Fragments of the human antimicrobial LL-37 and their interaction with model membranes

Dannehl, Claudia

January 2013

A detailed description of the characteristics of antimicrobial peptides (AMPs) is highly demanded, since the resistance against traditional antibiotics is an emerging problem in medicine. They are part of the innate immune system in every organism, and they are very efficient in the protection against bacteria, viruses, fungi and even cancer cells. Their advantage is that their target is the cell membrane, in contrast to antibiotics which disturb the metabolism of the respective cell type. This allows AMPs to be more active and faster. The lack of an efficient therapy for some cancer types and the evolvement of resistance against existing antitumor agents make AMPs promising in cancer therapy besides being an alternative to traditional antibiotics. The aim of this work was the physical-chemical characterization of two fragments of LL-37, a human antimicrobial peptide from the cathelicidin family. The fragments LL-32 and LL-20 exhibited contrary behavior in biological experiments concerning their activity against bacterial cells, human cells and human cancer cells. LL-32 had even a higher activity than LL-37, while LL-20 had almost no effect. The interaction of the two fragments with model membranes was systematically studied in this work to understand their mode of action. Planar lipid films were mainly applied as model systems in combination with IR-spectroscopy and X-ray scattering methods. Circular Dichroism spectroscopy in bulk systems completed the results. In the first approach, the structure of the peptides was determined in aqueous solution and compared to the structure of the peptides at the air/water interface. In bulk, both peptides are in an unstructured conformation. Adsorbed and confined to at the air-water interface, the peptides differ drastically in their surface activity as well as in the secondary structure. While LL-32 transforms into an α-helix lying flat at the water surface, LL-20 stays partly unstructured. This is in good agreement with the high antimicrobial activity of LL-32. In the second approach, experiments with lipid monolayers as biomimetic models for the cell membrane were performed. It could be shown that the peptides fluidize condensed monolayers of negatively charged DPPG which can be related to the thinning of a bacterial cell membrane. An interaction of the peptides with zwitterionic PCs, as models for mammalian cells, was not clearly observed, even though LL-32 is haemolytic. In the third approach, the lipid monolayers were more adapted to the composition of human erythrocyte membranes by incorporating sphingomyelin (SM) into the PC monolayers. Physical-chemical properties of the lipid films were determined and the influence of the peptides on them was studied. It could be shown that the interaction of the more active LL-32 is strongly increased for heterogeneous lipid films containing both gel and fluid phases, while the interaction of LL-20 with the monolayers was unaffected. The results indicate an interaction of LL-32 with the membrane in a detergent-like way. Additionally, the modelling of the peptide interaction with cancer cells was performed by incorporating some negatively charged lipids into the PC/SM monolayers, but the increased charge had no effect on the interaction of LL-32. It was concluded, that the high anti-cancer activity of the peptide originates from the changed fluidity of cell membrane rather than from the increased surface charge. Furthermore, similarities to the physical-chemical properties of melittin, an AMP from the bee venom, were demonstrated. / Aufgrund der steigenden Resistenzen von Zellstämmen gegen traditionelle Therapeutika sind alternative medizinische Behandlungsmöglichkeiten für bakterielle Infektionen und Krebs stark gefragt. Antimikrobielle Peptide (AMPs) sind Bestandteil der unspezifischen Immunabwehr und kommen in jedem Organismus vor. AMPs lagern sich von außen an die Zellmembran an und zerstören ihre Integrität. Das macht sie effizient und vor allem schnell in der Wirkung gegen Bakterien, Viren, Pilzen und sogar Krebszellen. Das Ziel dieser Arbeit lag in der physikalisch-chemischen Charakterisierung zweier Peptidfragmente die unterschiedliche biologische Aktivität aufweisen. Die Peptide LL-32 und LL-20 waren Teile des humanen LL-37 aus der Kathelizidin-Familie. LL-32 wies eine stärke Aktivität als das Mutterpeptid auf, während LL-20 kaum aktiv gegen die verschiedenen Zelltypen war. In dieser Arbeit wurde die Wechselwirkung der Peptide mit Zellmembranen systematisch anhand von zweidimensionalen Modellmembranen in dieser Arbeit untersucht. Dafür wurden Filmwaagenmessungen mit IR-spektroskopischen und Röntgenstreumethoden gekoppelt. Circulardichroismus-Spektroskopie im Volumen komplementierte die Ergebnisse. In der ersten Näherung wurde die Struktur der Peptide in Lösung mit der Struktur an der Wasser/Luft-Grenzfläche verglichen. In wässriger Lösung sind beide Peptidfragmente unstrukturiert, nehmen jedoch eine α-helikale Sekundärstruktur an, wenn sie an die Wasser/Luft-Grenzfläche adsorbiert sind. Das biologisch unwirksamere LL-20 bleibt dabei teilweise ungeordnet. Das steht im Zusammenhang mit einer geringeren Grenzflächenaktivität des Peptids. In der Zweiten Näherung wurden Versuche mit Lipidmonoschichten als biomimetisches Modell für die Wechselwirkung mit der Zellmembran durchgeführt. Es konnte gezeigt werden, dass sich die Peptide fluidisierend auf negativ geladene Dipalmitylphosphatidylglycerol (DPPG) Monoschichten auswirken, was einer Membranverdünnung an Bakterienzellen entspricht. Eine Interaktion der Peptide mit zwitterionischem Phosphatidylcholin (PC), das als Modell für Säugetierzellen verwendet wurde, konnte nicht klar beobachtet werden, obwohl biologische Experimente das hämolytische Verhalten zumindest von LL-32 zeigten. In der dritten Näherung wurde das Membranmodell näher an die Membran von humanen Erythrozyten angepasst, indem gemischte Monoschichten aus Sphingomyelin (SM) und PC hergestellt wurden. Die physikalisch-chemischen Eigenschaften der Lipidfilme wurden zunächst ausgearbeitet und anschließend der Einfluss der Peptide untersucht. Es konnte anhand verschiedener Versuche gezeigt werden, dass die Wechselwirkung von LL-32 mit der Modellmembran verstärkt ist, wenn eine Koexistenz von fluiden und Gelphasen auftritt. Zusätzlich wurde die Wechselwirkung der Peptide mit der Membran von Krebszellen imitiert, indem ein geringer Anteil negativ geladener Lipide in die Monoschicht eingebaut wurde. Das hatte allerdings keinen nachweislichen Effekt, so dass geschlussfolgert werden konnte, dass die hohe Aktivität von LL-32 gegen Krebszellen ihren Grund in der veränderten Fluidität der Membran hat und nicht in der veränderten Oberflächenladung. Darüber hinaus wurden Ähnlichkeiten zu Melittin, einem AMP aus dem Bienengift, dargelegt. Die Ergebnisse dieser Arbeit sprechen für einen Detergenzien-artigen Wirkmechanismus des Peptids LL-32 an der Zellmembran.

