All Small Nuclear RNAs (snRNAs) of the [U4/U6.U5] Tri-snRNP Localize to Nucleoli; Identification of the Nucleolar Localization Element of U6 snRNA

doi:10.1091/mbc.01-12-0596

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Vol. 13, Issue 9, 3123-3137, September 2002

All Small Nuclear RNAs (snRNAs) of the [U4/U6.U5] Tri-snRNP Localize to Nucleoli; Identification of the Nucleolar Localization Element of U6 snRNA

Susan A. Gerbi, and Thilo Sascha Lange^*

Division of Biology and Medicine, Brown University, Providence, Rhode Island 02912

Submitted December 27, 2001; Revised May 10, 2002; Accepted June 5, 2002
Monitoring Editor: Elizabeth H. Blackburn

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Previously, we showed that spliceosomal U6 small nuclear RNA (snRNA) transiently passes through the nucleolus. Herein, wereport that all individual snRNAs of the [U4/U6.U5] tri-snRNPlocalize to nucleoli, demonstrated by fluorescence microscopyof nucleolar preparations after injection of fluorescein-labeledsnRNA into Xenopus oocyte nuclei. Nucleolar localization of U6is independent from [U4/U6] snRNP formation since sites of directinteraction of U6 snRNA with U4 snRNA are not nucleolar localizationelements. Among all regions in U6, the only one required for nucleolarlocalization is its 3' end, which associates with the La proteinand subsequently during maturation of U6 is bound by Lsm proteins.This 3'-nucleolar localization element of U6 is both essentialand sufficient for nucleolar localization and also required forlocalization to Cajal bodies. Conversion of the 3' hydroxyl ofU6 snRNA to a 3' phosphate prevents association with the La proteinbut does not affect U6 localization to nucleoli or Cajalbodies.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The nucleolus is the site of ribosome biogenesis (for review, see Gerbi et al., 2001). However, the nucleolus seems to beplurifunctional and contains RNA used for other events, such asthe RNA component of RNase P, which catalyzes the 5' processingof pre-tRNA (Jacobson et al., 1997; Bertrand et al., 1998; Jarrouset al., 1999), signal recognition particle RNA that assembleswith proteins in the nucleolus (Jacobson and Pederson, 1998; Politzet al., 2000) and telomerase RNA (Mitchell et al., 1999; Narayananet al., 1999b).

Recently, it has been reported that several of the small nuclear RNAs (snRNAs) pass through the nucleolus before their nucleoplasmicdestination where splicing occurs. U6 snRNA transiently localizesto nucleoli (Lange and Gerbi, 2000) where it seems to undergo2'-O-methylation and pseudouridylation of defined nucleotides,guided by small nucleolar RNAs (snoRNAs) (Tycowski et al., 1998;Ganot et al., 1999). Similarly, U2 snRNA is found in nucleoli(Lange and Gerbi, 2000) where it seems to be modified by guidesnoRNAs, probably after reimport to the nucleus from the cytoplasm(Yu et al., 2001). In addition, guide snoRNAs for modificationof several spliceosomal snRNAs have also been identified (Hüttenhoferet al., 2001). In this report, we present direct evidence thattwo of the targets of modification, U4 and U5 snRNAs, localizeto nucleoli. Therefore, the list of snRNAs associated with nucleoliis expanded to U6 (Lange and Gerbi, 2000), U2 (Lange and Gerbi,2000; Yu et al., 2001), and U4 and U5 snRNAs (thisreport).

The observation of nucleolar localization of U6 snRNA raises the question at which point of its life cycle U6 enters the nucleolus.Upon transcription by RNA polymerase III (Dahlberg and Lund, 1991),the first protein to associate with U6 snRNA is La (Rinke andSteitz, 1985; Kunkel et al., 1986), which generally binds to the3' termini of nascent RNA polymerase III transcripts and a numberof viral RNAs (Chang et al., 1994; Simons et al., 1996). Subsequently,the 3'-poly U end of U6 elongates during maturation and then istrimmed to approximately five uridines with conversion of the3' end of U6 snRNA from a hydroxyl group to a 2',3'-cyclic phosphate(Lund and Dahlberg, 1992; Terns et al., 1992). At this point,La is replaced by the evolutionarily conserved Sm-like (Lsm) proteinsLsm 2-8 (Cooper et al., 1995; Séraphin, 1995; Pannone et al.,1998; Achsel et al., 1999; Mayes et al., 1999; Salgado-Garridoet al., 1999), which facilitate the formation of the [U4/U6] di-snRNP(Achsel et al., 1999). The Lsm proteins are specific in theirbinding to U6 snRNA and do not associate with U1, U2, U4, or U5snRNAs that instead are bound by Sm proteins (Achsel et al., 1999;Stevens and Abelson, 1999). Then, the [U4/U6.U5] tri-snRNP formsto which Lsm2-Lsm8 and other proteins are associated (Achsel etal., 1999; Gottschalk et al., 1999; Mayes et al., 1999; Salgado-Garridoet al., 1999; Stevens and Abelson, 1999), and the use of U6 snRNAin the nucleoplasm for splicingensues.

The experiments presented herein demonstrate that the 3' end of U6, which in vivo associates with the La protein and subsequentlywith the Lsm protein complex to form the [U4/U6.U5] tri-snRNP,is essential for nucleolar localization as well as localizationto Cajal (coiled) bodies but not for assembly with U4 snRNA. Furthermore,by alteration of the 3' end of U6 snRNA, we can exclude the possibilitythat La plays a role in localization of U6 to the nucleolus orto Cajal bodies. In addition, we demonstrate that all snRNAs ofthe [U4/U6.U5] tri-snRNP localize tonucleoli.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In Vitro Transcription and Labeling of RNA

In vitro transcription reactions using polymerase chain reaction (PCR)-generated DNA templates produced the labeled RNAs usedin the present study. The templates and primers used for PCR aregivenbelow.

Templates. The starting material for the template for in vitro transcription of U6 snRNA was the human U6 clone pT7U6 (Tycowski et al.,1998), which carries a U6 gene that is identical in sequence toXenopus tropicalis (Krol et al., 1987) except for a one base differenceat nucleotide (nt) 6. An appropriate 5' primer was used to givea PCR product identical to the Xenopus U6 snRNA gene sequence,as described previously (Lange and Gerbi, 2000); this was subclonedinto pCR3.1 (Invitrogen, Carlsbad, CA) and its sequence was confirmed.The template and primers for wild-type (WT) U6 snRNA have beendescribed in Lange and Gerbi (2000). The primers to generate templatesby PCR for in vitro transcription of mutant U6 snRNA and of wild-typeU4 or U5 snRNA are listed below. Clones containing the genes forXenopus laevis U5 snRNA (Kazmaier et al., 1987) and chicken U4BsnRNA (Hoffman et al., 1986) were kindly provided by I.W. Mattaj(European Molecular Biology Laboratory, Heidelberg, Germany) inthe pUC9 plasmid; the corresponding snRNAs were used in this studybecause their structure-function relationships were previouslyextensively characterized in Xenopus oocytes (Vankan et al., 1990,1992). Transcripts of U3 snoRNA were prepared as described previously(Lange et al., 1998c).

