Abstract
One of the most remarkable chromatin remodelling processes occurs during spermiogenesis, the post-meiotic phase of sperm development during which histones are replaced with sperm-specific protamines to repackage the genome into the highly compact chromatin structure of mature sperm. Here we identify Chromodomain helicase DNA binding protein 5 (Chd5) as a master regulator of the histone-to-protamine chromatin remodelling process. Chd5 deficiency leads to defective sperm chromatin compaction and male infertility in mice, mirroring the observation of low CHD5 expression in testes of infertile men. Chd5 orchestrates a cascade of molecular events required for histone removal and replacement, including histone 4 (H4) hyperacetylation, histone variant expression, nucleosome eviction and DNA damage repair. Chd5 deficiency also perturbs expression of transition proteins (Tnp1/Tnp2) and protamines (Prm1/2). These findings define Chd5 as a multi-faceted mediator of histone-to-protamine replacement and depict the cascade of molecular events underlying this process of extensive chromatin remodelling.
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Introduction
Spermatogenesis is an intricate biological process that transforms diploid spermatogonial stem cells into haploid spermatozoa in seminiferous tubules of testis. It consists of three major phases: mitosis, meiosis and spermiogenesis1. Spermatogonial stem cells first multiply by repeated rounds of mitosis and differentiate into primary spermatocytes, which subsequently undergo meiosis and become haploid round spermatids. Round spermatids then mature into highly specialized spermatozoa through spermiogenesis, the final phase of spermatogenesis1. During spermiogenesis, round spermatids undergo a number of characteristic changes including elongation and condensation of the nucleus, formation of the acrosome and flagellum, and removal of cytoplasm2. In mouse, spermatogenesis is subdivided into twelve stages (stages I–XII), whereas spermiogenesis is further divided into 16 steps (steps 1–16) mainly defined by changes in acrosome structure and nuclear morphology of the maturing spermatids1,3,4,5.
Extensive chromatin remodelling occurs during spermiogenesis, which results in the majority of nucleosomal histones being replaced by sperm-specific basic proteins, initially transition proteins and ultimately protamines6. Protamines are distinct from histones, packaging the sperm genome into a distinct toroid chromatin structure7. This dramatic histone-to-protamine remodelling repackages the sperm genome into a chromatin structure that is sixfold or more compact than that of somatic cells, and is essential for normal sperm development6,8. Given its extensive degree of chromatin remodelling, spermiogenesis offers a unique process to study mechanisms of chromatin remodelling. However, this process is currently understudied and still poorly understood, mainly due to the complexity of the process itself and lack of in vitro experimental systems for studying it. In particular, chromatin remodellers are believed to be essential for facilitating the extensive degree of chromatin remodelling during spermiogenesis, but their roles in this process are not well elucidated. In this study, we discovered that Chromodomain helicase DNA-binding protein 5 (Chd5) plays an orchestrating role in the histone-to-protamine remodelling process during spermiogenesis. Chd5 is a member of the CHD family of chromatin remodellers, which we identified as a dosage-sensitive tumour suppressor9. While recent studies reveal that Chd5 binds unmodified histone 3 (H3) via its dual plant homeodomains10,11 and that this interaction is essential for tumour suppression10, the ability of Chd5 to mediate chromatin dynamics in the context of normal cells is not well understood. We find that Chd5 is highly expressed during spermiogenesis and plays essential roles during sperm development. Inactivation of Chd5 in mice leads to sperm chromatin compaction defects and male infertility. We reveal that Chd5 both mediates a cascade of molecular events for histone removal and modulates the homeostasis of transition proteins and protamines, identifying Chd5 as a master regulator of the histone-to-protamine chromatin remodelling process during spermiogenesis.
Results
Chd5 is expressed in spermatids during spermiogenesis
Using immunofluorescence analyses with a previously validated antibody specific for Chd5 (refs 10, 12) we found that Chd5 is expressed in mouse testes specifically during spermiogenesis (Fig. 1, Supplementary Fig. 1). Chd5 was first detectable after meiosis, when it was expressed within nuclei of step 4 spermatids (Fig. 1). At this phase, Chd5 was weakly expressed throughout the nucleus but was highly expressed in an intense focal spot near the chromocentre, a cluster of centromeres and pericentromeric heterochromatin13. Chd5 expression peaked at steps 7–8, when it was expressed robustly throughout the nucleus and was enriched in the chromocentre, where Chd5 colocalized with the heterochromatin mark H3K9me3, and was expressed in a pattern similar to that of the repressive histone mark H3K27me3 (Fig. 1b, Supplementary Fig. 2). Chd5 expression decreased after step 9, when it remained enriched in heterochromatin, and was not detectable after step 10 (Fig. 1). The Chd5-intense focal spot juxtaposed to the edge of the chromocentre was present in round spermatids from steps 4–8, and was positioned at the junction between the chromocentre and the post-meiotic sex chromosome, both of which are DAPI-intense sub-nuclear structures within spermatids (Fig. 1, Supplementary Fig. 3a)14. In contrast to the chromocentre, the Chd5-intense focal spot was DAPI-weak and was negative for H3K9me3 (Fig. 1b, Supplementary Fig. 3a), suggesting that it marks transcriptionally active chromatin. We speculated that the Chd5-intense foci may be within nucleoli. Co-immunostaining of Chd5 with the nucleolar marker fibrillarin showed that the Chd5-intense spot was near the nucleolus in many spermatid nuclei, but was clearly separated in others (Supplementary Fig. 3b), raising the possibility that Chd5 transiently associates with the nucleolus. These findings indicate that Chd5 is expressed specifically in nuclei of round and early elongating spermatids during spermiogenesis where it is primarily enriched in heterochromatic regions, and that Chd5 is also expressed in an intense focal spot in a non-heterochromatic region juxtaposed to the chromocentre.
