Tudor-SN Interacts with Piwi Antagonistically in Regulating Spermatogenesis but Synergistically in Silencing Transposons in Drosophila

Hsueh-Yen Ku; Vamsi K. Gangaraju; Hongying Qi; Na Liu; Haifan Lin

doi:10.1371/journal.pgen.1005813

Abstract

Piwi proteins associate with piRNAs and functions in epigenetic programming, post-transcriptional regulation, transposon silencing, and germline development. However, it is not known whether the diverse functions of these proteins are molecularly separable. Here we report that Piwi interacts with Tudor-SN (Tudor staphylococcal nuclease, TSN) antagonistically in regulating spermatogenesis but synergistically in silencing transposons. However, it is not required for piRNA biogenesis. TSN is known to participate in diverse molecular functions such as RNAi, degradation of hyper-edited miRNAs, and spliceosome assembly. We show that TSN colocalizes with Piwi in primordial germ cells (PGCs) and embryonic somatic cells. In adult ovaries and testes, TSN is ubiquitously expressed and enriched in the cytoplasm of both germline and somatic cells. The tsn mutants display a higher mitotic index of spermatogonia, accumulation of spermatocytes, defects in meiotic cytokinesis, a decreased number of spermatids, and eventually reduced male fertility. Germline-specific TSN-expression analysis demonstrates that this function is germline-dependent. Different from other known Piwi interters, TSN represses Piwi expression at both protein and mRNA levels. Furthermore, reducing piwi expression in the germline rescues tsn mutant phenotype in a dosage-dependent manner, demonstrating that Piwi and TSN interact antagonistically in germ cells to regulate spermatogenesis. However, the tsn deficiency has little, if any, impact on piRNA biogenesis but displays a synergistic effect with piwi mutants in transposon de-silencing. Our results reveal the biological function of TSN and its contrasting modes of interaction with Piwi in spermatogenesis, transposon silencing, and piRNA biogenesis.

Author Summary

Piwi proteins bind to a large class of small noncoding RNAs called Piwi-interacting RNAs (piRNAs). These proteins have emerged as major players in germline development, stem cell self-renewal, transposon silencing, and gene regulation. However, it is not known whether these functions of Piwi proteins represent separate molecular mechanisms. Furthermore, although multiple Piwi interactors have been identified, including Tudor-domain-containing proteins, none of them regulates Piwi expression or interacts with Piwi antagonistically, or only impact on a subset of Piwi functions. Here we show that Drosophila Piwi interacts with a special Tudor-domain-containing protein called Tudor-SN (Tudor staphylococcal nuclease, TSN). TSN is drastically different from the known Piwi interactors because it represses Piwi mRNA and protein expression and interacts with Piwi antagonistically in spermatogenesis but synergistically in transposon silencing. However, this interaction is not required for piRNA biogenesis. Our study represents the first demonstration that different functions of Piwi are mediated by different molecular mechanisms. In addition, this is the first in vivo study that reveals the biological function of TSN protein in an organism.

Citation: Ku H-Y, Gangaraju VK, Qi H, Liu N, Lin H (2016) Tudor-SN Interacts with Piwi Antagonistically in Regulating Spermatogenesis but Synergistically in Silencing Transposons in Drosophila. PLoS Genet 12(1): e1005813. https://doi.org/10.1371/journal.pgen.1005813

Editor: Xuemei Chen, University of California Riverside, UNITED STATES

Received: March 17, 2015; Accepted: December 23, 2015; Published: January 25, 2016

Copyright: © 2016 Ku et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

Data Availability: All piRNA files files are available from the NCBI SRA database (accession number PRJNA307580).

Funding: This work was supported by the NIH (DP1CA174418) and a G. Harold & Leica Y. Mathers Award <http://www.mathersfoundation.org/> to HL and an NIH Pathway to Independence Award K99ES021736 to VKG. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

Competing interests: The authors have declared that no competing interests exist.

Introduction

PIWI proteins are a subfamily of the PIWI/ARGONAUTE protein family. Piwi proteins associate with Piwi-interacting RNAs (piRNAs) and function in germline stem cell (GSC) self-renewal, germline development, epigenetic programming, post-transcriptional regulation, and transposon silencing [1–3]. The defining member of the Piwi/AGONAUTE family is the Piwi protein in Drosophila (PIWI herein stands for the subfamily whereas Piwi specifically stands for the Drosophila Piwi protein), which is known to regulate GSC maintenance, germ cell proliferation, heterochromatin formation, and transposon silencing [4–8]. However, it is not known whether the diverse functions of these proteins are molecularly separable; nor it is known whether all Piwi functions are piRNA-dependent. Furthermore, although Piwi proteins are known to interact with multiple proteins, including Tudor-domain-containing proteins, no interactor is known to regulate Piwi expression or interacts with Piwi antagonistically, or only impact on only a subset of Piwi functions.

Here we report that Tudor-SN (Tudor staphylococcal nuclease, TSN), a member of the evolutionarily conserved Tudor protein family, as a novel and unique Piwi-interactor in Drosophila. TSN contains five staphylococcal nuclease-like domains (SN1-SN5) and a methyl lysine/arginine recognizing Tudor domain [9–11]. TSN is highly conserved during evolution from fission yeast to mammals, and it exists as a single gene in a species with no close homologue [12]. TSN has been reported to participate in a variety of molecular functions, such as transcriptional activation through interacting with STATs, formation of RNA-induced silencing complex (RISC) and stress granules, degradation of A-to-I hyper-edited miRNAs, and assembly of spliceosome [13–19]. In mice and humans, TSN (a.k.a. SND1) has been demonstrated to interact with mouse and human PIWI proteins MIWI and MILI via binding to the symmetrically dimethylated arginine (sDMA) resides in the PIWI proteins [20, 21], similar to other Tudor family proteins [20, 21]. In Drosophila, although Tudor protein family members, including PAPI (Partner of PIWIs) have been shown to interact with PIWI proteins via sDMA residues [22], TSN has not been demonstrated to interact with PIWI proteins. Moreover, the biological role of TSN has not been explored in any organism.

Here we report the biological function of TSN in Drosophila, its interaction with Piwi, and the regulatory effect of such interaction. We show that TSN is highly expressed in embryos and adult gonads. In testes, tsn mutations result in abnormal spermatogenesis, including a higher mitotic index of spermatogonia, drastically increased number of spermatocytes, defects in meiotic cytokinesis, a reduction in spermatids, and consequently a decline in male fertility. Furthermore, the phenotype of tsn mutants is rescued by the mutations of piwi, indicating an antagonistic relationship of TSN and Piwi in the germline during spermatogenesis. In support of this, we show that TSN down-regulates the expression of Piwi at both protein and RNA levels. Finally, we demonstrate that tsn mutants display little impact on the piRNA biogenesis but have synergistic impact with Piwi on transposon repression. Our data suggest that TSN negatively regulates piwi expression in germline development while it may work with the Piwi protein in piRNA biogenesis and transposon silencing.

Results

TSN is a novel Piwi interactor

In an attempt to identify novel molecular interactors of Piwi, we previously reported the fractionation of cytoplasmic extracts of 0–12 h w¹¹¹⁸ wild-type embryos using size-exclusion chromatography [23]. After the final chromatography column, Piwi migrated with an apparent molecular weight of ~150 kDa. We resolved the peak fraction for Piwi obtained from Superdex 200 chromatography on a 7.5% SDS polyacrylamide gel and stained it with silver stain. We obtained the identities of individual bands by excising bands from a gel stained with colloidal coomassie blue, followed by mass spectrometry [23]. Piwi-Hsp90 interaction was described in our earlier paper [23]. Here we report that TSN, an evolutionarily conserved Tudor protein family member, is another novel Piwi-interacting protein. TSN contains five staphylococcal nuclease-like domains (SN1-SN5) and a methyl lysine/arginine-recognizing Tudor domain (Fig 1A). To confirm Piwi and TSN interaction, we performed co-immunoprecipitation assays using 0–12 h wild-type embryos. Piwi was immunoprecipitated with TSN, and the interaction was further confirmed by reciprocal co-immunoprecipitations, suggesting that Piwi and TSN form a complex in vivo (Fig 1B and 1C and S1 Fig). Moreover, immunofluorescence microscopy in 0–2 h wild-type embryos revealed that Piwi is co-localized with TSN in the cytoplasm and nuclei of PGCs as well as in the nuclei of somatic cells (Fig 1D–1H). Taken together, our results suggest that Piwi and TSN physically interact during embryogenesis.

