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The Journal of Neuroscience, July 1, 1998, 18(13):4825-4832
Age-Related Changes in Neuronal Nicotinic Acetylcholine Receptor
Subunit  4 Expression Are Modified by Long-Term Nicotine
Administration
Scott W.
Rogers1,
Lorise C.
Gahring1,
Allan
C.
Collins2, and
Michael
Marks2
1 Salt Lake City Veterans Affairs Medical Center,
Geriatric Research, Education, and Clinical Center, and the University
of Utah School of Medicine, Salt Lake City, Utah 84112, and
2 University of Colorado, Institute for Behavioral
Genetics, Boulder, Colorado 80309
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ABSTRACT |
The distribution of the neuronal nicotinic acetylcholine receptor
subunit  4 (nAChR4) in the brains of young (2-4 months) or aged
(24-28 months) CBA/J mice was examined using immunohistochemical staining. Anti-nAChR4 immunoreactivity corresponded with nAChR4 RNA expression and high-affinity [3H]nicotine
binding. Immunostaining in aged mice relative to that in young animals
was diminished in the medial septum and diagonal band but was unchanged
in the globus pallidus and substantia nigra. The staining of neurons
was almost completely absent in the hippocampus of aged animals. The
oral administration of nicotine to aged animals for 6 weeks did not
alter nAChR4 expression relative to that in aged controls. However,
the long-term delivery of nicotine (11 months) to 14-month-old animals
corresponded with the highly specific preservation of nAChR4
expression in some neurons of the dentate gyrus region and in neurite
processes of remaining neurons of the hippocampal CA1 region. These
results support the conclusion that the loss of nAChR4 expression
occurs in key cholinergic regions during normal aging. Furthermore,
sustained long-term nicotine delivery may promote highly
region-specific retention of nAChR expression, but only if initiated
before normal age-related receptor decline.
Key words:
nicotine; acetylcholine; receptors; aging; neurobiology; mammal
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INTRODUCTION |
Changes in the expression of
nicotinic-cholinergic neurotransmitter receptor systems have been
implicated in the onset of age-related brain dysfunction. For example,
the cholinergic hypothesis of dementia is based on the well established
damage to or loss of cholinergic neurons of the forebrain as reflected
by the dramatic loss of cholinergic system markers including
acetylcholine transferase or acetylcholine esterase (e.g., see Shroder
et al., 1991 ; Giacobini, 1992). Even during normal aging, in which many
of the symptoms of cholinergic depletion are not manifested until later
in life (i.e., older than 80 years), there is an age-associated
diminished expression of high-affinity
[3H]nicotine ligand binding sites (Whitehouse et
al., 1986, 1988; Kellar et al., 1987, 1989; Shroder et al., 1991;
Giacobini, 1992). In addition to the depletion in humans, the normal
age-dependent depletion of [3H]nicotine binding
sites also occurs in the rodent brain (Araujo et al., 1990; Zhang et
al., 1990; Schulz et al., 1993; Flood and Coleman, 1996). Consequently,
the loss of these sites in the aging mammalian brain should coincide
with the loss or change in the expression of subunit proteins that
compose these receptors.
The family (see Sargent, 1993; Lindstrom, 1996) of related cDNAs that
encode mammalian neuronal nicotinic acetylcholine receptors (nAChRs)
includes at least seven -like subunits (2, 3, 4, 5,
6, 7, and 9) (Elgoyhen et al., 1994) and three  -like
subunits (2, 3, and 4). Mature receptors are composed of
pentameric combinations of these subunits that impart to these ion
channels their distinct functional properties. The expression of these subunits is in part regulated transcriptionally because each is expressed in unique, but overlapping, brain regions (see Deneris et
al., 1991; Marks et al., 1992). Post-transcriptional mechanisms also
influence receptor expression because the administration of nicotine to
rodents [either in their drinking water or by direct infusion into the
brain (Marks et al., 1985, 1991, 1992; Kellar et al., 1989; Collins et
al., 1996; Booker and Collins, 1997)] increases the binding of
[3H]nicotine by as much as threefold without
changing subunit transcript numbers (Marks et al., 1992). The principal
receptor subunit combination that composes the high-affinity
[3H]nicotine binding site in both mammals and
chickens consists of subunits 4 and 2 (Anand et al., 1991;
Whiting et al., 1991; Flores et al., 1992, 1996). Furthermore,
immunoprecipitation of nAChR4 or nAChR2 accounts for >80% of
the increase in high-affinity ligand binding after chronic nicotine
administration (Flores et al., 1992, 1996). When only these two
subunits are expressed in transfected cells, high-affinity ligand
binding sites are created, and they can also be upregulated by a
nicotine-related decrease in receptor degradation (Whiting et al.,
1991; Peng et al., 1997). Because the nAChR2 subunit is widely
expressed in the nervous system (Swanson et al., 1987; Deneris et al.,
1988, 1991; Hill et al., 1993) and exhibits relatively little
selectivity in associating with other nAChR subunits (e.g., Boulter
et al., 1987; Deneris et al., 1991; Flores et al., 1992, 1996;
Lindstrom, 1996), the detailed examination of immunoreactivity to the
nAChR4 subunit was selected to reflect most accurately the
expression of this receptor in the rodent brain.
