Two Xenopus Proteins That Bind the 3' End of Histone mRNA: Implications for Translational Control of Histone Synthesis during Oogenesis

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Molecular and Cellular Biology, January 1999, p. 835-845, Vol. 19, No. 1
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Two Xenopus Proteins That Bind the 3' End of Histone mRNA: Implications for Translational Control of Histone Synthesis during Oogenesis

Zeng-Feng Wang,¹^,² Thomas C. Ingledue,¹ Zbigniew Dominski,¹^,³ Ricardo Sanchez,¹^,³ and William F. Marzluff¹^,²^,³^,^*

Program in Molecular Biology and Biotechnology,¹ Department of Biology,² and Department of Biochemistry and Biophysics,³ University of North Carolina, Chapel Hill, North Carolina 27599

Received 6 August 1998/Returned for modification 21 September 1998/Accepted 12 October 1998

	ABSTRACT

Top Abstract Introduction Materials and methods Results Discussion References

Translationally inactive histone mRNA is stored in frog oocytes, and translation is activated at oocyte maturation. The replication-dependenthistone mRNAs are not polyadenylated and end in a conserved stem-loopstructure. There are two proteins (SLBPs) which bind the 3' endof histone mRNA in frog oocytes. SLBP1 participates in pre-mRNAprocessing in the nucleus. SLBP2 is oocyte specific, is presentin the cytoplasm, and does not support pre-mRNA processing invivo or in vitro. The stored histone mRNA is bound to SLBP2. Asoocytes mature, SLBP2 is degraded and a larger fraction of thehistone mRNA is bound to SLBP1. The mechanism of activation oftranslation of histone mRNAs may involve exchange of SLBPs associatedwith the 3' end of histonemRNA.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

In the early development of many organisms, the major level of gene regulation is translational. There is a "switch" fromtranslation of maternal mRNAs that are necessary for oogenesisand maintenance of the oocyte to translation of stored maternalmRNAs that encode essential products for embryogenesis. At thetime of translational activation there are a number of modificationsto the stored mRNP (reviewed in reference 15). These modificationsinclude cytoplasmic polyadenylation of selected mRNAs (35, 37,38, 43, 47), which is determined by a sequence, the cytoplasmicpolyadenylation element, in the 3' untranslated region (UTR) (11);modification of the cap (19); and removal of proteins whichinhibit translation (25, 28, 45). Some or all of these modificationsare involved in the selective activation of translation of mRNAsat oocyte maturation in the frog. The lengthening of the poly(A)tail during oocyte maturation is an essential modification fortranslation of the c-mos (14, 37) and cyclin mRNAs (38).The poly(A) tail has been implicated in the recruitment of mRNAsby the ribosome (18, 30), through an interaction of the poly(A)binding protein with translation initiation factor eIF4G in yeast(40, 41), or by interaction with other proteins that may forma larger complex with the initiation factors (7).

Histone mRNAs are unique among metazoan mRNAs in that they lack a poly(A) tail, ending instead in a conserved stem-loop thatfulfills many of the functions of the poly(A) tail on other mRNAs(23). The stem-loop interacts with a specific RNA-binding protein,termed the stem-loop binding protein (SLBP), which participatesin pre-mRNA processing (22, 46) and remains associated withthe mature histone mRNA as a component of the polyribosomal histonemRNP (8, 16). The stem-loop is essential for translation,presumably as a complex with SLBP (13, 39).

A common feature of all embryos that have a rapid cleavage stage is an extraordinary demand for histone proteins to incorporateinto chromatin. In order to provide the necessary amount of histoneprotein during early embryogenesis, there is not the normal couplingof DNA replication and histone synthesis. Instead histone mRNAsare stable and histone proteins often are stored for later assemblyinto chromatin. The demand for histone proteins increases exponentiallyas cleavage proceeds. Thus, as much new histone must be incorporatedinto chromatin as the embryo cleaves from 1,000 to 2,000 cellsas in the entire previous cleavage period. In the frog, all ofthe histone mRNA (and 75% of the histone protein) to support cleavageuntil the midblastula transition (MBT) (4,000 cells) is storedin the oocyte (51, 52), since there is no transcription untilthe MBT (31). After the MBT, there is active synthesis of histonemRNA to supply additional templates for the synthesis of new histones(42). Histone mRNA translation is activated at oocyte maturationto provide the remaining 25% of the histone protein needed priorto the MBT. The molecular basis of the activation of histone mRNAtranslation is not known, nor is it known how the histone mRNAis stored in an inactive form. It is known that some of the storedhistone mRNAs have short oligo(A) tails (20, 34) that havebeen added to the stem-loop (4). These oligo(A) tails are removedat oocyte maturation (4).

We report here that Xenopus oocytes have two SLBPs. One, SLBP1, is the homologue of the mammalian SLBP present in somaticcells. The other, SLBP2, is an oocyte-specific form. SLBP2 iscytoplasmic, is present in high levels during early oogenesiswhen histone mRNA is stored, and is destroyed early in embryogenesis.In contrast, SLBP1 is present in low levels in early oogenesisand increases in amount during late oogenesis and early embryogenesis.It is likely that exchange of the SLBPs bound to histone mRNAis part of the mechanism of translational activation at oocytematuration.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and methods Results Discussion References

Yeast three-hybrid screen. Four million transformants of Xenopus oocyte cDNA cloned into pGAD10 were screened as described previously with the stem loopsequence used as a bait (46). Plasmids were recovered from yeastthat had activated both the his3 and lacZ genes and tested forthe ability to activate these genes in yeast expressing a mutantstem-loop as the RNA bait (see Fig. 1A). Those plasmids that didnot activate the mutant stem-loop were sequenced, and each encodedan SLBP. The complete sequence of the longest SLBP2 clone wasobtained at the University of North Carolina DNA SequencingFacility.