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Fig 1. TSN is a novel Piwi-interacting protein.

(A) Schematic depiction of protein domain structures of TSN. TSN contains five staphylococcal nuclease-like domains (SN1-SN5) and a methyl lysine/arginine recognizing Tudor domain. (B) Co-immunoprecipitations of Piwi and TSN with anti-Piwi antibody. Input was the cytoplasmic fraction of the lysates from 0-12h WT embryos. 5% of input was used in the Western blot analysis. IgG was used as the control. F.L., flow-through; IP, immunoprecipitates. (C) Reciprocal co-immunoprecipitations of TSN and Piwi with mouse anti-TSN antibody. Input was the cytoplasmic fraction of lysates from 0–12 h WT embryos. 10% of input was used in the Western blot analysis. IgG was used as controls for the co-immunoprecipitations. F.L., flow-through; IP, immunoprecipitates. (D-F‴) Immunostaining of Piwi (green), TSN (using rabbit anti-TSN-N antibody, red), and the germ cell marker VASA (purple) in 0-1h WT embryos. DNA was labeled by DAPI (blue). (D-D‴) The whole embryo. PGCs, primordial germ cells. (E-E‴) Magnified images of E-E‴ showing the region of PGCs. Piwi and TSN were both highly enriched in the cytoplasmic region of PGCs. (F-F‴) Magnified images of D-D‴ showing the somatic cells. Piwi and TSN were both localized to the somatic nuclei. (G) Co-immunostaining of Piwi and TSN in PGCs, merged image of E and E’. (H) Co-immunostaining of Piwi and TSN in somatic cells, merged image of F and F’.

https://doi.org/10.1371/journal.pgen.1005813.g001

TSN expression during development

To investigate the biological function of TSN, we first analyzed the expression of TSN in different tissues and at key stages of development. Western blot analysis indicated that TSN is widely expressed in most developmental stages with the highest expression levels in embryos, adult ovaries and testes (Fig 2A). In addition, we used immunofluorescence microscopy to examine the expression pattern and subcellular localization of TSN in wild-type adult ovaries and testes. TSN is expressed in both the germline and somatic cells, from the germarium to advanced stage egg chambers (Fig 2B–2B”), where TSN is mainly present in the cytoplasm (Fig 2C–2D”). TSN is also expressed throughout spermatogenesis (Fig 2E) in both germ cells (labeled by VASA staining in Fig 2E’) and somatic cells (labeled by Tj staining in Fig 2E”), where TSN was also highly enriched in the cytoplasm (Fig 2F–2F”” and 2G–2G‴). As previously reported [5], Piwi is expressed in the nuclei of hub cells, early germ cells and somatic cyst cells (Fig 2G’ and 2G‴).

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Fig 2. TSN is highly expressed in embryos and adult gonads.

(A) Expression pattern of TSN protein in different key developmental stages and tissues. Western blot analysis using mouse anti-TSN antibody revealed that TSN was highly expressed in the embryonic stage as well as adult ovaries and testes. (B-D”) Immunostaining of TSN (using mouse anti-TSN antibody, green) in adult WT ovaries. DNA was labeled by DAPI (blue). TSN was localized to the cytoplasm of both germline and somatic cells in adult ovaries. G, germarium; S1-S5, stage 1–5 egg chambers, respectively; TF, terminal filament. (C-C”) Magnified images of a germarium including a S1 egg chamber. (D-D”) Magnified images of B-B” showing the S3 egg chamber. (E-F””) Immunostaining TSN (using mouse anti-TSN antibody, green) in WT adult testes. Germ cells were labeled with anti-VASA antibody (red) and somatic cells were labeled with anti-Tj antibody (purple). DNA was labeled by DAPI (blue). TSN was localized to the cytoplasm of germline and somatic cells in adult testes. Magnified images of the apical region of the testis are shown in F-F””. (G-G‴) Immunostaining of TSN (green) and Piwi (red) in WT adult testes. DNA was labeled by DAPI (blue). Piwi was localized in the nuclei of hub cells, early germ cells and somatic cyst cells. Asterisk: the hub.

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TSN is required in the germline for proper spermatogenesis

To determine the biological role of TSN, we first examined five ethyl-methane sulfonate (EMS) mutant alleles of TSN obtained from the Fly TILLING [24] for their molecular lesions. The tsn⁰⁵³⁶ and tsn⁰⁶¹⁴ are point mutations (282Ile→Phe and 320 Glu→ Lys, respectively) in the SN2 domain. The tsn⁰²⁵¹ and tsn¹²³⁶ are point mutations (368Gly→Glu and 501Gly→Arg, respectively) in the SN3 domain. The tsn¹¹²⁰ mutation is a deletion from +3009(A) to +3067(G) (per FlyBase coordinate of CG7008) that causes a frame shift from 437Ile on (Fig 3A). To determine whether tsn mutant alleles affect protein stability, we analyzed the protein level of TSN using the testicular lysates from each mutant allele transheterozygous to a deficiency (Df) allele uncovering the tsn genomic region. We found that TSN protein levels were undetectable in tsn ¹¹²⁰/Df mutants (Fig 3B). Moreover, antibodies recognizing epitopes in the N- or C-terminal region of TSN failed to recognize detectable protein levels in tsn ¹¹²⁰/Df testes, indicating that tsn ¹¹²⁰ is a protein-null allele.

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Fig 3. Mutations of tsn result in abnormal spermatogenesis.

(A) The EMS mutant alleles of tsn. The position of each mutation is indicated by an arrow above a schematic representation of the TSN protein. tsn⁰⁵³⁶ and tsn⁰⁶¹⁴ are point mutations at 282Ile→Phe and 320Glu→Lys of the SN2 domain, respectively. tsn⁰²⁵¹ and tsn¹²³⁶ are point mutations at 368Gly→Glu and 501Gly→Arg of the SN3 domain, respectively. tsn¹¹²⁰ is a deletion mutation which causes frameshift from 437Ile of the SN3 domain. (B) TSN protein expression level in the adult testes of each mutant allele heterozygous with a deficiency (Df) that disrupts the TSN genomic locus was analyzed by Western blots. TSN was undetectable in the lysates from tsn¹¹²⁰/Df testes. (C-H) Immunostaining of TSN (using mouse anti-TSN antibody, green) and VASA (red) in the testes from the five tsn mutant alleles heterozygous with the Df allele. DNA was labeled by DAPI (blue). tsn⁰⁶¹⁴/Df (F), tsn¹¹²⁰/Df (G), and tsn¹²³⁶/Df (H) resulted in the swollen apical tip of the testis. TSN was barely detectable in the tsn¹¹²⁰/Df testis (G). tsn⁰²⁵¹/Df (D) and tsn⁰⁵³⁶/Df (E) did not cause obvious testicular phenotype compared to the WT testis (C).

