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J. Biol. Chem., Vol. 276, Issue 39, 36163-36167, September 28, 2001
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From the Department of Physiology, University of Tennessee Health
Science Center, Memphis, Tennessee 38163 and the
Received for publication, July 25, 2001, and in revised form, August 8, 2001
We have previously shown that tyrosine
phosphorylation of the actin-regulatory protein villin is accompanied
by the redistribution of phosphorylated villin and a concomitant
decrease in the F-actin content of intestinal epithelial cells. The
temporal and spatial correlation of these two events suggested that
tyrosine phosphorylation of villin may be involved in the rearrangement
of the microvillar cytoskeleton. This hypothesis was investigated by
analyzing the effects of tyrosine phosphorylation of villin on the
kinetics of actin polymerization by reconstituting in vitro
the tyrosine phosphorylation of villin and its association with actin.
Full-length recombinant human villin was phosphorylated in
vitro by expression in the TKX1-competent cells that carry an
inducible tyrosine kinase gene. The actin-binding properties
of villin were examined using a co-sedimentation assay. Phosphorylation
of villin did not change the stoichiometry (1:2) but decreased the
binding affinity (4.4 µM for unphosphorylated
versus 0.6 µM for phosphorylated) of villin for actin. Using a pyrene-actin-based fluorescence assay, we
demonstrated that tyrosine phosphorylation had a negative effect on
actin nucleation by villin. In contrast, tyrosine phosphorylation
enhanced actin severing by villin. Electron microscopic analysis showed
complementary morphological changes. Phosphorylation inhibited the
actin bundling and enhanced the actin severing functions of villin.
Taken together our data show that tyrosine phosphorylation of villin
decreases the amount of villin bound to actin filaments, inhibits the
actin-polymerizing properties of villin, and promotes the
actin-depolymerizing functions instead. These observations suggest a
role for tyrosine phosphorylation in modulating the microvillar
cytoskeleton in vivo by villin in response to specific
physiological stimuli.
Villin, an epithelial cell-specific protein, belongs to a family
of actin-severing and -capping proteins, which includes gelsolin, severin, fragmin, and CapG among others. Villin is unique among this
family of proteins in that it can also cross-link and bundle actin
filaments. We have previously shown that villin is
tyrosine-phosphorylated both in intestinal epithelial cells (1) and
in vitro (2). Since our first demonstration of tyrosine
phosphorylation of villin, other proteins of this family, including
gelsolin, have been reported to be tyrosine-phosphorylated in
vitro (3). Thus, tyrosine phosphorylation may also be a common
feature of this family of proteins, and phosphorylation may play an
important role in the organization of the actin network by these
actin-binding proteins. Previous in vivo work from our
laboratory shows that tyrosine phosphorylation of villin is accompanied
by a decrease in the F-actin content of the cell (4). However, a causal
relationship between tyrosine phosphorylation and changes in the
distribution and/or kinetics of actin polymerization remains to be established.
In addition to actin, villin interacts with several signaling molecules
including phosphatidylinositol 4,5-bisphosphate (5), Ca2+ (6), and phospholipase C- In the present study, we have used the approach of reconstitution
in vitro to investigate the role of tyrosine phosphorylation of villin in the regulation of its actin-modifying functions. The
complexity of the various actin-remodeling abilities of villin makes
such an approach most useful in dissecting the in vivo
effect of villin phosphorylation on the actin network. Using
recombinant phosphorylated
(VILT/WT)1 or
unphosphorylated (VIL/WT) villin, we show that tyrosine phosphorylation promotes the actin-severing rather than actin-polymerizing
functions of villin. The results of our studies allow us to
propose a more general model for the actin-regulatory activities of
other villin-like proteins that are known to be
tyrosine-phosphorylated.
