Originally published In Press as doi:10.1074/jbc.M001124200 on April 14, 2000
J. Biol. Chem., Vol. 275, Issue 29, 22187-22195, July 21, 2000
A Kinesin Mutation That Uncouples Motor Domains and Desensitizes
the 
-Phosphate Sensor*
Katherine M.
Brendza
§,
Christopher A.
Sontag¶,
William M.
Saxton
, and
Susan P.
Gilbert**
From the Department of Biology, Indiana University,
Bloomington, Indiana 47405, the ¶ Department of Biochemistry,
University of Mississippi Medical Center, Jackson, Mississippi
39216-4505, and the ** Department of Biological Sciences, University of
Pittsburgh, Pittsburgh, Pennsylvania 15260
Received for publication, February 10, 2000, and in revised form, April 11, 2000
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ABSTRACT |
Conventional kinesin is a processive,
microtubule-based motor protein that drives movements of membranous
organelles in neurons. Amino acid Thr291 of
Drosophila kinesin heavy chain is identical in all
superfamily members and is located in 
-helix 5 on the
microtubule-binding surface of the catalytic motor domain. Substitution
of methionine at Thr291 results in complete loss of
function in vivo. In vitro, the T291M mutation disrupts the
ATPase cross-bridge cycle of a kinesin motor/neck construct, K401-4
(Brendza, K. M., Rose, D. J., Gilbert, S. P., and
Saxton, W. M. (1999) J. Biol. Chem. 274, 31506-31514). The pre-steady-state kinetic analysis presented here
shows that ATP binding is weakened significantly, and the rate of ATP
hydrolysis is increased. The mutant motor also fails to distinguish ATP
from ADP, suggesting that the contacts important for sensing the
-phosphate have been altered. The results indicate that there is a
signaling defect between the motor domains of the T291M dimer. The
ATPase cycles of the two motor domains appear to become kinetically
uncoupled, causing them to work more independently rather than in the
strict, coordinated fashion that is typical of kinesin.
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INTRODUCTION |
Structural analyses of kinesin (2-5) and family relatives Ncd (6,
7) and Kar3 (8) have revealed that the topography of the
nucleotide-binding pocket is quite similar to that of myosins and the G
proteins (9, 10). The results suggest further that these proteins may
share a common mechanism to sense the state of the nucleotide bound at
the active site and to respond through structural transitions to
communicate with protein partners. For dimeric kinesin, coordination of
the motor domains is controlled in part by the nucleotide state at the
active sites (11-13) and is required for the cyclic interaction with
the microtubule lattice for unidirectional, processive movement.
Through pre-steady-state kinetic analysis, it has been determined that
ATP binding by the microtubule-bound motor domain allows the partner
motor domain to bind to the microtubule and quickly release its ADP
(12-13). Other points of coordination are also evident. Thus, the two
motor domains of the kinesin heavy chain
(KHC)1 dimer are at different
stages in their ATPase cycles at any given time, keeping the heads out
of phase and allowing for processive movement (reviewed in Refs. 14 and
15).
Much has been learned about kinesin through structural studies. The
first motor domain structural intermediate to be determined was the
KHC·ADP intermediate (3-5). Recently, the structures of KHC under
conditions that mimic different nucleotide states were solved (16).
This work revealed that in the absence of microtubules there is little
change in KHC structure regardless of the nucleotide present. Thus,
with no existing structures of microtubule·kinesin intermediates, the
transition states important for efficient ATP hydrolysis remain
enigmatic. Because it is difficult to integrate mechanistic models with
the available information, alternative approaches are required to
understand the structural requirements for motor coordination and
processive movement.
Site-directed mutagenesis has already identified structural elements
that are important for certain aspects of KHC function. Studies by
Woehlke et al. (17) highlighted charged surface residues necessary for the interaction of KHC with microtubules. Romberg et al. (18) showed that the neck region of KHC is important for efficiency but is not essential for processive movement. They proposed a model in which interactions between the 
-sheet region of
the neck (9 and 10) and the catalytic domain are disrupted such
that the neck region could adopt a more extended conformation to allow
head separation during times when both heads are bound to the
microtubule. This hypothesis is supported by the cryo-EM diffraction
studies of microtubule·kinesin complexes by Hoenger et al.
(19).
Studies of mutant KHCs may help us understand both the ATPase mechanism
of kinesin and associated structural rearrangements that allow for
efficient utilization of the energy generated through ATP hydrolysis.
Moore et al. (20) determined that a point mutation in 6
of Ncd greatly reduces the affinity of the motor for microtubules and
reduces the velocity of microtubule-based movement. Song and Endow (21)
have shown that a point mutation in 4 of both Kar3 and Ncd uncouple
the nucleotide and microtubule-binding sites, perhaps due to a break in
Loop11-mediated communication between the two sites. Recent studies by
Rice et al. (22) have provided insight into structural
changes that may allow for force generation and plus end-directed
movement of KHC. They have shown that ATP binding promotes a large
conformational change in the kinesin neck linker that is directed
toward the plus end of the microtubule. These results with monomeric
kinesin K349 emphasize that there are conformational transitions in the
microtubule-bound kinesin dimer during ATP turnover that are beyond the
view of current crystallography efforts.
To gain insight into the mechanisms of kinesin mechanochemistry
in vivo, we screened for recessive lethal mutations in the kinesin heavy chain (Khc) that disrupt axonal transport (1, 23). One of the mutations found, Khc4, causes
in vivo phenotypes that suggest a nearly complete loss of
function. Sequencing revealed that there is a threonine to methionine
substitution at amino acid position 291, an almost completely conserved
residue in the kinesin
superfamily.2
Thr291 is located in -helix 5, which lies on the
microtubule-binding surface of the motor domain. The steady-state
ATPase kinetics showed that this mutation causes defects in both ATP
and microtubule binding. The kcat is very
similar to wild type, yet there is a 3-fold increase in both
Km, ATP and
K0.5, Mt (1). In an effort to determine more
precisely how this mutation alters the ATPase cycle and consequently
how Thr291 contributes to KHC mechanochemistry, we have
pursued a mechanistic analysis of K401-4.
