Michael J W Vangompel1, Eugene Y Xu. 1. Department of Obstetrics and Gynecology; Division of Reproductive Biology Research and Center for Genetic Medicine; Northwestern University; Chicago, IL USA.
Abstract
The DAZ family of genes are important fertility factors in animals, including humans. The family consists of Y-linked DAZ, and autosomal homologs Boule and Dazl. All three genes encode RNA-binding proteins that are nearly exclusively expressed in germ cells. The DAZ family is highly conserved, with ancestral Boule present in sea anemones through humans, Dazl conserved among vertebrates, and DAZ present only in higher primates. Here we review studies on DAZ family genes from multiple organisms, and summarize the common features of each DAZ gene and their roles during spermatogenesis in animals. DAZ family proteins are thought to activate the translation of RNA targets, but recent work has uncovered additional functions. Boule, Dazl, and DAZ likely function through similar mechanisms, and we present known functions of the DAZ family in spermatogenesis, and discuss possible mechanisms in addition to translation activation.
The DAZ family of genes are important fertility factors in animals, including humans. The family consists of Y-linked DAZ, and autosomal homologs Boule and Dazl. All three genes encode RNA-binding proteins that are nearly exclusively expressed in germ cells. The DAZ family is highly conserved, with ancestral Boule present in sea anemones through humans, Dazl conserved among vertebrates, and DAZ present only in higher primates. Here we review studies on DAZ family genes from multiple organisms, and summarize the common features of each DAZ gene and their roles during spermatogenesis in animals. DAZ family proteins are thought to activate the translation of RNA targets, but recent work has uncovered additional functions. Boule, Dazl, and DAZ likely function through similar mechanisms, and we present known functions of the DAZ family in spermatogenesis, and discuss possible mechanisms in addition to translation activation.
Infertility affects approximately 10% of couples, with half of these cases attributable to
the male partner.1 Though many of these cases are
idiopathic, a high proportion of men with non-obstructive azoospermia (no sperm produced)
have a microdeletion on the Y chromosome.2 The
discovery of such deletions led to the proposal of an “Azoospermia Factor” (AZF) as a
genetic cause for some cases of infertility.2 The AZF
region has been further mapped into the three candidate regions AZFa, AZFb and AZFc,3,4 each deleted in
subsets of infertile men. Among the handful of genes in these regions, Deleted in
Azoospermia (DAZ) was found to be deleted in 12–15% of a cohort
of azoospermic men, making it a strong candidate for the AZFc gene.5
DAZ is part of a large gene family (DAZ family) with
autosomal homologs Dazl (DAZ-Like) and
Boule, all of which encode RNA-binding proteins.6-9
DAZ family genes are reproduction-specific and present in nearly all
animals,10 making them an important gene family in
reproduction. The identification of the DAZ family has led to research into
genetic causes of infertility, and expansive work into understanding how the
DAZ family regulates fertility.RNA-binding proteins are abundant during spermatogenesis, largely involved in
post-transcriptional regulation. During spermatogenesis, extensive translational regulation
is used to control the proper timing of differentiation, particularly during spermiogenesis,
the differentiation of round spermatids into mature sperm (reviewed in refs. 11, 12). Many
genes are transcribed several days before translation occurs, necessitating a network of
mRNA storage and translational control. In addition to mRNA regulation, multiple species of
non-coding small RNAs have been identified in the testis. These include miRNAs, piRNAs and
MSY-RNAs, though how they intersect with translation regulation and sperm differentiation is
unclear.13-18 Some of this RNA storage and control has been proposed to occur at the
chromatoid body, a perinuclear structure most prevalent in round spermatids that contains
mRNA, miRNA and several RNA-binding proteins (reviewed in ref. 19). The presence of such a structure and the abundance of multiple
classes of small RNAs highlight the importance of RNA binding proteins during
spermatogenesis.The DAZ family of proteins is thought to be involved in the translation activation of mRNA
targets.20,21 In recent years, relevant candidate targets have been identified, and the
mechanism underlying this regulation is becoming clearer. Additionally, novel roles for
DAZ family genes in mRNA transport and stability have been discovered.
Here we review the functions of the DAZ family of genes during
spermatogenesis, and discuss the various models of their action.
Evolution of the DAZ Gene Family
After the discovery of DAZ as a candidate gene for AZF,5 the identification of homologs in other species revealed
a larger gene family. DAZ family genes have a common structure consisting
of a RNA-Recognition Motif (RRM) and at least one copy of a motif rich in basic amino acids
termed the DAZ repeat.5,6,8,22-24
Boule is the ancestral member of the family, and is widely conserved across
Metazoan, from the sea anemone through humans (Fig. 1).10,23,25
Boule is autosomal and has a single RRM and one DAZ repeat.8,23,25 The RRM is highly conserved among all
Boule homologs, with a distinct signature in the RNP1 and RNP2 motifs
within the RRM. Boule is not found in fungi or plants, indicating that the
DAZ family is an animal specific family of reproduction genes.10
Figure 1.DAZ family evolution. Boule is
the ancestral member of the family, and is conserved from the sea anemone through
humans, but is not present in Trichoplax, fungi or plants. A duplication of
Boule during early vertebrate evolution led to Dazl.
Dazl was then duplicated and transposed onto the Y chromosome in the
evolution of old world monkeys. It further expanded into a cluster of multiple
DAZ genes in the evolution of human lineage. Symbols at right
indicate sex-specific roles. Boule has predominantly testis functions
with occasional ovarian roles, Dazl functions in testes and ovaries,
while DAZ is testis-specific.