Chd5 deficiency impairs sperm development and fertility
The dynamics of Chd5 expression during spermiogenesis indicated that it might play a functional role in chromatin remodelling during spermatid maturation. To explore this possibility, we generated Chd5-deficient mice carrying the Chd5Aam1 null allele (Supplementary Fig. 4). Western blot analyses using a validated antibody10 recognizing a part of Chd5 protein not disrupted by gene targeting demonstrated that the Chd5 protein was not detected in testes of Chd5Aam1 homozygotes (Fig. 2a). Chd5Aam1−/− mice were viable and grossly normal. Mating tests revealed that whereas Chd5Aam1−/− female mice and Chd5Aam1+/− mice of both genders were fertile, Chd5Aam1−/− males were either sub-fertile or sterile (Supplementary Table 1). Chd5Aam1−/− mice had significantly lower sperm counts, and the sperm that were produced had compromised motility and a higher proportion of morphological abnormalities (Table 1, Fig. 2b and Supplementary Table 2). Using in vitro fertilization (IVF), we found that Chd5Aam1−/− sperm failed to fertilize wild-type oocytes (Supplementary Table 3). Although it might be expected that some functional sperm from sub-fertile Chd5Aam1−/− mice should be able to fertilize oocytes, none of the sperm obtained from three different Chd5Aam1−/− mice were able to generate blastocysts in vitro. This may be because each of the three males tested happened to be sterile rather than sub-fertile, or that IVF conditions compromised the sperm that would have been able to fertilize oocytes under in vivo conditions. A possible explanation for the range of severity of the fertility phenotype in different mice was genetic background, as 129Sv embryonic stem cells were used to generate the Chd5Aam1 allele, with mice being backcrossed for over four generations onto the C57BL/6 background before heterozygotes were intercrossed. To determine whether genetic background affected fertility, we established a second Chd5-deficient mouse model (carrying the Chd5Tm1b null allele15) that was in a 100% pure C57BL/6 genetic background, and assessed male fertility (Supplementary Fig. 5, Supplementary Table 4). We found that Chd5Tm1b−/− male mice were also either sterile or sub-fertile. Another Chd5-deficient mouse model in a pure 129E background also showed that homozygous male mice exhibited variable pathology ranging from absence of sperm to near-normal sperm count, although six homozygous males tested did not produce any progeny over the 2-month period analysed16. These data suggest that Chd5 deficiency compromises sperm production and male fertility and that this phenotype exhibits inherent variability in different individuals.
To assess chromatin integrity in sperm from Chd5-deficient mice, we used the sperm chromatin structure assay (SCSA) (Fig. 2c). SCSA revealed that DNA fragmentation was enhanced in Chd5Aam1−/− sperm, reflecting a compromise in chromatin integrity17. Consistent with this finding, transmission electron microscopy showed that whereas chromatin within nuclei of wild-type sperm is homogeneously condensed, less-condensed chromatin with a punctate texture and uneven density, as well as the presence of abnormal vacuoles, were observed in nuclei of Chd5Aam1−/− sperm (Fig. 2d). These findings show that Chd5 deficiency leads to defective chromatin compaction in sperm.
Since compromised fertility can be caused by a deregulation of sex hormones, we investigated this possibility (Supplementary Fig. 6). However, we did not detect a significant alteration in sex hormones in Chd5Aam1−/− male mice relative to controls. Histological analyses of testes revealed that seminiferous tubules of Chd5Aam1−/− mice contained fewer elongated spermatids relative to controls, with an abnormal retention of condensed spermatids within stage IX and X tubules (Fig. 2e, Supplementary Fig. 7). The extent of histological abnormalities varied among individual Chd5Aam1−/− mice (Supplementary Fig. 7), in agreement with the variable severity of infertility observed in male Chd5-deficient mice. In contrast to post-meiotic defects, we did not observe differences in spermatogenic cells (spermatogonia, spermatocytes, round spermatids) or in somatic cells (Sertoli cells, Leydig cells) in Chd5Aam1−/− testes (Fig. 2e, Supplementary Fig. 7). These findings indicate that Chd5 deficiency disrupts the elongation and condensation steps of post-meiotic sperm maturation, consistent with Chd5’s peak of expression in step 7–8 round spermatids, the phase immediately preceeding extensive chromatin remodelling.
To determine whether our findings from Chd5-deficient mice might be relevant to human cases of male infertility, we analysed a previously established gene expression data set of testes biopsies from 39 men (29 men with highly defined testicular pathology and 10 men with normal spermatogenesis)18. This analysis revealed that men with spermatogenic defects had lower CHD5 expression relative to controls and that the clinical grade of spermatogenic defect correlated inversely with CHD5 expression (Fig. 2f). While this is a correlation rather than evidence for causality, it suggests that future efforts should be made to determine whether compromised CHD5 contributes to male infertility in humans.
