Mice

Akt1 heterozygous breeding pairs in a C57BL/6 background were obtained from the laboratory of Dr. Morris Birnbaum (University of Pennsylvania, Philadelphia, PA). Heterozygous pairs were mated to obtain Akt1^+/+, Akt1 ^+/−, and Akt1^−/− females for experimental procedures. The frequency of obtaining Akt1^−/− mice is approximately 17.3 percent, which is less than the expected Mendelian frequency of 25%. Experiments were conducted at PNDs 25, 50, 56, and 90. The animal room climate was kept at a constant temperature (23.3 ± 2°C) at 30%–70% humidity, with an alternating 12L:12D cycle. All procedures involving animals were performed in accordance with the guidelines of the Institutional Animal Care and Use Committee of Brown University in compliance with the guidelines established by the National Institutes of Health.

Primers

For genotyping by PCR, the following primers were used in a single reaction: 853, 5′-GTGGATGTGGAATGTGTGCGAG-3′; 854, 5′-GCTCAGTCAGTGAGGCCAGACC-3′; 855, 5′-CACCCCACAAGCTCTTCTTCCA-3′. The PCR was run with an initial denaturing step of 94°C for 5 min, 39 cycles of 94°C for 30 sec, 63°C for 30 sec, 72°C for 45 sec, followed by a final extension at 72°C for 5 min. For PCR genotyping of progeny, the wild-type and targeted bands were 310 and 194 bp, respectively.

Fertility Analysis

To evaluate the reproductive performance of Akt1^−/− mice, seven individually housed Akt1^−/− females were bred to Akt1^+/+ males of proven fertility. Akt1^+/+ females were used as controls. The females were introduced to the males at 7 to 8 wk of age, and the number of litters and the number of pups were recorded over a minimum 6-mo period.

Assessment of Pubertal Onset and Estrous Cyclicity

To assess the onset of puberty in juvenile females, mice were observed daily for signs of vaginal opening. The onset of estrus was also monitored by daily vaginal lavage of females in the morning, for a period of at least 1 mo after vaginal opening based on vaginal cytology, according to the classification of Pedersen [25].

Classification of the Estrous Cycle and Tissue Collection

To examine the influence of genotype on the length of the estrous cycle, vaginal smears from wild-type and Akt1-deficient female mice at 12 wk of age were monitored daily between 0800 and 1000 h. The mouse's tail was raised and a 20-μl pipette tip filled with sterile PBS1X was inserted into the vagina and washed up and down. When the tip was removed, it was dropped onto a microscope slide. The smears were classified into one of four phases of estrus: elongated nucleated epithelium indicated proestrus; large cornified epithelial cells were exclusively found in estrus; metestrus was marked by a thick smear composed of equal numbers of nucleated epithelial cells and leukocytes; and a smear consisting almost exclusively of leukocytes depicted diestrus [26]. Each cycle length was determined as the length of time between two consecutive occurrences of estrus. After the mice had progressed through at least three consecutive estrous cycles, the length of the estrous cycle and the number of days spent at each stage of the cycle were evaluated.

Ovarian Histology

To determine whether lack of Akt1 influences ovarian development, ovaries from a minimum of three mice per genotype were collected and examined at PNDs 25 and 90. Both ovaries were removed, cleaned of extraneous tissue, weighed, and fixed in Bouins. Tissues were then embedded in paraffin and serial sections (7-μm thick) of ovaries were stained with periodic acid-Schiff (PAS).

Assessment of Follicle Development

In approximately every 10th ovarian section, the numbers of primordial, primary, early antral, and healthy antral follicles were counted. Only follicles containing an oocyte with a visible nucleus were counted to avoid double counting, and all counting was done without the knowledge of genotype. Follicles were counted as primordial if they contained an oocyte surrounded by flattened granulosa cells, or a mixture of less than seven flattened and cuboidal granulosa cells. Follicles were counted as primary if they contained an oocyte surrounded by a single layer of seven or more cuboidal granulosa cells. Secondary follicles were those containing an oocyte surrounded by two or more complete layers of granulosa cells. Early antral follicles were those with more than four complete layers of granulosa cells and an antrum <20 μm in diameter. Antral follicles were considered as those that had a visible antrum without a stalk. Graafian follicles were those with a large antrum, cumulous oophorus, and a corona radiata. Antral follicles were considered to be healthy if they had an intact oocyte and <10% pyknotic granulosa cells. Antral follicles were considered to be atretic if there were more than 10% pyknotic granulosa cells.

