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Phases of the estrous cycle (diestrus, proestrus, and estrus) were determined using daily vaginal smears, and cycles were followed for at least 2 weeks. Only rats with normal 4 d cycles were considered in the study. For estrogen replacement studies, ovaries were removed from female rats under isofluorane anesthesia (2% in 100% O2), using aseptic technique. Two weeks after the surgery, rats in the estrogen-replaced group (OVX + E) were injected subcutaneously with estradiol benzoate (10 µg) suspended in 0.2 ml of sesame oil (one time per day for 3 d). Rats in the control group (OVX + O) received similar injections of sesame oil only.
The Journal of Neuroscience, March 15, 2003, 23(6):2340
Estrogen Levels Regulate the Subcellular Distribution of Phosphorylated Akt in Hippocampal CA1 Dendrites
Vladimir Znamensky1, 2, Keith T. Akama2, Bruce S. McEwen2, and Teresa A. Milner1 1 Division of Neurobiology, Department of Neurology and Neuroscience, Weill Medical College of Cornell University, New York, New York 10021, and 2 Harold and Margaret Milliken Hatch Laboratory of Neuroendocrinology, The Rockefeller University, New York, New York 10021
ABSTRACT
TOP
ABSTRACT
Introduction
In addition to genomic pathways, estrogens may regulate gene expression by activating specific signal transduction pathways, such as that involving phosphatidylinositol 3-kinase (PI3-K) and the subsequent phosphorylation of Akt (protein kinase B). The Akt pathway regulates various cellular events, including the initiation of protein synthesis. Our previous studies showed that synaptogenesis in hippocampal CA1 pyramidal cell dendritic spines is highest when brain estrogen levels are highest. To address the role of Akt in this process, the subcellular distribution of phosphorylated Akt immunoreactivity (pAkt-I) in the hippocampus of female rats across the estrous cycle and male rats was analyzed by light microscopy (LM) and electron microscopy (EM). By LM, the density of pAkt-I in stratum radiatum of CA1 was significantly higher in proestrus rats (or in estrogen-supplemented ovariectomized females) compared with diestrus, estrus, or male rats. By EM, pAkt-I was found throughout the shafts and in select spines of stratum radiatum dendrites. Quantitative ultrastructural analysis identifying pAkt-I with immunogold particles revealed that proestrus rats compared with diestrus, estrus, and male rats contained significantly higher pAkt-I associated with (1) dendritic spines (both cytoplasm and plasmalemma), (2) spine apparati located within 0.1 µm of dendritic spine bases, (3) endoplasmic reticula and polyribosomes in the cytoplasm of dendritic shafts, and (4) the plasmalemma of dendritic shafts. These findings suggest that estrogens may regulate spine formation in CA1 pyramidal neurons via Akt-mediated signaling events.
Key words: sex steroids; hippocampus; signal transduction; rat; electron microscopy; protein synthesis
Introduction
Estrogen-regulated gene expression is one likely mechanism for regulation of synapse formation in the hippocampal formation (McEwen et al., 2001
). However, estrogens produce rapid effects at membranes via signal transduction intermediates, including those coupled with G-protein receptors (Kelly and Wagner, 1999
, but not ER
, activates PI3-K through interaction with p85
Akt (protein kinase B) is a serine/threonine kinase that mediates the downstream effects of PI3-K, including cell survival and proliferation (Kennedy et al., 1997
Previous studies showed a cyclic buildup and breakdown of synapses on CA1 pyramidal cell dendritic spines across the rat estrous cycle, with peak synaptogenesis occurring when brain levels of estrogen are highest (Gould et al., 1990
This study addresses whether estrogens activate Akt in hippocampal CA1 neurons and considers the implications of this for the regulation of signaling events by estrogen. First, light microscopic densitometry was used to measure the intensity of pAkt immunoreactivity (pAkt-I) in stratum radiatum of CA1 across the estrous cycle and in male rats. Second, the subcellular distribution of pAkt within dendrites, and its possible redistribution in the presence of estrogens, was determined using quantitative electron microscopy (EM).
