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- Direct Observation of Poloxamer 188 Insertion into Lipid Mon...Direct Observation of Poloxamer 188 Insertion into Lipid Monolayers
Biophysical Journal, Volume 82, Issue 3, 1 March 2002, Pages 1453-1459
Stacey A. Maskarinec, Jürgen Hannig, Raphael C. Lee and Ka Yee C. Lee
AbstractP188, a triblock copolymer of the form poly(ethylene oxide)-poly(propylene oxide)-poly(ethylene oxide) helps seal electroporated cell membranes, arresting the leakage of intracellular materials from the damaged cells. To explore the nature of the interaction between P188 and cell membranes, we have constructed a model system that assesses the ability of P188 to insert into lipid monolayers. Using concurrent Langmuir isotherm and fluorescence microscopy measurements, we find that P188 changes the phase behavior and morphology of the monolayers. P188 inserts into both dipalmitoylphosphatidlycholine and dipalmitoylphosphatidylglycerol monolayers at surface pressures equal to and lower than ∼22 mN/m at 30°C; this pressure corresponds to the maximal surface pressure attained by P188 on a pure water subphase. Similar results for the two phospholipids indicate that P188 insertion is not influenced by headgroup electrostatics. Because the equivalent surface pressure of a normal bilayer is on the order of 30 mN/m, the lack of P188 insertion above 22 mN/m further suggests the poloxamer selectively adsorbs into damaged portions of electroporated membranes, thereby localizing its effect. P188 is also found to be “squeezed out” of the monolayers at high surface pressures, suggesting a mechanism for the cell to be rid of the poloxamer when the membrane is restored.
Abstract | Full Text | PDF (197 kb) - Interaction between Lipid Monolayers and Poloxamer 188: An X...Interaction between Lipid Monolayers and Poloxamer 188: An X-Ray Reflectivity and Diffraction Study
Biophysical Journal, Volume 89, Issue 5, 1 November 2005, Pages 3159-3173
Guohui Wu, Jaroslaw Majewski, Canay Ege, Kristian Kjaer, Markus Jan Weygand and Ka Yee C. Lee
AbstractThe mechanism by which poloxamer 188 (P188) seals a damaged cell membrane is examined using the lipid monolayer as a model system. X-ray reflectivity and grazing-incidence x-ray diffraction results show that at low nominal lipid density, P188, by physically occupying the available area and phase separating from the lipids, forces the lipid molecules to pack tightly and restore the barrier function of the membrane. Upon compression to bilayer equivalent pressure, P188 is squeezed out from the lipid monolayer, allowing a graceful exit of P188 when the membrane integrity is restored.
Abstract | Full Text | PDF (320 kb) - The Reduction in Electroporation Voltages by the Addition of...The Reduction in Electroporation Voltages by the Addition of a Surfactant to Planar Lipid Bilayers
Biophysical Journal, Volume 75, Issue 2, 1 August 1998, Pages 880-888
Gregory C. Troiano, Leslie Tung, Vinod Sharma and Kathleen J. Stebe
AbstractThe effects of a nonionic surfactant, octaethyleneglycol mono -dodecyl ether (CE), on the electroporation of planar bilayer lipid membranes made of the synthetic lipid 1-pamitoyl 2-oleoyl phosphatidylcholine (POPC), was studied. High-amplitude (∼100–450mV) rectangular voltage pulses were used to electroporate the bilayers, followed by a prolonged, low-amplitude (∼65mV) voltage clamp to monitor the ensuing changes in transmembrane conductance. The electroporation thresholds of the membranes were found for rectangular voltage pulses of given durations. The strength-duration relationship was determined over a range from 10s to 10s. The addition of CE at concentrations of 0.1, 1, and 10M to the bath surrounding the membranes decreased the electroporation threshold monotonically with concentration for all durations (<0.0001). The decrease from control values ranged from 10% to 40%, depending on surfactant concentration and pulse duration. For a 10-s pulse, the transmembrane conductance 150s after electroporation () increased monotonically with the surfactant concentration (=0.007 for 10M CE). These findings suggest that CE incorporates into POPC bilayers, allowing electroporation at lower intensities and/or shorter durations, and demonstrate that surfactants can be used to manipulate the electroporation threshold of lipid bilayers.
Abstract | Full Text | PDF (153 kb) - …more
Copyright © 1996 The Biophysical Society. All rights reserved.
Biophysical Journal, Volume 71, Issue 6, 3229-3241, 1 December 1996
doi:10.1016/S0006-3495(96)79516-4
Research Article
Poloxamer 188 decreases susceptibility of artificial lipid membranes to electroporation
V. Sharma, K. Stebe, J.C. Murphy and L. Tung
Abstract
The effect of a nontoxic, nonionic block co-polymeric surface active agent, poloxamer 188, on electroporation of artificial lipid membranes made of azolectin, was investigated. Two different experimental protocols were used in our study: charge pulse and voltage clamp. For the charge pulse protocol, membranes were pulsed with a 10-micronsecond rectangular voltage waveform, after which membrane voltage decay was observed through an external 1-M omega resistance. For the voltage clamp protocol the membranes were pulsed with a waveform that consisted of an initial 10-microsecond rectangular phase, followed by a negative sloped ramp that decayed to zero in the subsequent 500 microseconds. Several parameters characterizing the electroporation process were measured and compared for the control membranes and membranes treated with 1.0 mM poloxamer 188. For both the charge pulse and voltage clamp experiments, the threshold voltage (amplitude of initial rectangular phase) and latency time (time elapsed between the end of rectangular phase and the onset of membrane electroporation) were measured. Membrane conductance (measured 200 microseconds after the initial rectangular phase) and rise time (tr; the time required for the porated membrane to reach a certain conductance value) were also determined for the voltage clamp experiments, and postelectroporation time constant (PE tau; the time constant for transmembrane voltage decay after onset of electroporation) for the charge pulse experiments. The charge pulse experiments were performed on 23 membranes with 10 control and 13 poloxamer-treated membranes, and voltage pulse experiments on 49 membranes with 26 control and 23 poloxamer-treated membranes. For both charge pulse and voltage clamp experiments, poloxamer 188-treated membranes exhibited a statistically higher threshold voltage (p = 0.1 and p = 0.06, respectively), and longer latency time (p = 0.04 and p = 0.05, respectively). Also, poloxamer 188-treated membranes were found to have a relatively lower conductance (p = 0.001), longer time required for the porated membrane to reach a certain conductance value (p = 0.05), and longer postelectroporation time constant (p = 0.005). Furthermore, addition of poloxamer 188 was found to reduce the membrane capacitance by approximately 4–8% in 5min. These findings suggest that poloxamer 188 adsorbs into the lipid bilayers, thereby decreasing their susceptibility to electroporation.
