Fig 1.
Presence and localization of CaMKKα in chicken sperm.
Chicken sperm lysates (45μg of protein) were analyzed by western blotting using anti- CaMKKα as primary antibody. Cell lysates from chicken muscle (40μg of protein) were used as positive control. A band of approximately 50kDa for CaMKKα was detected (1A). Indirect immunofluorescence of chicken sperm was carried out with the same antibody. Negative control: primary antibody was not added (1B). White arrows and circles in transmission images indicate areas of the acrosome (arrow 1), the nuclei (arrow 2), the midpiece (circle), and the principal piece of the flagellum (arrow 3) in sperm (1C). Immunofluorescence staining of CaMKKα (1D, green) was conducted; nuclei were stained with DAPI (1E, blue). Merged images of fluorescence with DAPI staining are shown in Fig 1F (white arrows and circles indicate regions containing CaMKKα immunoreactivity: arrow 1: acrosome; arrow 3: principle piece; circle: midpiece). Scale bar: 10μm.
Fig 2.
Presence and localization of CaMKKβ in chicken sperm.
Chicken sperm lysates (45μg of protein) were analyzed by western blotting using anti- CaMKKβ as primary antibody. Cell lysates from chicken muscle (40μg of protein) were used as positive control. A band of approximately 65kDa for CaMKKβ was detected (2A). Indirect immunofluorescence of chicken sperm was carried out with the same antibody. Negative control: primary antibody was not added (2B). White arrows and circles in transmission images indicate areas of the acrosome (arrow 1), the nuclei (arrow 2), the midpiece (circle), and the principal piece of the flagellum (arrow 3) in sperm (2C). Immunofluorescence staining of CaMKKβ (2D, green) was conducted; nuclei were stained with DAPI (2E, blue). Merged images of fluorescence with DAPI staining are shown in Fig 2F (white arrows indicate regions containing CaMKKβ immunoreactivity: arrow 1: acrosome; arrow 3: principle piece; circle: midpiece). Scale bar: 10μm.
Fig 3.
Presence and localization of CaMKI in chicken sperm.
Chicken sperm lysates (45μg of protein) were analyzed by western blotting using anti- CaMKI as primary antibody. Cell lysates from chicken muscle (40μg of protein) were used as positive control. A band of approximately 41kDa for CaMKI was detected (3A). Indirect immunofluorescence of chicken sperm was carried out with the same antibody. Negative control: primary antibody was not added (3B). White arrows and circles in transmission images indicate areas of the acrosome (arrow 1), the nuclei (arrow 2), the midpiece (circles), and the principal piece of the flagellum (arrow 3) in sperm (3C). Immunofluorescence staining of CaMKI (3D, green) was conducted; nuclei were stained with DAPI (3E, blue). Merged images of fluorescence with DAPI staining are shown in Fig 3F (white arrows indicate regions containing CaMKI immunoreactivity: arrow 1: acrosome; arrow 3: principle piece; circle: midpiece). Scale bar: 10μm.
Fig 4.
Presence and localization of CaMKIV in chicken sperm.
Chicken sperm lysates (45μg of protein) were analyzed by western blotting using anti- CaMKIV as primary antibody. Cell lysates from mouse testis (40μg of protein) are used as positive control. A band of approximately 60kDa for CaMKIV was detected (4A). Indirect immunofluorescence of chicken sperm was carried out with the same antibody. Negative control: primary antibody was not added (4B). White arrows and circles in transmission images indicate areas of the acrosome (arrow 1), the nuclei (arrow 2), the midpiece (circles), and the principal piece of the flagellum (arrow 3) in sperm (4C). Immunofluorescence staining of CaMKIV (4D, green) was conducted; nuclei were stained with DAPI (4E, blue). Merged images of fluorescence with DAPI staining are shown in Fig 4F (white arrows indicate regions containing CaMKIV immunoreactivity: arrow 3: principle piece). Scale bar: 10μm.
Fig 5.
Effect of extracellular Ca2+ on chicken sperm motility and viability.
Sperm were incubated for up to 60 min at 35°C in medium without Ca2+ (white) or containing different concentrations of Ca2+: 0.5mM (diagonal brick bars), 2.5mM (horizontal bars), 5mM (grey bar), 10mM (diamond bars). The percentages of motile (A) and viable (B) sperm after 5, 15, 30 and 60 min of incubation were determined as described in the Materials and Methods section. The results are expressed as mean ± SEM, n = 6. Different superscripts indicate statistically significant differences (P < 0.05).
Fig 6.
Effect of extracellular Ca2+ on chicken sperm AR.
Sperm were incubated for up to 60 min at 35°C in medium not supplemented with Ca2+ (-5mM Ca2+, white bar) or containing 5mM Ca2+ (+5mM Ca2+, grey bar). The percentages of successful sperm AR after 5, 15, 30 and 60 min of incubation were determined as described in the Materials and Methods section. The results are expressed as mean ± SEM, n = 6. Different superscripts letters indicate statistically significant differences (P < 0.05).
Fig 7.
Effect of extracellular Ca2+ on the AMPK phosphorylation in chicken sperm.
