* Department of Biochemistry, University of Leicester, Leicester LE1 7RH, United Kingdom; and Medical Research Council
Muscle and Cell Motility Unit, The Randall Institute, King's College London, 26-29 Drury Lane, London WC2B 5RL, United
Kingdom
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Abstract |
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We have used gene disruption to isolate two
talin (/
) ES cell mutants that contain no intact talin.
The undifferentiated cells (a) were unable to spread on
gelatin or laminin and grew as rounded colonies, although they were able to spread on fibronectin (b)
showed reduced adhesion to laminin, but not fibronectin (c) expressed much reduced levels of
1 integrin, although levels of
5 and
V were wild-type (d) were less
polarized with increased membrane protrusions compared with a vinculin (
/
) ES cell mutant (e) were unable to assemble vinculin or paxillin-containing focal adhesions or actin stress fibers on fibronectin, whereas
vinculin (
/
) ES cells were able to assemble talin-containing focal adhesions. Both talin (
/
) ES cell
mutants formed embryoid bodies, but differentiation was restricted to two morphologically distinct cell
types. Interestingly, these differentiated talin (
/
) ES
cells were able to spread and form focal adhesion-like
structures containing vinculin and paxillin on fibronectin. Moreover, the levels of the
1 integrin subunit were
comparable to those in wild-type ES cells. We conclude that talin is essential for
1 integrin expression and focal adhesion assembly in undifferentiated ES cells, but
that a subset of differentiated cells are talin independent for both characteristics.
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Introduction |
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THE interaction between animal cells and the adhesive glycoproteins of the extracellular matrix is mediated by the integrin family of cell adhesion molecules, the cytoplasmic domains of which are thought to be
linked in many, but not all cases, to the actin cytoskeleton
(Burridge et al., 1996). Proteins that have been suggested
to participate in this link include talin, vinculin and -actinin (Jockusch et al., 1995
) which colocalize with integrins
in the specialized cell-matrix junctions or focal adhesions
formed when cultured cells are grown on rigid supports. Initial in vitro biochemical studies based on equilibrium
gel filtration indicated that talin can bind directly to integrins (Horwitz et al., 1986
), and a putative talin-binding
site in the cytoplasmic region of the
1-integrin subunit
has been identified based on peptide inhibition experiments (Tapley et al., 1989
). In a more recent study, purified
IIb
3 integrin was shown to bind to talin deposited
on plastic, and a monoclonal antibody raised against the
cytoplasmic domain of the
3 subunit blocked binding
(Knezevic et al., 1996
). Talin was also found to bind to synthetic peptides corresponding to the cytoplasmic domain of the
3 subunit, but it also bound to an
IIb cytoplasmic
domain peptide suggesting that integrin
-subunits might
also participate in the interaction. In addition, talin (but
also filamin) has been shown to bind to recombinant
polypeptides containing the
1A cytoplasmic domain
(Pfaff et al., 1998
). Since talin is an actin-binding protein
(Muguruma et al., 1992
; Niggli et al., 1994
; Hemmings et
al., 1996
; McCann and Craig, 1997
), it may provide a direct
link between integrins and the actin cytoskeleton. However, talin also binds to vinculin (Burridge and Mangeat,
1984
; Gilmore et al., 1992
, 1993
) which has been shown to
contain two F-actin binding sites (Huttelmaier et al., 1997
)
as well as a binding site for
-actinin (McGregor et al.,
1994
), a well-characterized actin bundling protein (Blanchard et al., 1989
).
-Actinin has also been reported to
bind directly to
1-integrin cytoplasmic domain peptides
(Otey et al. 1990
). Such data have lead to a model of the
focal adhesion in which integrins are linked to F-actin either directly via talin or
-actinin, or indirectly via interactions between talin, vinculin and
-actinin (Burridge et al.,
1996).
Evidence in support of this model has come from a variety of experimental approaches. Experiments with Caenorhabditis elegans mutants have clearly established that
the localization of talin to focal adhesion-like structures
requires a -integrin, but not vinculin (Moulder et al.,
1996
). Similarly, studies with a chimeric molecule containing the extracellular domain of N-cadherin fused to the
transmembrane and cytoplasmic domains of
1-integrin
support the view that the
1-integrin cytoplasmic domain
plays a key role in localizing talin specifically to cell-
matrix rather than cell-cell junctions (Geiger et al., 1992
).
Microinjection of antibodies to vinculin (Westmeyer et al.,
1990
) and talin (Nuckolls et al., 1992
; Bolton et al., 1997
)
into fibroblasts disrupts actin stress fibers, as do proteolytic fragments of
-actinin (Pavalko and Burridge,
1991
) and recombinant talin polypeptides (Hemmings et al., 1996
), presumably via a dominant negative effect. Antisense mRNAs to vinculin (Rodriguez Fernandez et al.,
1993) and talin (Albiges-Rizo et al., 1995
) have been found
to reduce cell adhesion and cell spreading of BALB/c 3T3
cells and Hela cells, respectively, and a mouse F9 teratocarcinoma cell line in which the vinculin gene has been disrupted showed altered adhesive characteristics (Coll et al.,
1995
; Volberg et al., 1995
). However, the vinculin (
/
)
F9 mutants retained the capacity to assemble talin-containing focal adhesions suggesting that vinculin is not an
essential component of cell-matrix junctions, at least in
this cell type. In an attempt to define further the role of
talin in the adhesion of cells to the extracellular matrix, we
have used gene replacement vectors to isolate mouse ES
cells1 in which both copies of the talin gene have been disrupted. The phenotypic properties of these cells are consistent with the hypothesis that talin plays a key role in
cell-matrix interactions.
