Stem-Loop Binding Protein Facilitates 3'-End Formation by Stabilizing U7 snRNP Binding to Histone Pre-mRNA

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Molecular and Cellular Biology, May 1999, p. 3561-3570, Vol. 19, No. 5
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Stem-Loop Binding Protein Facilitates 3'-End Formation by Stabilizing U7 snRNP Binding to Histone Pre-mRNA

Zbigniew Dominski,¹^,² Lian-Xing Zheng,¹ Ricardo Sanchez,¹^,² and William F. Marzluff¹^,²^,^*

Department of Biochemistry and Biophysics¹ and Program in Molecular Biology and Biotechnology,² University of North Carolina, Chapel Hill, North Carolina 27599

Received 21 December 1998/Returned for modification 5 February 1999/Accepted 18 February 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The 3' end of histone mRNA is formed by an endonucleolytic cleavage of the primary transcript after a conserved stem-loopsequence. The cleavage reaction requires at least two trans-actingfactors: the stem-loop binding protein (SLBP), which binds thestem-loop sequence, and the U7 snRNP that interacts with a sequencedownstream from the cleavage site. Removal of SLBP from a nuclearextract abolishes 3'-end processing, and the addition of recombinantSLBP restores processing activity of the depleted extract. Todetermine the regions of human SLBP necessary for 3' processing,various deletion mutants of the protein were tested for theirability to complement the SLBP-depleted extract. The entire N-terminaldomain and the majority of the C-terminal domain of human SLBPare dispensable for processing. The minimal protein that efficientlysupports cleavage of histone pre-mRNA consists of 93 amino acidscontaining the 73-amino-acid RNA-binding domain and 20 amino acidslocated immediately next to its C terminus. Replacement of these20 residues with an unrelated sequence in the context of the full-lengthSLBP reduces processing >90%. Coimmunoprecipitation experimentswith the anti-SLBP antibody demonstrated that SLBP and U7 snRNPform a stable complex only in the presence of pre-mRNA substratescontaining a properly positioned U7 snRNP binding site. One roleof SLBP is to stabilize the interaction of the histone pre-mRNAwith U7snRNP.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Unlike all other metazoan mRNAs, the mature 3' ends of the replication-dependent histone mRNAs do not have poly(A) tails butare formed instead by an endonucleolytic cleavage of primary transcripts(pre-mRNAs) downstream from a highly conserved stem-loop sequence(11). This single-step processing reaction depends on two ciselements present in histone pre-mRNAs: the stem-loop sequenceitself and a purine-rich sequence located 11 to 12 nucleotidesdownstream of the cleavage site and referred to as the histonedownstream element (HDE) (26). The mature 3' end of histonemRNA consists of a 26-nucleotide sequence including a 6-nucleotidestem and a 4-nucleotide loop (21) and is recognized by a proteintermed the stem-loop binding protein (SLBP) (29, 45) or thehairpin binding protein (HBP) (20). Following the cleavage reaction,SLBP remains associated with the 3' end of mature histone mRNAs(6, 15). SLBP probably participates in all critical eventsin histone mRNA metabolism, including nucleo-cytoplasmic transport(7, 46), translation (9, 40), and mRNA degradation (28).

The HDE interacts with the U7 small nuclear ribonucleoprotein (U7 snRNP), a low-abundance particle present in about 10⁴ copies per mammalian nucleus, ~1 to 3% of the amount of the majorspliceosomal snRNPs (5, 14, 27). The U7 snRNP containsone molecule of the 63-nucleotide U7 snRNA and both the commonSm core and the U7 snRNP-specific proteins (34, 37). Geneticsuppression experiments have revealed that binding of the U7 snRNPto the histone pre-mRNA is mediated at least in part through basepairing between the 5' end of the U7 snRNA and the HDE (2,39). The stem-loop sequence and the SLBP are absolutely requiredfor 3'-end processing in vivo (30), but neither is essentialfor processing in vitro if the HDE has sufficient complementarityto U7 snRNA (38). Cleavage of the histone pre-mRNA occurs betweenthe two cis elements in a favorable sequence context containingpredominantly adenosine and cytidine residues (8) and requiresa third factor, termed the heat-labile factor (HLF; 12). Theheat labile factor, like U7 snRNP, is indispensable for the 3'-endprocessing and has been primarily characterized by its sensitivityto a mild heat treatment. Recent studies have shown that SLBPand the U7 snRNP, and possibly other components of the histonepre-mRNA 3' processing machinery, are found colocalized in spheres,the equivalent of coiled bodies in Xenopus oocytes (1, 48).

Efficient 3'-end processing of the histone pre-mRNA depends on proper juxtaposition of the stem-loop sequence and the HDE.If the distance between the two cis-acting elements is too small(3) or too large (10, 31, 32), processing is abolished.Moving the HDE only several nucleotides 3' of its normal position,resulting in a relatively small increase in the spacing betweenthe stem-loop sequence and the HDE, leads to both a moderate inhibitionof processing and a shift of the cleavage site by a comparablenumber of nucleotides (31). Scharl and Steitz have proposedthat U7 snRNP acts as a molecular ruler, a measuring device whichplaces the cleavage site at a fixed distance from the site ofU7 snRNP binding to the histone pre-mRNA (31, 32).

SLBP from several species has recently been cloned by using the three-hybrid system (20, 45) designed for screening RNAbinding proteins in the yeast Saccharomyces cerevisiae (33).This 31-kDa protein contains a centrally located RNA binding domainwith no similarity to any known motifs that bind RNA (45). Thusfar, SLBP is the only protein component of the histone pre-mRNA3' processing machinery available in large quantities for biochemicalanalysis. Here we describe experiments aimed at understandingthe role of SLBP in the processing reaction and determining theminimal regions of the protein required for cleavage of the histonepre-mRNA. We show that a 93-amino-acid fragment retains most ofthe processing activity of SLBP. One role of SLBP is to stabilizethe interaction of the U7 snRNP with the histone pre-mRNA, therebyincreasing the efficiency of the cleavagereaction.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction of the pre-mRNA substrates. The H2a-614 pre-mRNA was generated by subcloning a 59-nucleotide fragment of the mouse histone H2a-614 gene encompassing thestem-loop structure, the cleavage site, and the HDE between theKpnI and HindIII sites of the pGEM3 vector (Promega). To facilitateconstruction of H2a derivatives, an EcoRI site was inserted betweenthe cleavage site and the HDE by alteration of two nonconservednucleotides. The H1t and HDE clones were generated by replacement of the HDE in the H2a clonewith appropriate sequences (see Fig. 5A) with double-strandedoligonucleotides which were inserted between the EcoRI and HindIIIsites. The 4G clone and the clones with mutant stem-loops wereconstructed by subcloning the appropriate double-stranded oligonucleotidesbetween the EcoRI and KpnI sites. The U7 snRNA clone was constructedby inserting a double-stranded oligonucleotide encoding the 63-nucleotidemouse U7 snRNA (35) between the EcoRI and HindIII sites of thepGEM3 vector. Clones encoding various HDEs were generated by insertingthe EcoRI-HindIII restriction fragment of H2a, H1t, or HDE constructs into EcoRI and HindIII sites of the pGEM3 vector.Clones encoding truncated versions of the SLBP were generatedby deleting appropriate regions from the human SLBP gene by usingrestriction sites previously utilized to map the RNA binding domain(see Fig. 4A) (45). To construct the SLBP/20aa clone, the BamHI-PstIfragment in human SLBP cDNA was replaced by the PCR-amplifiedfragment encoding amino acids 174 to 193 of Xenopus SLBP2 (43).