Treatment of oocytes with antisense oligonucleotides. A series of 12 oligonucleotides (AX01 to AX12, each 15 nucleotides [nt]) were designed to hybridize to the SLBP1 mRNA every80 nucleotides, with the first, AX01, complementary to a regionin the 5' UTR and the last, AX12, complementary to a sequencein the 3' UTR. The oligonucleotides were dissolved in 10 mM Tris-1mM EDTA, extracted with phenol-chloroform, precipitated with ethanol,and then resuspended in water at a concentration of 1 mg/ml. Theseoligonucleotides were tested both for the ability to destroy SLBP1mRNA and for toxicity to the oocyte. Thirty nanoliters (30 ng)of each oligonucleotide was injected into the oocyte cytoplasm.Four hours later, RNA was prepared, resolved by gel electrophoresis,and assayed by Northern blotting with an SLBP1-specific probe.Injected oocytes were also harvested at various times and celllysates were assayed for SLBP by mobility shift assay, using aradiolabeled stem-loop probe. The oligonucleotide that destroyedSLBP1 mRNA and showed the least toxicity was AX03, which was complementaryto nt 457 to 471 of SLBP1 (accession no. U75681) (with theinitiator methionine at nt 1) and had the following sequence:5'-CATATCTTCCTTCCTT. Oocytes were injected with AX09 and allowedto recover for 16 h before subsequent injections with syntheticmRNAs. Injection of this oligonucleotide did not affect U7 snRNAlevels (data notshown).

Expression of proteins and characterization of antibodies. Glutathione S-transferase (GST) fusion proteins were expressed after cloning of full-length SLBP1 and SLBP2 into pGEX-KG.The SLBP1 fusion protein was purified on glutathione-agarose.The SLBP2 fusion protein was present in inclusion bodies and wassolubilized in sodium dodecyl sulfate (SDS) and resolved by preparativegel electrophoresis. The region containing SLBP2 was excised,and the gel was ground up and injected into rabbits. Full-lengthSLBP1 and SLBP2 were also expressed in baculovirus (Bac-to-Bac;GIBCO-BRL), and the resulting His-tagged proteins were purifiedby chromatography on Ni-agarose. The baculovirus-expressed SLBP2protein was used to boost the rabbits that had been injected withthe GST fusion protein. Baculovirus-expressed SLBP1 was injectedinto rabbits to prepare polyclonal antibodies. The SLBP2 antibodieswere purified by resolving the GST-SLBP2 fusion protein expressedin bacteria by SDS-polyacrylamide gel electrophoresis, transferringthe protein to nitrocellulose, and then incubating the serum withthe nitrocellulose strip containing the GST-SLBP2 protein for2 h at 4°C. The affinity-purified antibodies were eluted with0.1 M glycine at pH 2.8 and immediately neutralized. The antiserumto the complete SLBP1 protein disrupted the RNA-protein complexesand also cross-reacted weakly with the SLBP2 protein on Westernblots. To further purify these antibodies, a clone encoding anSLBP1-GST fusion protein with the RNA binding domain deleted wasconstructed and the SLBP1 antibody was purified by binding tothis protein immobilized on nitrocellulose, followed by elutionwith 0.1 M glycine-HCl, pH 2.8. Each of the affinity-purifiedantibodies detected a single polypeptide by Western blotting andefficiently supershifted the appropriate RNA-SLBP complexes. Polyclonalantibodies against the C-terminal 15 amino acids of SLBP1 coupledto keyhole limpet hemocyanin were also prepared. These antibodiesdid not recognize SLBP1 on Western blots and were useful onlyfor analyses of mobility shiftassays.

Mobility shift assays. Frog oocytes of different stages were homogenized in 5 to 10 µl of 15 mM Tris (pH 7.0)-0.1 mM PMSF (phenylmethylsulfonyl fluoride)per oocyte. Nuclei were manually dissected, and extracts wereprepared from nuclei and cytoplasm in the same buffer. The homogenatewas extracted with freon to remove the yolk (10). Similar resultswere obtained with extracts prepared without freon extraction,although not as much protein could be analyzed without affectingthe resolution of the gel. Mobility shift and competition assayswere performed essentially as previously described with 10% polyacrylamidegels (50).

Injection of oocytes. The SLBP1 and SLBP2 proteins were expressed at high levels by injection of a synthetic capped mRNA transcribed from the respectiveSLBPs cloned into a modified version of pSP64T (Promega), whichcontains the 5' and 3' UTRs of the human $beta$ -globin mRNA and a poly(A)tail (a gift of Enrique Amaya and Doug Melton, Harvard University).To express histone mRNAs, the mouse histone H2a-614 gene (15 nl,30 ng/µl) was injected into frog oocytes and RNA was prepared18 h later (49). To assay for both processed and unprocessedRNAs, a probe starting at the Sau3A site 163 nt from the 3' endof the mRNA and extending 33 nt past the stem-loop was constructed,labeled at the 3' end with [ $alpha$ -³²P]dCTP, and used for S1 nuclease mapping. The processed RNAs protecta 163-nt fragment, and the unprocessed RNAs protect a 196-nt fragment.The protected fragments were resolved by polyacrylamide gel electrophoresisand quantified on aPhosphorImager.

Western blots. Oocytes were homogenized in a solution of 0.3 M KCl, 2 mM MgCl₂, 20 mM HEPES (pH 7.4), 0.5% Nonidet P-40 (NP-40), 20% glycerol,2.5 mM dithiothreitol, and 0.1 mM PMSF (5 to 10 µl/oocyte). Thehomogenate was centrifuged for 10 min at 14,000 rpm, and the clearsupernatant was mixed with an equal volume of 2% SDS-10% glycerol-0.06M Tris (pH 6.8)-5% $beta$ -mercaptoethanol and boiled; proteins fromone to three oocytes were resolved by electrophoresis on 12% SDS-polyacrylamidegels and transferred to nitrocellulose. The filter was incubatedwith the affinity-purified antibody, and the bound antibodieswere detected by chemiluminescence with ECL technology(Amersham).