The results provide direct evidence that ATP binding is significantly
weakened by the T291M mutation and that the binding pocket has lost the
ability to distinguish ATP from ADP. These data suggest that structural
arrangements important for sensing the -phosphate have been
disrupted. Furthermore, the kinetics indicate that the two motor
domains of the mutant dimer are defective in their head-head
communication. Thus, the T291M substitution allows the motor domains to
work more independently rather than in the strictly coordinated fashion
that is characteristic of kinesin.
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EXPERIMENTAL PROCEDURES |
Materials--
[-32P]ATP (>3000 Ci/mmol) was
from NEN Life Science Products; polyethyleneimine-cellulose TLC plates
(EM Science of Merck, 20 × 20 cm, plastic-backed) were from VWR
Scientific (Bridgeport, NJ); Taxol (Taxus brevifolia) was
from Calbiochem-Novabiochem; ATP, GTP, AMP-PNP, and S-Sepharose were
from Amersham Pharmacia Biotech (Uppsala, Sweden); Bio-Rad Protein
Assay, ovalbumin, IgG, and DEAE-Sephacel were from Bio-Rad.
Protein Purification--
K401-4 was bacterially expressed,
purified, and characterized as described previously (1). Six
preparations of K401-4 were used in the experiments reported, and each
was evaluated to determine the steady state parameters:
kcat = 18 ± 0.6 s
1, Km, ATP = 224 ± 4.9 µM, and K0.5, Mt = 3.6 ± 0.01 µM. All experiments reported were
performed in ATPase buffer (50 mM HEPES, pH 7.2, with KOH,
5 mM magnesium acetate, 0.1 mM EGTA, 0.1 mM EDTA, 50 mM potassium acetate) at
25 °C.
Analytical Ultracentrifugation--
Experiments were conducted
at 42,000 rpm in a Beckman Optima XLA analytical ultracentrifuge
equipped with absorbance optics and an An60Ti rotor. ATPase buffer was
used at 24.7 °C. Velocity data were analyzed using DCDT+, version
1.12 (25). The reported weight average sedimentation coefficient values
(
20, w) obtained from
DCDT+ are corrected for the solution density and viscosity (26) and are
calculated by a weighted integration over the entire range of
sedimentation coefficients covered by the g(s)
distribution. To verify these results, the data were also analyzed with
DCDT (27) and, where appropriate, SVEDBERG, version 6.37 (28).
Microtubule Preparation for the Kinetic
Experiments--
Purified tubulin was cold-depolymerized and clarified
the morning of each experiment. Microtubules were assembled by the
addition of taxol to 20 µM. The microtubules were
collected by centrifugation, and the microtubule pellet was resuspended
in ATPase buffer plus 20 µM taxol to stabilize the
microtubules (29). For all of the experiments in which microtubules
were present, 20 µM taxol was included to maintain the
polymer state.
Stopped-flow Experiments--
The pre-steady-state kinetics of
mantATP binding, mantADP release, K401 binding to microtubules, and
detachment of K401 from microtubules were measured using a KinTek
StopFlow Instrument (SF-2001, KinTek Corp., Austin, TX) at
25 °C in ATPase buffer. N-methylanthraniloyl fluorescence
(mantATP and mantADP) was excited at 360 nm (mercury arc lamp)
and detected after being passed through a 400-nm cut-off filter.
mantATP binding data in Fig. 1B were fit to the
equation,
![k<SUB><UP>obs</UP></SUB>=k<SUB>+1</SUB>[<UP>mantATP</UP>]+k<SUB>−1</SUB>](/content/vol275/issue29/fulltext/22187/img002.gif)
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(Eq. 1)
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where kobs is the rate constant obtained
from the exponential phase of the fluorescence change,
k+1 defines the second order rate constant for
mantATP binding, and k1 corresponds to the
observed rate constant of mantATP release as determined by the
y intercept. The dissociation kinetics of Mt·K401 complex and association kinetics of K401 with microtubules were determined by
the change in turbidity monitored at 340 nm. All concentrations reported are final after mixing. For Fig. 3B, the observed
rate constants of microtubule association were fit to the
equation,
![k<SUB><UP>obs</UP></SUB>=k<SUB>+5</SUB>[<UP>tubulin</UP>]+k<SUB>−5</SUB>](/content/vol275/issue29/fulltext/22187/img003.gif)
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(Eq. 2)
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where kobs is the rate constant obtained
from the fast, exponential phase, k+5 defines
the second order rate constant for microtubule association, and
k5 corresponds to the observed rate constant
of motor dissociation as determined by the y intercept.
Rapid Quench Experiments--
The pre-steady-state experiments
to determine the rate constant of ATP hydrolysis were performed with a
rapid chemical quenched-flow instrument (KinTek Corp., Austin, TX) at
25 °C in ATPase buffer as described previously (30). For each time
point, a preformed Mt·K401 complex (10 µM K401, 25 µM tubulin, 20 µM taxol; final concentrations after mixing) was reacted with
[-32P]ATP for times ranging from 5 to 400 ms. The
reaction mixture was then quenched with 4 N HCl and
expelled from the instrument. Chloroform (100 µl) was added
immediately to the reaction mix to denature the protein, followed by
neutralization (pH 7-7.8) by the addition of 2 M Tris, 3 M NaOH. The acid quench stops the reaction and denatures
the protein; therefore, the product formed is the sum of three
intermediates:
K·[-32P]ADP·Pi,
K·[-32P]ADP, and
[-32P]ADP released from the active site. The
concentration of product ([-32P]ADP) was plotted as a
function of time, and the data were fit to the burst equation,
![<UP>Product</UP>=A∗[1−<UP>exp</UP>(<UP>−</UP>k<SUB>b</SUB>t)]+k<SUB>ss</SUB>t](/content/vol275/issue29/fulltext/22187/img004.gif)
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(Eq. 3)
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where A is the amplitude of the burst, representing
the formation of [-32P]ADP·Pi at the
active site; kb is the rate constant of the
pre-steady-state burst; kss is the rate constant of
the linear phase, corresponding to steady-state turnover; and t is the time in seconds.
