Hori T , Taguchi Y , Uesugi S , Kurihara Y .

	Figure 1. In vitro selection of RNA ligands for mPrrp using random RNA pools. (A) Schematic representation of the domain structure of mPrrp protein and mutants used in this study. The full-length mPrrp (405 amino acids) contains both RBDs in the N-terminal region and a proline-rich region in the C-terminal region. The bacterially expressed full-length mPrrp (mPrrp-FL, 1–405 amino acids), RNA-binding domain (mPrrp-2xRBD, 1–201 amino acids), and proline-rich region (mPrrp-Pro, 201–405 amino acids) derivatives contain a thioredoxin-tag, and His-tags at the N- and C- terminals. (B) Confirmation of the progress of the RNA selection was performed by gel mobility shift assay. Ten femtomoles of RNA prepared from each round of selection was labeled with 32P and incubated with 6 pmol mPrrp-2xRBD (final, 300 nM; lanes 1–6) or mPrrp-Pro (lane 8), and then the mixture was analyzed by electrophoresis. Free RNA probes and RNA–protein complexes are indicated by arrowheads. (C) The sequences of 22 unique clones obtained after five rounds of RNA selection are shown. The conserved sequence elements are indicated by hatched bold characters (E1) and underlined bold characters (E2). The individual sequences are classified into four groups: Group A containing both E1 and E2, Group B (E1 only), Group C (E2 only) and Group D (not containing any conserved elements). The sequences derived from the constant primer sequences are indicated in lower case characters.
	Figure 2. Binding experiments on several selected RNAs and mPrrp-2xRBD protein. (A) Gel mobility shift assay of mPrrp-2xRBD protein with several selected RNAs (S-2, lanes 1–4; S-13, lanes 5–8; and S-52, lanes 9–12). An aliquot of 10 fmol of 32P-labeled RNAs (final, 0.5 nM) was incubated with various concentrations of mPrrp-2xRBD protein: 0 nM (lanes 1, 5 and 9), 50 nM (lanes 2, 6 and 10), 100 nM (lanes 3, 7 and 11) and 300 nM (lanes 4, 8 and 12), and the mixtures were run on non-denaturing polyacrylamide gels. (B) Competitive RNA-binding experiments involving unlabeled RNAs. Ten femtomoles (final, 0.5 nM) of 32P-labeled S-13 RNA was incubated with mPrrp-2xRBD protein at a final concentration of 300 nM, and the following amounts of unlabeled competitor RNAs: 100 fmol (lanes 3 and 6), 1000 fmol (lanes 4 and 7) and 10 000 fmol (lanes 5 and 8). Free RNA probes and RNA–protein complexes are indicated by arrowheads. pBS RNA was transcribed from pBluescript SK(+) digested with XbaI.
	Figure 3. Minimum sequence requirement of S-13 RNA. (A) The sequences used for deletion mutant analysis of S-13 RNA are shown. The mutant names derive from the positions at the start and end of the full-length S-13 RNA. The minimum RNA sequence for binding to mPrrp is indicated at the bottom (positions 26–73). The lower case character sequence at 5′ terminal is derived from the sequence for transcription initiation by T7 RNA polymerase and the other one at the 3′ terminal is derived from the sequence of the restriction enzyme site (BamHI). (B) Gel mobility shift assay of mPrrp-2xRBD protein with deletion mutants. Ten femtomoles of 32P-labeled RNAs (final, 0.5 nM) was incubated with various concentrations of mPrrp-2xRBD protein: 0 nM (lanes 1, 4, 7, 10, 13 and 16), 100 nM (lanes 2, 5, 8, 11, 14 and 17) and 300 nM (lanes 3, 6, 9, 12, 15 and 18), and the mixtures were run on non-denaturing polyacrylamide gels. Free RNA probes and RNA–protein complexes are indicated by arrowheads as in previous figures.