Figure 1.DAZ family evolution. Boule is
the ancestral member of the family, and is conserved from the sea anemone through
humans, but is not present in Trichoplax, fungi or plants. A duplication of
Boule during early vertebrate evolution led to Dazl.
Dazl was then duplicated and transposed onto the Y chromosome in the
evolution of old world monkeys. It further expanded into a cluster of multiple
DAZ genes in the evolution of human lineage. Symbols at right
indicate sex-specific roles. Boule has predominantly testis functions
with occasional ovarian roles, Dazl functions in testes and ovaries,
while DAZ is testis-specific.Dazl arose from a duplication of Boule during vertebrate
evolution (Fig. 1).8,10Dazl homologs are also
autosomal with only one RRM and one DAZ repeat,6,9,22,24 and are distinguishable from Boule
homologs by unique sequences in the RNP1 and RNP2 motifs.8,10Dazl arose around the
time of vertebrate radiation, and homologs are conserved from bony fish through humans,6,9,10,22,24,26-28 but are not present in cartilaginous or jawless
fish.10During primate evolution, a duplication and transposition of Dazl onto the
Y chromosome led to DAZ (Fig. 1).6,7,29 Subsequent duplication and gene pruning led to four
DAZ genes in two clusters, each with multiple numbers of DAZ repeats and
two with duplications of the RRM.30 The number of DAZ
repeats among the DAZ genes is polymorphic both between and within
individuals.30,31
DAZ homologs are only present in humans and catarrhine primates (old world
monkeys).7,24,29,32Surprisingly, sequence analysis has shown that the presence of DAZ has had
little effect on either Dazl or Boule gene evolution in
primates, indicating strong functional constraint on these two genes.33
DAZ itself has a higher rate of genetic changes,34 but neither nonsense nor frameshift mutations affecting the ORF have
been detected, suggesting positive selection on DAZ.35
Dazl homologs have a higher rate of change than
Boule,33 while
Boule homologs have been shown to be under purifying selection.10 Indeed, no polymorphisms within the
Boule coding region were detected among more than 200 fertile and
infertile men examined in two different studies,8,36 further indicating a strong functional
constraint. Such a high level of conservation is rare among reproductive genes, suggesting
that Boule has an essential germ cell role in animals. Similarly, the
continued maintenance of multiple gene duplications suggests that all DAZ
family genes are critical regulators of fertility.
DAZ Family Gene Expression
Though each DAZ family gene has a unique expression pattern, the whole
family is restricted to germ cells in nearly all animals. Despite the presence of newer
members Dazl and DAZ, reproduction-specific expression has
been preserved for all three DAZ family genes. While there is some species
specific expression for each DAZ family homolog, each gene has maintained
the same general pattern across species. Gene families may often show similarities in
expression among species, but such clear conservation of homolog-specific expression is
unusual. This phenomenon allows a composite picture of common RNA and protein expression to
be constructed for each DAZ family homolog, summarized in Figure 2 (red and green lines, respectively). This summary
view does not represent the data from any single species, but rather the common expression
patterns seen in multiple organisms. Data from specific species is discussed below, with a
focus on each homolog’s common pattern of expression.
Figure 2. Common expression and functions of DAZ family
genes. Data from multiple species is combined to present a picture of common expression
patterns and functions for each DAZ gene during spermatogenesis. A
schematic of different steps of germ cell specification and spermatogenesis is shown at
top, and mRNA expression (red lines) and protein expression (green lines) relative to
these steps is shown for each gene. Black lines represent steps in spermatogenesis where
each gene is known to have a function. Solid lines represent data confirmed in at least
two studies, while dashed lines are either unconfirmed, or inferred from known
expression or function data. Boule protein is present in pachytene
spermatocytes through round spermatids (solid red line), and functions in both meiosis
and spermiogenesis (solid black line). Boule mRNA is presumed to be
present (dashed red line) in cells with Boule protein. Dazl homologs
are expressed continuously from embryonic stem cells through round spermatids (red and
green lines), and are known to function in ESCs, PGCs, gonocytes, spermatogonia and
early spermatocytes (solid black lines). Dazl likely functions in other
cells where it is expressed (dashed black line), but this has not been shown.
DAZ is known to be expressed in spermatogonia (solid green line), and
presumably functions in those cells, though it has not been shown (dashed black line).
For details, see text. ESC, embryonic stem cell; PGC, primordial germ cell; Spg,
spermatogonia; Early Spc, leptotene/zygotene spermatocyte; Pachy Spc, pachytene
spermatocyte; R. Spd, round spermatid; E. Spd, elongating spermatid.
Figure 2. Common expression and functions of DAZ family
genes. Data from multiple species is combined to present a picture of common expression
patterns and functions for each DAZ gene during spermatogenesis. A
schematic of different steps of germ cell specification and spermatogenesis is shown at
top, and mRNA expression (red lines) and protein expression (green lines) relative to
these steps is shown for each gene. Black lines represent steps in spermatogenesis where
each gene is known to have a function. Solid lines represent data confirmed in at least
two studies, while dashed lines are either unconfirmed, or inferred from known
expression or function data. Boule protein is present in pachytene
spermatocytes through round spermatids (solid red line), and functions in both meiosis
and spermiogenesis (solid black line). Boule mRNA is presumed to be
present (dashed red line) in cells with Boule protein. Dazl homologs
are expressed continuously from embryonic stem cells through round spermatids (red and
green lines), and are known to function in ESCs, PGCs, gonocytes, spermatogonia and
early spermatocytes (solid black lines). Dazl likely functions in other
cells where it is expressed (dashed black line), but this has not been shown.
