Your search keyword '"Amphipathic peptide"' showing total 7 results

1. A synthetic low density lipoprotein particle capable of supporting U937 proliferation in vitro

Author

G. Baillie, M.D. Owens, and G.W. Halbert

Subjects

U937, low density lipoprotein, amphipathic peptide, apoB, synthetic LDL, phosphate-buffered saline, Biochemistry, QD415-436

Abstract

A synthetic LDL (sLDL) has been prepared by combining a lipid microemulsion with amphipathic peptides containing the apoprotein B receptor domain. The biological properties of sLDL have been investigated using the U937 in vitro cell proliferation assay. sLDL exhibits a concentration dependent and saturable stimulation of U937 proliferation. By utilizing different amphipathic peptides, variable proliferation is achieved, indicating a specific interaction between sLDL and the U937 LDL receptor are possible. U937 proliferation is reduced by the addition of an anti-LDL receptor antibody, indicating that sLDL is assimilated via the LDL receptor pathway. The behavior of sLDL mimics that of native LDL, and this approach represents a viable technique for the production of an sLDL particle on a large scale for research and general application. —Baillie, G., M. D. Owens, and G. W. Halbert. A synthetic low density lipoprotein particle capable of supporting U937 proliferation in vitro. J. Lipid Res. 2002. 43: 69–73.

Published

2002

2. Peptides derived from the C-terminal domain of HIV-1 Viral Protein R in lipid bilayers: Structure, membrane positioning and gene delivery.

Author

Marquette A, Leborgne C, Schartner V, Salnikov E, Bechinger B, and Kichler A

Subjects

Amino Acid Substitution, Cell-Penetrating Peptides genetics, Cell-Penetrating Peptides metabolism, HEK293 Cells, HIV-1 chemistry, Humans, Isoleucine chemistry, Isoleucine genetics, Proline chemistry, Proline genetics, Protein Binding, Protein Conformation, alpha-Helical, Protein Multimerization, vpr Gene Products, Human Immunodeficiency Virus genetics, vpr Gene Products, Human Immunodeficiency Virus metabolism, Cell-Penetrating Peptides chemistry, Gene Transfer Techniques, Lipid Bilayers chemistry, vpr Gene Products, Human Immunodeficiency Virus chemistry

Abstract

Viral protein R (Vpr) is a small accessory protein of 96 amino acids that is present in Human and simian immunodeficiency viruses. Among the very different properties that Vpr possesses we can find cell penetrating capabilities. Based on this and on its capacity to interact with nucleic acids we previously investigated the DNA transfection properties of Vpr and subfragments thereof. We found that fragments of the C-terminal helical domain of Vpr are able to deliver efficiently plasmid DNA into different cell lines. As the amphipathic helix may play a role in the interactions with membranes, we investigated whether insertion of a proline residue in the α-helix modifies the transfection properties of Vpr. Unexpectedly, we found that the resulting Vpr55-82 Pro70 peptide was even more efficient than wild type Vpr55-82 in the gene delivery assays. Using circular dichroism, light scattering and solid-state NMR techniques, we characterized the secondary structure and interactions of Vpr and several mutants with model membranes. A model is proposed where the proline shifts the dissociation equilibrium of the peptide-cargo complex and thereby its endosomal release., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2020

3. Envelope-deforming antiviral peptide derived from influenza virus M2 protein.

Author

Jung Y, Kong B, Moon S, Yu SH, Chung J, Ban C, Chung WJ, Kim SG, and Kweon DH

Subjects

Amino Acid Sequence, Animals, Antiviral Agents chemical synthesis, Cell Membrane chemistry, Cell Membrane virology, Dogs, Hydrophobic and Hydrophilic Interactions, Influenza A Virus, H1N1 Subtype growth & development, Influenza A Virus, H1N1 Subtype ultrastructure, Inhibitory Concentration 50, Lipid Bilayers chemistry, Liposomes chemistry, Madin Darby Canine Kidney Cells, Peptides chemical synthesis, Structure-Activity Relationship, Viral Load drug effects, Antiviral Agents pharmacology, Cell Membrane drug effects, Influenza A Virus, H1N1 Subtype drug effects, Peptides pharmacology, Viral Matrix Proteins chemistry

