 |
Next Article 
The Journal of Neuroscience, March 1, 1999, 19(5):1541-1556
Integrin Subunit Gene Expression Is Regionally Differentiated in
Adult Brain
Jason K.
Pinkstaff1,
Jon
Detterich1,
Gary
Lynch2, 3, and
Christine
Gall1
Departments of 1 Anatomy and Neurobiology,
2 Psychiatry and Human Behavior, and the
3 Center for the Neurobiology of Learning and Memory,
University of California at Irvine, Irvine, California 92697-1275
 |
ABSTRACT |
Integrins are a diverse family of heterodimeric (  ) adhesion
receptors recently shown to be concentrated within synapses and
involved in the consolidation of long-term potentiation. Whether neuronal types or anatomical systems in the adult rat brain are coded
by integrin type was studied in the present experiments by mapping the
relative densities of mRNAs for nine and four subunits.
Expression patterns were markedly different and in some regions
complementary. General results and areas of notable labeling were as
follows: 1 limited neuronal expression, neocortical layer V,
hippocampal CA3; 3 and 5diffuse neuronal and glial labeling,
Purkinje cells, hippocampal stratum pyramidale, locus coeruleus (3);
4 discrete limbic regions, olfactory cortical layer II,
hippocampal CA2; 6most prominently neuronal, neocortical subplate,
endopiriform, subiculum; 7discrete, all neocortical layers,
hippocampal granule cells and CA3, cerebellar granule and Purkinje
cells, all efferent cranial nerve nuclei; 8discrete neuronal, deep
cortex, hippocampal CA1, basolateral amygdala, striatum; Vall
cortical layers, striatum, Purkinje cells; 4dentate gyrus granule
cells; 5broadly distributed, neocortex, medial amygdala,
cerebellar granule and Purkinje cells, efferent cranial nerve nuclei;
2, 2, and 3mRNAs not detected. These results establish that
brain subfields express different balances of integrin subunits and
thus different integrin receptors. Such variations will determine which
matrix proteins are recognized by neurons and the types of
intraneuronal signaling generated by matrix binding. They also
could generate important differences in synaptic plasticity across
brain systems.
Key words:
adhesion molecules; extracellular matrix; hippocampus; cortex; brainstem; in situ hybridization
| |
INTRODUCTION |
Integrins are membrane-spanning,
noncovalently bound heterodimers that act as cell-matrix and
cell-cell adhesion receptors throughout the body (Hynes, 1992 ). They
also activate intracellular signaling cascades, including tyrosine,
serine/threonine, and mitogen-activated protein kinase activities
associated with neurotrophic factors and cytokines (Clark and Brugge,
1995). A large body of work indicates that the integrins exert potent
influences over a diverse array of cellular functions, including
proliferation, differentiation, process outgrowth, gene expression, and
survival (Damsky and Werb, 1992; Yamada and Miyamoto, 1995; Giancotti, 1996; Katz and Yamada, 1997). Cell migration, axon guidance, and synapse formation in the developing nervous system are likely examples
of integrin-dependent operations (Dodd and Jessell, 1988; Sanes, 1989;
Reichardt and Tomaselli, 1991; Kil et al., 1996). Modifying synapses in
the adult brain may be another. Specifically, hippocampal slice
experiments have shown that peptides that block ligand binding by a
major subclass of integrins prevent the stabilization of long-term
potentiation (LTP) and the formation of in vitro kindling
while having no detectable effects on baseline physiology (Staubli et
al., 1990; Xiao et al., 1991; Grooms and Jones, 1997). LTP can be
partially disrupted by integrin antagonists several minutes
after its induction (Bahr et al., 1997; Staubli et al., 1998), as expected from the hypothesis that stabilization involves the
activation and engagement (matrix binding, attachment to cytoskeleton) of latent integrins. Memory consolidation across many paradigms has a
similar time course, but there are as yet no tests for integrin involvement in this phenomenon. However, Drosophila with a
mutation in a synapse-associated integrin subunit
(vol) have retention deficits that are alleviated by
vol transgene expression (Grotewiel et al., 1998).
Sixteen and eight subunits have been identified (Aplin, 1998),
which form a large number of heterodimeric receptor combinations. As a
consequence of differences in subunit composition, integrin receptors
differ in the specific matrix proteins they recognize (e.g., laminins,
collagens, vitronectin, etc.) and the intracellular cascades they
initiate (Hynes, 1992; Clark and Brugge, 1995; Jewell et al., 1995;
Ruoslahti, 1996; Katz and Yamada, 1997; Gong et al., 1998) and, in some
instances, can have opposing effects on gene expression (Huhtala et
al., 1995). Whether regions or neuron classes in adult brain are coded
by integrin type has not been studied. Biochemical experiments indicate
that synaptic fractions are greatly enriched in integrin receptors
(Bahr and Lynch, 1992; Capaldi et al., 1997; Nishimura et al., 1998),
whereas immunoelectron microscopy has identified two subunits (8,
8) concentrated in postsynaptic densities (Einheber et al., 1996;
Nishimura et al., 1998). Regional differences in levels of 8 and
8 immunoreactivities (Einheber et al., 1996; Nishimura et al., 1998)
and 1 mRNA (Pinkstaff et al., 1998) have been described, but there
are no data addressing the possibilities of regional patterns
associated with particular integrin classes or regional differences in
-subunit gene expression in brain. Given the diversity of integrin
effects, regional differences in receptor expression could be involved
in a wide range of neuronal specializations, including variants of
activity-dependent synaptic plasticity (Maren and Baudry, 1995). To
examine these possibilities, the studies reported here used in
situ hybridization to map the regional and cellular localization
of gene expression for nine and four integrin subunits in adult
rat brain.
| |
MATERIALS AND METHODS |
In situ hybridization. Adult male Sprague Dawley
rats (250-350 gm; Simonsen labs, Gilmore, CA) were used for all
procedures. For in situ hybridization analyses the rats
(n = 8) were killed with an overdose of sodium
pentobarbital (100 mg/kg) and perfused transcardially with 4%
paraformaldehyde in 0.1 M phosphate buffer (PPB). The
brains were post-fixed for 24-48 hr in PPB, cryoprotected in PPB/20%
sucrose for 24-36 hr, and sectioned on a freezing microtome (coronal,
25 µm) into cold PPB. Spaced series of tissue sections were processed
free-floating for in situ hybridization, as described in
detail elsewhere (Guthrie et al., 1995). This entailed hybridization with 35S-labeled antisense riboprobes (1 × 107 cpm/ml) at 60°C for 36-48 hr in buffer
containing 50% deionized formamide, 35× Denhardt's reagent (0.7%
polyvinylpyrrolidone, 0.7% bovine serum albumin, and 0.7% Ficoll),
and 0.14× SSC (1× SSC = 0.15 M NaCl/0.015
M sodium citrate). After hybridization the tissue was
treated with RNase A and washed through increasingly dilute SSC
solutions to a final wash in 0.1× SSC at 60°C. Then the tissue was
mounted onto gelatin-coated slides, air-dried, processed for film
(Amersham -Max, Arlington Heights, IL) and then emulsion (Kodak
NTB-2, Rochester, NY) autoradiography, stained with cresyl violet or
hematoxylin, and coverslipped with Permount (Fisher Scientific, Fair
Lawn, NJ). As a control for specificity, alternate sections were
processed (as above) for hybridization with 35S-labeled
sense transcripts transcribed from each of the cDNA templates used to
generate the antisense probes. No regional or cellular labeling was
obtained with sense probe hybridizations. The amino acid sequences for
the integrins are from ~30% (4 vs others) to 60% (3,
5, 6, and 1, 2) identical (Moyle et al., 1991), whereas the
integrins are more divergent with <30% (2, 4 vs others) to
<50% (all comparisons) identity (Hynes, 1992). Nevertheless, the
subunit specificity of hybridization was demonstrated by the fact that
the integrin subunit cRNAs used here yielded labeling patterns that
differed from each other in both positive and negative directions.
Moreover, all labeling patterns differed from those obtained with a
variety of other cRNAs, including those for integrin 1,
brain-derived neurotrophic factor, basic fibroblast growth factor, and
AMPA receptor subunit transcripts (data not shown).
To evaluate the potential colocalization of integrin 7 and 1
mRNAs, we processed sections through cerebellum and lower
brainstem for simultaneous in situ hybridization with
digoxigenin-labeled 7 cRNA and 35S-labeled 1 cRNA.
Labeling was localized by using anti-digoxigenin immunohistochemistry
with alkaline phosphatase as chromagen (DIG-Nucleic Acid Detection Kit;
Boehringer Mannheim, Indianapolis, IN) for 7 cRNA labeling and
Ilford K5.D emulsion (Polysciences, Warrington, PA) autoradiography for
1 cRNA labeling, as described in full detail elsewhere (Bizon et
al., 1995).
The distribution of hybridization of each cRNA probe was evaluated by
microscopic examination of the emulsion autoradiograms by two
investigators working independently; all labeling patterns that were
reported were verified by both investigators for at least three brains.
Regions were identified with reference to the atlases of Paxinos and
Watson (1986) and Swanson (1992).
Riboprobes. The radiolabeled cRNA probes were prepared by
transcription from linearized cDNA templates in the presence of 35S-UTP for in situ hybridization or
32P-CTP for RNA blots. Table
1 summarizes the information on plasmids and resultant cRNAs excepting those for 3 and V (see below). Restriction enzymes and polymerases were obtained from Boehringer Mannheim and Stratagene (La Jolla, CA), respectively.
The cDNAs for 3 and V were created by using the reverse
transcriptase PCR (RT-PCR). First-strand cDNA synthesis
consisted of reverse transcription of 1 µg of hippocampal total RNA,
using Maloney murine leukemia virus (MMLV) reverse transcriptase
(Promega, Madison, WI) and random primers. The complementary DNA was
amplified with 100 pmol of the appropriate primers and TAQ polymerase
(Promega). For 3, the primers 5'CACGGGTGTGGAACAGCAC3' and
5'-CAGTGCTTCTTGGTGGGTAG-3' corresponding to bases 62-578 of the mouse
3 mRNA sequence (Tamura et al., 1991) were used. The primers for
V were 5'-AAGGCGCAGAATCAAGGAG-3' and 5'-TAAGGCCACTGGAGGTTCAG-3',
corresponding to bases 76-592 of the rat V mRNA sequence (Shinar et
al., 1993). For both cDNAs the PCR consisted of 35 cycles at 94, 60, and 72°C for denaturing, annealing, and elongation steps,
respectively. After this PCR amplification the reaction products were
purified by the Boehringer Mannheim PCR Purification Kit and ligated
into PGEM-T vector (Promega). Clones were verified by dideoxynucleotide
sequencing (Sequenase 2.0, United States Biochemical, Cleveland, OH).