A triple repeat of the 3' end of U6 snRNA (nt 87-107, called 3'-end nucleolar localization element [NoLE]) was generated byPCR and its sequence confirmed. This NoLE construct was generatedusing 5' and 3' primers listed below. The minus strand templatewas 5'-TTG CCG AGG AGC TT(A AAA ATA TGG AAC GCT TCA CG)(A AAAATA TGG AAC GCT TCA CG)(A AAA ATA TGG AAC GCT TCA CG) C CCT ATAGTG AGT CGT ATT A-3'. The first 14 nucleotides of this oligonucleotideare derived from the genomic sequence (Krol et al., 1987

) thatfollows the 3' end of the U6 snRNA coding region of X. tropicalis.The 21 nt shown in parentheses and repeated three times are complementaryto nt 87-107 at the 3' end of U6 snRNA. The nt in italics arethe first 18 nucleotides of the T7 promotor. Restriction of the3'-end PCR template with MseI (site is underlined above) removedthe genomic sequence flanking the gene; subsequent in vitro transcriptionproduced the 65-nt 3'-end RNA construct (triple repeat precededby GG from the T7promoter).

The 3'-end NoLE construct just described was also tested for nucleolar localization in a heterologous context by couplingit to the 3' end of a synthetic control RNA (Lange and Gerbi,2000

). The template for this construct (control RNA/3' end) wascreated by annealing (complementary sequences are underlined)and PCR extension of the following two oligonucleotides: 5'-TAATAC GAC TCA CTA TAG GGT CCT GTC GAC TCC TCC TCC TCC TCC TCC GCG GAT TTA CCT CGG CAA CGT-3'and 5'-TAA ATG AGG AGC TT(A AAA ATA TGG AAC GCT TCA CG)(A AAAATA TGG AAC GCT TCA CG)(A AAA ATA TGG AAC GCT TCA CG)T TGC CGA GGT AAA TCC GCG GA-3';the T7 promotor is shown in italics and the 3'-end NoLE (nt 87-107)repeated three times are enclosed by parentheses. The syntheticcontrol RNA by itself was created by PCR by using the templateand primers described by Lange and Gerbi (2000)

. U2 snRNA wasused as a control for immunoprecipitation experiments and stabilityassays and was derived as described previously (Lange et al.,1998a

5' End Primers (T7 Promotor Shown in Italics). U4 WT 5'-TAA TAC GAC TCA CTA TAG GGA GCT TTG CGC AGT GGC AGT ATC-3'; U5 WT 5'-TAA TAC GAC TCA CTA TAG GGA TAC TCT GGT TTCTCT TCA AAT TCG AAT AAA TC-3'; U6 $Delta$ 1-19 5'-TAA TAC GAC TCA CTATAG GGA TAT ACT AAA ATT GGA-3'; U6 $Delta$ 20-25 5'-TAA TAC GAC TCA CTATAG GGT GCT TGC TTC GGC AGC ACT AAA ATT GG-3'; U6 sub20-25 (substitutionis underlined) 5'-TAA TAC GAC TCA CTA TAG GGT GCT TGC TTC GGCAGC ACG AGC GGT AAA ATT GG-3'; U6 $Delta$ 26-42 5'-TAA TAC GAC TCA CTATAG GGT GCT TGC TTC GGC AGC ACA TAT ACA GAG AAG AT-3'; and T7promoter for 3'-end construct 5'-TAA TAC GAC TCA CTA TAG GG-3'.

3' End Primers. U4 WT 5'-CAG TCT CCG TAG AGA CTG TCA-3'; U5 WT 5'-TAC CTG GTG TGA ACC AGG CTT C-3'; U6 $Delta$ 43-56 5'-AAA AAT ATG GAA CGC TTC ACGAAT TTG CGT GTC ATC CTT GCG CAG GGG CCA GTA TCG TTC C-3'; U6 $Delta$ 57-815'-AAA AAT ATG GAA CGC TTC ACG AAT TTT GCT AAT CTT-3'; U6 $Delta$ 43-815'-AAA AAT ATG GAA CGC TTC ACG AAT TTG TAT CGT TCC-3'; U6 $Delta$ 82-955'-AAA AAT ATG GAA GCG TGT CAT CCT TGC-3'; U6 $Delta$ 96-99 5'-AAA AATATC GCT TCA CGA ATT T-3'; U6 $Delta$ 100-102 5'-AAA AAG GAA CGC TTC ACGAAT TTG CGT GTC ATC CTT G-3'; U6 $Delta$ 103-107 5'-TAT GGA ACG CTT CACGAA TTT GCG TGT CAT CCT TG-3'; U6 $Delta$ 100-107 5'-GGA ACG CTT CACGAA TTT GCG TGT CAT CCT TG-3'; U6 $Delta$ 82-107 5'-GCG TGT CAT CCT TGCGCA GGG GCC-3'; and U6 3'-end 5'-TTG CCG AGG AGC TTA AA-3' (genomicsequence downstream ofU6).

In vitro transcripts of RNA were made with either fluorescein-12-UTP (PerkinElmer Life Sciences, Boston, MA) and/or $alpha$ -[³²P]UTP (PerkinElmer Life Sciences) label that was added to a T7megascript in vitro transcription kit (Ambion, Austin, TX). TheT7 transcripts were purified according to Lange et al. (1999)

.They all contained GG at their 5' ends from the T7 promoter andwere capped with m⁷G(5')ppp(5')G (Ambion) to improvestability.

Oocyte Microinjection

Stage V-VI oocytes from X. laevis were obtained as described previously (Lange et al., 1998a). For fluorescence analysis ofnucleolar localization as well as for stability assays, oocytenuclei were injected with 0.8 ng of wild-type U4, U5, and U6 snRNAor U3 snoRNA in 9.2 nl of H₂O. For the U6 snRNA mutants that wereshorter than the wild-type and for the 3'-end construct, amountsequimolar to the wild-type U6 RNA (0.8 ng = ~23 fmol of in vitro-transcribedWT U6 snRNA) were injected. The concentration of U6 used for injectionwas determined by titration to be the lowest possible that stillgave specific labeling of nucleoli (our unpublished data) andis in the range of the concentration of endogenous U6 (~7.5 fmol/stageV-VI oocyte as determined by Northern blot analysis), whereasthere is nuclear retention of up to ~500-600 fmol of U6 per Xenopusoocyte (Boelens et al., 1995; Terns et al., 1995). The concentrationused for injection of our transcripts is also in the range ofthose used by Gall et al. (1999) for oocyte injection of U1, U2,and U5 snRNA. For the 40-nt negative control RNA, 0.8 ng/oocytewas injected, which is equivalent to ~62 fmol/oocyte. A furthercontrol was the injection of an excess of fluorescein-labeledUTP at 5 pmol/oocyte. We confirmed that microinjected U4 and U6snRNA transcripts could participate in their normal functionalpathway and form a di-snRNP. This was achieved by coimmunoprecipitation(see section below) with an anti-Sm antibody as described previously(Vankan et al., 1990, 1992). Endogenous U6 and U4 snRNA were disruptedthrough RNase H-mediated destruction by two nuclear injectionsspaced 4 h apart of 9.2 nl of each of the following antisenseoligonucleotides at a concentration of 3 µg/µl (28 ng/oocyte):a combination of two oligonucleotides complementary to nt 20-53(5'-TAA TCT TCT CTG TAT CGT TCC AAT TTT AGT ATA T-3') and nt 75-102(5'-TAT GGA ACG CTT CAC GAA TTT GCG TGT C-3') was used for U6depletion. U4 depletion was carried out with an oligonucleotidecomplementary to nt 51-83 (5'-GGG TAT TGG GAA AAG TTT TCA ATTAGC AAT A-3').