Abstract

Molecules interfering with lipid bilayer function exhibit strong antiviral activity against a broad range of enveloped viruses, with a lower risk of resistance development than that for viral protein-targeting drugs. Amphipathic peptides are rich sources of such membrane-interacting antivirals. Here, we report that influenza viruses were effectively inactivated by M2 AH, an amphipathic peptide derived from the M2 protein of the influenza virus. Although overall hydrophobicity () of M2 AH was not related to antiviral activity, modification of the hydrophobic moment (<μH>) of M2 AH dramatically altered the antiviral activity of this peptide. M2 MH, a derivative of M2 AH with a <μH> of 0.874, showed a half maximal inhibitory concentration (IC 50 ) of 53.3 nM against the A/PR/8/34 strain (H1N1), which is 16-times lower than that of M2 AH. The selectivity index (IC 50 /CC 50 ), where CC 50 is the half maximal cytotoxic concentration, was 360 for M2 MH and 81 for M2 AH. Dynamic light scattering spectroscopy and electron microscopy revealed that M2 AH-derived peptides did not disrupt liposomes but altered the shape of viruses. This result suggests that the shape of virus envelope was closely related to its activity. Thus, we propose that deforming without rupturing the membranes may achieve a high selectivity index for peptide antivirals., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published

2019

4. Simultaneous membrane interaction of amphipathic peptide monomers, self-aggregates and cargo complexes detected by fluorescence correlation spectroscopy.

Author

Vasconcelos L, Lehto T, Madani F, Radoi V, Hällbrink M, Vukojević V, and Langel Ü

Subjects

Amino Acid Sequence, Animals, Biological Transport, Carbocyanines chemistry, Cell-Penetrating Peptides chemistry, Cell-Penetrating Peptides genetics, Hydrophobic and Hydrophilic Interactions, Lipopeptides chemistry, Lipopeptides genetics, Lipopeptides metabolism, Microscopy, Fluorescence, PC12 Cells, Protein Binding, RNA, Small Interfering chemistry, RNA, Small Interfering genetics, RNA, Small Interfering metabolism, Rats, Rhodamines chemistry, Cell Membrane metabolism, Cell-Penetrating Peptides metabolism, Protein Aggregates, Spectrometry, Fluorescence methods

Abstract

Peptides able to translocate cell membranes while carrying macromolecular cargo, as cell-penetrating peptides (CPPs), can contribute to the field of drug delivery by enabling the transport of otherwise membrane impermeable molecules. Formation of non-covalent complexes between amphipathic peptides and oligonucleotides is driven by electrostatic and hydrophobic interactions. Here we investigate and quantify the coexistence of distinct molecular species in multiple equilibria, namely peptide monomer, peptide self-aggregates and peptide/oligonucleotide complexes. As a model for the complexes, we used a stearylated peptide from the PepFect family, PF14 and siRNA. PF14 has a cationic part and a lipid part, resembling some characteristics of cationic lipids. Fluorescence correlation spectroscopy (FCS) and fluorescence cross-correlation spectroscopy (FCCS) were used to detect distinct molecular entities in solution and at the plasma membrane of live cells. For that, we labeled the peptide with carboxyrhodamine 6G and the siRNA with Cyanine 5. We were able to detect fluorescent entities with diffusional properties characteristic of the peptide monomer as well as of peptide aggregates and peptide/oligonucleotide complexes. Strategies to avoid peptide adsorption to solid surfaces and self-aggregation were developed and allowed successful FCS measurements in solution and at the plasma membrane. The ratio between the detected molecular species was found to vary with pH, peptide concentration and the proximity to the plasma membrane. The present results suggest that the diverse cellular uptake mechanisms, often reported for amphipathic CPPs, might result from the synergistic effect of peptide monomers, self-aggregates and cargo complexes, distributed unevenly at the plasma membrane., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2018

5. Vectofusin-1, a potent peptidic enhancer of viral gene transfer forms pH-dependent α-helical nanofibrils, concentrating viral particles.

Author

Vermeer LS, Hamon L, Schirer A, Schoup M, Cosette J, Majdoul S, Pastré D, Stockholm D, Holic N, Hellwig P, Galy A, Fenard D, and Bechinger B

Subjects

Cell Line, Humans, Lentivirus, Nanofibers chemistry, Peptides chemistry, Peptides pharmacology, Transduction, Genetic methods, Virion chemistry

