Onversion to the cyst cell lineage (Voog et al, unpublished data). To determine the fate of lost hub cells, we first assayed for conversion to the cyst lineage by combining expression of a hdcRNAi transgene with the G-TRACE lineage-tracing cassette; G-TRACE allows both a real-time readout of GAL4 activity (dsRed), as well as a permanent lineage marker (GFP) in cells that are expressing or derived from GAL4 expressing cells (Fig. 3) [25]. There was no indication that reduced levels of hdc influenced the ability of hub cells to maintain their identity, as similar numbers of marked (GFP+) cells were observed outside the hub in testes from control (7 , N = 44), hdcRNAi3 (12 , N = 85), and hdcRNAi1 (15 , N = 20) G-TRACE males dissected at 5, 10 and 15 days. No significant difference was found between controls and experimental conditions (Chi-square test, P = 0.68). Next, we assayed for the presence of apoptotic hub cells upon reduction 11967625 of hdc. Consistent with previous studies, apoptotic hub cells were rarely observed in wild-type testes (1/113 testes analysed) [18]. In contrast, a significant increase in the number of apoptotic hub cells was detected when hdc levels were reduced (12/131 testes analysed; Fisher’s exact test, P = 0.0036) (Fig. 4A). Based on hub cell counts at 1d vs 10d, approximately one hub cell is lost per day (Fig. 1B and 2B); therefore, the low frequency of testes found containing apoptotic cells is likely due to technical limitation of the detection method used. 1315463 Consistent with our observations, loss of hub cells due to reduction of hdc was suppressed by expression ofHeadcase Regulates Maintenance of the Clavulanic acid potassium salt chemical information Testis NicheFigure 2. Hub cell loss is evident using multiple paradigms and is not due to developmental defects. (A to A”’) Strong hub cell loss marked by staining for FasIII (see Fig. 1C and F) was confirmed with other hub cell markers [DE-Cadherin (DE-Cad), DN-Cadherin (DN-cad) and Armadillo (Arm)] Hub cells pointed by white dots. (B) Hub cell quantification in flies where hdcRNAi expression by updGal4 was suppressed at 18uC during development, and activated at 25uC (without Gal80ts; hdcRNAi2 and hdcRNAi3) or 29uC (with Gal80ts; hdcRNAi1) for 1, 10, and 15 days. Means and SD are shown; ***P,0.001 (Kruskal allis one-way analysis of variance). (C) Loss of hub cells is observed using an alternative hub driver (FasIIIGal4). Testis from FasIIIGal4; UAS-hdcRNAi1 male at 5 days (compare to Fig. 1E); Scale bars 20 mm. doi:10.1371/journal.pone.0068026.gthe anti-apoptotic baculovirus protein, p35, which has been shown to supress cell death efficiently in Drosophila (Fig. 4B ) [26]. In addition, a loss of hub cells was observed when the pro-apoptotic factors head involution defective (hid) and reaper (rpr) were co-expressed in hub cells (Table 1). Lecirelin Similarly, apoptotic hub cells were detected (N = 3/39) and hub cells were lost upon RNAi-mediated knockdown of the anti-apoptotic factor, DIAP2 (Fig. 4D ). Based on these results, we conclude that apoptosis was a likely cause for loss of hub cells in respose to reduced levels of hdc. These data represent the first, direct association of this gene with programmed cell death and highlight the role of cell survival pathways in maintenance of the apical hub.Hub Area, Rather than Number, Determines Stem Cell PoolHub cells represent a crucial component of the testis stem cell niche, serving both a structural role, as well as a localized source of self-renewal signals [8] [9] [27]. However, i.Onversion to the cyst cell lineage (Voog et al, unpublished data). To determine the fate of lost hub cells, we first assayed for conversion to the cyst lineage by combining expression of a hdcRNAi transgene with the G-TRACE lineage-tracing cassette; G-TRACE allows both a real-time readout of GAL4 activity (dsRed), as well as a permanent lineage marker (GFP) in cells that are expressing or derived from GAL4 expressing cells (Fig. 3) [25]. There was no indication that reduced levels of hdc influenced the ability of hub cells to maintain their identity, as similar numbers of marked (GFP+) cells were observed outside the hub in testes from control (7 , N = 44), hdcRNAi3 (12 , N = 85), and hdcRNAi1 (15 , N = 20) G-TRACE males dissected at 5, 10 and 15 days. No significant difference was found between controls and experimental conditions (Chi-square test, P = 0.68). Next, we assayed for the presence of apoptotic hub cells upon reduction 11967625 of hdc. Consistent with previous studies, apoptotic hub cells were rarely observed in wild-type testes (1/113 testes analysed) [18]. In contrast, a significant increase in the number of apoptotic hub cells was detected when hdc levels were reduced (12/131 testes analysed; Fisher’s exact test, P = 0.0036) (Fig. 4A). Based on hub cell counts at 1d vs 10d, approximately one hub cell is lost per day (Fig. 1B and 2B); therefore, the low frequency of testes found containing apoptotic cells is likely due to technical limitation of the detection method used. 1315463 Consistent with our observations, loss of hub cells due to reduction of hdc was suppressed by expression ofHeadcase Regulates Maintenance of the Testis NicheFigure 2. Hub cell loss is evident using multiple paradigms and is not due to developmental defects. (A to A”’) Strong hub cell loss marked by staining for FasIII (see Fig. 1C and F) was confirmed with other hub cell markers [DE-Cadherin (DE-Cad), DN-Cadherin (DN-cad) and Armadillo (Arm)] Hub cells pointed by white dots. (B) Hub cell quantification in flies where hdcRNAi expression by updGal4 was suppressed at 18uC during development, and activated at 25uC (without Gal80ts; hdcRNAi2 and hdcRNAi3) or 29uC (with Gal80ts; hdcRNAi1) for 1, 10, and 15 days. Means and SD are shown; ***P,0.001 (Kruskal allis one-way analysis of variance). (C) Loss of hub cells is observed using an alternative hub driver (FasIIIGal4). Testis from FasIIIGal4; UAS-hdcRNAi1 male at 5 days (compare to Fig. 1E); Scale bars 20 mm. doi:10.1371/journal.pone.0068026.gthe anti-apoptotic baculovirus protein, p35, which has been shown to supress cell death efficiently in Drosophila (Fig. 4B ) [26]. In addition, a loss of hub cells was observed when the pro-apoptotic factors head involution defective (hid) and reaper (rpr) were co-expressed in hub cells (Table 1). Similarly, apoptotic hub cells were detected (N = 3/39) and hub cells were lost upon RNAi-mediated knockdown of the anti-apoptotic factor, DIAP2 (Fig. 4D ). Based on these results, we conclude that apoptosis was a likely cause for loss of hub cells in respose to reduced levels of hdc. These data represent the first, direct association of this gene with programmed cell death and highlight the role of cell survival pathways in maintenance of the apical hub.Hub Area, Rather than Number, Determines Stem Cell PoolHub cells represent a crucial component of the testis stem cell niche, serving both a structural role, as well as a localized source of self-renewal signals [8] [9] [27]. However, i.