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Materials and Methods |
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Isolation and Characterization of Mouse Talin and Vinculin Genomic Clones
A mouse talin cDNA spanning nucleotides 286-1,187 was generated by
reverse transcription-PCR from mRNA purified from 4 × 107 mouse NIH
3T3 cells using acid guanidinium thiocyanate and oligo(dT)-cellulose. The
PCR primers contained BamHI sites, and the PCR product was subcloned
into the BamHI site in pBluescript SK+ (Stratagene, La Jolla, CA), and
authenticated by sequencing. The cDNA was labeled with [32P]dCTP using the Quick Prime kit (Nycomed Amersham Inc., Princeton, NJ), and
used to screen 1 × 106 recombinants of a C129 mouse ES (E14) cell genomic library in 2001 (kindly provided by Dr. Andrew Smith, Centre for
Genome Research, Edinburgh) plated onto Escherichia coli host strain Q358. Restriction enzyme mapping of clone 5T
2 with all combinations of
BamHI, HindIII, SacI, and EcoRI, and Southern blotting using oligonucleotides based on 5' talin cDNA sequence (nucleotides [nt] 163-206,
500-518, 940-957, and 1381-1398), and end labeled using an ECL kit (Nycomed Amersham Inc.), suggested that clone 5T
2 contained the first two
coding exons. Clone 5T
2 was mapped in more detail by subcloning a
1-kb SacI-HindIII fragment and a 1.7-kb BamHI fragment into pBluescript. These constructs were sequenced with pBluescript reverse and
20
M13 primers, as well as with primers spanning nt 163-206, 287-271, and
294-314 of the mouse talin cDNA sequence (X56123). Comparison of the
resulting genomic sequence with the cDNA sequence, and with consensus
eukaryotic splice sites (Mount and Steitz, 1981
) allowed definition of the boundaries of the first two coding exons. A mouse ES cell vinculin genomic clone containing exons 4-6 was isolated and characterized in a similar way.
Generation of Talin and Vinculin Gene Targeting Constructs
The talin genomic clone 5T2 was digested with BamHI and a 2.4-kb fragment cloned into the BamHI site of plasmid pX53 (Ohno et al., 1994
) in
the opposite transcriptional orientation to the Neomycin (Neo) gene to
give the vector pX53-5'arm. A 6.2-kb HindIII fragment from 5T
2 was
cloned into the HindIII site of pBluescript SK+ such that the ClaI site in
the multiple cloning site was 5' with respect to the genomic DNA fragment. This fragment was then excised from pBluescript using ClaI-NotI
and cloned into the pX53-5' arm vector digested with ClaI-NotI. A vinculin gene targeting vector was created by subcloning a 7.5-kb BamHI-XbaI
genomic fragment containing exons 4-6 into the BamHI-XbaI sites in
pBluescript. A BamHI-XhoI Neo cassette from the pX53 vector was then
blunt ended into the unique MscI site in exon 5. Equivalent constructs of
both the talin and vinculin gene targeting vectors were also made in which
the Neo gene was replaced with the Hygromycin (Hyg) gene. Plasmid
DNA was prepared using maxiprep columns (QIAGEN Inc., Chatsworth,
CA) and all constructs were linearized with NotI.
ES Cell Culture
Mouse ES cell clone HM1 (a generous gift of Dr. David Melton, University of Edinburgh) was cultured (37°C in 5% CO2 in air) on tissue culture
plates coated with 0.1% gelatin in Dulbecco's modified Eagle's medium/
Ham's F12 nutrient mix (GIBCO BRL, Gaithersburg, MD) containing
0.1% NaHCO3, -mercaptoethanol (0.001%), antibiotics/mycotics/kanamycin (GIBCO BRL), 15% batch-tested fetal calf serum, and sufficient leukemia inhibitory factor (LIF) to suppress differentiation. LIF was prepared by transiently expressing a plasmid containing a LIF cDNA construct (pXMT2) in monkey COS cells, and harvesting the culture medium.
The ability of each LIF preparation to suppress ES cell differentiation was
tested before use.
Electroporation of ES Cells with Targeting Constructs and Selection of Homologous Recombinants
Exponentially growing HM1 ES cells (1 × 108) were trypsinized, washed
2× with cold Hepes-buffered saline (2.5 mM Hepes buffer, pH 7.1, 0.75 mM Na2HPO4, 140 mM NaCl), and resuspended in 3.5 ml of Hepes-buffered saline on ice. The linearized (Not1) talin targeting construct (100 µg)
containing the Neo selection marker was added in 0.5 ml Hepes-buffered
saline, and 0.8-ml aliquots incubated in electroporation cuvettes for 10 min on ice. The cells were resuspended, then electroporated (240 volts,
500 µF) using a gene pulser (Bio-Rad Laboratories, Hercules, CA). The
cells were kept for 10 min at room temperature, then resuspended in 200 ml of culture medium and distributed in 20 × 9-cm gelatin-coated dishes.
After 24 h, the medium was changed and G418 (100 µg/ml) and 0.2 µM
gancyclovir added. The medium was changed daily until surviving colonies were visible (~10 d), and these were then picked using a Gilson micropipette into 96-well microtiter plates coated with gelatin, and dispersed
by pipetting. When confluent, cells were trypsinized to produce two replica plates. Genomic DNA was prepared from one plate and digested with
EcoRI using an "in well" procedure (Ramirez-Solis et al., 1992), before
screening for homologous recombinants by Southern blotting. The second
plate was stored at
70°C using 10% dimethyl sulfoxide as a cryoprotectant. Clones heterozygous at the talin locus were taken through a second round of electroporation using a targeting construct containing the Hyg selection marker to inactivate the remaining talin allele. Essentially
identical methods were used to target the vinculin gene in ES cells, except
that the construct used lacked the thymidine kinase gene (TK) negative
selection marker, and therefore gancyclovir was not added to the culture
medium.