Materials--
Monoclonal antibodies to villin were from
Transduction Laboratories; monoclonal antibodies to phosphotyrosine,
clone PY20, were from ICN; glutathione-Sepharose 4B Fast Flow was from
Amersham Pharmacia Biotech; GelCode Blue was from Pierce; BL21 and TKX1 competent cells were from Stratagene. The non-muscle actin
polymerization kit and the actin-binding kit were purchased from
Cytoskeleton (Denver, CO). Carbon-coated Formvar grids were purchased
from EM Science.
Tyrosine Phosphorylation of Villin in TKX1
Cells--
Full-length villin cDNA (human) cloned in pGEX-2T was
expressed in the Epicurian coli TKX1 cells as described
earlier (2). Briefly, TKX1 cells carry a plasmid with the Elk
tyrosine kinase (tk) gene controlled by the trp
promoter. The Elk tyrosine kinase has broad specificity and has been
shown to tyrosine phosphorylate a number of proteins in E. coli (10, 11). A two-step protocol involving first the induction
of expression of villin protein gene (by addition of
isopropyl- Cosedimentation of Phosphorylated and Unphosphorylated
Villin--
F-actin (non-muscle, 3 µM) was incubated
with varying concentrations of VILT/WT or VIL/WT (0-2
µM) in the presence of 2 mM EGTA. F-actin was
incubated with villin for 10 min at room temperature and sedimented for
15 min at 200,000 × g in a Beckman TL100
Ultracentrifuge. The supernatant was acetone-precipitated with 2 volumes of acetone. The pellet and the acetone-precipitated proteins
were resuspended in Laemmli sample buffer and analyzed by SDS-PAGE. The
amount of villin that sedimented with F-actin was compared with the
total amount of the protein. Trapping of soluble proteins in the pellet was estimated by sedimenting F-actin in the presence of bovine serum
albumin (2 µM) and was less than 1%. Similarly, the
amount of villin sedimenting in the absence of F-actin was negligible. The acrylamide gels were stained with GelCode Blue, and the proteins were quantified using the Stratagene Eagle Eye II system. Densitometric analysis was done using the software Scion Image.
Measurement of Actin Polymerization Kinetics by Phosphorylated
and Unphosphorylated Villin Using Fluorescence Spectroscopy--
The
kinetics of actin polymerization was determined using a non-muscle
actin polymerization kit according to the instructions of the
manufacturer and as described previously (2). The basis of this assay
is that the fluorescence intensity of pyrene actin is much greater for
polymeric than for monomeric actin (12). The ability of villin
to nucleate actin assembly or to sever actin filaments was determined
by its effect on the rate and extent of increase or decrease,
respectively, of fluorescence of pyrene-labeled actin. Fluorescence
measurements were performed at 25 °C using the
Fluorolog-3-Fluorometer. The excitation wavelength was set at 365 nm,
and the emission wavelength was set at 388 nm.
Critical Concentration of Actin Polymerization--
We first
measured the concentration of G-actin required for polymerization
(critical concentration) in the absence or presence of VIL/WT or
VILT/WT. Pyrene G-actin was polymerized at room temperature for 40 min
in actin polymerization buffer (5 mM Tris-HCl, pH 7.0, 150 mM KCl, 1 mM MgCl2, 0.2 mM CaCl2, 0.2 mM ATP) and then
diluted to different concentrations in the presence or absence of
equimolar concentrations of villin. After an 8-h incubation at room
temperature, the fluorescence intensity was measured.
Nucleation of Actin Polymerization--
G-actin (6 µM) in buffer containing 5 mM Tris-HCl, pH
7.0, 0.2 mM ATP, and 0.2 mM CaCl2
was preincubated with VIL/WT or VILT/WT (60 nM) for 10 min
on ice. Polymerization was induced by the addition of 150 mM KCl and 1 mM MgCl2. The increase
in fluorescence that occurs when pyrene G-actin forms pyrene F-actin
was measured over time. The rate at which actin polymerizes depends on
the concentrations of free actin monomers and the filament ends.
