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© The Rockefeller University Press,
0021-9525/2000//1177 $5.00
The Journal of Cell Biology, Volume 148, Number 6,
, 2000 1177-1186
Original Article |
Gemin4
: A Novel Component of the Smn Complex That Is Found in Both Gems and Nucleoli
b Department of Biochemistry and Biophysics, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104-6148
c European Molecular Biology Laboratory, 69012 Heidelberg, Germany
d Protein Interaction Laboratory University of Southern Denmark, DK-5230 Odense M, Denmark
Howard Hughes Medical Institute, University of Pennsylvania School of Medicine, 415 Curie Boulevard, Philadelphia, PA 19104-6148.215-573-2000215-898-0398
gdreyfuss{at}hhmi.upenn.edu
The survival of motor neurons (SMN) protein, the product of the neurodegenerative disease spinal muscular atrophy (SMA) gene, is localized both in the cytoplasm and in discrete nuclear bodies called gems. In both compartments SMN is part of a large complex that contains several proteins including Gemin2 (formerly SIP1) and the DEAD box protein Gemin3. In the cytoplasm, the SMN complex is associated with snRNP Sm core proteins and plays a critical role in spliceosomal snRNP assembly. In the nucleus, SMN is required for pre-mRNA splicing by serving in the regeneration of spliceosomes. These functions are likely impaired in cells of SMA patients because they have reduced levels of functional SMN. Here, we report the identification by nanoelectrospray mass spectrometry of a novel component of the SMN complex that we name Gemin4. Gemin4 is associated in vivo with the SMN complex through a direct interaction with Gemin3. The tight interaction of Gemin4 with Gemin3 suggests that it could serve as a cofactor of this DEAD box protein. Gemin4 also interacts directly with several of the Sm core proteins. Monoclonal antibodies against Gemin4 efficiently immunoprecipitate the spliceosomal U snRNAs U1 and U5 from Xenopus oocytes cytoplasm. Immunolocalization experiments show that Gemin4 is colocalized with SMN in the cytoplasm and in gems. Interestingly, Gemin4 is also detected in the nucleoli, suggesting that the SMN complex may also function in preribosomal RNA processing or ribosome assembly.
Key Words: gems • nucleoli • SMN • spinal muscular atrophy • snRNP biogenesis
© 2000 The Rockefeller University Press
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Introduction |
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The SMN protein is part of a multiprotein complex and two other proteins of the complex, Gemin2 (formerly SIP1) and Gemin3 (for component of gems 2 and 3, respectively) thus far have been characterized (Liu et al. 1997; Charroux et al. 1999). SMN, Gemin2, and Gemin3 localize in the cytoplasm and the nucleus of somatic cells. In the nucleus, they are concentrated in bodies called gems, which are similar in size and number to coiled bodies (CBs) and are often associated with them (Liu and Dreyfuss 1996; Liu et al. 1997; Charroux et al. 1999). In addition to SMN, Gemin2 and Gemin3, the large cytoplasmic complex of which they are part also contains Sm proteins that are components of spliceosomal small nuclear ribonucleoprotein (snRNPs; Liu et al. 1997; Charroux et al. 1999). SMN interacts directly with the Sm proteins and with Gemin2 and Gemin3 (Liu et al. 1997; Charroux et al. 1999; Pellizzoni et al. 1999). Antibody microinjection experiments in Xenopus oocytes revealed that Gemin2 has a critical role in the assembly of snRNPs (Fischer et al. 1997), a process which takes place in the cytoplasm where the Sm proteins combine with snRNAs that were exported from the nucleus (Mattaj and De Robertis 1985; Mattaj 1988; Luhrmann et al. 1990). Once properly assembled and modified, the snRNPs recruit the necessary nuclear import receptors and translocate into the nucleus where they function in pre-mRNA splicing (Mattaj 1986, Mattaj 1988; Luhrmann et al. 1990; Neuman de Vegvar and Dahlberg 1990; Zieve and Sauterer 1990). Transfections of a dominant negative form of SMN (SMN
N27) revealed that SMN also plays a critical role in the cytoplasmic assembly of snRNPs (Pellizzoni et al. 1998). In the nucleus, overexpression of the SMNN27 protein causes a striking rearrangement of the snRNPs, which accumulate with the mutant SMNN27 in enlarged gem/coiled body structures (Pellizzoni et al. 1998). SMN has been further shown to be required for pre-mRNA splicing, likely for the regeneration or recycling of snRNPs (Pellizzoni et al. 1998). Of the known components of the SMN complex, the recently described DEAD box protein Gemin3 is the most likely candidate to have the capacity to perform such functions (Charroux et al. 1999). Interestingly, SMN mutants found in SMA patients lack the snRNP regeneration activity likely because of their defective interaction with the Sm proteins as well as with Gemin3 (Pellizzoni et al. 1998, Pellizzoni et al. 1999; Charroux et al. 1999).