Chd5 deficiency disrupts histone-to-protamine replacement
During mammalian spermiogenesis, the majority of canonical histones are removed and replaced by histone variants and transition proteins, which are subsequently replaced by protamines6,7,19,20. This histone-to-protamine replacement process repackages the sperm genome at least sixfold more compact than its somatic counterpart8. To define the mechanism whereby Chd5 deficiency compromises chromatin compaction during spermiogenesis, we used western blotting to assess expression of a panel of somatic histones, transition proteins and protamines in elutriation-purified spermatids at different steps of spermiogenesis (Supplementary Fig. 8). The core nucleosomal histones (H1, H2A, H2B, H3 and H4) were quickly depleted after the round spermatid steps in wild-type testes, with minimal retention in condensing and condensed spermatids (Fig. 3a). In contrast, these core histones were retained to a higher extent in Chd5Aam1−/− differentiated spermatids, which implied ineffective histone removal. In addition, transition proteins (Tnp1 and Tnp2) and protamines (Prm1 and Prm2) had elevated expression in differentiated Chd5Aam1−/− spermatids (Fig. 3b,c), likely contributing to impaired fertility of Chd5Aam1−/− mice, as precise control of levels of Prm1 and Prm2 are critical for male fertility21,22. Prm2 is first translated as a precursor protein that is subsequently processed into mature Prm2 through a multistep proteolytic cleavage. In Chd5Aam1−/− spermatids, there was enhanced expression of the Prm2 precursor and partially processed Prm2 was present, indicating a defect in Prm2 processing, which may be because the overproduction of Prm2 in Chd5Aam1−/− spermatids exceeds the processing capacity of the cells. In addition, both Tnp1 and Tnp2 deficiency have been shown to increase levels of the Prm2 precursor and partially processed forms of Prm2 (refs 23, 24). Thus, the abnormal elevation of Tnp1 and Tnp2 in Chd5Aam1−/− spermatids may also contribute to defective Prm2 processing. Consistent with the observation in spermatids, western blotting of lysates from mature sperm also revealed enhanced retention of core nucleosomal histones and elevated Prm1 and Prm2 expression in Chd5Aam1−/− sperm (Fig. 3d). Furthermore, immunofluorescent analyses of testes showed enhanced expression of Tnp1, Tnp2, Prm1 and Prm2 in Chd5Aam1−/− spermatids (Fig. 3e, Supplementary Figs 9–12). In addition, Tnp1 was precociously expressed in step 9–10 spermatids and had extended expression until step 15 spermatids in Chd5Aam1−/− testes. These findings indicate that Chd5 deficiency perturbs the histone-to-protamine transition that occurs during spermiogenesis, leading to aberrant retention of nucleosomal histones and elevated levels of transition proteins and protamines.
Chd5 mediates histone removal and DNA repair
To assess the mechanism of how Chd5 deficiency leads to aberrant histone removal we focused on H4 hyperacetylation, a molecular event occurring in early elongating spermatids that is essential for histone-to-protamine replacement in Drosophila25, and considered the same for spermiogenesis in mammals6,25,26. Using immunofluorescence, we determined that Chd5 had similar expression dynamics as H4 hyperacetylation during spermiogenesis, but immediately preceded it (Fig. 4a). In step 9–10 spermatids, Chd5 colocalized with H4 acetylation, suggesting that Chd5 modulates H4 hyperacetylation during spermiogenesis (Fig. 4a). Consistent with this hypothesis, immunofluorescent analyses revealed that H4 acetylation was compromised in Chd5Aam1−/− spermatids (Fig. 4b). In Chd5Aam1+/+ testis, H4 hyperacetylation was detected in step 9 spermatids and showed peak expression in step 10–12. H4 acetylation decreased in step 13 spermatids, and was not detectable at later steps. Whereas H4 acetylation was detected within step 9–13 spermatids of Chd5Aam1−/− testis, its expression was substantially reduced in Chd5Aam1+/+ spermatids. Furthermore, western blotting of lysates from elutriation-purified spermatid fractions showed that whereas more total H4 was retained, H4Ac was severely compromised in differentiated Chd5Aam1−/− spermatids (Fig. 4c). Consistent with the findings in Chd5Aam1−/− mice, Chd5Tm1b−/− testes also showed compromised histone H4 acetylation (Supplementary Fig. 13). These findings indicate that acetylated H4 is compromised in Chd5-deficient testes.
Following H4 hyperacetylation, acetylated histone tails are recognized by Brdt, a testis-specific member of the BRD bromodomain-containing protein family that has been shown to induce eviction of nucleosomes6,27,28. However, how Brdt mediates nucleosome eviction is not clear. Likely, Brdt recruits chromatin remodelers to remodel and evict hyperacetylated nucleosomes. We therefore asked whether the compromised H4 acetylation and Chd5 deficiency perturbed nucleosome eviction in Chd5Aam1−/− spermatids. Using an antibody specific for intact nucleosomes29, we found that nucleosomes were detectable through step 11 of spermatid maturation in wild-type testes, but were depleted at later steps (Fig. 5a). However, we found that nucleosomes were aberrantly retained in Chd5Aam1−/− spermatids as late as step 14 (Fig. 5b), indicating that nucleosomes were ineffectively evicted. Thus, both H4 acetylation and nucleosome eviction are compromised by Chd5 deficiency.
Nucleosome eviction generates DNA supercoiling tension that needs to be relieved. Previous studies indicate that topoisomerase II beta (Top2β) catalyses resolution of such supercoils in elongating spermatids, during which double-strand breaks (DSBs) are generated. A DNA damage response is then triggered to repair the DSBs in order to maintain genome integrity30,31,32,33. We found that Chd5 expression is induced by DNA damage (Fig. 6a), suggesting that Chd5 plays a role in the DNA damage response as well. Indeed, TUNEL assays revealed an increase of DNA breaks in differentiated Chd5Aam1−/− spermatids, most notably at steps 13–14 (Fig. 6b), a time point when most DNA breaks are repaired in wild-type testes. In agreement with this finding, immunofluorescent analyses showed that whereas γ-H2A.X (a marker for the DSB-activated DNA damage response) is cleared in wild-type spermatids after step 12, it is detected in Chd5Aam1−/− spermatids as late as step 14 (Fig. 6c). Western blot analyses further confirmed an increase of γ-H2A.X in differentiated Chd5Aam1−/− spermatids (Fig. 6d). Together, these findings indicate that Chd5 deficiency impairs H4 hyperacetylation, nucleosome eviction, and DNA damage repair during spermiogenesis.