Because villin complexes with G-actin faster than spontaneous actin
nuclei can form, the initial rate of polymerization determined from the
rate of fluorescence increase is proportional to the number of
pointed-end nuclei formed and, therefore, the relative nucleation
activity of villin (12). To test the nucleating activity of VIL/WT and
VILT/WT, we measured their effects on the initial phase of actin
polymerization. The increase in fluorescence was recorded every 5 s.
Severing of Actin Filaments--
For assays of filament-severing
activity, a sample of pyrene-labeled F-actin was diluted below its
critical monomer concentration into solutions containing villin (60 nM). Because actin filaments depolymerize only from their
ends, the rate of fluorescence decrease, proportional to the
depolymerization rate, depends on the number of ends and therefore on
the number of cuts introduced by villin (12). To compare the severing
activity of VIL/WT and VILT/WT, we measured the decrease in
fluorescence/min in the linear range of the curve as described
previously (8). The decrease in fluorescence was recorded every 2 s.
Electron Microscopic Analysis of Bundling and Severing
Activities--
To test the bundling activity, G-actin in buffer
containing 5 mM Tris-HCl, pH 8.0, 0.2 mM ATP,
and 0.2 mM CaCl2 was polymerized by the
addition of 150 mM KCl and 1 mM
MgCl2 for 1 h at 20 °C. F-actin (3 µM) was incubated overnight at 4 °C with VIL/WT or VILT/WT (1.5 µM) in the presence of EGTA (2 mM). To study severing, incubation of 2 mM
F-actin and 0.7 mM VIL/WT or VILT/WT was performed for 1 min in the presence of 1 mM CaCl2 at 20 °C.
Samples were applied to carbon-coated Formvar grids. Excess sample was
carefully withdrawn, and the grids were stained with 2% aqueous uranyl
acetate after a brief fixation in 2% glutaraldehyde. For actin
bundling studies, samples were diluted 1:1 in actin polymerization
buffer immediately before applying the samples to the grids.
Grids were examined at 60 kV in a JEOL 2000 EX-II electron microscope.
Tyrosine Phosphorylation Decreases the Affinity of Villin for
F-actin--
The present work examines how villin and its
phosphorylation may contribute to the regulation of actin dynamics.
The finding that tyrosine phosphorylation of villin in
intestinal epithelial cells coincides with the redistribution of villin
from the actin cytoskeleton to the plasma membrane (1, 4) suggested
that perhaps tyrosine phosphorylation regulates the actin binding
properties of villin. To test this hypothesis, we first examined
whether the actin binding activity of villin was regulated by
phosphorylation. The binding affinity of villin for F-actin was
determined by co-sedimentation experiments performed in the presence of
villin (phosphorylated or not) and in the absence of Ca2+.
Full-length human recombinant villin was purified from TKX1 cells
either as a phosphorylated (VILT/WT) or unphosphorylated (VIL/WT)
protein (Fig. 1A). We had
previously demonstrated that full-length recombinant villin
demonstrates all the actin modifying properties of the native protein
(purified from chicken brush border) (2), thus allowing us to
reconstitute in vitro the kinetics of actin polymerization
by villin. Purified recombinant proteins (0-2 µM) were
mixed with polymerized filamentous actin (3 µM) and then
subjected to high-speed centrifugation. The partitioning of villin and
actin between the supernatant and pellet fractions was analyzed by
GelCode Blue staining and densitometry. The amount of villin bound to
actin was plotted against the total villin concentration; the
stoichiometry of binding and the ka values of the
interaction between villin and F-actin were calculated by
assuming a sigmoidal relationship between total villin concentration and villin bound to actin filaments (Hill equation). The stoichiometry of villin to actin was 1:2, consistent with two actin-binding sites/molecule of villin (13). Co-sedimentation experiments revealed
that the stoichiometry of villin-actin binding remained unchanged by
phosphorylation. However, tyrosine phosphorylation decreased the
binding affinity of villin for actin (Fig. 1B). Using the
Hill analysis, the binding affinity constant (ka) value for VIL/WT was 4.40 ± 0.30 µM
versus a ka value for VILT/WT of
0.60 ± 0.01 µM. These data show that
phosphorylation of villin decreases the amount of villin bound to actin
filaments and imply that the affinity of villin for actin could be
locally modulated by phosphorylation. In intestinal epithelial cells, tyrosine-phosphorylated villin is detergent soluble (1). A decrease in
the binding affinity of phosphorylated villin for actin filaments may
partially explain the redistribution of tyrosine phosphorylated villin
in vivo. Our studies so far suggest that phosphorylation may
be a signal for intracellular translocation of villin. Alternatively,
it could be the first step leading to the dissociation of the
villin-actin complex.
