Drosophila Importin Alpha 1 (Dα1) Is Required to Maintain Germline Stem Cells in the Testis Niche

Stem cell maintenance and differentiation can be regulated via the differential activity of transcription factors within stem cells and their progeny. For these factors to be active, they need to be transported from their site of synthesis in the cytoplasm into the nucleus. A tissue-specific requirement for factors involved in nuclear importation is a potential mechanism to regulate stem cell differentiation. We have undertaken a characterization of male sterile importin alpha 1 (Dα1) null alleles in Drosophila and found that Dα1 is required for maintaining germline stem cells (GSCs) in the testis niche. The loss of GSCs can be rescued by ectopic expression of Dα1 within the germline but the animals are still infertile, indicating a second role for Dα1 in spermatogenesis. Expression of a Dα1 dominant negative transgene in GSCs confirmed a functional requirement for Dα1 in GSC maintenance but expression of the transgene in differentiating spermatogonia did not exhibit a phenotype indicating a specific role for Dα1 within GSCs. Our data indicate that Dα1 is utilized as a regulatory protein within GSCs to facilitate nuclear importation of proteins that maintain the stem cell pool.


Introduction
Transport of proteins and RNA molecules across a nuclear membrane that separates the nucleus from the cell cytoplasm is an essential function of all eukaryotes.In development, cellular differentiation is dependent upon the efficient transportation of proteins that are synthesized in the cytoplasm but are required in the nucleus to interact with DNA.These can include transcription factors, histones and cell cycle regulators, all of which are important for the regulation of cell fate dynamics (reviewed in [1,2]).Karyopherins, a multigene family of nuclear transport receptors, mediate the transport of large macromolecules (cargo) across the nuclear pore complexes (NPCs) into the nucleus (importins) or out of the nucleus (exportins) (reviewed in [3,4]).
The purported classical nuclear import pathway asserts that cargo greater than about 50 kDa containing a classical nuclear localisation signal (cNLS) binds to a specific Importin α protein, which functions as an adaptor to link cNLS-cargos to Importin β1 [5,6].This complex then passes through the NPC by binding phenylalanine-glycine (FG) repeats present in many nucleoporins.Following translocation into the nucleus, the importin-cargo complex dissociates in the presence of high RAN-GTP and the free importin proteins are recycled back to the cytoplasm (reviewed in [3,7]).
Selective transport of cargo such as transcription factors is possible due to the capacity of individual importin αs to preferentially bind different cargoes [8,9].Vertebrate Importin αs are expressed in distinct cell-and tissue-specific patterns, further enabling the nuanced control of nuclear import [10][11][12].Importin α family members are divided into three clades: the 3rd chromosome approximately 12 kb in length and covers Dα1 and 6 other genes.The Z5234 loss of function allele is caused by a point mutation resulting in a premature stop codon at amino acid 202, while the Z1703 loss of function allele is caused by a point mutation resulting in a premature stop codon at amino acid 343; (B) Schematic depiction of Drosophila spermatogenesis.Germline stem cells (1) surround somatic hub cells (yellow).A pair of Cyst progenitor cells (grey) surround the GSC.Circular arrow depicts the self-renewal capacity of the GSC.Gonialblasts (2), progeny of GSCs, are surrounded by a pair of differentiated somatic cyst cells (grey).Gonialblasts undergo four rounds of mitosis (3)(4)(5)(6).Spermatogonia differentiate into spermatocytes (7) and undergo meiosis (8-9) to produce 64 round spermatids (9).(10) shows early elongating spermatids (only 4 depicted), (11) shows 4 elongating spermatids; (C,D) phase contrast microscopy shows the tip of the Drosophila testes.Testes have been outlined in red.(C) A testis dissected from a w 1118 newly eclosed adult shows the presence of germline cells at all stages of early spermatogenesis, including small undifferentiated germline stem cells and gonialblasts to differentiating spermatogonia and spermatocytes (the stem cell niche that includes stem cells, gonialblasts and spermatogonia is indicated by the white line); (D) Homozygous Df(3L)α1S1 testes lack young germ cells.Large germline cysts containing fewer than 16 cells are present in the apex of the homozygous Df(3L)α1S1 testis (outlined in yellow).Cells within the cyst appear to be spermatocytes.Scale Bars, 5 µm.