Here, we report the amino acid sequencing by nanoelectrospray mass spectrometry (Wilm et al. 1996) and molecular cloning of a novel component of the SMN complex designated Gemin4 (available from GenBank/EMBL/DDBJ under accession number AF173856). Several lines of evidence suggest that Gemin4 participates in the functions of the SMN complex. Together with SMN, Gemin2 and Gemin3, Gemin4 can be isolated in a complex with the spliceosomal snRNP proteins. The presence of Gemin4 in the SMN complex in vivo is a result of its direct interaction with Gemin3 but not with SMN. Gemin4 also interacts directly with several of the spliceosomal snRNP core Sm proteins, including SmB, SmD1-3, and SmE, and is associated with U snRNAs in the cytoplasm of Xenopus oocytes. Gemin4 is a novel protein and shows no significant homology to any other protein found in the databases. Its tight association with Gemin3 suggests that it may act as a cofactor of the putative ATPase and/or helicase activity of Gemin3. We have produced mAbs to Gemin4, and show by immunofluorescence microscopy that it colocalizes with SMN in gems. Interestingly, unlike other gems proteins described so far, Gemin4 is also detected in the nucleolus, suggesting that it may have additional functions in ribosome biogenesis.
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Materials and Methods |
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Production of mAbs to Gemin4
Anti-Gemin4 antibody 22C10 was prepared by immunizing Balb/C mice with a His-tagged COOH-terminal fragment of Gemin4. Hybridoma production, screening, and ascites fluid production were performed as previously described (Choi and Dreyfuss 1984).
Immunoprecipitation and Immunoblotting
Immunoprecipitations of in vitro translated proteins were carried out in the presence of 1% Empigen BB buffer as previously described (Choi and Dreyfuss 1984). Coimmunoprecipitations were carried out using total HeLa lysate in the presence of 0.5% Triton X-100 as previously described (Pinol-Roma et al. 1988). For immunoblotting, proteins were resolved on 12.5% SDS–polyacrylamide gels and transferred to nitrocellulose membranes (Schleider and Schuell, Inc.) using a BioTrans Transblot apparatus (model B; Gelman Science) according to the manufacturer's instructions. The membranes were incubated in blocking solution (PBS 5% nonfat milk) for at least 1 h at room temperature, rinsed with cold PBS, and incubated in blocking solution with primary antibody for at least 1 h at room temperature. Membranes were washed three times in PBS containing 0.05% NP-40, followed by incubation with peroxidase-conjugated secondary antibodies (Jackson ImmunoResearch Laboratories, Inc.), which were visualized by an ECL Western blotting kit (Amersham) after three additional washes with PBS containing 0.05% NP-40.
Cell Culture
HeLa cells were cultured in DME supplemented with 10% FBS (both from GIBCO BRL).
