Animal Procedures and Sperm Preparation

All animal procedures were performed in accordance with NIH guidelines and approved by the Animal Care and Use Committee of the National Institute of Environmental Health Sciences. Mice from 12 to 32 wk of age were euthanized by CO₂ asphyxiation followed by cervical dislocation. This study was performed with animals from the third and fifth generations backcrossed with wild-type (WT) C57BL/6N mice.

Cauda epididymides collected in 1× PBS (Ca²⁺/Mg²⁺-free) were carefully dissected to remove blood vessels and fat, several small cuts were made with iridectomy scissors, and sperm were allowed to swim out in 1 ml PBS for 10 min at room temperature (RT). To remove residual substrates present in the epididymal fluid, sperm were washed by dilution in 13 ml PBS and by gentle centrifugation (10 min at 300 × g) at RT. The sperm pellet was suspended in 1 ml TYH, and the number of spermatozoa determined using a hemocytometer. Sperm were diluted to the appropriate concentration in TYH medium and incubated for selected lengths of time at 37°C in 5% CO₂ in humidified air. Sperm viability was determined by dye exclusion using Hoechst 33258 [16]. In experiments involving use of sodium oxamate, the inhibitor was added to TYH medium, and the equivalent molar amount of NaCl was removed to maintain osmotic equivalence.

JC-1 Assay

Sperm mitochondrial membrane potential in WT, Ldhc^+/− (HET) and Ldhc^−/− (KO) sperm was examined by staining with the supravital fluorescent dye JC-1 (5,5′,6,6′-tetrachloro-1,1′,3,3′-tetraethylbenzimidazolyl-carbocyanine chloride). Sperm were incubated at 37°C in 5% CO₂ in humidified air in TYH medium containing 5 mM glucose and without (control) or with the mitochondria inhibitor carbonyl cyanide m-chlorophenylhydrazone (CCCP; 10 μM). Fluorescence (excitation 490 nm; emission 530, 590 nm) was monitored in a SpectraMax Gemini EM microplate reader (Molecular Device, Sunnyvale, CA) from the base of the plate. Ratio between red fluorescence (high membrane potential; excitation 490 nm, emission 590 nm) and green fluorescence (low membrane potential; excitation 490 nm, emission 530 nm) was calculated.

NAD:NADH Level Measurements

The NAD:NADH ratios in sperm were measured using the EnzyChrom NAD:NADH Assay kit (ECND-100; Bioassay Systems, Hayward, CA) following the manufacturer's instructions. Briefly, after incubation sperm were washed in PBS and the pellet was lysed in the buffer appropriate for either NAD or NADH by sonication and heating at 60°C for 5 min. Samples were neutralized with the opposite buffer and centrifuged at 14000 × g for 5 min. The subtraction of optical density (OD) at time 0 from OD at 30 min at 565 nm was used to determine sample NAD and NADH concentrations from standard curves. Protein levels in each sample were measured with the BCA protein assay kit (Pierce Biotechnology, Indianapolis, IN) and used to normalize the assay results.

Sperm Motility Assessment

Quantitative parameters of sperm motility were determined as previously described [13] using a computer-assisted sperm analysis instrument (software version 12; Hamilton Thorne Research, Beverly, MA). Sperm were counted as motile with any type of movement and as progressively motile when average path velocity > 50 μm/sec and straight line velocity > 50%. Hyperactive sperm were identified with the “sort fraction” function of the Hamilton Thorne analyzer by using these criteria: curvilinear velocity > 240 μm/sec, lateral head displacement > 18 μm, and beat-cross frequency < 40 Hz. Median values of each of the kinematic parameters were obtained for each sample.

ATP Level Measurements

Sperm ATP levels were measured as previously described [2] with slight modifications. After incubation for the indicated length of time at 37°C in 5% CO₂ in humidified air, sperm were centrifuged at 1000 × g for 5 min. The pellet was resuspended in buffer (100 mM Tris-HCl, 4 mM EDTA, pH 7.8) and boiled for 5 min. Samples were centrifuged at 10000 × g for 5 min and aliquots of the supernatant were analyzed in duplicate. ATP was measured using a luciferase bioluminescence assay according to the manufacturer's protocol (ATP Bioluminescence Assay kit CLS II; Roche Applied Science, Indianapolis, IN).