RNA blot analysis. Northern blot hybridizations were
conducted to verify that cRNAs for 1-8 and V and 2-5
detected transcripts corresponding to the predicted sizes of the target
subunit mRNAs. Untreated adult male rats (n = 2) were
anesthetized with isoflurane and decapitated; their brains were removed
for subfield dissections. Total RNA was extracted by homogenization in
Trizol reagent (Pharmacia, Piscataway, NJ), quantified by UV
spectrophotometry, and processed by RNA blotting techniques as
previously described (Pinkstaff et al., 1998). Each of the cRNAs
hybridized with mRNAs of the predicted size from total RNA extracts of
hippocampus or cortex, with the exception of transcripts for 2,
3, and 4, which were not detected in hippocampus or cortex of
control brains.
| |
RESULTS |
As summarized in Tables 2 and
3, in situ hybridization
analyses demonstrated highly region-specific patterns of integrin subunit mRNA expression in adult rat brain. Because the distributions and character of labeling differed dramatically across probes, the
descriptions that follow will focus on the cRNAs separately, with the
exception of 2, 2, and 3. Although each of these cRNAs detects
transcripts in non-neuronal systems (Wilson et al., 1989; Chiba et al.,
1996; Wu and Santoro, 1996) and, for 2 and 3 in experimental
brain tissue (J. Pinkstaff and C. Gall, unpublished observations), they
did not yield detectable in situ hybridization labeling in
tissue sections from untreated adult rat brain. For the remaining cRNAs
the distributions of hybridization are described for tissue sections
from the most rostral levels of frontal cortex through lower brainstem
or high cervical spinal cord. Autoradiographic exposure times varied
across probes to best visualize the distributions of abundant (e.g.,
7 mRNA) and rarer transcripts; as a consequence of this and of
differences in cRNA lengths, comments on the relative densities of
labeling between brain areas pertain to the cRNA at hand and are not
intended to connote differences in the abundance of the different
transcripts.
1 mRNA
Like many of the transcripts that were evaluated, the 1 cRNA
generated low-density and faintly patchy labeling throughout gray and
white matter, giving the impression of low expression levels by glial
cells. In addition, as summarized in Tables 2 and 3, integrin 1 mRNA
was highly expressed in a few discrete regions distributed across the
neuraxis; in these regions the hybridization appeared to be localized
to neurons on the basis of the sizes and cytoarchitectonic
distributions of labeled cells. In rostral telencephalon the labeling
was limited to a few cells in deep orbital frontal cortex and
intermediate layers of medial allocortex. Labeling in the latter
field continued caudally through prelimbic, cingulate, and
retrosplenial cortex. At the level of the hippocampal commissure a
second population of well labeled cortical cells was evident within the
suprarhinal region, and at progressively more caudal planes the
population extended dorsal from the rhinal fissure to encompass the
medial-to-ventral arc of neocortex fully (Fig.
1C). As shown in Figure 1,
D and E, these large, heavily labeled cells were
distributed within a superficial sublamina of layer 5.
View larger version (88K):
[in this window]
[in a new window]
|
Figure 1.
Integrin 1 mRNA is expressed by a few discrete
neuronal groups. Photomicrographs show the autoradiographic
localization of integrin 1 cRNA labeling in coronal tissue sections.
A, C, Sections through rostral
(A) and caudal (C)
hippocampus show dense labeling in CA3a and CA3b stratum pyramidale
(arrowhead in A) and the absence of
hybridization in stratum granulosum (sg) and CA1 stratum
pyramidale (CA1). C also shows the
labeling of a discrete intermediate layer of neocortical cells
(thin arrows), cortical blood vessels
(arrowhead), and the pia mater. D,
E, Higher magnification photomicrographs show the same
field of primary visual neocortex with dark-field
(D) and bright-field (E)
illumination (hematoxylin counterstain); in comparing these panels one
can see that the labeled cells (D) are
distributed within the more superficial aspect of cortical layer 5 (E). (Small arrows indicate the
same labeled cell in D and E; the
position of cortical layer 4 is shown in E.)
B, F, Sections through hypothalamus
(B) and lower brainstem (F)
show labeling within the paraventricular hypothalamic nucleus
(pvn) and area postrema (ap).
Scale bar (shown in F): A, 625 µm; B, D, E, 500 µm;
C, 1 mm; F, 720 µm.
|
|
A few neuronal groups in the limbic telencephalon (Table 2) also
expressed 1 mRNA. There was dense labeling of hippocampal CA3b and
CA3a stratum pyramidale (Fig. 1A,C) and light
labeling of cells in the bed nucleus of stria terminalis extending into the amygdala, the amygdalohippocampal transition area, and the horizontal limb of the diagonal bands of Broca/magnocellular
preoptic area (data not shown). In diencephalon the cRNA labeled
cells in the reticular and anteroventral ventrolateral thalamic
nuclei, the paraventricular (Fig. 1B), supraoptic,
and arcuate hypothalamic nuclei, and the median eminence at
moderate-to-low levels. There was little regionally differentiated
hybridization at lower levels of the neuraxis (Table 3), with lightly
labeled cells detected in the substantia nigra/ventral tegmental area,
the superior olivary complex, the trigeminal mesencephalic nucleus, and
the hypoglossal nucleus. Finally, labeling was distributed within the
circumventricular organs (i.e., area postrema and the subfornical
organ; Fig. 1F) and associated with blood vessels and
the pia mater (Fig. 1C,D).
3 mRNA
As illustrated in Figure 2, 3
mRNA was distributed broadly with both low-density labeling throughout
the neuropil in regions of gray and white matter (see hippocampal
molecular layers, Fig. 2A) and broadly distributed,
but nevertheless selective, labeling of neuronal groups. As shown in
Figure 2B, labeling was associated nonpreferentially
with neuronal fields in neocortex, olfactory cortex, claustrum, and the
endopiriform nuclei. Labeling extended from superficial olfactory
cortex into layer 2 of olfactory tubercle (Fig. 2B);
at these same planes the islands of Calleja and the tenia tecta were
not labeled. Labeling was light to moderately dense in corticomedial
and basolateral amygdala and less dense in the central and lateral
nuclear groups. Hybridization was relatively dense in cholinergic basal
forebrain regions, including the medial septal nucleus, the diagonal
bands of Broca (Fig. 2C), and nucleus basalis (data not
shown), and in association with a few scattered cells in the more
ventral caudate putamen, but it was low throughout the majority of
caudate putamen and lateral septum (Fig. 2B,C). Within the hippocampal formation, cells in the hilus and stratum pyramidale were labeled moderately densely (Fig. 2A).
In stratum pyramidale the labeling densities declined around the curve
of the cell layer from CA3c to CA1 and along the temporal-to-septal axis. Stratum granulosum was not labeled (Fig.
2A).
View larger version (155K):
[in this window]
[in a new window]
|
Figure 2.
Integrin 3 mRNA is broadly distributed.
Dark-field photomicrographs show the autoradiographic localization of
3 cRNA labeling in select brain regions. A, Rostral
hippocampal section showing that labeling is distributed within the
pyramidal cell layer (CA3, CA1), but not
within stratum granulosum (sg). B,
Rostral forebrain section shows that labeling is broadly distributed
within neocortex (asterisk), moderately dense within
superficial piriform cortex (arrow) and olfactory
tubercle (ot), but low within caudate putamen
(CPu). C, Within the septal region,
hybridization is moderately dense in the medial septal nucleus
(ms) and the diagonal bands of Broca (db)
but is at low neuropil levels within lateral septum
(ls). D, Section through hypothalamus
showing relatively dense labeling in the paraventricular
(pvn) and supraoptic (so) nuclei
(opt, optic tract). E, Photomicrograph
showing dense labeling of the cerebellar Purkinje cells
(arrow) (gc, granule cell layer;
wm, deep cerebellar white matter). F,
Section showing dense hybridization in the locus coeruleus
(lc) and in association with the large neurons of the
motor trigeminal nucleus (5Mo). G,
H, Sections through lower brainstem showing labeling
within the dorsal motor nucleus of the vagus (G;
Xdm), area postrema (G;
ap), and nucleus ambiguus (H; arrow).
Scale bar (shown in H): A, 400 µm; B, 1.2 mm; C, H, 900 µm; D, 320 µm; E, F,
250 µm; G, 450 µm.
|
|
In diencephalon the labeling was greatest in the magnocellular
hypothalamic nuclei (i.e., paraventricular, supraoptic; Fig. 2D) and was moderately dense in the anterodorsal,
midline, intralaminar, and medial geniculate thalamic nuclei, in the
subthalamic nucleus, and in association with scattered cells in the
lateral hypothalamus. Labeling was low in the ventral and lateral
thalamic nuclei. Within mesencephalon, cells in the substantia
nigra/ventral tegmental area and medial aspects of the oculomotor
nuclear complex were labeled the most densely.
At more caudal levels there was a scattering of densely labeled cells,
including neurons in the reticular formation, superior olivary complex,
motor trigeminal nucleus (Fig. 2F), dorsal motor nucleus of the vagus (Fig. 2G), nucleus ambiguus (Fig.
2H), and ventral medullary reticular nucleus.
Although cells were labeled in other cranial nerve nuclei (e.g.,
abducens, facial motor, and hypoglossal), these regions were not
labeled as densely or completely as those seen with other -integrin
cRNAs (e.g., 7, vida infra). In contrast, as shown in Figure
2F, the locus coeruleus was labeled very densely with
3 cRNA; this was the only integrin prominently expressed by this
noradrenergic cell group. In cerebellum the Purkinje cells were well
labeled, but the granule cell layer was not (Fig.
2E); indeed, the granule cell layer was labeled less densely than the underlying cerebellar white matter. Finally, there was
labeling in the subfornical organ and area postrema (Fig.
2G), but not in association with blood vessels, the
ventricular ependyma, or the pia mater.
4 mRNA
Of the various transcripts, 4 mRNA was distributed the most
narrowly, being limited almost entirely to discrete regions of the
limbic telencephalon. Hybridization was greatest in rostral planes,
with dense labeling of the tenia tecta (Fig.
3A,E) and moderate labeling of
rostral piriform cortex (Fig. 3A). Labeling continued
caudally through piriform (Fig. 3C) and entorhinal (Fig. 3B,D) cortex. In the hippocampal formation the labeling was
not dense but was greatest in region CA2 stratum pyramidale (Fig. 3D, arrowhead), the fasciola cinerium, and
stratum granulosum and was quite light in CA3 stratum pyramidale.