Superovulation

Female mice at 24–26 days of age were injected i.p. with 5.0 IU of ECG followed by 5.0 IU of hCG i.p. 48 h later. Oviducts and ovaries were excised from mice 18 h after hCG administration, and were fixed in 10% neutral buffered formalin. Tissues were then embedded in paraffin and serial sections (7-μm thick) of ovaries were stained with PAS. For analysis of the number of ovarian follicles, every sixth section was mounted and stained with hematoxylin and eosin.

Primary Oocyte Diameter

Ovaries from mice at PND25 were examined (n = 3–4 ovaries per genotype). A total of 87 and 118 primary follicles were measured from Akt1^+/+ and Akt1^−/− mice, respectively. Follicles were counted as primary if they contained an oocyte surrounded by a single layer of seven or more cuboidal granulosa cells. To prevent counting the same oocyte twice, oocytes were only measured when there was a visible nucleolus. Measurements were then averaged and expressed as the diameter of the oocyte.

Secondary Oocyte Diameter

Ovaries from mice at PND25 were examined (n = 3–4 ovaries per genotype). A total of 55 and 66 secondary follicles were measured from Akt1^+/+ and Akt1^−/− mice, respectively. Follicles were counted as secondary if they contained an oocyte surrounded by two or more complete layers of granulosa cells and no visible antrum formation. To prevent counting the same oocyte twice, oocytes were only measured when there was a visible nucleolus. Measurements were then averaged and expressed as the diameter of the oocyte.

Measurements of Hormone Levels

To measure serum FSH, LH, inhibin A and B, progesterone, and estradiol levels, blood samples were collected by cardiac puncture from randomly cycling Akt1^+/+ and Akt1^−/− female mice at specific ages. The serum was stored at −80°C until assayed. FSH, LH, inhibin A and B, progesterone, and estradiol levels were assayed by the University of Virginia Ligand Core Facility as described ( http://www.healthsystem.virginia.edu/internet/crr/ligand.cfm; Specialized Cooperative Center Program in Reproductive Research, National Institute of Child Health and Human Development/National Institutes of Health U54 HD28934).

Bromodeoxyuridine Incorporation

Assessment of granulosa cell proliferation by bromodeoxyuridine (BrdU) incorporation was performed. Hormonally primed mice (5 IU eCG) were injected intraperitoneally with 1 μg/g BrdU and killed after 1 h. The ovaries were dissected, fixed in formalin, and 7-μm serial sections were generated. Primary monoclonal anti-BrdU antibody (Dako) was used at a 1:100 dilution. After counterstaining with methyl green, the number of BrdU-positive cells per follicle was determined for comparison in a minimum of five follicles per experimental animal. Secondary follicles were analyzed in the eCG-treated groups.

Immunohistochemistry

Immunohistochemistry was performed on formalin-fixed, paraffin-embedded 7-μm sections using the VectaStain Elite Avidin-Biotin Complex Kit, as directed by the manufacturer (Vector Labs, Burlingame, CA). Sections were probed with primary antibodies against CCND1 and CCND3 both from Cell Signaling (Beverly, MA) and CCND2 from Santa Cruz Research (Santa Cruz, CA). Sections were visualized using a 3,3′-diaminobenzidine peroxidase Substrate Kit (Vector Labs). Digital images were captured using the Aperio Scanscope Imaging System (Vista, CA).