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To further examine the role of TSN in spermatogenesis, we performed immunostaining of 2-day-old mutant testes. Testes in tsn⁰²⁵¹/Df and tsn⁰⁵³⁶/Df mutants (Fig 3D and 3E) were similar to tsn⁺/tsn⁺ control testes (Fig 3C), suggesting these mutations fail to disrupt TSN function. However, tsn⁰⁶¹⁴/Df, tsn ¹¹²⁰/Df, and tsn¹²³⁶/Df alleles resulted in the swollen apical tips of testes containing an excessive number of early spermatogenic cells, with 42% (n = 84), 86% (n = 81), and 36% (n = 70) of the testes displaying this phenotype, respectively (Fig 3F–3H). Notably, TSN immunostaining signal was undetectable in tsn ¹¹²⁰/Df testes (Fig 3G), consistent with the result of our Western blot analysis (Fig 3B). In addition, we analyzed 2-day-old tsn ¹¹²⁰/tsn⁰⁶¹⁴, tsn ¹¹²⁰/tsn ¹²³⁶, and tsn ⁰⁶¹⁴/tsn¹²³⁶ transheterozygous males. Interestingly, testes from all of the three transheterozygous mutants exhibited the swollen apical tips, with 81% (n = 80), 78% (n = 79), and 45% (n = 71) of the testes displaying the phenotype, respectively. The knockdown of TSN using Actin5c-Gal4 driver (S2 Fig) also showed phenotype similar to tsn¹¹²⁰/tsn⁰⁶¹⁴ transheterozygous mutant, though at a lower frequency (36%, n = 42) (S2 Fig). The lower penetrance (compared to that of tsn ¹¹²⁰/tsn ⁰⁶¹⁴ transheterozygous mutant) may due to the modest knockdown efficiency of TSN in testes (S2 Fig). Although the knockdown efficiency of TSN in ovaries is much stronger, we did not observe any obvious defects in TSN knockdown ovaries (S3 Fig) or tsn¹¹²⁰/tsn⁰⁶¹⁴ transheterozygous mutant ovaries (S4C Fig). Together, these data indicate that tsn is required for normal progression of spermatogenesis but not oogenesis.

To determine whether the function of tsn in spermatogenesis is germline-dependent, we expressed wild-type TSN in germ cells using nosVP16-Gal4 driver (see Materials and Methods). This expression rescued the swollen testis apical tip phenotype of 68% of the tsn¹¹²⁰/tsn⁰⁶¹⁴ transheterozygous mutants to WT-like (n = 62; S5A Fig), indicating that the tsn function in spermatogeneis is germline-dependent.

tsn mutant testes display over-proliferation of spermatogonia and compromised differentiation of spermatocytes

To further investigate the spermatogenic defects of tsn mutants, we immunostained mutant testes from 2-day-old tsn ¹¹²⁰/tsn ⁰⁶¹⁴ transheterozygote males with VASA as a germ-cell marker, Hu-Li Tai Shao (Hts) as a fusome marker, and DAPI as a DNA marker. Fusome is a germline-specific organelle containing membrane skeletal proteins and connecting differentiating germ cells within a germline cyst [25]. In the testis, it connects spermatocytes derived from a single gonialblast (the differentiated daughter cell of a spermatogonial stem cell). The majority of cells in the swollen apical tip were VASA positive (Fig 4A, red) with branched fusomes (Fig 4A, arrow head) and faint DNA staining signal, indicating that these excessive number of early spermatogenic cells were likely spermatocytes. In addition, we found a few bundles of elongated spermatids with their heads resided at the apical tip of the testis. 62% of the testes examined displayed this phenotype (n = 42; Fig 4A, arrow), in contrast to their normal localization at the basal region of the testis. In order to assess whether the excess spermatocytes in tsn mutants are resulted from the defects in GSCs, we examine the number of GSC located next to the hub, the somatic niche of GSCs in testes. The average number of GSCs per tsn mutant testes was 6.5 (n = 12), which was similar to that in wildtype control testes (6.67, n = 12), even though all the mutant testes displayed the swollen tip phenotype (S6 Fig). This result indicates that the spermatocyte expansion phenotype of tsn mutants is not caused by abnormal GSC number.

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Fig 4. tsn mutations cause spermatogenic cell overproliferation, cytokinetic defects during meiosis, fewer spermatid bundles, and reduced male fertility.

(A) The apical tip region of 2-day-old adult tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant testes. Testes were stained with anti-VASA (germ cell, red) and anti-Hts (fusome, green) antibodies. DNA was labeled by DAPI (blue). The swollen apical tip of the mutant testis was filled with VASA-positive germ cells containing branched fusomes (arrow head) and faint DNA staining, indicating these cells are spermatocytes. A few bundles of elongated spermatids with their heads (arrow) resided at the apical tip of the mutant testis, in contrast to their normal localization at the basal region of the testis. Asterisk: the hub. (B) Phase contrast images of round spermatids from adult WT (left) and tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant (right) testes. In mutant testes, round spermatids containing a single Nebenkern (mitochondrial derivates) associated with two haploid nuclei were observed, indicating there were meiotic cytokinesis defects (see text). (C) The quantification of spermatid bundle number in 2-week-old adult testes revealed that tsn¹¹²⁰/tsn⁰⁶¹⁴ mutants had fewer spermatid bundles compared to the WT. (D-E) The third instar larval testes of WT and tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant were immunostained with anti-phospho-histone3 (pH3, mitotic index, red) and anti-Hts (fusome, green) antibodies. DNA was labeled by DAPI (blue). Asterisks indicate the hubs. The tsn mutant testis had more pH3-positive spermatogonia and was larger in size. (F) The quantification of pH3-positive spermatogonia per testis. The WT testes showed an average of 2.56 pH3-positive cells per testis (n = 27) and the tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant had an average of 3.44 pH3-positive cells per testis (n = 27) (see text). (G) The fertility of tsn mutant (red line) and WT (blue line) males. Initially, the tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant males showed a similar fertility as the WT controls, but the fertility was decreased faster over time compared to the WT males. Error bars represent mean ± standard error of the mean ((C) and (F) N ≧ 27; (G) N≧ 3). ** denotes P<0.01. The differences between WT and tsn mutant males In (G), p = 0.0000437 (by t-test) for the differences between WT and tsn mutant males.

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To determine whether the excess spermatocytes are due to a higher proliferation rate of spermatogonial cells, we immunostained tsn mutant third instar larval testes with anti-phospho-histone-3 (pH3) antibody to examine the mitotic index of spermatogonia. The mutant third instar testes show a higher mitotic index of spermatogonia and are already larger than tsn⁺/tsn⁺ wild-type larval testis, even though the mutant spermatogonia are similar in size to those in wild-type larval testes (cf. Fig 4D and 4E). Quantification revealed that the wild-type testes exhibited an average of 2.56 pH3-positive spermatogonia per testis (n = 27), yet the mutant testes had an average of 3.44 pH3-positive spermatogonia per testis (n = 27) (Fig 4F). The higher mitotic index of spermatogonia can be caused by two possibilities: a reduced differentiation from spermatogonia to spermatocyte and/or higher proliferation rate of spermatogonia. In the former case, the number of spermatocytes would decrease because the germ cells would be arrested at the spermatogonial stage. However, we did not observe a reduction of spermatocytes in tsn mutant testes. Thus, the higher mitotic index of spermatogonia indicates that there is likely a higher proliferation rate of spermatogonia in tsn mutant testes.

To further determine whether TSN regulates later stages of spermatogenesis, we used phase contrast microscopy to examine onion-stage spermatids in freshly squashed tsn mutant testes. In wild-type testes, each round spermatid contained a Nebenkern (mitochondrial derivates, Fig 4B, left panel, dark sphere) associated with a haploid nucleus (Fig 4B, left panel, white sphere). However, in 24% (n = 58) of tsn mutant testes, approximately 30% of round spermatids contain a single over-sized Nebenkern associated with two haploid nuclei (Fig 4B, right panel), indicating that these tsn mutant spermatids have succeeded in nuclear division but fail in proper cytokinesis. To assess if the spermatogenic defects are more severe in aged files, we examined the spermatid bundle numbers of 2-week-old mutant testes. The average numbers of spermatid bundle in wild-type and tsn mutants were 12.33 (n = 27) and 8.85 (n = 27), respectively. The reduction of spermatid bundles in the tsn mutants was significant (p = 2.24E-09, Fig 4C). This decreased instead of increased number of spermatid bundles in tsn mutant flies indicates that spermiogenesis (the process of spermatid morphogenesis) may be delayed and/or partially blocked in the mutants. Taken together, these results indicate that the tsn mutant testes likely have a higher proliferation of spermatogonia but a compromised differentiation of spermatocytes.