Hybridization densities increased along a septotemporal gradient in
both CA3 and stratum granulosum (Fig. 3B,D). CA1 stratum
pyramidale did not appear to be labeled although there was low-density
hybridization in the temporal subiculum (Fig. 3B, arrow)
and, as seen in the same sections, the posterior corticomedial amygdala
(Fig. 3B). Finally, at caudal levels only, labeling extended
from layers 2/3 of olfactory cortex and into the superficial neuronal
layers of neocortex; this neocortical labeling was sparse and
dissipated with distance from the rhinal fissure (Fig. 3D,
arrow). With the exception of sparse labeling lateral to the third
ventricle, further hybridization was not detected in diencephalon,
mesencephalon, cerebellum, or lower brainstem (Table 3). In distinction
with most other -integrin cRNAs, patchy labeling of the neuropil, as
might signify expression by glial cells, was not in evidence.
View larger version (145K):
[in this window]
[in a new window]
|
Figure 3.
4 mRNA is distributed discretely in
limbic forebrain. A, Section through the rostral
olfactory peduncle showing hybridization in tenia tecta
(tt) and rostral piriform cortex
(pc) (ac, anterior commissure).
B, Section through temporal hippocampal formation
showing labeling in the entorhinal cortex (ec),
posterior corticomedial amygdala (pomc), temporal
stratum granulosum (sg), CA3c (asterisk),
and subiculum (small arrow); the broad
arrow indicates the rhinal fissure. C,
Low-magnification photomicrograph showing exclusive labeling of the
piriform cortex (pc) in a section through the
level of the septum (s) and caudate putamen
(CPu). D, Section through the midcaudal
hippocampal formation shows prominent labeling of CA2 stratum
pyramidale (arrowhead) and entorhinal cortex
(ec) as well as faint labeling in superficial layers of
temporal cortex (thin arrow). In a comparison of
D and B one can see evidence for the
increasing septotemporal labeling gradient within stratum granulosum
(sg), with just faint labeling in the mid/dorsal dentate
gyrus (D) as compared with greater labeling in
the temporal field (B). E, Section
through rostral septum shows dense labeling of tenia tecta
(tt) (cc, corpus callosum). Scale bar
(shown in A): A, E, 500 µm; B, 720 µm; C, 1.6 mm;
D, 1 mm.
|
|
5 mRNA
Like 3 cRNA, the 5 cRNA generated low-density, diffuse
labeling throughout gray and white matter. In addition, variable density labeling was associated with neuronal cytoarchitectonics. As
exemplified by the section through the olfactory peduncle shown in
Figure 4A, labeling was
distributed evenly through the neuronal layers of the anterior
olfactory nucleus and tenia tecta. Labeling similarly was distributed
broadly in neuronal fields of neocortex and amygdala (data not shown)
and in the major neuronal cell layers of the hippocampal formation
(Fig. 4C). Just a few areas stood out as being more densely
labeled. In forebrain the most densely labeled cells were distributed
above the deep white matter of medial allocortex and neocortex (Fig.
4B); these cells scattered more broadly away from the
white matter in lateral, as compared with dorsal, fields and did not
extend all the way down to the rhinal fissure. In addition, labeling
was denser in hippocampal stratum pyramidale than in stratum granulosum
and was denser in the horizontal limb of the diagonal
bands/magnocellular preoptic area and the paratenial thalamic nuclei
than in surrounding fields. Low-density labeling was distributed
broadly to neuronal fields in midbrain and lower brainstem but was
conspicuously laminated in cerebellum. As shown in Figure
4D, the Purkinje cells were well labeled, and 5
cRNA labeling was lower in the internal granule cell layer than in
either the cerebellar molecular layer or the deep white matter.
View larger version (74K):
[in this window]
[in a new window]
|
Figure 4.
Relatively low-density 5 cRNA labeling is
distributed across most neuronal fields. Dark-field photomicrographs
show 5 cRNA labeling in (A) olfactory peduncle
(tt, tenia tecta; aon, anterior olfactory
nucleus), (B) deep neocortex (cc,
corpus callosum; CPu, caudate putamen),
(C) rostral hippocampus (sg,
stratum granulosum; sp, stratum pyramidale), and
(D) floccular lobe of cerebellum
(arrow indicates Purkinje cell layer; gc,
granule cell layer). Individual neurons were labeled densely in only
two areas: deep neocortex (C, arrow) and the Purkinje
cell layer of cerebellum (D, arrow). Scale bar (shown in
A): A, B, 500 µm;
C, 625 µm; D, 350 µm.
|
|
6 mRNA
6 cRNA labeling was diffuse over the neuropil of gray and white
matter, giving rise to patchy labeling within the hippocampal and
cortical molecular layers, but was associated most prominently with
sharply defined cortical laminae. As summarized in Table 2 and
illustrated in Figure 5, moderately dense
hybridization was associated with neurons in the deeper aspect of the
anterior olfactory nucleus (Fig. 5A) and formed an extremely
thin layer just above the subcortical white matter (Fig.
5D-G). Cells in the latter field spanned the full cortical
mantle, at some levels merging with broader fields of labeled cells in
the endopiriform nuclei (Fig. 5D). The piriform cortex was
not well labeled at rostral planes (Fig. 5A,D), but in the
caudal piriform and rostral entorhinal cortices the labeled cells were
scattered in deeper layers and were laminated sharply in layer 2 near
the rhinal fissure (Fig. 5B). At progressively more caudal
planes the latter field of cells broadened to encompass, eventually,
the full extent of entorhinal cortex (Fig. 5E,F).
Very little labeling was evident in the hippocampal formation (Fig.
5E,G). In rostral sections only CA2 stratum pyramidale was
labeled clearly, although at very low densities (Fig. 5G,
arrow). More caudally, labeling was associated with a few
scattered hilar neurons and was evident at low levels in stratum
granulosum (Fig. 5E). In contrast, cells in the caudal subicular pyramidal cell layer were well labeled (Fig.
5F).
View larger version (175K):
[in this window]
[in a new window]
|
Figure 5.
6 mRNA is distributed most prominently within
deep cortex. Dark-field photomicrographs show the distribution of 6
cRNA labeling in select brain regions. A, Labeled cells
are distributed in the anterior olfactory nucleus (aon),
but not rostral piriform cortex (pc) or tenia
tecta (tt). B, Shown are labeled cells in
layer 2 of entorhinal cortex (ec) and the ventral
endopiriform nucleus (en) (broad arrow in
B, E, and F indicates the
rhinal fissure). C, High-magnification photomicrograph
showing labeled cells (arrowheads) just above the white
matter in retrosplenial cortex; note that smaller, more densely
Nissl-stained cells are not autoradiographically labeled.
D, Section through rostral forebrain showing the
distribution of labeled cells above the cortical white matter
(arrowhead) extending ventrolaterally into the
endopiriform nucleus (en) and the absence of clear
labeling in the olfactory tubercle (ot) and caudate
putamen (CPu). E, F,
Photomicrographs of sections through caudal hippocampus
(E) and the more caudal subiculum
(F) showing labeled cells in (1) the deepest
layers of neocortex (arrowhead) and allocortex, (2)
entorhinal cortex (ec), (3) caudal hippocampal stratum
granulosum (sg), and (4) subiculum (sub).
G, Section through rostral hippocampus showing faint
labeling in CA2 stratum pyramidale (arrow) and denser
labeling in the overlying deep neocortex (arrowhead;
sg, stratum granulosum; h, hilus).
H, Section showing labeling of the reticular thalamic
nucleus (rt). I, J, The
same field of paravermal cerebellum is shown with dark-field
(I) and bright-field
(J) illumination to show labeling of the Purkinje
cell layer (arrow in I) relative
to the Nissl-stained cytoarchitectonics (J)
(gc, granule cell layer in
I). K, L, Sections
showing labeling of the facial motor nucleus
(VII) and the subfornical organ
(sfo). Scale bar (shown in A):
A, 480 µm; B, 685 µm;
C, 60 µm; D-F, 1.25 mm;
G, H, L, 600 µm;
I, J, 400 µm.
|
|
6 mRNA was detected in a few subcortical regions, but labeling in
these fields was generally not dense. In particular, the reticular
thalamic nucleus (Fig. 5H), the paraventricular,
dorsal ventromedial, and arcuate hypothalamic nuclei and median
eminence (data not shown) were labeled. Beyond this, there was
low-density labeling in the oculomotor, facial motor (Fig.
5K), and hypoglossal nuclei, the mesencephalic,
principal, and motor trigeminal nuclei, and the Purkinje cell layer
(Fig. 5I,J). Finally, labeling was moderately dense
in the subfornical organ (Fig. 5L) and area postrema and was
low overlying the pia mater and ventricle epithelium.
7 mRNA
Hybridization of 7 cRNA was distributed broadly across the
neuraxis (Tables 2, 3), including particularly dense labeling in the
hippocampal formation and brainstem cranial nerve nuclei. As described
for other transcripts above, there was very low-density, irregularly
distributed labeling across the neuropil and far higher density
labeling that was aligned with neuronal cytoarchitectonics. In rostral
sections (Fig. 6A,D),
scattered cells in the anterior olfactory nucleus, tenia tecta, and the
extreme rostral piriform cortex were lightly to moderately well
labeled. At all levels there was fairly low-density but clearly
laminated labeling of the neuronal layers of neocortex (Fig.
6A,B), with labeling of individual neurons being
greatest in upper layer 5 (Fig. 6B). In contrast to
the distribution of other transcripts, 7 mRNA expression was not
laminated in the majority of olfactory cortex (Fig.
6F) or superficial olfactory tubercle (Fig.
6A). Like neocortex, labeling in the amygdala was
generally low and not sharply differentiated, although grain densities
were higher in the posterodorsal medial and central nuclei as compared
with the cortical and basolateral nuclei (data not shown).
View larger version (125K):
[in this window]
[in a new window]
|
Figure 6.
