transgenicmRNA (Table 1). To specifically address the role of the HDEin mediating this destabilization, we inserted the HDE intothe 3' UTR of a transgene, R-R^lacZ-R, which comprises full-lengthgenomic rpA1 with a portion of the lacZ ORF inserted in frameinto the rpA1 coding sequence (to distinguish the transgenictranscripts from endogenous ones). R-R^lacZ-R was stable, withonly 14% ± 20% eliminated by 4 to 6 h AEL (Fig. 4I and J).Insertion of the HDE (R-R^lacZ-R^HDE) had a weak destabilizingeffect: 37% ± 14% of transgenic mRNA was eliminated by4 to 6 h AEL (Fig. 4I and J), essentially identical to thatseen for R-R-H (36% ± 15% eliminated) (Table 1).

We conclude that the HDE is an auxiliary instability elementthat functions together with the major instability elements,which are located in the Hsp83 ORF.

Translation of the Hsp83 mRNA and/or of the HIE is not required for transcript destabilization. We showed previously that Hsp83 mRNA is actively translatedin early embryos (30). To investigate whether translation ofan Hsp83 transcript is required to trigger its degradation,we inserted a strong, stable hairpin within the 5' UTR of thefull-length H-H-H transgene (position 18 of the 149-nt-long5' UTR) (Fig. 5 A). The identical hairpin inserted anywherebetween a 5' cap and an initiation codon has been shown previouslyto block translation by preventing 40S ribosome subunit scanningin vitro and, thus, to efficiently block translation of c-fosmRNA in mouse NIH 3T3 cells (20, 29). To control for any potentialstabilizing effect of disruption of the Hsp83 5' UTR per se,an additional construct was made in which a random sequenceof identical length was inserted at the same position (Fig.5A). Both of these transgenic transcripts, H^hairpin-H-H andH^random-H-H, were examined for translational status and stability.Western blot analysis showed that, as expected, H^random-H-HmRNA was translated while H^hairpin-H-H was not (Fig. 5B). Thus,the insertion of the hairpin efficiently and specifically blockedtranslation. We next assessed the decay kinetics of H^random-H-Hand H^hairpin-H-H mRNA (Fig. 5C and D). Both mRNAs were rapidlydegraded over a 6-hour time course and exhibited decay kineticssimilar to those of endogenous Hsp83 mRNA. These results demonstratethat Hsp83 mRNA translation in cis is not required for transcriptdegradation.

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FIG. 5. Hsp83 mRNA destabilization does not require translation in cis. (A to D) Insertion of a strong stable hairpin into full-length Hsp83 transgenic mRNA blocks translation in cis but does not prevent mRNA degradation. (A) Schematic representation of the insertion of either a strong stable hairpin or random nonhairpin sequence (inverted triangle) into the 5' UTR of H-H-H. Constructs are drawn to scale. (B) Western blot analysis using anti-p53 antibody demonstrates that protein was not detectable from 0- to 2-h unfertilized egg collections from H^hairpin-H-H transgenic mothers in contrast to H^random-H-H transgenic mothers. Specificity of the anti-p53 antibody and the proper sizes of the p53-tagged transgenic protein were demonstrated by looking at additional p53-tagged constructs such as H-H^HORF4-H and H-H^HORF4+lacZ-H. (C) Northern blot analysis of H^hairpin-H-H and H^random-H-H mRNA. Transgenic mRNAs were detected using a p53-specific probe, and rpA1 mRNA was used as a loading control. Lanes marked "–" denote unfertilized eggs lacking any transgene. (D) Quantification of Northern blot data in panel C. Average normalized transgenic mRNA levels from two independently derived transgenic fly lines are shown. The endogenous Hsp83 mRNA decay profile from Fig. 1 is included as a reference. Egg collection time points and normalization were as described for Fig. 1. (E and F) The HIE mediates the decay of stable rpA1 transgenic mRNA in a position-independent but orientation-dependent manner. (E) The HIE was inserted in sense and antisense orientations at two different locations within the rpA1 3' UTR (and thus downstream of the stop codon). Northern blot analysis of transgenic mRNAs in unfertilized eggs is shown below the schematic representations (drawn to scale). Blots were probed with the full-length rpA1 3' UTR, which detected both transgenic (experimental) and rpA1 (loading control) transcripts. (F) Quantification of Northern blot data in panel E. Average normalized transgenic mRNA levels from two independently derived transgenic fly lines are shown. Egg collection time points were the same, and normalizations were performed, as described in Materials and Methods. The decay profile of R-R^HORF4-R from Fig. 1C is included as a reference.

