Phospholipid bilayer surface configuration probed quantitatively by
            <sup>31</sup>
            P field-cycling NMR

Roberts, Mary F.; Redfield, Alfred G.

doi:10.1073/pnas.0407565101

Cited by 41 publications

(176 citation statements)

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“…25 In samples where phospholipid vesicles or large rod-shaped micelles form (e.g., diC 7 PC), there is a distinct rise in R 1 detected at very low fields (<0.06 T). 26 When well-separated from the nanosecond dispersion, a correlation time, τ v , that may reflect the contribution of particle tumbling to relaxation can be extracted. It has been proposed that τ v is equal to the rotational correlation time D r /6 where D r is the rotational diffusion constant of the individual lipid due to both diffusion of the entire aggregate, and translational diffusion of individual lipids relative to the aggregate.…”

Section: Characterization Of Dic 8 Pi Compoundsmentioning

confidence: 99%

“…It has been proposed that τ v is equal to the rotational correlation time D r /6 where D r is the rotational diffusion constant of the individual lipid due to both diffusion of the entire aggregate, and translational diffusion of individual lipids relative to the aggregate. 26 For micelles as opposed to vesicles, a detailed analysis is complicated by the fact that monomers and micelles coexist in fast exchange and that many micelles are usually rod-shaped rather than spherical. Nonetheless, the line shape of the R 1 versus field profile can indicate that micelles form, and whether they are large (such that a low field rise in R 1 is observed) or are small (in which case no low field rise is detected, but a minimum in rate at 1-2 T, suggesting a several ns correlation time).…”

Section: Characterization Of Dic 8 Pi Compoundsmentioning

confidence: 99%

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Insights into the Structural Specificity of the Cytotoxicity of 3-Deoxyphosphatidylinositols

et al. 2008

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D-3-Deoxy-phosphatidylinositol derivatives have cytotoxic activity against various human cancer cell lines. These phosphatidylinositols have a potentially wide array of targets in the phosphatidylinositol-3-kinase (PI3K)/Akt signaling network. To explore the specificity of these types of molecules, we have synthesized D-3-deoxy-dioctanoylphosphatidylinositol (D-3-deoxydiC 8 PI), D-3,5-dideoxy-diC 8 PI and D-3-deoxy-dioctanoylphosphatidylinositol-5-phosphate and their enantiomers, characterized their aggregate formation by novel high resolution field cycling 31 P NMR, and examined their susceptibility to phospholipase C (PLC) and their effects on the catalytic activity of PI3K and PTEN against diC 8 PI and dioctanoylphosphatidylinositol-3-phosphate substrates, respectively, as well as their ability to induce the death of the U937 human leukemic monocyte lymphoma cells. Of these molecules, only D-3-deoxy-diC 8 PI was able to promote cell death; it did so with an IC 50 of 40 μM, well below the CMC of 0.4 mM. Under these conditions, there was little inhibition of PI3K or PTEN observed in assays of recombinant enzymes (although the complete series of deoxy-PI compounds did provide insights into ligand binding by PTEN). The D-3-deoxydiC 8 PI was a poor substrate and not an inhibitor of the PLC enzymes. The in vivo results are consistent with the current thought that the PI analogue acts on Akt1 since the transcription initiation factor eIF4e, which is a downstream signaling target of the PI3K/Akt pathway, exhibited reduced phosphorylation on Ser209. Phosphorylation of Akt1 on Ser473, but not Thr308, was reduced. Since the potent cytotoxicity for U937 cells is completely lost with the L-3-deoxy-diC 8 PI as well as with modification of the hydroxyl group at the inositol C5 (either replacing the -OH with a hydrogen or phosphorylating it) in D-3-deoxy-diC 8 PI, both chirality of the phosphoinositol moiety and the hydroxyl group at C5 are major determinants of 3-deoxy-PI binding to its target in cells.

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Section: Characterization Of Dic 8 Pi Compoundsmentioning

confidence: 99%

Section: Characterization Of Dic 8 Pi Compoundsmentioning

confidence: 99%

Insights into the Structural Specificity of the Cytotoxicity of 3-Deoxyphosphatidylinositols

et al. 2008

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“…To cycle the magnetic field, the sample is mechanically shuttled between the center high field region of the commercial NMR magnet's probe and a substantially lower magnetic field located above the probe before and after the delay times normally used in conventional NMR relaxation sequences (8). Analysis of the field dependence of spin lattice relaxation rates over a wide field range (0.002-11.7 T) provides several correlation times () for each phospholipid molecule on time scales ranging from ps to s and also allows us to separate dipolar and CSA interactions (8,9). Of particular interest is the intermediate [5][6][7][8][9][10] ns c that appears to be dominated by the wobbling of each phospholipid in the membrane (10).…”

mentioning

confidence: 99%

“…Analysis of the field dependence of spin lattice relaxation rates over a wide field range (0.002-11.7 T) provides several correlation times () for each phospholipid molecule on time scales ranging from ps to s and also allows us to separate dipolar and CSA interactions (8,9). Of particular interest is the intermediate [5][6][7][8][9][10] ns c that appears to be dominated by the wobbling of each phospholipid in the membrane (10). This c provides a direct probe of lipid dynamics in these multicomponent membranes.…”