7 mRNA is expressed at high levels by neuronal
groups distributed across the neuraxis. Photomicrographs show the
distribution of 7 cRNA labeling in (A) rostral
forebrain with labeling evident in the tenia tecta (tt)
and neocortex, but not olfactory tubercle (ot);
(B) parietal cortex with most prominently labeled
cells evident in deep layer 5 (arrowhead; superficial to
the right); (C) spinal cord with
dense labeling of the spinal motor neurons (SpM);
(D) olfactory peduncle showing labeling of the
tenia tecta (tt) and the extreme rostrodorsal piriform
cortex (pc); (E) rostral
hippocampus showing labeling in stratum granulosum (sg)
and stratum pyramidale of regions CA3 and CA2 (between
arrows); and (F) temporal hippocampus and
entorhinal cortex (ec) showing labeling of scattered
cells in the subiculum (arrowhead). The same field of
cerebellar cortex in dark-field (G) and
bright-field (H) illumination is shown and
demonstrates 7 mRNA expression in the granule cell layer
(gc). I-L show extremely dense
labeling of neurons in motor cranial nerve nuclei and other discrete
nuclei of mesencephalon and lower brainstem, including the red
(rmc) and oculomotor (III) nuclei
(in I), the mesencephalic trigeminal
(arrowhead) and trochlear (IV)
nuclei (in J), the mesencephalic
(arrowhead) and motor (5Mo) trigeminal
nuclei (in K), and the facial motor nucleus
(VII; in L). Scale bar (shown in
L): A, 1.7 mm; B, G, H,
400 µm; C, D, K, 650 µm; E, F, 800 µm; I, J, L, 500 µm.
|
|
7 cRNA labeling differentiated the major hippocampal subfields. As
shown for the rostral hippocampal formation in Figure 6E, hybridization was dense in stratum granulosum,
CA2 stratum pyramidale, and the fasciola cinerium, moderately dense in
CA3 stratum pyramidale, and at general neuropil levels in CA1. The density of CA3 labeling and the incidence of labeled hilar neurons increased across the septotemporal axis of hippocampus. Moreover, in
temporal fields one could see relatively dense labeling of scattered
cells in the prosubiculum and subiculum (Fig. 6F,
arrowhead).
With the exception of moderately dense labeling in the supraoptic
nucleus, hybridization densities were low in the diencephalon, with
diffuse but greater than neuropil levels in the anteroventral, supramamillary, and medial geniculate nuclei. In sharp contrast, 7
mRNA levels were extremely high in discrete brainstem regions and, most
particularly, within all motor and several sensory cranial nerve nuclei (Table 3). Figure 6 shows the dense labeling of neurons in
the oculomotor nuclei and the red nucleus (Fig. 6I), the trochlear and mesencephalic trigeminal nuclei (Fig.
6J), the motor trigeminal nucleus (Fig.
6K), and the facial motor nucleus (Fig.
6L). In addition, 7 cRNA labeling was evident at
lower levels or in association with fewer cells in the vestibular,
cochlear, spinal trigeminal, and inferior olivary nuclei and in the
reticular formation (Fig. 6L, Table 3). High 7
mRNA expression by the many cholinergic efferent nuclei of brainstem
suggested that this transcript might be localized in spinal motor
neurons. As shown for the section of spinal cord illustrated in Figure
6C, the 7 cRNA labeled these motor neurons at extremely
high density.
Finally, 7 mRNA levels were high in the cerebellum. In distinction
from other transcripts, labeling was most prominent in the granule
cell layer (Fig. 6G,H), although at higher
magnification the labeling of Purkinje cells was evident as well.
8 mRNA
Prominent 8 cRNA labeling was entirely telencephalic (Tables 2,
3; Fig. 7). Labeled cells were
distributed within the anterior olfactory nucleus (Fig. 7A)
and adjacent to the deep cortical white matter (Fig. 7B),
extending into a broader, well labeled claustrum rostrally (Fig.
7D) and endopiriform nucleus caudally (Fig.
7G,H). Although deep cortical labeling was evident at
all levels, it was greatest in medial prelimbic and limbic cortex (Fig.
7C, arrow) and scattered away from the white matter to a variable degree among regions. For example, labeled cells were scattered well away from the white matter in the cingulate (Fig. 7B), insular, and auditory (Fig. 7G, arrow)
cortices but were limited to fewer cells near the white matter in
parietal, somatosensory cortex (Fig. 7D, arrowhead). The
distribution of these cells corresponded with that of large neocortical
layer 6 neurons, as seen in hematoxylin-stained tissue sections.
Labeling was generally low in superficial olfactory cortex (Fig.
7C,D), although labeled cells were scattered in deeper layers. A narrow field of rostral lateral septum was labeled densely (Fig. 7D), but hybridization was at background levels
throughout most of medial and lateral septum and in the diagonal bands
of Broca. The 8 cRNA also labeled caudate putamen, but not the
globus pallidus or nucleus accumbens. As shown in Figure 7D,
striatal labeling was patchy and increased along a
dorsomedial-to-ventrolateral gradient, being densest and extending
furthest caudal within the fundis of the striatum (Swanson, 1992).
View larger version (179K):
[in this window]
[in a new window]
|
Figure 7.
8 mRNA is expressed predominantly in forebrain.
Dark-field photomicrographs showing the distribution of 8 cRNA
labeling in (A) the olfactory peduncle
(aon, anterior olfactory nucleus);
(B) cortex overlying the corpus callosum
(cc) (cg, cingulate cortex; medial is to
the left); (C) rostral forebrain
in which there is dense labeling of neurons in deep prelimbic cortex
(arrow) and lesser labeling of cells above the remainder
of the subcortical white matter (arrowhead);
(D) the rostral caudate putamen
(CPu) and, in the same plane, cells above the cortical
white matter (arrowhead), within claustrum
(cl), and in a discrete field of lateral septum
(small arrow). Photomicrographs show labeling in
(E) field CA1 of rostral hippocampus
(sg, stratum granulosum), (F) the
hypothalamic suprachiasmatic nucleus (scn),
(G) temporal hippocampus (sub,
subiculum) and the amygdalohippocampal transition area
(arrowhead), and (H)
amygdala (bla, basolateral amygdala; la,
lateral amygdala dorsal part; en, endopiriform nucleus).
Note the regional differences in cortical lamination, with labeled
cells abutting the subcortical white matter in frontal and rostral
parietal cortices (arrowheads in C
and D, respectively) but being distributed more
diffusely in primary auditory cortex (arrow in
G). In a comparison of E and
G one can see that labeling in hippocampal fields CA1
and CA3 increases along a septotemporal gradient (septal pole is shown
in E; temporal pole is represented in the lower part of
G; asterisk indicates CA3c in both).
Scale bar (shown in H): A,
E, 640 µm; B, 500 µm;
C, D, 1.0 mm; F, 430 µm;
G, 800 µm; H, 575 µm.
|
|
Dense regionally differentiated labeling was observed in the
hippocampal formation and amygdala. As shown in Figure 7, E
and G, for rostral and caudal hippocampus, respectively, CA1
stratum pyramidale and the subiculum were well labeled, and
hybridization densities increased markedly across the septotemporal
axis. CA3c stratum pyramidale and hilar neurons did not appear to be
labeled, and the remainder of CA3 and the stratum granulosum were
labeled very lightly at rostral planes, but hybridization increased to moderate levels in each of these fields across the septotemporal axis.
CA2 stratum pyramidale was not labeled. As shown in Figure 7,
G and H, in amygdala the hybridization was dense
in the basolateral and dorsolateral nucleus, moderately dense in the
lateral nuclei and the amygdalohippocampal transition area, low and
irregularly distributed within the corticomedial nuclei, and at
neuropil levels in the central nucleus (Fig. 7G).
With the exception of moderately dense labeling of cells in the
suprachiasmatic (Fig. 7F) and arcuate nuclei, 8
cRNA labeling was low in diencephalon and at lower levels of the
neuraxis (Table 3).
V mRNA
As shown in Figure 8, among the
transcripts evaluated here V mRNA was the most abundant and broadly
distributed in neocortex. Labeling spanned the neuronal layers but was
relatively denser in layers 2/3 in rostral planes (Fig.
8B,H, Table 2). There was some diffuse and patchy
hybridization in cortical layer 1 and in molecular layers of other
regions, suggesting expression by glial cells. Expression was
relatively high in the anterior olfactory nucleus (Fig.
8A) and the superficial, but not deep, layers of piriform (Fig. 8B,C) and entorhinal (Fig.
8E,G) cortex. The piriform cortical labeling extended
into the superficial olfactory tubercle (Fig. 8C); in the
latter region the islands of Calleja and striatal bridge regions were
labeled at lower densities. Within the amygdala, labeling densities
were low and relatively undifferentiated, with the exception of
moderately well labeled cells in the posterior cortical nuclei (Fig.
8E). Within the hippocampal formation, expression was
moderate to low in stratum granulosum, low in CA1 stratum pyramidale,
and at neuropil levels within CA3 stratum pyramidale (Fig.
8G, Table 2). For this and all transcripts previously
described, there was no clear evidence for the labeling of neurons
within the hippocampal molecular layers.
View larger version (132K):
[in this window]
[in a new window]
|
Figure 8.
V mRNA is distributed broadly in cortex and
striatum. A, B, Sections through extreme
rostral (A) and somewhat more caudal
(B) forebrain show broadly distributed V cRNA
labeling in neocortex, anterior olfactory nucleus (aon),
caudate putamen (CPu), piriform cortex
(pc), and olfactory tubercle (ot).
C, Higher magnification view of basal forebrain shows
labeling is dense within piriform layer II (pc)
and scattered deeper cells and is light in the islands of Calleja
(ic). D, High-magnification bright-field
photomicrograph of superficial neocortex shows that labeling is
associated with larger cells with the Nissl-staining characteristics of
neurons (arrowheads) and not with smaller, more densely
stained glial-like cells (small arrows).
E-G, Sections show hybridization within posteromedial
cortical amygdala (pomc; E), area
postrema (ap; F), and caudal
hippocampus (G). G, Shown is light
labeling in hippocampal CA1 stratum pyramidale and stratum granulosum
(sg) and labeling in entorhinal cortex
(ec). H, I,
Photomicrographs of the same field of visual cortex, using dark-field
(H) and bright-field
(I) illumination to visualize the
distribution of V cRNA labeling (H)
relative to cytoarchitectonic lamination
(I); labeling is most prominent in layers
2/3 and in association with large cells in deep layer 5, with diffuse
and lower density labeling in the nonpyramidal layer 4. J, Field of cerebellar cortex showing rather continuous
labeling of the Purkinje cell layer (arrowhead;
gc, granule cell layer). Scale bar (shown in
A): A, B, 1.0 mm;
C, 50 µm; D, 40 µm; E,
G, 820 µm; F, 585 µm;
H, I, 410 µm; J, 340 µm.
|
|
As shown in Figure 8B, V mRNA was the most
abundant of the transcripts in striatum. Labeling was distributed
rather evenly across the full caudate putamen, with the exception of
distributed patches of lower hybridization densities, giving the
impression of expression by matrix neurons (Gerfen, 1992). In contrast,
labeling was at neuropil levels in nucleus accumbens and globus pallidus.
With the exception of dense to moderately dense labeling in the area
postrema (Fig. 8F), median eminence, and
tuberomamillary nuclei, V mRNA levels were low (e.g., medial
geniculate, pararubral field) or at neuropil levels throughout
diencephalon, mesencephalon, and lower brainstem (Table 3). However,
within cerebellum the Purkinje cell layer was labeled densely (Fig.
8J). In contrast to the very punctate cellular
distribution of the 5 and 3 mRNAs within this lamina, V cRNA
labeling appeared more diffuse, suggesting that the mRNA either was
distributed partly into neuronal processes (thereby blurring perikaryal
boundaries) or was localized within glial cells.
