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Experiments: how do we know what single motors do?. Optical tweezers. Optical trapping. Is simply a TM-00 (Gausian cross section) laser beam focussed to a diffraction-limited spot. Can use it to grab, and manipulate, small dielectric objects
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Optical trapping • Is simply a TM-00 (Gausian cross section) laser beam focussed to a diffraction-limited spot. • Can use it to grab, and manipulate, small dielectric objects • Vesicles, lipid droplets, cell membranes, small glass or plastic spheres are all small dielectric objects
Optical trap • Can position beads anywhere • Easy to see motor-microtubule binding events
How much force can the motor exert: Optical tweezers as a spring
Methods For Force calibration in Optical Tweezers(If interested, please see Dr. Yonggun Jun who has just spent a lot of time thinking about OT calibration!!)
How far can a single motor move a cargo? • Vesicle transport motors such as kinesin and Myosin-V are “processive” enzymes • Processive: go through repeated complete enzymatic cycles, while remaining bound to the substrate (in this case the MT or AF)
Microtubule motors are uni-directional Single Kinesin motor moving a bead in vitro A single motor moves ~ 1 m
Single motor bead assays: processivity Histogram Individual Traces
Does it take discrete steps, or move continuously? If steps, what size? • MT built of repeating subunits (dimers). Each dimer is 8 nm in length • If moves along a single protofilament, expect steps that are some multiple of 8nm. If lateral steps possible, could take smaller steps.
Single-molecule driven beads move in 8 nm steps at low [ATP], low load
Extraction of Step size from displacement records Pairwise Distance Function analysis Step Size ? Position Time You expect to see regular peaks in a histogram of such pairwise distance at multiples of the Step size
Step Detection Techniques—individual rapid steps AOD • Force Clamp • High Sampling Feedback Halogen Lamp L5 PSD 980nm IR Laser M1 DM1 BFPC L1 Condenser NA=1.4 XYZ Piezo-Stage 100x Objective NA=1.3 BFPO L2 DM2 L6 M2 CCD camera L4 L3 M3 Chi-squared Minimization Method B.C. Carter, et al “A Comparison of Step-Detection Methods: How Well Can You Do?”Biophys. J., 94(1):306-19, (2008) x
Step Size Measurements Kinesin
Label one head Selvin, Science
Distribution of steps: The average step-size is 17.3 ±3.3 nm; uncertanty of mean (SEM) is 0.27 nm
Kinesin Myosin-V Dynein Cargo Cargo KLC Dynactin binding KR2 KR1 Pi Ca2+ MR2 Head (ATPase) Stalk Pi 1 2 c KAPP 3 6 4 5 KR3 MR1 Lever (?) KHC Head (ATPase) MT binding Three families of molecular motors
Processivity: porters vs rowers Non-processive (rower) Processive (porter) Images: MCRI Molecular motors group
Kinesin is Processive; Myosin II (muscle) is not. Why? • A processive motor doesn’t let go of the substrate (MT or AF) so the cargo doesn’t diffuse away • Many processive motors could get in each others way--all bound to the filament at the same time • A non-processive motor lets go of the filament at some point in its enzymatic cycle. Thus, multiple motors don’t get in each others way--not active at exactly the same time • The ‘duty ratio’ is the ratio of (time bound to substrate)/(complete time for enzymatic cycle) • Duty ratio=1 for processive motor
Summary of single-molecule experiments Motor proteins: • Are uni-directional, and move along straight filaments • Exert 1-6 pN force • Typically go ~ 1m before detaching • Kinesin motors take 8 nm steps, Dynein takes a variety of step sizes, Myosins take 36 nm steps • Move between 0.1 and 2 m/s Is this how transport functions inside cells?
How do we go from single-molecule characterization to in vivo function?