Antimikrobielle Peptide

Zellmembranen

Lipide

Peptid-Membran-Wechselwirkung

Monoschichten

Antimicrobial Peptides

Membranes

Lipids

Peptide-Membrane-Interaction

Monolayer

Life sciences

Crumbs Affects Protein Dynamics In Anterior Regions Of The Developing Drosophila Embryo

Knust, Elisabeth, Firmino, João, Tinevez, Jean-Yves

18 January 2016

Maintenance of apico-basal polarity is essential for epithelial integrity and requires particular reinforcement during tissue morphogenesis, when cells are reorganised, undergo shape changes and remodel their junctions. It is well established that epithelial integrity during morphogenetic processes depends on the dynamic exchange of adherens junction components, but our knowledge on the dynamics of other proteins and their dynamics during these processes is still limited. The early Drosophila embryo is an ideal system to study membrane dynamics during morphogenesis. Here, morphogenetic activities differ along the anterior-posterior axis, with the extending germband showing a high degree of epithelial remodelling. We developed a Fluorescence Recovery After Photobleaching (FRAP) assay with a higher temporal resolution, which allowed the distinction between a fast and a slow component of recovery of membrane proteins during the germband extension stage. We show for the first time that the recovery kinetics of a general membrane marker, SpiderGFP, differs in the anterior and posterior parts of the embryo, which correlates well with the different morphogenetic activities of the respective embryonic regions. Interestingly, absence of crumbs, a polarity regulator essential for epithelial integrity in the Drosophila embryo, decreases the fast component of SpiderGFP and of the apical marker Stranded at Second-Venus specifically in the anterior region. We suggest that the defects in kinetics observed in crumbs mutant embryos are the first signs of tissue instability in this region, explaining the earlier breakdown of the head epidermis in comparison to that of the trunk, and that diffusion in the plasma membrane is affected by the absence of Crumbs.

Zellmembranen

Embryonen

Membranproteine

Embryos

Cell membranes

Membrane proteins

Drosophila melanogaster

Cell polarity

Curve fitting

Integral membrane proteins

ddc:610

rvk:XA 10000

The Role of Phosphoinositides in the Interaction of Myelin Basic Protein with the Oligodendroglial Cell Membrane / Die Rolle von Phosphoinositolen für die Interaction von Myelin Basisches Protein mit der Oliglodendrozyten-Zellmembran

Nawaz, Schanila

09 January 2009

No description available.