DAZ is known to be expressed in spermatogonia (solid green line), and
presumably functions in those cells, though it has not been shown (dashed black line).
For details, see text. ESC, embryonic stem cell; PGC, primordial germ cell; Spg,
spermatogonia; Early Spc, leptotene/zygotene spermatocyte; Pachy Spc, pachytene
spermatocyte; R. Spd, round spermatid; E. Spd, elongating spermatid.At least one DAZ family homolog is expressed in nearly every stage of spermatogenesis.
Though spermatogenesis begins when spermatogonia differentiate, it can be traced back to the
differentiation of a subset of embryonic stem cells (ESCs) into primordial germ cells
(PGCs). These migrate to the embryonic gonad and become gonocytes (also called
prospermatogonia), which proliferate further and eventually become spermatogonia, containing
the adult stem cell population. Spermatogonia proliferate further and give rise to primary
spermatocytes, which undergo meiosis to produce haploid round spermatids. Through a process
called spermiogenesis, round spermatids undergo dramatic morphological changes and first
become elongating spermatids, and are finally released from the testis as mature
spermatozoa.Boule homologs are predominantly transcribed in the testes of fruit flies,
sea urchins, chickens, mice and primates,10 though
mRNA expression is reported in the ovaries of C. elegans, medaka fish and
at low levels in mice.10,25,37,38 However, in these three species, testis transcription is also
observed. Furthermore, since the only instance of Boule protein in ovaries is in C.
elegans,37Boule
transcriptions in the ovaries of fish and mice may not lead to protein. Similarly, we have
seen low levels of Boule mRNA in embryonic gonocytes in mice,10 but do not detect protein (our unpublished
observations). Additionally, boule mRNA is detected in the brains of
flies,39,40
but this has not been reported in any other animals.In the testis, Boule proteins are first present in mid-pachytene spermatocytes and remain
through metaphase spermatocytes, with peak levels occurring just before the metaphase of
cell division. Boule protein then persists into round spermatids, but is gone by the time
elongation begins (Fig. 2, Boule green line).8,41,42 This is true in flies, mice and humans.8,41 Cell-type
specific Boule mRNA expression has only been examined in medaka fish, where
it is similarly present in both spermatocytes and spermatids.38 This mRNA pattern is likely the same in both flies and mammals, given the
similar protein expression patterns, but it has not been confirmed.Dazl homolog expression has diverged from Boule, and
homologs are expressed in both males and females in all species so far examined.10Dazl homologs are initially expressed
in ESCs through PGC specification in frogs, fish and mammals (Fig. 2, Dazl red and green lines). In Xenopus, Xdazl mRNA and
protein are both present in the embryonic germ plasm,26,43 and zebrafishzDazl
mRNA is detected in the vegetal pole of embryos,28 a
region that later gives rise to germ cells.44
Similarly, mouseDazl mRNA and humanDAZL mRNA and protein
are present in ESCs through PGCs.45-47 Together, these expression data indicate common
expression of Dazl during PGC determination of early embryogenesis.After germ cells are specified, Dazl homologs continue to be expressed in
gonocytes, through spermatogonia and spermatocytes, and into early round spermatids (Fig. 2). Such protein expression is seen in humans, mice
and frogs,8,48-50 while underlying mRNA expression has
been confirmed in mammals only through pachytene spermatocytes.22,51-53 Though reports of post-meiotic Dazl expression in mammals have
differed,8,33,48 we have detected Dazl protein in both
mouse and human spermatids (our unpublished observations), and Dazl is present
post-meiotically in Xenopus.50
Additionally, a transgenic reporter driven by the Dazl promoter in mice has shown a similar
transcription pattern.54 Furthermore, one study found
humanDAZL protein in sperm tails,55 but this result
has not been repeated. Such discrepancies in the reports of Dazl expression are likely due
to the use of different antibodies recognizing varying antigens that are differentially
accessible during spermatogenesis. Despite the absence of confirmed protein and mRNA data at
each stage and slight variations in species-specific Dazl expression,32 a common pattern of continuous Dazl expression from ESCs through
haploid spermatids is clear (Fig. 2).While several papers have reported DAZ gene expression, a consensus
pattern is not yet clear. In addition to differing antibodies, cross-reactivity with Dazl
proteins was sometimes unavoidable. Habermann et al. found DAZ2 protein in mature sperm
tails,56 but this was not repeated in two other
studies.48,57 Using several antibodies to control for cross-reactivity with Dazl, Reijo et
al. showed that DAZ is present only in spermatogonia and spermatocytes, with rare expression
in spermatids.48 DAZ protein has been confirmed in
human spermatogonia, though not in spermatocytes (Fig. 2, DAZ green line).57 All four
DAZ genes are transcribed in humans,57 further complicating expression studies of DAZ.Interestingly, though DAZ family proteins are predominantly present in the cytoplasm,
occasional nuclear localization is also observed. In flies, Boule protein is initially in
the nucleus of early spermatocytes, and then transits to the cytoplasm just before
metaphase,41 though this is not seen in
mammals.8 Similarly, human and mouseDazl is nuclear
in gonocytes,48,58 and may translocate from the nuclei of spermatogonia into the cytoplasm of
spermatocytes.48 This translocation of Dazl has not
been confirmed, but nonetheless raises an intriguing question of why DAZ family proteins
localize to the nuclei of certain cell types. DAZ family proteins may sequester certain
transcripts in the nucleus, or could be involved in mRNA processing. However, nuclear
localization of DrosophilaBoule is dispensable for its function, raising the possibility
that Boule is simply stored in the nucleus prior to its function in the cytoplasm.41 However, the common presence of Dazl in the nuclei of
spermatogonia in multiple species suggests important functionality. What this role is
remains to be seen, but will likely be important in fertility.