Western Blot Analysis

Ovaries were lysed by homogenization in cold lysis buffer (50 mM Tris 8.0, 250 mM NaCl, 1% NP-40, 0.1% SDS, 5 mM EDTA, 2 mM Na₃VO₄, 10 mM Na₂P₂O₇, 10 mM NaF) supplemented with 1 mM PMSF and 40 μl/ml Complete Protease Inhibitor Cocktail (Roche, Indianapolis, IN). Lysates were incubated on ice for 20 min with frequent vortexing and cleared by centrifugation (10 000 rpm, 10 min, 4°C). Protein concentrations were determined using the DC Protein Assay (Bio-Rad, Hercules, CA). Total protein (50 μg) was subjected to SDS-PAGE and transferred onto Immobilon-P polyvinylidene fluoride (Millipore, Billerica, MA). Membranes were blocked for 60 min at room temperature in 5% nonfat milk/Tris-buffered saline/0.1% Tween (TBST). Membranes were incubated for 2 h at room temperature, then overnight at 4°C in the following antibodies: phospho-AKT (Thr308) (#9275, 1:500 in 5% milk/TBST), phospho-AKT (Ser473) (#9271, 1:1000 in 5% milk/TBST), AKT1 (#2967, 1:1000 in 5% milk/TBST), AKT2 (#2964, 1:1000 in 5% milk/TBST), AKT3 (#4059, 1:1000 in 5% milk/TBST). All antibodies were obtained from Cell Signaling Technology (Danvers, MA). Membranes were washed three times (5 min/wash) in TBST, and incubated for 60 min at room temperature in horseradish peroxidase-conjugated goat anti-rabbit IgG or goat anti-mouse IgG (Cell Signaling), diluted 1:2000 in 5% milk/TBST. Membranes were washed three times (5 min/wash) in TBST, and once in TBS prior to visualization using enhanced chemiluminescence (GE Healthcare, Piscataway, NJ).

Quantitative RT-PCR

Total RNA (1 μg) was DNase-I (Invitrogen, Carlsbad, CA) treated and reverse transcribed using iScript cDNA Synthesis Kit (Bio-Rad) according to the manufacturer's protocols, and the cDNA templates were amplified with each of the primer pairs in independent sets of PCR using iQ SYBR Green Supermix (Bio-Rad) on an iCycler iQ Multicolor Real-Time PCR Detection System (Bio-Rad). The concentration of Mg²⁺ and the linear range of amplification of cDNAs with each primer pair first were optimized, and cDNAs subsequently were tested. Each sample was run in triplicate, and mRNA levels were analyzed relative to hypoxanthine phosphoribosyltransferase.

Mouse-specific primers were designed using Molecular Beacon Design 4.0 Software (Bio-Rad). Specific primer sequences for each gene for quantitative RT-PCR were as follows: Kitl = forward, 5′-ACAGCAGTAGCAGTAATAGG-3′ and Kitl = reverse, 5′-GACTTGACTGTTTCTTCTTCC-3′; Bcl2l1 = forward, 5′-CCGCTGTGTCTCTGGGTCTC-3′ and Bcl2l1 = reverse, 5′-GGTTCTGGTCCTTGTCTCATTATCC-3′; Ccnd1 = forward, 5′-ATGTTGTTACCAGAAGAGGAAG-3′ and Ccnd1 = reverse, 5′-TCAGATAGAAAGGAGAAAGATTAAGG-3′; Ccnd2 = forward, 5′-TGGCAGACAGTTAGGAGAC-3′ and Ccnd2 = reverse, 5′-AGCACCAACCAGACTCAG-3′; and Ccnd3 = forward, 5′-GGAGGTGTGTGAGGAGCAG-3′ and Ccnd3 = reverse, 5′-CCAGGTAGTTCATAGCCAGAGG-3′.

Statistical Analysis

The Student t-test or one-way ANOVA with Bonferonni post hoc analysis was performed using SigmaStat software (SPSS Inc., Chicago, IL). A P value < 0.05 was considered to be statistically significant.

Effect of Akt1 Null Mutation on Female Fertility

When Akt1^−/− female mice were mated to Akt1^+/+ males of proven fertility, we observed the Akt1^−/− females to be significantly less fertile relative to their Akt1^+/+ female counterparts (P < 0.05) (Table 1). This subfertility included both a reduction in the overall number of litters and the number of pups per litter in the Akt1^−/− females (Table 1). The average number of litters per month for Akt1^+/+ females bred with Akt1^+/+ males was 0.64 ± 0.1 (n = 5), and for Akt1^−/− females bred to Akt1^+/+ males, the average number of litters per month was 0.11 ± 0.1 (n = 8). The number of pups per litter was significantly reduced in Akt1^−/− female mice compared to Akt1^+/+ female mice, with 3.6 ± 0.8 pups per litter (n = 8) and 5.8 ± 0.5 pups per litter (n = 5), respectively (Table 1). The average maternal age for production of the first litter for Akt1^+/+ and Akt1^−/− females was 56 ± 5 days and 100 ± 7 days, respectively (P < 0.001).