Phase Contrast Microscopy
Testes were dissected in Ringers solution and 3-4 individual testes were immediately mounted under a glass coverslip in Ringers solution.The slide was then imaged immediately as the testes flatten under the pressure of a coverslip and removal of liquid by lateral flow.Testes were imaged using a Zeiss Axioskop2 Plus microscope (Carl Zeiss Pty Ltd., Macquarie Park, NSW, Australia).The images were taken using a 20X objective.

Statistical Analysis and Creation of Graphs
GraphPad Prism version 7.01 was used to analyse data and prepare graphs, significant difference was calculated using the students t-test.Results were considered significant if p < 0.05.Error bars on all graphs represent the standard error of the mean.

Mutations in Dα1 Cause a Loss of Spermatogonial Germline Stem Cells
The effects of Dα1 mutations on later stages of Drosophila spermatogenesis have previously been described [28]; however, no reports have detailed a functional requirement for Dα1 in the regulation or maintenance of germline stem cells (GSCs).To investigate this, we dissected and analysed testes from homozygous Df(3L)α1S1 flies, which carry a small chromosomal deletion covering the Dα1 gene and six neighbouring genes (Figure 1A).
Spermatogenesis in Drosophila adults is well described (Figure 1B; reviewed in [29,30]).GSCs reside at the apical tip of a tubular testis, and these stem cells asymmetrically divide to self-renew and produce differentiated daughter cells called gonialblasts (GB).In a process similar to mammalian spermatogenesis, each gonialblast undergoes four rounds of mitosis with incomplete cytokinesis to generate a cyst of 16 primary spermatocytes.Spermatocytes, after growth, undergo meiosis with incomplete cytokinesis to form a cyst of 64 interconnected haploid spermatids, which are then converted into mature sperm in a process known as spermiogenesis.Previous reports have attributed male sterility in homozygous Df(3L)α1S1 flies to loss of Dα1 since expression of a UAS-Dα1 transgene driven by an Act5CGal4 driver could rescue sterility [28].To further characterise the cause of male sterility, we dissected testes from Df(3L)α1S1 mutant flies and examined the cellular morphology of the testes using phase contrast microscopy.Testes dissected from homozygous Df(3L)α1S1 flies appeared aberrant in morphology, lacking early germ cells which are normally easily identifiable under phase contrast microscopy (Figure 1C,D).Additionally, atypical cysts of less than 16 large germ cells resembling spermatocytes were frequently observed at the apical tip of mutant testes, suggestive of early spermatogenesis defects (Figure 1D), which are not observed in wildtype testes (Figure 1C).We could not rule out the possibility that the morphological defects observed in homozygous Df(3L)α1S1 mutant testes were due to a loss of function of any of the six other genes affected by the chromosomal deletion.To explore the impact of Dα1 loss on the initial stages of spermatogenesis, we bred two Drosophila strains harbouring point mutations in the Dα1 gene (Figure 1A), previously induced by ethyl methanesulfonate (EMS) treatment [31], with Df(3L)α1S1 mutants.These alleles have been described as homozygous viable and male sterile [32], but in our hands, they were homozygous lethal but survived as adults when transheterozygous with Df(3L)α1S1.Subsequently, we examined the resulting transheterozygote mutant testes using immunofluorescence (Figure 2A-D).Compared to heterozygous Df(3L)α1S1/+ controls, the morphological defects in each of Df(3L)α1S1/Df(3L)α1S1, Df(3L)α1S1/Dα1 Z5234 and Df(3L)α1S1/Dα1 Z1703 appeared similar.A loss of Vasa-positive early germ cells from around the somatic quiescent hub cells (labelled with an antibody to detect Drosophila E-cadherin) was evident in all genotypes, as was the presence of spermatocytes close to the apical hub (Figure 2B-D).Quantification of the number of Vasa-positive GSCs in direct contact with the hub in adults at seven days posteclosion revealed a significant loss of GSCs from each of the mutant genotypes compared to w 1118 control testes.These results suggest an essential role for Dα1 in the maintenance of Drosophila GSCs.