To evaluate the impact of these spermatogenic defects on fertility, we analyzed the fertility of tsn mutant males by crossing them to w¹¹¹⁸ virgin females. Initially, the mutant males showed relatively normal fertility, but their fertility was decreased faster over time as compared to the control tsn⁺/tsn⁺ wild-type males (Fig 4G), causing a significantly reduced male fertility (P = 4.38E-05), as expected from their compromised spermatogenesis. Expression of one copy of wild-type tsn gene in germ cells using nosVP16-Gal4 driver in tsn mutant males rescued their fertility to 74% of wildtype males at 2wk-old age, as effective as introducing one copy of the endogenous wildtype tsn gene (on the TM3 balancer) into the tsn mutant background (S5B Fig). These results indicate the germline-dependence of tsn function in the testis. In addition, these results indicate the dose-dependence of the TSN function in spermatogenesis.

To further study the dose-dependence of TSN in spermatogenesis, we overexpressed TSN in either germline cells or all cells in wildtype testes and examined the potential phenotypical consequence (S8 and S9 Figs). No obvious abnormality was observed, except that only a slight increase of hub cells number was observed in Actin-gal4>Flag-tsn testes (S8 and S9B Figs). Hence, increasing TSN level to more than wildtype level does not generate more impact on germ cell differentiation.

Piwi and TSN antagonistically interact in the germline to regulate spermatogenesis

To investigate the biological significance of TSN and Piwi interaction in regulating spermatogenesis, we examined the phenotype of the piwi and tsn double mutants. We focused on piwi¹ and piwi² mutant alleles, which are strong recessive mutations of piwi [5, 6]. Remarkably, we found that introducing one or two copies of either piwi¹ or piwi² mutant alleles into the tsn mutant background rescued tsn mutant phenotype in a dosage-dependent manner (Fig 5A–5C). We categorized the phenotype into three classes based on the extent of swollen apical tip of the testis: severe (as shown in Fig 5A), moderate (as shown in Fig 5B), and WT-like (as shown in Fig 5C) phenotype. In tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant testes, only 5% of the testes showed WT-like morphology, 14% of the testes had moderate phenotype, and 81% of the testes displayed severe phenotype. However, introducing one copy of piwi¹ allele resulted in 18% and 63% of the testes showing WT-like and moderate phenotype, respectively. Introducing piwi¹/piwi² alleles led to 54% and 41% testes showing WT-like and moderate phenotype, respectively (Fig 5D). Moreover, the fertility of tsn mutants (Fig 5E, red line) was also restored by piwi mutations (Fig 5E, green line). Interestingly, Western blot and quantitative RT-PCR (qRT-PCR) analyses revealed that the protein and mRNA expression levels of piwi were upregulated in tsn mutant testes (Fig 5F and 5G). Immunostaining of Piwi in tsn mutant testes further showed that the expression pattern of Piwi did not change compared to that in the control (S7 Fig). Therefore, the upregulation of Piwi is not due to ectopic expression of Piwi, but is mostly, if not completely, due to increased Piwi expression within its expressing cells. Consistently, overexpression of TSN with actin5c-Gal4 driver in testes leads to slight decrease in Piwi expression, with no effect in Piwi localization (S9 Fig). The antagonistic interactions between Piwi and TSN at both genetic and molecular levels together define a functionally antagonistic relationship between TSN and Piwi in spermatogenesis.

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Fig 5. TSN antagonizes Piwi during spermatogenesis.

(A-C) Immunostaining of Hts (green) and VASA (red) in testes from tsn mutants, and piwi and tsn double mutants. The defects of tsn mutant testes were rescued by piwi mutations in a dosage-dependent manner. (D) Quantification of the results in A-C. The phenotype is categorized into three classes: WT-like (as shown in C), moderate (as shown in B), and severe (as shown in A) phenotype. In tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant testes, only 5% of the testes displayed WT-like phenotype, 14% of the testes revealed moderate phenotype, and 81% of the testes showed severe phenotype. However, introducing one copy of piwi¹ resulted in 18% and 63% of the testes showing WT-like and moderate phenotype, respectively. Introducing piwi¹/piwi² led to 54% and 41% of the testes showing WT-like and moderate phenotype, respectively. (N≧50 for each of the genotypes) (E) Fertility assay of piwi and tsn double mutant males. The reduced fertility of tsn mutant males (red line) was restored by introducing piwi mutations to the tsn mutant background (green line). The fertility of WT males is shown as the blue line. (F) Western blot analysis of Piwi expression level in piwi mutant, tsn mutant, and piwi and tsn double mutant testes. Piwi protein level was upregulated in tsn mutant testes, suggesting a negative regulation of TSN on Piwi expression. (G) qRT-PCR of Piwi and TSN in piwi mutant, tsn mutant, and piwi and tsn double mutant testes. Piwi mRNA level was upregulated in tsn mutant testes, indicating TSN negatively regulates Piwi expression at the mRNA level. Error bars represent mean ± standard error of the mean (N ≧ 3). **P<0.01.

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Interestingly, we observed similar regulatory relationship of Piwi and TSN in the ovary. Although tsn mutant ovaries did not show any obvious oogenesis defects (S4C Fig), the germline-depletion phenotype of piwi mutants (S4B Fig) was partially restored by introducing the mutations of tsn (S4D Fig). Furthermore, Piwi protein and mRNA expression levels were both significantly upregulated in the tsn mutant ovaries (S10 Fig), suggesting the antagonistic interaction between Piwi and TSN is conserved in spermatogenesis and oogenesis. Because TSN is involved in RNA metabolism [14–18], we performed TSN RNA immuneprecipitation using Flag antibody to examine if TSN binds to Piwi mRNA (see Materials and Methods). Piwi mRNAs are enriched more than 7-fold using two different sets of piwi primers (S10C Fig). These results together indicate that TSN regulate Piwi expression likely by directly binding to its mRNA.

As Piwi is expressed in both germline and somatic cells, we next asked whether TSN antagonizes the germline or the somatic function of Piwi. To address this question, we used nosVP16-Gal4 (germline) and tj-Gal4 (somatic) drivers to knockdown Piwi tissue-specifically in the tsn mutant background. Germline knockdown of Piwi rescued tsn mutant phenotype (72% of the testes examined were WT-like, n = 75; Fig 6); however, somatic depletion of Piwi did not (S11 Fig). These results suggest that TSN antagonizes the function of Piwi in germ cells to regulate spermatogenesis.

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Fig 6. TSN antagonizes the germline function of Piwi.

The testes were stained with anti-Piwi (green), anti-VASA (germ cell, red), and anti-Tj (somatic cells, purple) antibodies. DNA was labeled by DAPI (blue). (A-A‴) Germline knockdown of Piwi using nosVP16-Gal4 driver. (B-B‴) The tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant displayed a swollen apical tip of the testis. (C-C‴) The depletion of Piwi in germ cells rescued tsn mutant phenotype, suggesting TSN antagonizes the germline function of Piwi in regulating spermatogenesis.

https://doi.org/10.1371/journal.pgen.1005813.g006

TSN synergistically interacts with Piwi to silence transposons but has little role in piRNA biogenesis

Because Piwi plays an important role in the piRNA pathway [2], we wanted to know whether TSN regulates piRNA biogenesis and functions. To address this question, we first sequenced small RNA libraries prepared from an equal quantity of two-day-old tsn⁺/tsn⁺ wild-type and tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant testes. The composition of small RNA libraries from wild-type and tsn mutant testes are shown in Fig 7A. The size distribution profiles of small RNAs (excluding miRNAs and fragments of long cellular RNAs such as tRNAs and rRNAs) from wild-type and tsn mutant testes are shown in Fig 7B. It revealed that the tsn mutant testes have essentially identical piRNA profiles (Fig 7B). Moreover, the 1U-bias of piRNAs (a strong U bias at the most 5’ position) and the nucleotide composition were well maintained in the tsn mutants (Fig 7C). We further mapped all of the small RNAs to known piRNA clusters, and only clusters 4 and 7 showed ~3-fold upregulation in tsn mutants (Fig 7D). However, we noticed that relatively few deep sequence reads mapped to these two clusters, so the 3-fold increase could be due to or contributed by fluctuation in reads. These data indicate that, unlike Piwi, TSN either is not involved in piRNA biogenesis or plays only a very minor role in this process.