Preparation of RNA. The RNA was synthesized by either T7 or SP6 RNA polymerase with DNA templates linearized with either HindIII or EcoRI restrictionenzymes, respectively. The transcription reaction was carriedout in the absence of radioisotopes in a final volume of 150 µlaccording to a standard protocol. The RNA was subsequently gelpurified to remove pretermination products. The 5' phosphatesof the RNA were removed by treatment with the calf intestinalphosphatase (Boehringer Mannheim), and 50 ng of dephosphorylatedRNA was subsequently radiolabeled with 30 µCi of [ $gamma$ -³²P]ATP and 5 U of T4 polynucleotide kinase (New England Biolabs).The RNA was separated from the unincorporated ATP by G-50 spincolumns (Pharmacia) and used without additional purification.The in vitro processing reactions were carried out in the presenceof 86-nucleotide pre-mRNA substrates. Each substrate contained59 nucleotides encompassing all cis elements required for processingand 22 and 5 nucleotides of pGEM3 vector (Promega) on 5' and 3'RNA flanks, respectively. The U7 snRNA was detected on Northernblots by hybridization with radiolabeled RNA containing a 63-nucleotideregion complementary to the U7 snRNA and 13 and 5 nucleotidesof vector sequences on the 5' and 3' ends, respectively. ThisRNA was synthesized in the antisense orientation from the U7 snRNAconstruct in the presence of 10 µM unlabeled CTP and 50 µCi of[ $alpha$ -³²P]CTP. The remaining nucleoside triphosphates were used at a 500µM concentration. The unlabeled RNA containing the U7 snRNA sequenceused as an internal control for the Northern blots was synthesizedfrom the U7 snRNA construct in the sense orientation. The reactionwas carried out in the absence of radioisotopes in a final volumeof 150 µl, and the RNA was purified as described above. The stem-loopRNA oligonucleotides used in band shift assays and competitionexperiments were synthesized by T7 RNA polymerase with the appropriateoligonucleotide templates (24).

Nuclear extract preparation and in vitro processing. Nuclear extracts were prepared from mouse myeloma cells as described previously (6, 22). Each processing reaction wascarried out in a total volume of 10 µl containing 5 µl of thenuclear extract, 5 ng of the pre-mRNA substrate labeled at the5' end with [ $gamma$ -³²P]ATP, and 20 mM EDTA. Samples were incubated at 32°C for 60 min,and the RNA was isolated and analyzed as previously described(6, 22). Since the efficiency of in vitro processing reactionsvaried significantly, depending on the preparation of the nuclearextract and the batch of the pre-mRNA substrate, each experimentwas accompanied by appropriate controls. Whenever possible, acomplete set of experiments was carried out with the same preparationof the nuclearextract.

Expression and purification of the SLBP. Wild-type and mutant forms of the SLBP were expressed in Sf9 insect cells with the baculovirus expression system (Gibco BRL),as recommended by the manufacturer. For preparative purification,200 ml of the infected cell culture was grown for 72 h, and theSLBP was purified by chromatography on Ni-agarose, as recommended.The typical yield was 200 to 500 µg of the pureprotein.

Preparation of the SLBP-depleted extract and complementation of the in vitro processing reaction. The endogenous SLBP was removed from the nuclear extract with either the biotinylated RNA containing the stem-loop structure,as previously described (6), or anti-SLBP antibody, essentiallyas previously described (22, 45). Each preparation of thedepleted extract was tested for processing activity both aloneand in the presence of the full-length human recombinant SLBP.To complement the in vitro processing reaction, approximately20 to 50 ng of baculovirus-expressed SLBP was added to 5 µl ofthe depletedextract.

Mobility shift assay. The nuclear extract (2.5 µl; 12.5 µg of protein) or pure SLBP expressed in Sf9 insect cells (50 ng) was mixed on ice with1 ng of the 5' labeled 30-nucleotide stem-loop RNA and immediatelyapplied to 6 to 8% native polyacrylamide gels containing 1× Tris-borate-EDTAbuffer. The complexes were resolved by electrophoresis and detectedbyautoradiography.

Western blots. Proteins from nuclear extracts were separated on sodium dodecyl sulfate (SDS)-12% polyacrylamide gels and transferred to nitrocellulosefilters. The SLBP was detected with antibody against the C-terminal13 amino acids of the protein (45) by using the ECL system(Amersham).