Functions of DAZ Genes During Spermatogenesis
Because of the broad evolutionary conservation of the DAZ family, the
functions of DAZ genes have been examined in a number of species, revealing
requirements for DAZ family genes at multiple points during spermatogenesis
(summarized in Figure 2, black lines).
DAZ is known to be important in human spermatogenesis since its deletion
is associated with azoospermia.5 However, causative
point mutations in infertile men have yet to be identified, and some DAZ
deleted men still produce low levels of sperm.59
Indeed, men with DAZ deletions have fathered children both through the use
of reproductive technologies60,61 and, though rare, naturally,3,62 indicating that DAZ
is not absolutely required for spermatogenesis. However, the presence of
DAZ within the AZFc region as well as studies detailed below about
spermatogenesis requirements of other DAZ family members strongly suggest
that DAZ plays a critical role in normal spermatogenesis.In accordance with its broad expression pattern, Dazl has been shown to
have multiple roles throughout spermatogenesis. In frogs and mice, Dazl is
initially important for PGC proliferation and development. Knockdown of XenopusXdazl leads to few surviving PGCs, and those that do survive fail to
migrate.43 Similarly, Dazl
knockout mice have few germ cells that survive into the adult, in both males and
females.49 This defect is first evident at the
gonocyte stage in embryonic testes. In a mixed genetic background, Dazl
null testes are sparsely populated with germ cells by embryonic day 19 (E19),49 while increased germ cell apoptosis is seen by E14.5
in a pure C57/Bl6 background.63 Additionally,
Dazl null ESCs fail to differentiate to PGCs in vitro, while PGCs in vivo
fail to properly erase genomic methylation marks.45
These defects together indicate a problem in PGC development and differentiation, similar to
those seen in Xenopus. Though few PGCs are present in Dazl
null mice and frogs, the presence of germ cells indicates that germ cell specification is
occurring in the absence of Dazl. However, the in vitro ESC differentiation
defect may hint at a role in germ cell specification.Further studies on Dazl null mice on a mixed genetic background have shown
additional roles for Dazl in both spermatogonia and early spermatocytes.
Though most germ cells are absent at birth, some As (A-single) and Apr
(A-paired) spermatogonia survive, but most do not progress beyond the Aal
(A-aligned) stages, revealing a function for Dazl in spermatogonia
differentiation.64 The few cells that do pass this
block are able to enter meiosis, but synaptonemal complexes necessary for homologous
recombination fail to form in postnatal day 19 (p19) knockout mice, and spermatocytes cannot
progress beyond leptonema.65 Null germ cells in the
pure C57/Bl6 background fail to induce meiosis genes in response to the meiotic signal
retinoic acid, showing a further requirement for Dazl at the onset of
meiosis.66 This range of defects is specific to
germ cells, as wild type spermatogonia can colonize and repopulate a Dazl
null testis.67 Taken together, Dazl
has functions during PGC development and migration, spermatogonia differentiation and the
onset and progression of meiosis (Fig. 2).
Dazl presumably also functions between these known steps, corresponding
to known expression, but explicit demonstrations of such roles have not yet been shown.Boule functions complement those of Dazl, and homologs
are important for meiotic division and spermatid differentiation. In Drosophila,
boule mutant flies have a male-specific arrest at pachynema, prior to
metaphase.23 However, meiosis completes normally in
Boule knockout mice, and haploid round spermatids are abundant.42 Instead, there is a global arrest at step 6 of
spermiogenesis, with varying defects in acrosome biogenesis and a complete lack of
elongating spermatids.42 Despite the lack of a
meiosis phenotype in Boule null mice, Boule regulation of
meiosis is likely conserved among animals. A pachytene arrest similar to that seen in flies
occurs in C. elegans with a mutation in the Boule homolog
daz-1, but only in females.25 In
addition, a humanBOULE transgene can restore meiosis in
boule mutant flies,68 and a lack
of BOULE protein has been associated with meiotic arrest in men.36 We therefore proposed that Dazl and
Boule redundantly regulate the progression to meiotic metaphase in mice,
and that Dazl can compensate for the loss of Boule in
spermatocytes.42 While this model has not yet been
tested, the accumulating evidence suggests that Boule regulation of meiosis
is conserved in mammals.Additionally, though knockout mice revealed a novel role for Boule in
spermatid differentiation, this function may also be present in flies. In
boule mutant flies, it was noted that the pachytene-arrested
spermatocytes did not differentiate,23 a phenotype
not common to other meiosis-arrest mutants. For example, flies with a mutation in the
putative Boule target, twine, have a similar meiotic arrest, but many
meiosis-arrested spermatocytes in those flies begin to elongate.69,70 Since differentiation was
also disrupted in Drosophilaboule mutants, this suggests that the
spermiogenesis function of Boule is also conserved.Regardless of which specific spermatogenesis roles are conserved, the male-fertility
requirement of Boule is the same between flies and mice. Despite more than
500 million years of evolution separating mice and flies, Boule mutations
in both species lead to a complete lack of sperm due to a global arrest in spermatogenesis,
and the presence of similar-looking multinucleate cysts in the testis (Fig. 3). Furthermore, these testes defects are the only phenotype reported
in Boule null animals of either species,10,23,39,40,42 highlighting the conservation of a male fertility requirement of
Boule.