Sperm were incubated at 35°C in the –5mM Ca2+ or +5mM Ca2+ medium. Proteins from sperm lysates were analyzed by western-blotting using anti-phospho-Thr172-AMPKα or anti-AMPKα as primary antibody. Bands for phospho-Thr172-AMPKα were detected at 62kDa (top lanes). Total AMPKα (62kDa) was used as loading control (bottom lanes) and the phosphorylated protein AMPKα (Thr172)/total AMPKα ratio is shown at the bottom. A) Effects of increased intracellular 5mM Ca2+ on the AMPK phosphorylation after 5 min of incubation. B) Effect of STO-609 on AICAR induced AMPK phosphorylation: sperm were incubated with STO-609 for 5 min before adding 1mM AICAR and incubated 5 min more. The control: sperm incubated in the medium with DMSO. Results express the mean ± SEM of the mean from 6 different experiments. Different superscripts indicate statistically significant differences (P < 0.05).
Fig 8.
Effects of CaMKKs (STO-609) inhibitor on the AMPK phosphorylation in chicken sperm.
Sperm were incubated at 35°C in the –5mM Ca2+ or +5mM Ca2+ medium with or without CaMKKs inhibitor STO-609 (1; 10; 50 μM) for 5 min and 15 min. Proteins from sperm lysates were analyzed by western-blotting using anti-phospho-Thr172-AMPKα or anti-AMPKα as primary antibody. Bands for phospho-Thr172-AMPKα were detected at 62kDa (top lanes). Total AMPKα (62kDa) was used as loading control (bottom lanes) and the phosphorylated protein AMPKα (Thr172)/total AMPKα ratio is shown at the bottom. A) Effects of different concentrations of STO-609 on the AMPK phosphorylation in sperm incubated for 5 min or 15 min. The control (Ctrl): sperm incubated with or without Ca2+ in the absence of STO-609. B) Effects of 10μM STO-609 on the AMPK phosphorylation in sperm incubated for 5, 15, 30, 60 min. The control (Ctrl): sperm incubated 0 min with or without Ca2+ in the absence of STO-609. Results express the mean ± SEM of the mean from 6 different experiments. Different superscripts indicate statistically significant differences (P < 0.05).
Fig 9.
Effect of extracellular Ca2+ on the CaMKI phosphorylation in chicken sperm.
Sperm incubated at 35°C for 5 min in the –5mM Ca2+ or +5mM Ca2+ medium with or without CaMKKs inhibitor STO-609. The control (Ctrl): sperm incubated in the absence both +5mM Ca2+ and 10μM STO-609. Proteins from sperm lysates were analyzed by western-blotting using anti-phospho-Thr177-CaMKI or anti-CaMKI as the primary antibody. Bands for phospho-Thr177-CaMKI were detected at 41kDa (top lanes). Total CaMKI (41kDa) was used as loading control (bottom lanes) and the phosphorylated protein CaMKI (Thr177)/total CaMKI ratio is shown at the bottom. Results express the mean ± SEM of the mean from 4 different experiments. Different superscripts indicate statistically significant differences (P < 0.05).
Fig 10.
Effects of STO-609 on the CaMKI phosphorylation in chicken sperm.
Sperm incubated at 35°C in the –5mM Ca2+ or +5mM Ca2+ medium with or without CaMKKs inhibitor STO-609 (0; 1; 10; 50 μM) at 5 min and 15 min. The control (Ctrl): sperm incubated with or without Ca2+ in the absence of STO-609. Proteins from sperm lysates were analyzed by western-blotting using anti-phospho-Thr177-CaMKI or anti-CaMKI as the primary antibody. Bands for phospho-Thr177-CaMKI were detected at 41kDa (top lanes). Total CaMKI (41kDa) was used as loading control (bottom lanes) and the phosphorylated protein CaMKI (Thr177)/total CaMKI ratio is shown at the bottom. Results express the mean ± SEM of the mean from 4 different experiments. Different superscripts indicate statistically significant differences (P<0.05).
Fig 11.
Effects of STO-609 on the CaMKIV phosphorylation in chicken sperm.
Sperm incubated at 35°C in the –5mM Ca2+ or +5mM Ca2+ medium with or without CaMKKs inhibitor STO-609 (0; 1; 10; 50 μM) at 5 min and 15 min. The control (Ctrl): sperm incubated with or without Ca2+ in the absence of STO-609. Proteins from sperm lysates were analyzed by western-blotting using anti-phospho-Thr196-CaMKIV or anti-CaMKIV as the primary antibody. Bands for phospho-Thr196-CaMKIV were detected at 60kDa (top lanes). Total CaMKIV (60kDa) was used as loading control (bottom lanes) and the phosphorylated protein CaMKIV (Thr196)/total CaMKIV ratio is shown at the bottom. Results express the mean ± SEM of the mean from 4 different experiments. There were no significant differences between treatments (P<0.05).
Table 1.
Effect of STO-609 treatment on the percentage of sperm motility (%).
Table 2.
Effects of CaMKK inhibitor STO-609 (10μM) on sperm motility parameters.
Table 3.
Effect of STO-609 treatment on chicken sperm AR (%).
Table 4.
Effect of STO-609 treatment on chicken sperm viability (%).
Fig 12.
Proposed scheme of Ca2+ signaling pathways leading to regulation of AMPK activity in avian sperm.
This schematic diagram shows potential mechanisms of calcium role through CaMKK stimulation in chicken sperm. They all activate AMPK and CaMKI, which leads to metabolic improvements, leading themselves to the control of sperm functions. Solid arrows and blocked arrows illustrate more established relationships between stimuli, signals, improved metabolic status and control of avian sperm functions. Solid black arrows indicate Ca2+/CaMKKs/AMPK signaling pathway. Dashed black arrows indicate Ca2+/CaM/CaMKKs/CaMKI signaling pathway. Curved arrows (black) indicate AMPK phosphorylation, CaMKI phosphorylation; dashed grey arrows with a question mark are used for hypotheses.