The possibility that chronic exposure to nicotinic pharmacological
agents and the subsequent upregulation of ligand binding sites may be
exploited as a therapeutic strategy to combat age-associated cognitive
decline has gained considerable interest (e.g., Nicholson, 1994). Taken
together with the above reports, determining whether acute or long-term
nicotine administration alters the distribution or expression of
nAChR4 is an important first step in this assessment. We have used
antibodies to the nAChR4 subunit to examine the distribution and
expression of immunoreactivity to this subunit in the brains from young
(3-4 months) CBA/J mice and compared this pattern of expression with
that observed in the aged (24-27 months) CBA/J brain. In addition, we
have examined anti-nAChR4 immunoreactivity after the oral
administration of nicotine to aged animals for 6 weeks and to adult
animals (14 months) for 11 months.
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MATERIALS AND METHODS |
Antibodies. The preparation of rabbit polyclonal
anti-nAChR4 subunit antisera has been described previously (Rogers
et al., 1991a,b, 1992; Flores et al., 1992, 1996; Cauley et al., 1996). Immunogen in the rabbits designated 5008 or 5009 was a portion of the
cytoplasmic domain of rat nAChR4 expressed as a fusion protein in
bacteria (Rogers et al., 1991a,b; Flores et al., 1992).
Mouse strain, fixation, and immunohistochemistry. CBA/J mice
were obtained through the National Institute on Aging. Mice were perfused with fixative, and free-floating brain sections were prepared
and stained as described elsewhere (Gahring et al., 1996). Rabbit
anti-nAChR4 polyclonal serum was added at a 1:1000 dilution overnight at 4°C with gentle rocking; the sections again were washed
with PBS, and secondary goat anti-rabbit peroxidase (Jackson Immunolaboratories) was added at a 1:750 dilution in blocking PBS for 1 hr at room temperature. Immunoreactivity was revealed by adding
diaminobenzidine (DAB; 100 µg/ml) and H202
(0.0001%) in PBS to the sections at room temperature with gentle
rocking. Sections were washed with PBS to stop development, mounted on microscope slides, and coverslipped before analysis.
Data analysis. Serial sections were mounted on microscope
slides for imaging and subsequent analysis. In all cases, six to eight
fields including both ipsilateral and contralateral regions from the
same relative anatomical level were digitized and used for quantitative
comparisons with Image-Pro Plus software (Media-Cybernetics). For each
animal, at least three sections were scored bilaterally for
immunoreactivity. Double-label experiments (data not shown) included
rabbit anti-nAChR4 antiserum, and either mouse anti-neurofilament antibody (Sigma, St. Louis, MO; or Boehringer Mannheim, Indianapolis, IN), anti-glial fibrillary acidic protein (Boehringer Mannheim), or rat
monoclonal mAB299 to anti-nAChR4 (Research Biochemicals, Natick, MA)
confirmed neuronal staining and concordance between reagents. No cells
were detected that colabeled with anti-nAChR4 and anti-glial
fibrillary acidic protein (Sigma) (data not shown). All anatomical
regions were defined as described by Franklin and Paxinos (1997).