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Fig 7. TSN shows only subtle effects on piRNAs and transposon silencing.

(A) Small RNA composition in the WT (left) and tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant (right) testes. TE RNA, small RNAs derived from transposon regions; gene RNA, small RNAs derived from gene-coding regions; intergenic RNA, small RNAs derived from intergenic regions. (B) Size distribution of small RNAs (excluding miRNAs and fragments of long cellular RNAs such as tRNAs and rRNAs) in the WT (blue) and tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant (red) testes. The level of 25-nt small RNAs was slightly decreased in the tsn mutants. (C) Nucleotide compositions of small RNAs (excluding miRNAs and fragments of long cellular RNAs such as tRNAs and rRNAs) in the WT (top) and tsn¹¹²⁰/tsn⁰⁶¹⁴mutant (bottom) testes. The 1U-bias piRNA signature and nucleotide composition were not affected in tsn mutants. (D) Relative abundance of small RNAs derived from 19 previously reported piRNA clusters in tsn mutant testes compared to the WT testes are shown. Small RNAs uniquely mapped to these clusters were used for this analysis. These clusters are categorized into three groups according to the expression preference of their piRNAs [39–41], with the germline-enriched class colored in red, the intermediate class colored in blue, and the soma-enriched class colored in orange. No strong impact of tsn mutations on these piRNA clusters was observed (see text). (E) qRT-PCR was performed to determine the expression of multiple transposons, relative to rp49, in tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant testes. Transcript levels from the WT testes were set as 1, and fold-changes are indicated. Error bars represent mean ± standard error of the mean (N = 3). tsn mutants showed very moderate defects in transposon silencing (see text).

https://doi.org/10.1371/journal.pgen.1005813.g007

To investigate whether TSN is involved in piRNA biogenesis in the ovary and to test whether the mild effect of tsn mutations on small RNAs in the testis is caused by altered abundance of different cell types in the mutant testis, we sequenced and analyzed small RNAs prepared from wild-type and tsn mutant ovaries. The total small RNA composition profiles were shown in S12A Fig. Similar to the results observed in testes, the size distribution profiles of small RNAs from wild-type and tsn mutant ovaries are not significantly affected (S12B Fig). The 1U-bias and nucleotide composition were not affected in the mutant ovaries, either (S12C Fig). We next examined the abundance of piRNAs generated from known piRNA clusters, and did not observe any strong effects of tsn mutations on these piRNA clusters (S12D Fig). Together, these results indicate that TSN has a minor role, if any, in piRNA biogenesis in both testes and ovaries.

To exclude the possibility that the compensation of other Piwi-interacting Tudor proteins may rescue the loss of TSN, we examine the expression level of Papi and Tudor [22] in tsn mutant testes, and did not detect significant difference in their expression (S13 Fig). Therefore, TSN unlikely to be directly involved in piRNA biogenesis.

Because a primary function of Piwi is to silence transposons [2], we next examined whether tsn mutations results in any transposon desilencing and whether TSN interacts with Piwi in regulating transposons. To this end, we analyzed the expression of transposons in wild-type, tsn mutant, piwi mutant, and piwi and tsn double mutant testes by qRT-PCR. Consistent with the only slight reduction of piRNAs in tsn mutant testes shown in Fig 7B, transposons were only mildly upregulated (~2-6X change) in the tsn mutants compared with the wild-type controls (Fig 7E). In contrast, the upregulation of transposons in the piwi mutant is more significant (~4-18X for most transposons and 120X and 385X for gtwin and gypsy, respectively; Fig 7E). Remarkably, in tsn; piwi double mutants, the transposon upregulation is even much more drastic (~13-62X for most transposons and 280X and 620X for gtwin and gypsy, respectively). Similar results were observed in ovaries (S12E Fig). These results indicate that TSN and Piwi interact synergistically in transposon silencing in both testes and ovaries.

Discussion

Piwi is a multifunctional protein and its deficiency leads to abolishment of GSC self-renewal, abnormalities in germ cell proliferation and differentiation, defects in piRNA biogenesis, derepression of transposons, and aberrant epigenetic programming (reviewed in [1, 2]). However, it has not been reported that these functions are separable. In addition, no negative interactor of Piwi proteins has been identified. Here we have identified TSN as a novel Piwi interactor that interacts with Piwi antagonistically and demonstrated that this interaction is only for spermatogenesis but not for piRNA biogenesis or transposon silencing. The tsn mutant testis exhibits phenotypic defects, including germline overproliferation, meiotic cytokinesis abnormality, and a reduced number of spermatids, all of which contribute to a decrease in the fertility of these mutant males (Fig 4). The opposite phenotype of piwi and tsn mutants in germ cell proliferation, together with the negative regulation of Piwi by TSN, indicate an antagonistic relationship between Piwi and TSN that is essential for spermatogenesis. In support of this, the phenotype of tsn mutants in spermatogenesis and fertility is rescued by piwi mutations (Fig 5A–5E). Because TSN negatively regulates the expression of piwi mRNA and Piwi protein in the testis (Fig 5F and 5G), it is likely that the antagonistic interaction happens at level of Piwi expression. Furthermore, this regulation occurs mostly, if not exclusively, in the germline, since TSN function is germline-dependent (S5B Fig) and tsn phenotype is rescued by germline-specific piwi knockdown (Fig 6).

It is worth noting that the TSN function in spermatogenesis is not only germline dependent but also dose-dependent. Tsn/+ testes show intermediate degrees of defects between tsn/tsn and +/+ testes. Furthermore, the nos-Gal4-driven expression of one copy of tsn gene rescues defects of tsn/tsn mutants to that of tsn/+ testes. However, over-expression of TSN in either the germline or the entire testis does not have detectable effect, which suggests that the dose-dependence is capped at the +/+ level.

Our study indicates that the antagonistic regulatory relationship between Piwi and TSN is conserved between spermatogenesis and oogenesis. TSN also negatively regulates the expression of piwi mRNA and Piwi protein in the ovary (S10 Fig). Furthermore, TSN binds to the piwi mRNA in the ovary (S10C Fig). These results also support that TSN antagonizes Piwi function at least in part by directly binds to its mRNA and suppress its expression.

Despite the strong interaction between TSN and Piwi, it is surprising that TSN does not have obvious effects on piRNA biogenesis (Fig 7). Although a simple explanation would be that spermatogenesis is more sensitive to the dose of Piwi than piRNA biogenesis. This is unlikely because Piwi expression is up-regulated in tsn mutant, yet Drosophila strains with four copies and even six copies of piwi are perfectly fertile and can be maintained as stocks [7]. Therefore, we favor an alternative possibility that the antagonistic protein-protein interaction between TSN and Piwi is needed for spermatogenesis but not for piRNA biogenesis,

It is surprising to observe that, despite the antagonistic interaction between TSN and Piwi, they have synergistic effect on transposon silencing. This might reflect that TSN and Piwi act through independent pathways that silence transposons (S14 Fig). In piwi mutants, transposons are significantly de-silenced, as previously reported by many. Interestingly, tsn mutants display a milder de-silencing effect. This is likely because Piwi is significantly up-regulated in tsn mutants, which partially compensated for the loss of TSN-mediated transposon repression. In tsn; piwi double mutants, both TSN and Piwi-mediated repression mechanisms are abolished, which leads to an even more drastic transposon repression that has not been reported. Thus, PIWI/piRNA-mediated mechanism is not the only mechanism involved in transposon repression. It would be important to investigate the TSN-mediated transposon silencing mechanism and to determine whether it depends on piRNA.