In vitro processing. Nuclear extracts active in histone pre-mRNA processing were prepared from mouse myeloma cells, as previously described (8,24). To remove the endogenous mouse SLBP, an antibody to theC-terminal peptide of SLBP was incubated with 0.5 to 1.0 ml ofnuclear extract for 2 h at 4°C. Twenty microliters of proteinA beads were added per 100 µl of extract. The beads were precoatedby incubation with nuclear extract at 4°C for 30 min prior touse. The beads containing the bound antibody-SLBP complex wereremoved from the extract bycentrifugation.

To complement processing, 100 to 200 ng of purified baculovirus-expressed protein encoding human SLBP, frog SLBP1, or frogSLBP2 was added to the extract. The substrate used was derivedfrom the histone H2a-614 gene with the U7 snRNP binding site ofthe mouse histone H1t gene substituted for the U7 binding siteof the H2a-614 gene (35a). Processing reaction mixtures wereincubated for 1 h at 32°C, and the RNA was prepared and analyzedby gelelectrophoresis.

Histone mRNA immunoprecipitation. The histone mRNAs were precipitated by a modification of the method developed recently in our laboratory (46a). Fifty to100 frog oocytes or eggs were homogenized (2 µl/oocyte) in a solutionof 0.3 M KCl, 20 mM HEPES (pH 7.7), 2 mM MgCl₂, 0.5% NP-40, 2.5mM dithiothreitol, 1 mM cycloheximide, 100 units of the proteaseinhibitor ACE per ml, 1 mM PMSF, and 100 U of RNasin per ml. Thehomogenate was centrifuged for 10 min at 14,000 rpm in a microcentrifuge,and the clear supernatant was used for precipitation. An extractequivalent to five oocytes was incubated with affinity-purifiedantibody (2.5 µg) and 1 U of additional RNasin per µl for 4 hto overnight at 4°C on a rotator. Protein A beads (100 µl) wereincubated with 200 µl of nuclear extract from blastula-stage seaurchin embryos (21). The precoated beads were washed with bufferD (0.1 M KCl, 10 mM HEPES [pH 7.4], 0.1% NP-40, 20% glycerol).Ten microliters of the precoated protein A beads and 30 µl ofbuffer D were added to the oocyte extracts, and the mixture wasincubated for 2 h at 4°C on a rotator. The beads were collectedby centrifugation and washed three times (5 min, 1 h, and 5 min)with 1 ml of buffer D. One hundred microliters of 7 M urea, 2%SDS, 0.35 M NaCl, 10 mM EDTA, and 10 mM Tris (pH 7.5) containing10 µg of tRNA was added, the suspension was extracted once withphenol-chloroform, and the RNA was recovered by precipitationwith ethanol. RNA was also prepared from the supernatant of theincubation with protein A beads. The Xenopus histone H2a mRNAwas detected with an S1 nuclease protection assay using a XenopusH2a gene from a major histone gene cluster (32) cloned fromthe oocyte cDNAlibrary.

Northern blots. Total RNA was prepared from Xenopus oocytes and embryos, as previously described (49). The RNA was treated with formaldehydeand resolved on a 0.8% agarose gel, transferred to nitrocellulose,and hybridized with a mixture of probes from SLBP1, SLBP2, andhistone H3. The probes were prepared by random primer labelingwith [ $alpha$ -³²P]dCTP. The specific activity of the dCTP used to make the histoneH3 probe was 1/20 of that of the dCTP used to make the histoneH3probe.

Nucleotide sequence accession number. The complete nucleotide sequence of the longest SLBP2 clone obtained in this study has been assigned accession no. AF106799.

	RESULTS

Top Abstract Introduction Materials and methods Results Discussion References

We previously reported the isolation of two orthologous SLBPs from human (HeLa cell) and Xenopus oocyte two-hybrid libraries(46) by using the yeast three-hybrid system (36). We screenedfor proteins which bound the wild-type stem-loop sequence in vivobut did not bind a mutant sequence with the stem-loop reversed(Fig. 1A). We obtained multiple isolates of the major SLBP fromboth human and Xenopus libraries (46). However, one of the eightinitial clones selected from the Xenopus library encoded a proteindifferent from the major SLBP. Further analysis of this cloneconfirmed that it passed the selection criteria (specific bindingto the stem-loop in yeast). Sequencing of this clone revealedthat it encodes a 250-amino-acid polypeptide (Fig. 1B), whichwe have termed SLBP2. SLBP2 has similarity to the major SLBP (46),which we have now termed SLBP1, only in the 73-amino-acid RNAbinding domain (68% identity [Fig. 1C]). SLBP2, like SLBP1, issmall, about 28 kDa, and has its RNA binding domain located inthe central region of the protein.

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FIG. 1. Isolation of SLBP2. (A) Wild-type (WT) and mutant (RM) stem-loop sequences used in the yeast three-hybrid selection and RNA binding experiments reported in this paper. (B) Complete nucleotide sequence of the longest SLBP2 clone. The putative polyadenylation signal is underlined. (C) Comparison of the protein sequences of SLBP1 and SLBP2. The RNA binding domains of the two SLBPs are shown in boldface type and underlined. Vertical lines indicate identical amino acids, and double dots indicate similar amino acids.

Subsequent PCR analysis of the 30 clones we isolated from the frog oocyte library with the three-hybrid screen revealed that23 encoded the homologue of the human protein (SLBP1) and 7 encodedSLBP2. Like the SLBP1 clones, many of the SLBP2 clones were fusedto the Gal4 activation domain in the 5' UTR, in frame with therest of the protein. Since the baculovirus-expressed SLBP2 andin vitro-translated SLBP2 have electrophoretic mobilities similarto that of the SLBP2 we have detected in Xenopus oocytes by Westernblotting (not shown), we are confident that we have identifiedthe entire open reading frame. One of the clones we isolated hada poly(A) tail and polyadenylation signal, suggesting that itwas a near-full-length clone. The size of this clone (1,066 nt)agrees well with the size of the SLBP2 mRNA measured by Northernblots (see Fig. 5A).