For quantitative analysis, immunopositive cells were defined as those
exhibiting somal staining, and only cells with a stained unit area
sufficient to ensure that the majority of their volume was contained
within the section were scored. Values for each region and from each
animal were collected and summed, and an average was derived for each
age or treatment group. Both cell number per anatomically defined
region and cell number per unit area were calculated. In our
experience, both values gave similar results; however, because of the
possibility that section mounting to glass slides and poststaining
dehydration could alter the unit area measure, we have selected to
report our results in terms of immunopositive cells per region.
Statistical analyses were applied to indicate the relative significance
of differences between different regions of the young and aged brain as
reported in the text for each experiment using either the Student's
t test, ANOVA, or the Mann-Whitney rank sums nonparametric
statistical test. The best use of statistical approaches is somewhat
unclear in these studies. Although we draw on a random population of
young or aged animals available through the National Institute on
Aging, we cannot be certain that aged animals actually represent a
statistically defined normal population. For example, the analysis of
humans that live to be 100 years of age does not necessarily reflect the physical or mental conditions "typical" of an aged population, particularly because the majority of aged individuals have already died. Therefore, although the young or adult population would be
expected to be drawn from a "normal" population, caution must be
exercised when assuming this for the aged population. Consequently, we
chose to apply both parametric and nonparametric tests. Although we
present the results of only parametric tests, in this study both
statistical methods gave qualitatively the same answer.
Nicotine administration. Short- or long-term nicotine
delivery was done by supplementing the drinking water with saccharin (2%) and nicotine [experimental, nicotine tartrate (Sigma)] or with
saccharin alone (control group). For short-term experiments, aged
(24-month-old) CBA/J mice were given nicotine (25 µg/ml on day 1, 50 µg/ml on days 2-3, 100 µg/ml on days 4-6, and 200 µg/ml thereafter) for 6 weeks. The addition of nicotine to the drinking water
resulted in an increase by two- to fourfold as measured by
[3H]cytisine of the number of high-affinity
[3H]nicotine binding sites in the brains of mice
treated separately (data not shown), a result consistent with recent
studies (Collins et al., 1996; Booker and Collins, 1997). For long-term
exposure, CBA/J mice that were 14 months old were administered nicotine in their water as described above for 11 months before analysis. This
age group was selected because preliminary examination of neuronal
expression of nAChR4 immunoreactivity in these animals did not
differ from that in the young age group (data not shown). In each
group, the controls received no nicotine in the water. For all animals,
at 4 weeks after nicotine administration, a small blood sample was
collected from each animal to ensure nicotine uptake and metabolism by
measuring for the presence of cotinine (STC Corporation, Bethlehem,
PA). Although water administration of nicotine produces a less robust
response than does direct infusion of the brain and the administration
occurs principally at night when the animal is active and drinking
(Collins et al., 1996; Booker and Collins, 1997), this regime may more
closely resemble physiological administration than does direct
infusion. For animals that received long-term nicotine, this method of
administration presents a clear technical advantage over the
methodology required to infuse nicotine directly into the brain.
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RESULTS |
Anti-nAChR4 antiserum subunit specificity
The specificity of immunoreactivity of the rabbit anti-nAChR4
antiserum (rabbits 5008 and 5009) has been addressed in previous studies (Rogers et al., 1991a,b, 1992; Flores et al., 1992, 1996; Cauley et al., 1996). These results include the absence of staining by
preimmune serum, specific labeling of nAChR4 protein on Western blots and ELISA analysis, and specific immunoprecipitation of high-affinity [3H]cytisine binding sites (Flores
et al., 1992, 1996) but not receptors composed of 3+2 (Flores et
al., 1992, 1996) (data not shown), 2+2 (Rogers et al., 1991b)
(data not shown), or 3+4 (Flores et al., 1992, 1996) subunits. In
addition, single-cell reverse transcription-PCR and immunocytochemical
analysis of retinoic acid-differentiated P19 cells revealed the
appearance of nAChR4 transcripts and immunoreactivity consistent
with the appearance and presence of nAChR4 RNA expression as well as
high-affinity nicotine binding sites (Cauley et al., 1996).