Western Blotting
Confluent dishes (9 cm) of ES cells were washed twice with PBS, the cells
scraped into 0.5 ml lysis buffer (2% SDS in 75 mM Tris-HCl, pH 6.8, containing 10% glycerol, and 0.1 mM PMSF) and the sample heated at 100°C
for 10 min. Aliquots of cell lysate containing equivalent amounts of protein were subjected to SDS-PAGE (7% gels) and the proteins electroblotted to Hybond C membranes using a semi-dry blot apparatus (Bio-Rad
Laboratories). Excess protein binding sites were blocked by incubation in
5% dried milk in Tris-buffered saline, pH 7.4. Talin was detected using a
mouse monoclonal antibody TD77 raised against human platelet talin
(Bolton et al., 1997) and diluted 1:10,000 in blocking buffer. Vinculin was
detected using the mouse monoclonal antibody F9 diluted 1:400 (a generous gift from Dr. V. Koteliansky, CNRS Ecole Normal Superieure, Paris).
Antibodies to paxillin and the
3 integrin subunit were purchased from
Transduction Laboratories (Lexington, KY) and antibodies to
1,
V,
and
5 integrin subunits were purchased from Chemicon (Harrow, London, UK). An antibody to mouse pp125FAK was prepared by immunizing
rabbits with a recombinant polypeptide derived from the COOH-terminal
region of the protein. A rabbit polyclonal antibody raised against human
platelet VASP was a generous gift from Dr. M. Reinhard (Medizinische
Universitatsklinik, Wurzburg, Germany). Bound primary antibody was
detected by adding anti-mouse or anti-rabbit antibodies coupled to HRP
(1:3,500) in conjunction with an ECL kit (Nycomed Amersham Inc.).
Adhesion Assay
96-well Nunc-Immunoplates (MaxiSorp 439454A) were coated with either 25-50 µg /ml laminin or fibronectin (Sigma Chemical Co., St. Louis, MO) overnight at 4°C, and the wells washed three times with PBS. Excess protein-binding sites were blocked with 2% BSA (2 h at room temperature), and the wells washed with PBS. ES cells were trypsinized, the trypsin neutralized by addition of complete medium, and cells suspended (8 × 105/ ml) in serum-free medium. 100 µl of cell suspension was added to each well and the cells allowed to attach for 60 min at 37°C. Nonadherent cells were removed by washing 3× with PBS, and the attached cells were fixed with 10% formaldehyde (30 min) and stained with 1% toluidene blue for 60 min. The plates were washed extensively with water, air dried and the dye extracted with 2% SDS and the absorbance read at 630 nm using a microtiter plate reader. The assays were carried out in triplicate, and each experiment was repeated three times.
Immunofluorescence
ES cells cultured on glass coverslips coated with bovine fibronectin (50 µg/ml) for 24-48 h, were washed with PBS and fixed in 3.8% formaldehyde in PBS for 10 min at room temperature. Fixed cells were permeabilized with 0.2% Triton X-100 in PBS for 30 s, and incubated with 1% BSA in PBS for 1 h before staining for either talin or vinculin using mouse monoclonal antibodies TD77 and F9 respectively (1:50), and a Texas red- labeled anti-mouse Ig (Nycomed Amersham Inc.), all diluted in 0.2% BSA in PBS. Cells were counterstained for F-actin using FITC phalloidin (Sigma Chemical Co.) as per manufacturer's instructions.
Time-lapse Recording and Analysis of ES Cell Behavior Using Interference Microscopy
The phenotype of isolated, undifferentiated, ES cells cultured on fibronectin-coated coverslips was analyzed using the DRIMAPS method of
interference microscopy for recording cell behavior (Dunn et al., 1997).
This system produces digital images in which the intensity at each point is
directly proportional to the mass of nonaqueous cellular material in the
light path. Time-lapse recordings of wild-type cultures and of the two mutant types were made over 20-h periods at a lapse interval of 1 min. Individual cells in each sequence of images were next identified by tracking the cells with a mouse-operated cursor during playback of the sequence.
Computer processing then yielded for each cell in each frame, its dry
mass, its spread area, the coordinates of its mass centroid (center of gravity) and two parameters, elongation and dispersion, describing cell shape
(Dunn and Brown, 1986
). Comparison of consecutive frames yielded further parameters describing the protrusion and retraction of the cell margin. Protrusion is defined as the region of the substratum newly covered
by the cell during the frame interval whereas retraction is the region from
which the cell withdraws during the interval. The areas, positions of the
area centroid and changes in dry mass of these regions were measured.
For analysis of variance (ANOVA), data from each cell were partitioned
into 1-h runs, discarding any remainder, and mean values of parameters
were then calculated for each run. These means were then nested according to cells, cultures and genotypes and the significances of any differences
between the genotypes were assessed using a nested ANOVA which prevents false significances arising due to differences between cells or between cultures (Dunn et al., 1997
). Spectral analysis of rapid variations in
protrusion and retraction was performed using the Time Series Pack issued as a supplement to the MathematicaR package. Covariances were obtained from runs of data up to a lag of 50 min. Then the covariances for
all runs of one genotype were pooled by weighting according to run length
and the smoothed power spectrum was obtained using the Tukey-Hanning lag window of width 50 (Dunn et al., 1997
). Recordings from 16 wild-type cultures, 9 cultures of the talin (
/
) A28 mutant cells and 10 cultures of the vinculin (
/
) D7 mutant cells were analyzed. A total of
1,005 isolated cells were tracked and these yielded 3848 one hour runs.
ES Cell Differentiation
24-well tissue culture plates were coated with of 0.1% poly(2-hydroxyethylmethacrylate) (ICN) in 95% ethanol, and air dried at 37°C. 5 × 104 ES cells in 1 ml of complete medium plus LIF were added per well, and the following day, a further 1 ml of medium minus LIF was added to each well. On day three most of the medium was carefully aspirated from the wells while tilting the plate to allow the embryoid bodies to sink to the front of the well and fresh medium (1 ml) minus LIF was added to each well. On alternate days, the cells were either fed by addition of 1 ml of fresh medium (minus LIF) or the medium was replaced.