TABLE 1.

Effect of Akt1 null mutation on female fertility.^a

Comparison of Akt1^+/+, Akt1^+/−, and Akt1^−/− Female Body and Ovarian Weights

To characterize the female reproductive physiology of the Akt1^−/− female mice, body weights and ovarian weights were compared with those of Akt1^+/+ females at PNDs 25, 56, and 90 (Table 2). At all time points examined, significant decreases in the body weights of the Akt1^−/− mice were observed compared with that of Akt1^+/+ female mice. At PND56, Akt1^−/− female mice exhibited an approximate 20% decrease in body weight, and, at PND90, there was a 12% decrease in body weight relative to Akt1^+/+ counterparts. Similar to body weight, there was a significant decrease in ovarian weights in the Akt1^−/− mice at both PND56 and PND90 (Table 2). Ovarian weights at PND25 were reduced by 27.4% relative to Akt1^+/+ mice, and, at PND90, ovarian weights were reduced by 20.6% in Akt1^−/− mice relative to the Akt1^+/+ littermates. However, when adjusted for ovarian weight relative to body size (i.e., absolute ovarian weight), no differences were observed in Akt1^+/+ and Akt1^−/− females (Table 2).

TABLE 2.

Comparison of Akt1^+/+ and Akt1^−/− female body and ovarian weights at PND25, PND56, and PND90.^a

Effect of Akt1 Null Mutation on Sexual Maturity

Due to the significant decrease in body size of the Akt1^−/− mice, we determined if there was a delay in sexual maturity in the Akt1^−/− females by assessing the effect of Akt1 deletion on the age at pubertal onset and estrous cyclicity. As shown in Table 1, vaginal opening was not significantly delayed in Akt1^−/− females (PND33.2 ± 1.4; n = 10) when compared with Akt1^+/+ females (PND33.0 ± 1.5; n = 4). However, sexual maturity, as determined by first proestrus, was significantly delayed in Akt1^−/− females (PND44.8 ± 0.6) compared with Akt1^+/+ females (PND39.8 ± 1.1; n = 3), and the maternal age at first litter was significantly higher in Akt1^−/− females relative to Akt1^+/+ counterparts (100 ± 7.2 vs. 56 ± 5 days, respectively).

Extension of the Diestrous Cycle in Mature Akt1^−/− Female Mice

Due to the later age at first proestrus and the later maternal age for first litter in the Akt1^−/− mice, we examined the length of the estrous cycle of both Akt1^+/+ female mice and Akt1^−/− female mice at PND90. This age was examined because live litters are observed at this time in Akt1^−/− females. At PND90, Akt1^−/− females displayed abnormal cycling patterns, although the average cycle length was similar in Akt^+/+, Akt1^+/−, and Akt1^−/− mice (4.5 ± 0.2 days). Analysis of the estrous cycle profiles in Akt1^−/− female mice and Akt1^+/+ control mice did reveal a significantly longer diestrus phase in Akt1^−/− females of approximately 1.5 days longer in duration relative to Akt1^+/+ female mice (P < 0.05) (Fig. 1).

FIG. 1.

Akt1 influences estrus cycle phase in female mice at PND90. A) Graph depicts the mean estrous cycle length of Akt1^+/+ (black bar), Akt1^+/− (light gray bar), and Akt1^−/− (dark gray bar) female mice. B) Graph shows the average number of days that each genotype stayed within individual stages of the estrous cycle (P < 0.05). Asterisk indicates significant differences observed between Akt1^+/+ and Akt1^−/− animals.

