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The Journal of Neuroscience, July 15, 1998, 18(14):5294-5300
Comparison of Hippocampal Dendritic Spines in Culture and in Brain
Christopher Boyer, Thomas Schikorski, and Charles F. Stevens Molecular Neurobiology Laboratory, and Howard Hughes Medical Institute at The Salk Institute, La Jolla, California 92037
ABSTRACT
Top
Abstract
Introduction
We have quantified hippocampal spine structure at the light and ultrastructural levels in cell cultures ~1- 3 weeks old and in the brains of rodents 5 and 21 d old. The number of spines bearing synapses increases with age in cultures and in brain, but the structures are similar in both. In culture, about half of the synapses are formed on spines and the remainder are formed on dendritic shafts. In the 5-d-old brain, about half of the synapses occur on dendritic shafts, by 3 weeks of age only ~20% of synapses are found on dendritic shafts, and in the adult shaft synapses are very rare.
Key words: synapse; culture; ultrastructure; spines; hippocampus; morphometry
INTRODUCTION
In cortex and in the cerebellum, most excitatory contacts are made on spines, those peculiar thorn-like structures believed since Ramón y Cajal (1891
, 1896
Because synapses are so densely packed in the gray matter of the CNS
on the order of a billion per microliter, studies of synaptic function can sometimes be greatly facilitated by the use of neuronal cell cultures where the synapses are arrayed essentially in two dimensions at relatively low densities. To compare data obtained in culture with observations made in slices and in vivo, however, one must know how culture synapses compare with their brain counterparts. One property of synapses that is important for such comparisons is their structure. Schikorski and Stevens (1997)
Papa et al. (1995)
Our study had a second motivation. Because spines are believed to be of functional significance, particularly perhaps for synaptic plasticity, it is important to know what fraction of the synapses in culture are made on spines rather than on dendritic shafts. We thus estimated the spine/shaft synapse prevalence for cultures of the type used in physiological investigations and also for the young [postnatal day 21 (P 21)] rat brain, another preparation important for certain physiological studies. If spines are required to provide a separate biochemical compartment for specific synaptic functions, then synapses in culture and those in the young rodent brain may constitute a good model of mature brain synapses only to the extent that culture and young brain synapses occur on spines.
In confirmation of earlier studies, we find that the density of spine synapses increases as cultures mature. At comparable ages, however, spine synapses in culture are more than threefold less abundant per dendritic length than they are in brain. Most importantly, perhaps, we find that only ~50% of the excitatory synapses in culture are on spines, whereas 80% of such synapses occur on spines in the 2-week-old brain; in the adult brain, excitatory synapses on dendritic shafts are very rare. We believe that these observations have implications for studies of synaptic plasticity (long-term potentiation and depression) in culture and in brain slices from young animals.
MATERIALS AND METHODS
Primary neuronal cells were grown on inverted glass coverslips suspended above a feeding layer of astrocytes according to the method of Banker and Goslin (1991)
Preparation of the astrocyte feeder layer. To provide support for inverted coverslips, a hot soldering iron was used to make three to four small melted plastic beads in the bottom of each collagen/poly-D-lysine-coated well of a tissue culture dish (Costar, Cambridge, MA). Type 1 astrocytes were purified from 5-d-old heterogeneous hippocampal cell cultures through rigorous agitation for 24-48 hr. The purified astrocytes were trypsinized from the bottom of the flask, washed, and replated at a density of 5000 cells per beaded well in 0.5 ml growth medium [DMEM, 10% heat inactivated fetal calf serum (Life Technologies, Gaithersburg, MD), 20 mM glucose, 50 U/ml penicillin, 50 mg/ml streptomycin, N-2 supplement (1:200, Life Technologies), and phenol red]. Astrocytes were incubated for 3-4 d at 37°C and 5% CO2 until they developed confluent monolayers. Immediately before neuronal culture preparation, the growth medium was exchanged with neuronal medium [DMEM with 25 mM HEPES, 10% horse serum (Life Technologies), 20 mM glucose, penicillin/streptomycin, N-2 supplement (1:100), sodium pyruvate (1 mM), and 1 mg/ml biotin].
Neuronal culture preparation. Hippocampi from 1- to 2-d-old rats (Long-Evans) were dissected in Earl's buffered salt solution (EBSS, Life Technologies) with 10 mM HEPES. The dentate gyrus area was cut off, and the remaining hippocampal tissue was chopped into small blocks. These blocks of tissue were incubated with periodic agitation in Papain (~20 U/ml EBSS) for 0.75-1.5 hr at 37°C. Tissue was washed with growth medium and dissociated into single-cell suspension with multiple passages through a 5 ml plastic pipette. Cells were plated on collagen/poly-D-lysine-coated coverslips at a density of 6000-8000 cells per well in 0.5 ml neuronal medium. After 3-4 hr, coverslips were inverted and placed into the beaded wells containing established astrocyte feeder layers and 0.5 ml neuronal medium. Arabosylcytosine (5 mm) was added after 1-2 d to inhibit proliferation of non-neuronal cells.