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Results |
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The Use of Neo and Hyg Replacement Vectors to Target Both Copies of the Talin Gene in Mouse ES Cells
A mouse talin genomic clone (5T2) was analyzed by restriction enzyme digestion and Southern blotting using oligonucleotide probes from the 5' end of the talin cDNA.
Sequencing of genomic fragments hybridizing to these
probes allowed the boundaries of the first two coding exons to be identified (Fig. 1 A). The first coding exon is 163 bp long and contains 127 bp of coding sequence. Codon 44 is split by an intron between coding exons 1 and 2. The second coding exon contains 97 bp ending at codon 76. A
2.4-kb BamHI fragment containing the 5' end of the first
coding exon and a 6.2-kb HindIII fragment containing the
3' end of the second coding exon were cloned either side
of the Neo gene in the vector pX53, which also contains a
TK negative selection marker (Fig. 1 B). Homologous recombination of this construct with the talin gene should
lead to deletion of codons 37-66 and the fusion of the Neo
gene with the residual parts of coding exons 1 and 2.
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The construct was linearized with NotI and electroporated into 1 × 108 ES cells (clone HM1). G418 was used to
select for cells containing the plasmid, and gancyclovir was
used to select against cells in which the construct had integrated randomly. Resistant colonies were transferred to
four 96-well microtiter plates. The cells were then grown
to confluence, replica plated, and genomic DNA from one
set was analyzed by Southern blotting. The wild-type talin
gene gives rise to a 13.8-kb EcoRI fragment that is detected by the probe indicated, whereas the Neo targeted
allele gives rise to a novel 7.6-kb fragment due the presence of an EcoRI site within the Neo gene (Fig. 1, C and
D). The result for one clone (C39) which is heterozygous
at the talin locus is shown in Fig. 1 E. Gancylcovir lead to a
twofold enrichment in homologous recombinants, and the
talin gene was targeted in ~1 in 3 of the G418/gancyclovir-resistant clones. To inactivate the second talin allele, an
equivalent targeting vector was constructed in which the
Neo gene was replaced by a Hyg selection marker. This
was electroporated into the talin (+/) ES cell clone C39,
and EcoRI digests of genomic DNA from 384 hygromycin resistant clones screened for targeting of the second allele. The targeted allele should give rise to a novel 6.8-kb fragment, with corresponding loss of the remaining wild-type
13.8-kb fragment (Fig. 1, C and D). Only 1 clone (A28)
was obtained which displayed this genotype (Fig. 1 E).
This may be because the talin null cells adhere only weakly
to gelatin-coated plates (see Fig. 3), and are lost during the
selection procedures. The talin (+/
) ES cell clone C39
was used in a second experiment with the Hyg targeting vector, and an additional clone (J26) in which both talin alleles had been disrupted was isolated (Fig. 1 E).
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Western Blot Analysis of ES Cell Talin Mutants
The expression of talin in these various ES cell clones,
grown in the presence of LIF to suppress differentiation,
was analyzed by Western blotting using a monoclonal antibody (TD77) raised against human platelet talin. This antibody, which recognizes an epitope at the extreme COOH-terminal region (residues 2464-2541) of talin (Bolton et
al., 1997), detected a single talin polypeptide in the wild-type ES cells. The talin (+/
) ES cell clone C39 showed a
significant reduction in talin immunoreactivity. However,
these cells expressed two talin polypeptides, one which
comigrated with the wild-type protein, the other migrating
with slightly increased mobility (Fig. 2, A and B). The talin
(
/
) ES cell mutants A28 and J26 showed almost complete loss of talin immunoreactivity (Fig. 2, A and B), although prolonged exposure of the blots showed that clone
A28 (Fig. 2 A) and J26 (data not shown) expressed very low levels of a truncated talin polypeptide that comigrated
with the truncated talin polypeptide expressed in the (+/
)
C39 ES cell line. The results clearly establish that both the
talin (
/
) A28 and J26 ES cell mutants express no intact
talin. The levels of two other cytoskeletal proteins associated with the cytoplasmic face of focal adhesions, vinculin
and
-actinin, were also somewhat reduced in the talin (
/
)
A28 mutant, although the levels of paxillin and pp125FAK
were similar to those in wild-type cells (Fig. 2 A). There
was also a dramatic reduction in the levels of the
1 integrin subunit in both the talin (
/
) ES cell mutants (Fig.
2, A and B) whereas the levels of both
5 and
V integrin subunits were comparable to those in wild-type ES cells.
The results show that loss of talin is associated with a reduction in the levels of a number of other focal adhesion
proteins, most notably the
1 integrin subunit.
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Morphology of the Undifferentiated Talin (/
) ES
Cell Mutants
Undifferentiated wild-type ES cells and the two talin (/
)
ES cell mutants were trypsinized and plated onto gelatin-coated tissue culture plates in the presence of LIF, and
their morphology inspected after 4 or 48 h by phase contrast microscopy. After 4 h, many of the wild-type cells
had begun to spread, whereas both of the talin (
/
) ES
cell mutants remained rounded with evidence of extensive
surface protrusions (Fig. 3 A). After 48 h, the wild-type ES
cells formed large colonies in which the cells were well
spread. In contrast, both the talin (
/
) ES cell mutants formed rounded colonies that were only loosely attached
to the substrate, and contained very few spread cells. A
notable feature of both talin (
/
) ES cell mutants was
the higher frequency of macropinocytic vesicles compared
with wild-type cells (Fig. 3 A). Whereas the talin (
/
) ES
cell mutants also showed surface protrusions and macropinocytic vesicles when plated on fibronectin, they were able
to spread, although spreading occurred more slowly, and
was somewhat less extensive than the wild-type ES cells
(Fig. 3 B). The morphology of the talin (
/
) ES cell mutants plated on laminin was similar to that on gelatin with
a marked reduction in cell spreading compared with wild-type ES cells (data not shown).