Molecular Modeling--
All molecular modeling was performed on
a Silicon Graphics workstation using UCSF MidasPlus Molecular
Interactive Display and Simulation software (Computer Graphics
Laboratory, University of California, San Francisco, CA).
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RESULTS |
Pre-steady-state Kinetics of mantATP Binding--
To explore the
apparent weak binding of ATP by K401-4 revealed by the steady-state
Km, ATP (1), we began the
pre-steady-state kinetic analysis by measuring the kinetics of ATP
binding and ATP hydrolysis (Figs. 1 and
2). For the ATP binding studies, the
fluorescent ATP analog mantATP was used (Fig. 1). This analog has been
used in previous characterizations of kinesin motors and has been shown
experimentally to be a good ATP analog because of the fluorescence
enhancement and similarity to ATP (31, 32). For K401-wt, the
microtubule-activated steady-state kcat reported
was 19 s1 for both ATP and mantATP with
the Km, ATP = 62 µM and
Km, mantATP = 150 µM
(32). The preformed Mt·K401-4 complex (30 µM
microtubules, 10 µM K401-4) was rapidly mixed with
varying concentrations of mantATP in the stopped-flow apparatus, and
the change in fluorescence was monitored. A representative stopped-flow
record is shown in Fig. 1A. Binding of mantATP causes a
biphasic fluorescence transient with a rapid exponential increase in
fluorescence (associated with mantATP binding) followed by a
significantly slower exponential decrease in fluorescence. The observed
decrease in fluorescence is independent of substrate concentration
(kobs = 3.1-3.8 s1)
and is not fast enough to be attributed to ATP hydrolysis. This biphasic fluorescence transient is characteristic of kinesin and has
been observed by others (34, 36). The smooth line is the best fit of
the data to a double exponential, providing kobs
of the initial, fast reaction at 135 s1. The
rate of the fast exponential phase increased as a function of ATP
concentration, and the data were fit to Equation 1 (Fig. 1B). The slope of the line provided the second order rate
constant for mantATP binding, k+1 = 1 µM1
s1, which is similar to the observed rate
constant for K401-wt at 2 µM1
s1 (30, 34). The y intercept
predicts an off rate for mantATP with k1 = 157 s1.
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Fig. 1.
Kinetics of ATP binding. The preformed
Mt·K401-4 complex (30 µM tubulin, 10 µM
K401-4) was rapidly mixed in the stopped-flow apparatus with varying
concentrations of mantATP (20-200 µM). A, a
representative stopped-flow record (average of seven individual traces)
from an experiment at 20 µM mantATP. An increase in
fluorescence was observed, and the smooth line is
the fit of the data to a double exponential. The observed rate of the
initial fast exponential phase was 135 ± 4.3 s1. The slow, declining phase at 3.1 ± 0.9 s1 is too slow to be ATP hydrolysis and
is believed to represent an isomerization after initial mantATP
binding. B, the observed rate constant of the initial, fast
phase increased linearly with increasing mantATP concentration. The
data were fit to Equation 1, and the slope provides the apparent second
order rate constant for mantATP binding, k+1 = 1 ± 0.1 µM1
s1, and the y intercept provides
the off-rate, k1 = 157 ± 11.8 s1 (Scheme 1).
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Fig. 2.
Kinetics of ATP hydrolysis. A preformed
Mt·K401-4 complex (10 µM K401-4, 25 µM
tubulin) was rapidly mixed with varying concentrations of
[-32P]MgATP in a chemical quenched-flow instrument.
The reaction times varied from 5 to 400 ms, and the data were fit to
the burst equation (Equation 3). A, the transients for ATP
hydrolysis in the presence of 100 µM ( ), 200 µM ( ), 300 µM ( ), 400 µM ( ), 500 µM ( ), and 600 µM ( ) [-32P]MgATP. Only the first 200 ms of each transient are shown to expand the time domain of the initial
burst phase. B, the rate constants (kb)
of the pre-steady-state burst phase determined from each transient in
A were plotted as a function of [-32P]MgATP
concentration. Data from other experiments were included in this plot.
The fit of the data to a hyperbola provides the maximum rate constant
for the burst phase, kb = 257 ± 30 s1 and
Kd, ATP = 236 ± 62 µM. At high ATP concentrations, ATP binding no longer
limits the first order reaction of ATP hydrolysis; therefore, the rate
constant for ATP hydrolysis (k+2) = 257 ± 30 s1 (Scheme 1).
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Pre-steady-state Kinetics of ATP Hydrolysis--
We next measured
the kinetics of ATP hydrolysis for K401-4 through a series of acid
quench experiments (Fig. 2). The preformed Mt·K401-4 complex (25 µM microtubules, 10 µM K401-4) was rapidly mixed with [-32P]MgATP in the chemical quench
instrument. Fig. 2A shows the time course of ATP hydrolysis
by K401-4 at six different ATP concentrations. Each transient was
biphasic with an initial exponential rate of ADP·Pi
formation (the burst), followed by a slower rate of product formation
(the linear phase) corresponding to steady-state turnover. The
exponential burst of product formation at the active site indicates
that a step after ATP hydrolysis is rate-limiting for K401-4 as
observed for K401-wt (30). At high ATP concentrations, ATP binding
becomes faster than ATP hydrolysis. Because substrate binding is no
longer limiting, the maximum rate constant for the exponential burst
phase is the rate constant of ATP hydrolysis. The rate constant for ATP
hydrolysis (k+2 = 257 s1) was determined by plotting the burst
rates as a function of ATP concentration (Fig. 2B) and
fitting the data to a hyperbola. Note that the K401-4 rate constant
(257 s1) is significantly faster than the 100 s1 rate constant observed for dimeric K401-wt
ATP hydrolysis (30). It is interesting that a monomeric KHC motor
domain (K341) also shows a rapid rate of ATP hydrolysis at >300
s1 (35). For K401-4, the
Kd,ATP is 236 µM (Fig.
2B), which is equivalent to the steady-state
Km, ATP at 236 µM (1).