Effect of Akt1 Null Mutation on Follicle Development in Mice at PND25

To determine the effect of Akt1 deletion on folliculogenesis, we performed histological and morphometric analyses of follicle numbers at PND25, and compared them between Akt1^+/+ and Akt1^−/− mice. As expected, Akt1^+/+ females revealed follicles at all developmental stages (primordial, primary, secondary, and antral follicles) and corpora lutea (Fig. 2A). In contrast, the ovaries of Akt1^−/− mice contained fewer antral follicles compared with Akt1^+/+ controls. In Akt1^−/− ovaries, we observed follicles with multiple oocytes, as depicted in Figure 2B (dashed circle). Only once did we observe Akt1^+/+ females with more than one oocyte per follicle. The increase in multiple oocytes per follicle may indicate a defect in cyst breakdown in the Akt1^−/− ovary. Figure 2C shows follicle numbers at PND25 for both Akt1^+/+ and Akt1^−/− animals. The number of primordial and primary follicles was not significantly different in Akt1^−/− ovaries when compared to Akt1^+/+ ovaries; however, the number of preantral follicles in Akt1^−/− mice was significantly lower than in Akt1^+/+ ovaries, as was the number of antral and mature Graafian follicles (Fig. 2C), with a 2-fold increase in the number of atretic follicles with degenerate oocytes (Fig. 2C).

FIG. 2.

Effect of Akt1 null mutation on ovarian follicle development at PND25. A) Akt1^+/+ ovary at PND25. B) Akt1^−/− ovary at PND25. C) Follicle counts of Akt1^+/+ and Akt1^−/− females at PND25 (n = 3). The number of primordial (PF), primary(1⁰), secondary (2⁰), early antral (EAF), antral (AF), and mature Graafian follicles (GF) were determined in Akt1^+/+ and Akt1^−/− at PND25. Ovaries were serially sectioned, every 10th section was counted, and the total follicle numbers were determined. The total numbers of primordial, primary, secondary, early antral, antral, and mature follicles were multiplied by a factor of 10 to obtain an estimate of the total number of follicles per ovary. These data represent the mean ± SEM of combined results from the analysis of three mice per age group (P < 0.05). Asterisks indicate significant differences in follicle number observed between Akt1^+/+ and Akt1^−/− animals; bar = 200 μm.

Effect of Akt1 Null Mutation on Oocyte Size

Unexpectedly, we found the diameters of both primary and secondary oocytes to be larger in Akt1^−/− mice. Primary oocytes were found to have an average diameter of 27.9 ± 1.0 μm versus 22.4 ± 1.0 μm in Akt1^+/+ female primary oocytes. Secondary oocyte diameters were found to be 50.0 ± 1.0 μm in Akt1^+/+ and 53.0 ± 1.0 μm in Akt1^−/− ovaries.

Responsiveness of PND25 Akt1 Null Mutant Mice to Exogenous Gonadotropins

Due to the decrease in the number of mature follicles in Akt1^−/− mice, we examined whether Akt1 is involved in the maturation process of follicles by comparing the number of total mature follicles in immature mice after eCG/hCG treatment. As shown in Figure 3C, the number of secondary follicles in the ovaries of Akt1^−/− mice after eCG/hCG treatment was 2-fold higher than that of Akt1^+/+ mice; however, fewer mature follicles were observed, suggesting that follicular maturation is indeed impaired in Akt1^−/− mice.

FIG. 3.

Responsiveness of Akt1 null mutant mice to exogenous gonadotropins at PND25. Histology of ovaries from Akt1^+/+ (A) and Akt1^−/− (B) animals exposed to exogenous gonadotropins. Female mice at 24–26 days of age were injected i.p. with 5.0 IU of ECG followed by 5.0 IU of hCG i.p. 48 h later. Oviducts and ovaries were excised from mice 18 h after hCG. C) The number of primordial (PF), primary (1⁰), secondary (2⁰), early antral (EAF), antral (AF), and mature Graafian follicles (GF) were determined in Akt1^+/+ and Akt1^−/− at PND25 following exposure to exogenous gonadotropins. Ovaries were serially sectioned, every sixth section was counted, and the total follicle numbers were determined. The total numbers of primordial, primary, secondary, early antral, antral, and mature follicles were multiplied by a factor of six to obtain an estimate of the total number of follicles per ovary. These data represent the mean ± SEM of combined results from the analysis of three mice per age group (P < 0.05). Asterisks indicate significant differences in follicle number observed between Akt1^+/+ and Akt1^−/− animals; bar = 200 μm.