Our results using H^hairpin-H-H mRNA suggested that the HIE mightnot need to reside within the ORF for it to function as an instabilityelement. Constructs were therefore made to assess the positiondependence of the HIE by inserting it in both the sense andantisense orientations at two different sites within the 3'UTR of R-R-R (Fig. 5E). In each of these, since the HIE wasdownstream of the translation stop codon, it was "protected"from ribosome transit. Insertion of the HIE at either site inits sense orientation conferred strong transcript instability:77% ± 5% of R-R-R^sHORF4(Aat) and 77% ± 9% of R-R-R^sHORF4(Fse)transcripts were degraded by 4 to 6 h AEL (Fig. 5E and F). Incontrast, control antisense HIE insertions caused only 2% ±30% and 19% ± 27% of the mRNA to be eliminated, respectively,for R-R-R^asHORF4(Aat) and R-R-R^asHORF4(Fse) mRNAs. Thus, theHIE can mediate transcript degradation even when located inthe 3' UTR, and ribosome transit through the HIE is not necessaryfor its function.

We conclude that translation in cis of the Hsp83 mRNA and, specifically,of the HIE is not necessary for transcript degradation and thatthe HIE mediates transcript decay in a position-independentmanner.

The HIE mediates SMG-dependent mRNA degradation. We have shown previously that SMG function is required for destabilizationof endogenous Hsp83 mRNA (30). We therefore next assessed whetherHIE-dependent destabilization depends on SMG function. To doso, we determined the degradation profiles of R-R^HORF4-R, R-R-R^sHORF4(Fse),and R-R-R^asHORF4(Fse) transgenic mRNA in unfertilized eggs producedby smg mutant females.

The degradation of R-R^HORF4-R and R-R-R^sHORF4(Fse) mRNA wasseverely compromised—in a dose-dependent manner—byloss of SMG (Fig. 6 shows R-R^HORF4-R). In an smg¹ heterozygousbackground (i.e., in the presence of one dose of the smg⁺ gene),R-R^HORF4-R mRNA was partially stabilized relative to the wildtype (55% ± 13% versus 32% ± 1%, respectively,remaining by 4 to 6 h AEL in unfertilized eggs). In an smg¹homozygous mutant background (i.e., zero doses of the smg⁺ gene),transgenic R-R^HORF4-R mRNA was almost completely stabilizedwith 89% ± 2% of the mRNA remaining by 4 to 6 h AEL.This is almost identical to the stabilization of endogenousHsp83 mRNA in 2- to 3-h embryos from smg mutant females, inwhich 92% ± 4% of endogenous Hsp83 transcripts remain(30). Likewise, R-R-R^sHORF4(Fse) transcripts were stabilizedin smg¹ homozygotes (data not shown). We conclude that the HIEfunctions in an SMG-dependent manner, thus reflecting a trueendogenous major instability element.

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FIG. 6. SMG is required for the destabilization of R-R^HORF4-R transgenic mRNA. (A) Northern blot analysis of R-R^HORF4-R mRNA as assayed in smg¹ heterozygous and smg mutant backgrounds. smg¹ heterozygous and smg¹ mutant eggs were both derived from mothers containing a single copy of the R-R^HORF4-R transgene. smg mutant eggs were derived from females containing the smg¹ allele and the deficiency Df(3L)Scf^R6, which uncovers the smg region. Blots were probed as previously described for Fig. 3. (B) Quantification of Northern blot data in panel A. Average normalized transgenic mRNA levels between two independently derived transgenic fly lines are shown. The decay profile of R-R^HORF4-R in a +/+ background was taken from Fig. 1C and is included as a reference. Egg collection time points were the same, and normalizations were performed, as described for Fig. 1 and in Materials and Methods.