Two complexes which bind the 3' end of histone mRNA are present in Xenopus oocytes. To study the complexes containing the different SLBPs which are present in Xenopus oocytes, polyclonal antibodies were raisedagainst both recombinant SLBP1 and SLBP2 and were affinity purifiedto remove any cross-reacting antibodies. Synthetic mRNAs encodingSLBP1 and SLBP2 were translated in a rabbit reticulocyte lysate.SLBP1 has mobility similar to mammalian SLBP on SDS-polyacrylamidegels (45 kDa), and SLBP2 has mobility of 35 kDa, close to thepredicted molecular weight of 28 kDa (Fig. 2A). Specific complexeswere formed with each in vitro translation product (Fig. 2B).The complex formed with SLBP1 has mobility similar to the complexformed with the mammalian SLBP (not shown), and the complex wassupershifted by the antibody against SLBP1 but not against SLBP2(Fig. 2B, lanes 5 to 7). The SLBP2 in vitro translation productalso bound the stem-loop specifically (Fig. 2B, lanes 11 to 13)and reacted only with the antibody against SLBP2 (Fig. 2B, lanes9 and 10). The complex formed with SLBP2 has lower mobility thanthe complex formed with SLBP1 in both the reticulocyte lysateand in frog oocyte extracts (see below).

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FIG. 2. Two complexes are formed on the stem-loop in Xenopus oocytes. (A) Clones encoding SLBP1 (lane 1) and SLBP2 (lane 2) were transcribed in vitro and then translated in a rabbit reticulocyte lysate in the presence of [³⁵S]methionine. The products were resolved by electrophoresis on an SDS-12% polyacrylamide gel and detected by radioautography. (B) Reticulocyte lysates programmed with either SLBP1 (lanes 2 to 8) or SLBP2 (lanes 9 to 13) mRNAs were incubated with the radiolabeled probe containing the stem-loop, and the complexes were resolved by gel electrophoresis. The antibody to the C-terminal peptide of SLBP1 was added in lanes 5 to 7 and lane 9. The SLBP1 antibody was preincubated with the antigenic peptide in lane 6 and with control peptide from the N terminus of SLBP1 in lane 7. The affinity-purified antibody to SLBP2 was added in lanes 8 and 10. A 100-fold excess of competitor unlabeled RNAs containing the stem-loop (WT) (lanes 3 and 12) or the reverse-stem (RS) (lanes 4 and 13) sequence was added to some reaction mixtures. (C) Oocytes were fractionated into nuclei and cytoplasm, and proteins from three oocytes were resolved by SDS-polyacrylamide gel electrophoresis. The gel was transferred to nitrocellulose and probed with affinity-purified anti-SLBP1 (lanes 1 and 2) or anti-SLBP2 (lanes 2 and 3) antibodies. (D) Total extracts from frog oocytes were incubated with the wild-type stem-loop probe (lanes 1 to 3 and 6 to 8). A 100-fold excess of unlabeled reverse-stem RNA (RS) (lane 2) or wild-type RNA (WT) (lane 3) was included as competitor. The oocytes were fractionated into nuclei (lane 4) and cytoplasm (lane 5). Affinity-purified polyclonal antibodies to SLBP1 ( $alpha$ -X1) (lane 7) or SLBP2 ( $alpha$ -X2) (lane 8) were added to the reaction mixture. The complexes formed with SLBP1 and SLBP2 are denoted x1 and x2, respectively, and the supershifted complexes are denoted SP (lanes 7 and 8). (E) An extract from stage IV oocytes was incubated with the radiolabeled probe and increasing molar amounts of stem-loop competitor (lanes 2 to 6), and the complexes were resolved by gel electrophoresis. A similar extract from stage III oocytes was incubated with increasing amounts of radiolabeled probe (lanes 7 to 9), and the complexes were resolved by gel electrophoresis.

Extracts were prepared from stage VI Xenopus oocytes, incubated with a 30-nt radiolabeled stem-loop RNA, and then analyzedby electrophoresis under native conditions. Two complexes weredetected in extracts from the whole oocyte (Fig. 2D, lane 1).Formation of both complexes was competed by the wild-type stem-loopbut not by the reverse-stem RNA (Fig. 2D, lanes 2 and 3). To determinethe subcellular localization of the two activities, the oocyteswere manually fractionated into nucleus and cytoplasm. Complexx1 was present in both the nuclear and the cytoplasmic fractions,but complex x2 was found exclusively in the cytoplasm (Fig. 2D,lanes 4 and 5). Antibodies to SLBP1 specifically supershiftedcomplex x1, and antibodies to SLBP2 supershifted complex x2 (Fig.2D, lanes 7 and8).

We also measured the total amount (as compared to free active SLBP) of each SLBP protein in the nucleus and cytoplasm by Westernblotting with affinity-purified SLBP1 and SLBP2 antibodies. SLBP1was found in both the nucleus and the cytoplasm (Fig. 2C, lanes1 and 2), while SLBP2 was found almost exclusively in the cytoplasm(Fig. 2C, lanes 3 and 4). The small amount of SLBP2 in the nuclearfraction probably results from slight contamination withcytoplasm.

To assess the relative affinities of the two SLBPs for the stem-loop, we performed competition experiments with frog extractsthat contained both SLBP1 and SLBP2 binding activity. Two typesof assays were performed (Fig. 2E). When the assay was performedin probe excess and varying amounts of the wild-type competitorwere added to the extract, formation of both complexes was competedto a similar extent at all concentrations of competitor (Fig.2E, lanes 2 to 6). In the second assay, increasing amounts ofprobe were added to the extract to determine whether one SLBPbound preferentially to limiting amounts of probe. As increasingamounts of probe were added, the amounts of complex x1 and x2increased in parallel (Fig. 2E, lanes 7 to 9). Taken together,these results demonstrate that SLBP1 and SLBP2 have similar affinitiesfor the stem-loop.