For this study, the pattern of immunohistochemical staining was
compared with the distribution of nAChR4 RNA measured by in
situ hybridization or with the distribution of high-affinity [3H]nicotine binding sites in the mouse brain
(Fig. 1). As noted above, nAChR4 has a
very distinct pattern of RNA expression relative to other closely
related subunits, and it has been demonstrated to be a key participant
in defining high-affinity [3H]nicotine or
[3H]cytisine binding sites (Anand et al., 1991;
Whiting et al., 1991; Flores et al., 1992, 1996). Consequently, the
immunohistochemical staining pattern should be in close agreement with
both these ligand binding studies and the RNA distribution (Fig. 1).
The immunostaining pattern of anti-nAChR4 displayed only a subset of
the corresponding patterns of nAChR2 RNA (Deneris et al., 1988;
Marks et al., 1992) or protein (Swanson et al., 1987; Hill et al.,
1993) (data not shown) distribution as well as only a subset of the
sites bound by [3H]epibatidine (Perry and Kellar,
1995; Marks et al., 1998). Immunoreactivity to nAChR4 is in poor
agreement with the distribution of 125I--bungarotoxin
binding sites (Clarke et al., 1985; Marks et al., 1985).
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Figure 1.
Anti-nAChR4 immunoreactivity
(middle) corresponds with nAChR4 RNA distribution
(left) and [3H]nicotine binding
(right). Mouse brains were prepared for in
situ hybridization or [3H]nicotine binding
as described previously (Marks et al., 1992). The coronal sections
shown are from three different animals shown at approximately the same
anatomical level. The arrowhead points to the medial
habenula as an example of a region in which there is excellent
agreement between all three methods. Other regions described in the
text include the amygdala (Ama), corpus callosum
(cc), cortex (Ctx), fasciculus
retroflexus (fr), hippocampus
(Hi), hypothalamus (Hy), and thalamus
(Th).
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Some discrepancies between these independent measures of nAChR4 were
noted, but they may reflect protein transport from the cell soma to
more distal nuclei. For example, in the striatum, both RNA (Marks et
al., 1992) and immunoreactivity are detected in the globus pallidus,
but the majority of [3H]nicotine binding is
present in the caudate putamen. This is similar to the interpeduncular
nucleus (IPN) where the in situ hybridization signal is
conspicuously less than the strong [3H]nicotine
binding (Marks et al., 1992). Anti-nAChR4 immunoreactivity was also
strong in this region (data not shown) but diffuse, consistent with
localization in process terminals and electrophysiological studies
(Lena et al., 1993). This is also supported by the strong anti-nAChR4 immunoreactivity found in the cell bodies of the medial
habenula and the processes in the habenular-IPN pathway that extend
via the fasciculus retroflexus (data not shown). In other regions (see
Fig. 1), the nuclei of the lateral hypothalamic region and the amygdala
contain RNA and anti-nAChR4 staining but little or no
[3H]nicotine binding. This may reflect the
sensitivity in detecting [3H]ligand binding or the
possibility that nAChR4 forms a receptor with other subunits that do
not favor high-affinity [3H]ligand binding.
However, given the likelihood of transport of nAChR4 protein, there
was overall agreement between these independent measures of nAChR4
expression.
Anti-4 immunoreactivity in the brain of young and aged
CBA/J mice
This study focuses on anti-nAChR4 immunostaining in five major
anatomically distinguishable regions of the mouse brain: the globus
pallidus, medial septum, diagonal band (also termed the triangular
septal region) (Marks et al., 1992), hippocampus (occasional neurons of
the stratum oriens, CA1, and the polymorphic region of the dentate
gyrus [PoDG] [see Franklin and Paxinos (1997) for definition]), and
the substantia nigra. These regions were selected because they are
anatomically well defined, they exhibit prominent anti-4
immunoreactivity in the soma of resident neurons, and changes in the
expression of cholinergic system markers such as acetylcholinesterase
or choline acetyltransferase have been reported to occur in some, but
not all, of these regions in the aging mammalian brain (Araujo et al.,
1988, 1990). Furthermore, diminished expression of
[3H]nicotine binding sites and response to
nicotine administration in the aged mammalian brain, particularly in
basal forebrain structures, are well established for both the human and
rodent brain (Whitehouse et al., 1986, 1988; Kellar et al., 1987, 1989;
Zhang et al., 1990; Shroder et al., 1991).