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confidence: 99%

“…Thus, FCS allows us to screen different phospholipid compositions and to identify conditions that can be studied in detail by other techniques aimed at probing how protein binding alters the lipid environment. One such technique is high resolution field cycling 31 P NMR spectroscopy (fc-P-NMR) (8,9). Bacterial PI-PLCs recognize the headgroups of substrate, substrate analogue, and activator phospholipids, making 31 P NMR an obvious choice for studying protein-lipid interactions.…”

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confidence: 99%

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Correlation of Vesicle Binding and Phospholipid Dynamics with Phospholipase C Activity

Fang

Redfield

et al. 2009

Journal of Biological Chemistry

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The enzymatic activity of the peripheral membrane protein, phosphatidylinositol-specific phospholipase C (PI-PLC), is increased by nonsubstrate phospholipids with the extent of enhancement tuned by the membrane lipid composition. For Bacillus thuringiensis PI-PLC, a small amount of phosphatidylcholine (PC) activates the enzyme toward its substrate PI; above 0.5 mol fraction PC (X PC ), enzyme activity decreases substantially. To provide a molecular basis for this PC-dependent behavior, we used fluorescence correlation spectroscopy to explore enzyme binding to multicomponent lipid vesicles composed of PC and anionic phospholipids (that bind to the active site as substrate analogues) and high resolution field cycling 31 P NMR methods to estimate internal correlation times ( c ) of phospholipid headgroup motions. PI-PLC binds poorly to pure anionic phospholipid vesicles, but 0.1 X PC significantly enhances binding, increases PI-PLC activity, and slows nanosecond rotational/wobbling motions of both phospholipid headgroups, as indicated by increased c . PI-PLC activity and phospholipid c are constant between 0.1 and 0.5 X PC . Above this PC content, PI-PLC has little additional effect on the substrate analogue but further slows the PC c , a motional change that correlates with the onset of reduced enzyme activity. For PC-rich bilayers, these changes, together with the reduced order parameter and enhanced lateral diffusion of the substrate analogue in the presence of PI-PLC, imply that at high X PC , kinetic inhibition of PI-PLC results from intravesicle sequestration of the enzyme from the bulk of the substrate. Both methodologies provide a detailed view of protein-lipid interactions and can be readily adapted for other peripheral membrane proteins.Bacterial phosphatidylinositol-specific phospholipase C (PI-PLC) 2 enzymes aid in organism infectivity (1), whereas the structurally homologous mammalian PLC␦1 and related enzymes are required for phosphoinositide metabolism and are important for intracellular signaling (2, 3). These peripheral membrane proteins often have distinct binding modes for substrates and for other lipids that either anchor the protein to the surface or adjust its conformation to enhance catalysis (4). However, using traditional methods, it has been difficult to determine how lipid composition affects phospholipase binding and, conversely, how protein binding alters the lipid environment, particularly in multicomponent vesicles. Current methods for monitoring peripheral membrane protein binding to mixed component lipid vesicles, including centrifugation, gel filtration, and NMR, can provide information on bulk protein partitioning but do not usually provide insight into how the properties of the individual phospholipids change when protein is bound. Most of these methods also require protein concentrations well above the amounts used in enzyme kinetics. Therefore, even when binding to multicomponent vesicles can be measured, it has been difficult to separate how substrates (or substrate analogues)...

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“Seeing” Lipid Membranes by Solid-State NMR

Castro

NATO Security Through Science Series

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Phospholipid bilayer surface configuration probed quantitatively by ³¹ P field-cycling NMR

Cited by 41 publications

References 23 publications

Insights into the Structural Specificity of the Cytotoxicity of 3-Deoxyphosphatidylinositols

Insights into the Structural Specificity of the Cytotoxicity of 3-Deoxyphosphatidylinositols

Correlation of Vesicle Binding and Phospholipid Dynamics with Phospholipase C Activity

“Seeing” Lipid Membranes by Solid-State NMR

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Phospholipid bilayer surface configuration probed quantitatively by 31 P field-cycling NMR

Cited by 41 publications

References 23 publications

Insights into the Structural Specificity of the Cytotoxicity of 3-Deoxyphosphatidylinositols

Insights into the Structural Specificity of the Cytotoxicity of 3-Deoxyphosphatidylinositols

Correlation of Vesicle Binding and Phospholipid Dynamics with Phospholipase C Activity

“Seeing” Lipid Membranes by Solid-State NMR

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Phospholipid bilayer surface configuration probed quantitatively by ³¹ P field-cycling NMR