SLBP1, not SLBP2, functions in histone pre-mRNA processing. To determine whether both SLBP1 and SLBP2 can function in histone pre-mRNA processing, we expressed both SLBP1 and SLBP2 frombaculovirus vectors, and tested the ability of the recombinantproteins to participate in pre-mRNA processing in vitro. Bothof the baculovirus proteins bound to the stem-loop with similaraffinity (Fig. 3A). A nuclear extract highly active in pre-mRNAprocessing was prepared from mouse myeloma cell nuclei, as previouslydescribed (8, 24). The mouse SLBP was removed from this extractby using an antibody against the C-terminal peptide and proteinA-agarose. The depleted extract is inactive in pre-mRNA processing(Fig. 3B, lane 3), while a mock-depleted extract retained mostof its initial activity (Fig. 3B, lanes 1 and 2). Recombinantmouse SLBP, frog SLBP1, and frog SLBP2 expressed in baculoviruswere added back to the extract. Mouse SLBP and frog SLBP1 restoredprocessing to normal levels (Fig. 3B, lanes 4 and 5), demonstratingthat the only component necessary for processing depleted by theantibody was SLBP. Frog SLBP2 was totally inactive in pre-mRNAprocessing (Fig. 3B, lane 6) even though it bound the stem-loop(Fig. 3A, lane 4).

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FIG. 3. SLBP1, but not SLBP2, functions in histone pre-mRNA processing in vitro. (A) SLBP1, SLBP2, and human SLBP (hSLBP) were expressed in baculovirus, and 200 ng of protein was analyzed for binding to the stem-loop by mobility shift assay. (B) A 291-nt substrate was synthesized with T7 RNA polymerase from the mouse histone H1t gene. A nuclear extract prepared from mouse myeloma cells was very active in histone pre-mRNA processing (lane 1). The extract was depleted by using an antibody to the C terminus of mouse SLBP (lane 3), or was treated with immunoglobulin G purified from preimmune serum (lane 2). An equal amount (200 ng) of recombinant baculovirus-expressed mouse SLBP (M) (lane 4), frog SLBP1 (X1) (lane 5), or SLBP2 (X2) (lane 6) was added to the depleted extract. The extracts were incubated for 30 min at 27°C, and RNA was prepared and analyzed by electrophoresis on 8% polyacrylamide-7M urea gels.

We also tested the ability of the two Xenopus SLBPs to complement histone pre-mRNA processing in vivo. Injection of antisenseoligonucleotides into Xenopus oocytes results in degradation ofthe target mRNAs by RNase H and then subsequent degradation ofthe injected oligonucleotide (17). Often there is also reductionof the levels of the encoded protein as a result of destructionof the mRNA (17). We tested several antisense oligonucleotidesagainst SLBP1 for the ability to destroy SLBP1 mRNA. Many of theseresulted in complete cleavage of the SLBP1 mRNA (Fig. 4A, lanes1 to 8), while a control oligonucleotide had no effect on SLBP1mRNA (Fig. 4A, lane 13). One of these oligonucleotides, AX09 (Fig.4A, lane 3), also showed minimal toxicity to the oocytes and wasused for the subsequent studies. Extracts were prepared from oocytes48 h after injection of antisense oligonucleotide AX09. Theseextracts had greatly reduced amounts of free active SLBP1 proteinbut the same amount of free active SLBP2 protein as control oocytesor oocytes injected with a control oligonucleotide (Fig. 4B).Thus, the antisense treatment selectively removed the SLBP1 protein.

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FIG. 4. SLBP1, but not SLBP2, is involved in histone pre-mRNA processing. (A) A series of antisense oligonucleotides (AX07 to AX12, lanes 1 to 6; AX01 to AX06, lanes 7 to 12) directed against SLBP1 mRNA were injected into Xenopus oocytes, and RNA was prepared 4 h later. The RNA was resolved by electrophoresis on a 0.8% agarose gel and probed for SLBP1 mRNA. (B) Oocytes were injected with oligonucleotide AX09 and a control oligonucleotide, and extracts were prepared 48 h later. The extracts were assayed by mobility shift assay for the formation of complexes that bind to the stem-loop. (C) Oocytes were injected with synthetic mRNAs encoding SLBP1 (lanes 2 and 3) or SLBP2 (lane 3 and 4). Forty-eight hours later, the oocytes were fractionated into nuclei and cytoplasm and assayed for the presence of complexes that bound the stem-loop. Lane 1 shows an extract from uninjected oocytes. Extracts from one oocyte were analyzed in each lane. (D) Oocytes were injected with oligonucleotide AX09 (lanes 2 to 4) or with a control oligonucleotide (lane 1). Four hours later, synthetic mRNA encoding SLBP2 (lane 3) or SLBP1 (lane 4) was injected into some of the oocytes. After 48 h, histone H2a-614 DNA was injected into the nucleus. RNA was prepared 18 h after the injection of H2a-614 DNA, and the transcripts were assayed for processed and unprocessed histone mRNA by using an S1 nuclease assay, as shown at the bottom. In a separate experiment, untreated oocytes were injected with buffer (lane 5) or mRNAs encoding frog SLBP2 (lane 6) or frog SLBP1 (lane 7) 48 h prior to injection of histone H2a-614 DNA into the nucleus. RNA was prepared 18 h after injection of the DNA and analyzed by using S1 nuclease mapping.

We then demonstrated that the levels of SLBP1 could be restored by injection of synthetic SLBP1 mRNA. In order to complementthe oocytes deficient in histone pre-mRNA processing, we expressedthe SLBP1 and SLBP2 proteins in the oocyte by injecting mRNAsencoding either SLBP1 or SLBP2. In each case, a large amount ofactive SLBP was expressed as judged by a mobility shift assay.Expression of either SLBP from injected mRNA resulted in a 20-to 30-fold increase in SLBP over the amount already present inthe mature oocyte (Fig. 4C), and overexpressed SLBP1 and SLBP2had the same subcellular distributions as endogenous SLBP1 andSLBP2 (cf. Fig. 4C and Fig. 2C andD).