Talin (/
) ES Cell Mutants Show Reduced Adhesion
to Laminin but Not Fibronectin
The ability of wild-type ES cells, and the various talin ES
cell mutants to adhere to fibronectin and laminin is shown
in Fig. 4. Wild-type ES cells adhered to both fibronectin
and laminin to about the same degree over a 1-h period,
whereas adhesion to gelatin or collagen was very low
(OD630 < 0.1). Adhesion was abolished in the presence of
10 mM EDTA demonstrating a requirement for divalent
cations, a characteristic of integrin-mediated adhesion. Although both talin (/
) ES cell mutants expressed much
reduced levels of
1 integrin (Fig. 2), their adhesion to fibronectin was identical to that of wild-type ES cells. In
contrast, they showed a significant reduction in adhesion
to laminin. The reduced adhesion of the talin (
/
) ES
cell mutants to laminin is consistent with the fact that they
spread less well on laminin than fibronectin.
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Undifferentiated Talin (/
) ES Cell Mutants Fail to
Form Focal Adhesions on Fibronectin
Undifferentiated wild-type ES cells (HM1) and the talin
(/
) A28 ES cell mutant grown in the presence of LIF
were plated on coverslips coated with fibronectin and analyzed for their ability to form vinculin-containing focal adhesions and associated actin stress fibers after 48 h (Fig. 5).
Wild-type ES cells adopted a well-spread morphology and
assembled numerous actin stress fibers that terminated in
focal adhesions that stained for talin, vinculin, and paxillin.
In contrast, the talin (
/
) A28 ES cell mutant formed
large rounded colonies with few if any spread cells. They failed to assemble any actin stress fibers, and actin staining was limited to the cell margins with diffuse cytoplasmic
staining. There was no evidence of talin localized in focal
adhesions, although the cells showed some diffuse staining
for talin. Similarly, vinculin and paxillin staining was diffuse with only occasional punctate staining for vinculin at
the margins of the cell aggregates. The results for the J26
talin (
/
) ES cell mutant were identical (data not
shown). These findings establish that loss of talin compromises the ability of undifferentiated mouse ES cells to form focal adhesions and associated actin stress fibers on
fibronectin, although talin is not required to support integrin-mediated adhesion to fibronectin.
|
Phenotypic Properties of the Vinculin (/
) D7 ES
Cell Mutant
We have used a similar strategy to generate ES cells in
which both copies of the vinculin gene have been disrupted (Fig. 6, A and B). The vinculin (/
) D7 ES cell
line expressed no intact vinculin (Fig. 6 C), although low
levels of a truncated vinculin polypeptide could be detected on prolonged exposure of the Western blots. However, the levels of three vinculin-binding proteins, talin,
-actinin, and VASP (Fig. 6 C) as well as
1-integrin (data not shown) were comparable to those in wild-type ES
cells. The vinculin (
/
) D7 ES cell line showed a tendency to form rounded colonies when grown under standard culture conditions on gelatin-coated tissue culture
dishes, although on fibronectin, their morphology was similar to that of wild-type ES cells. These results are similar to those with the talin (
/
) ES cell mutants that also
formed rounded colonies on gelatin, but were able to
spread on fibronectin.
|
To establish whether the vinculin (/
) D7 ES cell mutant was able to form talin-containing focal adhesions,
cells were plated on fibronectin-coated glass coverslips
and stained for talin and F-actin. As expected, the wild-type ES cells formed prominent actin stress fibers that terminated in talin-containing focal adhesions (Fig. 6 E). Interestingly, the vinculin (
/
) D7 ES cell mutant retained
the capacity to assemble prominent actin stress fibers, but
these were invariably localized towards the outer cell margins. Talin was localized at the ends of these actin filaments, although the talin-containing structures were more elongated than in wild-type ES cells. Essentially identical
results were obtained with a second ES cell clone (DK022)
that also expressed no intact vinculin (data not shown).
The results establish that vinculin is not essential for the
assembly of talin-containing focal adhesions and associated actin stress fibers in undifferentiated ES cells, although the D7 ES cell clone that lacks vinculin, has a
somewhat different actin cytoarchitecture compared with
wild-type ES cells.
Analysis of the Behavior of Talin and Vinculin ES Cell Mutants
Wild-type ES cells and the talin (/
) A28 and vinculin
(
/
) D7 ES cell mutants were plated on fibronectin-coated coverslips and their behavior recorded over a period of 20 h using interference microscopy. The rate of increase in dry mass of individual cells served as a check on
the viability of the cultures. All cultures grew at a mean
rate of just over 5% h
1 with no significant differences due
to genotype in an ANOVA test. Cell spreading and cell
shape are all determined by the patterns of protrusion and
retraction of the cell margin (Dunn et al., 1997
) and, therefore, we examined these patterns directly. Fig. 7, a-c
shows a sample of protrusions (green) and retractions
(red) for cells of the three genotypes during a 2-min interval. Compared with the wild-type ES cells (Fig. 7 a), the
talin (
/
) A28 ES cell mutants (Fig. 7 b) showed large
bleb-like protrusions evenly interspersed with retractions
around the cell periphery, whereas the vinculin (
/
) D7
ES cell mutant (Fig. 7 c) showed greater polarity, with the
central cell displaying a large lamellar protrusion opposite
an extensive retracting margin. Fig. 7 d is a summary of
measurements of the mean polarity which we have previously defined as the distance in µm separating the centroids of protrusion and retraction over a 5-min period
(Dunn et al., 1997
). In this plot, the solid discs represent
the median values and the distributions of the data are indicated by the rectangles that span 50% of data values,
and the "bars" that span 80% of values. In ANOVA tests, the polarity of the talin (
/
) A28 ES cell mutant was significantly suppressed compared with wild-type ES cells (P < 0.05) whereas the polarity of the vinculin (
/
) D7 ES
cell mutant was significantly increased (P < 0.01).
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To quantify the rapid marginal blebbing observed in recordings of the talin (/
) A28 ES cell mutant, we performed a spectral analysis of the variations in protrusion.