Immunofluorescence Microscopy
Immunofluorescence staining was carried out essentially as previously described (Choi and Dreyfuss 1984). Double-labeled immunofluorescence experiments were performed by separate, sequential incubations of each primary antibody diluted in PBS containing 3% BSA, followed by the specific secondary antibody coupled to either FITC or Texas red. All incubations were carried out at room temperature for 1 h. Laser confocal fluorescence microscopy was performed with a Leica TCS 4D confocal microscope. Images from each channel were recorded separately and, where indicated, the files were merged. Antibodies used in these experiments were as follows: mouse IgG1 monoclonal anti-Gemin4 (22C10; this work); mouse IgG1 monoclonal anti-SMN (2B1; Liu and Dreyfuss 1996); rabbit polyserum anti-p80 coilin (R288; Andrade et al. 1991); mouse IgG3 monoclonal anti-Sm (Y12; Lerner et al. 1981); human autoimmune antibody against fibrillarin 1881 (Reimer et al. 1987); and rabbit affinity-purified anti-SMN exon 7 epitope antibody (Liu et al. 1997).
In Vitro Protein-binding Assay
Purified GST or GST fusion proteins (2 µg) bound to 25 µl of glutathione-Sepharose beads were incubated with 106 cpm of in vitro translated protein in 1 ml of binding buffer (50 mM Tris-HCl, pH 7.5, 200 mM NaCl, 2 mM EDTA, 0.1% NP-40, 2 µg/ml leupeptin and pepstatin A, and 0.5% aprotinin). After incubation for 1 h at 4°C, the resin was washed five times with 1 ml of binding buffer. The bound fraction was eluted by boiling in SDS-PAGE sample buffer and run on SDS-PAGE. The gels were fixed for 30 min and the signal was enhanced by treatment with Amplify solution (Amersham). For direct in vitro binding, we used 5 µg of purified His-tagged SmB and a binding buffer (50 mM Tris-HCl, pH 7.5, 100 mM NaCl, 2 mM EDTA, 0.05% NP-40, 2 µg/ml leupeptin and pepstatin A, and 0.5% aprotinin). The binding experiment was performed as described above, except that bound His-tagged SmB proteins were immunodetected by Western blot using a rabbit polyclonal anti-His tag antibody (Santa Cruz Biotechnology).
Gel Filtration
Total HeLa cell extract prepared in RSB-100 was loaded on a Superose 6 HR 10/30 column (Pharmacia). The column was washed with RSB-100 at a flow rate 0.5 ml/min. Fractions (1 min) were collected, and 1:20 of each fraction was resolved on SDS-PAGE followed by Western blotting.
Oocyte Injections and Immunoprecipitation of RNA–Protein Complexes
Injections were carried out as previously described (Fischer et al., 1993). In brief, oocytes were incubated for 3 h in modified Barth's solution containing 0.2% collagenase type II (Sigma Chemical Co.). Defolliculated stage V and VI oocytes were collected and usually used the day after for microinjection. In a typical injection experiment, 30 nl of 32P-labeled RNA (106 cpm/µl; total concentration of 0.7 µM) was injected into the cytoplasm. For immunoprecipitation of RNA–protein complexes (Fisher et al., 1993), the injected oocytes were homogenized in 300 µl of ice-cold PBS, pH 7.4. The insoluble fraction was pelleted by centrifugation, and the clear supernatant was transferred into a new 1.5-ml Eppendorf tube containing antibodies bound to protein G–Sepharose (Pharmacia). This mixture was incubated with constant shaking for 1 h at 4°C and subsequently washed five times with 1 ml of ice-cold PBS. Bound RNAs were isolated by phenol extraction for 1 h, precipitated with ethanol, and analyzed by denaturing gel electrophoresis.
Plasmid DNA and In Vitro Transcription
In vitro transcription of 32P-labeled RNAs was carried out as described in Fisher et al. (1993) from plasmids encoding for U1, U2, U4, and U5 snRNAs. The plasmid encoding the chicken 
-crystallin pre-mRNA was previously described (Pellizzoni et al. 1998). The plasmid encoding the chicken -crystallin mRNA was constructed by elution of the chicken -crystallin mRNA from polyacrylamide gel followed by reverse transcriptase–PCR and subcloning into pSP65 (pSP1415m; Promega Corp). The plasmids used for in vitro transcription and translation of SMN, Gemin2, Gemin3, and the Sm proteins have been previously described (Charroux et al. 1999; Pellizzoni et al. 1999).