Nucleolar Localization Assay

After incubation of the oocytes for a stipulated time (1.0-1.5 h unless specified otherwise), nuclear spreads were made asdescribed previously (Lange et al., 1999) using a method for preparationof lampbrush chromosomes (Gall et al., 1991). For Cajal body immunostaining,the slides were fixed for 1 h in 2% paraformaldehyde in phosphate-bufferedsaline (PBS) (137 mM NaCl, 3 mM KCl, 6.4 mM Na₂HPO₄, and 1.5 mMKH₂PO₄, pH 7.0), washed in PBS, and unspecific binding sites saturatedwith 10% bovine serum albumin in PBS for 20 min. Subsequently,rabbit polyclonal serum against a synthetic 21 amino-acid fragmentof Xenopus coilin (kindly provided by J.G. Gall, Carnegie Institution,Baltimore, MD) was applied as a primary antibody for immunostainingof Cajal bodies at a dilution of 1:1000 in PBS for 20 min at 4°C.The preparations were rinsed 3× for 5 min each in PBS and incubatedfor 20 min at 4°C with the secondary antibody (goat anti-rabbit;Molecular Probes, Eugene, OR) coupled to the dye Alexa 594. Subsequently,slides were washed 3× with PBS for 5 min each and the DNA stainedwith 200 ng/ml 4'-6-diamidino-2-Phenylindole (DAPI) in PBS for5 min. Fluorescence microscopy was performed as described previously(Lange and Gerbi, 2000) with the exception that ProLong mountingmedium (Molecular Probes) was used. Nucleolar preparations wereanalyzed with an Axiophot epifluorescence microscope (Carl Zeiss,Thornwood, NY) equipped with a 100× Neofluar Ph 3 objective anda 100-W mercury lamp. Pictures were taken with constant exposuresfor each filter set (for DAPI, Alexa 594, or fluorescein) by usingEktachrome 400× professional film (Eastman Kodak, Rochester, NY).Therefore, any difference in signal strength between various samplesis directly visualized without the interference of software orautomatic camerasettings.

snoRNA Stability Assay

To determine the stability of the various in vitro transcripts after injection into oocyte nuclei, U2 snRNA was coinjectedand served as an internal control to normalize for any differencesin injection or recovery of the samples. At defined time pointsafter injection of the oocytes with [ $alpha$ -³²P]UTP-labeled RNAs, the RNA of four nuclei per sample was recoveredand analyzed as described previously (Lange and Gerbi, 2000).

Immunoprecipitation of U6 snRNA from Oocytes

For immunoprecipitation experiments, 0.8 ng/oocyte of the purified U6 snRNA (colabeled with $alpha$ -[³²P]UTP and with fluorescein-12-UTP) and either 0.8 ng/oocyte fluorescein-12-UTP-labeledU4 snRNA or $alpha$ -[³²P]UTP-labeled U3 snoRNA were coinjected into Xenopus oocytes andincubated for 1 or 4 h (depending on the experiment) at 20°C.For each sample, 10 nuclei were homogenized on ice in 50 µl ofisolation buffer (50 mM NaCl, 10 mM Tris pH 8.0, 1 mM dithiothreitol,100 U/ml RNase inhibitor [Roche Applied Science, Mannheim, Germany],one tablet of protease inhibitor cocktail [Roche Applied Science]per 10 ml of isolation buffer), and spun for 1 min in a microcentrifugeat 10,000 rpm. The supernatant was removed, spun again twice,and then added to 240 µl of IP 150 (150 mM NaCl, 10 mM Tris pH8.0, 0.1% NP-40, 1 mM dithiothreitol, 10 U/ml RNase inhibitor[Roche Applied Science], and one tablet of protease inhibitorcocktail [Roche Applied Science] per 10 ml of isolation buffer),and 20 µl of protein A-Sepharosebeads.

The beads had been coupled either to rabbit-anti-Xenopus La antibody (immune serum 79, provided by S. Clarkson, UniversityMedical Center-CMU, Geneva, Switzerland; Lin-Marq and Clarkson,1998) or to preimmune serum as a control, or in other cases tomonoclonal Y12 mouse anti-Sm antibody (Lerner et al., 1981) ormouse IgG as a control by incubation of 150 µl of preswollen beadswith 150 µl of IP 500 (500 mM NaCl, 10 mM Tris pH 8.0, 0.1% NP-40,and 0.1% sodium azide) and 200 µl of antibody for 4 h at 4°C withend over end rotation before they were spun and washed 3× in IP150 in a microcentrifuge at 1000 rpm. The mixture of nuclear extractand antibody-coupled beads was rotated end over end for 90 min(anti-La antibody) or 8 h (anti-Sm antibody) at 4°C before thebeads were spun and washed 5× in IP 150 in a microcentrifuge at1000 rpm. Then the RNA was isolated and purified. PrecipitatedRNA and supernatant were analyzed on a denaturing 7 M urea, 8%polyacrylamide gel (1 mm in thickness, 35 cm in length). It isimportant to note that although U4 transcript association withSm proteins and U6 is initiated upon injection into the oocyte,further association can also occur during coincubation of nuclearlysate with antibody-coupled beads. Therefore, accurate kineticsof in vivo association of U4/U6 cannot be carriedout.

For alteration of the 3'-hydroxyl end of U6 to a 3'-phosphate group, 10 µl with the in vitro transcript (~1 µg) was incubatedin Whitfield's reagent (25 mM NaIO₄ and 1 M lysine, pH 8.5) for2 h at 45°C (Lund and Dahlberg, 1992; Terns et al., 1992). Thistreatment of oxidation- $beta$ elimination also shortens the input RNAby 1 nt (Terns et al., 1992).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Nucleolar Localization of U4 and U5 snRNA

U4 snRNA and subsequently U5 snRNA and U2 snRNA associate with U6 to form the [U4/U6] di-snRNP, [U4/U6.U5] tri-snRNP, and[U2.U4/U6.U5] tetra-snRNP (Konarska and Sharp, 1988; Hall andKonarska, 1992; Wassarman and Steitz, 1992; Raghunathan and Guthrie,1998b). To complete the picture, we analyzed whether U4 and U5snRNAs associate with nucleoli, like U6 (Lange and Gerbi, 2000)and U2 (Lange and Gerbi, 2000; Yu et al. 2001). This was monitoredby a technique used previously to define the nucleolar localizationelements (NoLEs) of snoRNAs from various families (Lange et al.,1998a,b,c, 1999; Narayanan et al., 1999a,b) as well as nucleolarlocalization of U6 snRNA (Lange and Gerbi, 2000). Fluorescein-labeledin vitro transcripts were injected into Xenopus oocyte nucleito allow direct visualization of the labeled RNA in nucleolarpreparations madesubsequently.

In the present study, fluorescein-labeled in vitro transcripts of U4 snRNA and U5 snRNA were injected into Xenopus oocytenuclei. Controls included injection of nucleolar U3 snoRNA asa positive control, and injection of a 40-nt synthetic RNA orfluorescein-UTP as negative controls to rule out nonspecific nucleolarstaining (e.g., by diffusion of excess material). After 8 min,1 h, and 24 h (the longest time point feasible to be studied),the oocytes were manually dissected and the nuclear contents,including nucleoli, were centrifuged onto a microscope slide.As shown in Figure 1a, strong fluorescent signals depicting nucleolarlocalization of U4 and U5 snRNA were detected 8 min and 1 h afterinjection of 0.8 ng of transcript per oocyte nucleus. Likewise,nucleoli were stained by a positive control (U3 snoRNA), injectedat the same concentration that had been previously optimized forthe nucleolar localization assay (Lange et al., 1998c). In contrast,negative controls (40-nt synthetic RNA = control RNA, or unincorporatedfluorescein-UTP), both injected in excess (see MATERIALS AND METHODS)did not stain nucleoli. Twenty-four hours after incubation, onlyU3 snoRNA retained strong signals in nucleoli, whereas U4 snRNAlabeling was reduced and U5 snRNA signals were close to background(Figure 1a). This observation is consistent with the nucleolusbeing the functional compartment for U3 snoRNA and with the predictedtransient nature of snRNA localization to nucleoli, as has beenalready shown for U6 snRNA in the same system (Lange and Gerbi,2000).