Compared with other protrusions, blebs tend to have small
areas but high mass density, and the parameter we eventually chose for detecting rapid blebbing was therefore the
areal mass density of the protrusion regions measured in
units of pg/µm2. The power spectrum of variations in protrusion density for the three genotypes is shown in Fig. 7 e.
A single strong peak in any of these three spectra would
indicate a significant periodicity in the marginal activity of
the corresponding cells. In fact there are several weak
peaks in all three traces though their height in each case is
only ~20-30% of the total height of the spectrum. These
weak peaks indicate that there are multiple minor periodicities in the marginal activity at different frequencies, but
the net result is much closer to a random sequence than to
a periodic one. It is clear from the spectra that the power
of this random marginal activity is about seven times
greater in the talin (
/
) A28 ES cell mutant than in the
wild-type ES cells, whereas the vinculin (
/
) D7 mutant
showed only about half the power of the wild-type.
Talin (/
) ES Cell Mutants Form Embryoid
Bodies, but Extensive Morphological Differentiation
Is Inhibited
Both wild-type ES cells and the talin (/
) A28 ES cell
mutant form embryoid bodies of a similar size and appearance when grown in the absence of LIF for 8 d (Fig. 8).
This is not unexpected as the process is dependent on cadherin-mediated cell-cell interactions (Larue et al., 1996
),
and talin is specifically localized to integrin-containing cell-matrix junctions (Geiger et al., 1985
). When wild-type
embryoid bodies were plated on gelatin-coated tissue culture dishes, cells spread out from the central cell mass as a
continuous sheet over a period of 24-48 h (Fig. 8 A), and
formed an extensive cell monolayer within 5 d. In contrast,
only a few cells had begun to spread out from the margins
of the embryoid bodies formed by the talin (
/
) A28 ES
cell mutants after 24 h, and those cells that did migrate
over a 48-h period migrated as individual cells rather than
as a continuous cell sheet (Fig. 8 A). The leading edge of the migrating cells from the wild-type embryoid bodies always contained giant cells (Fig. 8 A, arrowheads). These
were never seen in the cells emerging from the talin (
/
)
A28 embryoid bodies. After 7 d on gelatin, wild-type embryoid bodies gave rise to a variety of cell types with distinct morphologies, including beating cardiomyocytes and
giant cells (Fig. 8 B, arrowheads), as well as organized
structures (Fig. 8 B, arrows). In contrast, the talin (
/
)
A28 embryoid bodies typically gave rise to only two morphologically distinct cell types, and no organized structures were observed (Fig. 8 B). Essentially identical results
were obtained with the talin (
/
) J26 ES cell mutant
(data not shown). Deletion of
1-integrins in mouse F9
teratocarcinoma cells has also been reported to block morphological differentiation (Stephens et al., 1993
).
|
Differentiated Talin (/
) ES Cell Mutants
Can Form Focal Adhesion-like Structures and Express
Normal Levels of
1 Integrin
Because the differentiated talin (/
) A28 and J26 ES
cells that migrate out of embryoid bodies are able to adopt
a spread morphology on gelatin-coated dishes, we investigated whether these cells could form focal adhesions and
actin stress fibers when plated on fibronectin. The differentiated cells derived from wild-type embryoid bodies
showed a variety of morphologies, and the organization of
the actin cytoarchitecture within these cells took on a variety of forms. However, in all cases there was prominent
staining for talin, vinculin and paxillin at the ends of actin
filaments (Fig. 9). Interestingly, the differentiated talin (
/
)
A28 cells also contained actin filaments, and in some cells,
the ends of these filaments showed staining for vinculin
and paxillin, but not talin. Identical results were obtained
with the talin (
/
) J26 ES cell mutant (data not shown).
|
Western blot analysis of both the differentiated talin (/
)
ES cell mutants showed that although these cells still expressed no intact talin, the levels of
1 integrin subunit as
well as vinculin were comparable with those in differentiated wild-type ES cells (Fig. 10). Therefore, it is apparent
that differentiation of the talin (
/
) ES cell mutants in
vitro generates cells in which neither
1 integrin subunit
levels or the assembly of focal adhesions and associated
actin filaments is dependent on talin.
|
![]() |
Discussion |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
We have used gene disruption technology to isolate two
talin (/
) ES cell mutants (A28 and J26) that contain no
intact talin, although both express low levels of a truncated
talin polypeptide. The most notable features of the undifferentiated talin (
/
) ES cell mutants are extensive
membrane blebbing, an accumulation of macropinocytic
vesicles and an inability to spread on gelatin or laminin on
which the cells grow as loosely attached colonies. Adhesion to laminin was significantly reduced, but adhesion to fibronectin was unaffected despite the fact that the cells
showed a dramatic reduction in levels of the
1 integrin
subunit. However, the talin (
/
) ES cell mutants were
unable to assemble focal adhesions or associated actin
stress fibers on fibronectin-coated coverslips, whereas a
vinculin (
/
) mutant (D7) was able to do so. These results provide compelling evidence that talin plays a crucial
role in the assembly of focal adhesions in undifferentiated ES cells. Interestingly, the talin (
/
) ES cell mutants
were able to form apparently normal embryoid bodies, but
when these were cultured on gelatin, cell migration from
the central cell mass was much slower than wild-type, and
differentiation was limited to just two morphologically
distinct cell types. These expressed normal levels of
1 integrin, and were able to spread and assemble focal adhesion-like structures with associated actin filaments on fibronectin. These results raise the possibility that loss of
talin restricts ES cell differentiation to a subset of cell types in which
1-integrin levels and focal adhesion assembly are talin independent.
The increase in membrane protrusions or blebs shown
by the undifferentiated talin (/
) ES cell mutants was
observed in cells plated on both gelatin and fibronectin.
