Role of Secondary Structure in Protein−Phospholipid Surface Interactions:  Reconstitution and Denaturation of Apolipoprotein C-I:DMPC Complexes

Benjwal, Sangeeta; Jayaraman, Sundararajan; Gursky, Olga

doi:10.1021/bi062175c

Cited by 10 publications

(34 citation statements)

References 53 publications

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“…Due to the analogous position of Glu19 in the N-terminal helix of apoC-I to glutamate residues in 22-residue amphipathic ␣ -helices of apoA-I that activate lecithin:cholesterol acyltransferase ( 29 ), the apolar face of the N-terminal helix was extended to include Glu19 and Leu8. The phospholipid-bound structure of apoC-I in proline mutagenesis studies is more consistent with the C-terminal helix, spanning residues 34-47 ( 38,39 ) instead of residues 38-52 predicted via NMR ( 18 ).…”

mentioning

confidence: 52%

“…Stock solutions were prepared by dissolving lyophilized peptides in 2 mM sodium phosphate buffer, pH 7.4 (standard buffer), to a peptide concentration of 1.0 mg/ml, as measured by Lowry assays. The helical content of aqueous peptides was verifi ed by far-UV circular dichroism (CD) ( 38 ).…”

Section: Methodsmentioning

confidence: 99%

“…On binding to phospholipid, the average helical content of apoC-I increases to 65-75%. The helical content of apoC-I in solution and on phospholipid can be altered by single Ala or Pro substitutions in either ␣ -helix ( Table 1 ) ( 37,38 ). We speculate that this is unique to small apolipoproteins, as point mutations in single helices of larger proteins would likely have little effect on protein helical content.…”

mentioning

confidence: 99%

“…Studies using apoC-I point mutants and discoidal lipoproteins reconstituted from 1, 2-dimyristoylphosphatidylcholine (DMPC) showed that, as the aqueous ␣ -helical content of apoC-I increased, the rate and temperature range of DMPC clearance increased (37)(38)(39)(40)(41). However, these studies were limited by a nonphysiologic interface [DMPC is found only in trace amounts on lipoproteins ( 42,43 )] and the inability to monitor real-time surface modifi cations induced by protein binding.…”

mentioning

confidence: 99%

“…ApoC-I is predicted to contain two class A, amphipathic ␣ -helices spanning the residues 7-29 and 34-47 ( 18,37,38 ). Fig.…”

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confidence: 99%

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Changes in helical content or net charge of apolipoprotein C-I alter its affinity for lipid/water interfaces

Meyers

Wang

Gursky

et al. 2013

Journal of Lipid Research

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mentioning

confidence: 52%

Section: Methodsmentioning

confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

“…ApoC-I is predicted to contain two class A, amphipathic ␣ -helices spanning the residues 7-29 and 34-47 ( 18,37,38 ). Fig.…”

mentioning

confidence: 99%

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Changes in helical content or net charge of apolipoprotein C-I alter its affinity for lipid/water interfaces

Meyers

Wang

Gursky

et al. 2013

Journal of Lipid Research

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Proteogenomic review of the changes in primate apoC-I during evolution

Puppione

Whitelegge

2013

Front. Biol.

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Apolipoprotein C-I has evolved more rapidly than any of the other soluble apolipoproteins. During the course of primate evolution, the gene for this apolipoprotein was duplicated. Prompted by our observation that the two resulting genes encode two distinct forms of apoC-I in great apes, we have reviewed both the genomic and proteomic data to examine what changes have occurred during the course of primate evolution. We have found data showing that one of the duplicated genes, known to be a pseudogene in humans, was also a pseudogene in Denisovans and Neandertals. Using genomic and proteomic data for primates, we will provide in this review evidence that the duplication took place after the divergence of New World monkeys from the human lineage and that the formation of the pseudogene took place after the divergence of the bonobos and chimpanzees from the human lineage.

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Apolipoprotein C-I Binds More Strongly to Phospholipid/Triolein/Water than Triolein/Water Interfaces: A Possible Model for Inhibiting Cholesterol Ester Transfer Protein Activity and Triacylglycerol-Rich Lipoprotein Uptake

2012

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ApolipoproteinC-I (apoC-I) is an important constituent of high-density lipoprotein (HDL) and is involved in the accumulation of cholesterol ester in nascent HDL by inhibiting cholesterol ester transfer protein (CETP) and potentially activating lecithin:cholesterol acyltransferase (LCAT). As the smallest exchangeable apolipoprotein (57 residues), apoC-I transfers between lipoproteins via a lipid-binding motif of two amphipathic α-helices (AαHs), spanning residues 7–29 and 38–52. To understand apoC-I’s behavior at hydrophobic lipoprotein surfaces, oil drop tensiometry was used to compare the binding to triolein/water (TO/W) and palmitoyloleoylphosphatidylcholine/triolein/water (POPC/TO/W) interfaces. When apoC-I binds to either interface, the surface tension (γ) decreases by ~16–18 mN/m. ApoC-I is exchangeable at both interfaces, desorbing upon compression and readsorbing on expansion. The maximum surface pressure at which apoC-I begins to desorb (ΠMAX) was 16.8 and 20.7 mN/m at TO/W and POPC/TO/W interfaces, respectively. This suggests that apoC-I interacts with POPC to increase affinity for the interface. ApoC-I is more elastic on POPC/TO/W than TO/W interfaces, marked by higher elasticity modulus (ε) values on oscillations. At POPC/TO/W interfaces containing an increasing POPC/TO ratio, the pressure at which apoC-I begins to be ejected increases as phospholipid surface concentration increases. The observed increase in apoC-I interface affinity due to higher degrees of apoC-I/POPC interactions may explain how apoC-I can displace larger apolipoproteins, such as apoE, from lipoproteins. These interactions allow apoC-I to remain bound to the interface at higher Πs, offering insight into apoC-I’s rearrangement on triacylglycerol-rich lipoproteins as they undergo Π changes during lipoprotein maturation by plasma factors such as lipoprotein lipase.

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Role of Secondary Structure in Protein−Phospholipid Surface Interactions: Reconstitution and Denaturation of Apolipoprotein C-I:DMPC Complexes

Cited by 10 publications

References 53 publications

Changes in helical content or net charge of apolipoprotein C-I alter its affinity for lipid/water interfaces

Changes in helical content or net charge of apolipoprotein C-I alter its affinity for lipid/water interfaces

Proteogenomic review of the changes in primate apoC-I during evolution

Apolipoprotein C-I Binds More Strongly to Phospholipid/Triolein/Water than Triolein/Water Interfaces: A Possible Model for Inhibiting Cholesterol Ester Transfer Protein Activity and Triacylglycerol-Rich Lipoprotein Uptake

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