Tyrosine Phosphorylation Decreases the Actin-nucleating and
Increases the Actin-severing Functions of Villin--
Because the
phosphorylated villin retained its ability to bind to F-actin, we
wanted to determine whether phosphorylation would affect the nucleating
activity of villin. We investigated the influence of villin
phosphorylation on the kinetics of actin polymerization. First, the
concentration of G-actin required for polymerization (critical
concentration) in the presence of VIL/WT and VILT/WT was determined.
Fluorescence measurements were made at steady state to determine
polymer concentration as a function of total actin concentration.
Tyrosine phosphorylation led to a very small change in the critical
concentration of actin required for polymerization in the presence of
villin (0.10 ± 0.008 µM for VIL/WT
versus 0.15 ± 0.005 µM for VILT/WT). We
next determined the actin nucleating activity of VIL/WT and VILT/WT. In
comparison with the polymerization kinetics of actin alone (control),
the addition of VIL/WT (60 nM) in the presence of 20 mM Ca2+ abolished the lag phase and increased
the initial rate of actin polymerization (Fig.
2A). In contrast, VILT/WT
resulted in a lag phase and decreased the rate of actin polymerization.
It was noted that although actin polymerized in the presence of
VILT/WT, phosphorylation significantly reduced the nucleating ability
of villin (74.7 ± 2.5% with VIL/WT versus 39.2 ± 1.3% with VILT/WT). There was no change in actin nucleation in the
presence of GST (data not shown). These data show that phosphorylation
of villin inhibits its actin nucleating activity. Further, they suggest
that tyrosine phosphorylation may decrease the ability of villin to
initiate the formation of F-actin filaments in vivo, thus
leading to the reorganization of the actin cytoskeleton.
Next, we examined the effect of tyrosine phosphorylation of villin on
F-actin depolymerization. Pyrene F-actin (1 µM) in the presence of either VIL/WT or VILT/WT (60 nM) was diluted to
a concentration of 0.1 µM, and the fluorescence intensity
was monitored over time. VIL/WT significantly increased the
depolymerization of F-actin compared with control (43.7 ± 3.2%
versus 12.9 ± 0.9%, respectively; n = 9, p < 0.01). Furthermore, phosphorylation of villin
increased its actin-depolymerizing property. Fluorescence measurements
show a 22% (n = 9, p < 0.01) increase
in actin severing by VILT/WT compared with VIL/WT. These results are
consistent with an increase in the actin depolymerizing function of
phosphorylated villin. These data support our hypothesis that tyrosine
phosphorylation of villin and a decrease in the intestinal cell F-actin
content are not mutually exclusive.
Tyrosine Phosphorylation Alters the Actin Filament
Organization--
To further explore the correlation between
phosphorylation and regulation of the actin-modulating properties of
villin, we examined the effects of VIL/WT and VILT/WT on actin
filament morphology. Actin polymerized in the absence of villin shows
long, curved F-actin filaments that are not cross-linked (Fig.
3A). In the presence of
saturating amounts of VIL/WT relative to actin (villin:actin, 1:2) and
in the absence of Ca2+, VIL/WT organizes the F-actin
filaments into long, straight, closely aligned, well organized, tight
bundles (Fig. 3, B and B'). In contrast,
phosphorylation of villin led to reorganization of the actin filaments,
which now showed thicker bundles, which at higher magnification
appeared to have loose, poorly organized filament structure. The
bundles showed no distinct alignment of filament but contained loosely
packed filaments with some associated electron dense material (Fig.