Figure 3.Boule testis function is conserved in flies and
mice. Despite the wide divergence of flies and mice, Boule mutations in
each species leads to male-only sterility due to a global arrest of spermatogenesis.
Mature sperm (red arrowhead) and elongating spermatids (black arrowhead) are abundant in
the testis tube of wild type flies, the same is true for the wild type mouse testis
section. Mature sperm (red arrowhead) are seen in the lumen of seminiferous tubules and
elongating spermatids are often located next to the lumen (black arrowhead). However
both mature sperm and elongating spermatids are completely absent in
Boule knockout testes of both species. Multinucleate cysts are
prevalent throughout null testes of both animals (arrows), further highlighting the
conserved spermatogenesis function of Boule. Fly testes are from 1-d
old males, and images taken at 10x. Mouse testes are from 3 mo old mice, and images
taken at 10x. Myr-million years.
Figure 3.Boule testis function is conserved in flies and
mice. Despite the wide divergence of flies and mice, Boule mutations in
each species leads to male-only sterility due to a global arrest of spermatogenesis.
Mature sperm (red arrowhead) and elongating spermatids (black arrowhead) are abundant in
the testis tube of wild type flies, the same is true for the wild type mouse testis
section. Mature sperm (red arrowhead) are seen in the lumen of seminiferous tubules and
elongating spermatids are often located next to the lumen (black arrowhead). However
both mature sperm and elongating spermatids are completely absent in
Boule knockout testes of both species. Multinucleate cysts are
prevalent throughout null testes of both animals (arrows), further highlighting the
conserved spermatogenesis function of Boule. Fly testes are from 1-d
old males, and images taken at 10x. Mouse testes are from 3 mo old mice, and images
taken at 10x. Myr-million years.Many experiments have shown a remarkable ability of the DAZ family genes
to functionally replace each other. Both humanDAZ and
DAZL can partially restore germ cell numbers in Dazl
null mice, though the rescue was moderate and variable among animals.71,72 These experiments showed
that humanDAZ can function during mammalian spermatogenesis, despite the
lack of direct evidence that DAZ is necessary for human spermatogenesis.
Interestingly, XenopusXdazl can restore meiosis in boule
mutant flies,26 similar to the humanBOULE rescue discussed above,68
further supporting the model of Boule and Dazl redundancy
during mammalian meiosis.42Finally, all three DAZ family genes have been shown to enhance human ESC
differentiation into germ cells in vitro, with overexpression of each DAZ
family gene alone or in combination leading to varying degrees of enhancement.46 When all three were expressed together, ESCs were able
to differentiate into germ cells with molecular features of spermatids, highlighting the
wide range of functions DAZ family genes play in spermatogenesis. A similar
transient overexpression of Dazl in mouse ESCs was also able to promote
germ cell differentiation.73 These ectopic expression
studies may not reflect in vivo functions, however. For example, Boule
overexpression enhanced PGC differentiation in XX (female) ESCs, but not XY (male)
ESCs.46 However, Boule expression
has not been reported in ESCs of either sex, and Boule null female mice
have no germ cell defects.10,42 While these experiments suggest in vivo roles for the ESC-expressed
Dazl, the results for Boule and DAZ
underscore the ability for compensation among the DAZ family when expressed
in the right time and place. Together with the data that different homologs can functionally
replace each other, the similar in vitro results for each DAZ family gene
suggest that all DAZ family genes can function through similar
mechanisms.
Candidate RNA Targets for DAZ Family Proteins
Though many functions of DAZ family genes are known (discussed below),
relevant and validated RNA targets are less clear. Drosophilaboule
enhances translation of a Lac-Z reporter carrying the 3′ UTR of the Cdc25
homolog twine in vivo, suggesting that the fly germ cell-specific
Cdc25 homolog is the downstream target of Boule.74 In addition, a twine transgene with a
tubulin 3′ UTR was able to rescue meiosis in boule
mutant flies, indicating that twine translation is absent in mutants.
Though this model nicely explains the observed meiosis arrests in both Drosophila and
C. elegans,8,25,74 no direct interaction
between any Boule and Cdc25 homologs has been shown.Subsequent research into targets has focused on Dazl homologs. In
homopolymeric binding studies, frog, mouse and humanDazl preferentially
bind polyU RNA.26,75 A SELEX approach identified a (G/CUn)n motif which is
found in the 5′UTR of mouseCdc25c,76 and zebrafishzDazl binds to GUUC, a site found in the 3′UTR
of Drosophila twine RNA.77 Using
GST-Dazl bound to a column, a 26bp motif was identified that is present in the
Cdc25a 3′ UTR.78 Another study
identified targets bound by both Dazl and Pumilio2 (Pum2),79 an RNA-binding protein shown to interact with Dazl.80 Follow-up studies confirmed Dazl binding to a U-rich
motif in Sdad1 mRNA, another cell-cycle regulator first identified in
yeast.79However, despite multiple reports of candidate targets, there is no overlap between lists,
and a discrepancy in the Dazl binding site, perhaps due to the in vitro approaches used in
these experiments. Binding conditions are unlikely to match those found in vivo, mRNAs
normally in separate cells from Dazl are inappropriately brought together, or legitimate
targets may be tightly bound by endogenous protein, therefore preventing their binding to
Dazl in vitro. To determine in vivo targets, Reynolds et al. used endogenous
immunoprecipitation from whole mouse testes followed by a microarray on co-precipitating
RNA, and identified 15 targets with high confidence.81 Targets were further validated by IP followed by RT-PCR on UV-crosslinked
testes to reduce non-specific interactions. Dazl binding to Mvh
(Mousevasa homolog) and Sycp3 (Synaptonemal
complex protein 3) has been confirmed, and translation defects for both of these
targets occurs in Dazl null animals.81,82Additionally, the presence of the proposed binding sites in the 15 target genes was
analyzed.81 The initial 26bp motif78 was only found in six targets, and was not present
significantly more than predicted by chance.81 The
SELEX defined (G/CUn)n motif, however, was statistically
over-represented in the 3′UTRs of targets, and was found to be in evolutionarily conserved
regions of the transcripts. This motif was also found in the eight targets previously
reported by Jiao et al.,81 providing strong support
for a common U2–10(G/C)U2–10 binding motif among Dazl targets. It is
not known how prevalent this motif is among testis transcripts, but the flexible nature of
this motif suggests that Dazl may bind a wide range of mRNAs.Notably, using in vivo UV-crosslinking followed by IP and RT-PCR, Reynolds et al. failed to
detect Dazl binding to Prm2,81 a
target identified by an in vitro screening method.79
This experiment showed that while in vitro binding studies can correctly uncover a
particular binding motif, the specific targets identified may not be relevant in vivo.