Pyruvate and Lactate Level Measurements

Pyruvate and lactate levels were determined using a commercial kit based on an enzymatic reaction by lactate oxidase and interaction of the product with a probe to produce fluorescence (at excitation/emission = 535/587 nm). After a 4-h incubation in TYH medium (lactate- and pyruvate-free), sperm were centrifuged and the pellet was resuspended in the appropriate assay buffer (BioVision, Mountain View, CA). The concentration of each sample was calculated using a standard curve.

NMR Spectroscopy

Proton decoupled ¹³C-[¹H] NMR spectra were obtained at 25°C on a Varian INOVA 500 NMR spectrometer using a 5-mm broadband probe tuned to 125.869 MHz. A 45° pulse angle with a 2.3 recycle time was employed in order to minimize intensity perturbations due to overpulsing. Data were collected using a 30000-Hz sweep width and 78000 data points. Ten percent D₂O was added to the samples for locking. Each sample contained 15 million viable spermatozoa in HEPES-TYH without substrates. Samples were shimmed (magnetic field homogeneity optimized) prior to addition of labeled substrate. They were then spiked with either 6 mM of [1-¹³C]-glucose or [3-¹³C]-pyruvate (Isotec/Sigma-Aldrich) and NMR acquisition quickly initiated. In the studies utilizing [1-¹³C]-glucose, data were collected in 1-h blocks of time and followed over a total period of 20 h. In the studies utilizing [3-¹³C]-pyruvate, data was collected in 10-min blocks of time for 1 h.

Glycolytic Enzyme Activity

Whole sperm were suspended in a nondenaturing buffer (0.1 M Tris-HCl pH 7, 0.1% Triton-X100) and placed on ice for 30 min. The protein concentration was measured using the BCA protein assay kit. Enzymatic activity was assayed in solution by monitoring the NADH or NADPH concentrations at 340 nm with a spectrophotometer over a period of 1–30 min as recommended [17] with minor modifications.

Glucose Uptake

Glucose uptake was determined using radiolabeled [1,2-³H]-2-deoxy-d-glucose [18]. Sperm were incubated 30 min at RT with 0.5 μCi [1,2-³H]-2-deoxy-d-glucose (52 Ci/mmol) in 1 ml modified HEPES-TYH medium without glucose. Uptake of [1,2-³H]-2-deoxy-d-glucose was stopped by addition of 0.2 ml of an ice-cold 0.6 M glucose solution. After 4 washes in cold PBS, sperm were solubilized in 0.2 ml of 4% SDS solution and transferred to scintillation vials containing 1 ml of scintillate. Radioactivity was determined in a scintillation counter. An aliquot (100 μl) of the last PBS wash also was counted to determine the residual amount of [1,2-³H]-2-deoxy-d-glucose present in the extracellular medium and was subtracted as background. Cytochalasin B (20 μM) was used to inhibit glucose uptake, and competition with 5 mM nonlabeled glucose was used as a negative control. This provided an estimate of radioactivity in the extracellular space within the sperm pellet.

Coimmunoprecipitation and Western Blot

Proteins were extracted from freshly isolated sperm using lysis buffer (50 mM Tris pH 8, 150 mM NaCl, 1% Triton X-100) supplemented with EDTA-free 1× protease inhibitor cocktail (Roche Applied Science), and the samples were sonicated on ice 3 times for 5 sec. After centrifugation at 4°C for 5 min at 10000 × g, the protein concentration in the supernatant was determined using the BCA protein assay kit. Lysate (containing 200 μg protein) from WT mouse sperm was precleared with 100 μl protein G magnetic microbeads (Miltenyi Biotec, Auburn, CA) following manufacturer's instructions, and then incubated with antiserum to LDHC (1/10000; [19]; IP_LDHC) plus 1% BSA or in normal rabbit IgG as a negative control (ab-37415; Abcam, Cambridge, MA; C−) for 2 h at 4°C. Protein G magnetic microbeads (100 μl) were added for 30 min at 4°C. Immunopurification was performed using microcolumns and a microMACS separator. Samples obtained from coimmunoprecipitation were subjected to mass spectrometry (see Supplemental Experimental Procedure; all supplemental data are available online at www.biolreprod.org) after separation on a 4%–20% polyacrylamide gel (Biorad, Hercules, CA) and Coomassie blue staining. Western blots using the Clean-blot IP detection kit from Pierce Biotechnology were performed to validate the mass spectrometry results.