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97 kD (Fig. 2 B). Finally, 22C10 specifically immunoprecipitated a single protein of 97 kD from [35S]methionine-labeled HeLa and mouse 3T3 cell lysates (Fig. 2 C), suggesting that Gemin4, like SMN, is conserved in vertebrates.
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Gemin4 Is in a Complex with SMN, Gemin2 and Gemin3
To characterize the Gemin4-containing complex, we tested for its presence in the SMN complex in vivo by coimmunoprecipitation and Western blotting experiments. The anti-Gemin4 mAb 22C10 was used for immunoprecipitation from HeLa cell total extracts, and these were resolved by SDS-PAGE, immunoblotted, and probed with the anti-SMN antibody 2B1 (Liu and Dreyfuss 1996). As shown in Fig. 4 A (lane 22C10 IP), 2B1 readily detects SMN in the 22C10 immunoprecipitates, indicating that SMN is coimmunoprecipitated with Gemin4. Because SMN forms a stable complex with Gemin2 in vivo and in vitro (Liu et al. 1997), we also investigated whether Gemin2 could be coimmunoprecipitated with Gemin4. As shown in Fig. 4 A, the anti-Gemin2 mAb 2S7 clearly detects Gemin2 in the anti-Gemin4 immunoprecipitates (lane 22C10 IP). We also examined whether Gemin4 can be coimmunoprecipitated with Gemin3, which is a recently identified novel component of the SMN complex (Charroux et al. 1999). Fig. 4 A shows that, like SMN and Gemin2, Gemin4 is present in the anti-Gemin3 (lane 11G9 IP) immunoprecipitate (Charroux et al. 1999). In a reciprocal experiment, the Gemin4 protein could also be coimmunoprecipitated by the anti-SMN, the anti-Gemin2, and the anti-Gemin3 mAbs (Fig. 4 B). No SMN, Gemin2, Gemin3, or Gemin4 proteins were detected in the control nonimmune (SP2/0) immunoprecipitate (data not shown and lane SP2/O, Fig. 4 B). These results suggest that SMN, Gemin2, Gemin3, and Gemin4 are associated in vivo in one or more complexes that can be immunoprecipitated by either anti-SMN, anti-Gemin2, anti-Gemin3, or anti-Gemin4 antibodies.
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800 kD, indicating that they are components of a large macromolecular complex (Fig. 4 B). Gemin4 is also detected in a second complex of 550 kD that lacks SMN and Gemin2 but does contain a faster migrating form of Gemin3. Thus, there appear to be at least two different Gemin4-containing complexes.
A second peak containing SMN and Gemin2, but lacking Gemin3 and Gemin4, is observed at lower molecular mass fractions that correspond to 100 kD. The SMN protein present in these fractions was not detectable with a rabbit polyclonal antibody specific to the peptide sequence encoded by exon 7 of SMN (Liu et al. 1997; Fig. 4 B). Thus, this smaller SMN–Gemin2 complex contains the oligomerization-deficient form of SMN lacking amino acids encoded by exon 7, which is most likely produced by the SMN2 gene (see Discussion; Gennarelli et al. 1995; Lefebvre et al. 1995; Pellizzoni et al. 1999).
Gemin4 Interacts Tightly with the DEAD Box Protein Gemin3
To investigate the interactions of Gemin4, we performed in vitro protein binding assays using Gemin4 and several constituents of the SMN complex. For this assay, purified GST or GST-Gemin4 fusion immobilized on gluthathione-Sepharose were incubated with [35S]methionine-labeled SMN, Gemin2, Gemin3, and Gemin4 produced by in vitro transcription and translation in rabbit reticulocyte lysate. As shown in Fig. 5 A, full-length Gemin3 is the only protein of the SMN complex that binds specifically to immobilized GST-Gemin4 (Fig. 5 A). No binding to GST alone was observed (data not shown).