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Figure 1. Nucleolar localization of U4 and U5 snRNA. (a) Fluorescein-labeled U4 snRNA or U5 snRNA were injected into the nuclei of X. laevis oocytes to analyze nucleolar localization. Controls included injection of nucleolar U3 snoRNA as well as synthetic RNA or fluorescein-UTP to rule out nonspecific nucleolar staining. After 8 min, 1 h, or 24 h, nuclear spreads were prepared and analyzed by phase contrast (PC) or fluorescence microscopy. Nucleoli can be distinguished from other nonchromosomal nuclear bodies by staining of the rDNA (DAPI, blue). Strong nucleolar labeling (FL, green) is seen as early as 8 min after nuclear injection of U4 or U5 snRNA and continues at 1 h after injection. Likewise, nucleoli were stained by a positive control (U3 snoRNA) at these time points, whereas negative controls (control RNA or unincorporated fluorescein-UTP), both injected in excess (see MATERIALS AND METHODS), did not stain nucleoli. Twenty-four hours after incubation only U3 snoRNA retains strong signals in nucleoli, whereas U4 snRNA labeling is reduced and U5 snRNA signals are close to background. Stronger nucleolar staining by U4 snRNA compared with U5 snRNA or U6 snRNA was generally observed at all time points. Bar, 10 mm. (b) ³²P-Labeled transcripts of U4 and U5 snRNA were injected into oocyte nuclei to determine their stability; the RNAs were isolated and analyzed by gel electrophoresis as described previously (Lange et al., 1999

). U2 snRNA transcripts were coinjected and served as an internal control to normalize for any differences in injection or recovery of the samples. U4 and U5 snRNA are stable 24 h after oocyte injection, compared to the 0-h control. Similarly, as published previously (Lange and Gerbi, 2000

) U3 snoRNA, U6 snRNA, or the control RNA were stable through 24 h.

The nucleolar localization of fluorescent U4 and U5 snRNA was specific, because injection of an unrelated control RNA, evenat ~3 times the molar amount of U4 or U5, did not stain nucleoli.Additional controls demonstrated that the observed fluorescentsignals were not due to degradation of fluorescent snRNA and subsequentreutilization of the label by other nuclear components. First,injection of a ~75-fold molar excess of fluorescein-UTP alonedid not label the nucleoli (Figure 1a). Second, stability assaysusing ³²P-labeled transcripts demonstrated that U4 and U5 snRNA transcriptswere stable at the times the nucleolar localization assay wasperformed (Figure 1b). Similarly, as previously published forU3 snoRNA, U6 snRNA, or the control RNA (Lange and Gerbi, 2000),U4 and U5 snRNAs were stable over 24h.

Sequences of U6 snRNA Essential for Nucleolar Localization

To define cis-acting elements of U6 snRNA necessary for nucleolar localization, the localization of mutant transcripts wascompared with that of wild type. The scheme in Figure 2 (modifiedfrom Vankan et al., 1990 and Tycowski et al., 1998) points outareas of functional interest in wild-type U6 snRNA and also givesan overview of the various U6 mutants designed for the presentstudy. Sequences of mature wild-type U6 snRNA and of the mutantsare listed in detail below the scheme.

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Figure 2. Sequence and mutations of U6 snRNA. The sequence of Xenopus U6 snRNA (Krol et al., 1987

), which is highly conserved across the eukaryotic kingdom (Brow and Guthrie, 1988

), is shown. The figure has been modified from Vankan et al. (1990)

and Tycowski et al. (1998)

. Shaded areas are sites of base pairing with U2 snRNA in the spliceosome and nt 49-74 base pairs with U4 snRNA before association with the spliceosome. Several of the modifications ( $psi$ , pseudouridine; m, methylated nucleotides) occur in areas of U6 snRNA involved in intermolecular base pairing during splicing (Vankan et al., 1990

, 1992

). Most mutations designed for this study were deletions covering the nucleotides indicated by lines. $Delta$ 1-19 was designed to remove the 5'-terminal stem. Nucleotides used for substitution of nt 20-25, which is a sequence needed for nuclear import after injection of U6 into the cytoplasm (Hamm and Mattaj, 1989

), are shown in a box. In various mutations of the middle part of the molecule, sites of base pairing with U2 and U4 snRNA were removed. In addition various deletions were introduced between nt 82 and 107, which includes regions that base pair in the spliceosome with U2 snRNA as well as the 3' terminus of U6 that binds the La protein and subsequently the Lsm proteins (see text). Furthermore, a triple repeat of nt 87-107 of the U6 3' end (3' end) was designed (open box at top of diagram). The lower portion of this figure lists the sequences of mutant U6 snRNAs. Nucleotides that are the same as in wild-type U6 are shown by dots in the sequence alignment, and deletions are indicated by dashes.

There is no previous information at which stage of its life cycle U6 enters nucleoli. It might enter nucleoli as the individualsnRNP or in a complex as a di-snRNP or tri-snRNP directly boundto U4 and in conjunction with U5 snRNA, both of which are alsofound in nucleoli (see above; Figure 1a). Therefore, it was ofparticular interest to analyze whether the sites in U6 (nt 49-74)that base pair with U4 before association with the spliceosomeand that are important for snRNP assembly (Vankan et al., 1990)might play a role in U6 nucleolar localization. However, deletionswithin that sequence ( $Delta$ 43-56, $Delta$ 57-81; Figure 3) or total deletionof the entire middle part of the molecule, including the entireU4 binding site ( $Delta$ 43-81; Figure 3), do not appreciably influencenucleolar localization of U6 snRNA compared with the wild type.This area also contains all sites for nucleolar posttranscriptionalmethylation of U6 as well as a region that base pairs with U2snRNA in the spliceosome (Figure 2). Similarly, U6 snRNA carryinga deletion of the 5' stem ( $Delta$ 1-19) or a deletion of nt 26-42 containinga U2-binding site retained the ability to localize to nucleoli(Figure 3). Therefore, areas of U6 snRNA that will base pair withU4 snRNA or later with U2 snRNA during splicing are not requiredfor nucleolar localization. Interestingly, a deletion or substitutionof nt 20-25 does not affect U6 nucleolar localization (Figure3). This sequence element is responsible for nuclear import ofU6 snRNA after injection into the cytoplasm (Hamm and Mattaj,1989). Although U6 during maturation normally does not travelto the cytoplasm, a mutation of this region was used previouslyto study the effect of additional mutations on the natural nuclearretention of U6 by preventing nuclear reimport of molecules leakinginto the cytoplasm (Boelens et al., 1995).