Loss of LDHC Alters Glycolysis: NMR Experiments

An NMR assay was used to follow in real time the utilization of ¹³C-labeled glucose by freshly isolated epididymal sperm in HEPES-TYH medium in a system without oxygen supplementation. WT and KO sperm were incubated for 20 h with 6 mM [1-¹³C]-glucose (Fig. 2) and the fraction converted to lactate was calculated by integration of the peak area. This method was not sufficiently sensitive to detect peaks corresponding to other metabolites. After 20 h incubation, 94.9% ± 7.2% of glucose was metabolized to lactate by WT sperm (Fig. 2A; Supplemental Fig. S1A). As expected, KO sperm produced a low level of lactate, but most of the glucose remained unutilized (Fig. 2B). After 20 h incubation, only a small percentage of the glucose was metabolized to lactate by KO sperm (Supplemental Fig. S1B). Based on these data, glucose utilization (G_ut) was calculated in nanomole per hour and per million spermatozoa (nmol per h per million sperm; Fig. 2C). We found that with WT sperm G_ut = 12.9 ± 3.4 nmol per h per million sperm, and with KO sperm G_ut = 0.4 ± 0.3 nmol per h per million sperm. The lactate production (L_prod nmol per h per million sperm) was calculated as two times the percentage of lactate derived from the intensity of the NMR resonance, because only one of the two lactate molecules derived from [1-¹³C]glucose will be labeled as [3-¹³C]lactate. The L_prod equaled 25.9 ± 6.9 for WT and 0.8 ± 0.7 nmol per h per million sperm for KO sperm. These results are consistent with the L_prod found previously [13] using an enzymatic assay (L_prod = 35.7 ± 7.3 for WT and 2.9 ± 2.5 nmol per h per million sperm for KO sperm). No differences in sperm viability were observed between WT and KO sperm after 22 h (Fig. 2D), indicating that the low level of G_ut in KO sperm was not due to cell death.

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FIG. 2.

[1-¹³C]-glucose consumption by WT (A) and KO (B) sperm followed in real time by NMR spectroscopy. Six millimolar [1-¹³C]-glucose was initially added to the sperm preparation and corresponded to 100%. C) G_ut and L_prod expressed in nanomole per hour and per million spermatozoa WT and KO sperm. Values for G_ut and L_prod (1) were calculated from the NMR assay. Values for L_prod (2) were calculated from an enzymatic assay determining the quantity of lactate secreted by 4 × 10⁶ spermatozoa in 1 ml TYH, 5.5 mM glucose at different times. D) Percentage of WT and KO sperm live after 22 h incubation in TYH medium containing 6 mM glucose, determined by a dye exclusion assay [16]. Values are the mean ± SEM, n = 3, *P < 0.01 compared to WT.

Absence of LDHC Does Not Affect NAD, NADH, or Pyruvate Levels

The inhibition of LDHC was hypothesized [13] to lead to an accumulation of its substrate (pyruvate) and cofactor (NADH) and an absence of its products (lactate and NAD⁺). Therefore, the levels of NAD⁺ and NADH were measured in WT and KO sperm directly after isolation, and after incubation for 1.5 h and 4 h in TYH containing 5.5 mM glucose (Fig. 3). No significant differences were detected in the levels of NAD⁺ (Fig. 3A), NADH (Fig. 3B), or NAD_t (total = NAD⁺ + NADH; Fig. 3C), or in the NAD⁺:NADH ratio (Fig. 3D). A decrease in the NAD⁺:NADH ratio in KO sperm compared to WT sperm was observed after 4 h incubation, but the difference was not statistically significant (P = 0.13). Because variability between animals and assays may have obscured small changes important for regulation of glycolysis, we used an alternative functional approach. Sperm from WT and KO mice were treated with methylene blue, a redox dye capable of oxidizing NADH [20, 21]. However, this treatment did not rescue the phenotype of KO sperm (Supplemental Fig. S2).