Typical results for young and aged animals of nAChR4
immunohistochemical localization in the regions examined are shown in Figure 2. In all cases, 25 µm sections
collected at 125 µm intervals from the brains of 13 young mice (3-5
months old; five males and eight females) or 15 aged mice (24-28
months old; seven males and eight females) were examined. Quantitative
analyses of staining are presented in Figure
3. Overall, there were no differences between the average number of immunopositive neurons detected in young
and aged CBA/J mice in the globus pallidus and the substantia nigra
(staining was dominant in the pars compacta but was present in
occasional cell bodies of the pars reticulata). A statistically significant decrease (p < 0.05) in the number
of immunopositive neurons was detected in the medial septum and
diagonal band in aged mice relative to young animals. These regions
were, however, notable for the considerable variability in the number
of stained neurons between individuals of the same age, and it was
common to find a twofold difference in the number of immunopositive
cells. This was particularly evident in the diagonal band of aged
animals, where staining ranged from the typical nearly undetectable
signal (Fig. 2) to one notable male animal that exhibited
immunostaining that was indistinguishable from young mice (data not
shown). This single aged animal suggests either that animals with
reduced staining in this region tended to be enriched in our aged
population or that some animals fail to exhibit diminished nAChR4
immunoreactivity with age. More animals or a systematic study of the
animal population during aging will be required to distinguish
unambiguously between these possibilities.
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Figure 2.
Comparison of anti-nAChR4 immunoreactivity in
five brain regions of young or aged CBA/J mice. Anti-nAChR4 antisera
reveal putative neuronal cell staining in representative brain sections
taken from a young (A-C, upper;
D, left) or aged (A-C,
lower; D, right) CBA/J
male mouse. The regions emphasized are the globus pallidus
(gp) in A; the hippocampus [CA1,
the polymorphic layer of the dentate gyrus, and the stratum oriens
(Or)] in B; the substantia nigra
[compacta (SNC) and reticulata (SNR)]
in C; and the medial septum (MS),
diagonal band (DB), and anterior commissure
(ac) in D.
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Figure 3.
Quantitative analysis of anti-nAChR4
immunoreactivity in young and aged CBA/J mice. The data from sections
such as those shown in Figure 2 were compiled from 13 young (3-5
months old; five males and eight females) or 15 aged (24-28 months
old; seven males and eight females) CBA/J mice as described in the
text. The results are grouped to show the mean immunopositive cell
number (± SEM) for each region by age and by sex (males, light
gray box; females, open box) and the average for
the group (dark gray box). Brackets
define t test pairs in which the results were
statistically significant (*p < 0.05 level;
**p < 0.01).
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Changes in anti-nAChR4 neuronal immunostaining in the
hippocampus were conspicuous between young and aged groups. As
shown in Figure 2 and with greater magnification in Figure
4, columns 1 and
2, immunoreactivity was restricted to a small number of neurons in CA1 that were mostly in association with the inner or outer
margin of the CA1 pyramidal cell layer, the dorsal margin of the
stratum oriens, and the PoDG. Stained neurons in the PoDG were greatly
diminished in the aged brain, as will be discussed in greater detail
below. The stained cells of CA1 occurred predominantly as solitary
neurons, but in certain sections they could be observed as evenly
spaced groups of three to six. In all young animals, these neurons were
distinguished by prominent processes that extended through the entire
stratum radiatum and the lacunosum molecular layer of the hippocampal
field (Fig. 4, column 1). These processes also exhibit
prominent and regularly spaced varicosities, giving them a
bead-on-a-string appearance (Fig. 4, column 1,
bottom row). Both processes and varicosities were
essentially absent from the hippocampus of all aged animals (Fig. 4,
compare columns 1 and 2, bottom
row). In the stratum oriens, a distinct population of neurons distinguished by prominent processes that extended laterally was present in young animals but absent in aged mice.
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Figure 4.
Anti-4 immunoreactivity in hippocampal sections
from representative young and aged male CBA/J mice that were grouped
according to receiving no nicotine (control) or nicotine in their water
for 6 weeks (short-term) or 11 months (long-term). As described in
Materials and Methods, three male CBA/J mice were given nicotine and
saccharin in their water for 6 weeks (24 months old at start of
treatment) or 11 months (14 months old at start of treatment). Controls
received water with saccharin but without nicotine. In the top
row is a representative section from the dentate gyrus of each
group exhibiting the immunoreactivity of neurons to anti-nAChR4
antibodies. The arrow (left) points to a
stained neuron in the polymorphic layer. Other labels show the granule
cells (GC) of the dentate gyrus and neurons of the CA3.