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Figure 3. Nucleolar localization of U6 snRNA mutated in various positions throughout the molecule. Fluorescein-labeled U6 snRNA mutants were injected into the nuclei of X. laevis oocytes and 1.5 h later the localization assay performed. U6 snRNA carrying a deletion of the 5' stem ( $Delta$ 1-19) or a deletion or substitution of nt 20-25 localized as well to nucleoli as the wild-type (WT) molecule (FL, green). Similarly, various mutants with deletions throughout the middle part of the molecule ( $Delta$ 26-42, $Delta$ 43-56, $Delta$ 57-81, and $Delta$ 43-81) retained full ability to localize to nucleoli. In contrast, a deletion of nt 82-107 completely abolished nucleolar localization. Other details as in Figure 1a.

In contrast to the mutations described above, nucleolar localization of U6 could be completely abolished by a deletion ofnt 82-107 of U6 snRNA (Figure 3). This area contains the 3' terminusof U6, which binds the La protein and subsequently the Lsm proteins(see INTRODUCTION). The 3'-terminal U residues also may somewhatassist nuclear retention of U6, although after deletion of the3' end the majority of U6 injected into Xenopus oocytes stillremained in the nucleus even after long incubation times (Boelenset al., 1995). The present study now demonstrates that the 3'end of U6 snRNA is essential for nucleolar localization, whereasthe remainder of the molecule representing more than three-quartersof the U6 snRNA sequence, including sites absolutely requiredfor [U4/U6] di-snRNP formation, splicing complex assembly, andsplicing activity (Vankan et al., 1990, 1992), lacks elementsimportant for nucleolarlocalization.

In additional control experiments (Figure 4), we confirmed that nucleolar localization is indeed mediated independently from[U4/U6] snRNP assembly because 1) the synthetic U6 snRNA and U4snRNA transcripts generated here by in vitro transcription retaintheir functional activity to form a [U4/U6] snRNP, 2) the mutantU6 $Delta$ 43-81 still localizes to nucleoli even though it lacks theU4 base-pairing sites and cannot interact with U4, and 3) the3'-NoLE U6 mutant that does not localize to nucleoli ( $Delta$ 82-107)is still able to assemble in a [U4/U6] snRNP. The experimentsleading to these observations involved coinjection of U6 snRNA(colabeled with [³²P]UTP and fluorescein-UTP) with U4 snRNA transcripts (labeledwith fluorescein-UTP) into U6- and U4-depleted Xenopus oocytesand subsequent coimmunoprecipitation of these snRNAs with an anti-Smantibody. Because the Sm proteins are bound to U4 and not to U6snRNA, precipitation of U6 occurs only if it is associated withU4 snRNA; this technique was used by Vankan et al., (1990) toidentify domains of U4 and U6 required for snRNP assembly. Figure4 shows that U6 WT and the NoLE 3'-mutant ( $Delta$ 82-107) but not U6mutated in nt 43-81 were coprecipitated with U4 when using ananti-Sm antibody. Moreover, in the converse experiment, U4 carryinga deletion of the base-pairing sites for U6 ( $Delta$ 1-18/56-63) failedto precipitate wild-type U6 snRNA.

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Figure 4. [U4/U6] snRNP assembly after nuclear injection. U6 snRNA (colabeled with [³²P]UTP and fluorescein-UTP) and U4 snRNA transcripts (labeled with fluorescein-UTP) were coinjected into Xenopus oocytes depleted of endogenous U4 and U6 snRNA. After 4 h of incubation the functional ability of the in vitro transcripts to form a [U4/U6] snRNP was analyzed by immunoprecipitation from the nuclear lysate with an anti-Sm protein antibody. The equivalents of 10 nuclei/sample of the precipitated RNA (pellet) and 0.1 nuclei/sample of the supernatant (control for equal amounts injected) were analyzed on a denaturing 8% polyacrylamide, 8 M urea gel and by autoradiography. [U4/U6] snRNP assembly occurs between wild-type U6 snRNA (U6 WT) and wild-type U4 snRNA (U4 WT), also with the U6 NoLE mutant ( $Delta$ 82-107), and even with the truncated 3'end mutant ( $Delta$ 82-107), consistent with Vidal et al. (1999)

. Ability of the transcripts to form a snRNP was disrupted by using either mutant U6 ( $Delta$ 43-81) or mutant U4 ( $Delta$ 1-18/ $Delta$ 56-63) that lack the sites to base pair with each other and that are important for snRNP assembly before association with the spliceosome (Vankan et al., 1990

). It is notable that this U6 mutant ( $Delta$ 43-81) is still capable of localizing to nucleoli (see Figure 3). None of the samples were precipitated by beads coupled to control antibody.

Although not the primary focus of the present study, we also analyzed association of U6 with Cajal bodies, identified by theirimmunostaining for coilin (Figure 5). One hour after nuclear injectionof fluorescein-labeled wild-type U6 snRNA, the Cajal bodies arestained, although not as strongly as nucleoli (Figure 5). Fourhours after injection, consistent with the previously reportedkinetics of nucleolar localization of U6 snRNA (Lange and Gerbi,2000), the nucleoli are weakly stained. At this time point, Cajalbody staining by U6 snRNA remains at low levels (our unpublisheddata). It has been reported that snoRNA lacking the box C/D NoLEaccumulates in Cajal bodies (Narayanan et al., 1999a), and sowe investigated whether a similar phenomenon occurred for U6 snRNA.However, U6 snRNA lacking its NoLE no longer localized to Cajalbodies or nucleoli (Figure 5). Therefore, the 3'-end of U6 snRNAis essential not only for localization to nucleoli but also toCajal bodies.

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Figure 5. The 3' end of U6 is essential for localization to Cajal bodies. Fluorescein-labeled wild-type U6 snRNA as well as the 3' mutant ( $Delta$ 82-107) were injected into the nuclei of Xenopus oocytes and the localization assay performed. Immunostaining of Cajal bodies (CB, red) was carried out in addition to DNA staining of nucleoli (DAPI, blue) to distinguish between these two sites of U6 snRNA localization (FL, green). Injection of wild-type U6 snRNA results in strong labeling of nucleoli and weaker labeling of Cajal bodies 1 h after injection. In contrast, deletion of the U6 3' end ( $Delta$ 82-107) completely abolished localization to nucleoli as well as to Cajal bodies, comparable with background levels seen in uninjected control oocytes (no injection). Other details as in Figure 1a.

Further mutational analysis was carried out to reveal whether specific sequences of a few nucleotides within the 3' part ofU6 are essential for nucleolar localization, similar to the discreteNoLEs of snoRNAs. Four mutations were designed that spanned theregion of interest in U6 snRNA ( $Delta$ 82-95, $Delta$ 96-99, $Delta$ 100-102, and $Delta$ 103-107) (Figure 2). In addition, a mutation spanning the last8 nt ( $Delta$ 100-107) was used, which drastically decreased the interactionof U6 with the La protein in Xenopus oocytes (Boelens et al.,1995). All five mutations of the 3' end of U6 ( $Delta$ 82-95, $Delta$ 96-99, $Delta$ 100-102, $Delta$ 103-107, and $Delta$ 100-107) significantly impaired localization(Figure 6). However, weak fluorescent signals were still obtainedby all five U6 mutants and localization was not entirely abolished.This is in contrast to the U6 mutant, which lacks the entire 3'end ( $Delta$ 82-107) and which was entirely incapable of localizationto nucleoli (Figure 3). Therefore, nucleolar localization of U6snRNA relies on many nucleotides in the 3'-end region, ratherthan on just a few nucleotides.