Why do cargos need multiple motors?Many intercellular distances are longerthan 1 micron
Motion in cells is different from what might be expected based on single-molecule properties Cargos can move long distances Maybe multiple motors? Bead moved by multiple kinesin motors
So, multiple motors can move a cargo long distances. Now, lets look more carefully… Start to build complexity in a controlled environment, i.e. in vitro, and understand how motors work together
Poisson statistics: Getting down to the single molecule limit… • Catch Dynein- or kinesin-coated beads, bring in contact with MT • Find probability for Binding/motion (Bind fraction) • Repeat at different motor:Bead ratios • Plot the Bind fraction Vs motor:Bead ratio • Stay where probability for “doubles” is negligible For single motor, use Binding/moving fraction ≤ 0.3
Motor - polystyrene bead assays Kinesin I: single motor 30% or less of beads bind to MTs Force production Run Length (Processivity) Peak center ± SEM : 4.8±0.06 pN Decay constant ± SEM : 1.46±0.16 µm
Poisson statistics: Getting down to the single molecule limit…and then back to multiple motors • Catch motor-coated beads, bring in contact with MT • Find probability for Binding/motion (Bind fraction) • Repeat at different motor:Bead ratios • Plot the Bind fraction Vs motor:Bead ratio • Now, use concentration where probability for “doubles” is high: mixed population Mixed bead population--> How do we know how many motors are moving a specific bead?
What we think is going on Bf~1.0 Bf~0.7 Bf~0.3 Bf~1.0 Increasing Kinesins per bead
Evolution of force production with increasing kinesins per bead 1-2 motor Mostly single motor (Bf ~1) Single motor (Bf ~0.3)
Conclusion: for multiple-motor driven transport, binding fraction cannot tell you how many motors engaged. Stalling forces are additive at low motor number; use this as a readout of the number of instantaneously engaged motors
Motor - polystyrene bead assays Kinesin I: ~two motors driving polystyrene bead Run Length Force production
Summary for ~2 engaged Kinesins:* Velocities unchanged (not shown) * Stall forces ~ additive* Cargo travel lengths very long, but this is not really correct (see next)>> Similar results for cytoplasmic dynein (see Mallik et al, Curr. Bio, 2005)More: see website bioweb.bio.uci.edu/sgross
Conclusion: motion in cells is different from what might be expected based on single-molecule properties We have three ‘systems’ level questions to understand: Cargos can move long distances Cargos can reverse course, move bi-directionally Cargo transport can be regulated
What single-molecule properties are particularly important for how multiple motors function together?
Cartoon of processive motion of a cargo moved by two motors
From cartoon… On-rate Off-rate Overall number of motors
Back of the envelope calculation for how far 2 motors will go on average…. Assume single-motor processivity of 1200 nm, velocity of 800 nm/sec, on rate of 5/sec First motor detaches at t0 . How long to rebind? T(rebind) ~ 1/Kon =1/5 sec. Does second motor detach before first rebinds? What is off rate? Processivity (mean travel): 1200 nm, vel 800 nm/sec avg duration of run: 1200 nm/800 nm/sec=1.5 sec Off rate: 1/avg duration = Koff= 1/1.5 Prob of second motor detaching is Koff*(rebinding time)=(1/1.5)*(1/5)= 0.1333 i.e. ~13% chance of failing to make it though cycle. Adjust this to 26% (ignored second motor detaching right before first motor) On avg make it through ~ 4 cycles.
Regulation: how? From expression <X>= ½*(D/N)*(Kon/Koff)N-1 Kon: On-rate, i.e. rate at which single motor binds MT Koff: Off-rate in time, i.e. rate at which single motor detaches from MT D=processivity, i.e. mean travel (distance) before detaching. Note that Koff and D are NOT independent: Koff = V/D V=Motor velocity can tune mean travel by altering N, Kon, or Koff (V or D, or both).
Analytic Mean-field theory of average cargo travel carried by two motors Velocity: crucial initial condition p: binding rate (1/s) e: unbinding rate (1/s) d=v*(1/ e)=v/ e Klumpp and Lipowsky, PNAS, 2005
Experiment: established for single-motor study Valentine et al., Nat. Cell Bio., 2006
Experiment: established for single-motor study Valentine et al., Nat. Cell Bio., 2006