In the middle row is shown the hippocampal CA1 region
for each group. The asterisks note an
anti-nAChR4-immunopositive cell in each treatment group. The
pyramidal cell layer (PyC) and the Or are
noted. The bottom row shows at high magnification the
immunopositive processes that extend ventrally from stained cells of
the CA1 (middle row). These cells exhibit extensive
dendritic-like processes that exhibit regular varicosities on greater
magnification (arrowheads). A typical young animal (3 months) is shown on the left; a typical older animal (25 months) is shown on the right. These cells are less
abundant, and the large processes exhibiting varicosities are
diminished or entirely absent in the older animals except in the aged
group that was supplied with nicotine in their water for 11 months.
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Comparison of males and females within the young or aged groups
revealed one statistically significant difference. In the CA1 region of
the hippocampus, the number of immunopositive neurons was significantly
greater (p < 0.01) in young males relative to young females (Fig. 3). This difference was restricted to the CA1
region, and it was not observed in the stratum oriens or PoDG (data not
shown). This sex-related difference did not occur in the aged animal
group. Although other regions did not exhibit a sex-related difference
in expression, the loss of nAChR4-immunopositive neurons found in
aged animals was driven predominantly by the strong loss of
immunopositive cells in males as shown in Figure 3. This was observed
for the medial septum and the diagonal band, where the decrease in
immunoreactivity was greatest between young and aged males, but the
decline in immunopositive cells between young and aged females was not
statistically different. Although both sexes exhibited a substantial
decrease in hippocampal nAChR4-expressing neurons in aged animals
(Fig. 3), this decline was approximately fourfold in males compared
with a less than twofold decrease in females.
Long-term, but not short-term, nicotine administration
alters age-related changes in nAChR4 immunoreactivity in the
hippocampus
The administration of nicotine to rodents results in the well
established increased in expression of high-affinity
[3H]nicotine binding sites in the brain (Marks et
al., 1985, 1991, 1992; Kellar et al., 1989; Flores et al., 1992).
Because of the dramatic age-related decrease in the expression of
anti-nAChR4-immunopositive cells in the hippocampus, we tested the
possibility that the oral administration of nicotine to age- and
sex-matched CBA/J mice would modify nAChR4 neuronal expression in
aged mice. This was tested in male mice because of the pronounced
difference observed in staining between young animals relative to aged
ones (Fig. 3). The experimental groups were as follows. First,
24-month-old CBA/J male mice were divided into two groups of three
animals each, and one group was administered nicotine in their water
for a period of 6 weeks (short-term); the other group received no nicotine. Second, another group consisted of 14-month-old CBA/J male
mice that were placed on either water with saccharin or water with
saccharin and nicotine for a period of 11 months (long-term, see
Materials and Methods). As shown in Figures 4, column
3, and 5, aged mice
administered nicotine for 6 weeks exhibited no change in
anti-nAChR4-immunopositive cells relative to aged mice controls that
did not receive nicotine. In contrast, 14-month-old CBA/J mice given
nicotine orally for 11 months exhibited notable differences in
anti-nAChR4 immunoreactivity relative to controls (Fig. 5). Immunopositive neurons of the PoDG region were retained when compared with aged controls not receiving nicotine, and the number of
immunopositive cells did not differ significantly from that in young
animals (Figs. 4, 5). Conversely, there was an almost complete loss of immunopositive cell staining in the stratum oriens and in the CA1
region, where the number of labeled cells diminished similarly to that
in aged animals not given nicotine or those aged animals that received
nicotine for 6 weeks (Figs. 4, column 4, middle row, 5). Despite the loss of neuronal staining in CA1, there
was a notable difference between the subcellular distribution of
anti-nAChR4 immunoreactivity in long-term nicotine-treated animals
relative to controls. As seen in Figure 4, column 4,
bottom row, the presence of long dendritic-like
processes complete with varicosities seen in young animals was retained
in the adult mice receiving 11 month nicotine administration. Similar
immunoreactivity in the processes originating from neurons of the CA1
in aged animals given nicotine for only 6 weeks was absent (Fig. 4,
column 3, middle row). Notably, the
neurons and their processes that exhibit these varicosities resemble
closely the neurons in the hippocampus identified by Alkondon et al.