Effect of Akt1 Null Mutation on Ovarian Steroid Synthesis in Female Mice at PND50

Both the inability to obtain a significant number of fertile Akt1^−/− females and the decrease in the number of preantral and antral follicles in the Akt1^−/− females led us to examine the levels of FSH, estradiol, progesterone, and LH in the serum of these mice at PND50. As depicted in Table 3 at PND50, Akt1^−/− mice showed a trend for lower levels of FSH. FSH levels in Akt1^+/+ mice were 8.0 ± 1.6 ng/ml (n = 6) and 7.32 + 1.3 ng/ml (n = 6) in Akt1^+/− mice versus 4.8 ± 1.1 ng/ml (n = 8) in Akt1^−/− females. Estradiol levels were found to be elevated in Akt1^−/− mice (12.2 + 3.0 pg/ml) relative to Akt1^+/+ mice (7.0 ± 3.2 pg/ml). Significantly higher levels of LH were found in Akt1^−/− females at PND50, with serum levels of 0.91 ± 0.3 ng/ml (n = 8) versus 0.25 ± 0.04 ng/ml (n = 11) in Akt1^+/+ female mice and 0.38 ± 0.15 ng/ml (n = 6) in Akt1^+/− female mice. Progesterone levels were found to be lower in Akt1^−/− females (1.1 + 0.1 ng/ml) (n = 18) relative to Akt1^+/+ females (3.0 ± 0.8 ng/ml) (n = 12). Interestingly, there was a trend toward higher inhibin A levels at PND50 in the Akt1^−/− mice than in the Akt1^+/+ mice (114 pg/ml ± 19.5 [n = 8] versus 99.8 ± 21.8 pg/ml [n = 4], respectively), and there was a trend toward reduced inhibin B serum levels in the Akt1^−/− mice relative to Akt1^+/+ mice (33.5 ± 11.0 pg/ml [n = 8] versus 57.4 ± 16.6 pg/ml [n = 8], respectively).

TABLE 3.

Serum hormone levels in Akt1^+/+, Akt1^+/−, and Akt1^−/− mice at PND50.^a

Analysis of Estradiol and Progesterone in Akt1^−/− Females at PND90

Because Akt1^−/− females are capable of delivering pups to term, we examined the levels of estradiol and progesterone at PND90. We found both estradiol and progesterone levels to be similar in both Akt1^−/− and Akt1^+/+ ovaries at this time point (Table 4). It should be noted that, on several occasions, we observed that Akt1^−/− females exhibit weight gain as if pregnant with no pups delivered, suggest-ing that AKT1 may serve other functions in female reproduction, including placentation, parturition, and/or lactation.

TABLE 4.

Serum hormone profiles of Akt1^+/+ and Akt1^−/− females at PND90.^a

Folliculogenesis in Akt1^−/− Females at PND90

To determine the effect of Akt1 deletion on folliculogenesis at PND90, we performed histological and morphometric analyses of follicle numbers and compared them between Akt1^+/+ mice (Fig. 4A) and Akt1^−/− mice (Fig. 4B). Both Akt1^+/+ and Akt1^−/− females revealed follicles at all developmental stages (primordial, primary, secondary, and antral follicles) and corpora lutea (Fig. 4, A and C). In contrast, the ovaries of Akt1^−/− mice contained significantly fewer primordial follicles compared with Akt1^+/+ controls (Fig. 4, B and C). The number of primary and secondary follicles was not significantly different in Akt1^−/− ovaries when compared to Akt1^+/+ ovaries. Mature Graafian follicles were observed in both genotypes; however, fewer Graafian follicles were observed in the Akt1^−/− ovaries.

FIG. 4.

Effect of Akt1 null mutation on the primordial follicle pool at PND90. A) Akt1^+/+ ovary at PND90. B) Akt1^−/− ovary at PND90. C) Follicle counts of Akt1^+/+ and Akt1^−/− females at PND90 (n = 3). The number of primordial (PF), primary (1⁰), secondary (2⁰), early antral (EAF), antral (AF), and mature Graafian follicles (GF) were determined in Akt1^+/+ and Akt1^−/− at PND90. Ovaries were serially sectioned, every 10th section was counted, and the total follicle numbers were determined. The total numbers of primordial, primary, secondary, early antral, antral, and mature follicles were multiplied by a factor of 10 to obtain an estimate of the total number of follicles per ovary. These data represent the mean ± SEM of combined results from the analysis of three mice per age group (P < 0.05). Asterisk indicates significant difference in primordial follicle number observed between Akt1^+/+ and Akt1^−/− animals; bar = 200 μm.