Expression of Dα1 in the Germline of Df(3L)α1S1/Df(3L)α1S1 Mutants Can Rescue GSC Loss, but Not Sterility
Although we have shown the necessity for Dα1 for sustaining Drosophila GSCs through analysis of homozygous or transheterozygote flies, it remains unclear if its requirement is intrinsic to GSCs or if Dα1 is required within the surrounding somatic cells, which serve as the GSC niche.To further assess whether Dα1 is required in GSCs for their maintenance, we expressed a UAS-Dα1 transgene in the germline of Df(3L)α1S1/Df(3L)α1S1 mutants using a nanos-Gal4 driver, which selectively drives ex- Although we have shown the necessity for Dα1 for sustaining Drosophila GSCs through analysis of homozygous or transheterozygote flies, it remains unclear if its requirement is intrinsic to GSCs or if Dα1 is required within the surrounding somatic cells, which serve as the GSC niche.To further assess whether Dα1 is required in GSCs for their maintenance, we expressed a UAS-Dα1 transgene in the germline of Df(3L)α1S1/Df(3L)α1S1 mutants using a nanos-Gal4 driver, which selectively drives expression in GSCs and spermatogonial cells [33], and subsequently assayed for GSC rescue.Newly eclosed control UAS-Dα1/CyO; Df(3L)α1S1/TM6B heterozygous males were fertile, and immunofluorescence confirmed that testes displayed no obvious morphological abnormalities (Figure 3A-A"').In contrast, UAS-Dα1/CyO; Df(3L)α1S1/Df(3L)α1S1 males in the absence of nanos-Gal4 were sterile as expected, and testes dissected from newly eclosed males exhibited a loss of early Vasapositive germ cells from around the hub (Figure 3B-B"').After driving expression of UAS-Dα1 with nanos-Gal4 in the Dα1 deficiency background, testes dissected from newly eclosed nos-Gal4/UAS-Dα1; Df(3L)α1S1/Df(3L)α1S1 exhibited no obvious morphological defects indicative of a rescue of early germ cells, including GSCs (Figure 3C-C"').Additionally, a significantly higher number of GSCs were observed in testes dissected from nos-Gal4/UAS-Dα1; Df(3L)α1S1/Df(3L)α1S1 newly eclosed males compared to testes dissected from UAS-Dα1/CyO; Df(3L)α1S1/Df(3L)α1S1 males at the same age point (Figure 3D), supporting the notion that Dα1 is required for the proper regulation and maintenance of GSCs.We mated at least nine individual nos-Gal4/UAS-Dα1; Df(3L)α1S1/Df(3L)α1S1 males with 3-4 w 1118 females, and all remained sterile despite the rescue of early germ cells, which suggests a requirement for Dα1 at different stages or within multiple cell types throughout spermatogenesis.This observation is consistent with the pattern of Dα1 mRNA, which is detected in early germ cells and more highly in spermatocytes (Supplementary Figure S1).Our analysis to date has shown a requirement for Dα1 in the maintenance of GSCs.Interestingly, quantification of GSC numbers in testes dissected from newly eclosed Dα1 mutant adults (Figure 3D) and aged flies (Figure 2E) indicated that loss of Dα1 results in the progressive loss of GSCs over time.We questioned whether challenging Dα1 mutants by increasing the temperature at which they were raised would affect the rate of GSC loss, as ezymatically driven developmental processes may be expected to be more rapid at higher temperatures, perhaps pointing to a function for Dα1 in regulating the rate of GSC division.To this end, we characterised (by immunofluorescence) testes dissected from newly eclosed Df(3L)α1S1/Dα1 Z5234 mutant flies raised at either 18 • C, 25 • C or 29 • C from the time of mating.Testes dissected from w 1118 (control) adult males reared at 25 • C and Df(3L)α1S1/Dα1 Z5234 mutants reared at 18 • C appeared similar in morphology (Figure 4A-B"'), and mutant testes exhibited no obvious cellular defects (Figure 4B-B"').In contrast, testes dissected from Df(3L)α1S1/Dα1 Z5234 reared at either 25 • C or 29 • C exhibited a loss of Vasa-positive germ cells (Figure 4C-C"').Quantification of the number of GSCs in each of these samples confirmed that the severity of stem cell loss in Df(3L)α1S1/Dα1 Z5234 correlated with an increase in temperature (Figure 4E), with mutants reared at 29 • C exhibiting similar GSC numbers to testes dissected from newly eclosed Df(3L)α1S1 homozygotes raised at 25 • C (Figure 4E).This is suggestive of the temperature-sensitive nature of Dα1 Z5234, but these results also raise the possibility that other genes lost as a result of the deficiency could contribute to the loss of function phenotype in the homozygote deficiency strain.notion that Dα1 is required for the proper regulation and maintenance of GSCs.We at least nine individual nos-Gal4/UAS-Dα1; Df(3L)α1S1/Df(3L)α1S1 males with 3females, and all remained sterile despite the rescue of early germ cells, which sugg requirement for Dα1 at different stages or within multiple cell types throughout spe ogenesis.This observation is consistent with the pattern of Dα1 mRNA, which is de in early germ cells and more highly in spermatocytes (Supplementary Figure S1).