Chd5 loss alters gene expression in spermatids
Tnp1, Tnp2, Prm1 and Prm2 are transcribed in round spermatids, but their transcripts are stored in translationally repressed ribonucleoprotein particles before being later translated into protein within elongating spermatids34,35,36. To determine whether the increase in transition proteins and protamines within Chd5-deficient spermatids was due to enhanced expression at the transcript level, we used qRT–PCR to assess Tnp1, Tnp2, Prm1 and Prm2 expression in Chd5Aam1−/− and Chd5Aam1+/+ round spermatids. Whereas only a slight increase of Tnp1, Tnp2 and Prm2 transcripts were detected, Prm1 transcript was increased ~\n2.5-fold in Chd5Aam1−/− round spermatids (Fig. 7a). Using chromatin immunoprecipitation-qPCR (ChIP-qPCR) analyses of nuclear lysates from testicular cells, we found an enrichment of Chd5 binding at the Prm1 promoter (region P: −77 bp to +135 bp) (Fig. 7b). Less-pronounced Chd5 binding was observed at region A (−860 to −672 bp), B (−444 bp to −239 bp) and C (+397 bp to +585 bp), but not at region 5′ (−1,319 bp to −1,164 bp). Collectively, these data suggest that Chd5 represses Prm1 transcription, whereas it negatively modulates expression of Tnp1, Tnp2 and Prm2 mainly post-transcriptionally.
As described above, a Chd5-intense focus near the edge of chromocentre in round spermatids showed proximity to the nucleolar marker fibrillarin (see Supplementary Fig. 3b), suggesting that Chd5 may play a role in rRNA biogenesis and translational control. qRT–PCR analyses of 45S and 28S rRNA expression revealed that 45S rRNA was reduced by ~\n30%, and 28S rRNA expression was reduced by >50%, in Chd5Aam1−/− round spermatids (Fig. 7c), indicating compromised rRNA biogenesis in Chd5Aam1−/− spermatids. These results suggest a role of Chd5 in rRNA biogenesis during spermiogenesis, which is consistent with the known function of other CHD proteins such as CHD4 and CHD7 in positively regulating rRNA biogenesis37,38.
In addition to H4 hyperacetylation, replacement of canonical core nucleosomal histones with histone variants including those that are testis-specific is another key mechanism facilitating nucleosome destabilization and histone removal during spermatogenesis39,40,41. We examined expression of a panel of general and testis-specific histone variants in Chd5Aam1+/+ and Chd5Aam1−/− round spermatids via qRT–PCR, and discovered that expression of the H2B variant Hist1h2bc was elevated over fivefold in Chd5Aam1−/− round spermatids (Fig. 7d). Although little is known about the functions of Hist1h2bc, its substantial increase in Chd5Aam1−/− round spermatids suggests that it might impact histone variant exchanges during spermiogenesis. In addition, an ~\n30% decrease in expression of histone H1 variant Hist1h1e, histone H3 variant Hist2h3c1 and testis-specific H1 variant H1t were consistently observed in Chd5Aam1−/− spermatids (Fig. 7d). These findings indicate that Chd5 deficiency alters transcript levels of specific histone variants during spermiogenesis.
In order to gain insight into the global gene expression changes resulting from Chd5 deficiency and to identify candidate Chd5 targets, we performed RNA sequencing (RNA-Seq) (Fig. 8). Chd5 is mainly expressed in round spermatids, where transcription is most active during spermiogenesis, with transcription globally being ceased afterwards. Using RNA-Seq, we compared mRNA expression profiles of round spermatids that had been elutriation-purified from five sets of Chd5Aam1+/+, Chd5Aam1+/− and Chd5Aam1−/− littermates. Expression of 14,206 transcripts was detected in at least one of the three genotypes. Two-hundred and sixty-one transcripts, or 1.8% of all the transcripts detected, showed a twofold or greater expression change in Chd5Aam1−/− round spermatids compared with Chd5Aam1+/+ counterparts (false discovery rate q=0.05). Among the 261 transcripts, 156 transcripts or 59.8% were downregulated, whereas 105 transcripts, or 40.2%, were upregulated in Chd5Aam1−/− round spermatids. Together, these results suggest that Chd5 deficiency leads to a rather limited alteration in global gene expression in round spermatids, and that Chd5 both activates and suppresses gene expression in round spermatids with a slight preference for activation. Gene ontology (GO) analysis of the gene expression changes showed clustering of GO terms including chromosome organization, response to DNA damage, acetylation, alternative splicing, nuclear export, protein transport, ubl (ubiquitin) conjugation, intracellular transport, endocytosis, cell cycle and MAPK pathway (Supplementary Fig. 14). Since Chd5Aam1+/− male mice were fertile, we reasoned that genes that had expression changes only in Chd5Aam1−/− spermatids but not in Chd5Aam1+/− spermatids, or genes that had gradual expression changes dependent on Chd5 dosage, would be candidates most likely to contribute to the infertility of Chd5Aam1−/− male mice. We thus further filtered the 261 transcripts through clustering with manual examination and identified a list of 155 transcripts that had expression changes only in Chd5Aam1−/− spermatids, or that had gradual expression changes that correlated with Chd5 dosage (Fig. 8a, Supplementary Fig. 15). Among the list, 90 transcripts were downregulated and 65 transcripts, including Hist1h2bc, were upregulated in Chd5Aam1−/− spermatids (Fig. 8a). qRT–PCR analyses for expression of 11 genes from this list, which included the positive control Hist1h2bc and represented a range of expression changes, was used to validate the expression changes revealed by RNA-Seq, attesting to the reliability of the RNA-Seq data and analyses (Fig. 8b). GO analysis of this list showed clustering of a subset of GO terms revealed from the original list, which include chromosome organization, response to DNA damage stimulus, alternative splicing, ubl conjugation, regulation of DNA metabolic process, cell cycle and MAPK signalling (Fig. 8c). A number of candidates implicated in acetylation (1700019G17Rik), DNA damage response (Wrnip1), RNA processing and translational control (Cstf2t) and nuclear structure maintenance (Syne3) were further verified using qRT–PCR (Fig. 8d, Supplementary Fig. 16). Altogether, these GO terms are consistent with the phenotypic impacts of Chd5 deficiency on chromatin compaction, DNA damage response and post-transcriptional modulation of transition proteins and protamines during spermiogenesis. Alterations in gene expression within these GO terms are likely contributing, at least partially, to the spermatogenic abnormalities of Chd5Aam1−/− male mice.