	Figure 4. Point mutation analysis of the putative binding sites in S-13 RNA by gel mobility shift assay. Point mutations were introduced in to E1 (lanes 1–21) and E2 (lanes 22–39) in S-13 RNA. An aliquot of 10 fmol of 32P-labeled RNAs (final, 0.5 nM) was incubated with various concentrations of mPrrp-2xRBD protein: 0 nM (lanes 1, 4, 7, 10, 13, 16, 19, 22, 25, 28, 31, 34 and 37), 100 nM (lanes 2, 5, 8, 11, 14, 17, 20, 23, 26, 29, 32, 35 and 38) and 300 nM (lanes 3, 6, 9, 12, 15, 18, 21, 24, 27, 30, 33, 36 and 39), and the mixtures were run on non-denaturing polyacrylamide gels. Free RNA probe and RNA–protein complexes are indicated by arrowheads as in previous figures.
	Figure 5. Secondary structure analysis of the selected RNAs. 5′-32P-labeled full-length S-13 RNA (A) and S-52 RNA (B) were subjected to partial digestion with sequence- or structure-dependent nucleases, and then run on 12% polyacrylamide sequencing gels. (A and B): Al (lane 1), alkaline hydrolysis products as size marker; C (lanes 2), untreated RNAs as a control; T1 (lane 3), RNase T1; V1 (lanes 4), RNase V1; and MB (lanes 5), mung bean nuclease. The secondary structure models superimposed with RNase digestion results, S-13 (C), S-2 (D) and S-52 (E), are shown. Cleavage sites for RNase V1 and mung bean nuclease are indicated by filled and open arrowheads, respectively, and relative cleavage intensities are indicated. The G residues cleaved by RNase T1 are indicated by open circle, and relative cleavage intensities are shown.
	Figure 6. Secondary structure comparison of full-length S-13 RNA and its deletion mutants. 5′-32P-labeled full-length S-13 RNA and its truncated, from the 3′-end (A) or from the 5′-end (C), mutants were subjected to partial digestion with sequence- or structure-dependent nucleases, and then run on 12 or 20% polyacrylamide sequencing gels, respectively. Al [lane 1 in (A); lanes 1 and 6 in (C)], with alkaline hydrolysis products as markers; T1 [lane 2 in (A); lanes 3 and 8 in (C)], RNase T1; C [lanes 3, 6, 9 and 12 in (A); lanes 2 and 7 in (C)], untreated RNAs as a control; V1 [lanes 4, 7, 10 and 13 in (A); lanes 4 and 9 in (C)], RNase V1; and MB [lanes 5, 8, 11 and 14 in (A); lanes 5 and 10 in (C)], mung bean nuclease. The secondary structure models mapped with RNase digestion results, DM 1–67 (B), and DM 26–89 and 32–89 (D), are shown. Cleavage sites for RNase V1 and mung bean nuclease are indicated by filled and open arrowheads, respectively, relative cleavage intensities are shown. The nucleotide positions of the mutants are numbered according to full-length S-13 RNA. The two G residues at the 5′ end of the RNAs required for transcription by T7 RNA polymerase and additional sequences of 3′ end restriction enzyme sites (BamHI) are indicated in lower case characters.