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FIG. 3.

NAD⁺ (A) and NADH (B) levels (μM/μg proteins), were measured in WT and KO sperm after 0, 1.5, and 4 h incubation at 37°C in 5% CO₂ in humidified air in TYH, 5.5 mM glucose. Total NADt (NADt = NAD⁺ + NADH; C) and NAD:NADH ratio (D) were calculated from these values. Pyruvate (E) and lactate (F) levels were measured in sperm extract after 4 h incubation in TYH, 5.5 mM glucose. Values are the mean ± SEM, n = 5 minimum for the NAD⁺ and NADH assays, n = 4 for pyruvate and lactate assays; *P < 0.01 compared to WT.

Pyruvate and lactate levels were measured by an enzymatic method in sperm extracts from WT, HET, and KO mice, after 4 h incubation in TYH containing 5.5 mM glucose. No differences in pyruvate concentrations (Fig. 3E) were observed, but the lactate level (Fig. 3F) was significantly lower in KO sperm compared to WT and HET sperm.

KO Sperm Metabolize Pyruvate Like WT Sperm

We also followed the utilization of pyruvate by NMR. With WT sperm, we observed that 6 mM [3-¹³C]-pyruvate was quickly metabolized. After 1 h, all pyruvate was consumed, and around 80% of the pyruvate was converted to lactate (Fig. 4A). Two minor peaks were detected at 25.8 ppm and 23.5 ppm and remain to be identified. Surprisingly, the same profile was found with sperm lacking LDHC (Fig. 4A). We calculated that for WT and KO sperm respectively, 4.9 ± 1.2 and 5.0 ± 1.5 nmol of pyruvate were consumed per min per 10⁶ sperm, and 4.1 ± 1.0 and 4.5 ± 1.4 nmol of lactate per min per million sperm were produced from pyruvate.

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FIG. 4.

A) [3-¹³C]-pyruvate consumption by WT and KO sperm followed in real time by NMR. Initially, 6 mM [3-¹³C]-pyruvate was added to the sperm preparation and corresponded to 100%. B) L_prod by WT and KO sperm incubated at 37°C in 5% CO₂ in humidified air in medium containing 5 mM pyruvate as sole substrate. Lactate levels were measured with an enzymatic assay. Values are the mean ± SEM, n = 3.

Similar results were observed with another approach. WT and KO sperm were incubated in TYH containing 5 mM pyruvate as the sole substrate, and lactate levels were measured in medium at different times (Fig. 4B). WT and KO sperm were able to produce a high quantity of lactate. The L_prod calculated at 10 min was 3.41 ± 0.56 and 3.21 ± 0.31 nmol of lactate per min per million sperm for WT and KO sperm, respectively.

Differences Between Loss of LDHC and Inhibition of LDH Activity

The pyruvate analog sodium oxamate was used as a competitive inhibitor of LDH activity. In sperm extracts, all LDH activity was inhibited by 20 mM sodium oxamate for WT sperm and 5 mM for KO sperm (Supplemental Fig. S3A). Live sperm were incubated for 2 h at 37°C in TYH containing 5 mM glucose plus different concentrations of sodium oxamate (0–100 mM). We determined that 100 mM was the maximum sodium oxamate concentration that could be used without changing the osmolarity of the medium, and that even at this high concentration sperm were as viable, as determined by dye exclusion, as in control medium (data not shown). The endpoint used was inhibition of sperm hyperactivation and the maximum effect observed was at 100 mM (Supplemental Fig. S3B). However, ATP levels and sperm motility were not affected. Treatment with 100 mM sodium oxamate inhibited lactate production: 1) by 85% in WT and 52% in KO sperm when glucose was the substrate (Fig. 5A), and 2) by 53% in WT and 55% in KO sperm when pyruvate was the sole substrate (Fig. 5B). Therefore, this concentration (100 nM sodium oxamate) was chosen to treat WT and KO sperm for 2 h at 37°C in TYH medium containing 5 mM glucose.