Relevantly, the Piwi-TSN protein interaction may only affect piRNA-independent function of Piwi such as miRNA regulation [7] or other unidentified roles of Piwi. Both TSN and Piwi have been implicated in the miRNA pathway [7, 26]. Since miRNAs play an important role during germline development, it would be intriguing to examine whether TSN interacts with Piwi to mediate miRNA regulation which in turn exerts different effects on spermatogenesis and transposon silencing. In any case, the above data allow us to conclude that the function of Piwi in spermatogenesis can be separated from piRNA biogenesis and transposon silencing.

It has been shown that the expression of human TSN (a.k.a., SND1) is upregulated in various human cancers such as colon, prostate, breast, and hepatocellular cancers [27–30]. In prostate cells, SND1 recruits splicing factor SAM68 and other spliceosomal components on CD44 pre-mRNA, promotes the inclusion of CD44 variable exons, which correlates with increased proliferation, motility, and invasiveness of cancer cells [27]. Moreover, SND1 interacts with Metadherin (MTDH) to promote metastasis and was also shown to promote resistance to apoptosis and to regulate the expression of genes associated with metastasis and chemoresistance [28]. However, both the function of TSN during normal development and the molecular mechanism of TSN in cancer cells still remain elusive. Importantly, PIWI proteins are also implicated in cancers [31–33]. Therefore, our study of TSN and Piwi interaction provides a possible mechanism in tumorigenesis, and it may be due to the multifunctional nature and the broad interacting partners and targets of TSN.

Materials and Methods

Drosophila stocks, transgene expression, and RNAi

All fly stocks were raised at 25°C on yeast-containing molasses/agar medium. Both yw and w¹¹¹⁸ flies were used as the wild-type controls. The tsn EMS mutant alleles were generated and screened using Fly TILLING [24]. The deficiency allele that disrupts the tsn genomic region, w¹¹¹⁸; Df(3L)BSC125/TM6B, Tb¹, was obtained from Bloomington Stock Center. The tsn RNAi strain HMS00184 was obtained from TRiP at Harvard. The knockdown of tsn was induced by Actin5C-Gal4 driver obtained from Bloomington Drosophila stock center. UASp-driven Flag-tagged tsn transgenic strains, carrying a functional tsn gene, were generated with standard protocols using pVALIUM10-roe vector from TRiP at Harvard. Germline-specific expression of the Flag-tagged tsn transgene was achieved by introducing nosVP16-Gal4 (Bloomington Drosophila stock center) and Flag-tagged tsn transgene in the tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant background. piwi¹ and piwi² alleles were generated by P-element insertions as previously described [5, 6]. The piwi RNAi strain w¹¹¹⁸; P{GD11827}v22235 was obtained from Vienna Drosophila RNAi Center. The knockdown of piwi was induced by nosVP16-Gal4 driver (Bloomington Drosophila stock center) and tj-Gal4 driver (Drosophila Genetic Resource Center).

Biochemical purification and identification of cytoplasmic Piwi interacting peptides

All chromatographic steps and mass spectrometry analysis were described previously [23].

Embryo extraction and Immunoprecipitation

Cytoplasmic extracts of w¹¹¹⁸ embryos were collected as described previously [23]. All steps in extract preparation were performed at 4°C. A total of 1 mg of total protein in a volume of 1 ml H(0.15) buffer (25 mM HEPES-NaOH, pH 7.8, 150mM NaCl, 0.5 mM EGTA, 0.1 mM EDTA, 2 mM MgCl2, 0.02% NP-40 and 20% glycerol) was used for each immunoprecipitation reaction. The lysates were pre-cleared using Protein A/G PLUS-Agarose (Santa Cruz) for 1h at 4°C. Pre-cleared lysates were incubated with the monoclonal mouse anti-Piwi antibody (a gift from M.C. Siomi)[34] or the monoclonal mouse anti-TSN antibody, a gift from O. Silvennoinen [35], overnight at 4°C with gentle agitation. 60 μl of beads were then added to the lysate-antibody mixture and incubated further for 3 h at 4°C. Beads were then washed five times with 1 ml of H(0.15) buffer at 4°C and finally analyzed by Western blotting.

Western blot analysis

For Western blot analysis, the following antibodies were used: monoclonal mouse anti-Piwi (1:200), a gift from M.C. Siomi [34], monoclonal mouse anti-TSN (1:5000), a gift from O. Silvennoinen [35], polyclonal rabbit anti-GAPDH antibody (1:5000, Sigma), polyclonal Guinea Pig anti-Papi antibody (1:5000) and polyclonal mouse anti-β-tubulin (1:10000, Developmental Studies Hybridoma Bank) antibodies. Peptides corresponding to the 26 residues of the N-terminal and the 27 residues of the C-terminal of Drosophila TSN were synthesized and used for generating polyclonal rabbit anti-TSN-N and anti-TSN-C antibodies, respectively (Cocalico Biologicals). Both antibodies were purified and used at 1:5000 dilution. The specificity of each anti-TSN antibody is shown in S1 Fig.

Immunostaining

The preparation of embryos, ovaries, and testes was performed as previously described [25, 36]. For immunofluorescence staining, the following primary antibodies were used: monoclonal mouse anti—Flag M2 (1:500; Sigma-Aldrich), monoclonal mouse anti-Piwi (1:20), a gift from M.C. Siomi [34], monoclonal mouse anti-TSN (1:500), a gift from O. Silvennoinen [35], polyclonal rabbit anti-VASA (1:400, Santa Cruz), polyclonal rabbit anti-Ser10-phospho-histone H3 (1:200, Cell Signaling), polyclonal rabbit anti-TSN-N and anti-TSN-C (both at 1:1000 dilution), polyclonal mouse anti-Hts (1:40, Developmental Studies Hybridoma Bank), and polyclonal guinea pig anti-Tj (1:100, a gift from D. Godt, University of Toronto) antibodies. Alexa Fluor -488, -568, or -633-conjugated goat anti-rabbit, anti-guinea pig, and anti-mouse IgG secondary antibodies were purchased from Jackson Immunoresearch Laboratory and were used at 1:400 dilution. Immunofluorescently labeled samples were counterstained with DAPI with standard protocol. Images were taken using Leica TCS SP5 Spectral Confocal Microscope in the sequential scanning mode and then processed using Photoshop (Adobe).

Live testicular squashes and phase contrast microscopy

Testes were dissected from 3-day-old adults in phosphate-buffered saline (PBS) and transferred into a 2-μL drop of PBS on a coverslip. The testes were then torn open using tungsten needles and slightly squashed by putting a slide over the coverslip. Phase contrast images of squashed testes were obtained using a Leica DM6000 microscope with a 40X objective.

Male fertility assay

Individual 2-day-old males of the indicated genotypes were crossed with three 2-day-old virgin w¹¹¹⁸ females. For every 3 days, each vial was visually examined to ensure eggs had been laid. The females were then discarded and each male was transferred to a new vial and mated with three 2-day-old virgin females. The number of adult progeny in each vial was counted on the 20^th day after each mating. A minimum of 15 males for each genotype was used for testing.