Whether this reflects a failure of the cells to develop stable
adhesions with the extracellular matrix, or is due to membrane instability per se remains to be established. Increased membrane blebbing activity has been noted in
melanoma cells lacking the actin-binding protein ABP-280
(Cunningham et al., 1992
), and cleavage of the actin-binding
proteins talin,
-actinin (Miyoshi et al., 1996
), and fodrin
(Vanaga et al., 1996
) has been implicated in membrane
blebbing in apoptosis. Myosin light chain phosphorylation
and activation of actomyosin contraction has also been
shown to be involved in the membrane blebbing associated with apoptosis in PC12 cells (Mills et al., 1998
). The
authors speculate that actomyosin contraction in cells that
lack the structural proteins that normally couple cortical
actin to the plasma membrane may lead to cytoplasmic extrusion and membrane blebbing. Despite the much increased membrane blebbing activity displayed by the talin
(
/
) ES cell mutants, there was no evidence of an increase in apoptosis, and they showed no obvious difference in growth rate compared with wild-type ES cells
(data not shown).
The fact that the undifferentiated talin (/
) ES cell
mutants grew as poorly spread colonies on gelatin- and
laminin-coated substrates, and showed reduced adhesion
to laminin, is probably linked to the dramatic reduction in
1 integrin subunit expression, although we have not analyzed the levels of
1 integrins on the cell surface. Laminin
receptors are all members of the
1 integrin family (Newham and Humphries, 1996
), and reduced adhesion of the talin (
/
) ES cell mutants to laminin is not unexpected
therefore. Why adhesion to fibronectin was not reduced is
unclear as it has been reported that ES cells lacking the
1
integrin subunit fail to adhere to both laminin and fibronectin (Fassler et al., 1995
). ES cells express the
V integrin subunit (see Fig. 2 and Fassler et al., 1995
), and
those used in this study also expressed a protein of 90 kD
that reacted with an anti-
3 integrin antibody (data not
shown).
V
3 can act as a receptor for fibronectin, and
may compensate for the effects of any reduction in surface
expression
1 integrins in the talin (
/
) ES cell mutants.
However, others have failed to detect
3 integrin in ES
cells, although
1 integrin (
/
) ES cell mutants were
able to adhere to vitronectin (Fassler et al., 1995
). Although loss of talin did not affect adhesion of the undifferentiated talin (
/
) ES cell mutants to fibronectin, the
rate of cell spreading was reduced, and the cells were completely unable to assemble vinculin or paxillin-containing
focal adhesions or actin stress fibers. We conclude that
talin plays a key role in the assembly of focal adhesions
and the organization of the actin cytoarchitecture in undifferentiated ES cells. However, the fact that
1 integrin
subunit levels were dramatically reduced in both talin (
/
)
ES cell lines suggests that loss of talin may compromise focal adhesion assembly by more than one mechanism.
A number of observations suggest that talin is important
in the early stages of cell adhesion and spreading including
the formation of filopodia and lamellipodia. In Dictyostelium discoidum, talin accumulates at the tips of filopodia
formed in response to cAMP (Kreitmeier et al., 1995), and
microscale chromophore-assisted laser inactivation of talin
in neuronal growth cones results in temporary cessation of
filopodial extensions (Sydor et al., 1996
). In chick embryo
fibroblasts, talin is found in membrane ruffles as well as focal adhesions (Burridge and Connell, 1983
; Bolton et al.,
1997
), and it is recruited to nascent focal adhesions before
vinculin (DePasquale and Izzard, 1991
). Moreover, microinjection of antibodies to talin disrupt focal adhesions
(Nuckolls et al., 1992
; Bolton et al., 1997
), and downregulation of talin expression in Hela cells slowed down the
rate of cell spreading and lead to a reduction in the size of
focal adhesions (Albiges-Rizo et al., 1995
).
Analysis of the sequence of mouse (Rees et al., 1990)
and chicken (Hemmings et al., 1996
) talin (2541 amino acids), and the biochemical properties of the protein shows
that it has a number of features that make it highly suited
to act as a key element in the assembly of focal adhesions.
Talin is a dimeric elongated flexible protein (Goldmann et
al., 1994
; Winkler et al., 1997
) that binds
1- and
3-integrins (Horwitz et al., 1986
; Tapley et al., 1989
; Kenzevic
et al., 1996; Pfaff et al., 1998
), vinculin (Burridge and
Mangeat, 1984
; Gilmore et al., 1992
, 1993
), and F-actin
(Muguruma et al., 1992
; Hemmings et al., 1996
; McCann and Craig, 1997
), and is reported to possess actin nucleation (Niggli et al., 1994
) and bundling activity (Zhang et
al., 1996
). The NH2-terminal 433 residues of talin, which
can be liberated as a 47-kD polypeptide by calpain II, contain sequences that target the protein specifically to cell-
matrix junctions (Nuckolls et al., 1990
), and are capable of
binding acidic phospholipids (Niggli et al., 1994
). Interestingly, residues 165-363 show homology with the ERM
family of proteins that also act as linkers between the membrane and the actin cytoskeleton (Vaheri et al., 1997
).
The 190-kD COOH-terminal talin polypeptide liberated
by calpain II, which is composed of multiple
-helical alanine-rich repeats (McLachlan et al., 1994), contains the
dimerization site (Winkler et al., 1997
), three vinculin-binding sites (Gilmore et al., 1993
), and several actin-binding sites (Hemmings et al., 1996
) including an actin nucleation site (Niggli et al., 1994
). Although the 190-kD talin
polypeptide is reported to bind integrins (Horwitz et al., 1986
), the binding site has yet to be defined. However, the
finding that differentiated talin (
/
) ES cell can form focal adhesion-like structures, and express normal levels of
the
1 integrin subunit, suggests that talin is not required
for focal adhesion assembly in all cell types, and that there
are alternative pathways for the assembly of such structures. The actin-binding proteins
-actinin (Otey et al.,
1990
, 1993
) and filamin (Pfaff et al., 1998
) have been
shown to bind to the cytoplasmic face of
1 integrins, and may provide a mechanism for linking integrins to F-actin.
We have yet to investigate the mechanisms involved in
the downregulation of 1 integrins in talin (
/
) ES cells.