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Gemin4 Is Associated with Spliceosomal snRNPs in the Cytoplasm
To further characterize the Gemin4 complex, immunoprecipitations using anti-Gemin4 mAbs from [35S]methionine-labeled HeLa cells were carried out, and the immunoprecipitated proteins were analyzed by SDS-PAGE. As references for these immunoprecipitations, we also performed immunoprecipitation with the anti-Sm mAb Y12 (Lerner and Steitz 1979; Lerner et al. 1981) and with the anti-SMN mAb 2B1. As shown in Fig. 6 A, several proteins are coimmunoprecipitated with anti-Gemin4 antibodies, and the pattern is very similar to the one obtained with anti-SMN antibodies. Besides SMN, Gemin2, Gemin3, and Gemin4, the Sm core proteins B/B', D1-3, E, F, and G proteins were also coimmunoprecipitated with the 22C10 anti-Gemin4 antibody. Additional proteins coimmunoprecipitated specifically with anti-SMN (at 175, 95, 60, and 50 kD) or anti-Gemin4 (at 80 kD) mAbs. Note that the U1-specific A protein, but not the U1-specific C protein, coimmunoprecipitates with SMN and Gemin4. This indicates that the SMN complexes are not associated with mature snRNP particles.
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To determine whether Gemin4 was associated with snRNAs in vivo, we used the Xenopus oocyte that provides a particularly advantageous system in which to study spliceosomal snRNP biogenesis by use of microinjection (Mattaj and De Robertis 1985; Mattaj 1986). We first wished to determine whether Gemin4 is present in Xenopus cells and whether it can be recognized by 22C10 antibody. The 22C10 mAb showed both gems and nucleolar staining on Xenopus XL177 somatic cells, strongly suggesting that Gemin4 is conserved in Xenopus (data not shown). However, immunoblotting with the anti-human Gemin4 mAb 22C10 on Xenopus tissue culture cells or on Xenopus oocyte lysates did not detect any protein (data not shown). To determine if Gemin4 is associated with U snRNAs in vivo, various 32P-labeled RNAs including chicken -crystallin mRNA, chicken -crystallin pre-mRNA, and the spliceosomal snRNAs U1 and U5 were produced by in vitro transcription and a mixture of these RNAs was microinjected into the cytoplasm of oocytes. After 3 h, immunoprecipitations were carried out with anti-Gemin4 (22C10) and, as a positive control, anti-Gemin2 (2E17) antibodies (Fischer et al. 1997). Fig. 7 A shows that only U1 and U5 snRNAs are efficiently and specifically precipitated, indicating that they associate with Gemin4. A similar, but less efficient, immunoprecipitation of U1 and U5 snRNAs was observed with the anti-Gemin2 antibody. We further asked whether the other spliceosomal U snRNAs, U2 and U4, were associated with Gemin4 as well, and whether the association of Gemin4 with mature U snRNPs was also observed in the nucleus. To do so, a mixture of 32P-labeled U snRNAs were injected into the cytoplasm of oocytes followed by an 18-h incubation (Fig. 7 B). After this incubation period, 50% of the injected snRNA was imported into the nucleus while the rest remained in the cytoplasm. Immunoprecipitations from the nuclear and cytoplasmic fractions were carried out with either anti-Gemin4 antibody, anti-Sm antibody as a positive control, or SP2/O as a negative control. The coimmunoprecipitated RNAs were analyzed by gel electrophoresis. As previously reported, U1, U2, U4, and U5 were efficiently immunoprecipitated by Y12 in approximately equal amounts from the nucleus and the cytoplasm (Fig. 7 B; Mattaj 1986; Fisher and Luhrmann, 1990). In contrast, Gemin4 associated more efficiently with U1 and U5 than U2 and U4, and this association was only observed in the cytoplasm (Fig. 7 B).