Small RNA cloning and analysis

Low-molecular-weight RNAs were isolated from the adult testes of w¹¹¹⁸ and tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant males (approximately 200 pairs for each genotype) using a mirVana miRNA isolation kit (Life Technologies). Small RNAs ranging in size between 16 and 29 nucleotides (nt) (below 2S rRNA) were gel-purified, and small RNA libraries were prepared using a small RNA sample prep kit (Illumina) according to the alternative v1.5 protocol. The clones were sequenced using Genome Analyzer II. Only sequences perfectly matching the Drosophila melanogaster release 5 genome (excluding Uextra) were analyzed. As TSN is known to regulate miRNAs [17], here we used the total reads instead of the reads of miRNAs to normalize the two libraries. After removal of miRNAs and fragments of long cellular RNAs such as tRNAs and rRNAs, we mapped 18–32-nt unique piRNAs to a subset of known piRNA clusters and to the complete collection of Drosophila melanogaster transposable elements (Repbase) [37].

Total RNA extraction and quantitative RT-PCR

Thirty pairs of testes were dissected from 2-day-old adults in ice-cold PBS. Total RNA was then extracted using TRIzol (Invitrogen) following manufacturers’ protocols. RNA was finally eluted in 30μl nuclease-free water and quantified by Nanodrop. 2 μg of eluted RNA was used to generate cDNA in a 20 μl reaction using High Capacity cDNA Reverse Transcription kit (Applied Biosystems).

Quantitative RT-PCR of the Piwi, TSN, and transposon transcripts was performed as previously described [38]. The following primer pairs were used- Piwi: forward (5’-TGCCATGAGCAGTTATACGC-3’) and reverse (5’-TGTCCA GTTCCATGTTCCAG-3’); TSN: forward (5’-GGCAACATGTGTTCGCTATC-3’) and reverse (5’- GTGGCGTTATCCTTCTTTGC-3’); 412: forward (5’-CACCGGTTTGGTCGAAAG-3’) and reverse (5’-GGACATGCCTGGTATTTTGG-3’); blood: forward (5’-TGCCACAGTACCTGATTTCG-3’) and reverse (5’-GATTCGCCTTTTACGTTTGC-3’); diver: forward (5’-GGCACCACATAGACACATCG-3’) and reverse (5’-GTGGTTTGCATAGCCAGGAT-3’); gtwin: forward (5’-TTCGCACAAGCGATGATAAG-3’) and reverse (5’-GATTGTTGTACGGCGACCTT-3’); gypsy: forward (5’-GTTCATACCCTTGGTAGTAGC-3’) and reverse (5’-CAACTTACGCATATGTGAGT-3’); HetA: forward (5’-CGCGCGGAACCCATCTTCAGA-3’) and reverse (5’-CGCCGCAGTCGTTTGGTGAGT-3’); invader1: forward (5’-GTACCGTTTTTGAGCCCGTA-3’) and reverse (5’-AACTACGTTGCCCATTCTGG-3’); max: forward (5’-TCTAGCCAGTCGAGGCGTAT-3’) and reverse (5’-TGGAAGAGTGTCGCTTTGTG-3’); mdg1: forward (5’-AACAGAAACGCCAGCAACAGC-3’) and reverse (5’-CGTTCCCATGTCCGTTGTGAT-3’); rt1a: forward (5’-CCACACAGACTGAGGCAGAA-3’) and reverse (5’-ACGCATAACTTTCCGGTTTG-3’); rp49: forward (5’-CCGCTTCAAGGGACAGTATCTG-3’) and reverse (5’-ATCTCGCCGCAGTAAACGC-3’).

Immunoprecipitation and quantitative RT-PCR of TSN-associated RNA

Adult testes from wildtype or actin5c-Gal4>UASp Flag-TSN were dissected in ice-cold PBS and homogenized in H(0.15) buffer. Testes lysates were collected by centrifugation at 10,000g for 30 min at 4°C. Immunoprecipitation was performed using mouse anti-Flag (Sigma) with Protein G magnetic beads (Invitrogen). Immunoprecipitates were washed five times with H(0.15) buffer at 4°C. Immunoprecipitated RNAs were then isolated from the immunopurified complexes with Trizol and precipitated with ethanol. Reverse transcription and qRT-PCR were then done following the protocol described above. Primer pairs used are the same as described above except piwi #2: forward (5’- TGCCATGAGCAGTTATACGC-3’) and reverse (5’- TGTCCAGTTCCATGTTCCAG-3’).

Supporting Information

S1 Fig. Specificity of anti-TSN antibodies.

Western blot analysis using the ovarian lysates prepared from tsn knockdown and control females. The blots were probed with polyclonal rabbit anti-TSN-N (left), polyclonal rabbit anti-TSN-C (middle), and monoclonal mouse anti-TSN (right) antibodies. TSN is ~100 kDa.

https://doi.org/10.1371/journal.pgen.1005813.s001

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S2 Fig. The knockdown of tsn resulted in the swollen apical tip of the testis.

(A) Western blot analysis using mouse anti-TSN antibody showing the knockdown efficiency of tsn in testes. (B) Testes from tsn knockdown and control males were immunostained with mouse anti-TSN antibody. DNA was labeled by DAPI (blue). The knockdown of tsn caused the swollen apical tip of the testis (see text). Arrow indicates a bundle of elongated spermatids with their heads resided at the apical tip region of the testis.

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S3 Fig. The knockdown of tsn did not cause any obvious phenotype in ovaries.

(A) Western blot analysis using mouse anti-TSN antibody showing the knockdown efficiency of tsn in ovaries. (B) Ovaries from tsn knockdown and control females were immunostained with mouse anti-TSN antibody. DNA was labeled by DAPI (blue). The knockdown of tsn did not generate any obvious defects in oogenesis.

https://doi.org/10.1371/journal.pgen.1005813.s003

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S4 Fig. TSN antagonizes Piwi during oogenesis.

Immunostaining of VASA (green) and Hts (red) and in ovaries from WT (A-A‴), piwi mutants (B-B‴), tsn mutants (C-C‴), and piwi and tsn double mutants (D-D‴). The defect of piwi mutant ovaries (B-B‴) was significantly rescued by tsn mutations (D-D‴). This antagonistic relationship between TSN and PIWI in oogenesis parallels that in spermatogensis (Fig 4A–4D).

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S5 Fig. Germline expression of tsn transgene rescued tsn mutant phenotype and fertility.

(A). Flag-TSN was expressed in germ cells by nosVP16-Gal4 in the tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant background. The testes were immunostained with anti-Flag (Flag-TSN), anti-Tj (somatic cells), and anti-VASA (germ cells) antibodies. DNA was labeled by DAPI (blue). Asterisk indicates the hub. tsn mutant phenotype was rescued by the expression of full-length WT TSN. (B). Fertility assay of piwi and tsn double mutant males. The reduced fertility of tsn mutant males (red line) was restored largely by expression of Flag-tagged TSN in the germline cells driven by VP16-NosGal4 driver at the tsn mutant background (gray line). The fertility of WT males is shown as the light blue line.

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S6 Fig. GSC number is normal in adult tsn mutant testes.

Germ cells were labeled with anti-VASA antibody (red) and DNA was labeled by DAPI (blue). The average numbers of GSCs in WT and tsn mutant testes was 6.67 (n = 12) and 6.5 (n = 12), respectively. There were no obvious abnormalities in GSCs of tsn mutant testes, suggesting the phenotype of tsn mutants may not be due to defects in GSCs.

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S7 Fig. The upregulation of Piwi caused by the mutations of tsn is within the Piwi-expressing cells.

Immunostaining of Piwi in testes from adult WT and tsn mutant males. DNA was labeled by DAPI. Piwi was expressed in early germ cells and somatic cyst cells in both WT and tsn mutant testes. This result suggests the upregulation of Piwi is in the Piwi-expressing cells, but not caused by ectopic expression of Piwi.

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S8 Fig. Overexpression of tsn in germ cells of the wildtype testis.

Germline-specific expression of the Flag-tagged tsn transgene was induced by nosVP16-Gal4 in w¹¹¹⁸ male flies. (A, B) Testes from 2-day-old males were immunostained with mouse anti-Flag M2 antibody. (A’, B’) DNA was labeled by DAPI (blue). (A”, B”) merged images for Flag and DAPI staining. Asterisks indicate the hubs. Overexpression of tsn in WT germ cells does not cause any obvious phenotype.