Discussion
In this study, we show that Chd5 mediates a cascade of molecular events underlying histone removal during spermiogenesis including H4 hyperacetylation, histone variant expression, nucleosome eviction and DNA damage repair. Chd5 deficiency leads to disruption of these biological processes and increases histone retention in both spermatids and sperm. We reveal that Chd5 also modulates the homeostasis of transition proteins and protamines by suppressing expression of Prm1 transcriptionally and expression of Tnp1, Tnp2 and Prm2 post-transcriptionally. Chd5 deficiency results in elevated levels of both transition proteins and protamines. These findings unravel pleiotropic functions of Chd5 and highlight its multi-faceted role in orchestrating the extensive histone-to-protamine remodelling that occurs during male germ cell development.
Chd5 contains multiple domains (PHD domains, chromodomains, SNF2-like ATPase domain, DEAD/DEAH-box Helicase domain, SANT domain and DNA-binding motifs), which may enable its diverse functions during spermiogenesis. The SNF2-like ATPase domain defines the nucleosome remodelling function of CHD proteins42,43. Chd5 may facilitate nucleosome eviction during spermiogenesis through its ATPase domain, whose absence in Chd5-deficient spermatids would thus lead to inefficient nucleosome eviction. The ATPase domain is also implicated in DNA damage repair in somatic cells44 and may play a direct role in the DNA damage response during spermiogenesis and contribute to the increased DNA damage in Chd5-deficient spermatids. The DEAD/DEAH-box helicase domain may implicate Chd5 in RNA processing and the characteristic repression of mRNA translation in round spermatids, which could contribute to the abnormal post-transcriptional elevation of transition proteins and protamines in Chd5-deficient spermatids. It is known that the dual PHD domains of Chd5 preferentially bind H3 tails lacking H3K4me3 in mouse embryonic fibroblasts10, whereas the chromodomains bind to H3K27me3 in neurons, both of which are important for Chd5 to mediate gene expression in somatic cells10,45. We also observe such patterns in mouse spermatids, as Chd5 is enriched in the chromocentre of spermatids, a heterochromatic region marked with H3K9me3 and H3K27me3, but lacking H3K4me3 (Fig. 1, Supplementary Fig. 2). This suggests that the PHD and/or chromodomains of Chd5 may also play important roles in regulating gene expression in spermatids, as RNA-Seq revealed that Chd5 deficiency leads to expression changes of specific gene sets. These multiple functional domains of Chd5 may work independently or in concert, enabling the diverse functions of Chd5 observed during spermiogenesis.
It is possible that there is a functional connection between the histone removal process and homeostasis of transition proteins and protamines. For example, transition proteins have been implicated in DNA repair during spermiogenesis46,47, thus the abnormal levels of transition proteins may contribute to the increased DNA damage in Chd5Aam1−/− spermatids. On the other hand, deficient H4 acetylation may alter the chromatin structure of the Prm1 locus, thereby contributing to its increased transcription, although it is counterintuitive that a decrease in H4 acetylation would result in transcriptional activation.
Chromatin remodellers are thought to be critical for the extensive chromatin remodelling taking place during the post-meiotic phase of spermiogenesis; however, little is known about their roles in this process. The chromatin remodeller Brg1 is essential for meiosis, and its deficiency leads to meiotic arrest with global alterations in histone modifications and chromatin structure in mice48. Acf1, which binds to chromatin remodeller Snf2h within the ACF complex, plays an essential role during post-meiotic spermiogenesis49. Deletion of Acf1 results in male infertility with increased DNA damage and spermiation defects, but without any detectable alterations in chromatin composition49. Previous studies have also suggested roles of chromatin modifier Rnf8, a E3 ubiquitin ligase, in spermiogenesis. Lu et al.50 revealed that Rnf8 mediates H2A and H2B ubiquitination in elongating spermatids, and is critical for H4K16 acetylation and histone-to-protamine replacement. However, Sin et al.51 later reported that Rnf8 deficiency does not affect H4K16 acetylation and histone-to-protamine exchange in spermatids, but instead compromises gene activation from inactive sex chromosomes in round spermatids. Thus, while a number of nuclear proteins have been implicated in spermatogenesis, Chd5, to our knowledge, is the first chromatin remodeller identified to play an orchestrating role in chromatin remodelling during post-meiotic spermiogenesis.