4 mRNA
Labeling with 4 cRNA was extremely rare. Neuronal labeling was
limited to the granule cell layer of the dentate gyrus (Fig. 9A) and to a few cells
scattered within the dorsal motor nucleus of the vagus. In addition,
the circumventricular organs, ventricular ependyma (Fig.
9B), and pia mater were clearly labeled.
View larger version (95K):
[in this window]
[in a new window]
|
Figure 9.
Localization of transcripts for integrin
subunits 4, 5, and 1. A, B,
Shown is the autoradiographic localization of 4 cRNA labeling in the
dentate gyrus stratum granulosum (sg; A)
and the epithelium of the third ventricle (VE;
B); arrows indicate labeled cells
scattered near the ventricle in B. Shown is 5 cRNA
labeling in (C) parietal cortex (layers
II/III and VI are indicated),
(D) lateral cerebellar cortex
(arrowhead indicates labeled Purkinje cell layer;
gcl, granule cell layer), and (E)
the motor (Mo5) and mesencephalic (Mes5)
trigeminal nuclei. The scatter of 5 cRNA labeling into the
cerebellar molecular layer (D) and surrounding
the well labeled perikarya in the trigeminal nuclei
(E) suggests that mRNAs may be localized within
proximal dendrites. F, Shown are double-labeled cells in
the hypoglossal nucleus of a tissue section processed for the
simultaneous colorimetric and autoradiographic localization of 7 and
1 mRNAs, respectively. As in this example, all labeled neurons
within the hypoglossal and other efferent cranial nerve nuclei were
double-labeled, indicating total 71 colocalization in these
fields. Scale bar (shown in B): A, B, D,
E, 1 mm; C, 720 µm; F, 72 µm.
|
|
5 mRNA
Similar to the distribution of 3 cRNA labeling, the 5 cRNA
generated both diffuse, low-density labeling throughout most regions of
neuropil and greater hybridization densities in specific neuronal
fields distributed across the neuraxis (Tables 2, 3). In telencephalon
the labeling was most prominent within cortex and basal forebrain. In
the neocortex low-to-moderate hybridization densities spanned layers
2-5, with densities being greatest in layers 4/5 (Fig. 9C).
In allocortex the labeling was distributed in the deeper layers, being
conspicuously low in layer 2 of the granular cingulate and
retrosplenial cortices. Labeling was diffuse and at low densities in
olfactory cortical regions and amygdala, with the exception of the
posterodorsal medial amygdala, which stood out as being moderately
densely labeled. Within the hippocampal formation there was diffuse and
somewhat patchy labeling over much of the neuropil and a few well
labeled cells scattered within the hilus and hippocampal molecular
layers. At high magnification the latter cells were Nissl-pale and
appeared neuron-like. In addition, labeling increased across the
septotemporal axis of CA1 and CA3 stratum pyramidale and was moderately
dense in the temporal subicular cell layer. In diencephalon there was
low to moderately dense labeling in the paratenial, anteroventral, and ventroposterior thalamic nuclei, the ventral thalamus, and much of
hypothalamus (Table 3).
Labeling with the 5 cRNA was denser and regionally differentiated at
lower levels of the neuraxis. As summarized in Table 3, in addition to
low-density hybridization over much of the reticular formation,
hybridization was dense to moderately dense in association with the
efferent cranial nerve nuclei; this is illustrated for the
mesencephalic and motor trigeminal nuclei in Figure 9E. In
addition, ventral horn neurons evident at the lowest levels of
brainstem were labeled very densely. Within cerebellum, hybridization
was dense in both the Purkinje and granule cell layers and low to
moderately dense in the deep cerebellar nuclei. Labeling of the
Purkinje cell layer appeared to dissipate into the overlying molecular
layer, suggesting that transcripts were, in part, distributed into dendrites.
Colocalization of 7 and 1 mRNAs
As summarized in Table 3, the distribution of 7 mRNA within
lower brain centers and, in particular, within efferent cranial nerve
nuclei overlaps the brainstem distribution of 1 integrin mRNA
described in an earlier study from this laboratory (Pinkstaff et al.,
1998). To determine whether 7 and 1 mRNAs are coexpressed by
individual brainstem neurons, we processed sections through cerebellum,
lower brainstem, and spinal cord for the simultaneous colorimetric and
autoradiographic localization of 7 and 1 mRNAs, respectively.
Labeling with the two cRNAs was fully colocalized in the efferent
cranial nerve nuclei; i.e., all labeled cells were double-labeled. This
colocalization is illustrated for neurons of the hypoglossal nucleus in
Figure 9F. In addition, vestibular, reticular formation, and
ventral horn spinal neurons were double-labeled. The relative density
of labeling did vary between regions. A majority of labeled cells in
the efferent cranial nerve nuclei and spinal ventral horn were labeled
densely by both the 7 and 1 cRNAs. In contrast, neurons of the
vestibular nuclei were labeled only moderately densely with the two
probes, and cells in the dorsal motor nucleus of the vagus were densely
labeled with 1 cRNA and lightly labeled with 7 cRNA. The
cerebellar granule cells and some scattered cells in the reticular
formation were labeled with 7 cRNA alone.
| |
DISCUSSION |
The present results demonstrate that mRNA expression for eight and two integrin subunits is regionally differentiated in the adult
brain. Only transcripts for 2, 2, and 3 were not detected.
Dense neuronal labeling was evident at all levels of the neuraxis. Some
transcripts also were expressed at low levels within molecular layers
and white matter. Although the latter labeling was never densely
clustered over individual cells, it is typical of astroglial labeling
obtained with isotopic in situ hybridization (Pinkstaff et
al., 1998). Expression by both neurons and glia was expected from
studies of mRNA and protein content in dissociated cells (Neugebauer
and Reichardt, 1991; Tomaselli et al., 1993; Tawil et al., 1994;
DeFreitas et al., 1995; Shaw et al., 1996) and brain (Grooms et al.,
1993; Einheber et al., 1996; Cousin et al., 1997; Nishimura et al.,
1998), but the distributions and levels of gene expression for subunits
that were evaluated here were not anticipated in the literature. A
previous study demonstrated that integrin 1 mRNA is expressed at
high levels by select neuronal groups in adult brain (Pinkstaff et al.,
1998). The present findings show that the general features of 1
expression (prominently neuronal and region- and cell-specific) are
indeed typical of other integrin subunits and that neurons containing moderate-to-high levels of each of the integrin subunit mRNAs are
distributed differentially.
Both and integrin subunits contribute to ligand recognition
(Aplin et al., 1998) and to the specificity of integrin/matrix interactions that are considered critical for neuronal migration, process outgrowth, and synaptogenesis (Dodd and Jessell, 1988; Sanes,
1989; Reichardt and Tomaselli, 1991; Zhang and Galileo, 1998). In
regard to this, it is intriguing that subunit expression profiles
differentiated brain systems and levels of the neuraxis. For example,
4 mRNA expression was limited to defined regions of limbic
forebrain. The 8 and V mRNAs were also predominantly, although
more broadly, expressed in forebrain: 8 mRNA was localized within
discrete neuronal groups in limbic telencephalon (hippocampus, amygdala), whereas V mRNA levels were greatest in neocortex. In
contrast, 3 and 5 mRNAs were distributed broadly and diffusely across the neuraxis.
Within some regions the subunit expression patterns were complementary.
For example, neocortical layers 2/3, 5, and deep 6 most prominently
expressed different subunits (V, 1, and 8, respectively).
Within the hippocampal formation the principal neurons of the dentate
gyrus, CA3, CA2, and CA1 were distinguished by higher mRNA levels for
the 7, 1, 4, and 8 subunits, respectively. In cerebellum,
7 and 5 mRNAs were abundant in the granule cells, whereas 3
and 1 mRNAs were highly expressed by the Purkinje cells but were not
detected in the granule cells. Together with the results described
above, these observations indicate that integrins provide functional
cell surface markers that discriminate morphologically distinct
populations of neurons between and within regions of adult brain.
Although there are many potential integrin combinations, the
true diversity of integrin receptors appears to be much more limited.
As reviewed elsewhere (Hynes, 1992; Schnapp et al., 1995), all of the
subunits that were studied here can associate with 1. V also
forms heterodimers with 3, 5, 6, and 8, and subunits 4
and 6 can associate with 7 and 4, respectively. In some instances, subunits compete for association with limiting
concentrations of the appropriate dimer partner (Moyle et al., 1991).
With these constraints in mind, the mRNA distributions reported here
and for 1 by Pinkstaff et al. (1998) (summarized on Tables 2 and 3
for comparison purposes) give rise to specific predictions about the
integrin receptors likely to be expressed by different neuronal groups
in adult brain (see Table 4). For
example, the colocalization of 7 and 1 mRNAs in the efferent
cranial nerve nuclei and spinal ventral horn suggests that the 71
laminin receptor is highly expressed by these groups of motor neurons. Overlapping mRNA distributions suggest that within the hippocampal formation the 71 and 11 (laminin, collagen) receptors are abundant in CA3 stratum pyramidale, but not in CA1 stratum pyramidale or stratum granulosum, whereas 81 (tenascin, fibronectin,
vitronectin) is abundant in CA1. Similarly, the V5 vitronectin
receptor would be predicted to be expressed by Purkinje cells, but not
by granule cells within cerebellum. Nishimura et al. (1998) recently
demonstrated that 8 and V immunoreactivities are similarly
localized to synapse-like puncta throughout the neuropil of
telencephalon and in cerebellum. Thus, the V8 vitronectin
receptor appears to be expressed by V mRNA-positive hippocampal,
striatal, and cortical neurons.
View this table:
[in this window]
[in a new window]
|
Table 4.
Potential integrin heterodimer combinations in select brain
regions: predictions from regional mRNA distributions and known
pairings in other systems
|
|
The nearly exclusive localization of 4 mRNA to the ventricular
epithelium and the dentate gyrus granule cells is intriguing in light
of the proposed role of the 64 laminin receptor in maintaining
the integrity of cytoplasmic plaques associated with hemidesmosomes
(Spinardi et al., 1995). Although 6 mRNA was not detected in the
granule cells in untreated rats, it is upregulated in these neurons by
seizures (J. Pinkstaff and C. Gall, unpublished observations). The
granule cells form puncta adherens (Ribak and Anderson, 1980), and
ventricular epithelial cells form macula adherens (Peters et al.,
1976). Thus, 64 expression may be linked to the
organization of tight junctions with submembranous plaques in brain as
in other tissues.