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Figure 6. Sequences within the 3' end of U6 snRNA that mediate nucleolar localization. Mutational analysis of the 3' portion of U6 snRNA was carried out to analyze whether specific sequences within this region are essential for nucleolar localization. Various deletion mutants of the 3' end of U6 ( $Delta$ 82-95, $Delta$ 96-99, $Delta$ 100-102, $Delta$ 103-107, and $Delta$ 100-107) were impaired in their nucleolar localization 1.5 h after injection. However, they still labeled nucleoli weakly, unlike the larger deletion of the 3' end of U6 ( $Delta$ 82-107; Figure 3) that had no nucleolar signal. Therefore, nucleolar localization relies on many nucleotides in the 3' region. In addition, a triple repeat of the NoLE (3'-end) was tested in the nucleolar localization assay and revealed that nt 87-107 are not only important but also sufficient for nucleolar localization because the construct was able to localize to nucleoli. Similarly, this 3'-end NoLE also localized to nucleoli when it was coupled to a synthetic control RNA (control RNA/3'-end), whereas the control RNA by itself did not. Other details as in Figure 1a.

It was important to ascertain the stability of each mutant U6 snRNA transcript, to guard against the possibility that failureof some mutants to localize to nucleoli was simply due to theirdegradation. Stability assays using ³²P-labeled transcripts demonstrated that all transcripts were sufficientlystable 1.5 h after injection into oocyte nuclei (the time whenlocalization assays were carried out) (Figure 7). This includedU6 mutant $Delta$ 82-107 that failed to localize to nucleoli, as wellas the control RNA. In addition, the use of U6 wild-type as wellas U6 mutants ( $Delta$ 43-81 and $Delta$ 82-107) in immunoprecipitation experimentsconfirmed their stability when labeled with fluorescein-12-UTPand [ $alpha$ -³²P]UTP. Although well beyond the time frame of the localizationassay, we were also interested to see whether any of the U6 mutantswould show significant instability after longer incubation periodsin oocytes. By assaying the long-term stability of transcripts24 h after injection, we found that several U6 mutants of the3' end as well as the 3'-end NoLE constructs (3' end, controlRNA/3' end) were significantly less stable than wild-type U6 snRNA(our unpublished data). This precluded us from carrying out long-termlocalization studies.

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Figure 7. Stability of wild-type and mutated U6 snRNA. ³²P-Labeled U6 snRNAs (mutants or wild type or the 3'-end NoLE constructs) were injected into oocyte nuclei, and the RNAs were isolated and analyzed by 8% polyacrylamide, 8 M urea gel electrophoresis. The top panel shows the 0-h controls and the bottom panel shows the short-term stability at 1.5 h (the time when localization assays were carried out) after injection into oocyte nuclei. To determine the stability of the various RNAs after nuclear injection, U2 snRNA transcripts were coinjected and served as an internal control to normalize for any differences in injection or recovery of the samples. All the U6 mutants as well as the control RNA were stable at the time point used for analysis of nucleolar localization.

For some snoRNAs it has been shown that the NoLEs not only are essential but also are sufficient for nucleolar localizationbecause just the box C/D core structure of C/D snoRNAs can targetsynthetic RNA sequences to the nucleolus (Lange et al., 1998a).Therefore, we analyzed if the 3' sequence of U6 snRNA by itselfis not only essential but also sufficient for nucleolar targeting.As shown in Figure 6, a transcript of just the 3' end of U6 issufficient for nucleolar localization. Similarly, this 3'-endNoLE construct also localized to nucleoli when it was coupledto a synthetic control RNA (control RNA/3' end), whereas the 40-ntcontrol RNA by itself did not (Figure 6). Thus, the nucleotidesthat are both essential and sufficient for nucleolar localizationare nt 87-107, which represent the NoLE for U6snRNA.

Does the 3' End of U6 snRNA Function as a NoLE by Binding to the La Protein?

It has been hypothesized that NoLEs of snoRNAs act by binding protein(s) that either transport the snoRNA from the nucleoplasmto the nucleolus and/or anchor it within the nucleolus. Similarly,binding of specific protein(s) to the NoLE of U6 might initiatenucleolar localization. Deletion of the 8 nt of the U6 NoLE atthe 3' end drastically decreases the interaction of U6 with theLa protein in Xenopus oocytes (Boelens et al., 1995). La is thefirst protein to associate with U6 snRNA, and later it is replacedby the evolutionarily conserved Lsm proteins, which leads to formationof the di- and tri-snRNPs (see INTRODUCTION). It has been shownthat a 3'-end alteration modulates the binding of La protein toU6 snRNA (Lund and Dahlberg, 1992; Terns et al., 1992). This alterationallowed us to find out whether interaction of U6 with La mightbe involved in U6 nucleolarlocalization.

The La protein binds the stretch of uridylates at the 3'-hydroxyl end of newly synthesized U6 snRNA both in vivo and in vitrobut is unable to bind to U6 snRNA that lacks a 3' hydroxyl, andconversion of the U6 3' end in vivo to a 2',3'-cyclic phosphateleads to a replacement of La by Lsm proteins (Lund and Dahlberg,1992; Terns et al., 1992). Consequently, we generated an in vitrotranscript of U6 with an altered 3' end that was unable to bindLa but would allow the nucleolar localization assay to be carriedout to determine whether La plays a role in nucleolar localization.For alteration of the 3'-hydroxyl end, U6 snRNA was incubatedwith Whitfield's reagent; this treatment via oxidation- $beta$ eliminationconverts the 3' hydroxyl to a 3'-phosphate group, resulting ina loss of La binding (Lund and Dahlberg, 1992; Terns et al., 1992).Figure 8a shows migration on a polyacrylamide gel of U6 transcripts(with or without a 3'-hydroxyl group) that were colabeled with³²P for immunoprecipitation and with fluorescein for further studiesin a nucleolar localization assay. The transcripts were coinjectedinto Xenopus oocytes, and binding to the La protein was analyzedby immunoprecipitation (Figure 8b) to confirm that only U6 snRNAwith a 3'-hydroxyl group but not a 3'-phosphate group effectivelybinds to La and can be precipitated by anti-La antibodies. Thesame antibodies precipitated only traces of U3 snoRNA transcriptsthat were coinjected as a control, and the control serum did notprecipitate any of the samples. The gel also shows that the transcriptsremain stable over the time of incubation in the oocyte, whichis equivalent to the time of incubation for the localization assay(1.5 h). Regardless of the alteration, both the 3'-OH and 3'-phosphateforms of U6 localized strongly to nucleoli and, although weaker,to Cajal bodies as well (Figure 8c), indicating that the mechanismof U6 localization to either nuclear subcompartment does not requirea 3'-hydroxyl terminus nor binding of the La protein to the 3'NoLE.