Materials and Methods
Animals
Adult male (N = 7) and female (N = 25) Sprague Dawley rats (275-300 gm) were obtained from Taconic (Germantown, NY) and housed in groups of three with ad libitum access to food and water. All methods were approved by the Weill Medical College of Cornell University Institutional Animal Care and Use Committee and conform to National Institutes of Health guidelines.Antiserum
A polyclonal rabbit antibody against phospho-Akt (Thr308) was purchased from Cell Signaling Technology (CST; Beverly, MA). Specificity of the antibody was determined using Western blot analysis. This antibody does not detect nonphosphorylated Akt or Akt phosphorylated at other sites; it also does not cross-react with related family members such as PKC or p70 S6 kinase. To confirm the pAkt immunolocalization, a second rabbit polyclonal antiserum to pAkt [anti-phospho-Akt (Thr308); catalog number 06-678] was purchased from Upstate Biotechnology (Waltham, MA). With immunoperoxidase, the topographical distribution of the pAkt-I in the hippocampal formation was similar to that observed using the CST antiserum (data not shown). The pAkt antiserum dilutions for quantitative light microscopy were determined on the basis of criteria described by Reis et al. (1982)Tissue preparation
Rats were deeply anesthetized with sodium pentobarbital (150 mg/kg, i.p.) and perfused through the ascending aorta sequentially with solutions of the following: (1) 10-15 ml of physiological saline (0.9% NaCl) containing 1000 IU/ml heparin; (2) 50 ml of 3.75% acrolein (Polysciences, Warrington, PA) and 2% paraformaldehyde in 0.1 M phosphate buffer (PB), pH 7.4; and (3) 200 ml of 2% paraformaldehyde in PB. The region of the forebrain containing the hippocampal formation was removed and cut into a 5-mm-thick coronal block and postfixed in 2% paraformaldehyde for 30 min. Sections (40 µm thick) through the hippocampal formation were cut on a Vibratome (VT1000S; Leica, Nussloch, Germany) and collected in PB. Sections from each rat were marked and divided into sets consisting of either (1) a male, proestrous, diestrous 1, and estrous females or (2) OVX + E and OVX + O. To maximize uniformity of immunocytochemical labeling conditions for the purposes of quantification, sections from each set of animals were pooled and processed together. Previous studies (Auchus and Pickel, 1992Light and electron microscopic labeling of pAkt
Peroxidase labeling. Tissue was processed for the immunocytochemical localization of pAkt according to the avidin-biotin complex (ABC) procedure (Hsu et al., 1981Data analysis
Quantitative LM. For quantitative comparisons of labeling density, hippocampal sections were measured as described previously (Chang et al., 2000
Results
In the hippocampal formation, pAkt-I is most prominent in CA1 pyramidal neurons
By LM, pAkt-I was observed predominantly in the CA1 subfield of the hippocampal formation, whereas less was observed in the CA3 subfield (Fig. 1A). Much lower levels of pAkt-I were detected in the dentate gyrus. Within the CA1 region, intense pAkt labeling was associated with pyramidal cell somata and their dendrites in stratum radiatum (Fig. 1B, sr). Diffuse pAkt-I also was noticeable in stratum lacunosum-moleculare (SLM) of CA1 (Fig. 1A, slm).
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Figure 1. By LM and EM, pAkt-I is prominent in dendritic processes within stratum radiatum of the hippocampal CA1 region. A, Low magnification LM photomicrograph shows the distribution of pAkt-I (as demonstrated by peroxidase) in a coronal section through the dorsal rat hippocampal formation [corresponds to level 34 of Swanson (1992)
Qualitative EM analysis of the CA1 region in immunoperoxidase-labeled sections confirmed that pAkt-I was prominently associated with the cell bodies, but not the nuclei, of neurons in the pyramidal cell layer (PCL) (data not shown) and with dendritic profiles in stratum radiatum (Fig. 1C,D). Within dendrites, pAkt-I was found throughout the shafts and in select spines (Fig. 1C). However, in some cases, spines emanating from pAkt-labeled dendritic shafts appeared unlabeled (Fig. 1D).