Aspects of the present results are surprising and raise issues that
will require further information for resolution. Prominent examples
here include the absence of obvious dimer partners for 7 and 5 in
the dentate gyrus and cerebellar granule cells, respectively. The 7
subunit reportedly associates exclusively with 1 (Hynes, 1992), but
1 mRNA levels are negligible in dentate granule cells (Pinkstaff et
al., 1998). Similarly, 5 is thought to associate with V alone
(Hynes, 1992), but V mRNA was not detected in cerebellar granule
cells. It is possible that heterodimer partners are lacking in these
instances and that the unpaired subunits are degraded. However, it is
also possible that novel integrin proteins are expressed and form
previously uncharacterized receptors in these regions. Alternatively,
the conventional heterodimer partners may be present but are
transcribed at such low levels that mRNAs were not detected. This
interpretation also could account for discrepancies between the brain
distributions of mRNAs and immunoreactivities for 8 (Einheber et
al., 1996) and 1 (Murase and Hayashi, 1998). For these subunits the
immunostaining patterns overlap but extend beyond the mRNA
distributions reported here. These region-specific inconsistencies
suggest that brain subdivisions and neuronal populations differ not
only in the types of integrins they express but also in the rates at
which these receptors are metabolized: slow turnover would be
associated with low and potentially undetectable mRNA levels. This
further implies that neurons differ in the rates at which adhesive
contacts are modified or replaced. Possibly relevant to the idea that
integrin mRNA levels reflect structural plasticity are results showing
that seizures, which induce synaptic remodeling (Gall et al., 1997),
increase 1 (Pinkstaff et al., 1998) and 1 (J. Pinkstaff and C. Gall, unpublished observations) gene expression in hippocampus and
cortex and, in the latter instance, reveal synthetic capacity that
accords with immunocytochemical results.
Integrins are not catalytically active but are linked to the
cytoskeleton and to cytoplasmic signaling cascades by association with
other molecules (Clark and Brugge, 1995; Katz and Yamada, 1997); the
specific molecular interactions are determined mainly by the subunit
composition of the receptor (Huhtala et al., 1995; Jewell et al., 1995;
Giancotti, 1996; Sastry et al., 1996; Pfaff et al., 1998). These
integrin-driven cascades have profound subunit-specific effects on
proliferation, differentiation, gene expression, and cell survival in a
variety of tissues (Clark and Brugge, 1995; Lafrenie and Yamada, 1996),
and recent studies suggest that integrins mediate similar processes in
the adult brain. For example, depending on the integrin expression
profile, disruption of integrin/matrix binding can lead to apoptosis
(Frisch and Francis, 1994; Judware et al., 1998). Chen and Strickland
(1997) recently reported that disruption of laminin adhesion within
hippocampus exacerbates the excitotoxic effects of kainic acid on CA1
and CA3 stratum pyramidale, but not on stratum granulosum. Subunit
expression profiles reported here suggest that 1-containing laminin
receptors (e.g., 11, 31, 71; Table 4) expressed
within stratum pyramidale, but not stratum granulosum, mediate this
effect. The integrins regulate the responsiveness of peripheral cells
to cytokines and growth factors (Miyamoto et al., 1996; Sastry et al.,
1996; Katz and Yamada, 1997). Recent studies point to the conclusion
that the integrins also influence trophic factor signaling in the adult brain, albeit via a novel mechanism. Specifically, integrin antagonists selectively increase gene expression for brain-derived neurotrophic factor and its receptor trkB in mature cultured hippocampal
slices, thereby indicating that integrins tonically suppress these
growth-related genes in differentiated central neurons (J. Pinkstaff,
A. Yong, C. Gall, G. Lynch, unpublished data).
On matrix binding the integrin receptor cytoplasmic domains nucleate
the formation of elaborate protein complexes, with strong influences on
the actin-based cytoskeleton (Clark and Brugge, 1995; Katz and Yamada,
1997). Precisely how these aggregates vary is not known, but, because
of differences in subunit-associated proteins, it reasonably can be
assumed that different integrins will favor different cytoskeletal
arrangements. If so, the class or classes of integrin receptors
inserted into individual synapses could shape the morphology of
postsynaptic densities and dendritic spines. Subunit composition is
also likely to affect the ease with which synaptic integrins are
activated, broken down, and replaced, variables that may be of primary
importance with regard to modifying synaptic structure. Related to
this, integrin antagonists block the consolidation of LTP; i.e.,
potentiation develops normally but decays gradually toward baseline
(Xiao et al., 1991). LTP is accompanied by changes in synaptic
morphology (Lee et al., 1980; Desmond and Levy, 1983; Buchs and Muller,
1996), and modifications to integrin-dependent adhesive relationships
are an obvious route for adjusting and then stabilizing local anatomy.
From this it follows that the types of integrins and other adhesion
molecules (Lüthi et al., 1994; Tang et al., 1998) expressed by a
neuron could be responsible for the different forms of plasticity
exhibited by the diverse populations of synapses in adult brain.
| |
FOOTNOTES |
Received Sept. 23, 1998; revised Dec. 7, 1998; accepted Dec. 9, 1998.
This work was supported by National Institute of Neurological and
Communicative Disorders and Stroke Grants NS26748 and NS37799 to C.M.G.
and Air Force Office of Scientific Research Grant F49620-J-0304 to G.L.
We thank Dr. Julie Lauterborn for comments on this manuscript and the
following persons who generously provided cDNAs used in this project:
Drs. L. Reichardt (University of California, San Francisco; 1 and
8), S. Santoro (Washington University, St. Louis, MO; 2), J.-J.
Cassiman (University of Leuven, Belgium; 4), R. Hynes (Massachusetts
Institute of Technology, Cambridge, MA; 5), V. Quaranta (The Scripps
Research Institute, La Jolla, CA; 6), S. Kaufman (University of
Illinois; 7), L. Rome (University of California, Los Angeles; 1),
S. Teitelbaum (Washington University, St. Louis, MO; 3), and S. Kennel (Oak Ridge National Laboratory, TN; 4).
Correspondence should be addressed to Christine M. Gall, Ph.D.,
Department of Anatomy and Neurobiology, University of California at
Irvine, Irvine, CA 92697-1275.
| |
REFERENCES |
-
Aplin A,
Howe A,
Alahari S,
Juliano R
(1998)
Signal transduction and signal modulation by cell adhesion receptors: the role of integrins, cadherins, immunoglobulin-cell adhesion molecules, and selectins.
Pharmacol Rev
50:197-263[Abstract/Free Full Text].
-
Bahr B,
Lynch G
(1992)
Purification of an Arg-Gly-Asp selective matrix receptor from brain synaptic plasma membranes.
Biochem J
281:137-142.
-
Bahr B,
Staubli U,
Xiao P,
Chun D,
Ji Z,
Esteban E,
Lynch G
(1997)
Arg-Gly-Asp-Ser-selective adhesion and the stabilization of long-term potentiation: pharmacological studies and the characterization of a candidate matrix receptor.
J Neurosci
17:1320-1329[Abstract/Free Full Text].
-
Bizon JM,
Lauterborn JC,
Isackson PJ,
Gall CM
(1995)
Acidic fibroblast growth factor mRNA is expressed by basal forebrain and striatal cholinergic neurons.
J Comp Neurol
366:379-389.
-
Buchs PA,
Muller D
(1996)
Induction of long-term potentiation is associated with major ultrastructural changes of activated synapses.
Proc Natl Acad Sci USA
93:8040-8045[Abstract/Free Full Text].
-
Capaldi D,
Rosario R,
Esteban E,
Bahr B
(1997)
A 27-kDa matrix receptor from rat brain synaptosomes: selective recognition of the Arg-Gly-Asp-Ser domain and unique resistance to calcium-dependent proteolysis.
Neurosci Res
28:275-279[Web of Science][Medline].
-
Chiba M,
Teitelbaum S,
Cao X,
Ross F
(1996)
Retinoic acid stimulates expression of the functional osteoclast integrin V 3: transcriptional activation of the 3 but not the V gene.
J Cell Biochem
62:467-475[Web of Science][Medline].
-
Clark E,
Brugge J
(1995)
Integrins and signal transduction pathways.
Science
268:233-239[Abstract/Free Full Text].
-
Cooper H,
Tamura R,
Quaranta V
(1991)
The major laminin receptor of mouse embryonic stem cells is a novel isoform of the 6 1 integrin.
J Cell Biol
115:843-850[Abstract/Free Full Text].
-
Cousin B,
Leloup C,
Penicaud L,
Price J
(1997)
Developmental changes in integrin -subunits in rat cerebral cortex.
Neurosci Lett
234:161-165[Web of Science][Medline].
-
Damsky C,
Werb Z
(1992)
Signal transduction by integrin receptors for extracellular matrix: cooperative processing of extracellular information.
Curr Opin Cell Biol
4:772-781[Medline].
-
DeFreitas M,
Yoshida C,
Frazier W,
Mendrick D,
Kypta R,
Reichardt L
(1995)
Identification of integrin 3 1 as a neuronal thrombospondin receptor mediating neurite outgrowth.
Neuron
15:333-343[Web of Science][Medline].
-
De Meirsman C,
Schollen E,
Jaspers M,
Ongena K,
Matthijs G,
Marynen P,
Cassiman J
(1994)
Cloning and characterization of the promoter region of the murine -4 integrin subunit.
DNA Cell Biol
13:743-754[Web of Science][Medline].
-
Denda S,
Muller U,
Crossin KL,
Erickson HL,
Reichardt LF
(1998)
Utilization of a soluble integrin-alkaline phosphatase chimera to characterize integrin 8 1 receptor interactions with tenascin: murine 8 1 binds to the RGD site in tenascin-C fragments, but not to native tenascin-C.
Biochemistry
37:5464-5474[Medline].
-
Desmond NL,
Levy WB
(1983)
Synaptic correlates of associative potentiation/depression: an ultrastructural study in the hippocampus.
Brain Res
265:21-30[Web of Science][Medline].
-
Dodd J,
Jessell T
(1988)
Axon guidance and the patterning of neuronal projections in vertebrates.
Science
242:692-699[Abstract/Free Full Text].
-
Einheber S,
Schnapp L,
Salzer J,
Cappiello Z,
Milner T
(1996)
The regional and ultrastructural distribution of the 8 integrin subunit in the developing and adult rat brain suggests a role in synaptic plasticity.
J Comp Neurol
370:105-134[Web of Science][Medline].
-
Falcioni R,
Cimino L,
Gentileschi M,
D'Agnano I,
Zupi G,
Kennel S,
Sacchi A
(1994)
Expression of 1, 3, 4, and 5 integrins by human lung carcinoma cells of different histotypes.
Exp Cell Res
210:113-122[Web of Science][Medline].
-
Frisch SM,
Francis H
(1994)
Disruption of epithelial cell-matrix interactions induces apoptosis.
J Cell Biol
124:619-626[Abstract/Free Full Text].