Immunoprecipitation of processing complexes and detection of the U7 snRNA. An equivalent of 10 individual processing reaction mixtures, containing 50 ng of unlabeled RNA substrate, 50 µl of the nuclearextract, and 20 mM EDTA, was set up on ice in a total volume of100 µl and incubated for 5 min at 22°C to allow complex formation.Ten microliters of anti-SLBP antibody purified on protein A agarosewas added, and the samples were rotated at 4°C for 1.5 h and thentransferred to a new tube containing 20 µl of protein A agarosebeads. The protein A agarose beads were preincubated in a nuclearextract from sea urchin blastula nuclei (17) and washed withbuffer to reduce nonspecific binding. The samples were rotatedfor 1.5 h, and the beads were collected, rinsed twice with bufferD (20 mM HEPES-KOH [pH 7.9], 100 mM KCl, 0.5 mM dithiothreitol,0.2 mM EDTA [pH 8.0], 20% glycerol) containing 0.1% Nonidet P-40detergent, suspended in 1 ml of the same buffer, and rotated at4°C for an additional 1.5 h. The protein A agarose beads weresuspended in 100 µl of 0.3 M sodium acetate containing 10 µg ofglycogen and 0.1 ng of the in vitro-synthesized U7 snRNA, andthe mixture was extracted with phenol. The RNA was recovered byprecipitation with ethanol, resolved on an 8.5% polyacrylamide-7M urea denaturing gel, and transferred to a HyBond-N⁺ membrane (Amersham) by using the Genie electrophoretic blotter(Idea Scientific). The blot was irradiated with UV light in aStratalinker apparatus (Stratagene), preincubated in Quikhyb solution(Stratagene) for 1 h at 62°C, and then hybridized overnight atthe same temperature with antisense U7 snRNA probe (10⁵ cpm). Following several washes in 0.015 M NaCl, 0.0015 M Na₃citrate, and 0.1% SDS at 62°C, the U7 snRNA was detected byautoradiography.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Importance of high-affinity binding of SLBP in histone pre-mRNA processing. SLBP binds with high affinity to a conserved 26-nucleotide sequence immediately preceding the 3' cleavage site in nonpolyadenylatedhistone pre-mRNAs. This sequence consists of a 16-nucleotide stem-loopstructure flanked on either side by five conserved nucleotides(21). As shown by mobility shift assays and competition experiments,mutations in any region of this sequence affect its binding toSLBP (47). In vitro processing of commonly used histone pre-mRNAsubstrates, including the H2a-614 pre-mRNA, is not absolutelydependent on SLBP and the stem-loop sequence (6, 25, 38).When binding of SLBP to the H2a-614 substrate is prevented byremoving the protein from the extract or by using a high molarexcess of a 30-nucleotide competitor RNA containing the wild-typestem-loop sequence, the processing reaction still proceeds with5 to 10% efficiency (6, 45). A similar reduction in processingefficiency is achieved by reversing the sequence of the stem inthe H2a-614 pre-mRNA (RS; Fig. 1A, lane 7). The RS mutation virtuallyabolishes binding of SLBP to the stem-loop sequence as demonstratedby the inability of the mutant RNA oligonucleotide to form anydetectable complex in a mobility shift assay and to effectivelycompete with the wild-type sequence for SLBP binding (47; Fig.1C). In order to determine the importance of high-affinity bindingof SLBP to the pre-mRNA in 3'-end processing, the stem-loop sequenceof H2a pre-mRNA was altered by mutations having a less drasticeffect on SLBP binding than the RS mutation. The mutant pre-mRNAsubstrates were subsequently tested in the in vitro processingassay with a nuclear extract from mouse myeloma cells. Base substitutionsaltering the conserved base pair at the top of the stem from UAto AU, CG, or UG result in 5- to 10-fold-lower affinity of SLBPfor the stem-loop sequence (47). These mutations decreased processingefficiency from approximately 60% for the wild-type substrate(Fig. 1A, lane 1) to less than 20% (Fig. 1A, lanes 2 to 4). Amuch stronger effect on the in vitro processing was exerted bya 1-nucleotide expansion of the loop (U4C; Fig. 1A, lane 6) oralteration of the region 5' to the stem-loop (5'FL; Fig. 1A, lane5). These two mutations reduced cleavage efficiency to a levelcomparable with the RS mutation (5 to 10%). Interestingly, whilethe RNA oligonucleotide containing the RS mutation had very lowaffinity for SLBP (Fig. 1C, lanes 9 and 10), the U4C and 5'FLRNAs at high concentrations were able to compete binding of SLBPto the wild-type RNA (Fig. 1C, lanes 5 to 8). Binding of the wild-typesequence to SLBP was reduced at least 90% with a 100-fold excessof these RNAs and abolished with a 500-fold molar excess of theseRNAs (Fig. 1C, lanes 5 and 8, respectively). The RS mutant RNAwas inactive even at a 1,000-fold excess (Fig. 1C, lane 11) (47),while the wild-type competitor completely abolished binding ofradiolabeled probe to SLBP at an excess of 20-fold (data not shown)and greater (Fig. 1C, lanes 3 and 4) (6, 47). These resultsindicate that high affinity of SLBP for the histone pre-mRNA substrateis required to effectively support 3' processing in vitro as itdoes in vivo (30).

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FIG. 1. Effect of altering the affinity of the pre-mRNA for SLBP. (A) Each of the six mutant stem-loops shown was introduced into the mouse histone H2a-614 pre-mRNA. The radiolabeled synthetic pre-mRNAs were incubated for 30 min in a nuclear extract prepared from mouse myeloma cells, as described in Materials and Methods. The RNA was purified, resolved by gel electrophoresis, and detected by autoradiography. The input pre-mRNA (top band) and the shorter cleavage product (bottom band) are indicated. (B) Sequence of 26 nucleotides encompassing the stem-loop structure in the various mutants. (C) Thirty-nucleotide RNAs were synthesized by T7 RNA polymerase with the appropriate oligonucleotide templates. Each RNA consists of 26 nucleotides encompassing the stem-loop structure shown and the GCCC sequence at the 5' end facilitating synthesis of RNA by T7 polymerase. The 30-nucleotide RNA containing the wild-type stem-loop structure was labeled at the 5' end with [ $gamma$ -³²P]ATP and used to detect SLBP in the nuclear extract (NE) by using a mobility shift assay. The samples were analyzed on a 7% polyacrylamide gel under nondenaturing conditions. Unlabeled 30-nucleotide RNA competitors containing the wild-type or mutant stem-loop sequences were added to the reaction at a molar excess, as indicated above each lane. Lanes 2 and 9, no competitor added; lane 1, probe.

Construction of a processing substrate absolutely dependent on SLBP. The requirement for SLBP in the processing reaction varies among different substrates and depends on the extent of complementaritybetween the U7 snRNA and the HDE (38). Substrates containingvery strong HDEs, e.g., the mouse H4-12 pre-mRNA, are actuallycleaved with normal efficiency in some nuclear extracts in whichSLBP is sequestered by the wild-type stem-loop RNA oligonucleotide(38). Under the same conditions, the cleavage efficiency ofthe H2a-614 pre-mRNA containing a weaker HDE declines to 5 to10% of the control level (6) (Fig. 2). Based on these observationsit has been proposed that SLBP functions in processing by stabilizingthe interaction of the U7 snRNP with the HDE in the histone pre-mRNA(38).

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FIG. 2. Comparison of H2a-614 and H1t pre-mRNAs as processing substrates. (A) The sequences of the H2a and H1t pre-mRNAs encompassing the stem-loop and HDE are shown. The sequence of the 5' end of the U7 snRNA and its potential to form base pairs with the HDE are depicted below each pre-mRNA substrate. Watson-Crick base pairs are indicated by vertical lines, and GU base pairs are indicated by dots. (B) The 86-nucleotide H2a-614 pre-mRNA substrate was incubated in a nuclear extract (NE) for 60 min under processing conditions (lane 1). RNA oligonucleotides containing the sequence of either the mutant HDE (HDE) (see Fig. 5A), the H2a-614 HDE, or the H1t HDE were added to the reaction samples at a 100-fold molar excess relative to the substrate (lanes 2, 3, and 4, respectively). The RNA was purified, resolved by gel electrophoresis, and detected by autoradiography. (C) The in vitro processing reaction was carried out with either the H2a-614 (top panel) or H1t (bottom panel) pre-mRNAs under standard conditions (lane 1) or in the presence of a 100-fold molar excess of the competing 30-nucleotide RNAs shown in Fig. 1B, as indicated above each lane (lanes 2 to 5).