The density of pAkt-I in stratum radiatum is greatest at proestrus
To determine whether the levels of circulating steroids across the estrous cycle and in males influence the expression of pAkt-I in stratum radiatum of CA1, LM quantitative densitometry was used. Densitometric analysis revealed that the intensity of pAkt-I in SR was significantly greater in proestrus rats compared with diestrus and male rats (ANOVA: pro-estrus/diestrus, p = 0.02; proestrus/male, p = 0.0003) (Fig. 2). A similar trend was seen in the PCL, SLM, and dorsal blade of the dentate molecular layer (ML); however, statistical significance was found only between proestrus female rats and male rats in these regions (ANOVA; PCL, p = 0.005; SLM, p = 0.006; ML, p = 0.03).
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Figure 2. The density of pAkt-I in CA1 stratum radiatum is highest in proestrus rats. Representative LM micrographs showing peroxidase pAkt labeling in the CA1 region of a coronal hippocampal section from a diestrus (A) and proestrus (B) rat. C, The density of pAkt-I (measured in pixel density units) in CA1 stratum radiatum differs between female rats across estrus and male rats. Asterisk indicates significant differences from proestrus (ANOVA; Fisher's post hoc). pcl, Pyramidal cell layer; so, stratum oriens; sr, stratum radiatum. N, Number of animals per condition. Scale bar: (in B) A, B, 100 µm.
Consistent with these findings, increased pAkt-I was observed in SR of CA1 in OVX + E rats compared with OVX + O [OVX + E: 17.4 ± 0.9 PDU (N = 5); OVX + O: 12.6 ± 0.5 PDU (N = 5); t test; p < 0.0001). Significantly higher densities of pAkt-I in OVX + E compared with OVX + O rats also were observed in the PCL (OVX + E: 30.0 ± 1.4; OVX + O: 25.2 ± 1; t test; p = 0.002), SLM (OVX + E: 17.6 ± 0.8; OVX + O: 14.1 ± 0.7; t test; p = 0.002), and dentate ML (OVX + E: 8.6 ± 0.3; OVX + O: 7.3 ± 0.4; t test; p = 0.009).
pAkt-I increases in dendritic spines at proestrus
To determine whether the changes in stratum radiatum pAkt-I densities by LM across the estrous cycle and between females and males occur within particular cellular compartments, pAkt-IG-labeled sections from three sets of rats were examined by EM. In agreement with the immunoperoxidase localization of pAkt, pAkt-I identified by immunogold was predominantly in dendritic profiles (Figs. 3A-C, 4A, 5A, 6A). Moreover, pAkt-IG could be discretely localized to the spine apparatus (Fig. 3A,B), the plasma membrane (Fig. 3C) of dendritic spines, and the smooth endoplasmic reticula or plasma membrane of dendritic shafts (Figs. 4B or 6A, respectively). Dendritic shafts and spines containing pAkt labeling appeared morphologically similar between male and female rats.
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Figure 3. By EM, pAkt-IG labeling associated with dendritic spines is significantly higher in proestrus rats. A-C, Representative electron micrographs showing the distribution of pAkt-IG particles (arrowheads) associated with the spine apparatus (A, B) or the plasma membrane (C) of dendritic spines. Unlabeled terminals (uT) contact both labeled spines. In B, the labeled spine arises from a pAkt-IG-labeled dendritic shaft (pAKT-D). D, The total number of pAkt-IG particles in dendritic spines (number of pAkt-IG particles associated with both cytoplasm and plasma membrane of spines per 100 µm2 of tissue) is significantly higher in proestrus rats. E, The relative number of labeled spines is highest in proestrus. The relative number of labeled spines was calculated as the number of dendritic spines containing pAkt-IG particles (i.e., pAkt-labeled) divided by the total number of dendritic spines (i.e., labeled + unlabeled) as represented per 100 µm2 of the total field of 9632 µm2 for each rat. Asterisk indicates significant differences from proestrus (unpaired t test). N, Number of rats per condition. Scale bar: (in C) A, B, C, 50 µm.