570 Biowissenschaften

Biologie

Myelin

Lipide

Signalwege

Myelin

Lipids

signalling

42.00

WHC 100: Zellmembranen

Zelloberfläche

Zellwand

intrazelluläre Membranen {Cytologie}

Crumbs Affects Protein Dynamics In Anterior Regions Of The Developing Drosophila Embryo

Knust, Elisabeth, Firmino, João, Tinevez, Jean-Yves

18 January 2016

Maintenance of apico-basal polarity is essential for epithelial integrity and requires particular reinforcement during tissue morphogenesis, when cells are reorganised, undergo shape changes and remodel their junctions. It is well established that epithelial integrity during morphogenetic processes depends on the dynamic exchange of adherens junction components, but our knowledge on the dynamics of other proteins and their dynamics during these processes is still limited. The early Drosophila embryo is an ideal system to study membrane dynamics during morphogenesis. Here, morphogenetic activities differ along the anterior-posterior axis, with the extending germband showing a high degree of epithelial remodelling. We developed a Fluorescence Recovery After Photobleaching (FRAP) assay with a higher temporal resolution, which allowed the distinction between a fast and a slow component of recovery of membrane proteins during the germband extension stage. We show for the first time that the recovery kinetics of a general membrane marker, SpiderGFP, differs in the anterior and posterior parts of the embryo, which correlates well with the different morphogenetic activities of the respective embryonic regions. Interestingly, absence of crumbs, a polarity regulator essential for epithelial integrity in the Drosophila embryo, decreases the fast component of SpiderGFP and of the apical marker Stranded at Second-Venus specifically in the anterior region. We suggest that the defects in kinetics observed in crumbs mutant embryos are the first signs of tissue instability in this region, explaining the earlier breakdown of the head epidermis in comparison to that of the trunk, and that diffusion in the plasma membrane is affected by the absence of Crumbs.

info:eu-repo/classification/ddc/610

ddc:610

Der Syntaxin 1-Cluster - Organisation und Dynamik einer supramolekularen Struktur der Plasmamembran / The Syntaxin 1 Cluster - Organisation and Dynamics of a plasmalemmal supramolecular structure

Sieber, Jochen Josef

04 May 2007

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

Syntaxin

Membran

Plasmamembran

Mikrodomäne

Membrane-Patterning

Membrane-Raft

SNARE

syntaxin

membrane

plasma membrane

microdomain

membrane patterning

membrane raft

SNARE

42.15

Distinct roles of PI4P 5-kinase isoforms in polar tip growth of pollen tubes / Unterschiedliche Funktionen von PI4P 5-Kinasen in der Kontrolle des polaren Spitzenwachstums von Pollenschläuchen

Ischebeck, Till

29 October 2008

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

Pollenschlauch

Phosphoinositide

Phosphatidylinositol-4-phosphat 5-Kinase

polares Wachstum

Pektinsekretion

pollen tube

phosphoinositides

polar growth

pectin secretion

42.15

42.42

Fluoreszenzmikroskopische Studien an Plasmamembranen zur Untersuchung der molekularen Mechanismen der neuronalen Exocytose / Fluorescence Microscopy Studies of Plasma Membranes to Analyse the Molecular Machinery of Neuronal Exocytosis

Zilly, Felipe Emilio

06 July 2006

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

SNARE

Syntaxin

Munc18

Exocytose

PC12

SNARE

syntaxin

Munc18

exocytosis

PC12

35.70

42.13

42.15

Subcellular localization of Kv10.1 (Eag1): functional ion channels on the inner nuclear membrane / Subzelluläre Lokalisation von Kv10.1 (Eag1): funktionelle Ionenkanäle auf der inneren Kernmembran

Chen, Ye

29 April 2010

No description available.

570 Biowissenschaften

Biologie

Eag1

Kv10.1

Kaliumkanal

Tumoren

Gehirm

Subzelluläre Lokalisation

inneren Kernmembran

Eag1

Kv10.1

potassium channel

tumor

brain

subcellular localization

inner nuclear membrane

44.90

WHC 100: Zellmembranen

Zelloberfläche

Zellwand

intrazelluläre Membranen {Cytologie}

Fluoreszenzmikroskopische Studien an Plasmamembranen zur Untersuchung der molekularen Mechanismen der neuronalen Exocytose / Fluorescence Microscopy Studies of Plasma Membranes to Analyse the Molecular Machinery of Neuronal Exocytosis

Zilly, Felipe Emilio

06 July 2006

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

SNARE

Syntaxin

Munc18

Exocytose

PC12

SNARE

syntaxin

Munc18

exocytosis

PC12

35.70

42.13

42.15

Submembrane cytoskeleton-regulated assembly and functional activity of gap junctions / Funktionelle Regulation von gap junctions und ihrer Anordnung durch das Sub-membranale Zytoskelett

Butkevich, Eugenia

29 June 2004

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

Gap junctions

Connexin43

Drebrin

FRET

gap junctions

connexin43

drebrin

FRET

42.13

42.15