Lucifer yellow injections. At different ages (6, 10, 14, 21 d in vitro), individual coverslips were fixed in 4% paraformaldehyde for 5-10 min at room temperature. Single cells were impaled under visual control with sharp microelectrodes, and a constant current of
2-5 nA injected Lucifer yellow for 5-15 min. Successful injected cells were post-fixed further with 4% paraformaldehyde for 5 min.
Immunocytochemistry. Coverslips with Lucifer yellow-filled cells were permeabilized in methanol for 5-10 min at
Image analysis. Images of all dendrites of successfully filled cells were acquired with a video microscope at a magnification of 60×, with a filter set for Lucifer yellow and for Texas Red. Image pairs were contrast-enhanced, and measurements were made by using the MetaMorph Tools (Universal Imaging Corporation, West Chester, PA).
Electron microscopy. One 5-d-old and one 21-d-old Long-Evans rat were perfused through the heart under deep Nembutal anesthesia (80 gm/25 gm body weight). A short perfusion with oxygenated saline was followed by a perfusion with 70 ml of 4% glutaraldehyde in 100 mM phosphate buffer, pH 7.4. The brains were dissected and immersed in the same fixative overnight at room temperature. Vibratome sections including the hippocampus were cut and post-fixed in 1% OsO4 for 1 hr at 4°C. After dehydration in ethanol, sections were contrasted en bloc in 0.5% uranyl acetate and flat-embedded in Epon.
Cultured hippocampal cells were fixed and processed as described previously (Schikorski and Stevens, 1997
RESULTS
Quantitative analysis of serial electron micrograph sections is the preferred way to study a structure, such as a spine, that is so close to the light microscope limit of resolution. Unfortunately, such an analysis is prohibitively difficult for a large sample of synapses. Therefore, we have made the same compromise advocated by earlier investigators: use of the light microscope to obtain a relatively large sample size (~7000 spines here) supplemented with limited electron microscopic analysis for confirmation of major conclusions based on the lower resolution observations. We have filled cells with Lucifer yellow to visualize spines and have identified synapses with synaptophysin immunohistochemistry (Fig. 1).
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Figure 1. Original fluorescence staining of the same dendrite of a hippocampal cell in culture. A, Dendrite after filling with Lucifer yellow. B, The corresponding immunocytochemical staining against synaptophysin. The arrows in both images point to the sites of spines, and the arrowheads point to the site shaft synapses.
Because most electrophysiological studies of cultured neurons use cells grown for 2-3 weeks in vitro, we have studied cultures that were maintained for 6, 10, 14, and 21 d. We defined a spine as a fine protrusion from the dendritic shaft that occurs in close apposition to an anti-synaptophysin positive bouton (Fig. 1). A presynaptic element adjacent to the spine head was not the only criterion for inclusion. Fine protrusions with a bouton at their base were counted as well as spines, because we frequently found synapses in culture on spine necks at the ultrastructural level. We identified a synapse as occurring on a dendritic shaft when we could not detect a fine protrusion adjacent to the immunolabeled bouton. Because the dendritic shaft in some cases could obscure a short spine, our inclusion criteria probably led to some undercounting of spine synapses. We return to this issue in Discussion. Electron microscopy was performed on cultures at 14 d in vitro (DIV; approximately equivalent to postnatal age) and for comparison on a rat brain at P5 and P21 (Fig. 2).
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Figure 2. Ultrastructure of developing synapses. A, The largest spine (star) we encountered in our sample of synapses at P21. All typical structural features are present at that age; the postsynaptic density is aligned with the active zone. The spine had the typical grainy dense appearance, and the spine apparatus is visible. B, Spines from hippocampal neurons in culture after 14 DIV. Spines (stars) in culture show no qualitative difference from their counterparts in situ. Shaft synapses are marked with a star on a white background. Scale bars, 0.5 µm.
