Determination of the Stability of the Noncovalent Phospholipid Transfer Protein−Lipid Complex by Electrospray Time-of-Flight Mass Spectrometry

Brouwer, Arjan P.M. de; Versluis, Cees; Westerman, Jan; Roelofsen, B.; Heck, Albert J. R.; Wirtz, K.W.A.

doi:10.1021/bi016055a

Cited by 35 publications

(26 citation statements)

References 31 publications

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“…This coil-helix transition upon ligand binding may to some degree explain the ''tightening'' of secondary structure we observe when SCP2 is loaded with stearoyl CoA. ''Soft'' ESI-MS has frequently been used to study biomolecular complexes in a nearly native state in the gas phase, for example protein/protein [35], enzyme/cofactor [36] and protein/lipid [25,37]. We have adapted this kind of assay to analyse SCP2/lipid.…”

Section: Discussionmentioning

confidence: 99%

“…The potential between the electrospray needle and the sample cone was generally set around 1500 V and the cone voltage (CV) was varied (between 40 and 200 V) to analyse the dissociation of the complexes. Electrospray needles were prepared as described [25]. Data were collected and analysed using MassLynx 3.5 (Waters, Elstree, UK).…”

Section: Circular Dichroism Spectropolarimetrymentioning

confidence: 99%

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Investigation of the ligand spectrum of human sterol carrier protein 2 using a direct mass spectrometry assay

Stanley

Versluis

Schultz

et al. 2007

Archives of Biochemistry and Biophysics

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Sterol carrier protein 2 (SCP2) has been investigated by nearly native electrospray ionisation mass spectrometry in the presence of long chain fatty acyl CoAs (LCFA-CoAs) and carnitine derivatives of equivalent fatty acid chain length (LCFA-carnitines). Four SCP2 constructs were compared to examine the influence of the N-terminal presequence and the C-terminal peroxisomal targeting signal on ligand binding. Removal of N-or C-terminal residues did not influence ligand binding. The observation that LCFA-CoAs are high affinity ligands for SCP2 was confirmed, while LCFA-carnitines were demonstrated for the first time not to interact with SCP2. LCFACoAs formed non-covalent complexes with SCP2 of 2:1 and 1:1 stoichiometry, which could be dissociated by elevating the energy of the ions upon entrance to the mass spectrometer. A fluorescence-competition assay using Nile Red butyric acid confirmed the mass spectrometric observations in solution. The physiological significance of the lack of LCFA-carnitine binding by SCP2 is discussed.

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Section: Discussionmentioning

confidence: 99%

Section: Circular Dichroism Spectropolarimetrymentioning

confidence: 99%

Investigation of the ligand spectrum of human sterol carrier protein 2 using a direct mass spectrometry assay

Stanley

Versluis

Schultz

et al. 2007

Archives of Biochemistry and Biophysics

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“…Given the hydrogen bonding with the inositol moiety we may presume that PI is more tightly bound to the protein than PC. This was confirmed by electrospray time-of-flight mass spectrometry analysis of the PI-TPa-lipid complexes (De Brouwer et al, 2002). Both structures indicate that the sn-1 and sn-2 fatty acyl chain of either ligand occupy distinct sites with the methyl ends being close to the opening of the lipid-binding cavity which is shielded from the outside by the lipid exchange loop (helix B) and the C-terminal end (residues 261-271) as part of helix G (Fig.…”

Section: D-structure and Phospholipid Specificity Pi-tpamentioning

confidence: 56%

Phosphatidylinositol transfer proteins: From closed for transport to open for exchange

Wirtz

Schouten

Gros

2006

Advances in Enzyme Regulation

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“…NMR, UV circular dichroism, infrared spectroscopy and electron spin resonance). Nano-electrospray ionization time-of-flight mass spectroscopy (ESI-TOF) was developed to study the interaction of phospholipids with the phosphatidylinositol transfer protein alpha and the phosphatidylcholine transfer protein in the gas phase (1). Fluorescent modification of phosphatidylcholine (PC) was used to study its binding to the phosphatidylcholine transfer protein by fluorometric techniques (2).…”

Section: Introductionmentioning

confidence: 99%

Isoelectric Point Mobility Shift Assay for Rapid Screening of Charged and Uncharged Ligands Bound to Proteins

et al. 2003

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SummaryThree human proteins (hTAP1, hTAP2 and hTAP3) that are related to the yeast phosphatidylinositol/phosphatidylcholine transfer protein SEC14p were recently cloned in our laboratory. These proteins contain a relatively large hydrophobic pocket, the so called CRAL-TRIO domain, which is present also in other human proteins, such as CRALBP, a-TTP and MEG2. The CRAL-TRIO domains in these proteins bind ligands such as retinaldehyde, tocopherols and polyphosphoinositides, respectively. To screen for potential hTAPs ligands, we developed a semi-quantitative isoelectric point mobility shift assay (IPMS-assay) that allows assessing the binding of potential hydrophobic ligands to proteins. Purified proteins occupied with a charged ligand migrate differently on isoelectric focusing gels when compared with free protein.Competition of bound charged ligands with uncharged ones reverses the mobility shift, so that the relative affinities of the two ligands to the protein can be estimated.

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Determination of the Stability of the Noncovalent Phospholipid Transfer Protein−Lipid Complex by Electrospray Time-of-Flight Mass Spectrometry

Cited by 35 publications

References 31 publications

Investigation of the ligand spectrum of human sterol carrier protein 2 using a direct mass spectrometry assay

Investigation of the ligand spectrum of human sterol carrier protein 2 using a direct mass spectrometry assay

Phosphatidylinositol transfer proteins: From closed for transport to open for exchange

Isoelectric Point Mobility Shift Assay for Rapid Screening of Charged and Uncharged Ligands Bound to Proteins

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