Consistent with Chd5 deficiency disrupting histone acetylation, DNA damage response and homeostasis of transition proteins and protamines during spermiogenesis, RNA-Seq reveals that Chd5 deficiency alters expression of genes encoding proteins underlying these processes, but does not cause a major change in global gene expression in round spermatids. We validate a number of candidate Chd5 target genes (for example, Cstf2t, 1700019G17Rik, Wrnip1 and Syne3) implicated in these processes. Notably, Cstf2t encodes the RNA polyadenylation protein tauCstF-64, which is expressed during haploid spermatid differentiation52. Deletion of Cstf2t in mice disrupts post-meiotic development and leads to male infertility52. Similar to the heterogeneity of histopathology among Chd5Aam1−/− testes, Cstf2t−/− male mice also display variable expressivity of sperm defects52. These intriguing parallels suggest that deficient expression of Cstf2t in Chd5Aam1−/− spermatids may contribute to the infertile phenotypes of Chd5Aam1−/− mice. In addition, the compromised expression of Cstf2t in Chd5Aam1−/− spermatids may compromise polyadenylation and translational repression of transition protein and protamine mRNAs, thereby leading to an elevation in protein production, since translational repression of mRNAs in spermatids involves binding of protein repressors to poly (A) tails, and shortening of poly (A) tails of Tnp1, Tnp2, Prm1 and Prm2 mRNAs accompanies their translation activation53,54. 1700019G17Rik encodes a putative N-acetyltransferase that is highly enriched in mouse testis but is absent in most other tissues (Supplementary Fig. 16a). We also found that 1700019G17Rik expression increases as round spermatids differentiate into elongating spermatids, the time point at which H4 hyperacetylation occurs (Supplementary Fig. 16b). These data suggest 1700019G17Rik as a potential acetyltransferase affecting H4 acetylation during spermiogenesis, and the >80% decrease in expression may compromise H4 acetylation in Chd5Aam1−/− spermatids. Wrnip1 stimulates the activity of DNA polymerase delta, rapidly accumulates at laser-irradiated sites and is required for maintaining genome integrity55,56,57. Syne3 is a component of the nuclear envelope that tethers the nucleus to the cytoskeleton, and is critical for maintaining nuclear organization and structural integrity, as well as for development of the sperm head58,59,60,61,62. Compromised expression of Wrnip1 and Syne3 may contribute to the enhanced DNA damage and abnormal sperm head morphology, respectively, in Chd5Aam1−/− testis. However, it is not yet clear whether these genes and other candidates revealed by RNA-Seq are direct Chd5 target genes, a question that could be addressed by defining the global pattern of Chd5-bound loci in spermatids. A small proportion of histones and nucleosomes are retained in chromatin of wild-type sperm, preferentially at loci encoding proteins of developmental importance63. It would be interesting to know whether the aberrant histone retention in Chd5Aam1−/− sperm disrupts such a pattern, where the aberrantly retained histones locate in the genome of Chd5Aam1−/− sperm, and to understand these implications for the developmental potency of the sperm. Future studies to characterize genome-wide distribution of Chd5, nucleosomal histones and specific histone modifications in Chd5-deficient spermatids and sperm should shed additional light on these questions.
We observed variation ranging from sterility to sub-fertility among individual Chd5Aam1−/− male mice in a mixed C57BL/6 and 129S background, as well as among individual Chd5Tm1b−/− male mice in a pure C57BL/6 background. Such variability in infertility is similarly observed in Tnp1−/− and Tnp2−/− male mice, as ~\n40 and 89% of Tnp1−/− and Tnp2−/− male mice, respectively, are sub-fertile23,24. The aberrant Tnp1 and Tnp2 levels in Chd5-deficient testes may contribute to the variable infertility among individual Chd5-deficient male mice. In addition, we observed increased DNA damage in Chd5-deficient spermatids and sperm. The intrinsically variable extent of DNA damage may be more severe in testes of some Chd5-deficient mice than in others, thus contributing to the variability of infertility.
H4 hyperacetylation in early elongating spermatids is shown to be essential for histone-to-protamine replacement in Drosophila25 and has been considered the same for mammalian spermiogenesis6,25,26. Our study shows that Chd5 deficiency leads to substantial deficiency in H4 acetylation in elongating spermatids and subsequent defects in nucleosome eviction and histone removal, supporting the notion that H4 hyperacetylation is indeed critical for efficient nucleosome eviction and histone removal during mouse spermiogenesis. However, most nucleosomes and histones eventually get removed in late Chd5Aam1−/− spermatids. This suggests that whereas H4 hyperacetylation is important for efficient nucleosome eviction and histone removal during mammalian spermiogenesis, it seems non-essential. Thus, whether H4 hyperacetylation is required for histone-to-protamine replacement during mammalian spermiogenesis warrants further investigation. In addition, the enzymes responsible for H4 hyperacetylation during spermiogenesis remain unidentified and are of great interest in the field. Our study identifies 1700019G17Rik as a candidate acetyltransferase for H4 hyperacetylation, providing a new promising target for future study.
The cascade of defects in H4 hyperacetylation, nucleosome eviction and DNA break repair during Chd5Aam1−/− spermatid maturation provide functional evidence demonstrating the sequential order of these events, and suggest a model for the molecular events underlying the histone-to-protamine replacement process during spermiogenesis: H4 is first hyperacetylated, which along with other epigenetic modifications, leads to chromatin loosening and nucleosome eviction to facilitate histone removal and exposure of the DNA to allow for deposition of transition proteins and eventually protamines. DSBs are generated during nucleosome eviction to resolve supercoiling tension, and DNA damage response is activated to repair the DSBs, ensuring integrity of the sperm genome. This sequence of molecular events is in agreement with the model proposed by Leduc et al.30. Our findings establish functional evidence revealing the cascade of major molecular events underlying the histone-to-protamine replacement process, and provide a foundation to further elucidate this critical but elusive process.
Methods
Generation of Chd5-deficient mouse models
To generate the Chd5Aam1 mouse model, Chd5 locus was disrupted in AB2.2 ES cells using the MHPN20h05 MICER vector64, and targeted ES cells were injected into C57BL/6 blastocysts through standard procedures. All animals were housed and utilized according to the Cold Spring Harbor Institutional Animal Care and Use Committee (IACUC) and the Association for Accreditation of Laboratory Animal Care International (AAALAC) policies. Progeny resulting from germline transmission were backcrossed to wild-type C57BL/6 mice, and Chd5Aam1+/− mice were intercrossed to obtain homozygotes. To generate the Chd5Tm1b mouse model, ES clones with Chd5Tm1a(EUCOMM)Wtsi allele, which has exon 2 of Chd5 locus flanked by LoxP sites, were obtained from EUCOMM (European Conditional Mouse Mutagenesis)65. ES cells were from the C57BL/6N-A/a background and were injected into albino B6 (C57BL/6J-Tyr c-2J) blastocysts through standard procedures. Progeny resulting from germline transmission, designated as Chd5Tm1a+/− mice harboured a Chd5 allele with exon 2 flanked by LoxP sites. Chd5Tm1a+/− mice were mated to CMV-Cre mice in the C57BL/6 background to obtain Chd5Tm1b+/− mice (which had a Chd5 allele with exon 2 excised), and Chd5Tm1b+/− mice were intercrossed to obtain Chd5Tm1b−/− progeny.