Spine densities
We found that spine densities are low at 6-10 DIV and then double or triple in number by 14-21 DIV (Fig. 3). Specifically, the younger cultures exhibit approximately 0.2 spine synapses per micrometer of dendritic length, whereas the older cultures (2-3 weeks) have approximately 0.5 spine synapses per micrometer of dendritic length. Compare these spine densities with modern estimates of 1.7 spine synapses per micrometer of dendritic length in adult hippocampus (Trommald et al., 1995
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Figure 3. Comparison of synaptic density in culture as a function of time. The different bars depict the number of spine synapses (white bars), the number of shaft synapses (gray bar, calculated as the differences from total synapses minus spine synapses), and the number of all synapses (striped bars). Between 10 and 14 DIV there is a significant increase of synaptic density. Before and after this age the density of spine and shaft synapses is constant. Note that the relationship between shaft and spine synapses is equal for all ages.
Interestingly, the density of synapses (the number of spine synapses per length of dendrite) changes little from 2 to 3 weeks in culture. At 2 weeks, we counted 0.44 spines per micrometer of dendritic length, and at 3 weeks the density was 0.45 spines per micrometer. One would expect synaptogenesis to continue in the third week, so this constancy presumably represents a dynamic balance between synapse formation and elimination.
In addition, we measured all spine-like objects (innervated and not innervated) on dendrites at the various times in vitro. This measure should be comparable to the data of Papa et al. (1995)
Shaft versus spine synapses
In brain, excitatory synapses on the shafts of spiny dendrites are very rare (Harris and Kater, 1994
Length distributions
The distributions of spine lengths for each of the age groups are presented in Figure 4. In our images a single pixel had the length of 0.17 µm, and we have sorted spine lengths into bins of 0.5 µm, which corresponds to approximately three image pixels. Any spines shorter than ~0.5 µm were not included in our measurements. As is apparent from all of the distributions, a spine length of 1-1.5 µm is most common for every age. In the 2- to 3-week-old cultures, however, the prevalence of longer spines decreases, so that the mean spine length decreases with age (Fig. 4, inset). By the time cultures are 2-3 weeks old, almost all of the spines are 1-1.5 µm long.
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Figure 4. Spine length distribution in culture at different ages. Most of the spines have a length of 1-1.5 µm. Note that the occurrence of longer spines in young cultures is significantly increased. The inset depicts the decreasing mean spine length and SE over time.
Electron microscopic studies of synapses in culture
Because structural features of spines are near or below the resolution of the light microscope, we felt that it was important to confirm our major light microscopic observations with electron microscopy, especially the ratio of spine/shaft synapses. Therefore we have counted shaft and spine synapses in culture in electron microscopic images from serial sections and have confirmed that they appear in approximately equal numbers. In a sample of 29 synapses, we found 14 on spines and 15 on the dendritic shaft at 14 DIV in culture. All of these synapses were morphologically classed excitatory, with the typical asymmetric structure and round synaptic vesicles. We found only two symmetric contacts on dendritic shafts, and these were not included within our sample. The spine head volume was on average 0.058 ± 0.034 µm3. For data on postsynaptic density area and number of docked vesicles, see Schikorski and Stevens (1997)
Ultrastructure of synapses at P5
At P5, for 14 CA1 synapses in two series of sections (27 sections total), we found 5 (36%) spine synapses and 9 (64%) shaft synapses. All spines were innervated by only one presynaptic bouton, and no bouton formed more than one synapse. The synaptic density is very low compared with that in older animals (in our series, approximately six times lower than at P21), which is the reason for our small sample size. For a quantification of synaptic structure at this age, we pooled all synapses; the result is shown in Table 1. With the exception of bouton volume, all structural features of synapses are highly correlated, whereas the bouton volume is correlated significantly only with the total number of vesicles. Because we encountered only five spines in our sample, we did not include spine head volume data in the table. The spine head volumes were 0.0323, 0.0516, 0.0716, 0.0837, and 0.1314 µm3.
