Coupling supported lipid bilayer electrophoresis with matrix-assisted laser desorption/ionization-mass spectrometry imaging.

Herein, we describe a new analytical platform utilizing advances in heterogeneous supported lipid bilayer (SLB) electrophoresis and matrix-assisted laser desorption/ionization-mass spectrometry (MALDI-MS) imaging. This platform allowed for the separation and visualization of both charged and neutral lipid membrane components without the need for extrinsic labels. A heterogeneous SLB was created using vesicles containing monosialoganglioside GM1, disialoganglioside GD1b, POPC, as well as the ortho and para isomers of Texas Red-DHPE. These components were then separated electrophoretically into five resolved bands. This represents the most complex separation by SLB electrophoresis performed to date. The SLB samples were flash frozen in liquid ethane and dried under vacuum before imaging with MALDI-MS. Fluorescence microscopy was employed to confirm the position of the Texas Red labeled lipids, which agreed well with the MALDI-MS imaging results. These results clearly demonstrate this platform's ability to isolate and identify nonlabeled membrane components within an SLB.

Phosphatidylserine reversibly binds Cu2+ with extremely high affinity.

Phosphatidylserine (PS) embedded within supported lipid bilayers was found to bind Cu(2+) from solution with extraordinarily high affinity. In fact, the equilibrium dissociation constant was in the femtomolar range. The resulting complex formed in a 1:2 Cu(2+)-to-PS ratio and quenches a broad spectrum of lipid-bound fluorophores in a reversible and pH-dependent fashion. At acidic pH values, the fluorophores were almost completely unquenched, while at basic pH values significant quenching (85-90%) was observed. The pH at which the transition occurred was dependent on the PS concentration and ranged from approximately pH 5 to 8. The quenching kinetics was slow at low Cu(2+) concentrations and basic pH values (up to several hours), while the unquenching reaction was orders of magnitude more rapid upon lowering the pH. This was consistent with diffusion-limited complex formation at basic pH but rapid dissociation under acidic conditions. The tight binding of Cu(2+) to PS may have physiological consequences under certain circumstances.

Protein separation by electrophoretic-electroosmotic focusing on supported lipid bilayers.

An electrophoretic-electroosmotic focusing (EEF) method was developed and used to separate membrane-bound proteins and charged lipids based on their charge-to-size ratio from an initially homogeneous mixture. EEF uses opposing electrophoretic and electroosmotic forces to focus and separate proteins and lipids into narrow bands on supported lipid bilayers (SLBs). Membrane-associated species were focused into specific positions within the SLB in a highly repeatable fashion. The steady-state focusing positions of the proteins could be predicted and controlled by tuning experimental conditions, such as buffer pH, ionic strength, electric field, and temperature. Careful tuning of the variables should enable one to separate mixtures of membrane proteins with only subtle differences. The EEF technique was found to be an effective way to separate protein mixtures with low initial concentrations, and it overcame diffusive peak broadening to allow four bands to be separated simultaneously within a 380 µm wide isolated supported membrane patch.

Supported bilayer electrophoresis under controlled buffer conditions.

A pH controlled flow cell device was constructed to allow electrophoretic movement of charged lipids and membrane associated proteins in supported phospholipid bilayers. The device isolated electrolysis products near the electrodes from the electrophoresis process within the bilayer. This allowed the pH over the bilayer region to remain within ±0.2 pH units or better over many hours at salt concentrations up to 10 mM. Using this setup, it was found that the electrophoretic mobility of a dye conjugated lipid (Texas Red 1,2-dihexadecanoyl-sn-glycero-3-phosphoethanolamine (TR-DHPE)) was essentially constant between pH 3.3 and 9.3. In contrast, streptavidin, which was bound to biotinylated lipids, shifted from migrating cathodically at acidic pH values to migrating anodically under basic conditions. This shift was due to the modulation of the net charge on the protein, which changed the electrophoretic forces experienced by the macromolecule. The addition of a polyethylene glycol (PEG) cushion beneath the bilayer or the increase in the ionic strength of the buffer solution resulted in a decrease of the electroosmotic force experienced by the streptavidin with little effect on the Texas Red-DHPE. As such, it was possible in part to control the electrophoretic and electroosmotic contributions to streptavidin independently of one another.

Antibody-antigen exchange equilibria in a field of an external force: design of reagentless biosensors.