Since the presence of SLBP-independent processing will obscure understanding of the role played by SLBP in the cleavage reaction,we constructed a substrate fully dependent on SLBP. Histone pre-mRNAencoded by the histone H1 gene specifically expressed in testis(H1t) is unique among natural processing substrates in that itsHDE substantially departs from the consensus sequence and displaysonly limited complementarity to the U7 snRNA (44) (Fig. 2A).The HDE in the histone H2a-614 pre-mRNA can form a nearly perfectduplex with U7 snRNA, consisting of 14 bp (including 2 GU pairs),interrupted by only one mismatch. The HDE in the H1t pre-mRNAcan form only 11 bp separated by several noncomplementary nucleotides(Fig. 2A). Moreover, the H1t HDE has relatively weak complementarityto the CUCUUU sequence (nucleotides 12 to 17 of the U7 snRNA)which base pairs with the core of the HDE in the somatic histonepre-mRNAs (2) and instead has the potential to base pair withthe extreme 5' end of the U7 snRNA. Additional base pairs withthe pre-mRNA substrate and this region of the U7 snRNP have beenreported previously for other histone pre-mRNAs (36). We reasonedthat both the decreased number and more sparse distribution ofbase pairs formed between the H1t pre-mRNA and the U7 snRNA shouldresult in a relatively weak interaction between the two RNAs.To demonstrate that the H1t HDE has a lower affinity for the U7snRNP than the H2a-614 HDE, we synthesized RNA competitors containingeither the H2a-614 or H1t HDE. Each RNA competitor was added tothe in vitro processing reaction at a 100-fold molar excess overthe H2a-614 pre-mRNA substrate and tested for its ability to affectefficiency of the cleavage. About 90% of the H2a-614 pre-mRNAwas processed in the absence of any RNA competitor (Fig. 2B, lane1). The cleavage reaction proceeded with similar efficiency inthe presence of a 100-fold molar excess of a control RNA competitorwith no complementarity to the U7 snRNA (Fig. 2B, lane 2). CompetitorRNA containing the H2a-614 HDE virtually abolished processing(>95% reduction of the initial efficiency; Fig. 2B, lane 3), presumablyby binding to the 5' end of the U7 snRNA and inactivating theU7 snRNP in the nuclear extract. The RNA oligonucleotide containingthe H1t HDE at the same concentration had no effect (Fig. 2B,lane 4). These results show that the extent of base pairing betweenthe H1t HDE and the 5' end of the U7 snRNA is not sufficient toallow stable binding of the U7 snRNP to this competitorRNA.

The 86-nucleotide histone H1t pre-mRNA substrate was constructed by substituting the HDE in the histone H2a-614 pre-mRNA withthe corresponding element from the H1t pre-mRNA. The H1t pre-mRNAwas processed in vitro at least 50% as efficiently as the H2a-614substrate. To compare the dependence of processing of the H1tpre-mRNA on SLBP, we carried out the reaction in the presenceof competitor RNA capable of titrating out SLBP from the nuclearextract. A 100-fold molar excess of 30-nucleotide RNA containingthe wild-type stem-loop structure prevents binding of SLBP tothe pre-mRNA substrate and causes substantial reduction, but notcomplete inhibition, of the processing of the H2a-614 pre-mRNA(6) (Fig. 2C, top panel, lane 2). Processing of the histoneH1t pre-mRNA substrate is abolished under the same conditions(Fig. 2C, bottom panel, lane 2). Complete dependence of H1t pre-mRNAprocessing on SLBP was further confirmed by using RNA competitorsthat have lower affinity for SLBP due to either a uridine insertionin the loop (SL^U4C, Fig. 1B) or placing a UUUG sequence 5' to the stem-loop (5'FL; Fig. 1B). Each competitor at a 100-fold molar excess almostcompletely inhibited cleavage of the H1t pre-mRNA (Fig. 2C, bottompanel, lanes 4 and 5) but had only a moderate effect on processingof the H2a substrate (Fig. 2C, top panel, lanes 4 and 5). At thesame concentrations, these competitors reduced binding of SLBPto the wild-type stem-loop probe more than 95% as determined bythe mobility shift assay (Fig. 1C). Addition of the RS RNA competitor,which has the stem sequence reversed (Fig. 1B) and at least a100-fold-lower affinity for SLBP (47), did not affect processingof either substrate (Fig. 2C, lane 3, both panels). The differentialeffect of the U4C and 5'FL oligonucleotides on processing of thetwo substrates is discussed below (see Discussion). We concludethat SLBP is an essential and indispensable trans-acting factorin the in vitro 3'-end processing of the H1t pre-mRNA. This substratewas used in the majority of the subsequentexperiments.

Complementation of the SLBP-depleted extract with recombinant baculovirus SLBP. We have previously shown that depleting the SLBP from the nuclear extract with anti-SLBP antibody has an effect similar tothat caused by the addition of an excess of the stem-loop RNAto the reaction and results in a substantial decrease in the processingof the histone H2a-614 pre-mRNA (45). To definitively show thatremoval of SLBP is solely responsible for the reduced efficiencyof the reaction, we developed a complementation assay in whichthe depleted extract was supplemented with recombinant SLBP. Boththe H2a-614 and the H1t pre-mRNAs were used as substrates to assessprocessing activity of the reconstituted nuclear extract. Withan antibody to the 13 C-terminal amino acids of SLBP (45), morethan 95% of SLBP was removed from the extract, as determined bothby mobility shift assay (Fig. 3A, lane 5) and by Western blotting(Fig. 3D, lane 3). Depletion of SLBP resulted in a decrease inprocessing efficiency of the histone H2a pre-mRNA substrate fromapproximately 90 to about 10% (Fig. 3B, top panel, lane 4) andcompletely abolished processing of the H1t substrate (Fig. 3B,bottom panel, lane 4). An identical reduction in processing efficiencywas caused by sequestering SLBP by addition of an excess of wild-typeSL RNA competitor (Fig. 3B, lane 2). Mock depletion carried outwith preimmune serum caused irreversible loss of some (about 25%)of the processing activity (Fig. 3B, lane 3) but did not significantlyaffect the amount of SLBP, as demonstrated by the mobility shiftassay (Fig. 3A, lane 4). This loss of activity is most likelya result of prolonged incubation at 4°C or of nonspecific adsorptionof processing factors to the protein A beads.

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FIG. 3. Depletion of SLBP from the nuclear extract and complementation with recombinant SLBP. (A) The 30-nucleotide radiolabeled wild-type stem-loop RNA (lane 1) was incubated in a nuclear extract (NE), and the complex was resolved by gel electrophoresis (lane 2). Lane 3, nuclear extract plus a 100-fold excess of unlabeled competitor 30-nucleotide stem-loop RNA; lane 4, extract treated with preimmune serum (mock depletion); lane 5, extract depleted with anti-SLBP antibody; lane 6, anti-SLBP-depleted extract supplemented with 50 ng of recombinant human SLBP. (B) The same extracts as those in panel A were used in processing reactions with the histone H2a-614 pre-mRNA (top panel) or the H1t pre-mRNA substrates (bottom panel). The RNAs were purified, resolved by electrophoresis in a denaturing polyacrylamide gel (8%; 7 M urea), and detected by autoradiography. Processing in the nuclear extract (NE) under standard conditions and in the presence of a 100-fold excess of 30-nucleotide competitor RNA with wild-type stem-loop sequence is shown in lanes 1 and 2, respectively. Lane 3, mock-depleted extract (preimmune serum); lane 4, extract depleted with anti-SLBP antibody; lane 5, anti-SLBP-depleted extract plus recombinant human SLBP. (C) Processing of the histone H2a-614 pre-mRNA (top panel) or the H1t pre-mRNA (bottom panel) in the nuclear extract depleted of SLBP with biotinylated RNA oligonucleotide containing the wild-type stem-loop. Lane 1, mock-depleted extract (nonspecific biotinylated oligonucleotide); lane 2, extract depleted with biotinylated stem-loop RNA; lane 3, depleted extract complemented with 50 ng of recombinant human SLBP. (D) Equal amounts (50 µg of protein) of the nuclear extracts (NE) used in panels B and C were resolved by electrophoresis on a 12% polyacrylamide-SDS gel, and SLBP was detected by Western blotting. The top band represents the intact 45-kDa SLBP, and the bottom band is a proteolytic cleavage product lacking part of the N terminus of the protein.