Abstract

Gene transfer using lentiviral vectors has therapeutic applications spanning from monogenic and infectious diseases to cancer. Such gene therapy has to be improved by enhancing the levels of viral infection of target cells and/or reducing the amount of lentivirus for greater safety and reduced costs. Vectofusin-1, a recently developed cationic amphipathic peptide with a pronounced capacity to enhance such viral transduction, strongly promotes the entry of several retroviral pseudotypes into target cells when added to the culture medium. To clarify the molecular basis of its action the peptide was investigated on a molecular and a supramolecular level by a variety of biophysical approaches. We show that in culture medium vectofusin-1 rapidly forms complexes in the 10 nm range that further assemble into annular and extended nanofibrils. These associate with viral particles allowing them to be easily pelleted for optimal virus-cell interaction. Thioflavin T fluorescence, circular dichroism and infrared spectroscopies indicate that these fibrils have a unique α-helical structure whereas most other viral transduction enhancers form β-amyloid fibrils. A vectofusin-1 derivative (LAH2-A4) is inefficient in biological assays and does not form nanofibrils, suggesting that supramolecular assembly is essential for transduction enhancement. Our observations define vectofusin-1 as a member of a new class of α-helical enhancers of lentiviral infection. Its fibril formation is reversible which bears considerable advantages in handling the peptide in conditions well-adapted to Good Manufacturing Practices and scalable gene therapy protocols., (Copyright © 2017 Acta Materialia Inc. Published by Elsevier Ltd. All rights reserved.)

Published

2017

6. Amphiphilic peptide-loaded nanofibrous calcium phosphate microspheres promote hemostasis in vivo.

Author

Wu J, Lemarié CA, Barralet J, and Blostein MD

Subjects

Adsorption, Animals, Factor X metabolism, Liver drug effects, Liver pathology, Male, Mice, Mice, Inbred C57BL, Tail, Calcium Phosphates chemistry, Hemostasis drug effects, Hemostatics pharmacology, Microspheres, Nanofibers chemistry, Peptides pharmacology, Surface-Active Agents pharmacology

Abstract

Most fatalities from trauma occur due to severe blood loss. There is a need for improved hemostatic biomaterials that can address this problem. The aim of this study was to determine the in vivo efficacy of nanofibrous microspheres (NFM) loaded with hemostatic peptides, specifically ideal amphipathic peptides (IAP) that have been demonstrated to possess both procoagulant and antifibrinolyic activities. We demonstrate that IAP can be coupled to NFM (IAP-NFM) to form matrices that exhibit substantial hemostatic activity. IAP-NFM matrices were compared to a commercial zeolitic hemostatic biomaterial (QuikClot) and have superior efficacy in reducing bleeding in vivo. In both a murine tail transection and a murine hepatic injury model, bleeding times were significantly reduced (P<0.05) with the use of IAP-NFM as compared with equal masses of either QuikClot or NFM alone, or no treatment. Importantly, histological examination revealed no tissue injury when IAP-NFM or NFM were applied to hepatic lacerations. In contrast, QuikClot caused widespread hepatocyte degeneration and necrosis, with higher average injury zone thickness as determined by semiquantitative analysis. In summary, NFM was able to maintain the pro-coagulant properties of IAP in our preclinical model, caused no observable tissue damage at the site of application and had better performance than QuikClot controls., (Copyright © 2013 Acta Materialia Inc. Published by Elsevier Ltd. All rights reserved.)

Published

2013

7. A fluorescence method to detect and quantitate sterol esterification by lecithin:cholesterol acyltransferase.

Author

Homan R, Esmaeil N, Mendelsohn L, and Kato GJ

Subjects

Anemia, Sickle Cell blood, Anemia, Sickle Cell enzymology, Cholesterol analysis, Enzyme Activation, Esterification, Humans, Phosphatidylcholine-Sterol O-Acyltransferase blood, Sterols chemistry, Time Factors, Fluorescence, Phosphatidylcholine-Sterol O-Acyltransferase metabolism, Sterols analysis, Sterols metabolism

Abstract

We describe a simple but sensitive fluorescence method to accurately detect the esterification activity of lecithin:cholesterol acyltransferase (LCAT). The new assay protocol employs a convenient mix, incubate, and measure scheme. This is possible by using the fluorescent sterol dehydroergosterol (DHE) in place of cholesterol as the LCAT substrate. The assay method is further enhanced by incorporation of an amphiphilic peptide in place of apolipoprotein A-I as the lipid emulsifier and LCAT activator. Specific fluorescence detection of DHE ester synthesis is achieved by employing cholesterol oxidase to selectively render unesterified DHE nonfluorescent. The assay accurately detects LCAT activity in buffer and in plasma that is depleted of apolipoprotein B lipoproteins by selective precipitation. Analysis of LCAT activity in plasmas from control subjects and sickle cell disease (SCD) patients confirms previous reports of reduced LCAT activity in SCD and demonstrates a strong correlation between plasma LCAT activity and LCAT content. The fluorescent assay combines the sensitivity of radiochemical assays with the simplicity of nonradiochemical assays to obtain accurate and robust measurement of LCAT esterification activity., (Copyright © 2013 Elsevier Inc. All rights reserved.)

Published

2013