The HIE directs association with SMG protein. We previously used real-time RT-PCR to show that endogenousHsp83 transcripts are present in an SMG-containing messengerribonucleoprotein complex (mRNP): after immunoprecipitationwith anti-SMG antibody, Hsp83 transcripts were fivefold enrichedrelative to normal rat serum; a positive control, nanos, wasalso fivefold enriched; and a negative control, rp49, was only1.7-fold enriched (30). To assess whether the HIE is sufficientto target a hybrid mRNA to the SMG-containing mRNP, here weagain used real-time RT-PCR to study the R-R^HORF4-R and R-R-R^sHORF4(Fse)mRNAs. We found that the R-R^HORF4-R and R-R-R^sHORF4(Fse) transcriptswere enriched 3.3- ± 0.5-fold and 5.6- ± 1.2-fold,respectively, while endogenous Hsp83 transcripts were enriched5.6- ± 0.5-fold and 4.5- ± 0.3-fold and rp49 transcriptswere enriched 1.3- ± 0.0-fold and 1.6- ± 0.4-foldin their respective experiments.

We conclude that the HIE can direct transcripts into an SMG-containingmRNP.

SMG's RNA-binding ability is necessary for Hsp83 mRNA destabilization. Alanine₄₉₈ of the budding yeast homolog of SMG, VTS1, is foundin its RNA-binding domain (RBD) and makes direct contact withthe third base in the loop of the SRE (1). A single amino acidmutation (to histidine) of either alanine₄₉₈ within the VTS1SAM domain or the analogous residue within the SMG SAM domain,alanine₆₄₂, completely abolishes the ability of these SAM domainsto bind consensus SREs in vitro but does not disrupt proteinfolding (2).

To assess whether direct binding of SMG to Hsp83 mRNA is requiredfor transcript destabilization, we therefore made full-lengthSMG "rescue" constructs expressing either wild-type protein(SMG^WT) or an A642H mutant protein (SMG^RBD, for RBD mutant).Using the modified GAL4/upstream activation sequence (UAS) systemto drive expression of the transgenic mRNAs during oogenesis(27, 41), we assessed the ability of SMG^RBD and SMG^WT to rescuethe severe Hsp83 mRNA degradation defects observed in smg mutants.In these experiments, because we had shown that Hsp83 mRNA degradationis SMG dependent in both unfertilized and fertilized eggs (30)and the amount of material was limiting, embryos rather thanunfertilized eggs were used.

Expression of SMG^WT in embryos from smg mutant females fullyrescued endogenous Hsp83 mRNA destabilization (Fig. 7A to C,genotype 8). In sibling controls, Hsp83 mRNA decay was observedin smg¹ heterozygous backgrounds (Fig. 7A to C, genotypes 5and 6), while Hsp83 mRNA was completely stabilized in embryosfrom smg¹ mutant mothers lacking the SMG^WT transgene (Fig. 7A to C,genotype 7). In striking contrast, embryos expressing SMG^RBDfailed to degrade endogenous Hsp83 mRNA (Fig. 7A to C, genotype2); this decay profile was indistinguishable from that observedin the smg¹ mutant background alone (Fig. 7A to C, genotype1). Embryos from their smg¹ heterozygous siblings, in contrast,displayed normal Hsp83 mRNA decay (Fig. 7A to C, genotypes 3and 4).