Braun, Genomic organization of profilin-III and evidence for a transcript expressed exclusively in testis. 2002, Pubmed

Braun, Genomic organization of profilin-III and evidence for a transcript expressed exclusively in testis. 2002, Pubmed
Buckanovich, The neuronal RNA binding protein Nova-1 recognizes specific RNA targets in vitro and in vivo. 1997, Pubmed
Burd, RNA binding specificity of hnRNP A1: significance of hnRNP A1 high-affinity binding sites in pre-mRNA splicing. 1994, Pubmed
Cho, The relative levels of translin-associated factor X (TRAX) and testis brain RNA-binding protein determine their nucleocytoplasmic distribution in male germ cells. 2004, Pubmed
Claussen, Xvelo1 uses a novel 75-nucleotide signal sequence that drives vegetal localization along the late pathway in Xenopus oocytes. 2004, Pubmed , Xenbase
Gertler, Mena, a relative of VASP and Drosophila Enabled, is implicated in the control of microfilament dynamics. 1996, Pubmed
Ghisolfi-Nieto, Nucleolin is a sequence-specific RNA-binding protein: characterization of targets on pre-ribosomal RNA. 1996, Pubmed
Hecht, Molecular mechanisms of male germ cell differentiation. 1998, Pubmed
Hudson, Xpat, a gene expressed specifically in germ plasm and primordial germ cells of Xenopus laevis. 1998, Pubmed , Xenbase
Imai, The neural RNA-binding protein Musashi1 translationally regulates mammalian numb gene expression by interacting with its mRNA. 2001, Pubmed
Jansen, RNA-cytoskeletal associations. 1999, Pubmed
Jiao, Identification of target messenger RNA substrates for the murine deleted in azoospermia-like RNA-binding protein. 2002, Pubmed
Kajita, The UUAG-specific RNA binding protein, heterogeneous nuclear ribonucleoprotein D0. Common modular structure and binding properties of the 2xRBD-Gly family. 1995, Pubmed
Linnen, Two related localized mRNAs from Xenopus laevis encode ubiquitin-like fusion proteins. 1993, Pubmed , Xenbase
Lowman, On the recognition of helical RNA by cobra venom V1 nuclease. 1986, Pubmed
López de Heredia, mRNA localization and the cytoskeleton. 2004, Pubmed
Melton, Translocation of a localized maternal mRNA to the vegetal pole of Xenopus oocytes. , Pubmed , Xenbase
Mowry, Vegetal messenger RNA localization directed by a 340-nt RNA sequence element in Xenopus oocytes. 1992, Pubmed , Xenbase
Niebuhr, A novel proline-rich motif present in ActA of Listeria monocytogenes and cytoskeletal proteins is the ligand for the EVH1 domain, a protein module present in the Ena/VASP family. 1997, Pubmed
Pollard, Quantitative analysis of the effect of Acanthamoeba profilin on actin filament nucleation and elongation. 1984, Pubmed
Rebagliati, Identification and cloning of localized maternal RNAs from Xenopus eggs. 1985, Pubmed , Xenbase
Reijo, DAZ family proteins exist throughout male germ cell development and transit from nucleus to cytoplasm at meiosis in humans and mice. 2000, Pubmed
Reinhard, The proline-rich focal adhesion and microfilament protein VASP is a ligand for profilins. 1995, Pubmed
Ruggiu, The mouse Dazla gene encodes a cytoplasmic protein essential for gametogenesis. 1997, Pubmed
Scherly, Identification of the RNA binding segment of human U1 A protein and definition of its binding site on U1 snRNA. 1989, Pubmed , Xenbase
Scherly, Major determinants of the specificity of interaction between small nuclear ribonucleoproteins U1A and U2B'' and their cognate RNAs. 1990, Pubmed , Xenbase
Steger, Haploid spermatids exhibit translationally repressed mRNAs. 2001, Pubmed
Tanaka, Imino proton NMR analysis of HDV ribozymes: nested double pseudoknot structure and Mg2+ ion-binding site close to the catalytic core in solution. 2002, Pubmed
Tsai, U1-snRNP-A protein selects a ten nucleotide consensus sequence from a degenerate RNA pool presented in various structural contexts. 1991, Pubmed
Tsui, Identification of two novel proteins that interact with germ-cell-specific RNA-binding proteins DAZ and DAZL1. 2000, Pubmed
Venables, The RNA-binding specificity of the mouse Dazl protein. 2001, Pubmed
Vera, Deleted in azoospermia associated protein 1 shuttles between nucleus and cytoplasm during normal germ cell maturation. 2002, Pubmed
Weeks, A maternal mRNA localized to the vegetal hemisphere in Xenopus eggs codes for a growth factor related to TGF-beta. 1987, Pubmed , Xenbase
Zhang, Xenopus VegT RNA is localized to the vegetal cortex during oogenesis and encodes a novel T-box transcription factor involved in mesodermal patterning. 1996, Pubmed , Xenbase
Zhao, A proline-rich protein binds to the localization element of Xenopus Vg1 mRNA and to ligands involved in actin polymerization. 2001, Pubmed , Xenbase
Zuker, On finding all suboptimal foldings of an RNA molecule. 1989, Pubmed