This correspondence presents a new strategy for detecting biological molecules that relies on competitive exchange interactions of an analyte with two-component molecular tethers attaching superparamagnetic microspheres (4 microm in diameter) to a sensor surface. The individual tethers consist of an antibody-antigen complex and are designed to selectively detect antigenic proteins in a sensitive reagentless fashion. In order to impart a driving force to the otherwise free energy neutral antibody-antigen exchange equilibrium, a small mechanical force of approximately 10 pN was applied to stretch the antibody-antigen tethers using a massively parallel magnetic tweezers device. The experimental work was carried out with human cardiac troponin I. This serum heart attack marker was used as an example of analytes of credible relevance to biomedical diagnostics. The initial results illustrate the functioning of a cardiotroponin sensor and offer a preliminary estimate of its sensitivity of 16 pM.

Ion diffusion in channels containing random arrays of microspheres: an electrochemical time-of-flight method.

Rates of chloride ion diffusion in narrow (ca. 3 microm thick), rectangular (ca. 0.1 x 1.0 mm(2)) channels partially filled with polystyrene microspheres are investigated by a potentiometric electrochemical time-of-flight (P-ETOF) method. Lithographically fabricated on glass slides, P-ETOF devices consist of a centrally positioned 10 microm wide, ca. 1 mm long generator microelectrode and two sensor microelectrodes of the same dimensions symmetrically positioned on both side of the generator at a distance of 50 microm. The electrodes are silver-plated and partially oxidized in a chloride electrolyte to form Ag/AgCl deposits. Constant current reduction of AgCl on the generator electrode is used to produce chloride ions at a constant rate. Ag/AgCl deposited on the sensor microelectrodes allows time-dependent potentiometric monitoring of the increasing concentration of chloride ions diffusing across the interelectrode gap. The device is enclosed with a parallel glass plate to form a narrow channel with the polystyrene microbeads serving as spacers. The packing density of the microspheres expressed in terms of the fractional void volume (rho) varied from ca. 0.6 to 1.0. Using rho, we modified a diffusion equation describing the change of chloride ion concentration at the sensor microelectrode to include the effect of the microspheres restricting the void volume. We rely on digital simulations as well as on direct P-ETOF experiments to show that the proposed equation does accurately account for the effect of rho on the diffusion processes. We thus demonstrate that P-ETOF can be used to measure the number of identical microspheres in the active region of a narrow channel device. In the latter context, a future application of P-ETOF as a signal transduction mechanism in biosensors is outlined.

Electrochemistry of TEMPO in the aqueous liquid/vapor interfacial region: measurements of the lateral mobility and kinetics of surface partitioning.

A new method is described to simultaneously determine the kinetics of surface partitioning and the lateral diffusion constant of redox active amphiphiles. It concerns water-soluble amphiphiles for which the surface adsorption equilibrium constant and the solution diffusion constant are measured independently. The method involves cyclic voltammetric experiments carried out at the air/water interface with microband electrodes aligned with the plane of the water surface. Typically, 100 nm wide, 1.0 cm long microband electrodes are fabricated by the vacuum vapor deposition of gold films on glass. The front face of the electrode substrates are coated with impermeable, dimensionally stable, polymer barrier films with thickness L in the range of approximately 0.1-1.0 microm. Fracturing such gold-coated glass substrates exposes gold microbands. The recorded voltammetric current sensitively depends on the barrier film thickness, the surfactant surface diffusion constant, Dsurf, and its rate constant of desorption, kdes. For a given surfactant, such as the nitroxyl piperidine free radical TEMPO featured in this report, large currents are observed with microband electrodes that do not carry a barrier film (L = 0). This is because the surfactant surface population diffusing along the air/water interface can be directly electro-oxidized at the edge of the microband. Smaller currents are measured in the presence of a barrier film, since, in those instances, the surface population may contribute to the voltammetric current only via a mechanism involving surfactant desorption from the water surface into bulk, where it contributes to the three-dimensional solution diffusion processes. The quantitative interpretation of the voltammetric experiments was made possible with finite element simulations with FEMLAB. These produce a set of calibration curves, Dsurf versus log kdes, for each value of the barrier film thickness. The intersection of the calibration curves determines the unique values of Dsurf and kdes. For TEMPO, Dsurf = 4.4 +/- 1.2 x 10(-5) cm2/s and kdes >/= 2 x 10(4) s(-1). Surfactant desorption rate constants of this magnitude have not been previously experimentally accessible. Since, in our earlier report (Wu, D. G.; Malec, A. D.; Head-Gordon, M.; Majda, M. J. Am. Chem. Soc. 2005, 27, 4490-4496), we showed that TEMPO is not immersed in water and that it diffuses along the interface hydrogen-bonded to just one or two water molecules, its Dsurf value approximates the water diffusion constant in the aqueous liquid-vapor interfacial region.