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Figure 4. In dendritic shafts, pAkt-IG labeling associated with endoplasmic reticula and polyribosomes is highest in proestrus rats. A, Representative electron micrograph showing pAkt-IG particles associated with endoplasmic reticula (arrowheads) of a pAkt-IG-containing dendritic shaft profile (pAKT-D). B, Variations in the number of pAkt-IG particles per 1 µm2 of dendritic area that are associated with endoplasmic reticula and polyribosomes in dendritic shafts of female rats across estrous and male rats. Asterisk indicates significant differences (unpaired t test) from proestrus rats. n = number of dendrites analyzed from three rats per condition. Scale bar, 50 µm.
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Figure 5. pAkt-IG labeling near the base of dendritic spines is highest in proestrus rats. A, Representative electron micrograph showing a pAkt-IG particle (arrowhead) affiliated with a portion of the spine apparatus located within 0.1 µm from the base of a dendritic spine. B, Variations in the number of pAkt-IG particles within 0.1 µm of the bases of dendritic spines in female rats across estrous and male rats, calculated per dendrite. Asterisk indicates significant differences from proestrus (unpaired t test). n = number of dendrites analyzed from three rats. Scale bar, 50 µm.
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Figure 6. The number of pAkt-IG particles on the plasma membrane of dendritic shafts is highest in proestrus rats. A, Representative electron micrograph of a dendritic shaft profile showing pAkt-IG particles in the cytoplasm (arrows) and on the plasma membrane (arrowheads). B, The total number of pAkt-IG particles per 1 µm of dendritic plasma membrane of dendritic shafts is significantly different in proestrus rats compared with disestrus rats (unpaired t test; *p < 0.05). C, Cytoplasmic pAkt-IG particles in dendritic shafts (expressed per 1 µm2) are not significantly different between female rats across estrous and male rats. n = number of dendrites analyzed from three rats per condition. Scale bar, 50 µm.
Quantitative EM analysis revealed an almost a sixfold increase in the number of pAkt-IG particles associated with the dendritic spines (both cytoplasmic and plasma membrane) of proestrus rats compared with diestrus and estrus rats (t test; p < 0.0001) and an approximately threefold increase in the number of pAkt-IG particles associated with dendritic spines in proestrus female rats compared with male rats (t test; p < 0.0001) (Fig. 3D). To address the possibility that the increase in pAkt-IG labeling simply reflects a scaling up with the overall increases in spine number that occur in the proestrus phase of the estrous cycle (Woolley, 1998
In dendritic shafts, significantly more pAkt-IG particles were associated with endoplasmic reticula (Fig. 4A) and structures resembling polyribosomes (Steward and Falk, 1991
To determine whether the increases in pAkt-I seen at the light level were a result of increased levels of pAkt-I within dendritic shafts, the total number of pAkt-IG particles was determined. The total number (i.e., cytoplasm + plasma membrane) of pAkt-IG particles per square micrometer of dendritic shaft profiles was not significantly different across estrous females and in males [proestrus (n = 150): 0.30 + 0.01/µm2; diestrus (n = 150): 0.30 + 0.1/µm2; estrus (n = 150): 0.30 + 0.1/µm2; male (n = 150): 0.27 + 0.01/µm2; p > 0.05]. However, when the distribution of pAkt-IG particles on the plasma membrane and within the cytoplasm was analyzed separately, proestrous rats had a significantly higher number of pAkt-IG particles on the plasmalemma (t test; p < 0.0001) compared with diestrous rats (Fig. 6B). No significant differences between the groups (t test; p = 0.05) were found in the number of gold particles within cytoplasm (Fig. 6C). These results show that pAkt-IG particles redistribute, without changing in number in dendritic shafts, in response to fluctuating ovarian hormone levels.