Effect of Akt1 Null Mutation on Granulosa Cell Proliferation In Vivo

To better understand the cellular basis of the observed folliculogenesis defects in the Akt1^−/− ovaries, we assessed the proliferation of granulosa cells in the presence versus absence of Akt1. BrdU incorporation in vivo was utilized to directly label granulosa cells in the S phase of the cell cycle and measure granulosa cell proliferation. At 24 h prior to BrdU labeling, matched 21-day-old Akt1^+/+ and Akt1^−/− female mice were stimulated with a single injection of eCG to stimulate proliferation of follicular granulosa cells. Ovaries were harvested the next day following 1 h in vivo BrdU treatment, and ovary sections generated from these mice were labeled with an anti-BrdU antibody. BrdU incorporation was readily detectable in granulosa cells derived from both Akt1^+/+ mice (Fig. 5A) and Akt1^−/− mice (Fig. 5B). However, there was a reduction in the number of positively stained granulosa cells labeled with BrdU in the Akt1^−/− ovaries in response to hormonal treatment (Fig. 5C).

FIG. 5.

Effect of Akt1 null mutation on granulosa cell proliferation in vivo at PND25. Immunohistochemical detection of BrdU incorporation into the nuclei of secondary follicular granulosa cells in 25-day-old Akt1^+/+ ovary (A) and Akt1^−/− ovary (B). Mice were stimulated with 5 IU ECG for 24 h. C) Negative control with primary antibody omitted. D) Quantification of percent positive nuclei in secondary follicles in the ovary. GC denotes granulosa cells in the follicles. Average values from two independent experiments are presented; error bars indicate SEM. Statistically significant differences between Akt1^−/− mice and matched controls are indicated with asterisks (P < 0.05); bar = 200 μm.

Neither Akt2 nor Akt3 Compensate for Akt1 Deficiency at the mRNA or Protein Level

Although the Akt gene family is implicated in a survival response to genotoxic injury in multiple cell types, it is not known to what degree there is functional overlap between these family members in the ovary. We first examined the activation of Akt in the ovary at PND50, and found decreased phosphorylation at the threonine 308 site in Akt1^−/− ovaries (Fig. 6A), but not at Ser473 (Fig. 6A). Next, we examined both the level of Akt2 and Akt3 mRNA and protein in Akt1^+/+ and Akt1^−/− ovaries at PND50. We found similar levels of expression for Akt2 mRNA (Fig. 6B) and protein (Fig. 6A) in both Akt1^+/+ and Akt1^−/− mice. There was a trend toward reduced Akt3 mRNA expression in the Akt1^−/− ovaries (Fig. 6C) relative to Akt1^+/+ ovaries, suggesting that Akt3 may contribute to the Akt1^−/− phenotype. However, we did not observe a decrease in Akt3 at the protein level (Fig. 6A).

FIG. 6.

Neither Akt2 nor Akt3 compensates for Akt1^−/− at the mRNA or protein level at PND50. A) Representative Western blots of Akt1^+/+, Akt1^+/−, and Akt1^−/− ovaries at PND50. Shown are phosphorylated Ser⁴⁷³ AKT and Thr³⁰⁸ AKT1, and AKT1, AKT2, and AKT3 total protein; β-actin was used as a loading control. Changes in the relative mRNA expression of Akt2 (B) and of Akt3 (C) in Akt1^−/− (gray bars) ovaries relative to Akt1^+/+ (black bars) control ovaries. Expression was determined by using the Pfaffl method.

Kitl and Bcl2l1 Are Significantly Reduced in Akt1^−/− Ovaries

Kitl plays a role in oocyte growth, survival, and maturation [27]. Therefore, we examined the level of Kitl mRNA in both Akt1^+/+ and Akt1^−/− ovaries. There was a 2-fold reduction in the levels of Kitl mRNA in Akt1^−/− ovaries relative to Akt1^+/+ ovaries (Fig. 7A). Because of the role of Kitl in granulosa cell survival and protection of the oocyte, we examined Bcl2l1 (Fig. 7B), an antiapoptotic factor and well-known downstream target of the AKT1 signaling pathway [28]. Again, we found significantly reduced levels of Bcl2l1 in the Akt1^−/− ovaries, suggesting that the PIK3/AKT1 signaling pathway plays a role in folliculogenesis.