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S9 Fig. Overexpression of tsn in both germline and somatic cells of the wild-type testis.

Overexpression of Flag-tagged TSN was induced by Actin5C-Gal4 in w¹¹¹⁸ male flies. 2-day-old testes were used for the analysis. (A) Western analysis of TSN and Piwi. Overexpressed Flag-TSN was examined with mouse anti-Flag M2 antibody. Piwi expression level is slightly reduced in TSN overexpressed testes comparing to WT testes. (B) Immunostaining of Flag-TSN and Piwi in Flag-TSN overexpressing testes. DNA was labeled by DAPI (blue). Asterisks indicate the hubs. Piwi localization is normal while its expression level especially in somatic cyst cells is reduced.

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S10 Fig. TSN negatively regulates Piwi expression at the mRNA level in ovaries.

(A) Western blot analysis of Piwi expression level in piwi mutant, tsn mutant, and piwi and tsn double mutant ovaries. Piwi protein level was upregulated in tsn mutants, suggesting a negative regulation of TSN on Piwi expression. (B) qRT-PCR of Piwi and TSN in piwi mutant, tsn mutant, and piwi and tsn double mutant ovaries. Piwi mRNA level was upregulated in tsn mutant ovaries, indicating TSN negatively regulates Piwi expression at the mRNA level. (C). TSN binds to piwi mRNA in Drosophila ovaries. qRT-PCR to detect piwi mRNA (using two sets of primers: piwi and piwi#2) and tsn mRNA from RNA co-immunoprecipitated from wildtype and Flag-TSN overexpressing ovaries using anti-Flag antibody. Error bars represent mean ± standard error of the mean (N ≧ 3). *P < 0.05 and **P<0.01.

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S11 Fig. Somatic knockdown of Piwi does not rescue tsn mutant phenotypes.

The testes were immunostained with anti-Piwi (green), anti-VASA (germ cell, red), and anti-Tj (somatic cells, purple) antibodies. DNA was labeled by DAPI (blue). (A-A‴) Somatic Piwi was knockdown using tj-Gal4 driver. The knockdown of somatic Piwi resulted in an expansion of Piwi-expressing spermatogonial cells. (B-B‴) The tsn mutant testis. (C-C‴) The depletion of somatic Piwi did not rescue tsn mutant phenotype.

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S12 Fig. TSN shows little effects on piRNAs and transposon silencing in ovaries.

(A) Small RNA composition in ovaries from the WT (left) and tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant (right) females. TE RNA, small RNAs derived from transposon regions; gene RNA, small RNAs derived from gene-coding regions; intergenic RNA, small RNAs derived from intergenic regions. (B) Size distribution of small RNAs (excluding miRNAs and fragments of long cellular RNAs such as tRNAs and rRNAs) in the WT (blue) and tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant (red) ovaries. The level of 25-29-nt small RNAs was slightly decreased in the tsn mutants. (C) Nucleotide composition of small RNAs (excluding miRNAs and fragments of long cellular RNAs such as tRNAs and rRNAs) in the WT (top) and tsn¹¹²⁰/tsn⁰⁶¹⁴mutant (bottom) ovaries. The 1U-bias piRNA signature and nucleotide composition were not affected in tsn mutants. (D) Relative abundance of small RNAs derived from 19 previously reported piRNA clusters in tsn mutant ovaries compared to the WT ovaries are shown. Small RNAs uniquely mapped to these clusters were used for the analysis. These clusters are categorized into three groups according to the expression preference of their piRNAs (see references 39–41 in the main text), with the germline-enriched class colored in red, the intermediate class colored in blue, and the soma-enriched class colored in orange. No significant impact of tsn mutations on these piRNA clusters was observed. (E) qRT-PCR was performed to determine the expression of multiple transposons, relative to rp49, in tsn¹¹²⁰/tsn⁰⁶¹⁴ mutant ovaries. Transcript levels from the WT ovaries were set as 1, and fold-changes are indicated. Error bars represent mean ± standard error of the mean (N = 3). tsn mutant ovaries displayed modest defects in transposon silencing, which is consistent with the data from testes (Fig 7E).

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S13 Fig. Papi and Tudor do not compensate for the loss of TSN in tsn mutant testes.

Western blotting analysis of Papi and Tudor in tsn mutant and WT testes. No significant difference of Papi or Tudor expression was found between tsn mutant and WT control testes.

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S14 Fig. A model on the synergistic effect of TSN and Piwi in transposon silencing.

TSN and Piwi act through independent pathways to silence transposons. In wildtype flies, the two pathways are both functional, which leads to complete silencing of transposons. In piwi mutants, a typical effect of transposon de-silencing is observed, as previously reported. In tsn mutants, a milder de-silencing effect is observed. This may not reflect that the TSN-mediated silencing has less function but rather because Piwi is significantly up-regulated in tsn mutants, which partially compensated for the loss of TSN-mediated transposon repression. In tsn; piwi double mutants, both TSN and Piwi-mediated repression mechanisms are abolished, which leads to an even more drastic transposon repression that has not been reported.

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Acknowledgments

We thank Drs. Mikiko C. Siomi, Olli Silvennoinen, and Dorothea Godt for providing the antibodies. We also thank the TRiP at Harvard Medical School (NIH/NIGMS R01-GM084947) for the transgenic RNAi fly stock and the expression vector used in this study. We also thank the anonymous reviewers and Jacob Gonzales for their valuable comments of this manuscript, especially a reviewer’s comments on the synergistic interaction between TNS and Piwi in transposon silencing.

Author Contributions

Conceived and designed the experiments: HL HYK VKG. Performed the experiments: HYK VKG HQ. Analyzed the data: HYK NL HQ VKG HL. Wrote the paper: HYK HL HQ.

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Figures

Abstract

Author Summary

Introduction

Results

TSN is a novel Piwi interactor

TSN expression during development

TSN is required in the germline for proper spermatogenesis

tsn mutant testes display over-proliferation of spermatogonia and compromised differentiation of spermatocytes

Piwi and TSN antagonistically interact in the germline to regulate spermatogenesis

TSN synergistically interacts with Piwi to silence transposons but has little role in piRNA biogenesis

Discussion

Materials and Methods

Drosophila stocks, transgene expression, and RNAi

Biochemical purification and identification of cytoplasmic Piwi interacting peptides

Embryo extraction and Immunoprecipitation

Western blot analysis

Immunostaining

Live testicular squashes and phase contrast microscopy

Male fertility assay

Small RNA cloning and analysis

Total RNA extraction and quantitative RT-PCR

Immunoprecipitation and quantitative RT-PCR of TSN-associated RNA

Supporting Information

S1 Fig. Specificity of anti-TSN antibodies.

S2 Fig. The knockdown of tsn resulted in the swollen apical tip of the testis.

S3 Fig. The knockdown of tsn did not cause any obvious phenotype in ovaries.

S4 Fig. TSN antagonizes Piwi during oogenesis.

S5 Fig. Germline expression of tsn transgene rescued tsn mutant phenotype and fertility.

S6 Fig. GSC number is normal in adult tsn mutant testes.

S7 Fig. The upregulation of Piwi caused by the mutations of tsn is within the Piwi-expressing cells.

S8 Fig. Overexpression of tsn in germ cells of the wildtype testis.

S9 Fig. Overexpression of tsn in both germline and somatic cells of the wild-type testis.

S10 Fig. TSN negatively regulates Piwi expression at the mRNA level in ovaries.

S11 Fig. Somatic knockdown of Piwi does not rescue tsn mutant phenotypes.

S12 Fig. TSN shows little effects on piRNAs and transposon silencing in ovaries.

S13 Fig. Papi and Tudor do not compensate for the loss of TSN in tsn mutant testes.

S14 Fig. A model on the synergistic effect of TSN and Piwi in transposon silencing.

Acknowledgments

Author Contributions

REFERENCES