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FIG. 7. RNA-binding ability of SMG is necessary for degradation of endogenous Hsp83 mRNA. Full-length SMG transgenes driven by the GAL4/UAS system were tested for their ability to rescue the Hsp83 mRNA degradation phenotype in smg¹ mutant embryos. The function of the wild-type rescue construct (SMG^WT) was compared to that of a mutated SMG construct (SMG^RBD) which contains a single point mutation within the sequence encoding the SMG RBD, which is predicted to abolish SMG's ability to bind its cognate RNA sequence, the SRE. Rescue constructs were expressed using pUASP vectors and were driven via the maternal driver, nosGAL4^VP16. (A) Genetic background of transgenic mothers with sibling control lines included. (B) Northern blot analysis of total RNA extracted from fertilized embryos over a 4-hour time course. Embryos were examined at 0 to 1, 1 to 2, 2 to 3, and 3 to 4 h AEL. Blots were probed for Hsp83 (experimental) and rpA1 (loading control) mRNAs. Genotypes are described in the legend to panel A. (C) Quantification of Northern blot data in panel B. Only a single experiment was performed. Normalization was as described for Fig. 1. (D) Western blot analysis of 0- to 3-h embryos demonstrating the production of SMG protein from the rescue constructs SMG^WT and SMG^RBD. The anti-SMG antibody recognizes both the endogenous and the transgenic SMG proteins, as well as the truncated form of the protein derived from the smg¹ allele. Anti-DDP1 antibody was used as a loading control. The gray arrow represents a cross-reacting band that migrates just above the SMG protein.

Western blot analysis confirmed that pUASP-SMG^WT and pUASP-SMG^RBDproduced equivalent levels of SMG protein (Fig. 7D); therefore,the lack of rescue by SMG^RBD was not attributable to lower proteinlevels. The results shown in Fig. 7 derive from single transgeniclines for SMG^WT and SMG^RBD; almost-identical results were obtainedfor two additional transgenic lines for each construct (datanot shown). Thus, a point mutation that abrogates the SRE bindingability of SMG also blocks the ability of SMG to mediate Hsp83mRNA destabilization, consistent with direct binding of SMGto the Hsp83 mRNA being a prerequisite for transcript destabilization.

Simultaneous mutation of all eight computationally predicted SREs in the Hsp83 ORF stabilizes the transcript. SMG recognizes its target mRNAs via stem-loop structures calledSREs (12, 32, 33). Initially, the consensus SRE sequence wasdefined as either a 4- or a 5-nt loop with the sequence CNGGor CNGGN, respectively, on a nonspecific stem (2, 11). Fourcopies of this consensus SRE, present within the ORF of endogenousHsp83 mRNA, were shown by us to be dispensable since simultaneousmutation of all four elements did not affect transcript instability(30). Subsequent to those analyses, it was shown that the lengthof an SRE loop can be increased to 7 nt (CNGGN_0-3) and the SREcan remain fully functional (1). In addition, structural analysesrevealed that the VTS1 RBD makes contact with the phosphategroups between the third and fourth bases of the stem, suggestingthat the length of the stem may also be important for RNA recognition(1). A computational search of the entire Hsp83 transcript forthe revised SRE consensus (CNGGN_0-3 on a stem of at least 4bp) revealed an additional four predicted SREs within the Hsp83mRNA. Thus, there are a total of eight predicted SREs in theHsp83 mRNA: all map within the ORF, six of the eight residewithin the HIE, and seven of the eight are removed by the 1.8-kbdeletion used in our analyses reported above (in Fig. 9 thefour potential SREs that were mutated in our 2005 study areindicated with asterisks; see also Fig. S1 in the supplementalmaterial for the complete sequence of the ORF and location ofthe SREs).

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FIG. 9. Potential SREs in the Hsp83 mRNA and their relationships to fragments of the ORF that are sufficient to destabilize the rpA1 transcript. The diagrams and color coding are as in Fig. 1 to 4. Predicted SREs (defined as in the text) are shown at their approximate locations in the Hsp83 mRNA but are drawn larger than scale. Asterisks indicate the predicted SREs that were mutated in our previous study (30). The braces indicate the 1,821-nt deletion that incompletely abrogates instability of the Hsp83 transcript. The ability of the full-length ORF and its subfragments to confer instability as defined in Table 1 is indicated to the right: ++, strong instability element; +, moderate instability element; –, no destabilizing activity.