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Table 1. Sizes of various structures at hippocampal synapses at P5 and their intercorrelations Ultrastructure of synapses at P21
Because many physiological experiments use hippocampal slices from several week-old rodents, we have, in addition to examining spines in culture, quantified some of the aspects of spine morphology at P21 at the ultrastructural level. It is potentially important to know how different the spine morphology is compared with the adult animal for the interpretation of physiological experiments. We found that 82% (71/87) of the synapses in a region of stratum radiatum were found on spines; thus, spine synapses predominate at P21 in contrast to the P5 hippocampus, where most synapses are on dendritic shafts. Nevertheless, nearly one fifth (16/87) of the excitatory synapses in hippocampus (CA1) at P21 were formed on shafts. We encountered in the young animals the entire spectrum of spine morphologies that have been described for the adult. From the total number of 87 synapses, we reconstructed 26 synapses fully contained in serial sections. two spines (7.7%) made contact with two different boutons, and one spine (3.8%) was innervated by three boutons. All other spines formed only one synapse. On the presynaptic side, one (3.8%) bouton formed four synapses (which had four distinct active zones opposite four different postsynaptic elements), and five boutons formed two synapses. Two of those boutons formed one spine and one shaft synapse. Schikorski and Stevens (1997)
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Table 2. Sizes of various structures at hippocampal synapses at P21 and their intercorrelations
DISCUSSION
We found that dendrites of hippocampal cells in culture possess at most only one third of the spine density observed on their counterparts in brain at a comparable age. Furthermore, about half of the excitatory synapses in culture were on the dendritic shaft, whereas the vast majority of excitatory synapses in mature brain are formed on spines (Harris and Kater, 1994
Our data confirm and extend those published previously (Papa et al., 1995
We are confident that shaft and spine synapses occur at the ultrastructural level in approximately equal numbers as we report here, because we have found this to be true in many electron micrographs of cultures not formally included in the present study. Nevertheless, we must stress the limitations of the use of electron microscopy for the quantitative analysis of synapses in culture. The basic problem is the low density of synapses in cultures (of the type used for electrophysiological studies) as compared with brain. Because synapses are so abundant in brain, a typical set of 30 serial sections contains an adequate sample of synapses for reconstruction and measurement. The same series of sections made from culture will provide only 10-20 synapses. Furthermore, measurement of the length of extended structures, such as spines, is correspondingly more difficult in culture. Because of our small sample of culture synapses, one must recognize that measured sizes are less certain than for brain.
At P5, the ultrastructures of spines and synapses appear quite similar to their counterparts in older animals (Harris et al., 1989
When we compared our ultrastructural data at P21 with data from Harris et al. (1992)
A quantitative comparison of spine synapses at P21 with their counterparts in culture at 14 DIV shows that the postsynaptic density/active zone sizes are comparable, whereas the spine head volume is smaller in brain synapses. The synaptic density at P21 is rather similar to that of the adult and thus much higher then after 14 DIV.
We used t test to compare our data of P21 with the data from adult mouse (Schikorski and Stevens, 1997
Several groups have reported that long-term depression (LTD) in culture is resistant to the NMDA receptor antagonist 5-amino-pyridine (AP-5) (Deisseroth et al., 1996
Long-term potentiation (LTP) is know to "wash out" with whole-cell recording, a phenomenon attributed to the need for a distinct postsynaptic compartment. The greater difficulty in inducing LTP in culture and in slices from young animals might relate to the relatively large fraction of shaft rather than spine synapses in these neurons. In any case, the investigator of synaptic plasticity must be aware that the anatomical situation in culture and young animals is not identical to that in older animals and be alert to possible differences that derive from the structural factors noted here.
The picture of central synaptogenesis originally proposed by Morest (1969a
Conclusion
Because we do not fully understand the function of spines, the full significance of our findings for understanding synaptic function is still uncertain. Qualitatively, most structural properties of synapses are indistinguishable between culture and hippocampus at P5 forward, but some quantitative features are quite different. The relative abundance of shaft synapses in culture may be the most prominent difference. Additionally, spines in culture have a relatively larger volume, comparable to spines at P5. On the other hand, the postsynaptic density/active zone sizes in cultured spines are similar to their in situ counterparts at P21 or in adults. It seems that the reduction in spine size seen in brain may not be necessary in culture, because cells and their processes are not as densely packed as in the brain (a similar statement can be made about the bouton volume in culture and in young animals). The synaptic physiologist must ensure that such differences do not limit the range of validity for conclusions about synaptic function based on observations in culture and in slices from young brains.
FOOTNOTES Received March 23, 1998; revised May 4, 1998; accepted May 6, 1998.
This work was supported by the Howard Hughes Medical Institute, National Institutes of Health Grant NS 12961 (C.F.S.), and National Institutes of Health, Neuroplasticity of Aging training Grant (T.S.). We thank Dr. Reinhard Jahn for his gift of anti-synaptophysin antibody (G96), Richard Jacobs for his technical assistance, and Carrie Musick for her help with this manuscript.
Correspondence should be addressed to Dr. Charles F. Stevens, Molecular Neurobiology Laboratory, and Howard Hughes Medical Institute at The Salk Institute, 10010 N. Torrey Pines Road, La Jolla, CA 92037.
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Copyright © 1998 Society for Neuroscience 0270-6474/98/18145294-07$05.00/0
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Ultrastructural Correlates of Quantal Synaptic Function at Single CNS Synapses
J. Neurosci., June 15, 1999; 19(12): RC13 - RC13.
[Abstract] [Full Text] [PDF]
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