Recombinant human SLBP containing a histidine tag at the N terminus was expressed in Sf9 insect cells by using the baculovirussystem and purified by Ni affinity chromatography. Complementationof the SLBP-depleted extract with the exogenous protein restoredboth SLBP binding activity (Fig. 3A, lane 6) and processing ofthe H2a-614 and H1t pre-mRNA substrates (Fig. 3B, lane 5, bothpanels). Addition of the SLBP to a complete extract resulted onlyin a slight stimulation of processing, suggesting that SLBP isnot the limiting component of the processing extract (data notshown).

SLBP was also removed from the nuclear extract via binding to a biotinylated 30-nucleotide RNA containing the wild-type stem-loopsequence followed by adsorption of RNA-protein complexes to streptavidinbeads (6, 20). Unlike immunodepletion, RNA-mediated depletionmay result in removal of factors other than SLBP that bind tothe stem-loop sequence. On the other hand, this approach wouldnot lead to removal of inactive SLBP molecules unable to bindRNA. This procedure was equally effective in depleting SLBP fromthe nuclear extract, as assayed by mobility shift (6) and Westernblotting (Fig. 3D, lane 5) and resulted in the same reductionof processing efficiency as immunodepletion (Fig. 3C, lane 2,both panels). Processing of both the H2a and the H1t pre-mRNAsubstrates was restored to the initial level by addition of therecombinant human SLBP to the depleted extract (Fig. 3C, lane5). This result demonstrates that no other essential processingfactors are quantitatively bound to the SLBP-RNA complex and removedfrom the extract during RNA-mediated SLBPdepletion.

Mapping of the regions of SLBP involved in histone pre-mRNA processing. In order to determine which regions of human SLBP participate in processing of the histone pre-mRNA, truncated versions ofSLBP were expressed in the baculovirus system and tested for theirability to complement immunodepleted nuclear extract. All deletionswere made outside the central region of SLBP encompassing theRNA binding domain (Fig. 4A). As determined by mobility shiftassays, all the mutant proteins bound the stem-loop RNA (datanot shown) (45). Complementation experiments were carried outin the immunodepleted nuclear extract by using the H1t pre-mRNAas a processing substrate. Due to a small amount of SLBP leftin this depleted extract, processing of the H1t substrate wasnot completely abolished but proceeded with about 5% efficiency(Fig. 4B, lane 2).

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FIG. 4. Regions of human SLBP required for histone pre-mRNA processing. (A) The restriction map of the human SLBP cDNA with the boundaries of the three regions of the protein corresponding to the N-terminal domain (N-ter), the RNA binding domain (RBD), and the C-terminal domain (C-ter) is outlined at the top. The constructs are named according to the number of amino acids deleted from the N or C terminus. The hSLBP/20aa has the 20 amino acids immediately after the RNA binding domain (196 to 215) changed to the 20 amino acids present at this position in frog XSLBP2, an SLBP which does not function in pre-mRNA processing (43). The ability of the mutant SLBP to restore processing in the SLBP-depleted extract is summarized to the right of each construct. (B) The nuclear extract (lane 1) was depleted of SLBP with anti-SLBP antibody and was assayed for the ability to cleave the H1t pre-mRNA when complemented with 50 ng of the indicated mutant human SLBP. Depletion of the extract resulted in an almost complete loss of processing activity (lane 2) which was fully restored when the depleted extract was supplemented with the full-length human SLBP (lane 3). Complementation of the depleted extract with the mutant proteins is shown in lanes 4 to 8. (C) Processing activity of the nuclear extract (NE; differing from that in Fig. 1B) before and after immunodepletion is shown in lanes 1 and 2, respectively. Fifty nanograms of human SLBP (lane 3) or mutant proteins was added to the depleted extract, as indicated (lanes 4 to 6). (D) The recombinant proteins were tested for their ability to bind to the stem-loop RNA oligonucleotide. Fifty nanograms of the recombinant protein indicated at the top of each lane was incubated with the radiolabeled stem-loop RNA, and the complexes were resolved by native gel electrophoresis.

The baculovirus-expressed deletion proteins $Delta$ 13C, $Delta$ 68N- $Delta$ 13C, and $Delta$ 124N- $Delta$ 13C restored activity of the depleted extract to controllevels (Fig. 4B, lanes 4, 6, and 7, respectively), indicatingthat the last 13 amino acids of the protein and the entire 124amino acids of the N-terminal domain are not necessary for processing.The $Delta$ 52C mutant protein, which contains only 20 amino acids afterthe RNA binding domain, restored processing activity to 40% ofthe control level (Fig. 4B, lane 5). Since deletion of the 13C-terminal amino acids did not affect the activity of SLBP, weconclude that the remaining 39 amino acids (amino acids 218 to256) play a role in enhancing the processing efficiency. A recombinantfragment of SLBP containing only the RNA binding domain did nothave any activity in processing (Fig. 4B, lane 8; Fig. 4C, lane5), although it bound the stem-loop RNA with high affinity (Fig.4D, lane5).

Deletion mutagenesis suggested that a 93-amino-acid fragment of SLBP, containing only the RNA binding domain and subsequent20 amino acids, has processing activity. This protein (hSLBP/min)was expressed in baculovirus and tested for its ability to complementthe immunodepleted extract. The hSLBP/min restored processingto 40% of the control level (Fig. 4C, lane 4), similar to theactivity of the $Delta$ 52C deletion protein (Fig. 4B, lane 5). To definitivelyconfirm the importance of the 20 amino acids after the RNA bindingdomain, we replaced this region in the intact SLBP with an unrelatedsequence. We used the sequence found adjacent to the RNA bindingdomain of the Xenopus SLBP2, a protein that does not functionin histone pre-mRNA processing (43). This protein, hSLBP/20aa,bound strongly to the stem-loop (Fig. 4D, lane 3) but retainedonly slight activity in stimulating the cleavage reaction (<5%;Fig. 4C, lane 6). Thus, in vitro processing requires only high-affinitybinding of the SLBP to the RNA target via its RNA binding domainand the 20 amino acids adjacent to the C terminus of thisdomain.

Coprecipitation of the U7 snRNP with SLBP and histone pre-mRNA. To initiate studies on the function of SLBP in the processing reaction, we used the anti-SLBP antibody to isolate any complexesthat might form on the histone pre-mRNA. Since time course experimentsindicate that histone pre-mRNA processing proceeds without a significanttime lag (6, 11, 27), reactions containing an unlabeledpre-mRNA substrate and nuclear extract were briefly (5 min) incubatedat 22°C (below the optimum 32°C) to allow complex formation andimmediately cooled on ice. As determined by using radiolabeledsubstrate, incubation under these conditions resulted in bindingof more than 95% of the pre-mRNA to SLBP and yielded less than2% of the cleavage product (data not shown). Anti-SLBP antibodywas then added to the reactions, and complexes were isolated bybinding to protein A-agarose. RNA was recovered from the immunoprecipitates,and the U7 snRNA was detected by Northern analysis. More than95% of the substrate RNA was recovered in the immunoprecipitates(data not shown), since SLBP is present in excess over the substratein these reactions. An internal standard RNA containing the U7snRNA sequence was added to each sample prior to phenol extractionto control for the efficiency of RNA isolation andhybridization.