-
Gall C,
Lauterborn J,
Guthrie K,
Stinis C
(1997)
Seizures and the regulation of neurotrophic factor expression: associations with structural plasticity in epilepsy.
Adv Neurol
72:9-23[Medline].
-
Gerfen C
(1992)
The neostriatal mosaic: multiple levels of compartmental organization.
Trends Neurosci
15:133-139[Web of Science][Medline].
-
Giancotti FG
(1996)
Signal transduction by the 64 integrin: charting the path between laminin binding and nuclear events.
J Cell Sci
109:1165-1172[Web of Science][Medline].
-
Gong J-G,
Ko TC,
Brattain MG
(1998)
Disruption of fibronectin binding to the 51 integrin stimulates the expression of cyclin-dependent kinases and DNA synthesis through activation of extracellular signal-regulated kinase.
J Biol Chem
273:1662-1669[Abstract/Free Full Text].
-
Grooms S,
Jones L
(1997)
RGDS tetrapeptide and hippocampal in vitro kindling in rats: evidence for integrin-mediated physiological stability.
Neurosci Lett
231:139-142[Web of Science][Medline].
-
Grooms S,
Terracio L,
Jones L
(1993)
Anatomical localization of 1 integrin-like immunoreactivity in rat brain.
Exp Neurol
122:253-259[Web of Science][Medline].
-
Grotewiel M,
Beck C,
Wu K,
Zhu X,
Davis R
(1998)
Integrin-mediated short-term memory in Drosophila.
Nature
391:455-460[Medline].
-
Guthrie K,
Nguyen T,
Gall C
(1995)
Insulin-like growth factor-1 mRNA is increased in deafferented hippocampus: spatiotemporal correspondence of a trophic event with axon sprouting.
J Comp Neurol
352:147-160[Web of Science][Medline].
-
Huhtala P,
Humphries M,
McCarthy J,
Tremble P,
Werb Z,
Damsky C
(1995)
Cooperative signaling by 5 1 and 4 1 integrins regulates metalloproteinase gene expression in fibroblasts adhering to fibronectin.
J Cell Biol
129:867-879[Abstract/Free Full Text].
-
Hynes R
(1992)
Integrins, versatility, modulation, and signaling in cell adhesion.
Cell
69:11-25[Web of Science][Medline].
-
Ignatius M,
Large T,
Houde M,
Tawil J,
Barton A,
Esch F,
Carbonetto S,
Reichardt L
(1990)
Molecular cloning of the rat integrin 1-subunit: a receptor for laminin and collagen.
J Cell Biol
111:709-720[Abstract/Free Full Text].
-
Jewell K,
Kapron-Bras C,
Jeevaratnam P,
Dedhar S
(1995)
Stimulation of tyrosine phosphorylation of distinct proteins in response to antibody-mediated ligation and clustering of 3 and 6 integrins.
J Cell Sci
108:1165-1174[Abstract].
-
Judware R,
McCormick TS,
Mohr S,
Yun JK,
Lapetina EG
(1998)
Propensity for macrophage apoptosis is related to the pattern of expression and function of integrin extracellular matrix receptors.
Biochem Biophys Res Commun
246:507-512[Web of Science][Medline].
-
Katz BZ,
Yamada KM
(1997)
Integrins in morphogenesis and signaling.
Biochimie
79:467-476[Medline].
-
Kil S,
Lallier T,
Bronner-Fraser M
(1996)
Inhibition of cranial neural crest adhesion in vitro and migration in vivo using integrin antisense oligonucleotides.
Dev Biol
179:91-101[Web of Science][Medline].
-
Lafrenie R,
Yamada K
(1996)
Integrin-dependent signal transduction.
J Cell Biochem
61:543-553[Web of Science][Medline].
-
Lee K,
Schottler F,
Oliver M,
Lynch G
(1980)
Brief bursts of high-frequency stimulation produce two types of structural change in rat hippocampus.
J Neurophysiol
44:247-258[Free Full Text].
-
Lüthi A,
Laurent J,
Figurov A,
Muller D,
Schachner M
(1994)
Hippocampal long-term potentiation and neural cell adhesion molecules L1 and NCAM.
Nature
372:777-779[Medline].
-
Malek-Hedayat S,
Rome L
(1994)
Expression of a 1-related integrin by oligodendroglia in primary culture: evidence for a functional role in myelination.
J Cell Biol
124:1039-1046[Abstract/Free Full Text].
-
Maren MS,
Baudry M
(1995)
Properties and mechanisms of long-term synaptic plasticity in the mammalian brain: relationships to learning and memory.
Neurobiol Learn Mem
63:1-18[Web of Science][Medline].
-
Miyamoto S,
Teramoto H,
Gutkind J,
Yamada K
(1996)
Integrins can collaborate with growth factors for phosphorylation of receptor tyrosine kinases and MAP kinase activation: roles of integrin aggregation and occupancy of receptors.
J Cell Biol
135:1633-1642[Abstract/Free Full Text].
-
Moyle M,
Napier MA,
McLean JW
(1991)
Cloning and expression of a divergent integrin subunit 8.
J Biol Chem
266:19650-19658[Abstract/Free Full Text].
-
Murase S,
Hayashi Y
(1998)
Integrin 1 localization in murine central and peripheral nervous system.
J Comp Neurol
395:161-176[Web of Science][Medline].
-
Neugebauer K,
Reichardt L
(1991)
Cell-surface regulation of 1-integrin activity on developing retinal neurons.
Nature
350:68-71[Medline].
-
Nishimura SL,
Boylen KP,
Einheber S,
Milner TA,
Ramos DM,
Pytela R
(1998)
Synaptic and glial localization of the integrin V8 in mouse and rat brain.
Brain Res
791:271-282[Web of Science][Medline].
-
Paxinos G,
Watson C
(1986)
In: The rat brain in stereotaxic coordinates. New York: Academic.
-
Peters A,
Palay SL,
Webster H
(1976)
The fine structure of the nervous system.
In: The neurons and supporting cells. Philadelphia: Saunders.
-
Pfaff M,
Liu S,
Erle D,
Ginsberg M
(1998)
Integrin -cytoplasmic domains differentially bind to cytoskeletal proteins.
J Biol Chem
273:6104-6109[Abstract/Free Full Text].
-
Pinkstaff J,
Lynch G,
Gall C
(1998)
Localization and seizure-regulation of integrin 1 mRNA in the adult rat brain.
Mol Brain Res
55:265-276[Medline].
-
Reichardt L,
Tomaselli K
(1991)
Extracellular matrix molecules and their receptors: functions in neural development.
Annu Rev Neurosci
14:531-570[Web of Science][Medline].
-
Ribak CE,
Anderson L
(1980)
Ultrastructure of the pyramidal basket cells in the dentate gyrus of the rat.
J Comp Neurol
192:903-916[Web of Science][Medline].
-
Ruoslahti E
(1996)
Integrin signaling and matrix assembly.
Tumour Biol
17:117-124[Medline].
-
Sanes J
(1989)
Extracellular matrix molecules that influence neural development.
Annu Rev Neurosci
12:491-516[Web of Science][Medline].
-
Sastry S,
Lakonishok M,
Thomas D,
Muschler J,
Horwitz A
(1996)
Integrin -subunit ratios, cytoplasmic domains, and growth factor synergy regulate muscle proliferation and differentiation.
J Cell Biol
133:169-184[Abstract/Free Full Text].
-
Schnapp LM,
Hatch N,
Ramos DM,
Klimanskaya IV,
Scheppard D,
Pytela R
(1995)
The human integrin 8 1 functions as a receptor for tenascin, fibronectin, and vitronectin.
J Biol Chem
270:23196-23202[Abstract/Free Full Text].
-
Shaw C,
Milner R,
Compston A,
ffrench-Constant C
(1996)
Analysis of integrin expression on oligodendrocytes during axo-glial interaction by using rat-mouse xenocultures.
J Neurosci
16:1163-1172[Abstract/Free Full Text].
-
Shinar DM,
Schmidt A,
Halperin D,
Rodan GA,
Weinreb M
(1993)
Expression of V and 3 integrin subunits in rat osteoclasts in situ.
J Bone Miner Res
8:403-414[Web of Science][Medline].
-
Song W,
Wang W,
Foster R,
Bielser D,
Kaufman S
(1992)
H36-7 is a novel integrin alpha chain that is developmentally regulated during skeletal myogenesis.
J Cell Biol
117:643-657[Abstract/Free Full Text].
-
Spinardi L,
Einheber S,
Cullen T,
Milner TA,
Giancotti FG
(1995)
A recombinant tail-less integrin 4 subunit disrupts hemidesmosomes but does not suppress 64-mediated cell adhesion to laminins.
J Cell Biol
129:473-487[Abstract/Free Full Text].
-
Staubli U,
Vanderklish P,
Lynch G
(1990)
An inhibitor of integrin receptors blocks long-term potentiation.
Behav Neural Biol
53:1-5[Web of Science][Medline].
-
Staubli U,
Chun D,
Lynch G
(1998)
Time-dependent reversal of long-term potentiation by an integrin antagonist.
J Neurosci
18:3460-3469[Abstract/Free Full Text].
-
Swanson L
(1992)
In: Brain maps: structure of the rat brain. Amsterdam: Elsevier.
-
Tamura R,
Cooper H,
Collo G,
Quaranta V
(1991)
Cell type-specific integrin variants with alternative alpha chain cytoplasmic domains.
Proc Natl Acad Sci USA
88:10183-10187[Abstract/Free Full Text].
-
Tang L,
Hung CP,
Schuman EM
(1998)
A role for the cadherin family of cell adhesion molecules in hippocampal tong-term potentiation.
Neuron
20:1165-1175[Web of Science][Medline].
-
Tawil N,
Wilson P,
Carbonetto S
(1994)
Expression and distribution of functional integrins in rat CNS glia.
J Neurosci Res
39:436-447[Web of Science][Medline].
-
Tomaselli K,
Doherty P,
Emmett C,
Damsky C,
Walsh F,
Reichardt L
(1993)
Expression of 1 integrins in sensory neurons of the dorsal root ganglion and their functions in neurite outgrowth on two laminin isoforms.
J Neurosci
13:4880-4888[Abstract].
-
Wilson R,
O'Brien W,
Beaudet A
(1989)
Nucleotide sequence of the cDNA from the mouse leukocyte adhesion protein CD18.
Nucleic Acids Res
17:5397[Free Full Text].
-
Wu J,
Santoro S
(1996)
Differential expression of integrin -subunits supports distinct roles during lung branching morphogenesis.
Dev Dyn
206:169-181[Web of Science][Medline].
-
Xiao P,
Bahr B,
Staubli U,
Vanderklish P,
Lynch G
(1991)
Evidence that matrix recognition contributes to stabilization but not induction of LTP.