(1997) to express to nAChR42-type receptors and regulate GABA
release. The examination of the globus pallidus and substantia nigra
from both of these groups exhibited no quantitative difference in
immunopositive cells compared with that in aged-matched controls or in
young animals (data not shown).
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Figure 5.
Quantitative analysis of anti-nAChR4
immunoreactivity between young and aged CBA/J mice given nicotine in
their water for 6 weeks or 11 months. The number of neurons stained for
nAChR4 immunoreactivity in the designated region was obtained from
sections such as those shown in Figure 4 and was compiled from three
mice in each group as described in the text. Error bars reflect the
mean number (± SEM) of immunopositive cells in each region counted
from at least eight sections for each animal. A, Stained
neurons in the polymorphic area of the dentate gyrus from 25-month-old
mice that were supplied nicotine for 11 months (chronic) versus aged
mice (24-27 months old) either not given nicotine or administered
nicotine for only 6 weeks (acute) were counted. The double
asterisks denote a significant difference
(p < 0.01). B, The number of
immunopositive neurons observed in the CA1 region of each group was
similarly scored. A significant decrease in the number of stained
neurons in all aged groups relative to young animals
(p < 0.01) was observed in this region of
the hippocampus (see text).
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DISCUSSION |
The expression of nAChR4 immunoreactivity in the brain of young
and aged CBA/J mice was examined, and it was determined whether short-
or long-term nicotine administration alters patterns of expression.
Rabbit polyclonal antiserum with specificity to nAChR4 revealed a
pattern of immunostaining that closely resembles that of RNA expression
for this subunit and of high-affinity [3H]nicotine
binding. We selected the CBA/J mouse because of both availability and
the observation in preliminary studies that this strain had
particularly robust neuronal staining for this subunit. Other strains,
including DBA/2 or C57Bl/6, exhibited relatively poor immunoreactivity
to nAChR4 (data not shown). The well documented difference between
strains (e.g., Marks et al., 1991) with respect to high-affinity
[3H]nicotine binding and sensitivity in behavioral
tests to nicotine (Marks et al., 1991) suggests that considerable
variation in anti-nAChR4 immunoreactivity could be expected, but
this remains to be thoroughly examined. If true, however, strain
selection for studying the influence of aging on nicotinic receptors
will be critical. In the CBA/J mice selected for this study,
anti-nAChR4 immunoreactivity was localized to both putative axonal
and dendritic processes of discrete neuronal populations.
Anti-nAChR4 immunoreactivity was diminished in aged animals in many,
but not all, regions of the brain. Specifically, the loss of
immunoreactivity was notable in the medial septum and diagonal band,
and it was dramatic in the hippocampus.
When aged male CBA/J mice were given nicotine in their water for 6 weeks, the loss of immunoreactivity was not reversed. In contrast,
administration of nicotine to adult mice for at least 11 months seemed
to preserve neuronal staining in the polymorphic layer of the dentate
gyrus but not in the hippocampal CA1 region. Nevertheless, neurons of
the CA1 region that exhibited immunoreactivity also retained strong
staining of their processes that was not observed in any other aged
animal group. This result suggests that long-term nicotine
administration may have very specific and highly selective regional
effects on various neuronal populations. Furthermore, this result
suggests that these effects may not be manifested via simple mechanisms
of receptor upregulation, because this occurs in mice within 10 d
of oral nicotine delivery (Collins et al., 1996; Booker and Collins,
1997) (data not shown). An interesting possibility is that long-term
administration may enhance or alter synaptic connectivity, resulting in
the retention of immunopositive neurons.