Only a small amount of the U7 snRNA bound nonspecifically to the protein A-agarose in the absence of the pre-mRNA substrate(Fig. 5C, lane 1). After addition of unlabeled H2a pre-mRNA largeamounts of U7 snRNP coimmunoprecipitated with SLBP (Fig. 5C, lane2). Precipitation of the U7 snRNP was specific, since it was completelyabolished by sequestering the antibody with the antigenic peptide(Fig. 5C, lane 3). Coimmunoprecipitation of the U7 snRNP in thepresence of H2a pre-mRNA was also abolished by addition of a 2'-O-methyloligoribonucleotide complementary to the first 19 nucleotidesof the U7 snRNA (Fig. 5C, lane 5) and was not affected by a largeexcess of a nonspecific 2'-O-methyl oligoribonucleotide (Fig.5C, lane 4). The anti-U7 2'-O-methyl oligoribonucleotide has beenpreviously shown to completely inhibit the cleavage reaction bymasking the 5' end of the U7 snRNA and preventing the U7 snRNPfrom base pairing with the HDE (4, 6, 31). This resultdemonstrates that stable binding of the U7 snRNP to the substraterequires base pairing between the 5' end of the U7 snRNA and thepre-mRNA substrate. Consistently, the HDE mutant substrate, whichcannot base pair with the U7 snRNA (Fig. 5A), is inactive in processing(Fig. 5B, lane 2) and is not able to form a stable complex withthe U7 snRNP (Fig. 5C, lane 9). No U7 snRNA was recovered whenthe H2a/RS substrate containing the reversed stem sequence wasused (Fig. 5C, lane 10). This mutation virtually abolishes bindingof SLBP to the histone pre-mRNA and prevents immunoprecipitationof the substrate by anti-SLBP antibody. Finally, coimmunoprecipitationof the U7 snRNP was completely blocked by the addition of excessstem-loop RNA oligonucleotide which sequestered all free SLBPand prevented binding of SLBP to the pre-mRNA substrate (Fig.5C, lane 6). This result demonstrates that the SLBP-stem-loopRNA complex formed under these conditions does not stably associatewith the U7 snRNP and confirms that stable interaction betweenthe two factors requires that both cis-acting elements be presenton the same pre-mRNA molecule.

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FIG. 5. Formation of a stable complex containing the SLBP and the U7 snRNP on the pre-mRNA substrate. (A) Sequences of the substrates used for assaying U7 snRNP binding. The sequence of the parental H2a pre-mRNA comprising the stem-loop structure, the cleavage site represented by an arrow, and the U7 binding site are shown at the top. The nucleotides at the 5' and 3' ends of the RNA encoded in the pGEM3 vector are not included. The nucleotide substitutions introduced into the H2a pre-mRNA in order to generate the other pre-mRNA substrates are shown below the H2a sequence. The unchanged sequences are represented by solid lines. The RS mutant of the H2a-614 pre-mRNA contains reversed sequence of the stem-loop structure, as shown in Fig. 1B. (B) The H2a/4G (lane 1) and HDE (lane 2) substrates shown in panel A were incubated in a nuclear extract under standard processing conditions. The RNA was analyzed as described in the legend to Fig. 2. (C) The H2a-614 substrate (lanes 2 to 6) and the indicated mutant substrates (lanes 7 to 10) were briefly incubated in nuclear extract to allow the formation of processing complexes. The complexes were immunoprecipitated with anti-SLBP antibody, RNA prepared, resolved by electrophoresis on 8.5% polyacrylamide gel containing 7 M urea, and assayed for the presence of U7 snRNA by Northern blotting. Immunoprecipitation was carried out in the presence of the H2a-614 pre-mRNA (lanes 2 to 6) or mutant pre-mRNAs, as indicated (lanes 7 to 10). Lane 1, no substrate added; lane 3, 10 µg of antigenic peptide was added to the reaction mixture prior to addition of the antibody; lanes 4 and 5, immunoprecipitation in the presence of 0.5 µg of a nonspecific 2'-O-methyl oligoribonucleotide or 2'-O-methyl oligoribonucleotide complementary to the 5' end of U7 snRNA, respectively. Lane 6, immunoprecipitation in the presence of a 100-fold excess of the 30-nucleotide RNA containing the stem-loop sequence. Control, 0.1 ng of a synthetic 77-nucleotide RNA containing the complete sequence of the U7 snRNA added to each sample as an internal standard for RNA recovery and hybridization efficiency.

Guanosines are not found at the cleavage site of any natural histone pre-mRNAs, and substitution of guanosine for cytosineat this site greatly reduces processing (8). We constructedthe H2a/4G mutant substrate derived from the H2a pre-mRNA by replacingthe CACU sequence at the cleavage site with four guanosines (Fig.5A). The H2a/4G substrate was inactive in processing (Fig. 5B,lane 1). In spite of that, the H2a/4G pre-mRNA supported formationof stable complexes with U7 snRNP with an efficiency similar tothat of the parental H2a substrate (Fig. 5C, lane 7). Thus, stableassociation with the U7 snRNP is necessary but not sufficientfor cleavage of histone pre-mRNAs. The H1t pre-mRNA, which containsa weaker HDE than the H2a and H2a/4G pre-mRNAs, was significantlyless efficient in the formation of stable complexes with U7 snRNP.This substrate bound about 25% of the amount of U7 snRNA immunoprecipitatedwith H2a-614 pre-mRNA (Fig. 5C, lane8).

We conclude from the above results that histone pre-mRNAs support formation of a stable processing complex containing SLBPand the U7snRNP.

Function of SLBP in processing. The above immunoprecipitation experiments confirmed previous results that the U7 snRNP and the histone pre-mRNA can form astable complex dependent on base pairing between the U7 snRNAand the HDE but did not definitively show that SLBP is requiredfor this interaction. Since in our experiments isolation of theprocessing complexes is dependent on the anti-SLBP antibody, mutatingthe stem-loop structure to prevent binding of the SLBP to thepre-mRNA or removing SLBP from the extract prevents subsequentisolation of the histone pre-mRNAsubstrate.

Increasing the distance between the stem-loop structure and the HDE results in a shift of the cleavage site by a comparablenumber of nucleotides (31, 32). In addition to movement ofthe cleavage site, insertions between the stem-loop and the HDEresult in a progressive decline of processing efficiency as thedistance between the two elements increases, leading eventuallyto a complete loss of activity (31, 32). To determine whetherthe spacing between the stem-loop and the HDE was critical forstable association of U7 snRNP with the pre-mRNA, we constructedthe H2a/+4 and H2a/+12 pre-mRNA substrates by inserting 4 or 12nucleotides between the cleavage site and the HDE, respectively(Fig. 6A). The inserted sequences were compatible with known cleavagespecificity, containing highly preferred adenosine residues (8)or a duplicated cleavage site (H2a/+4 and H2a/+12 pre-mRNA, respectively;Fig. 6A). The H2a/+4 construct was processed relatively efficiently,and in agreement with the results of Scharl and Steitz (31),the cleavage site was shifted about four nucleotides downstreamof the wild-type site (Fig. 6B, lane 2). The H2a/+12 substratewas essentially inactive in processing (Fig. 6B, lane 3), althoughlonger exposures resulted in detection of minor products resultingfrom cleavage 10 to 15 nucleotides 3' of the wild-type site (datanot shown). The overall efficiency of processing at these sitesapproximately equaled the efficiency of SLBP-independent processingof the H2a-614 substrate, suggesting that large insertions betweenthe stem-loop and the HDE are functionally equivalent to mutatingthe stem-loop or depleting SLBP from the nuclear extract.