To assess whether destabilization of Hsp83 mRNA requires bindingto these predicted SREs, we constructed a transgene encodingan mRNA—H-H^8xSRE(-)-H—in which all eight sites weremutated simultaneously (Fig. 8; see also Fig. S1 in the supplementalmaterial). In seven out of eight cases, third-base mutationsensured that the transgene retained identical amino acid codingcapacity; in one case it was necessary to introduce a conservativesubstitution (see Materials and Methods and Fig. S1 in the supplementalmaterial).

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FIG. 8. Mutation of eight predicted SREs in the Hsp83 ORF results in transcript stabilization. (A) Northern blot analysis of H-H^8xSRE(-)-H transcripts [8xSRE(-)] and endogenous Hsp83 mRNAs in unfertilized eggs. H-H^8xSRE(-)-H transcripts were detected by probing with the p53-LNA-3'-digoxigenin probe described in Materials and Methods. Endogenous Hsp83 mRNA from non-8xSRE(-) eggs served as a positive control for instability, and endogenous rpA1 mRNA was used as a loading control for normalization. H-H^8xSRE(-)-H transcripts were strongly stabilized: by 4 to 6 h AEL in unfertilized eggs, 76% ± 27% of transgenic transcripts were present compared with only 13% ± 4% of endogenous Hsp83 transcripts. (B) Quantification of Northern blot data in panel A. Error bars represent standard deviations calculated from at least two independent experiments.

Northern blot analysis of H-H^8xSRE(-)-H mRNA showed that itwas strongly stabilized: by 4 to 6 h AEL in unfertilized eggs76% ± 27% of transgenic transcripts remained, comparedwith only 13% ± 4% of endogenous Hsp83 transcripts incontrols (Fig. 8). Strong stabilization also occurred in embryos,with 68% ± 12% of the H-H^8xSRE(-)-H transcripts remainingat 3 to 4 h AEL (data not shown).

Together with our results obtained by point mutation of SMG'sRBD, we conclude that SMG interacts directly with the SREs inthe Hsp83 ORF to destabilize the mRNA. Since mutation of fourout of the eight predicted SREs did not abrogate transcriptdestabilization (30) while mutation of all eight did, we concludethat SMG is likely to bind to more than four SREs to destabilizethe Hsp83 transcript.

DISCUSSION

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DISCUSSION

We have shown here that the Drosophila Hsp83 mRNA contains onemajor and several minor instability elements that direct transcriptdegradation upon egg activation via what we previously termedthe "maternal degradation pathway" (4). The major instabilityelement (the HIE) resides in the 3'-most 615 nt of the ORF butdoes not require ribosome transit for its destabilizing function.The HIE contains six of the eight predicted SREs in the Hsp83transcript and is able to direct an mRNA to associate with anSMG-containing mRNP, thus conferring SMG-dependent destabilizationon that transcript. Two additional predicted SREs are presentoutside the HIE, in the more-5' part of the Hsp83 ORF. Mutationof the SMG RBD or of all eight SREs results in stabilizationof the Hsp83 transcript. Thus, SMG directly interacts with multipleSREs in the Hsp83 ORF to recruit the CCR4-NOT deadenylase andtrigger decay. The only previously identified Drosophila transcriptshown to be directly bound by SMG is nanos, which has two SREsin its 3' UTR (11, 12, 32, 33). However, precedent for an ORF-locatedSRE comes from budding yeast, where it has been shown that theORF of the NNF1 mRNA contains a single SRE, which confers VTS1-dependentinstability (1).

Our analyses have also shown that an auxiliary instability element(the HDE [4]) resides in the Hsp83 3' UTR. The HDE is capableof weakly destabilizing an otherwise stable mRNA (rpA1); however,its role in the context of the Hsp83 mRNA is revealed only ina situation in which more than 80% of the ORF is deleted—includingseven of the eight predicted SREs—thus partially stabilizingthe transcript and sensitizing it to deletion of the HDE.