Despite the evidence of nAChR decline in aging and perhaps in more
severe diseases of neurodegeneration, it remains controversial as to
how this excitatory system could exert its effect on the brain. One
likely possibility is that nAChRs exert the majority of their effect
presynaptically, possibly via modulation of release of
neurotransmitters such as dopamine or GABA (Grady et al., 1992; Lena et
al., 1993; McGhee et al., 1995; Bertolino et al., 1997; Wonnacott,
1997). Consequently, the hypothesis has been advanced that relatively
small numbers of nAChRs placed at key regulatory synapses could be
crucial in regulating or modulating the concentration of
neurotransmitter during synaptic activation. Our antibodies can address
this issue only indirectly because they were prepared to a cytoplasmic
domain of nAChR4 and consequently they do not necessarily
discriminate between mature and assembling receptors. In general, axons
are difficult to identify without double labeling, but the staining of
processes in some white-matter tracts [e.g., the anterior commissure
(see Fig. 2) and the fasciculus retroflexus (data not shown)] in young
animals is consistent with substantial axonal transport and presynaptic
localization. This staining was diminished or absent in aged animals
(see Fig. 2; data not shown). The immunostaining of the prominent
processes extending from cells of the hippocampal CA1 region and the
presence of varicosities in young animals suggest a more somal and
dendritic localization in these cells. In any case, the prominence of
nAChR4 immunoreactivity in neurons and their location (e.g.,
thalamus, neostriatal pathway, and the cells of the PoDG) are
consistent with the location and shape of cells generally described as
dopaminergic neurons or inhibitory interneurons. The similarity of
morphology between these neurons with GAD-staining neurons (data not
shown) and the recently described GABA-responsive neurons in the
hippocampus using electrophysiology and dye-fill experiments (Aarne et
al., 1994; Geula and Mesulam, 1994; Alkondon et al., 1997; Bertolino et
al., 1997) also suggests that these cells could be inhibitory. In any
case, their relatively infrequent but regular distribution suggests
that these neurons could play an important role in regulating excitation in the hippocampus, particularly via modulation of GABA
release (Alkondon et al., 1997), and their loss could seriously alter
this balance of local synaptic transmission. Consequently, the region-
and cell-specific loss of nAChR4 immunoreactivity during aging could
have profound effects on retaining the critical balance between
excitation and inhibition in key brain regions that are subject to
failure and neurodegeneration with age. The retention of these neurons
in a nondysfunctional state, which seems to be the effect of long-term
nicotine application, would likely slow the onset of such
processes.
Despite the significant limits of using the aging-mouse model to
understand age-related neurodegenerative diseases in humans, these
results may provide some insight into the mechanisms through which
chronic nicotine administration by smoking might lead to the slowing of
the onset of Parkinson's disease or senile dementia of the
Alzheimer's type (vanDuijn and Hofman, 1991; vanDuijn et al., 1991;
Morens et al., 1994; Nicholson, 1994). In particular, whether the
neurons that express these markers die or whether they become
dysfunctional in their expression with age remains a question to be
resolved. In humans, the depletion of ChAT via neuronal loss in the
basal forebrain seems to be a contributor to Alzheimer's disease
(Geula and Mesulam, 1994), but in the cortex this loss is greater than
can be accounted for by neuronal loss (Geula and Mesulam, 1994). In
this study, both in the hippocampus (where the most dramatic changes in
nAChR4-immunopositive cells were observed) and in the diagonal band
(data not shown), the administration of nicotine to aged animals was in
general not effective in recovering or deterring the loss of stained
neurons except in the polymorphic layer of the dentate gyrus.
Nevertheless, there was a dramatic retention of immunopositive
processes complete with varicosities in the immunopositive neurons that
remained that were not present in the other aged-mouse groups. However, this retention of expression required nicotine administration for ~11
months of a 25 month life span of these mice and was initiated before
nAChR4 expression decline. Consequently, these data support the
notion that nicotine exerts a positive influence in the aged animal via
promoting the retention of neuronal connections that are normally lost
during normal aging but does so only if supplied in advance for a
prolonged period before the onset of age-related cholinergic neuronal
decline.
| |
FOOTNOTES |
Received Feb. 2, 1998; revised April 6, 1998; accepted April 13, 1998.
These studies were supported by Veterans Administration Merit funding
to S.W.R. and L.C.G. and by National Institutes of Health Grants
AG04418 and DA03194 and Research Scientist Award DA00197 to A.C.C. We
gratefully note the outstanding technical assistance of Rachael Kulmer
and Robert Simmons.
Correspondence should be addressed to Dr. Scott W. Rogers, Building
533, Room 2410, University of Utah, Salt Lake City, UT 84112.
| |
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Abstract
Introduction