Discussion
This study demonstrates that proestrus rats compared with diestrus, estrus, and male rats contained a significantly higher number of pAkt-IG particles associated with (1) dendritic spines (both the cytoplasm and plasma membrane), (2) spine apparati located within 0.1 µm of dendritic spine bases, (3) endoplasmic reticula and polyribosomes in the cytoplasm of dendritic shafts, and (4) the plasma membrane of dendritic shafts. Because previous studies have shown that both brain estrogen levels and synaptogenesis are elevated during the proestrus phase of the cycle (Gibbs, 1996
Methodological considerations
The present study discovered differences in pAkt-I at the light microscopic level by comparing densitometric measurements of immunoperoxidase reaction product. When sufficiently high dilutions of primary antisera are used, this method has proven reliable for quantifying differences in immunolabeling across experimental conditions (Pierce et al., 1999
Estrogens increase pAkt-I in pyramidal cell bodies
By light microscopy, the intensity of pAkt-I in the pyramidal cell layer was highest in proestrous or OVX rats with estradiol supplements. Estrogen-mediated stimulation of PI3-K and the subsequent phosphorylation of pAkt in cell bodies may be linked to a wide array of signaling effects, including neuroprotection, cell proliferation, metabolic regulation, differentiation, and protein synthesis (Downward, 1998
Estrogens may induce pAkt translocation to dendritic membranes
By light microscopy, the density of pAkt-I in stratum radiatum of CA1 was highest in proestrus rats and OVX rats supplemented with estradiol benzoate. Moreover, by electron microscopy, the number of pAkt-IG particles on the plasmalemma of dendritic profiles was increased in proestrus rats (although the total number of pAkt-IG particles in dendritic shafts was not changed). Akt is known to translocate to the plasma membrane after association of its pleckstrin homology domain with lipids produced by PI3-K; such steps are necessary for presentation of Akt to upstream activating kinases (Hemmings, 1997
Putative pAkt involvement in estrogen-regulated synaptogenesis
During proestrus, pAkt-I is significantly increased in dendritic spines but not dendritic shafts in stratum radiatum of the CA1 region. Previous studies have shown that both brain estrogen levels and synaptogenesis are highest during this phase of the cycle (Gibbs, 1996
Involvement of pAkt in estrogen-mediated signaling events
The present demonstration that estrous cycle-dependent pAkt-I is found in dendritic spines, together with our previous findings that ER
pAKT may be involved in local protein synthesis
Synapses that undergo changes in strength are in need of newly synthesized proteins; in addition to transporting new proteins from the soma, another possible mechanism is local protein synthesis regulated by synaptic activation (Steward and Schuman, 2001
In conclusion, our findings that the highest levels of estrous cycle-dependent pAkt-I in dendritic spines are observed when dendritic spine and synapse formation also are highest supports a mechanism whereby estrogens regulate local signal transduction in vivo, via the Akt/4E-BP1 pathway. Such a localized mechanism responsive to estrogen would be instrumental to the rapid, hormone-regulated cyclic formation of synapses that occurs in the CA1 region of the hippocampus.
FOOTNOTES Received Aug. 5, 2002; revised Dec. 13, 2002; accepted Jan. 2, 2003.
This work was supported by National Institutes of Health Grants NS07080, DA08259 (T.A.M.), HL18974 (T.A.M.), and MH12977 (K.T.A.) and the Ares-Serono Foundation (K.T.A.). We thank Dr. Joseph P. Pierce for his assistance with quantitative immunocytochemical methodology and statistical analysis and Dr. Carrie T. Drake for her helpful suggestions on this manuscript.
Correspondence should be addressed to Dr. Teresa A. Milner, Division of Neurobiology, Weill Medical College of Cornell University, 411 East Sixty-ninth Street, New York, NY 10021. E-mail: tmilner{at}mail.med.cornell.edu.
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