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FIG. 6. The stimulation of binding of the U7 snRNP by SLBP is distance dependent. (A) The sequence of the H2a-614 mutant substrates containing either 4- or 12-nucleotide insertions between the normal cleavage site and the HDE. (B) The radiolabeled substrates shown in panel A and indicated above each lane were incubated in nuclear extract under standard processing conditions, and RNA was analyzed as described above. (C) The anti-SLBP antibody was used to isolate processing complexes assembled on the pre-mRNA substrates, as described in Fig. 5C. Immunoprecipitation with no pre-mRNA added (lane 1) or in the presence of the substrates shown in panel A (lanes 2 to 4). (D) The anti-SLBP antibody was used to isolate processing complexes assembled on the H2a-614 substrate (lanes 2 and 3) in the control nuclear extract (NE) or in extract which had been heat inactivated at 50° for 15 min. Lane 1, no RNA was added to the control extract.

In order to determine the ability of the H2a/+4 and H2a/+12 pre-mRNAs to form stable complexes with U7 snRNP, each substratewas incubated in the nuclear extract to form processing complexesthat were subsequently immunoprecipitated by the anti-SLBP antibodyand analyzed for the presence of the U7 snRNA. The H2a/+4 pre-mRNAsupported formation of processing complexes containing the U7snRNP at least as efficiently as the control H2a pre-mRNA (Fig.6C, lanes 2 and 3, respectively), although it was less efficientlyprocessed (Fig. 6B, lane 2). Strikingly, immunoprecipitation ofprocessing complexes assembled on the H2a/+12 pre-mRNA containingthe same HDE yielded only a small amount of the U7 snRNA, about10% of the control levels but significantly higher than the backgroundlevel (Fig. 6C, lane 4). The small amount of U7 snRNP stably associatedwith the H2a/+12 pre-mRNA probably represents a complex formedindependently of SLBP. The basal level of the U7 snRNP bindingto the HDE is most likely responsible for residual processingof the H2a/+12 pre-mRNA at heterogeneous sites and less than 10%efficient processing of the H2a pre-mRNA at the normal site inthe absence of bound SLBP. We conclude that formation of a stablecomplex of U7 snRNP with the HDE is very inefficient without theassistance of SLBP bound close to the HDE. Thus, one role of theSLBP in histone pre-mRNA processing is to help recruit U7 snRNPinto a stable complex on histone pre-mRNA. SLBP-mediated stabilizationof the interaction between the U7 snRNP and the histone pre-mRNAis not dependent on the HLF. Brief treatment of a nuclear extractat 50°C results in inactivation of this essential processing factor(12), and in our hands resulted in only a 50% reduction in theamount of SLBP activity as judged by mobility shift and has noeffect on the U7 snRNP (12, 23). Although the heat-treatedextract was completely inactive in processing (data not shown),the U7 snRNP still formed a stable complex with the histone pre-mRNAwith only a slightly reduced efficiency compared to the controlextract (Fig. 6D, lanes 3 and 2, respectively). Thus, the heat-labilefactor is not essential for formation of the complex containingthe histone pre-mRNA, SLBP, and U7snRNP.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We (45) and others (20) have previously reported the cloning and preliminary analysis of the SLBP, a trans-acting factorwhich plays an important role in 3'-end processing of the replication-dependenthistone pre-mRNAs. SLBP is not similar to any other protein inthe database and contains a novel RNA binding domain. Here wehave determined the regions of SLBP required for histone pre-mRNAprocessing and a role of SLBP in the processingreaction.

A 93-amino-acid region of SLBP supports efficient in vitro processing. The processing activity of extracts depleted by either a biotinylated stem-loop or anti-SLBP was efficiently restored by additionof the full-length human SLBP expressed in Sf9 insect cells byusing the baculovirus system. The ability of purified SLBP tocomplement the depleted extract indicates that no other componentof the processing machinery is removed from the extract duringthe depletion procedure. This suggests that the HBF, which haspreviously been functionally defined as the factor which interactswith the stem-loop (41), is comprised only ofSLBP.

SLBP contains a 73-amino-acid region in the center of the protein responsible for binding to the stem-loop sequence in histonepre-mRNAs. The entire amino-terminal region of the SLBP can beremoved without affecting 3'-end histone pre-mRNA processing invitro. This 124-amino-acid region may play a role in some of theother processes in histone mRNA metabolism, such as nucleocytoplasmictransport of the histone mRNP, translation, or regulation of histonemRNA stability. The RNA binding domain alone was not sufficientto support processing, but the addition of only 20 amino acidsto the C-terminal side of the RNA binding domain restored about50% of the activity of the intact SLBP. Additional amino acidsin the C-terminal region of SLBP must contribute to the maximalactivity of the protein. Replacement of this entire 20-amino-acidregion in the context of the full-length SLBP greatly reducedprocessing without affecting its ability to bindRNA.

Processing of the H1t pre-mRNA is fully dependent on SLBP. SLBP (HBF) is required for maximal processing efficiency of all commonly used histone pre-mRNA substrates, including H2a-614,H3-614, H3-53, H4-1, and H4-12 pre-mRNAs (38). In the absenceof SLBP, processing occurs at a reduced rate. In contrast, theH1t pre-mRNA substrate is processed with efficiency similar tothat of the H2a-614 histone pre-mRNA in the complete extract butis absolutely dependent on SLBP for processing. The strength ofthe HDE is also important for high efficiency of processing invivo. For example, the H2a-614 pre-mRNA capable of forming withthe U7 snRNA 14 bp (including 2 GU bp) is expressed very efficientlyin vivo (13). Other histone pre-mRNAs that have much weakerHDEs (18, 45) are expressed at a lower level in vivo, partlydue to a decreased efficiency of 3'-end formation (18).

The U7 snRNP forms a stable complex with the histone pre-mRNA and SLBP. Processing of histone pre-mRNA involves assembly of a multifactor complex on the histone pre-mRNA, followed by cleavage ofthe histone pre-mRNA (23). Since SLBP alone can form a stablecomplex with histone pre-mRNA, the initial event in processingin vivo is likely binding of the SLBP. The immunoprecipitationexperiments with the anti-SLBP antibody allowed us to detect formationof a stable complex containing at least three components: SLBP,the pre-mRNA substrate, and the U7 snRNP. This complex was formedrapidly and was resistant to extensive washing with isotonic solutionscontaining nonionic detergents. Stable binding of the U7 snRNPto the pre-mRNA was absolutely dependent on formation of a duplexRNA between the U7 snRNA and the HDE. While these results confirmthat the HDE is a primary site of binding for the U7 snRNP, theydo not preclude existence of an independent but weaker bindingof the U7 snRNP to the stem-loop (or stem-loop-SLBP complex) inthe initial phase of the processing reaction, as suggested previouslyby a combination of RNase protection and anti-Sm-mediated immunoprecipitationexperiments (26). Such an interaction, which could involve protein-proteininteractions between SLBP and a protein in U7 snRNP, might bedisrupted by the stringent washing conditions used during ourimmunoprecipitationexperiments.