NeuroReport
2:461-464[Web of Science][Medline].
-
Yamada KM,
Miyamoto S
(1995)
Integrin transmembrane signaling and cytoskeletal control.
Curr Opin Cell Biol
7:681-689[Web of Science][Medline].
-
Yang J,
Rayburn H,
Hynes R
(1993)
Embryonic mesodermal defects in 5 integrin-deficient mice.
Development
119:1093-1105[Abstract].
-
Zhang A,
Galileo DS
(1998)
Retroviral transfer of antisense integrin 6 or 8 sequences results in laminar redistribution or clonal cell death in developing brain.
J Neurosci
18:6928-6938[Abstract/Free Full Text].
Copyright © 1999 Society for Neuroscience 0270-6474/99/1951541-16$05.00/0
This article has been cited by other articles:
|
|
|
|
 
M. R. Andrews, S. Czvitkovich, E. Dassie, C. F. Vogelaar, A. Faissner, B. Blits, F. H. Gage, C. ffrench-Constant, and J. W. Fawcett
{alpha}9 Integrin Promotes Neurite Outgrowth on Tenascin-C and Enhances Sensory Axon Regeneration
J. Neurosci.,
April 29, 2009;
29(17):
5546 - 5557.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. LLorens-Martin, I. Torres-Aleman, and J. L. Trejo
Reviews: Mechanisms Mediating Brain Plasticity: IGF1 and Adult Hippocampal Neurogenesis
Neuroscientist,
April 1, 2009;
15(2):
134 - 148.
[Abstract]
[PDF]
|
|
|
|
|
|
|
X.-b. Wang, O. Bozdagi, J. S. Nikitczuk, Z. W. Zhai, Q. Zhou, and G. W. Huntley
Extracellular proteolysis by matrix metalloproteinase-9 drives dendritic spine enlargement and long-term potentiation coordinately
PNAS,
December 9, 2008;
105(49):
19520 - 19525.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
A. Kostic, J. Sap, and M. P. Sheetz
RPTP{alpha} is required for rigidity-dependent inhibition of extension and differentiation of hippocampal neurons
J. Cell Sci.,
November 1, 2007;
120(21):
3895 - 3904.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. Zhao, Y.-S. Choi, K. Obrietan, and S. M. Dudek
Synaptic Plasticity (and the Lack Thereof) in Hippocampal CA2 Neurons
J. Neurosci.,
October 31, 2007;
27(44):
12025 - 12032.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
C. Bourgin, K. K. Murai, M. Richter, and E. B. Pasquale
The EphA4 receptor regulates dendritic spine remodeling by affecting {beta}1-integrin signaling pathways
J. Cell Biol.,
September 24, 2007;
178(7):
1295 - 1307.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
C.-S. Chan, J. M. Levenson, P. S. Mukhopadhyay, L. Zong, A. Bradley, J. D. Sweatt, and R. L. Davis
{alpha}3-Integrins are required for hippocampal long-term potentiation and working memory
Learn. Mem.,
September 6, 2007;
14(9):
606 - 615.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
C. Schachtrup, P. Lu, L. L. Jones, J. K. Lee, J. Lu, B. D. Sachs, B. Zheng, and K. Akassoglou
Fibrinogen inhibits neurite outgrowth via beta3 integrin-mediated phosphorylation of the EGF receptor
PNAS,
July 10, 2007;
104(28):
11814 - 11819.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
A. von Holst, U. Egbers, A. Prochiantz, and A. Faissner
Neural Stem/Progenitor Cells Express 20 Tenascin C Isoforms That Are Differentially Regulated by Pax6
J. Biol. Chem.,
March 23, 2007;
282(12):
9172 - 9181.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
Z. Huang, K. Shimazu, N. H. Woo, K. Zang, U. Muller, B. Lu, and L. F. Reichardt
Distinct Roles of the beta1-Class Integrins at the Developing and the Mature Hippocampal Excitatory Synapse
J. Neurosci.,
October 25, 2006;
26(43):
11208 - 11219.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
Y. Shi and I. M. Ethell
Integrins Control Dendritic Spine Plasticity in Hippocampal Neurons through NMDA Receptor and Ca2+/Calmodulin-Dependent Protein Kinase II-Mediated Actin Reorganization
J. Neurosci.,
February 8, 2006;
26(6):
1813 - 1822.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
C.-S. Chan, E. J. Weeber, L. Zong, E. Fuchs, J. D. Sweatt, and R. L. Davis
{beta}1-Integrins Are Required for Hippocampal AMPA Receptor-Dependent Synaptic Transmission, Synaptic Plasticity, and Working Memory
J. Neurosci.,
January 4, 2006;
26(1):
223 - 232.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
J. M. Proctor, K. Zang, D. Wang, R. Wang, and L. F. Reichardt
Vascular Development of the Brain Requires {beta}8 Integrin Expression in the Neuroepithelium
J. Neurosci.,
October 26, 2005;
25(43):
9940 - 9948.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
E. M. Y. Moresco, S. Donaldson, A. Williamson, and A. J. Koleske
Integrin-Mediated Dendrite Branch Maintenance Requires Abelson (Abl) Family Kinases
J. Neurosci.,
June 29, 2005;
25(26):
6105 - 6118.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
R. S. Schmid, S. Shelton, A. Stanco, Y. Yokota, J. A. Kreidberg, and E. S. Anton
{alpha}3{beta}1 integrin modulates neuronal migration and placement during early stages of cerebral cortical development
Development,
December 15, 2004;
131(24):
6023 - 6031.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
A. Saito, T. Hayashi, S. Okuno, T. Nishi, and P. H. Chan
Oxidative Stress Affects the Integrin-Linked Kinase Signaling Pathway After Transient Focal Cerebral Ischemia
Stroke,
November 1, 2004;
35(11):
2560 - 2565.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. L. T. Mercado, A. Nur-e-Kamal, H.-Y. Liu, S. R. Gross, R. Movahed, and S. Meiners
Neurite Outgrowth by the Alternatively Spliced Region of Human Tenascin-C Is Mediated by Neuronal {alpha}7{beta}1 Integrin
J. Neurosci.,
January 7, 2004;
24(1):
238 - 247.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
C.-S. Chan, E. J. Weeber, S. Kurup, J. D. Sweatt, and R. L. Davis
Integrin Requirement for Hippocampal Synaptic Plasticity and Spatial Memory
J. Neurosci.,
August 6, 2003;
23(18):
7107 - 7116.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
B. Lin, A. C. Arai, G. Lynch, and C. M. Gall
Integrins Regulate NMDA Receptor-Mediated Synaptic Currents
J Neurophysiol,
May 1, 2003;
89(5):
2874 - 2878.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
D. V Vasilyev and M. E Barish
Regulation of an inactivating potassium current (IA) by the extracellular matrix protein vitronectin in embryonic mouse hippocampal neurones
J. Physiol.,
March 15, 2003;
547(3):
859 - 871.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
E. A. Kramar, J. A. Bernard, C. M. Gall, and G. Lynch
Integrins Modulate Fast Excitatory Transmission at Hippocampal Synapses
J. Biol. Chem.,
March 14, 2003;
278(12):
10722 - 10730.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
K. Beumer, H. J. G. Matthies, A. Bradshaw, and K. Broadie
Integrins regulate DLG/FAS2 via a CaM kinase II-dependent pathway to mediate synapse elaboration and stabilization during postembryonic development
Development,
March 9, 2003;
129(14):
3381 - 3391.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
R. S. Schmid and E.S. Anton
Role of Integrins in the Development of the Cerebral Cortex
Cereb Cortex,
March 1, 2003;
13(3):
219 - 224.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
J. A. Rodriguez, E. Piddini, T. Hasegawa, T. Miyagi, and C. G. Dotti
Plasma Membrane Ganglioside Sialidase Regulates Axonal Growth and Regeneration in Hippocampal Neurons in Culture
J. Neurosci.,
November 1, 2001;
21(21):
8387 - 8395.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. L. Condic
Adult Neuronal Regeneration Induced by Transgenic Integrin Expression
J. Neurosci.,
July 1, 2001;
21(13):
4782 - 4788.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. Sixt, B. Engelhardt, F. Pausch, R. Hallmann, O. Wendler, and L. M. Sorokin
Endothelial Cell Laminin Isoforms, Laminins 8 and 10, Play Decisive Roles in T Cell Recruitment Across the Blood-Brain Barrier in Experimental Autoimmune Encephalomyelitis
J. Cell Biol.,
May 21, 2001;
153(5):
933 - 946.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
A. H Kashani, B.-M. Chen, and A. D Grinnell
Hypertonic enhancement of transmitter release from frog motor nerve terminals: Ca2+ independence and role of integrins
J. Physiol.,
January 15, 2001;
530(2):
243 - 252.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
C. Rampon, C. H. Jiang, H. Dong, Y.-P. Tang, D. J. Lockhart, P. G. Schultz, J. Z. Tsien, and Y. Hu
Effects of environmental enrichment on gene expression in the brain
PNAS,
November 7, 2000;
97(23):
12880 - 12884.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
J. Rohrbough, M. S. Grotewiel, R. L. Davis, and K. Broadie
Integrin-Mediated Regulation of Synaptic Morphology, Transmission, and Plasticity
J. Neurosci.,
September 15, 2000;
20(18):
6868 - 6878.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
J. K. Ivins, P. D. Yurchenco, and A. D. Lander
Regulation of Neurite Outgrowth by Integrin Activation
J. Neurosci.,
September 1, 2000;
20(17):
6551 - 6560.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. W. Cohen, B. G. Hoffstrom, and D. W. DeSimone
Active Zones on Motor Nerve Terminals Contain alpha 3beta 1 Integrin
J. Neurosci.,
July 1, 2000;
20(13):
4912 - 4921.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
G X Zhang, C M Baker, D L Kolson, and A M Rostami
Chemokines and chemokine receptors in the pathogenesis of multiple sclerosis
Multiple Sclerosis,
February 1, 2000;
6(1):
3 - 13.
[Abstract]
[PDF]
|
|
|
|
|
|
|
K. Beumer, J Rohrbough, A Prokop, and K Broadie
A role for PS integrins in morphological growth and synaptic function at the postembryonic neuromuscular junction of Drosophila
Development,
January 12, 1999;
126(24):
5833 - 5846.
[Abstract]
[PDF]
|
|
|
|
|
|
|
D. Mielenz, S. Hapke, E. Poschl, H. von der Mark, and K. von der Mark
The Integrin alpha 7 Cytoplasmic Domain Regulates Cell Migration, Lamellipodia Formation, and p130CAS/Crk Coupling
J. Biol. Chem.,
April 13, 2001;
276(16):
13417 - 13426.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
Top
Abstract
Introduction