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Figure 8. U6 localization to nucleoli and Cajal bodies does not require a 3'-hydroxyl terminus nor binding of the La protein. (a) U6 snRNA in vitro transcripts with either a 3'-hydroxyl (3'-OH) or a 3'-phosphate (3'-P) group (colabeled with [³²P]UTP and fluorescein-UTP [FL]) were run on a denaturing 8% polyacrylamide, 8 M urea gel and analyzed by autoradiography (left two lanes) and under UV light (right two lanes). Because the 3' modification via oxidation- $beta$ elimination also results in shortening of the RNA by one nucleotide, the transcripts can be distinguished by their different migration. (b) Colabeled U6 snRNA (³²P; FL) with either a 3'-OH or 3'-P group and a control (³²P-labeled U3 snoRNA) were coinjected into Xenopus oocytes. One hour after injection, binding of the injected RNA to the La protein was analyzed by immunoprecipitation with anti-Xenopus La (La) or preimmune serum as a control (Ctr). The equivalents of five nuclei per sample of the precipitated RNA (pellet) and 0.2 nuclei per sample of the supernatant were analyzed by PAGE as in (a). Only U6 snRNA with a 3'-OH group but not a 3'-P group effectively binds to La and can be found in the precipitate. The control preimmune serum did not precipitate any of the samples. (c) Colabeled U6 snRNA transcripts with either a 3'-OH or 3'-P group were injected into the nuclei of X. laevis oocytes and the localization assay carried out. Both transcripts (FL, green) localized strongly to nucleoli (DAPI, blue) and with weaker signals to Cajal bodies (CB, red), indicating that the conversion of the 3'-OH group to a 3'-P group, which blocks La-binding does not affect localization to nucleoli or to Cajal bodies. Other details as in Figure 1a.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

All snRNA Components of [U4/U6.U5] Tri-snRNP Localize to Nucleoli

There are significant differences in the maturation and trafficking of U6 snRNA compared with other spliceosomal snRNAs, includingU4 and U5 of the [U4/U6.U5] tri-snRNP, and it was unknown whetherthese snRNAs localize to nucleoli, similar to U6 snRNA (Langeand Gerbi, 2000). U6 is transcribed by RNA polymerase III andretained in the nucleus (Vankan et al., 1990; Terns and Dahlberg,1994; Boelens et al., 1995; Terns et al., 1995). In contrast,the other spliceosomal snRNAs are transcribed by RNA polymeraseII and are exported to the cytoplasm where the 5' cap is convertedfrom a monomethyl G (7mGpppG) to a trimethyl G (2,2,7mGpppG) andSm proteins are bound; after these events these snRNAs are reimportedback into the nucleus to function in splicing (for review, seeIzaurralde and Mattaj, 1995). The data presented herein demonstratethat U4 and U5 snRNAs, like U2 snRNA (Lange and Gerbi, 2000; Yuet al., 2001) and U6 snRNA (Lange and Gerbi, 2000), associatewith nucleoli. These conclusions are based on the nucleolar localizationof injected synthetic T7 polymerase U4 and U5 snRNA transcriptswith a monomethyl G cap like their newly synthesized in vivo counterparts.Previous studies showed that such transcripts microinjected intoXenopus oocytes exhibit normal nucleo/cytoplasmic traffic as theirendogenous counterparts (Fischer et al., 1991). In addition, functionalityof the synthetic RNAs was shown by the specificity of their nucleolarlocalization and also confirmed by the ability of U5 (our unpublisheddata) and U4 snRNA to associate with Sm proteins and, moreover,by the capacity of U4 to form the [U4/U6] snRNP via basepairing.

Injection of synthetic transcripts allows the visualization of RNA that transiently passes through the nucleolus. In contrast,detection by in situ hybridization of endogenous RNA can onlydetect steady state levels, which for U4 and U5 are weak at backgroundlevels for nucleoli in contrast to snurposomes (Gall et al., 1999).Injection of synthetic transcripts also allows a kinetic analysisof nucleolar localization, which showed that U4 snRNA labelingwas reduced and U5 snRNA signals were close to background 24 hafter incubation. This observation is consistent with the predictedtransient nature of snRNA localization to nucleoli, as has beenalready shown for U6 snRNA in the same system (Lange and Gerbi,2000).

Furthermore, the kinetic analysis in the present study suggests that nucleolar localization of U4 snRNA and U5 snRNA can occurearly during their maturation and before export to the cytoplasm.It seems that nuclear import after microinjection of various snRNAs,including U4 and U5 snRNA, into Xenopus oocytes is a time-limitingfactor and consumes several hours (Fischer et al., 1991), whereasefficient nuclear export occurs within 2 h (Terns and Goldfarb,1998, and references therein). Even when U5 snRNA was equippedwith a mature trimethyl G cap instead of a monomethyl G cap, efficientnuclear import still required 4 h of incubation (Fischer et al.,1991). In the present study, nucleolar localization of injectedU4 and U5 snRNA with a monomethyl G cap (same as after synthesisin vivo), however, took place within 8 min after nuclear injection.Thus, it is unlikely that the snRNAs traveled to the cytoplasmand were reimported into the nucleus within that short time frame.It is probable that the injected snRNAs localized to nucleolibefore export to thecytoplasm.

Because U4 and U5 snRNAs localize to nucleoli similar to U6 snRNA (Lange and Gerbi, 2000), it was possible that U6 snRNA mightpassively be carried to the nucleolus as part of the [U4/U6] di-snRNPor [U4/U6.U5] tri-snRNP. The present study rules out this possibility.First, we have shown herein that deletions of the proposed [U4/U6]interaction domain as well as the sequences flanking the interactiondomain, which are essential for [U4/U6] snRNP assembly (Vankanet al., 1990), do not affect nucleolar localization. Second, the3' end of U6 is identified herein as the NoLE; it is not onlyessential but also sufficient for nucleolar localization and canbe targeted to nucleoli by itself. The U6 3' end alone, however,is unable to assemble into a [U4/U6.U5] tri-snRNP (Vankan et al.,1990, 1992). In contrast, the 3'-NoLE U6 mutant that does notlocalize to nucleoli is still able to assemble into a [U4/U6]snRNP (Figure 4); similarly, 3'-truncated U6 can form a tri-snRNP(Vidal et al., 1999).

Although [U4/U6] snRNP formation is one prerequisite for splicing, recent studies have shown that regions of U6 essentialfor splicing exceed those essential for [U4/U6] snRNP assembly(Vankan et al., 1990) and cover most of the molecule, includingits middle part and 3' terminus. An important conclusion of thepresent study is that the 3' sequence of U6, while equally importantfor further function in splicing, enjoys a role as a NoLE fundamentallydistinct from internal sequences in U6 that are used for [U4/U6]snRNP formation. Similarly, functionally important regions ofbox C/D snoRNAs involved in pre-rRNA processing are distinct fromthe box C/D NoLEs needed for nucleolar targeting of these RNAs(Lange et al., 1998a,b,c). Thus, formation of a [U4/U6] snRNPis not a qualifying event for nucleolar localization because U6snRNA seems fully capable of localizing to nucleoli independentof an association with U4 snRNA. Nevertheless, this capacity mightbe retained when U6 is part of the di-snRNP or tri-snRNP.

Alternatively, it could be hypothesized that nucleolar localization of U6 snRNA requires association with the snoRNAs guidingits modification; they might anchor U6 snRNA in the nucleolus.Just as in the scenario discussed above, U6 snRNA would passivelylocalize in nucleoli due to interactions with other moleculesthat themselves contained the NoLEs. We have ruled out this possibilitybecause the U6 3' construct of nt 87-107 (3' end) by itself canlocalize to nucleoli, although it does not include any of thesites to be methylated or pseudouridylated. Thus, the interactionof guide snoRNAs with regions to be modified in U6 snRNA cannotbe essential for nucleolar localization ofU6.