3C'). There was also an appreciable decrease in the average
length of the filaments (Fig. 3C). Thus, although VILT/WT
can bind actin filaments albeit with lower binding affinity for actin,
it does not bundle filaments like VIL/WT. Negative charges exposed on
the surface of the actin filaments favor their alignment into bundles,
and polyanions can disintegrate actin bundles into single filaments
(14). Basic amino acids in villin have been shown to promote villin
binding to actin (15). This may explain why introduction of negative
charges by phosphorylation weakens villin-actin interactions, and the
phosphorylated villin shows poor bundling activity.
We next obtained electron micrographs of the actin-severing functions
of villin. In the presence of Ca2+ and the absence of
villin, the morphology of actin filaments is indistinguishable from
pure actin filaments seen in the presence of EGTA (compare Figs.
4A and 3A). In the
presence of Ca2+, the addition of VIL/WT to F-actin severs
actin filaments (Fig. 4B). The filaments are much shorter
than those observed in preparations of pure actin (Fig.
4B'). In contrast, the addition of VILT/WT has a profound
effect on actin morphology. In samples briefly (1 min) treated with
VILT/WT, no actin filaments were observed. The samples contained
fibrillar material, which at higher magnification showed very small
filamentous fragments of heterogeneous size (Fig. 4C').
Because VILT/WT does not significantly elevate the critical
concentration for actin assembly, the obvious conclusion from these
morphological studies is that phosphorylation promotes actin
disassembly through fragmentation of filaments into small pieces rather
than through depolymerization. Interestingly, in anoxic proximal tubule
a coincident microvillar actin bundle disruption was shown to be
associated with severing of actin bundles rather than depolymerization
of F-actin (16). Tyrosine phosphorylation of villin could explain such
severing of actin bundles during anoxia.
Analysis of the actin polymerization kinetics in the presence of
tyrosine phosphorylated villin revealed that tyrosine
phosphorylation promotes the actin disassembling properties rather than
assembling properties of villin. In vivo,
tyrosine-phosphorylated villin may dissociate actin bundles and promote
severing, thus leading to a breakdown of the microvillar network.
Phosphorylated villin could prevent actin assembly by distinct
mechanisms including lower binding affinity for F-actin, inhibiting
nucleation of new filaments, and cutting pre-existing filaments.
Phosphorylation of villin and a local decrease in the affinity of
villin for actin could generate a dynamic state and an increase in the
fluidity of the cytoskeleton. A decrease in the affinity of villin for actin could also affect the mechanical properties of the actin cytoskeleton. For instance it is known that a change in the affinity of
cross-linkers for actin could change the cytoplasm from a solid to a
fluid and thus from a rigid to a dynamic network. These temporal changes in the physical properties of the cytoskeleton could enhance cell motility, which might clarify the role of villin in
intestinal restitution, for example (17, 18).
The structural and functional relationships between tyrosine
phosphorylation of villin and actin polymerization kinetics are likely
to extend to other actin-binding proteins. Identification of the
tyrosine phosphorylation sites in villin will be instructive in
understanding the structural basis of actin filament modifying activities and the relationship of phosphorylation with these functions, in both villin and other proteins that share sequence homology with villin. The kinetics of filament assembly may be a
function of not only the concentrations of various intracellular messengers such as Ca2+ and phosphatidylinositol
4,5-bisphosphate but also the phosphorylation state of actin regulatory
proteins. The actin-binding proteins may be novel substrates for
tyrosine kinases, also suggesting that these proteins may target
signaling molecules to effector sites as well as recruit actin
complexes to modify the cytoskeleton at these sites. Interestingly,
phosphorylation (serine/threonine phosphorylation) of the few
actin-binding proteins studied so far demonstrates a decrease in the
actin binding affinities, or actin bundling properties, and/or decrease
in the nucleation of actin (19, 20). Thus, phosphorylation, whether on
serine, threonine, or tyrosine residues in the actin-modifying
proteins, appears to be a negative regulator of actin assembly.