Genotyping
For Southern blot genotyping of the Chd5Aam1 model, the MHPN20h05 MICER vector was cut with AflII and the 2.6 kb excised fragment was gel-purified and used as a probe. Southern blotting of genomic DNA digested with BglII yielded the expected 7.8 and 10.4 kb endogenous and targeted alleles, respectively. Genotypes were differentiated based on dosage of the targeted allele (Chd5Aam1+/+, 0 copies; Chd5Aam1+/−, 1 copy; Chd5Aam1−/−, 2 copies). All genotypes had two copies of the endogenous band, which serve as an internal loading control and reference for dosage. For PCR-based genotyping, relative dosage of the neo-cassette in different genotypes (Chd5Aam1+/+, 0 copies; Chd5Aam1+/−, 1 copy; Chd5Aam1−/−, 2 copies) was quantified using qPCR, with Neo-cassette dosage being normalized to dosage of Actb. Genotyping of Chd5Tm1b mice was performed by PCR using primers (Supplementary Fig. 16) that amplify a 674-bp endogenous band specific for the wild-type Chd5 allele and a 456-bp targeted band specific for the targeted Chd5Tm1b allele.
Antibodies
Antibodies used for western blot, immunoflurorescence and ChIP are as follows: anti-H3K27me3 (Cell Signaling no. 9756, 1:100 for IF, that is, immunofluorescence), anti-H2A (Cell Signaling no. 2578, 1:300 for WB, that is, Western blotting; for uncropped images, see Supplementary Fig. 17), anti-H4 (Cell Signaling no. 2935, 1:800 for WB), anti-γ-H2A.X (Cell Signaling no. 9718, 1:200 for IF; 1:1,500 for WB), anti-H3K9me3 (Active Motif no. 39385, 1:100 for IF), anti-H1 (Active Motif no. 39707, 1:800 for WB), anti-H2B (Active Motif no. 39125, 1:800 for WB), anti-H4Ac-pan (Active Motif no. 39243, 1:1,000 for WB; 1:200 for IF), anti-H3 (Abcam no. ab1791, 1:15,000 for WB), anti-Chd5 (Santa Cruz Biotechnology no. sc-68389, 1:1,500 for WB; 1:200 for IF), anti β-Actin (Sigma no. A2228, 1:2,000 for WB), anti-H4K5/8/12/14Ac (Millipore no. 05-1335, 1:100 for IF ), anti-lectin PNA Alex Fluor 568 (Invitrogen no. L32458, 1:4,000 for IF), anti-Prm1 (Briar Patch Biosciences, Hup1N, 1:300 for WB; 1:150 for IF), antiPrm2 (Briar Patch Biosciences, Hup2B, 1:800 for WB; 1: 200 for IF), anti-Tnp1 (gift from Dr Stephen Kistler, University of South Carolina, 1:500 for WB; 1: 100 for IF ), anti-Tnp2 (gift from Dr Stephen Kistler, University of South Carolina, 1:1,000 for WB; 1: 200 for IF) and anti-nucleosome (mab no. 32, gift from Dr Jo H.M. Berden, Radboud University Nijmegen Medical Center, 1:300 for IF).
Histology and immunostaining
Testes were fixed in Bouin’s fixative or 4% paraformaldehyde, embedded in paraffin and sectioned at 5 μm. Sections were deparaffinized in xylene and subjected to either PAS staining for histological analyses or immunofluorescent staining using the indicated antibodies.
Sperm counts and motility analysis
Individual caudal epididymi were minced in 200 μl HTF medium (Irvine Scientific). After 30 min incubation at 37 °C, the tissue pieces were separated from sperm by pipetting and passaging through a 70-μm filter. Sperm counts and motility assessment were performed using the DRM-600 CELL-VU Sperm Counting Cytometer.
Sperm morphology
Air-dried smears were prepared from sperm suspended in PBS, stained with haematoxylin, and examined using light microscopy at × 100 magnification. Head, neck and tail morphology was determined independently for each mouse, with separate counts of at least 100 cells per sample.
Sperm chromatin structure assay
SCSA was carried out as previously described24 using a LSR II flow cytometer (Becton Dickinson). Briefly, a 0.2 ml aliquot of sperm nuclei in TNE buffer (0.1 M Tris, 0.15 M NaCl and 1 mM EDTA (pH 7.4)) was mixed with 0.4 ml acid detergent solution (0.15 M NaCl, 0.08 N HCl and 0.1% Triton X-100, pH 1.4). After 30 s, 1.2 ml acridine orange staining solution (6 μg ml−1 acridine orange, 0.1 M citric acid, 0.2 M Na2HPO4, 1 mM EDTA and 0.15 M NaCl, pH 6.0) were added to the denatured sperm nuclei. After staining for 3 min, samples were measured for green and red fluorescence using LSR II with a 488-nm excitation wavelength. For the SCSA assay, acid-treated sperm were stained with acridine orange, which emits red or green fluorescence when binding to single-stranded or double-stranded DNA, respectively. Sperm with impaired chromatin generate more single-stranded DNA after denaturation with acid treatment, and therefore emit more red fluorescence. DNA Fragmentation Index (DFI) is defined as the percentage of red/green+red fluorescence.
Transmission electron microscopy
Testes were fixed with 2% paraformaldehyde and 2% glutaraldehyde in 0.1 M sodium phosphate buffer (pH 7.4), dehydrated and embedded in Epon. Sections were contrasted and imaged in a Hitachi H7000T transmission electron microscope.