Therefore, while multiple studies have examined targets of Dazl, only a few candidates have
in vivo significance.The most promising in vivo targets are Mvh, Sycp3, and
Cdc25 homologs (Table 1). Three
reports showing Dazl binding to Cdc25 homologs76-78 together with meiosis rescue
studies in flies26,68,74 is strong evidence for in vivo
Cdc25 binding. Mice have three Cdc25 genes,83,84 and Venables
et al. only detected binding to Cdc25c,76 while Jiao et al. could only detect binding to Cdc25a.78 Both of these Cdc25 genes are
abundantly expressed in the testis,83,84 and whether the differential binding is due to the
different techniques used, or represents artificial binding due to the in vitro systems
remains to be seen.
Table 1. Candidate in vivo mRNA targets
Gene
Candidate Target
Motif Bound
References
Fly boule, Zebrafish zDazl
twine
GUUC
74, 77
Mouse Dazl
Cdc25
Cdc25c 5′ UTR
GU7GU10GU10GU7
76
Cdc25a 3′UTR
U/AA/GUUC/UAGUAU/AAANAACUUUG/UGAAU/AUG/A
78
Mvh
UUCUUCUGUUCUU
81
Sycp3
U6GU3GU3GU4
81, 82
Though many mRNA targets have been reported, the in vivo candidates shown fulfill
three criteria: (1) demonstrated in vivo binding, (2) reported translational defect in
Boule or Dazl null animal model and (3) functional
relevance to Boule or Dazl null phenotype.
Though many mRNA targets have been reported, the in vivo candidates shown fulfill
three criteria: (1) demonstrated in vivo binding, (2) reported translational defect in
Boule or Dazl null animal model and (3) functional
relevance to Boule or Dazl null phenotype.Mvh and Sycp3 were both identified by the in vivo
approach,81 and are related to known
Dazl functions. Mvh is highly expressed in all germ
cells, similar to Dazl, and Vasa homologs have conserved
roles in PGC differentiation.85 In addition, the male
sterile phenotype in Mvh knockout mice is due to a final arrest at
zygonema,85 close to the reported leptotene arrest
seen in mixed background Dazl null mice.65 Similarly, Sycp3 is an essential part of the synaptonemal
complex that forms during the early stages of meiosis, a time when Dazl has
been shown to function.45,65,66 A demonstrated in vivo
interaction, translation defects in knockouts and relevance to the observed phenotype
together make these genes the best candidate targets so far reported, though none of these
targets are a “magic bullet” that explains the primary Dazl null phenotype.
Similar physiologically relevant data are needed for other reported targets in order to
confirm their in vivo regulation by Dazl.Using a similar in vivo immunoprecipitation approach, we have identified the first
candidate targets for Boule in mice (VanGompel and Xu, in preparation). We were able to
detect interactions between Boule and Prm1 and Prm2 mRNAs,
genes important for round spermatid differentiation. While not a complete list, these
targets are directly relevant to the major phenotype of spermiogenesis arrest in
Boule null mice.
The DAZ Family as Translational Activators
Most studies have focused on the DAZ family as translational activators.
This model was first established through the studies in Drosophila discussed above,
implicating boule in the translational regulation of
twine.74 Similarly, zebrafishzDazl can stimulate translation of a luciferase reporter fused to the
twine 3′ UTR in cell culture.77
Using a tethered assay in Xenopus oocytes in which proteins were forced
into proximity of reporter mRNAs, Dazl homologs stimulated translation through enhanced
recruitment of 80S ribosomes.86 This translation
activation was dependent on an interaction with Poly(A) Binding Protein 1 (PABP1), but still
occurred in the absence of poly(A) tails on reporter constructs. This led to a model in
which Dazl recruits PABP1 to mRNAs in the absence of an adequate poly(A) tail, and thus
promotes translation.86 This model is particularly
intriguing in the context of mammalian spermatogenesis because several transcripts are known
to be deadenylated prior to translation.87,88 Xdazl was similarly shown to activate translation of
RINGO/Spy mRNA, but in a Pum2 dependent manner.89 Dazl bound target mRNA, but could not activate translation until the
translational repressor Pum2 dissociated from the transcript. This shows that the function
of the DAZ family is context dependent, and may vary depending on the stage
of spermatogenesis and what other proteins are present at any given time (Fig. 4). Additionally, while the general mechanisms are
likely to be broadly conserved, the specific contexts and players involved may differ among
species. Further studies into how other interacting proteins regulate DAZ family function
will prove fruitful.