To determine whether the reduction in free SLBP1 protein resulted in a reduction in the ability to process histone mRNA, wedeveloped an S1 nuclease protection assay that allowed us to measureboth processed and unprocessed mRNA from an injected mouse histonegene (Fig. 4D). This assay maps both the properly processed RNAand any transcripts which extend more than 33 nt past the 3' endof histone mRNA. These heterogeneous longer transcripts all protectthe same size fragment. The ratio of the two protected fragmentsis a measure of the efficiency of processing. When a control oligonucleotidewas injected into the oocytes prior to injection of the mousehistone H2a-614 gene, the majority (70 to 80%) of the transcriptswere processed (Fig. 4D, lane 1). When the oocytes were injectedwith antisense oligonucleotide AX03 prior to injection of theH2a-614 gene, reducing the amount of free SLBP1, the processingefficiency was reduced to about 35% (Fig. 4D, lane 2). Expressionof SLBP1, but not SLBP2, by injection of the appropriate syntheticmRNA restored processing to >80% efficiency in vivo (Fig. 4D,lane4).

We also injected mRNAs encoding either SLBP1 or SLBP2 into oocytes that had not been injected with antisense oligonucleotides.After 48 h, to allow expression of SLBP, the mouse histone H2a-614gene was injected into the oocyte nucleus, and RNA was preparedfrom the oocytes 16 h later. This batch of oocytes processed about80% of the histone transcripts, as did oocytes injected with theSLBP2 mRNA (Fig. 4D, lanes 5 and 6). Oocytes injected with theSLBP1 mRNA processed >95% of the histone transcripts (Fig. 4D,lane 7). Thus, both of these experiments demonstrate that SLBP1,but not SLBP2, functions in histone pre-mRNA processing invivo.

Differential expression of SLBP1 and SLBP2 during development. We used Northern blots, mobility shift assays, and Western blots to measure the expression of SLBP mRNAs and protein duringoogenesis and embryogenesis. Northern blots were done to comparethe levels of histone H3 mRNA, SLBP1 mRNA, and SLBP2 mRNA. SLBP1is encoded by an mRNA which is 6 to 7 kb long (the largest cDNAclone we obtained was 4.5 kb), SLBP2 is encoded by a 1.3-kb mRNA,and histone H3 is encoded by a family of mRNAs about 500 nt inlength. Therefore, we were able to resolve these three mRNA speciesby hybridizing a single blot with all three probes. The specificactivity of the probe for histone mRNA was deliberately made 20times lower than the two SLBP probes, which were of similar specificactivities, to allow the abundant histone mRNA to be readily detectedon the same blot. Some histone mRNA was already present in stageI oocytes, and it reached a constant level by stage III (Fig.5A). There was no further increase in histone mRNA until the MBT(Fig. 5A), when transcription is activated, as previously reported(42). SLBP1 mRNA and SLBP2 mRNA are expressed in stage I oocytesand reach constant levels by stage III of oogenesis. SLBP1 mRNAremains present at the same level in early embryogenesis, andthe amount of SLBP1 mRNA increases after the MBT. In contrast,SLBP2 mRNA is destroyed by the MBT (Fig. 5A, stages 7 and 9) andis not expressed later in embryogenesis or in somatic cells (notshown).

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FIG. 5. Expression of SLBP1 and SLBP2 during oogenesis and early embryogenesis. (A) RNA was prepared from oocytes and early embryos and resolved by gel electrophoresis on a 1% agarose gel. RNA from two oocytes or embryos was analyzed. The gel was transferred to nitrocellulose and hybridized with a mixture of probes to SLBP1, SLBP2, and histone mRNA. The histone probe was made at one-half of the specific activity of the other two probes. The identity of the bands was confirmed by hybridizing with single probes. (B) Extracts were prepared from oocytes and embryos and assayed for SLBP1 and SLBP2 by mobility shift assay. Each lane is analysis of one oocyte. (C) Protein from one oocyte (top) or four oocytes (bottom) was analyzed by Western blotting with either affinity-purified anti-SLBP1 (top) or affinity-purified anti-SLBP2 (bottom). Lanes P show oocytes matured by treatment with progesterone, and lanes E show eggs. The apparent higher mobility of SLBP1 in eggs in this experiment was not seen in other experiments.

To measure the relative amounts of the SLBP1 and SLBP2 proteins, extracts were prepared from the six stages of oogenesis andseveral embryonic stages and assayed by mobility shift assay (Fig.5B) and Western blotting (Fig. 5C). The mobility shift assay measuressoluble, active SLBP. It may not detect SLBPs that are tightlycomplexed with RNA (16) and will not detect any SLBPs that existin modified forms which do not bind RNA with high affinity. Therewere higher levels of SLBP2 binding activity than of SLBP1 bindingactivity in stage I oocytes, and these high ratios persisted throughstage III of oogenesis (Fig. 5B). Later in oogenesis (stages IVto VI), the amount of SLBP1 activity was higher than the amountof SLBP2 activity, due largely to an increase in the amount ofactive SLBP1, although there was also a decrease in the amountof active SLBP2 (Fig. 5B). In eggs and early embryos, there wasvery little SLBP2 activity and large amounts of SLBP1 activity(Fig. 5B). Note that in these assays, which are done in probeexcess, we measure the actual relative amounts of free activeSLBP1 and SLBP2 protein, since they bind the stem-loop with similaraffinities (Fig. 2D).

Qualitatively similar results were obtained when total SLBP1 and SLBP2 protein were measured by Western blotting. We assayedtotal protein from equal numbers of oocytes from different stages.SLBP2 was readily detectable in stage I oocytes and increasedthrough stages III and IV. There was a subsequent slight declinein SLBP2 levels as oocytes matured to stage VI (Fig. 5C, bottom).The levels of SLBP2 protein dropped dramatically in eggs comparedto stage VI oocytes, indicating that most of the SLBP2 is degradedin the transition from oocytes to eggs. SLBP2 was also degradedwhen oocytes were matured in vitro by treatment with progesterone(Fig. 5C, lane P). In contrast, the levels of SLBP1 were verylow in stage I oocytes and gradually increased throughout oogenesis(Fig. 5C, top). There was a further twofold increase in SLBP1when the oocytes were matured to eggs (Fig. 5C). The levels ofSLBP1 continued to increase during early embryogenesis (notshown).