In agreement with previous observations (23), the efficiency of complex formation was dependent on the stability of theRNA duplex formed between the 5' end of the U7 snRNA and the HDE.In the immunoprecipitation experiments, about 20% of the totalU7 snRNP in the extract and 3% of the H2a-614 pre-mRNA substrateare involved in formation of stable complexes. SLBP was presentin the extract in excess of the substrate, and all of the substratewas precipitated by the anti-SLBP antibody, ruling out the possibilitythat there are substrate molecules that form a stable complexonly with U7 snRNP. The histone H1t pre-mRNA also formed a stablecomplex with SLBP and U7 snRNP, although less efficiently, despitethe fact that the H1t HDE alone could not stably interact withthe U7 snRNP (Fig. 2B). These results suggest that stable bindingof the U7 snRNP to the H1t pre-mRNA is dependent on additionalinteractions with SLBP, presumably due to protein-protein interactionswith a protein(s) in the U7snRNP.

Subsequent to formation of the complex containing the pre-mRNA, SLBP and the U7 snRNP, additional factors must be recruitedfor cleavage to occur. Since only a small fraction of the substrateand a large fraction of the U7 snRNP are present in the complex,the same U7 snRNP must function in cleavage of multiple substratesduring the 1 h in vitro reaction incubation, which normally yieldsmore than 50% of the mature product. It is not necessary for assemblyof the complex that the substrate becleavable.

Proper spacing between the stem-loop and the HDE is necessary for stable binding of U7 snRNP. A role for SLBP in stabilizing the interaction between the U7 snRNP and pre-mRNA was first suggested by the observation thatpre-mRNAs with weak HDEs are more dependent on SLBP (HBF) (38).This role of SLBP (HBF) was further supported by demonstratingthat mutations within the HDE which allowed more extensive basepairing with the U7 snRNA resulted in a reduced requirement forSLBP (38). Additional experimental support for the role of SLBPin recruiting the U7 snRNP to pre-mRNA substrates with weak HDEis provided by the immunoprecipitation experiments with the H2a/+12pre-mRNA. Insertion of 12 nucleotides between the stem-loop sequenceand the HDE virtually abolished processing, most likely by precludingproductive interaction between factors binding to both elements.The failure to process the H2a/+12 pre-mRNA was accompanied bysignificant reduction in the amount of the U7 snRNP coassembledon this substrate. These experiments provide direct biochemicalevidence that stable association of the U7 snRNP with the histonepre-mRNA is not determined solely by the sequence of the HDE butis stimulated by SLBP bound to the stem-loop sequence at the appropriatedistance from theHDE.

In a previous study with psoralen cross-linking and immunoprecipitation with antitrimethylguanosine antibodies, no differencewas observed in the ability of the U7 snRNP to bind H2a-614 mutantpre-mRNAs containing variable insertions between the stem-loopsequence and the HDE (31). These experiments were performedunder processing conditions, and indeed there was more U7 snRNPbound to the substrates that were not efficiently cleaved thanto the wild-type H2a-614 substrate (31). Our results show aclear dependence on the proper positioning of the HDE for stableU7 snRNP binding to the H2a-614 pre-mRNA (Fig. 6). This discrepancyis most likely due to efficient processing of the wild-type substrateunder the conditions used by Scharl and Steitz, which would resultin rapid dissociation of complexes containing the U7 snRNP (31).During the short time and at the lower temperature (22°C) we used,there is complex formation but virtually no cleavage. We believethis complex is on the pathway to histone pre-mRNA processing,since subsequent warming of the reaction sample results in efficientprocessing. We observed a low level of binding of the U7 snRNPto the H2a/+12 substrate, which is probably due solely to basepairing of the U7 snRNA with the HDE and occurs independentlyofSLBP.

Efficient processing requires high-affinity binding of SLBP. Stabilization of binding of the U7 snRNP to the HDE by SLBP requires that SLBP binds to the stem-loop sequence on the samepre-mRNA molecule. Substrates which lack strong SLBP binding sitesare processed less efficiently, and a reduction of 5- to 10-foldin the affinity of SLBP for the stem-loop has a large effect onprocessing efficiency, even on the efficient H2a-614 substrate,in vitro (Fig. 1) and in vivo (30). An increase in the off rateof SLBP effected by a reduction in affinity suggests that theformation and assembly of the initial stable processing complexrequires binding of SLBP to the pre-mRNA for a significant amountof time. The affinity of both SLBP and U7 snRNP for their respectivesites on the histone pre-mRNA is critical for determining therate of the in vitro processing reaction. If the U7 snRNP bindsstably to the pre-mRNA due to a high degree of complementaritybetween the HDE and the 5' end of U7 snRNA, then it can also recruitthe additional factors necessary for processing, albeit with lowerefficiency.

An initially puzzling result, that the U4C and 5'FL RNA competitors have very different effects on processing of the H2a-614pre-mRNA and the H1t mRNA, is understandable in this scenario.In the case of the H2a-614 pre-mRNA, U7 snRNP associates withthe HDE relatively stably. Binding of the small amount of freeSLBP present in the reaction mixture containing competitors issufficient to form significant amounts of a stable processingcomplex, which is resistant to the competitors. In contrast, theU7 snRNP does not associate for a significant amount of time withthe H1t pre-mRNA; rather, the formation of the processing complexis absolutely dependent on bound SLBP, which is greatly reducedin the presence of the competitors. U7 snRNP bound stably to thehistone pre-mRNA is also capable of ultimately recruiting theother factors necessary for processing in the absence of SLBP,although the formation of the stable complex is greatly enhancedby the presence of SLBP. These results are consistent with previousresults that suggested cooperative binding of SLBP and U7 snRNPto the histone pre-mRNA (25, 26, 41) and provide additionalevidence for interaction between these two trans-acting factorsin 3'-endprocessing.

Other trans-acting factors involved in histone pre-mRNA processing. The immunoprecipitation experiments with anti-SLBP antibody revealed that formation of stable processing complexes containingthe histone pre-mRNA and the U7 snRNP is not dependent on theHLF, the third known trans-acting processing factor (12). Howmany other components are necessary for 3'-end processing of thehistone pre-mRNAs? A large number of polypeptides are requiredfor cleavage of the other pre-mRNAs prior to polyadenylation,although no snRNA is required in this reaction (16, 19, 42).The coimmunoprecipitation procedure with anti-SLBP and a nuclearextract labeled with [³⁵S]methionine may allow detection of other factors coassembledwith U7 snRNP on the histone pre-mRNA. These experiments are inprogress.

	ACKNOWLEDGMENTS

This work was supported by a grant from the NIH (GM29832) to W.F.M. and a faculty research award from the University of NorthCarolina to Z.D.

We thank members of the Marzluff laboratory for comments on themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Program in Molecular Biology and Biotechnology, CB# 7100, University of North Carolina,Chapel Hill, NC 27599. Phone: (919) 962-8920. Fax: (919) 966-6821.E-mail: marzluff{at}med.unc.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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26.	Mowry, K. L., and J. A. Steitz. 1987. Both conserved signals on mammalian histone pre-mRNAs associate with small nuclear ribonucleoproteins during 3' end formation in vitro. Mol. Cell. Biol. 7:1663-1672[Abstract/Free Full Text].
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