Expression of a Dα1 Dominant Negative Transgene in GSCs Confirms a Functional Requirement for Dα1 in GSC Maintenance
Whole-mutant analysis has revealed the importance of Dα1 in the regulation of GSC maintenance.To further determine the specificity of the role of Dα1 in germ cell maintenance, we generated a Dα1 dominant negative transgene (UAS-Dα1 DN ), which could be expressed in a cell-specific manner using the bipartite GAL4-UAS system.Based on sequence conservation of importin genes between Drosophila melanogaster, Xenopus, Yeast and Human, we generated a truncated copy of the Dα1 coding sequence, which would result in the removal of the conserved importin β binding site [34][35][36] at the N terminus (Figure 5A).This construct was subsequently cloned into a pTMW Gateway vector with a 5x Myc tag and a pUASt promoter sequence.Driving expression of UAS-Dα1 DN in GSCs using nanos-Gal4 resulted in the loss of Vasa-positive GSCs from the somatic hub (Figure 5C-C"'), a phenotype that was observed in Df(3L)α1S1 homozygotes and Df(3L)α1S1/Dα1 Z5234 transheterozygotes.Quantification of the number of GSCs in testes dissected from nanos-Gal4; UAS-Dα1 DN flies showed a significant loss of GSCs in both newly eclosed and aged adults (Figure 5D), and consistent with our previous results, we observed a progression of the severity of the phenotype with age.The persistence of Vasa-positive mature spermatocytes in the apex of the testis at 7 days post-eclosion (Figure 5C"') suggested to us that GSCs are progressively lost from the niche through premature differentiation rather than cell death and is consistent with the observation that in Dα1 mutants, GSCs are lost over time.

Expression of a Dα1 Dominant Negative Transgene in Differentiated Germ Cells Does Not Affect Germ Cell Development/Differentiation
Our analysis has suggested that the loss of Dα1 from GSCs results in their premature differentiation.We hypothesised that if the Dα1 dominant negative transgene caused excess death in early germ cells, then driving the transgene in differentiated daughters should similarly lead to a loss of spermatogonial cells.To test this, we drove the dominant negative transgene specifically in differentiated germ cells using the bam-Gal4 driver.The native bam gene is expressed in spermatogonia, but bam is repressed in GSCs by BMP signalling [37].Testes dissected from both newly eclosed and aged bam-Gal4; UAS-Dα1 DN flies appeared morphologically similar to testes dissected from control flies when analysed by immunohistochemistry and confocal microscopy, with no obvious cellular defects (Figure 6A-C).These results support a requirement for Dα1 in GSC maintenance and prevention of premature differentiation of stem cells in the Drosophila testis.

Expression of a Dα1 Dominant Negative Transgene in Differentiated Germ Cells Does Not Affect Germ Cell Development/Differentiation
Our analysis has suggested that the loss of Dα1 from GSCs results in their premature differentiation.We hypothesised that if the Dα1 dominant negative transgene caused excess death in early germ cells, then driving the transgene in differentiated daughters should similarly lead to a loss of spermatogonial cells.To test this, we drove the dominant negative transgene specifically in differentiated germ cells using the bam-Gal4 driver.The native bam gene is expressed in spermatogonia, but bam is repressed in GSCs by BMP signalling [37].Testes dissected from both newly eclosed and aged bam-Gal4; UAS-Dα1 DN flies appeared morphologically similar to testes dissected from control flies when analysed by immunohistochemistry and confocal microscopy, with no obvious cellular defects (Figure 6A-C).These results support a requirement for Dα1 in GSC maintenance and prevention of premature differentiation of stem cells in the Drosophila testis.