Comparison of the Kd, ATP for K401-wt
at 60 µM (30) with the
Kd, ATP for K401-4 indicates that the
mutant motor binds ATP much more weakly. The acid quench experiments
provide direct evidence that the T291M mutation significantly weakens
ATP binding and increases the rate of ATP hydrolysis.
Association Kinetics of K401-4 and Microtubules--
We next
looked at the rate of K401-4·ADP binding to the microtubule (Fig.
3) to determine if a microtubule binding
defect was indeed contributing to the abnormally high
K0.5, Mt measured through steady-state analysis
(1). The rate of formation of the Mt·K401-4 complex was monitored by
turbidity measurements in the stopped-flow instrument. K401-4·ADP (4 µM) was rapidly mixed with taxol-stabilized microtubules
(7 µM), and the change in turbidity was recorded. In this
experiment, an increase in turbidity was interpreted as binding of K401
to the microtubule. A representative stopped-flow record is shown in
Fig. 3A. The solid line is the best
fit of the data to a single exponential function and a linear term,
providing the kobs of the fast exponential phase
at 70 s1. Fig. 3B shows that the
observed rates of microtubule association increased linearly as a
function of microtubule concentration. These data were fit to Equation 2, the slope of which provides the apparent second order rate constant
for binding k+5 = 8 µM1
s1; this constant is somewhat less than
K401-wt measured at 11-15 µM1
s1 (15, 32). The y intercept
predicts a significant off-rate (k5 = 14 s1), which was not seen for K401-wt (32).
Therefore, the T291M mutation appears to weaken the binding between the
KHC motor domains and the microtubule.
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Fig. 3.
Kinetics of microtubule binding. 4 µM K401-4·ADP was rapidly mixed with varying
concentrations of microtubules (2.5-12 µM), and
turbidity was monitored in the stopped-flow apparatus. A, a
representative stopped-flow record at 7 µM microtubules,
which is the average of seven traces. The smooth
line is the best fit of the data to a single exponential
plus a linear term. The rate constant of the initial exponential phase
is 70 ± 1.6 s1. The second phase at a
rate of 0.07 ± 0.001 s1 is too slow to
be considered on the pathway and is attributed to a conformational
change after microtubule association. B, the rate constant
from the initial fast phase of each transient was plotted as a function
of microtubule concentration. The data were fit to Equation 2, the
slope providing the apparent second order rate constant for microtubule
association, k+5 = 8.2 ± 0.5 µM1
s1, and the y intercept providing
k5 = 14.3 ± 3.7 s1.
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ADP Release Kinetics from Mt·K·ADP--
We also measured the
kinetics of ADP release from the Mt·K401-4·ADP intermediate (Fig.
4) using mantADP. K401-4 was incubated with mantADP at a ratio of 4:1 to allow for exchange of ADP resident at
the active site with mantADP. A preformed K401-4·mantADP complex (3 µM K401-4, 12 µM mantADP) was rapidly mixed
with microtubules plus MgATP in the stopped-flow apparatus. As mantADP
was released from the more hydrophobic environment of the active site
into the aqueous buffer, its fluorescence was quenched. The MgATP (1 mM) present in solution blocked the subsequent rebinding of
any mantADP to K401. Fig. 4A shows a representative
stopped-flow record. The solid line is the fit of
the data to a single exponential function and a linear term, providing
the kobs of the fast exponential reaction at 31 s1. Fig. 4B shows that the
exponential rate constant associated with the fluorescence change upon
mantADP release increased with increasing microtubule concentration.
The fit of the data to a hyperbola provides a maximum rate constant of
mantADP release, k+6 = 234 s1 with a K0.5, Mt at
34 µM. The rate constant of mantADP release is consistent
with the fast ADP dissociation kinetics reported for K401-wt at
200-300 s1 (32), yet the
K0.5, Mt for K401-4 is larger than that for
K401-wt (15 µM). These results are consistent with the
interpretation that the T291M mutant protein requires a higher
concentration of microtubules both for half-maximal activation of
steady-state turnover at 3.6 versus 1 µM for
K401-wt (1) and for mantADP release (34 versus 15 µM for K401-wt).
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Fig. 4.
Kinetics of mantADP release. The
K401-4·mantADP complex (3 µM K401-4, 12 µM mantADP) was preformed such that K401-4 contained
mantADP bound to both heads. The complex was rapidly mixed in the
stopped-flow apparatus with varying concentrations of microtubules
(3-40 µM) plus 1 mM MgATP. A, a
representative stopped-flow record (average of seven traces) at 5 µM microtubules. The smooth line is
the fit of the data to a single exponential plus a linear term. The
kobs of the fast exponential phase was 31 ± 0.4 s1. B, the rate constant
from the exponential phase increased as a function of microtubule
concentration. The fit of the data to a hyperbola provided the maximum
rate constant of mantADP release, k+6 = 234 ± 41 s1 with
K0.5, Mt at 34.2 ± 10 µM.
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ATP-promoted Dissociation Kinetics of the Mt·K401-4
Complex--
The effects of the T291M mutation on ATP-promoted
detachment of K401·ADP from the microtubule were examined by
following changes in turbidity (Fig. 5).
The preformed Mt·K401-4 complex (2.9 µM microtubules, 3 µM K401-4) was rapidly mixed with MgATP plus 100 mM KCl in the stopped-flow apparatus. In this experiment, a
decrease in turbidity was interpreted as release of the motor from the microtubule. The addition of 100 mM KCl weakens rebinding
of the motor to the microtubule after detachment to allow for accurate measurement of the dissociation kinetics (32). Fig. 5A shows a representative stopped-flow record. The solid
line is the best fit of the data to a double exponential,
providing a kobs of the initial fast exponential
phase at 49 s1. The
kobs increased as a function of ATP
concentration, and the fit of the data to a hyperbola provides a
maximum rate constant of detachment, k+3 = 60 s1 with a K0.5, ATP
of 280 µM (Fig. 5B). This
K0.5, ATP is in agreement with both the
Km, ATP at steady-state conditions (1)
and the Kd,ATP determined by acid quench experiments (Fig. 2B), reinforcing the interpretation that
K401-4 binds ATP weakly.