Basic protein extraction and acid-urea gel electrophoresis
Testes were surgically decapsulated and homogenized in buffer (10 mM Tris–HCl (pH 7.2), 0.32 M sucrose, 5 mM MgCl2, 0.1% Triton X-100 and 0.5 mM PMSF). After centrifugation, cell pellets were resuspended in sonication buffer (10 mM Tris–HCl (pH 7.5), 25 mM 2-mercaptoethanol) and sonicated using a Diagenode Bioruptor UCD-200 to obtain sonication-resistant spermatids, which represent step 12–16 spermatids. After centrifugation, sonication-resistant spermatid pellets were resuspended in 10 mM Tris–HCl (pH 7.5) by brief vortexing and HCl was added to a final concentration of 0.5 M. Samples were incubated on ice for 30 min to extract basic proteins. After centrifugation, the supernatant was transferred to a new tube and 20% trichloroacetic acid (final concentration) was added to precipitate basic proteins. Protein pellets were washed with acetone, dried and dissolved in buffer containing 5 M urea, 0.5% acetic acid and 1% β-2-mercaptoethanol. Proteins were separated by electrophoresis in acid-urea-15% polyacrylamide gels and were subjected to either staining with Coomassie brilliant blue or western blot using the indicated antibodies.
TUNEL assay
TUNEL assays were performed with the In Situ Cell Death Detection Fluorescein Kit (Roche), following the manufacturer’s instruction. Briefly, testes sections were deparaffinized, rehydrated and digested with 20 μg ml−1 Proteinase K in 10 mM (Tris pH 7.5) for 30 min at 37 °C. After washes, sections were incubated with TUNEL reaction mixture for 1 h at 37 °C, followed with lectin PNA (1:4,000, 1 h) and DAPI (1:5,000, 5 min) staining to visualize acrosomes and DNA, respectively.
ChIP
ChIP was performed using SimpleChIP Enzymatic Chromatin IP Kit (Cell Signaling) with the indicated antibodies. Primers for ChIP-qPCR are listed in Supplementary Table 5.
Centrifugal elutriation
Fractionation of spermatogenic cells through centrifugal elutriation was performed as previously described66 using a Beckman Coulter Avanti J-26XP centrifuge with JE-5.0 rotor.
RNA-Seq
Five sets of Chd5Aam1+/+: Chd5Aam1+/−: Chd5Aam1−/− littermate male mice with matched background and age (~\n3 months old) were used for elutriation. Round spermatids were purified through centrifugal elutriation of the testes pooled from five mice of the same genotype. Total RNA was prepared from the round spermatid samples using RNeasy kit (Qiagen) with DNase I treatment. RNA-Seq libraries were prepared from RNA samples using Illumina TruSeq protocol. RNA-Seq libraries were barcoded and sequenced on Illumina HiSeq 2000.
RNA-Seq data analysis
The quality of raw data was assessed and passed by FastQC. Reads were mapped to the mm9 reference genome with OLego (ref. 67). Cufflinks (v2.0.2)68 was used to estimate transcript expression levels represented by FPKM (fragments per kilo bases per million mapped reads) for all the samples. Ensembl transcripts annotation was provided (−g) to guide transcriptome reconstruction. Cuffdiff (ref. 68) was run to detect differential expression between samples. Transcripts showing twofold or more expression changes in Chd5Aam1−/−spermatids compared with Chd5Aam1+/+ spermatids were selected (false discovery rate q=0.05), and further filtered via hierarchical clustering using Genesis (v1.7.6)69. Clusters that either showed expression changes only in Chd5Aam1−/− spermatids but not in Chd5Aam1+/− spermatids, or those that showed gradual expression changes from Chd5Aam1+/+ spermatids to Chd5Aam1+/−spermatids to Chd5Aam1−/− spermatids, were selected for GO analysis using DAVID (v6.7)70.
qRT–PCR validation of RNA-Seq hits
qRT–PCR was first performed on the same RNA samples used for RNA-Seq, and then repeated using another set of RNA samples that were prepared from round spermatids that had been elutriation-purified from three different sets of Chd5Aam1+/+, Chd5Aam1+/− and Chd5Aam1−/− littermate male mice with matched background and age. All qRT–PCR results were pooled and data are presented as mean±s.d. from four to five independent experiments. Primers for qRT–PCR and ChIP-qPCR are listed in Supplementary Table 5.
Additional information
Accession codes: RNA-seq data are deposited in the NCBI Short Read Archive under accession number SRPO40711.
How to cite this article: Li, W. et al. Chd5 orchestrates chromatin remodelling during sperm development. Nat. Commun. 5:3812 doi: 10.1038/ncomms4812 (2014).
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Acknowledgements
We thank W. Stephen Kistler for anti-Tnp antibodies, Jo H.M. Berden for anti-nucleosome antibodies, Emma Vernersson-Lindahl for critical reading of the manuscript, and Lisa Bianco and Aigoul Nourjanova for technical assistance. This project was supported by the Office of the Director, National Institutes of Health under award numbers R01CA127383 (to A.A.M.) and R21OD018332 (to A.A.M.), NIH HG001696 (to M.Q.Z.), and NSFC 91019016 (to M.Q.Z.); the content is the sole responsibility of the authors. This work was performed with assistance from Cold Spring Harbour Laboratory Shared Resources, which are funded, in part, by the Cancer Center Support Grant 5P30CA045508.
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W.L. and A.A.M. designed the experiments and prepared the manuscript with input from co-authors. W.L. and A.A.M. generated Chd5-deficient mouse models. W.L. performed experiments with assistance from S.-Y.K. for sperm analyses and IVF, with assistance from S.A.H. for electron microscopy, and with assistance from M.Z. and M.L.M. for centrifugal elutriation. W.L. and A.A.M. interpreted the data, with RNA-Seq data being analysed by J.W., W.L. and M.Q.Z.
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Li, W., Wu, J., Kim, SY. et al. Chd5 orchestrates chromatin remodelling during sperm development. Nat Commun 5, 3812 (2014). https://doi.org/10.1038/ncomms4812
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DOI: https://doi.org/10.1038/ncomms4812
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