Discussion
The original characterisation of Df(3L)α1S1 reported that homozygotes were malesterile and that dissected testes contained morphologically abnormal cysts of spermatocytes.This chromosomal deficiency deletes the coding sequence of six genes in addition to Dα1, but the phenotype was specifically associated with the loss of Dα1 function due to the ability of Act5C-Gal4 and UASp-Dα1 to rescue the fertility defect [28].Phase contrast imaging of live testes and immunostaining of fixed tissue both allowed us to identify that Dα1 is also required for maintaining GSCs in the niche.We too observed abnormal spermatocyte cysts, and immunofluorescence studies using anti-Vasa to mark pre-meiotic germ cells enabled us to determine that, in addition to a loss of GSCs, the apical region of the testis contained cysts of spermatocytes (in positions where we would normally expect to find GSCs and spermatogonia) that contained variable numbers of cells, less than the normal number of 16 spermatocytes per cyst.This suggests to us that GSCs and spermatogonia are lost from the testis due to premature differentiation into spermatocytes.We also confirmed that the loss of early germ cells was specifically associated with the loss of Dα1 function, as transheterozygotes of two independent alleles of Dα1 (containing premature termination codons) combined with Df(3L)α1S1 recapitulated the phenotype observed in Df(3L)α1S1 homozygotes.
We were also able to determine that the loss of GSCs and spermatogonia was due to a cell intrinsic requirement for Dα1, as we could rescue the germ cell loss via the expression of a Dα1 transgene from a germ cell-specific promoter.Studies in mammalian cells have utilised dominant negative importin alpha alleles that have deletion of the importin-beta binding domain, which blocks importin alpha function by preventing it from transporting targets through the nuclear pore [34][35][36].We generated an analogous transgene in Drosophila, which demonstrated a similar phenotype to the loss of Dα1 alleles when driven by a germ cell-specific promoter.Moreover, this transgene displayed the loss of GSC and spermatogonia phenotype when combined with a Gal4 driver that expressed in GSCs and spermatogonia (nanos-Gal4) but not when combined with a driver that only expressed in the 4-16 cell stages of spermatogonia (bam-Gal4).These data imply that Dα1 is specifically required in GSCs (and potentially very early spermatogonial stages) and that a reduction in Dα1 function in maturing spermatogonia does not impact cell survival or differentiation of early germ cells.Df(3L)α1S1 homozygotes exhibit degradation of spermatocytes (Supplementary Figure S1), suggesting that Dα1 is required in later germ cells, so it is also possible that the level of expression from bam-Gal4 was not sufficient to induce a dominant negative phenotype.
We also found the phenotype associated with loss of Dα1 (in a truncation mutant in trans to the deficiency) to be temperature-sensitive, with a more severe phenotype associated with elevated temperature.The reason for this sensitivity is not clear at present, but it may be associated with increased cellular metabolism and cell turnover at higher temperatures.Interestingly, the loss of GSCs in Df(3L)α1S1 at 25 • C was only equivalent to Dα1 Z5234 /Df(3L)α1S1 at 29 • C, suggesting that although it has been reported that Act5c-Gal4-driven-Dα1 can rescue the fertility of Df(3L)α1S1 homozygotes [28], one of the other six genes included within the deficiency may also play a role in GSC maintenance.
The Ratan (2008) study also showed that ectopic expression of Dα2 or Dα3 could not rescue infertility associated with Df(3L)α1S1 homozygotes, implying a paralogue-specific role for importins in the testis.These data are consistent with importin alpha genes having different targets, and therefore specific importins are associated with specific cell biological and developmental roles.All three importin alpha genes are highly expressed in spermatocytes but appear not to be redundant, as loss of only Dα1 in Df(3L)a1S1 (Supplementary Figure S1) results in these cells eventually degrading and not producing spermatids.
The importance of ensuring that the correct importin is expressed at the correct time can be demonstrated by a study that showed Dα2 must be excluded from Drosophila primordial germ cells (pole cells) for their development.A critical aspect of germ cell development is the prevention of inappropriate expression of somatic genes [38].The RNA-binding protein Nanos has been shown to inhibit translation of maternally supplied Dα2 in pole cells, and this inhibition of Dα2 activity is required to prevent nuclear import of the Ftz-F1 transcription factor, which subsequently allows transcription of somatic genes if inappropriately expressed in the germline [39].
There may also be sex-specific requirements for importin alphas, as the Sex lethal mRNA-binding protein regulates Dα3 expression in Drosophila female primordial germ cells.Experiments that knocked down the combination of maternal and zygotic Dα3 activity in embryos demonstrated a subsequent decrease in the number of GSCs present in adults in ovaries, with some ovaries being devoid of germ cells, but no apparent effect in testes [40].
Although Dα1 mutants have been reported as viable but infertile, they do have other phenotypes.Dα1 plays an important role in setting the circadian clock within specific neurons via regulating the nuclear entry of the Period and Timeless clock proteins.Flies that have Dα1 knocked down within clock neurons exhibit arrhythmic behaviour [41], demonstrating that Dα1 has a unique set of functional requirements within specific tissues.
A greater understanding of importin function will not only facilitate our understanding of developmental processes but may uncover an important mechanism to combat disease phenotypes.Pathological variants of the Tau protein have been linked to Alzheimer's disease, and, more broadly, are associated with a group of neurodegenerative diseases known as tauopathies.A study that utilised pharmacological inhibitors of importin activity was able to prevent nuclear importation of pathological Tau proteins and inhibit the cell death that is associated with their expression [42].In a similar manner, genetic experiments in Drosophila have shown that Dα3 is required for the transportation of a pathogenic truncated Ataxin-3 variant protein into nuclei, which then results in neuronal toxicity [43].