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Fig. 5.
ATP-promoted dissociation of the Mt·K401-4
complex. The preformed Mt·K401-4 complex (3 µM
K401-4, 2.9 µM tubulin) was rapidly mixed with varying
concentrations of MgATP (10 µM to 2 mM) plus
100 mM KCl, and turbidity was monitored in the stopped-flow
apparatus. The salt was added to slow rebinding of K401-4 to
microtubules after dissociation. A, a representative
stopped-flow record (average of six traces) for 1 mM MgATP.
The smooth line is the fit of the data to a double exponential. The
kobs of the initial exponential phase was
49.4 ± 0.8 s1. The second exponential
phase was too slow to be considered on the pathway. B, the
rate constant of the exponential phase for each transient was plotted
as a function of MgATP concentration. The data were fit to a hyperbola,
providing the maximum dissociation rate constant
k+3 of 59.8 ± 2.9 s1 and K0.5, ATP = 280 ± 57.1 µM.
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It is striking that for both K401-wt and a dimeric human KHC construct
K379 (36), this ATP-promoted dissociation step was observed at rates of
12-14 s1, substantially slower than the 60 s1 observed for K401-4. The motor domains of
wild type dimeric KHC are coupled at this step such that ATP binding by
the microtubule-attached motor domain stimulates microtubule binding of
the partner motor domain and rapid release of its ADP (11-13). Johnson
and colleagues proposed that the intrinsic rate constant for
ATP-promoted detachment for a single motor domain is 50 s1 (13). This constant is faster than the
observed rate of 12-14 s1 measured for the
motor domain dimer because the alternating site mechanism only allows
one motor domain to be active at a time (13, 15, 32, 34). Thus, the net
rate of any step occurring in sequence is influenced by the rates of
the other steps. The intrinsic reaction rates for K401-wt have been
determined through global fitting of the data to a complete kinetic
mechanism using computer simulation (34). The observed rate of
detachment for K401-4 (60 s1) is very
different from the observed rate of 12-14 s1
but is very similar to the intrinsic rate constant of detachment for
K401-wt at 50 s1. These results suggest that
if the motor domains of K401-4 were dimerized as expected, they are no
longer tightly coupled and are acting more independently.
mantADP Dissociation Kinetics from the Mt·K401-4·mantADP
Complex--
To evaluate further the possible loss of motor domain
cooperativity in K401-4, a series of mantADP dissociation experiments were performed. Previously, it was reported that microtubule-stimulated ADP release from dimeric KHC is biphasic. ADP release from the first
head is fast, but release from the second head is delayed until the
first head can bind ATP (11-13). If the T291M mutation in K401-4 frees
the dimer from the constraint of cooperativity, the biphasic nature of
ADP release should be altered. Initially, we examined the rate of
mantADP release from both sites of K401-wt in the presence of ATP or
ADP (Fig. 6A,
inset). As in our previous experiments, ADP at the active
site was exchanged with mantADP. The K401·mantADP complex (3 µM K401, 6 µM mantADP) was rapidly mixed
with microtubules (10 µM tubulin) plus 2 mM
MgATP or 2 mM MgADP. Representative stopped-flow records
for K401-wt and K401-4 are shown in Fig. 6A. For K401-wt,
ATP promoted rapid release of mantADP from both motor domains, and ADP
caused a dramatic biphasic response with rapid release of mantADP from
the first motor domain (approximately 50% of the amplitude) and very
slow release of mantADP from the second motor domain (approximately 50% of the amplitude). Fig. 6A shows representative
stopped-flow records from the same experiment performed with K401-4. In
contrast to the K401-wt results, there was rapid release of mantADP
regardless of the nucleotide added (ATP or ADP); thus, the two curves
superimpose, and the rate constants for mantADP release were fast (116 s1 with ADP and 108 s1 with ATP). These results indicate that the
T291M mutation completely eliminates the biphasic nature of
microtubule-stimulated ADP release from dimeric K401. Similar kinetics
of mantADP release have been seen with K341, a monomeric KHC motor
domain construct (13).
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Fig. 6.
mantADP release in the presence of ATP or
ADP. A, kinetics of mantADP release from mutant K401-4
promoted by ATP or ADP. These are representative stopped-flow records
(average of six traces) in which the K401-4·mantADP complex (3 µM K401-4, 12 µM mantADP; preformed such
that K401-4 contained mantADP bound to both heads) was rapidly mixed
with 10 µM microtubules plus either 1 mM
MgATP or 1 mM MgADP. It is noteworthy that the mantADP
release transients promoted by ADP and ATP are indistinguishable
(115.8 ± 4.5 and 107.7 ± 4.0 s1,
respectively). Only 15% of the total amplitude is associated with the
second phase. Time domains are 0-400 ms and 400 ms to 3 s.
Inset, mantADP release from K401-wt initiated by ATP and
ADP. The experiment shown in a was repeated with wild type
(3 µM K401 6 µM mantADP). Note that the
ADP-promoted kinetic transient shows that approximately 50% of the
release amplitude was associated with the initial fast exponential
phase (53.6 ± 0.7 s1), and 50% was
associated with the second, much slower exponential phase (4.5 ± 0.02 s1). Time domains are 0-100 ms and 100 ms to 2 s. B, kinetics of mantADP release from the high
affinity nucleotide binding site of K401-4 and K401-wt as a function of
ATP or ADP. The Mt·K401-4·mantADP complex was preformed (6 µM K401-4, 3 µM mantADP, 15 µM microtubules; one mantADP bound per K401-4 dimer) and
mixed with either 1 mM MgATP or 1 mM MgADP.