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FIG. 5.

Effect of 100 mM sodium oxamate treatment on L_prod when WT and KO sperm were incubated at 37°C in 5% CO₂ in humidified air in TYH containing 5 mM glucose (A) for 2 h or 1 mM pyruvate (B) for 30 min. Values are the mean ± SEM, n = 3. Letters (a, b) above the means denote no significant difference if identical or significant difference if not identical.

We compared the levels of NAD⁺, NADH, and ATP, and of sperm motility in treated and untreated WT and KO sperm (Table 1). We observed 1) no differences between untreated and treated KO sperm in motility or in ATP, NAD, and NADH levels; 2) a lower level of ATP and no difference in NAD⁺ and NADH levels in KO sperm compared to the control WT sperm; 3) that treated WT sperm failed to hyperactivate, as seen for KO sperm; 4) that treated WT sperm differed from KO sperm in that ATP levels in treated WT sperm were comparable to those of control WT sperm; 5) that NADH levels in treated WT sperm were higher, resulting in a lower NAD:NADH ratio.

TABLE 1.

Sodium oxamate treatment in WT and KO sperm: consequences on NAD, NADH, ATP levels, and sperm motility.*

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KO Sperm Are Able to Take Up and Consume Glucose

Because LDHC is relatively hydrophobic and thus could associate with the plasma membrane, loss of LDHC might interfere with glucose uptake. Therefore, we measured the uptake of radiolabeled [1,2-³H]-deoxy-glucose. Following 30 min incubation, sperm were carefully washed to remove residual [1,2-³H]-deoxy-glucose. No differences in radioactive content were observed between WT, HET, and KO sperm (Fig. 6A). The levels of radioactivity were barely detectable in sperm following incubation in [1,2-³H]-deoxy-glucose (0.5 μCi/ml = 9.6 μM) containing excess cold glucose (5 mM), and more than 10 times lower with cytochalasin B treatment (inhibitor of facilitative glucose transporters). These results indicate that glucose uptake was not disrupted in sperm from KO mice.

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FIG. 6.

A) Levels of radiolabeled [1,2-³H]-2-deoxy-d-glucose detected in sperm extract from WT, HET, and KO mice after a 30-min incubation at RT without (control) or with cytochalasin B treatment (CB) or competition with nonlabeled glucose (glucose). Values are the mean ± SEM, n = 6 minimum for control and cytochalasin B-treated assays, n = 3 for cold glucose competition assay. B) ATP level and progressive motility in WT and KO sperm incubated 1.5 h at 37°C in 5% CO₂ in humidified air in TYH with no substrates (NS) or with 1 mM glucose (G). Letters (a, b) above the means denote no significant difference if identical or significant difference (P < 0.05) if not identical; n = 4.

Proteins from Triton X-100 permeabilized WT, HET, and KO sperm were aliquoted and used in parallel assays to measure hexokinase, glyceraldehyde-3-phosphate dehydrogenase, phosphoglycerate kinase, pyruvate kinase, and LDH enzymatic activities. The total LDH activity in extracts of sperm from KO mice was confirmed to be significantly lower than that in extracts of sperm from WT and HET mice. In contrast, no differences in the activities of the other enzymes were observed (Table 2), indicating that the lack of LDHC does not compromise the functional abilities of these other glycolytic enzymes under these conditions.

TABLE 2.

Enzymatic activity of different glycolytic enzymes in WT, HET, and KO sperm.^a

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In addition, we observed that in medium containing no substrates (NS in Fig. 6B), ATP levels were 3 times lower in WT and 2 times lower in KO sperm than in medium containing glucose (G in Fig. 6B). In assays done in parallel, progressive motility was around six times lower for both WT and KO sperm in the absence of glucose than when glucose was present (Fig. 6B).

We thank Drs. Christopher Geyer, Polina Danshina, and Huanghui Tang for critically reading this manuscript and for their constructive suggestions.