FIG. 7.

Reduced levels of Kitl, Ccnd3, and Bcl2l1 in Akt1^−/− mouse ovaries at the mRNA level at PND50. Changes in the relative mRNA expression of Kitl (A), Bcl2l1 (B), Ccnd1 (C), Ccnd2 (D), and Ccnd3 (E) are depicted in graphic form in Akt1^+/+ (black bars) and Akt1^−/− (gray bars) ovaries. Expression was determined by using the Pfaffl method. The data are shown as means ± the SEM. Significance was determined by ANOVA; *P < 0.05.

Localization Patterns and Decreased mRNA Expression of Members of the Cyclin D Family in Akt1^+/+ and Akt1^−/− Ovaries

Due to the decreased proliferative rates of the granulosa cells, as measured by BrdU labeling in the secondary follicles of Akt1^−/− ovaries, we examined the expression levels of Ccnd1, Ccnd2, and Ccnd3 (Fig. 7, C–E). Members of the cyclin D family are implicated in the regulation of proliferation of granulosa cells [29, 30]. We found that Ccnd3 mRNA expression levels (Fig. 7E) were reduced 3-fold in the Akt1^−/− ovary relative to the Akt1^+/+ ovary, and that there was a 2-fold reduction in Ccnd1 mRNA expression levels (Fig. 7C) as well, although it did not reach statistical significance. Importantly, Ccnd2 mRNA expression levels (Fig. 7D) remained the same in both Akt1^+/+ and Akt1^−/− animals.

To localize Ccnd1, Ccnd2, and Ccnd3 to particular cells within the ovary, ovaries were examined at PND50 by immunohistochemistry. Ccnd1 staining was found to be relatively weak in the ovary, with minimal staining detected in thecal cells of both Akt1^+/+ (Fig. 8A, arrows) and Akt1^−/− ovaries (Fig. 8D, arrow). Staining of Ccnd1 did appear less intense in the Akt1^−/− ovary. We also observed weak cytoplasmic staining of Ccnd1 in the primordial follicles (Fig. 8D, bracket). As a positive control, oviduct stained positive for Ccnd1 within the same ovarian tissue sections examined (Fig. 8I). Ccnd2 expression was localized primarily to the cytoplasm of granulosa cells in both the Akt1^+/+ (Fig. 8B) and Akt1^−/− (Fig. 8E) ovaries. Ccnd3 localized to the nuclei of primordial (Fig. 8, C and F, asterisks) and primary follicles (Fig. 8, C and F, arrows) in both Akt1^+/+ (Fig. 8C) and Akt1^−/− ovaries (Fig. 8F).

FIG. 8.

Localization of Ccnd1, Ccnd2, and CCnd3 Family members in Akt1^+/+ and Akt1^−/− ovaries at PND50. CCND1, CCND2, and CCND3 protein were analyzed by immunohistochemistry. Immunodetection of CCND1 in Akt1^+/+ (A) and Akt1^−/− (D) ovaries, and immunodetection of CCND1 in the oviduct (I). Weak positive staining for CCND1 is observed in the thecal cells of both genotypes (A and D, arrows). Immunodetection of CCND2 in Akt1^+/+ (B) and Akt1^−/− (E) ovaries. Positive staining, as indicated by diaminobenzidine signal (brown staining), for CCND2 is observed in granulosa cells (GC) of both genotypes (B and E). Immunodetection of CCND3 in Akt1^+/+ (C) and Akt1^−/− (F) ovaries. Positive staining is observed in the nuclei of oocytes from primordial (C and F, asterisks) and primary follicles (C and F, arrows). G) Higher magnification of nuclear staining for CCND1 in Akt1^+/+ follicle (A), which can be observed around the perimeter of the follicle (arrows). H) Higher magnification of nuclear staining for CCND1 in Akt1^−/− follicle (D), which can be observed around the perimeter of follicle (arrows). Cytoplasmic staining for CCND1 is also observed in primordial follicles (bracket). I) Strong nuclear staining for CCND1 is observed in the oviduct; bar = 200 μm.