Note that the kinetics of mantADP release promoted by ADP and ATP are
similar with kobs = 61.1 ± 2.7 s1 for ATP (yellow) and 54.3 ± 2.5 s1 for ADP (blue). This
experiment was repeated with K401-wt (red), and similar
results were observed with 1 mM MgATP,
kobs = 73.3 ± 1.7 s1. Inset, the same experiment
repeated with K401-wt with 1 mM MgADP. Note that the rate
of ADP release in the presence of ADP is significantly slower for
K401-wt; kobs = 6.6 ± 0.1 s1.
|
|
These results and those from ATP-promoted detachment of K401-4·ADP
from microtubules suggest that the T291M mutation induces nearly
independent, monomeric behavior. K401-4, with ~60 coiled-coil-forming amino acids of the neck, should be dimeric. To determine the
correctness of this supposition, sedimentation velocity studies (26)
were performed with monomeric K341, dimeric K401-wt, and K401-4 (Fig. 7). We found that K401-wt and K401-4 had
similar 20, w values
(5.50 and 5.42, respectively), and these were substantially greater
than the 20, w value for
monomeric K341 at 3.32. In the case of K401-wt, there is a shift in the g(s) curves to higher sedimentation coefficient values with
increasing protein concentration, which reflects the previously
observed 1-2-4 self-association mechanism for K401-wt (26). In Fig. 7, the g(s) curves of K401-4 do not show the same
degree of shift in the g(s) curves with
increasing protein concentration, indicative that the mutant form of
K401 is more stable as a dimer. There is some centrifugal tailing in
the g(s) curves for K401-4, suggesting that it
may still associate to form a tetramer, but this degree of association
is much weaker than that observed for K401-wt. The majority of the
K401-4 protein sediments near a peak position of 4.9 S, as determined
by a two-species fit by SVEDBERG (version 6.37); therefore, the
predominant species of the mutant is the dimer. Because K401-4 is
dimeric, the mantADP release kinetics indicate that the two motor
domains behave in a more kinetically independent manner. We conclude
that the T291M mutation alters structural features that are important
for the communication between motor domains and required for the
alternating site ATP hydrolysis mechanism.
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Fig. 7.
Sedimentation coefficient distribution
profiles for K341, K401-wt, and K401-4. The sedimentation velocity
data were analyzed for sedimentation distribution
g(s) in the presence of 20 µM MgATP
with motor concentrations from lowest to highest (bottom to
top): 2.0, 2.75, and 3.5 µM. The average
20, w value for each
construct is reported based on the
20, w data obtained at
three different protein concentrations for each: K341
20, w = 3.32 ± 0.10, K401-wt 20, w = 5.50 ± 0.08, and K401-4
20, w = 5.42 ± 0.20.
|
|
mantADP Dissociation Kinetics from Each Site of Dimeric
K401-4--
The observation that microtubules in the presence of ADP
elicit rapid release of mantADP from both motor domains of K401-4 (Fig.
6A) suggests that the active site responds to ADP in the same manner that it responds to ATP. Both seem to serve equally well to
stimulate microtubule binding by the second motor domain. To evaluate
this hypothesis further, we examined the rate of mantADP release from
the second motor domain; the head that keeps ADP more tightly bound in
the presence of microtubules and is believed to be detached or weakly
bound to the microtubule (Fig. 6B). An equilibrium mixture
was prepared in which 6 µM K401-4 (or K401-wt) was
incubated with 3 µM mantADP and 15 µM
microtubules. At these conditions, only one mantADP is expected to be
bound per kinesin dimer (12). mantADP release is then activated by
rapidly mixing with either ATP or ADP in the stopped-flow instrument.
Under these conditions, the added ATP or ADP should bind the active
site of the microtubule-attached head, allowing the second motor domain to bind the microtubule to drive release of its mantADP (12). For
K401-wt, mantADP release promoted by ATP was fast at 73 s1 (Fig. 6B, red
trace), yet ADP-promoted release of mantADP was extremely
slow at 6.6 s1 (Fig. 6B,
inset). In contrast, for K401-4 there was no appreciable difference in the mantADP dissociation kinetics using either ATP (kobs = 61 s1, Fig.
6B, yellow trace) or ADP
(kobs = 54 s1, Fig.
6B, blue trace) to promote mantADP
release from the high affinity site of K401-4. These data show that
K401-4 is able to hold mantADP at the high affinity site despite the
fact that this mutant binds nucleotide much more weakly than wild type
kinesin. Therefore, there is some degree of cooperativity between the
motor domains to establish a difference in nucleotide binding at head 1 versus head 2. More importantly, because ATP and ADP both
stimulate rapid release of mantADP from the high affinity site, yet
buffer does not (data not shown), the results indicate that the low
affinity site (head 1) has lost the ability to distinguish ATP from ADP.
| |
DISCUSSION |
To gain a deeper understanding of the mechanisms employed by
kinesin to produce processive movement,
we examined in detail the effects of a specific amino acid substitution
on the mechanochemical cycle (see Schemes
1 and 2).
Our steady-state kinetic analysis indicated that the T291M mutation
causes defects in both ATP and microtubule binding (1). The
pre-steady-state kinetics presented here show that the mutant motor
binds ATP and microtubules more weakly than K401-wt. Moreover, our
analysis reveals a defect in the signaling mechanism between the motor
domains of the mutant dimer, suggesting that the T291M change
significantly disrupts the alternating site mechanism of ATP turnover
for dimeric kinesin.
In our initial studies, we reported an almost 4-fold increase in the
K0.5, Mt and attributed it to weaker
microtubule binding by K401-4 (1). Through our mantADP release studies
(Fig. 4), the measured K0.5, Mt at 34 µM is much larger than that for K401-wt (15 µM). The microtubule association kinetics (Fig. 3) also
reveal an appreciable off-rate for microtubules
(k5 = 14 s1), which
is not seen with K401-wt (32). These results confirm that microtubule
binding for K401-4 is much weaker than that seen for K401-wt.
We also reported a 3-fold increase in the
Km, ATP and attributed it to weaker ATP
binding by K401-4 (1). There is a significant off-rate
(k1 = 157 s1)
observed in the mantATP binding experiment (Fig. 1), which shows weak
mantATP binding. This finding is reinforced by our ATP hydrolysis studies, which define the Kd, ATP at
236 µM. For K401-wt, the
Kd,ATP at 60 µM (30) indicates
significantly tighter ATP binding by wild type kinesin. Thus, the
pre-steady-state kinetic analysis confirms our original supposition
that ATP binding by K401-4 is significantly weaker than K401-wt.