Although the results of the Western blot and mobility shift assays were qualitatively similar, there were significant quantitativedifferences. Western blotting measures all of the SLBP protein,while the mobility shift assay measures the amount of free activeprotein. First, there is a large increase in the SLBP1 activitymeasured by the mobility shift assay at stage IV of oogenesis.In contrast, there is a gradual increase in SLBP1 protein fromstages II to V of oogenesis, as analyzed by Western blotting.These results are consistent with some SLBP1 being released fromhistone mRNA or becoming activated between stage III and stageIV of oogenesis. Second, there is not a dramatic decrease in theamount of free SLBP2 binding activity as oocytes are matured toeggs, as measured by the mobility shift assay, while there isa dramatic drop as measured by Western blotting. This result suggeststhat much of the SLBP2 protein in stage VI oocytes is either boundto histone mRNA or is in an inactive form. These results are consistentwith the accumulation of free SLBP1 late in oogenesis, while mostof the SLBP2 is bound to stored histone mRNA. At oocyte maturation,the degradation of SLBP2 may then allow SLBP1 to associate withthe histonemRNA.

Different SLBPs are associated with histone mRNA during different developmental stages. To determine which SLBPs were associated with histone mRNAs at each stage of oogenesis, we used antibodies to the two SLBPsto precipitate complexes containing the SLBPs from oocyte andegg extracts. RNA was prepared from the antibody precipitatesand the histone H2a mRNA detected by S1 nuclease mapping of thebound and unbound mRNAs. A portion of the unbound fraction wasanalyzed by Western blotting to demonstrate that the SLBPs hadindeed been removed from the extracts (not shown). In each experimentwe performed the precipitations with each extract with the threeantibodies (SLBP1, SLBP2, and mouse SLBP) in parallel. The absoluteamounts of the histone mRNA precipitated varied some from experimentto experiment, but the relative amounts precipitated by anti-SLBP1and anti-SLBP2 were similar for extracts from the same stage indifferent experiments. When stage IV or VI oocytes were analyzed,very little histone H2a mRNA was precipitated by anti-SLBP1. Instage II oocytes, about twice as much histone mRNA was precipitatedby anti-SLBP2 as by anti-SLBP1 (Fig. 6, lanes 1 and 5). More than70% of the histone H2a mRNA was precipitated by anti-SLBP2 instage IV oocytes (Fig. 6, lanes 6), and less than 10% was precipitatedby anti-SLBP1. In stage VI oocytes, three times as much histonemRNA was precipitated by the SLBP2 antibody as the SLBP1 antibody,even though most of the SLBP present in stage VI oocytes is SLBP1.Thus, throughout oogenesis, the bulk of the histone mRNA is associatedwith SLBP2. Since in both stage IV and stage VI oocytes the mostabundant free SLBP is SLBP1 (Fig. 5B), while most of the histonemRNA isolated by antibody precipitation is bound to SLBP2, itis unlikely that there has been significant rearrangement of theSLBPs during the isolation and precipitation procedures.

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FIG. 6. Determination of SLBPs bound to histone mRNA during oogenesis. Extracts from stage II (lanes 1, 5, and 9), stage IV (lanes 2, 6, and 10), and stage VI (lanes 3, 7, 11, 13, 15, and 17) oocytes, oocytes matured in vitro with progesterone (lanes 4, 8, and 12), or eggs (lanes 14, 16, and 18) were incubated with antibodies to either frog SLBP1 (lanes 1 to 4, 13, and 14), frog SLBP2 (lanes 5 to 8, 15, and 16), or mouse SLBP (lanes 9 to 12, 17, and 18). The RNAs bound to the antibodies were isolated and assayed by S1 nuclease mapping for frog histone H2a mRNA (top). RNA was also prepared from the supernatant after incubation with antibody and protein A-agarose and assayed for frog histone H2a mRNA by S1 nuclease mapping (bottom). The protected fragments were resolved by gel electrophoresis and detected by autoradiography. The results are representative of three independent experiments. A diagram of the S1 nuclease assay is shown. The mRNA from this H2a gene protects a 224-nt fragment (H2a), and the mRNAs from other H2a genes protect a 180-nt fragment (H2a_x) which maps to the stop codon.

When eggs were analyzed by an identical procedure using the same two antibodies, the results were strikingly different. Morehistone mRNA was precipitated by the anti-SLBP1 antibody thanby the anti-SLBP2 antibody (Fig. 6, lanes 14 and 16). Essentiallyidentical results were obtained when extracts from oocytes maturedby treatment with progesterone in vitro were analyzed (Fig. 6,lanes 4 and 8). During this period, there is a dramatic decreasein the total amount of SLBP2 protein measured by Western blotting(Fig. 5C). Thus, during the transition from an oocyte to an egg,much of the histone mRNA loses its SLBP2 protein and then bindsto SLBP1 (Fig. 7), and the SLBP2 protein is degraded. This transitionoccurs at the time of activation of histone mRNA translation (51),suggesting that this is one of the molecular events involved intranslational regulation.

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FIG. 7. Model for histone mRNA metabolism during oogenesis in Xenopus.

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

Early in oogenesis, the frog stores most of the maternal mRNAs which will be utilized in early embryogenesis. Storage of mRNAsoccurs concomitantly with the biosynthesis of the mRNA, and someof the essential events, including association with the generaltranslational repressor FRGY2, require that the RNA be synthesizedin the nucleus (6, 26, 29). The stored inactive mRNAs generallyhave short poly(A) tails (47). Other mRNAs that are translatedin oocytes have longer poly(A) tails and are presumably not complexedwith FRGY2 or other translational repressors. At oocyte maturation,a translational program is activated (48) which controls developmentuntil the MBT, when zygotic transcription is activated (31).This program involves default deadenylation of the majority ofmRNAs (12) and selective cytoplasmic adenylation of many RNAsthat are then translated (5, 15). In addition, there aregeneral and sequence-specific RNA binding proteins that are involvedin translational repression, which must also be removed from mRNAsat this time (15). Similar programs of translational controlare present in many early embryos (15, 44, 48).