Phosphorylation of villin suggests that filament turnover in cells may
be defined by the regulated action of actin-binding proteins
interacting with signaling molecules. Thus, the cell may use villin
phosphorylation as an important regulatory switch to modify the actin
cytoskeleton in the epithelial microvillar core.
*
This work has been supported by grants from the American
Digestive Health Foundation (Industry Research Scholar award) and the
NIDDK, National Institutes of Health (DK-54755) (to S. K.).The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
§
To whom correspondence should be addressed: Dept. of Physiology,
University of Tennessee Health Science Center, Nash 402, 894 Union
Ave., Memphis, TN 38163. Tel.: 901-448-3410; Fax: 901-448-3505; E-mail: skhurana@utmem.edu.
Published, JBC Papers in Press, August 10, 2001, DOI 10.1074/jbc.C100418200
The abbreviations used are:
VILT/WT, full-length
recombinant human tyrosine-phosphorylated villin;
VIL/WT, full-length
recombinant human villin;
GST, glutathione S-transferase;
IAA, 3-
Tyrosine Phosphorylation of Villin Regulates the Organization of
the Actin Cytoskeleton*
, and Department of Biophysics and Biophysical Chemistry, Johns
Hopkins University, Baltimore, Maryland 21205
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
REFERENCES
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
REFERENCES
1 (1, 2).
Tyrosine phosphorylation of villin and its ligand binding properties
suggest that in addition to its role in regulating the actin
cytoskeleton, villin may also be a regulatory target. Thus, villin may
function as a structural scaffold for signaling proteins or participate
in translating cell surface receptor-mediated biochemical reactions to
the cell movement machinery. Severing of actin filaments and nucleation of actin polymerization are essential for the remodeling of the cortical actin network that accompanies nearly all types of cell activation. Precise actin cytoskeleton remodeling requires tight spatial and temporal regulation of actin filament assembly and organization. Cells accomplish this by stimulating or inhibiting the
activity of several actin-associated proteins. The actin-modifying properties of these proteins are regulated by several different factors
including calcium (6), phospholipids (5), pH (7), and
serine/threonine phosphorylation (8, 9). In recent years several
actin-regulatory proteins have been shown to be
tyrosine-phosphorylated, adding yet another level of regulation. Less
well characterized are the tyrosine phosphorylation of these proteins
and the effect of phosphorylation on the actin-modifying properties of
these proteins.
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
REFERENCES
-D-thiogalactopyranoside followed by induction
of the tk gene (by addition of 3-indoleacrylic acid (IAA)), allowed for the accumulation of GST-tagged
tyrosine-phosphorylated villin (VILT/WT). TKX1 cells cultured in the
absence of IAA were used to obtain unphosphorylated villin (VIL/WT).
VIL/WT and VILT/WT were affinity purified from bacterial lysates using
glutathione-Sepharose 4B columns. The proteins were eluted with 5 mM glutathione in 1-ml fractions. Purity of the
fractions was assessed by SDS-PAGE and staining with GelCode Blue.
Tyrosine phosphorylation of villin was determined by Western analysis
of the samples using phosphotyrosine monoclonal antibodies. This method
is an alternative to in vitro phosphorylation of recombinant
villin by c-src, and we have previously shown that villin
phosphorylated by either method behaves similarly (2). Several
advantages of using the TKX1 cells compared with in vitro
phosphorylation by c-src include the following: (i) one relatively simple purification protocol allows us to obtain recombinant tyrosine phosphorylated villin; (ii) in vitro
phosphorylation by c-src is less efficient in that it
requires additional chromatographic steps to separate phosphorylated
from unphosphorylated villin; (iii) the culture of TKX1 cells in the
presence or absence of IAA allows us to purify both phosphorylated and
unphosphorylated villin simultaneously.