The most striking difference in the ATPase cycles of mutant and wild
type K401 is seen in the kinetics of rate-limiting detachment from
microtubules. The rate of detachment for K401-4
(k+3 = 60 ± 3 s1) is quite fast relative to wild type
dimeric kinesin constructs at 12-14 s1 (32,
36). Furthermore, the observed rate constant at 60 s1 is very similar to the intrinsic rate
constant of detachment for K401-wt at 50 ± 8 s1 (34), and the centrifugation analysis
documents that K401-4 is dimeric (Fig. 7). These results show that the
mutant motor domains exhibit some degree of kinetic uncoupling.
The observation of motor domain uncoupling in K401-4 indicates that the
alternating site catalysis mechanism must be compromised and that
strict coordination of the motor domains must be disrupted. A series of
mantADP release experiments were used to dissect the pathway of motor
interaction with the microtubule for wild type dimeric kinesin (12, 13,
32, 36). These experiments showed that head 1 binds to the microtubule
with rapid release of mantADP, and it is ATP binding at this empty site
that signals the second motor domain to bind the microtubule and
quickly release its mantADP. ADP binding at head 1 does not elicit
rapid release of mantADP from head 2. We pursued these same experiments
with K401-4 to examine the degree of cooperative interactions between
the motor domains of the mutant. Our results show that there was rapid
release of mantADP from head 2; however, both ADP and ATP binding at
head 1 can induce rapid dissociation of mantADP from this high affinity site (Fig. 6). These results indicate that the mechanism of
communication between the motor domains of K401-4 is defective.
However, the results also show that there is some degree of
communication between the motor domains, because mantADP release from
head 2 does require nucleotide binding (ADP or ATP) at head 1. Buffer
will not stimulate rapid release of mantADP from head 2. These results
imply that K401-4 cannot sense the absence of the -phosphate and
that the breakdown in signal transmission between the motor domains
results in an ATPase mechanism in which the motor domains are no longer strictly coordinated.
Another key difference in the ATPase cycle of K401-4 that probably
contributes to disruption of the wild type alternating site ATP
hydrolysis mechanism (Schemes 1 and 2) is the more rapid rate of ATP
hydrolysis observed in the mutant. Our mantADP release experiments have
documented mantADP release from the high affinity site (head 2) at
70-100 s1, and both ATP and ADP can activate
rapid mantADP release from head 2. With ATP hydrolysis by head 1 occurring at 257 s1, it is possible that
subsequent release of head 1 from the microtubule occurs before head 2 can bind the microtubule, resulting in detachment of the dimer from the
microtubule (Scheme 2, path 1). An alternative possibility is that because signaling between the motor domains is
aberrant, the first head does not detach after ATP hydrolysis and the
second head binds the microtubule followed by concomitant ADP release
(Scheme 2, path 2). Path 2 results in a kinesin
intermediate in which both heads are bound to the microtubule and both
active sites are empty. Thus, the motor domains of the dimer are in
phase with each other after ATP turnover rather than out of phase where the two motor domains are always at different stages of the ATPase cycle as required by the alternating site ATPase mechanism of wild type kinesin.
To discriminate between these two paths, we performed ATP-promoted
detachment assays at low salt conditions (50 mM; Fig.
8). In low salt, K401-wt remains bound
for several ATP turnover cycles before detaching, and the observed
kinetics of motor detachment appear quite slow. However, if path 1 were
the mechanism, the motor should detach immediately after the first
turnover with the rate constant at 60 s1. In
low salt, K401-wt dissociates with an observed rate constant of 1.7 s1, indicating that the dimeric motor is in
association with the microtubule for 0.6 s. This transit time
suggests multiple steps along the microtubule, each coupled to a single
ATP turnover. For K401-4, the kinetics are more complex and biphasic,
with the initial exponential phase at 1.4 s1
and the second slower phase at 0.1 s1. Our
interpretation is that K401-4 remains associated with the microtubule
for multiple ATP turnovers; therefore, these kinetics exclude path 1 and favor path 2 as the mechanism of the K401-4 ATPase. Although the
results show prolonged association with the microtubule at these
conditions, the mechanistic basis of K401-4 microtubule association is
more difficult to interpret and is probably not reflecting processive
ATP movement with one ATP turnover tightly coupled to one productive
step.
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Fig. 8.
ATP-promoted dissociation at low salt.
The preformed Mt·K401-wt and Mt·K401-4 complexes (3 µM K401-4, 2.9 µM tubulin) were rapidly
mixed with 1 mM MgATP, and turbidity was monitored in the
stopped-flow apparatus. For this experiment, additional salt was
not added to the ATP syringe to evaluate whether the mutant
motor detaches directly after ATP hydrolysis (Scheme 2, path
1) or the mutant motor follows path 2 and results in an
intermediate with both heads bound to the microtubule and at the same
stage in the ATPase cycle (Scheme 2, path 2). The
dissociation kinetics of K401-wt at 1.7 s1
indicate that the wild type motor is in association with the
microtubule for 0.6 s (transit time = 1/kobs). For K401-4, the dissociation kinetics
are biphasic with the exponential phase at 1.4 s1 (transit time = 0.7 s) followed
by a second slower phase at 0.1 s1.
|
|
In Drosophila, the T291M mutation is recessive lethal (23).
The timing of lethality and the prelethal, paralytic behavioral phenotype indicates a complete loss of function (1). The earliest cellular defects seen in mutants is the stochastic accumulation of
mitochondria, vesicles, and other organelles in large "traffic jams" that force axonal swellings (24). Disruption of fast axonal transport by kinesin mutations causes motor neuron disease phenotypes in Drosophila. Therefore, the in vivo effects,
the slow motility promoted by K401-4 in microtubule-gliding assays
in vitro (1), and the kinetics presented here, lead us to
believe that processive movement is severely impaired by the T291M mutation.