Figure 4. Model for DAZ family gene functions. DAZ family
proteins likely function through similar mechanisms and a composite model representing
known cytoplasmic functions of DAZ family proteins is presented. A generic DAZ family
protein (orange circle labeled “D”) bound to RNA is represented in the middle of the
figure. DAZ family proteins have multiple functions, likely dependent on which protein
partner they are bound to. Binding to PABP1 promotes association with ribosomes and
translation, while binding to the repressor Pum2 inhibits translation. Interactions with
Dynein may mediate transport of mRNA targets. Where mRNA is transported is unknown, but
DAZ family proteins may transport targets to and from RNA granules, such as the
chromatoid body, or to polysomes for translation activation. DAZ family proteins may
promote mRNA stability either through the inhibition of miRNA-mediated degradation, or
the promotion of polyadenylation through binding to an unknown factor (beige circle
labeled “?”). Increased stability may enhance translation, or vice versa. Solid lines
represent known mechanisms, while open double-sided arrows represent speculated links
between known roles.
Figure 4. Model for DAZ family gene functions. DAZ family
proteins likely function through similar mechanisms and a composite model representing
known cytoplasmic functions of DAZ family proteins is presented. A generic DAZ family
protein (orange circle labeled “D”) bound to RNA is represented in the middle of the
figure. DAZ family proteins have multiple functions, likely dependent on which protein
partner they are bound to. Binding to PABP1 promotes association with ribosomes and
translation, while binding to the repressor Pum2 inhibits translation. Interactions with
Dynein may mediate transport of mRNA targets. Where mRNA is transported is unknown, but
DAZ family proteins may transport targets to and from RNA granules, such as the
chromatoid body, or to polysomes for translation activation. DAZ family proteins may
promote mRNA stability either through the inhibition of miRNA-mediated degradation, or
the promotion of polyadenylation through binding to an unknown factor (beige circle
labeled “?”). Increased stability may enhance translation, or vice versa. Solid lines
represent known mechanisms, while open double-sided arrows represent speculated links
between known roles.While these studies examined the mechanism of DAZ family function in vitro, others have
shown a similar translational role in vivo. MammalianDazl is present in active polysomes in
mouse testes,75 and Drosophilaboule
enhances the translation of a transgenic reporter through the twine 3′
UTR.74 As discussed previously, translation of the
two Dazl candidate targets, Mvh and
Sycp3, was reduced in Dazl null testes, further suggesting
that Dazl is a translational activator in vivo.81,82 Protein of these targets was still
detectable in Dazl knockouts, however, indicating that Dazl is acting as an
enhancer of translation, and not an essential activator as proposed in the
Boule-Cdc25 model. While the combined evidence for the
translational regulation of mRNA targets is strong, it is important to note that these data
cannot yet account for the dramatic loss of germ cells in Dazl null mice.
Key targets that regulate germ cell numbers may not yet be identified, or alternate
functions that have broader effects may cause the observed phenotype.
Non-Translational Roles for the DAZ Family
In addition to translation activation, DAZ family genes have other roles.
Several binding partners have been identified (Table
2, Figure 4), and interactions with other
RNA-binding proteins is a common theme. The mammalian proteins can form homo- and
heterodimers,8,58,80,90 further indicating similar functions, and suggesting a possible mechanism for
the flexibility in functionality observed in ectopic rescue studies. The translational
repressor Pum2 can bind all three DAZ members in humans.80,90 PABP1 can interact with Boule, Dazl
and DAZ homologs from frog, mouse and humans,86 while
Xdazl also interacts with ePABP (embryonic PABP),86,89 and C. elegansDAZ-1
interacts with the CPEB (Cytoplasmic Polyadenylation Element Binding protein) homolog
Cpb-3.91 Both humanDAZ and DAZL have also been
shown to interact with RNA-binding proteins hQK3 and DAZAP1.80,92 In addition, novel, non-RNA-binding
proteins DZIP1, and DAZAP2 have been identified as binding partners through interaction
screens with DAZ and DAZL.80,92,93 Such a variety of
interactions further supports a model of context-dependent DAZ family function, where
specific protein partners mediate a range of roles (Fig. 4). Indeed, which RNA targets DAZ family proteins are bound to may also
depend on the context of other protein partners. The Pumilio family of RNA-binding proteins
has been shown to differentially bind RNA targets based on what protein partners they are
bound to,90 and DAZ family proteins may utilize a
similar mechanism for binding different targets.
Table 2.