Mechanism of HIE function. Studies of c-fos and c-myc mRNA decay in mammalian cells andMAT ${alpha}$ 1 mRNA decay in S. cerevisiae have provided a detailed mechanisticunderstanding of how coding region determinants (CRDs) act todestabilize their mRNAs (7-9, 18, 22, 29). The rapid decay ofc-fos mRNA involves the formation of a pre-translation-initiationmRNP that acts to bridge the coding region instability elementwith the poly(A) tail via the RNA-binding proteins UNR, PABP,PAIP, hnRNP D, and NSAP. Upon ribosome transit, mRNP reorganizationpermits access of the CCR4-NOT deadenylase to the poly(A) tail,leading to mRNA degradation. In contrast, degradation of c-mycand MAT ${alpha}$ 1 mRNAs is due to ribosome pausing at rare codons foundin the vicinity of the CRDs. It is believed that ribosome stallingcreates a downstream region devoid of ribosomes, which can beaccessed by the degradation machinery unless the regions downstreamof the rare codons are bound by protective RNA-binding factors.

Translation-independent CRDs, which function either to stabilizeor to destabilize mRNAs, have been identified in several transcripts.Stabilizing elements reside in the ORF of the yeast OLE1 mRNA(42), and destabilizing elements map to the ORFs of mammalianPAI-2 and MnSOD mRNAs (14, 40). The CRDs in PAI-2 and MnSODmRNAs do not require ribosome transit and function when insertedinto a 3' UTR. trans-acting RNA-binding proteins required forthe function of the CRDs of PAI-2 and MnSOD have yet to be identified,and their decay mechanisms remain unknown.

Formally, the HIE resembles the PAI-2 and MnSOD CRDs. Maternallyloaded Hsp83 mRNA is actively translated in the early Drosophilaembryo (30), and we have shown here that a 5' UTR hairpin thatinhibits translation has no effect on Hsp83 transcript instability.Despite the fact that the HIE maps within the coding region,it continues to function when inserted into a 3' UTR. Thus,ribosome transit is not required for HIE function. Below wepresent a model for the role of the HIE—and its residentSREs—in transcript destabilization.

The role of the HDE. Our previous work identified the 97-nt HDE in the Hsp83 3' UTRas an instability element that functions in the maternal degradationpathway (3, 4). We have shown here that these earlier resultswere a consequence of the use of a reporter mRNA (H-H^1.8kb+lacZ-H)lacking most of the ORF-located instability elements (sevenof eight SREs) and sensitized to deletion of the auxiliary element.Deletion of the HDE in this context (H-H^1.8kb+lacZ-H^HDE) thusresulted in strong transcript stabilization while the same reporterwithout the HDE deletion was only weakly unstable.

Our previous analyses also suggested that the HDE might functionboth as an instability element and as a translational enhancer(4). We have recently identified a multiprotein complex thatbinds the HDE and mediates translational enhancement (24). Threeproteins—DDP1, HRP48, and PABP—function togetherto stimulate translation. To date, none of these proteins hasbeen implicated in the transcript destabilization function ofthe HDE.

SMG, SREs, and Hsp83 mRNA destabilization. In a previous study we identified and simultaneously mutatedfour potential SREs in the Hsp83 ORF without affecting transcriptdestabilization (30). Identification of those SREs was basedon the loop consensus CNGGN_0-1 (2). More recently, a revisedloop consensus sequence (CNGGN_0-3) (1) enabled us to identifyfour additional predicted SREs within the Hsp83 transcript.Thus, there are a total of eight predicted SREs in the Hsp83mRNA, all in the ORF (Fig. 9; see also Fig. S1 in the supplementalmaterial). Of the large fragments of the ORF that were testedfor sufficiency, only HORF4 (the HIE) was able to confer stronginstability, and it contains six of the predicted SREs. Theother three large fragments (HORF1, HORF2, and HORF3) each containa single predicted SRE and did not, by themselves, confer instability.Of the subfragments of HORF4 that were sufficient to conferweak instability, two contain three predicted SREs (HORF4-7and HORF4-8), one contains two predicted SREs (HORF4-1), andone (HORF4-6) carries a single predicted SRE. In contrast, ofthe four subfragments of ORF4 that were not sufficient to conferinstability, three contain a single predicted SRE (HORF4-3,HORF4-4, and HORF4-5) and one (HORF4-2) contains no predictedSRE. Thus, there is a good correlation between the number ofpredicted SREs in a fragment and its ability to destabilizea hybrid mRNA. Based on this correlation, a plausible hypothesisis that multiple SREs in the Hsp83 mRNA's ORF function togetherto bind strongly to SMG and recruit the transcript to an SMG-containingmRNP, following which deadenylation by the CCR4-NOT deadenylasetriggers decay.