A fraction of the frog oocyte histone mRNA binds to oligo(dT) cellulose (20, 34) due to a small number of adenosines addedto the end of the stem-loop (4). These terminal adenosinesare removed at oocyte maturation (4). However, only a smallfraction of the stored histone mRNAs with stem-loops in stageVI oocytes are polyadenylated, as judged by binding to oligo(dT)cellulose (35b). This modification does not affect the relativeaffinity of the two different SLBPs (45a), and hence this modificationcannot be essential for the global activation of histone mRNAtranslation.

In organisms with very rapid cleavage stages, there is an exponentially increasing demand for histone proteins to assemblechromatin as development proceeds. Many different strategies haveevolved for dealing with this problem. Some organisms (e.g., seaurchins) have a set of histone genes that are present in multiplecopies and are expressed only during the rapid cleavage stages(27). These zygotic genes supply histone mRNAs during the cleavagestages and then are not used again. In Drosophila, there is storedhistone mRNA utilized initially as well as synthesis of histonemRNA from a set of repeated genes (2, 3).

Since there is no transcription in frog embryos until the MBT (approximately 4,000 cells), the frog embryo must rely solelyon stored histone protein and increased histone mRNA translationto supply the histones necessary to assemble chromatin prior tothe MBT. Histone synthesis is translationally regulated in earlyfrog embryos. During oogenesis, there is synthesis of histonesin stages II and III of oogenesis and then a decrease to a verylow level in oocyte stages IV to VI (51). There is a 17-foldincrease in the rate of histone protein synthesis at oocyte maturation(1, 51). Adamson and Woodland (1) showed that the increasein histone mRNA translation is greatly reduced in enucleated oocytes,suggesting that some component in the nucleus is necessary foractivation of translation of histone mRNA, as it is for regulationof polyadenylation of other oocyte mRNAs (11). There is a furtherincrease in the translation rate during early development, priorto the increase in histone mRNA levels after the MBT, resultingin an ultimate 50-fold increase in the rate of histone proteinsynthesis (51). The same histone mRNAs are expressed in oogenesis,during early development, and in somatic cells (33). Since histonemRNAs are not polyadenylated, they must be translationally regulatedby a mechanism distinct from the regulation of polyadenylatedmRNAs. The different SLBPs are likely candidates to play a keyrole in this translational regulation, and SLBP2 may be a proteinthat has evolved as a specific translationalrepressor.

The 3' end of histone mRNA is essential for association of the mRNA with polyribosomes (39) and translation of histone mRNA(13) in mammalian cells. Since the mammalian homologue of theSLBP1 is a component of the histone mRNP (16), frog SLBP1 isprobably associated with the translationally active histone mRNA.There is synthesis of histone protein during stage II of oogenesisand a lower rate of synthesis in mature oocytes (51, 52).During stage II of oogenesis, the oocyte synthesizes about 75%of the histone protein necessary for early cleavage over a periodof at least 1 to 2 weeks (9). The other 25% of the histoneprotein is synthesized from stored maternal RNA in a few hours.Only a small proportion of the total histone mRNA would be requiredfor production of the histone protein in stage II oocytes. Itis possible that a fraction of the histone mRNA synthesized instage II remains associated with SLBP1 and is translated whilethe remainder of the histone mRNA associates with SLBP2 and isstored.

In support of this possibility, we have found a larger proportion of histone mRNA bound to SLBP1 in stage II oocytes thanin stage IV oocytes (Fig. 6). Early in oogenesis, when histonemRNA is synthesized, the histone mRNA must be processed by SLBP1and subsequently associate with SLBP2 (Fig. 7). A fraction ofthe histone mRNAs may remain associated with SLBP1 and be translatedin stage II, while the rest is transferred to SLBP2 and is stored.Alternatively, all of the histone mRNAs may be translated forsome time prior to association with SLBP2, resulting in storage.There is probably not sufficient SLBP1 to associate with all ofthe histone mRNA in stage II, implying that SLBP1 may functionessentially catalytically rather than stoichiometrically duringthis stage. By stage IV of oogenesis, accumulation of histonemRNA has ceased and the great majority of the histone mRNA isbound to SLBP2. Once bound to SLBP2, the histone mRNA remainsbound to SLBP2 and is translationally inactive throughout theremainder of oogenesis, even while the oocyte accumulates largeamounts of SLBP1 protein. At oocyte maturation, there is a lossof SLBP2 from much of the histone mRNA, the histone mRNA is thenbound by SLBP1, and SLBP2 is degraded (Fig. 7). One of the changeswhich occurs to activate translation of the histone mRNA at oocytematuration likely involves removal of SLBP2, followed by associationof SLBP1 with the stored histone mRNA. During embryogenesis, thereis a further increase in the amount of histone mRNA translation,presumably as the rest of the SLBP2 is removed from the histonemRNA and is replaced bySLBP1.

	ACKNOWLEDGMENTS

This work was supported by grants GM29832 and GM27789 from the NIH to W.F.M. T.C.I. was supported by a postdoctoral fellowshipfrom the Andrew W. MellonFoundation.

We thank Sally Kornbluth for some of the frog eggs used in these experiments and Mike Whitfield for advice on the mRNA immunoprecipitationexperiments and for critical comments on themanuscript.

Z.-F.W. and T.C.I. contributed equally to thiswork.

	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
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Sanchez, R., Marzluff, W. F. (2002). The Stem-Loop Binding Protein Is Required for Efficient Translation of Histone mRNA In Vivo and In Vitro. Mol. Cell. Biol. 22: 7093-7104 [Abstract] [Full Text]
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Sullivan, E., Santiago, C., Parker, E. D., Dominski, Z., Yang, X., Lanzotti, D. J., Ingledue, T. C., Marzluff, W. F., Duronio, R. J. (2001). Drosophila stem loop binding protein coordinates accumulation of mature histone mRNA with cell cycle progression. Genes Dev. 15: 173-187 [Abstract] [Full Text]
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