Conclusions
This study has demonstrated a role for Dα1 in maintaining the germline stem cell pool within the Drosophila testis niche.We do not yet know what proteins are imported via a Dα1-specific mechanism that is critical for GSC function.This will clearly be important to understand why Dα1 has a specific requirement in male GSCs.Future studies are also needed to determine if Dα1 is required in other stem cell populations within adult Drosophila or if paralogous importin alphas have specific roles in stem cells associated with other tissues.

Figure 1 .Figure 1 .
Figure 1.Loss of Dα1 gene function results in defects in spermatogenesis.(A) Image of Dα1 and surrounding genes modified from Flybase.Deficiency Df(3L)α1S1 deletes a region of the left arm on the 3rd chromosome approximately 12 kb in length and covers Dα1 and 6 other genes.The Z5234 loss of function allele is caused by a point mutation resulting in a premature stop codon at amino acid 202, while the Z1703 loss of function allele is caused by a point mutation resulting in a premature stop codon at amino acid 343; (B) Schematic depiction of Drosophila spermatogenesis.Germline stem cells (1) surround somatic hub cells (yellow).A pair of Cyst progenitor cells (grey) surround the GSC.Circular arrow depicts the self-renewal capacity of the GSC.Gonialblasts (2), progeny of Figure 1.Loss of Dα1 gene function results in defects in spermatogenesis.(A) Image of Dα1 and surrounding genes modified from Flybase.Deficiency Df(3L)α1S1 deletes a region of the left arm on

Figure 5 .
Figure 5. Expression of a dominant negative Dα1 transgene driven in early germ cells results in a failure of stem cell maintenance.(A) Alignment of the Xenopus Importin α (isoform 1b) importin β binding domain against Human Rch1, Yeast SRP1, Human Importin α homologue, Drosophila Dα3, Human SRP1, Drosophila Dα1 and Drosophila Dα2.Full length amino acid sequence for Dα1 with the sequence removed in the creation of the dominant negative highlighted in yellow.Representative confocal micrographs of testes dissected from (B-B''') w 1118 and (C-C''') nanos-Gal4; UAS-Dα1 DN

Figure 5 .
Figure 5. Expression of a dominant negative Dα1 transgene driven in early germ cells results in a failure of stem cell maintenance.(A) Alignment of the Xenopus Importin α (isoform 1b) importin β binding domain against Human Rch1, Yeast SRP1, Human Importin α homologue, Drosophila Dα3, Human SRP1, Drosophila Dα1 and Drosophila Dα2.Full length amino acid sequence for Dα1 with the sequence removed in the creation of the dominant negative highlighted in yellow.Representative confocal micrographs of testes dissected from (B-B"') w 1118 and (C-C"') nanos-Gal4; UAS-Dα1 DN adult

Figure 6 .
Figure 6.Expression of a dominant negative Dα1 transgene in differentiated germ cells results in no visible defects in early spermatogenesis.Representative confocal micrographs of testes dissected from (A-A''') w 1118 control adults, and testes dissected from (B-B''') newly eclosed bam-Gal4; UAS-Dα1 DN adults and (C-C''') aged adults.Labelling of testes with Dapi (DNA), Myc (to control for the presence of the tagged dominant negative transgene), D-Cad (hub and cyst cells) and Vasa (germ cells) reveals no obvious defects when the transgene is driven in the differentiated germ cells as opposed to GSCs.Scale Bars, 20 µm.

Figure 6 .
Figure 6.Expression of a dominant negative Dα1 transgene in differentiated germ cells results in no visible defects in early spermatogenesis.Representative confocal micrographs of testes dissected from (A-A"') w 1118 control adults, and testes dissected from (B-B"') newly eclosed bam-Gal4; UAS-Dα1 DN adults and (C-C"') aged adults.Labelling of testes with Dapi (DNA), Myc (to control for the presence of the tagged dominant negative transgene), D-Cad (hub and cyst cells) and Vasa (germ cells) reveals no obvious defects when the transgene is driven in the differentiated germ cells as opposed to GSCs.Scale Bars, 20 µm.