Two complementary approaches were used to prove that SMG bindingto multiple SREs in the Hsp83 ORF is required to trigger destabilization.First, a single-amino-acid substitution, A462H, in the RBD ofSMG completely stabilized the endogenous Hsp83 mRNA. Second,simultaneous mutation of all eight predicted SREs (without significantlyaffecting the coding capacity of the ORF) stabilized a transgenicHsp83 transcript.

The fact that mutation of four of the predicted SREs (two inthe HIE) did not stabilize the mRNA (30) whereas mutation ofall eight predicted SREs (six in the HIE) did suggests a requirementfor multiple SREs in Hsp83 transcript destabilization. Usingmetabolic labeling with [³⁵S]methionine, we showed previouslythat, in early embryos, Hsp83 transcripts are in fact translatedas well as destabilized (30). In light of this fact, the locationof all of the predicted SREs in the Hsp83 ORF rather than itsUTRs has mechanistic implications for transcript destabilizationsince SMG cannot remain bound while a ribosome transits throughan SRE. First, it is possible that only a fraction of Hsp83mRNA is translated in early embryos; thus, most of the maternalHsp83 transcripts may exist in an untranslated state with SMGbound and, therefore, able to recruit the deadenylase. Alternatively,most Hsp83 transcripts may be translated and their destabilizationmay result from the distribution of multiple SREs over a largedomain rather than clustered as a pair as in the 3' UTR of thenanos mRNA (11, 12, 32, 33). A plausible model is that multiple,widely spaced SREs ensure that some SMG molecules remain boundto an Hsp83 mRNA molecule even as ribosomes transit its ORF.The Hsp83 mRNA could, then, be targeted for deadenylation anddecay even though it was simultaneously being translated. Thus,the SREs in the ORF permit transcript destabilization in spiteof—but not because of—translation.

ACKNOWLEDGMENTS

We thank Arash Bashirullah for designing and Tyler Davies formaking the H-H-H^HDE construct. Najeeb Siddiqui and Wael Tadroskindly provided critical comments on a draft of the manuscript.

Trainee support came from the following sources: a Natural Sciencesand Engineering Research Council of Canada (NSERC) GraduateScholarship (J.L.S.), a Canada Graduate Scholarship from theCanadian Institutes for Health Research (CIHR) (J.L.S.), studentshipsfrom the Ontario Student Opportunity Trust-Hospital for SickChildren Foundation Student Scholarship Program (J.L.S. andR.L.C.), and a scholarship from the CIHR (R.L.C.). H.D.L. isCanada Research Chair (Tier 1) in Developmental Biology at theUniversity of Toronto. This research was supported by an operatinggrant to C.A.S. from the National Cancer Institute of Canadawith funds from the Terry Fox Run and an operating grant (MOP-14409)to H.D.L. from the CIHR.

FOOTNOTES

* Corresponding author. Mailing address: Department of Molecular Genetics, University of Toronto, Medical Sciences Building, Room 4384D, 1 King's College Circle, Toronto, Ontario M5S 1A8, Canada. Phone: (416) 946-5296. Fax: (416) 971-2494. E-mail: howard.lipshitz{at}utoronto.ca

Published ahead of print on 15 September 2008.

Supplemental material for this article may be found at http://mcb.asm.org/.

REFERENCES

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