RESULTS AND DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
REFERENCES
View larger version (25K):
[in a new window]
Fig. 1.
Phosphorylation negatively regulates the
binding of villin to actin. A, recombinant human villin
phosphorylated (VILT/WT) or unphosphorylated
(VIL/WT) was purified from TKX1 cells as described under
"Experimental Procedures." This is an immunoblot of VIL/WT and
VILT/WT with monoclonal antibodies to phosphotyrosine (upper
panel) or villin (lower panel). This blot is
representative of three blots with similar results. B,
increasing amounts of villin (VIL/WT or VILT/WT) were added to
prepolymerized actin (3 µM). The samples were incubated
for 10 min at 25 °C and then subjected to high-speed centrifugation.
The supernatant and pellet fractions were separated by SDS-PAGE, and
the partitioning of villin between the supernatant and pellet fractions
was determined by GelCode Blue staining. The gels were analyzed by
densitometry, and the percentage of villin in the pellet relative to
the total amount of villin was calculated for each sample. Bound villin
was plotted as a function of total villin. Data are the mean of three
experiments and are fitted with the Hill equation.
View larger version (14K):
[in a new window]
Fig. 2.
Effect of phosphorylated villin on actin
dynamics. A, effect of villin phosphorylation on
kinetics of actin polymerization. Pyrene G-actin (6 µM)
was incubated with VIL/WT or VILT/WT (60 nM) in
polymerization-inducing buffer, and fluorescence intensity was measured
over time. Control represents the polymerization of actin in
the absence of villin. Fluorescence was recorded every 5 s as
described under "Experimental Procedures." B, effect of
villin phosphorylation on actin depolymerization. Pyrene-F-actin (1 µM) in the presence of VIL/WT or VILT/WT (60 nM) was diluted to 0.1 µM in
actin-polymerizing buffer, and the decrease in fluorescence intensity
was followed over time. Control represents the
depolymerization of actin in the absence of villin. Fluorescence was
recorded every 2 s as described under "Experimental
Procedures." Values represent the mean of three independent
experiments.
View larger version (162K):
[in a new window]
Fig. 3.
Effect of phosphorylated villin on F-actin
bundling. Electron micrographic images of negatively stained
preparations containing F-actin, 2 mM EGTA, and purified
recombinant villin, phosphorylated (VILT/WT), or unphosphorylated
(VIL/WT). For actin bundling studies, samples were diluted 1:1 in actin
polymerization buffer (as described under "Experimental
Procedures") immediately before applying samples to the grids.
A, F-actin alone; B, VIL/WT; C,
VILT/WT. Arrows indicate electron-dense regions within the
microfilament bundle that are visible in the presence of VILT/WT.
A', B', and C' are electron
micrographs showing actin bundles visualized in A,
B, and C at a higher magnification.
Bars: 0.2 µM, same magnification for
A-C; 0.05 µM, same magnification for
A'-C'.
View larger version (144K):
[in a new window]
Fig. 4.
Effect of phosphorylated villin on F-actin
severing. Electron micrographic images of negatively stained
preparations containing F-actin, 1 mM CaCl2,
and purified recombinant villin, phosphorylated (VILT/WT), or
unphosphorylated (VIL/WT). To study severing, F-actin was incubated
with VIL/WT or VILT/WT for 1 min in the presence of 1 mM
CaCl2 at 20 °C. A, F-actin alone;
B, VIL/WT; C, VILT/WT. A',
B', and C' are electron micrographs showing actin
filaments visualized in A-C at a higher magnification.
Bars: 0.2 µM, same magnification for
A-C; 0.05 µM, same magnification for
A'-C'.
FOOTNOTES
ABBREVIATIONS
-indoleacrylic acid;
PAGE, polyacrylamide gel
electrophoresis.
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
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