Thr291, which is conserved throughout the kinesin
superfamily, is located in a hydrophobic pocket, internal to the
microtubule-binding site at Loop12 (Fig.
9). Scrutiny of KHC crystal structures
suggests that Thr291 forms a hydrogen bond with the
carbonyl group of Tyr285 (HIPYR), which is also highly
conserved and located near the end of Loop12. Upon substitution of
Thr291 with methionine, interactions with
Tyr285 as well as with a number of hydrophobic residues
(Leu294, Leu268, Leu298, and
Phe89) must be altered (Fig. 9).
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Fig. 9.
Location of the K401-4 mutation.
A, crystal structure of the kinesin motor domain (rat 2kin;
Ref. 4). This view has the microtubule-binding surface forward, and the
active site in the rear (ADP is yellow). The side chain of
Thr291 on 5 is identified in green (amino
acid designation based on Drosophila KHC sequence).
Thr291 appears to be part of a hydrophobic pocket that
includes (in yellow) Tyr285, Leu298,
Leu268, Leu294, and Phe89. All of
these residues are highly conserved throughout the kinesin superfamily,
suggesting that the fine structure of this pocket is critical for
normal function. Note that Loop12, important in microtubule binding, is
located between 4 and 5 to the top left in
this view. B, view identical to that in A with
the side chain of Thr291 substituted with methionine and
identified in green. Note that the methionine is longer and
must disrupt the critical contacts that the threonine normally makes.
We propose a disruption of the hydrogen bond between Thr291
and the carbonyl of Tyr285 as well as disruption of the
hydrophobic core involving Leu298, Leu268,
Leu294, and Phe89.
|
|
Disturbance of this hydrophobic pocket by the T291M mutation may
explain the kinetics of K401-4. It has been proposed that 4/Loop11
is analogous to the G-protein switch II region that senses the
-phosphate of ATP (9). In vitro mutagenesis studies of
KHC in the switch II region have documented the importance of the
conserved glycine and glutamic acid (VDLAGSE) for ATP hydrolysis and
the conformational change necessary to generate force and movement
(22). The authors proposed that the glycine in kinesin forms a hydrogen
bond with the -phosphate and triggers a conformation change between
the ATP and ADP states. Further experimental work suggests that this
region is important in the coupling of the nucleotide pocket and
microtubule-binding surface (1, 21). Thus, the observed weak binding of
ATP and microtubules by K401-4 may reflect a shift in the switch II
element at the beginning of Loop11. Disruption of the hydrogen bond
between Thr291 and Tyr285 could cause a
structural "ripple effect" altering the positions of the adjacent
Loop12, 4, and Loop11. Shifting the switch II element at the
beginning of Loop11 could affect its hydrogen bond interaction with the
-phosphate, explaining the insensitivity of K401-4 to the absence of
the -phosphate during microtubule-stimulated ADP release.
Another consequence of the T291M substitution is the lowered affinity
for ATP. One of the residues in the hydrophobic pocket, Phe89 (Fig. 9), is located on 3, two amino acids away
from the P-loop consensus sequence in Loop4 which is critical for
contact with the , phosphates of ATP (9). Disruption of the
hydrophobic pocket could disrupt the position of Phe89 and
alter the conformation or position of the P-loop, changing contacts
with the - and -phosphates of the nucleotide and altering both
ATP binding and switch I-switch II interactions for ATP hydrolysis.
In summary, we have identified a single amino acid change that has a
dramatic effect on the ATPase cycle of kinesin by altering communication between the motor domains. The results presented for
T291M illustrate the importance of understanding the functionally relevant transition states and the structural requirements for motor
coordination and processive movement. Through the use of this
multifaceted approach, we hope to advance the understanding of the
structural requirements for motor coordination and processive movement.
| |
ACKNOWLEDGEMENTS |
We thank John M. Rosenberg for assistance
with molecular modeling and structural interpretation and Eckhard
Mandelkow for stimulating discussions about KHC structure. We
particularly thank Jack Correia and the University of Mississippi
Medical Center Analytical Ultracentrifuge Facility for assistance with
the sedimentation studies.
| |
FOOTNOTES |
*
This work was supported by National Institutes of Health
Grants GM-54141 (to S. P. G.) and GM-46295 (to W. M. S.), American Cancer Society (ACS) Grant IRG-58-35 (to S. P. G.), and March of
Dimes Birth Defects Foundation Grant 5-FY95-1136 (to S. P. G.).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.
§
Supported by a Predoctoral Fellowship from the American Heart
Association (AHA), Indiana Affiliate, Inc. Present address: Dept. of
Biochemistry and Molecular Biophysics, Washington University School of
Medicine, 660 S. Euclid Ave., St. Louis, MO 63110.
Supported by an AHA Established Investigatorship with funds
contributed in part by the AHA, Indiana Affiliate, Inc.
Supported in part by an ACS Junior Faculty Research Award
(JFRA-618). To whom correspondence should be addressed: Dept. of Biological Sciences, University of Pittsburgh, 518 Langley Hall, Fifth
and Ruskin, Pittsburgh, PA 15260. Tel.: 412-624-5842; Fax: 412-624-9311; E-mail: spg1+@pitt.edu.
Published, JBC Papers in Press, April 14, 2000, DOI 10.1074/jbc.M001124200
2
Greene, E. A., and Henikoff, S., The kinesin
home page. 2000.http://www.blocks.fhcrc.org/~kinesin/.
| |
ABBREVIATIONS |
The abbreviations used are:
KHC, kinesin heavy
chain;
Khc, Drosophila kinesin heavy chain gene;
K401, KHC fragment containing the N-terminal 401 amino acids;
K401-wt, wild type K401;
K401-4, K401 with T291M amino acid substitution;
AMP-PNP, 5'-adenylyl imidodiphosphate;
Mt, microtubule;
Mt·K401, microtubule-K401 complex;
mantATP, 2'(3')-O-(N-methylanthraniloyl)-adenosine
5'-triphosphate;
mantADP, 2'(3')-O-(N-methylanthraniloyl)-adenosine
5'-diphosphate.
| |
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TOP
ABSTRACT
INTRODUCTION