DAZ family interacting proteins
Gene
Category
Partners
References
Boule
DAZ Family
Boule, Dazl, DAZ
8, 80, 90
RNA-Binding Proteins
PABP1, Pum2, Cpb-3
86, 90, 91
Dazl
DAZ Family
Boule, Dazl, DAZ
8, 55, 80, 90
RNA-Binding Proteins
PABP1, ePABP, Pum2, hQK3,
DAZAP1
80, 86, 90, 92
Other
Dynein, Dzip1, DAZAP2
80, 92, 95
DAZ
DAZ Family
Boule, Dazl
55, 80
RNA-Binding Proteins
PABP1, Pum2, hQK3, DAZAP1
80, 86, 92
Other
Dzip1, DAZAP2
80, 92, 93
MouseDazl was also found to interact with dynein light chain in mouse testes, and can move
on the microtubule network in cell culture (Fig. 4).94 In a dynein-dependent manner in
vitro, Dazl can transport mRNA carrying putative binding sites, including those found in
candidate targets Tpx-1, Cdc25c and Mvh,
on microtubules. These mRNAs formed perinuclear aggregates, at structures presumed to be
stress granules, where ectopic Dazl also accumulated.94 Active mRNA transport in male germ cells is not well-studied, but has been
reported. The testis specific kinesin KIF17b can shuttle protein-RNA complexes in and out of
the nucleus,95 and also associates with Miwi and the
chromatoid body (CB),96 suggesting transport of mRNA
to and from the CB. In other cell types, mRNA is stored in stress granules to protect
transcripts from degradation,97,98 a parallel the authors propose occurs with Dazl-bound targets.94 Further studies are needed to determine if Dazl
transports targets to the CB or other RNA granules in germ cells, and whether other DAZ
family proteins are similarly involved in transport.Could the DAZ family transport RNA for safe storage? If protecting mRNA from degradation is
important in spermatogenesis, what is the targeting mechanism? A likely candidate is through
specific miRNAs (Fig. 4). miRNAs are known to inhibit
translation of targets, and this inhibition is often due to miRNA-mediated mRNA
degradation.99 ZebrafishzDazl was
recently shown to prevent miRNA mediated decay of nanos1 and
tdrd7 transcripts,100though
direct binding to these mRNAs was not shown. Using injections into zebrafish
embryos, the authors showed that zDazl prevents miRNA mediated inhibition
of reporters, dependent on the presence of the GUUC binding motif. Furthermore, this motif
does not overlap with the miRNA binding site, but was necessary for zDazl to stabilize the
mRNA.100 Since miRNA is present in the chromatoid
body, it is an intriguing possibility that DAZ family proteins are either protecting targets
from miRNA within the CB, or are involved in transporting them away from miRISC (microRNA
Induced Silencing Complex) in germ cells.While surprising, reduction of mRNA levels of Dazl targets has also been
reported. Though reduced translation was noted for Mvh and
Sycp3 in Dazl null mice, transcripts were reduced in
postnatal day 5 (P5) null testes, a result that contributed to their identification as
targets.81 This instability was presumed to be a
consequence of reduced translation, but a direct stability effect could not be ruled
out.81 Furthermore, quantitative RT-PCR using
Dazl null embryonic testes has also shown a reduction in mRNA of both of
these targets.45,66 Those experiments focused on the ability of Dazl null germ
cells to respond to meiosis signals, so the reduction was noted only as a failure to
initiate meiosis. Additionally, a microarray study on P7 wild type and Dazl
null testes found a large number of transcripts that were reduced in knockouts.101 A similar result was obtained in a human microarray
study on men with DAZ deletions.102
These studies hint at a potential role for the DAZ family in maintaining
RNA levels, though a direct role for this in vivo has not yet been shown. Determining if
reductions in transcript levels are due to a direct loss of DAZ family
genes will clarify these new data.Finally, in the zebrafish miRNA study described above, zDazl induced polyadenylation of
transcripts, a novel function for the DAZ family. This polyadenylation was
independent of translation, indicating that mRNA stability is independent from translation
activation. Furthermore, polyadenylation may be an alternate method of PABP recruitment and
subsequent translation activation. How zDazl mediates polyadenylation is not known, but it
is likely through an as yet unidentified binding partner (Fig. 4). Cytoplasmic polyadenylation is well described during oogenesis (reviewed
in ref. 103), and is beginning to be appreciated in
spermatogenesis.104 In one well-studied mechanism
in females, CPEB binds to cytoplasmic polyadenylation elements and recruits the
polyadenylation apparatus. As mentioned, C. elegansDAZ-1 interacts with a
CPEB homolog,91 suggesting a role for
DAZ family genes in polyadenylation in worms. In mice, knockout of the
testis-specific cytoplasmic poly(A) polymerase Tpap leads to a
spermiogenesis arrest similar to that seen in Boule knockouts.42,105 Whether
Boule and Tpap interact is not known, but the similar knockout phenotypes suggest that they
may function in the same pathway, perhaps through regulation of mRNA stability. It is also
possible that translation activation is a consequence of increased mRNA stability through
polyadenylation, and not a direct function of the DAZ family. Determining
how Boule regulates targets will help determine if such mechanisms are
broadly used, and what roles they play in spermatogenesis.
Conclusion
Recent findings are painting a new picture for DAZ family-mediated
regulation of targets, beyond the simple model of translation activation. Their roles in
translation activation have been well-established using many systems, but likely represent
only one of many functions. Specific mechanisms may differ in the broad range of cell types
in which this family functions, and DAZ family genes may play multiple
roles within the same cells. This range of functions may be determined in part by which
proteins the DAZ family is bound to at any given time. Yet despite the variety of functions
and mechanisms, the DAZ proteins have been highly conserved, and can still functionally
replace each other in limited contexts. Such strong selective pressure on reproductive genes
is rare, and suggests an essential role for these genes in the germ cells of animals. While
possible mechanisms are emerging, why these functions are required in germ cells of all
animals, and why humans require more DAZ family genes than other species,
are puzzles that remain. Much work is needed to address these interesting questions.
Authors: Amander T Clark; Megan S Bodnar; Mark Fox; Ryan T Rodriquez; Michael J Abeyta; Meri T Firpo; Renee A Reijo Pera Journal: Hum Mol Genet Date: 2004-02-12 Impact factor: 6.150