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Discussion |
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Unlike Gemin2 and Gemin3, Gemin4 does not interact with SMN directly and its presence in the SMN complex is probably the result of its direct and stable interaction with Gemin3. The observation that Gemin4 and the DEAD box protein Gemin3 interact with each other directly and avidly suggests that they function together. Previous studies have shown that the RNA helicase activity of the translation initiation factor eIF4A, also a DEAD box protein, is dependent on the presence of a second initiation factor, eIF4B. Interestingly, in a series of preliminary experiments we have so far not been able to detect RNA helicase or RNA-dependent ATPase activity for recombinant Gemin3 (Charroux et al. 1999). It is possible that such activity will only manifest itself when Gemin3 is associated with other proteins such as Gemin4.
Gel filtration experiments revealed the presence of two SMN complexes in HeLa cells. The high molecular mass complex is the most abundant and contains all the components of the SMN complex thus far identified (SMN, Gemin2, Gemin3, and Gemin4) and likely represents an active form of the complex (see below). The large size of this complex is likely the result of the capacity of SMN to form large oligomers (Pellizzoni et al. 1999). The second complex probably represents a monomeric, COOH-terminal–truncated form of SMN (SMNEx7) associated with Gemin2 (Pellizzoni et al. 1999). While SMN1 produces only full-length mRNA, SMN2 mainly produces an alternatively spliced form of SMN mRNA lacking exon 7 (Gennarelli et al. 1995; Lefebvre et al. 1995). Exon 7 skipping is due to the presence of a single nucleotide change in the SMN2 gene compared with SMN1 (Lorson et al. 1999), and the ratio of alternatively spliced versus full-length SMN2 mRNA correlates with the severity of SMA (Gavrilov et al. 1998). Nevertheless, no evidence for the presence of SMN protein lacking exon 7–encoded amino acids in vivo has been reported. The absence of the amino acid sequence encoded by exon7 is thought to generate a nonfunctional SMN protein that lacks the capacity to oligomerize and, thus, cannot interact with Sm proteins (Burghes 1997; Lorson et al. 1998; Pellizzoni et al. 1999). The absence of Gemin3 and Gemin4 from the SMNEx7–Gemin2 complex probably results from the defective interaction of SMNEx7 with Gemin3 (Charroux et al. 1999). We have shown that SMNEx7 is a nonfunctional protein that is incapable, unlike wild-type SMN, of regenerating splicing extracts in vitro (Pellizzoni et al. 1998). Thus, the loss of function of SMNEx7 is likely due to its defective interaction with the Sm proteins as well as with the Gemin3–Gemin4 complex (Charroux et al. 1999; Pellizzoni et al. 1999). Therefore, we suggest that the SMNEx7–Gemin2 complex represents an inactive form of the SMN complex, whereas the high molecular mass complex containing SMN, Gemin2, Gemin3, and Gemin4 represents the active complex that can bind substrates such as the Sm proteins and carry out the functions of the complex (Fig. 8; Fischer et al. 1997, Pellizzoni et al. 1998, Pellizzoni et al. 1999).
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Acknowledgments |
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-crystallin mRNA was a gift from Dr. Naoyuki Kataoka (our laboratory). We are grateful to members of our laboratory for stimulating discussions and, in particular, Drs. Westley Friesen, Zissimos Mourelatos, and Sara Nakielny for helpful discussions and critical comments on this manuscript. This work was supported by a grant from the National Institutes of Health. G. Dreyfuss is an Investigator of the Howard Hughes Medical Institute.
Submitted: 22 November 1999
Revised: 1 February 2000
Accepted: 4 February 2000
Abbreviations used in this paper: CB, coiled body; Gemin2, 3, and 4; component of gems number 2, 3, and 4, respectively; ORF, open reading frame; SMA, spinal muscular atrophy; SMN, survival of motor neurons; snRNP, small nuclear ribonucleoprotein (RNP); snoRNP, small nucleolar RNP.
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