However, our findings are reminiscent of those of Albiges-Rizo et al. (1995)
, who used an antisense RNA construct
to downregulate talin in Hela cells. Cells in which talin levels were reduced by 38-60% showed loss of immunofluorescence staining for
1 integrins, although there was no
reduction in
1 integrin mRNA levels. Surface labeling studies showed that both
5 and
1 integrin subunits appeared on the cell surface in an abnormal form, suggesting
that there was a defect in integrin processing. Loss of talin
might compromise integrin trafficking at several levels. A
number of actin-binding proteins have recently been
shown to be localized in the Golgi apparatus (reviewed in
Stow et al., 1998
) including myosin I which supports transport of vesicles along actin filaments towards the barbed
membrane-attached end (Fath et al., 1994
). Although
there is no evidence that talin is localized in the Golgi, the
fact that loss of talin leads to a marked change in actin cytoarchitecture might result in the inhibition of vesicular
transport of integrins via such a pathway. It is also conceivable that talin plays a more specific role in
1 integrin
transport by binding transport vesicles containing integrins to actin filaments. The actin cytoskeleton and myosin
I have also been implicated in endocytic pathways (Durrbach et al., 1996
), and loss of talin may also effect the endocytic pathways thought to be important in integrin recycling (Bretscher, 1996
). An alternative explanation for the
down regulation of the
1 integrin subunit in the talin (
/
)
ES cell mutants is suggested by recent evidence that
poly(A)+ RNA and ribosomes are recruited to the focal
adhesion complexes formed in response to binding of fibronectin-coated beads to the cell surface (Chicurel et al.,
1998
). The authors speculate that certain mRNAs may be
translated in focal adhesions. Whether the mRNA encoding
1 integrin falls into this category remains to be investigated, but were this the case, loss of talin and the consequent inability of undifferentiated ES cells to assemble such structures might reduce translation of the
1 integrin
mRNA.
The origin of the truncated talin polypeptide expressed
by both talin (/
) ES cell mutants has not yet been established. The Neo gene (unlike the Hyg gene) was cloned
into the targeting vector in the opposite transcriptional
orientation to the talin gene. As a consequence, the Neo
polyadenylation signal and translation stop codons would
not be expected to halt transcription or translation from
this allele. Translational initiation at an internal in frame methionine (codon 79) downstream of the Neo sequence
would lead to a talin polypeptide lacking the first 78 amino
acids and differing in apparent molecular mass by 8,708 D. Such a deletion is consistent with the size of the truncated
talin polypeptide expressed by the talin ES (
/
) mutants. Alternatively, the targeted coding exons 1 and 2 could be spliced out of the primary transcript to give a
novel talin mRNA lacking codons 1-76. Translation could be initiated internally at methionine codon 79 or at any
number of in frame downstream AUG's, albeit with low
efficiency. Interestingly, a mouse F9 teratocarcinoma vinculin (
/
) mutant, which was originally null for vinculin
protein, was found to express a truncated vinculin polypeptide after a few passages in culture due to alternative splicing of the exon containing the Neo gene (Coll et
al., 1997
). The possibility that such a truncated talin
polypeptide might act as a dominant negative mutant
seems unlikely as it is expressed at very low levels, and the
talin (+/
) ES cell mutants that also express this polypeptide are essentially indistinguishable from wild-type ES
cells.
Interestingly, the undifferentiated vinculin (/
) D7
null mutant was able to assemble talin-containing focal adhesions and stress fibers, although the morphology of the
structures formed was distinctly different from those in
wild-type ES cells. Others have previously reported that
vinculin is not essential to focal adhesion assembly. A
mouse F9 teratocarcinoma vinculin (
/
) mutant (Volberg et al., 1995
), as well as immortalized cells from vinculin (
/
) mouse embryos (Xu et al., 1998) were both able
to assemble focal adhesions in the absence of vinculin, although microinjection of antibodies to vinculin disrupted
focal adhesions in chick embryo fibroblasts (Westmeyer et
al., 1990
), and antisense RNA downregulation of vinculin
in BALB/c 3T3 cells reduced the number and size of focal
adhesions (Rodriguez Fernandez et al., 1993). The finding that vinculin, which can bind both talin (Gilmore et al.,
1992
) and F-actin (Huttelmaier et al., 1997
) is not essential
to focal adhesion assembly, and the fact that cells expressing little (Rodriguez Fernandez et al., 1992) or no vinculin
(Coll et al., 1995
) are more motile, suggests a role in stabilising focal adhesions rather than in assembly. The proline-rich region in vinculin contains a binding site for VASP
(Brindle et al., 1996
), a protein that can bind profilin (Reinhard et al., 1995
). Since profilin binds to G-actin and catalyses the exchange of ADP for ATP (Goldschmidt-Clermont et al., 1992
), it is possible that vinculin also facilitates
talin-mediated actin nucleation by recruiting a VASP/profilin/G-actin/ATP complex. We anticipate that the ability
to express both wild-type and mutant talin and vinculin
polypeptides in the ES cell mutants described here should
allow us to address these various possibilities.
![]() |
Footnotes |
---|
Received for publication 2 January 1998 and in revised form 9 June 1998.
The work was supported by the Medical Research Council and the Wellcome Trust.The authors are grateful to Mr. Paul E. Fraylich for technical assitance, to Dr. D. Melton (University of Edinburgh) for the HM1 clone of ES cells, to Dr. W. Colledge (University of Cambridge) and Dr. C. Pritchard (University of Leicester) for advice on the design of targeting constructs, and to Dr. R.O. Hynes (MIT, Cambridge, MA) for advice on ES cell electroporation.
![]() |
Abbreviations used in this paper |
---|
ANOVA, analysis of variance; ES cell, embryonic stem cell; Hyg, hygromycin; LIF, Leukemia inhibitory factor; Neo, neomycin; nt, nucleotides; TK, thymidine kinase.
![]() |
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