In line with previous reports (Carmo-Fonseca et al., 1992; Matera and Ward, 1993; Bauer et al., 1994), we have also shownhere that U6 snRNA localizes to Cajal bodies. The relationshipbetween Cajal bodies and nucleoli is not yet fully understood.However, data from yeast suggest that box C/D snoRNAs pass throughCajal bodies when trafficking to nucleoli (Verheggen et al., 2001).Moreover, it has been reported that disruption of the snoRNA C/Dmotif seemed to block transfer from Cajal bodies to nucleoli (Narayananet al., 1999a). Those results suggest that the sequence essentialfor nucleolar localization of box C/D snoRNAs is not involvedin localization to Cajal bodies. To date, only one sequence essentialfor RNA localization to Cajal bodies has been identified, namely,the Sm site in U7 (Wu et al., 1996), an snRNA that is not foundin nucleoli. The present study shows that U6 snRNA after mutationof the 3' NoLE loses its ability to localize to both nucleoliand Cajal bodies, suggesting that this sequence may be both aCajal body localization element (CaBLE) and aNoLE.

It seems that the nucleolus is an organelle where specific internal posttranscriptional modifications of snRNAs (2'-O-methylationand $psi$ ) may be carried out by snoRNAs. Three box C/D snoRNAs havealready been identified as guide RNAs for the 2'-O-methylationof U6, and other results suggest that factors needed to form 2'-O-methylationand $psi$ of U6 snRNA function in the nucleolus (Tycowski et al.,1998; Ganot et al., 1999). In addition, correlative evidence suggeststhat U2 snRNA modifications occur in the nucleolus rather thanthe Cajal bodies (Yu et al., 2001). Because the 3' end of U6 snRNAis required for localization to both nucleoli and Cajal bodies,it cannot be discerned whether snRNA modification occurs in justone or both of theseorganelles.

Candidate Proteins That May Interact with the 3' NoLE of U6 snRNA

NoLEs of snoRNAs are recognized by proteins that might transport the snoRNA from the nucleoplasm to the nucleolus and/or anchorit within the nucleolus. Recent evidence supports this idea, becauseall four proteins associated with the box C/D motif are neededfor efficient nucleolar localization of U14 snoRNA (Verheggenet al., 2001). Yeast box C/D snoRNAs interact with Srp40p in theCajal body and then seem to be delivered by Nsr1p to the nucleolus(Verheggen et al., 2001).

Similarly, the nucleolar localization of U6 might be mediated by proteins that assemble on its NoLE before engagement in adi- or tri-snRNP. Although, several proteins make direct contactwith U6 snRNA during conversion from free U6 to the tri-snRNP(Vidal et al., 1999), only the La protein and the Lsm proteincomplex bind to the 3' end of U6 snRNA (see INTRODUCTION), whichis the NoLE essential for U6 nucleolar localization as shown inthe present report. La is the first protein to associate withU6 snRNA upon transcription (Rinke and Steitz, 1985; Kunkel etal., 1986), and it also has been shown that deletion of the 8nt at the U6 3' end decreases the interaction of U6 with the Laprotein (Boelens et al., 1995) and significantly reduces nucleolarlocalization ( $Delta$ 100-107; this study). Although La is found predominantlyin nuclear speckles (Bachmann et al., 1989), it might transientlyand/or in low amounts appear in nucleoli where it has been observed(Deng and Tan, 1985; Graus et al., 1985). Various RNA polymeraseIII transcripts, which require binding of La to their precursorsto guarantee a normal pathway of maturation (Yoo and Wolin, 1997),are found in nucleoli (Maraia, 2001), including pre-tRNAs (Bertrandet al., 1998) and U6 (Lange and Gerbi, 2000). All these observationssuggest that La could be involved in nucleolar localization ofRNAs. It has even been proposed that La is needed to stabilizesome RNA polymerase II transcripts like U4 (Xue et al., 2000),shown here to localize to nucleoli and also binds U3 snoRNA (Kufelet al., 2000). Intriguing although the idea may be, in the presentreport we have ruled out a role of La for U6 snRNA nucleolar localization.We show herein that U6 snRNA that lacks a 3'-hydroxyl group andtherefore cannot associate with the La protein localizes efficientlyto nucleoli nonetheless. Therefore, we conclude that it is notLa but instead is another factor that mediates nucleolar localizationby binding to the 3' NoLE of U6. Similarly, it seems unlikelythat La mediates nucleolar localization of certain other RNA polymeraseIII transcripts (e.g., SRP RNA, RNase P RNA; for review, see Maraia,2001).

In the in vivo situation, during the maturation of U6 snRNA, La is replaced with the Sm-like protein complex Lsm2-8, whichis a likely candidate to play an important role in nucleolar localizationof U6 snRNA. Interestingly, Lsm proteins also associate with pre-RNaseP RNA (Salgado-Garrido et al., 1999), which is found in nucleoli(Jacobson et al., 1997; Bertrand et al., 1998; Jarrous et al.,1999). The Lsm complex binds to the 3' end of U6 snRNA with a3'-hydroxyl end and to mature U6 snRNA (Achsel et al., 1999) whose3' end is a 2',3'-cyclic phosphate (Lund and Dahlberg, 1992; Ternset al., 1992). Similarly, we found that U6 snRNA with either a3' hydroxyl or a 3' phosphate end localized to nucleoli. Moreover,no other part than the U6 3' end associates with the Lsm proteinsstably enough to be coprecipitated with an anti-Lsm4 antibodies(Achsel et al., 1999; Stevens and Abelson, 1999). Our findingthat the 3' end of U6 is the NoLE is consistent with the hypothesisthat the Lsm complex might mediate U6 nucleolar localization.Although the five uridine residues at the extreme 3' end are requiredfor Lsm binding (Achsel et al., 1999), they are not sufficient.Similarly, we found that U6 mutants with deletion of areas withinnt 82-107 showed weak although greatly diminished nucleolar localization,suggesting that the NoLE cannot besubdivided.

Another protein, Prp24, interacts with Lsm proteins and binds to U6 snRNA, promoting formation of the [U4/U6] di-snRNP (Ghettiet al., 1995; Jandrositz and Guthrie, 1995; Raghunathan and Guthrie,1998a; Vidal et al., 1999; Fromont-Racine et al., 2000), but itcannot play an independent role in nucleolar localization of U6because it binds to U6 at positions 39-56 and 64-76 (Ghetti etal., 1995) that are not NoLEs as we have demonstratedhere.

Nucleolar localization of U6 snRNA via the 3' NoLE might occur after U6 engagement in a di- or tri-snRNP. However, in themore likely scenario, nucleolar localization is initiated fornoncomplexed U6 before formation of the di- or tri-snRNP, becausewe have shown herein that association with U4 snRNA is not a prerequisitefor localization. Therefore, the present report suggests the nucleolarentry of U6 snRNA at a point during its life cycle when Lsm proteinsreplace La in binding to the NoLE of U6 and before associationof U6 with U4 in the di-snRNP.

	ACKNOWLEDGMENTS

This article is dedicated to Willmar W. Lange. We thank J.G. Gall, S.G. Clarkson, and G.J.M. Pruijn for providing antibodies;I.W. Mattaj for the clones of U2 snRNA, U4 snRNA, and U5 snRNA;and J.A. Steitz for the clone of U6 snRNA. This research was supportedby Grant MCB 0091166 from the National Science Foundation (toT.S.L.).

	FOOTNOTES

^* Corresponding author. E-mail address: thilo_lange{at}brown.edu.

DOI: 10.1091/mbc.01-12-0596.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Achsel, T., Brahms, H., Kastner, B., Bachi, A., Wilm, M., and Lührmann, R. (1999). A doughnut-shaped heteromer of human Sm-like proteins binds to the 3'-end of U6 snRNA, thereby facilitating U4/U6 duplex formation in vitro. EMBO J. 18, 5789-5802[CrossRef][Medline].
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