Downloaded from orbit.dtu.dk on: Jun 18, 2017
Cholesterol – a biological compound as a building block in bionanotechnology
Hosta-Rigau, Leticia; Zhang, Yan; Teo, Boon M.; Postma, Almar; Städler, Brigitte
Published in:
Nanoscale
DOI:
10.1039/c2nr32923a
Publication date:
2013
Document Version
Final published version
Link to publication
Citation (APA):
Rigau, L. H., Zhang, Y., Teo, B. M., Postma, A., & Städler, B. (2013). Cholesterol – a biological compound as a
building block in bionanotechnology. Nanoscale, 5, 89-109. DOI: 10.1039/c2nr32923a
General rights
Copyright and moral rights for the publications made accessible in the public portal are retained by the authors and/or other copyright owners
and it is a condition of accessing publications that users recognise and abide by the legal requirements associated with these rights.
• Users may download and print one copy of any publication from the public portal for the purpose of private study or research.
• You may not further distribute the material or use it for any profit-making activity or commercial gain
• You may freely distribute the URL identifying the publication in the public portal
If you believe that this document breaches copyright please contact us providing details, and we will remove access to the work immediately
and investigate your claim.
Nanoscale
View Article Online
FEATURE ARTICLE
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Cite this: Nanoscale, 2013, 5, 89
View Journal | View Issue
Cholesterol – a biological compound as a building block
in bionanotechnology
Leticia Hosta-Rigau,a Yan Zhang,ab Boon M. Teo,a Almar Postmac
and Brigitte Städler*a
Cholesterol is a molecule with many tasks in nature but also a long history in science. This feature article
Received 26th September 2012
Accepted 31st October 2012
highlights the contribution of this small compound to bionanotechnology. We discuss relevant chemical
aspects in this context followed by an overview of its self-assembly capabilities both as a free molecule
and when conjugated to a polymer. Further, cholesterol in the context of liposomes is reviewed and its
DOI: 10.1039/c2nr32923a
impact ranging from biosensing to drug delivery is outlined. Cholesterol is and will be an indispensable
www.rsc.org/nanoscale
player in bionanotechnology, contributing to the progress of this potent field of research.
Introduction
Bionanotechnology is aiming to learn from nature’s approach
to assemble and run “nano-machines” and to mimic these
concepts by engineering functional nano-devices e.g. making
use of the self-assembly capability of biological building blocks
or imitate nature’s way of motility.1–3 In the latter case, attempts
a
iNANO, Aarhus University, Aarhus, Denmark. E-mail: [email protected]; Tel: +45
8715 6668
b
State Key Laboratory for Modication of Chemical Fibers and Polymer Materials,
College of Material Science and Engineering, Donghua University, Shanghai 201620,
People’s Republic of China
c
CSIRO Materials Science and Engineering, Ian Wark Laboratory, Bayview Ave,
Clayton, Victoria 3168, Australia
Leticia Hosta-Rigau received her
PhD in Chemistry from the
University of Barcelona, Spain,
in 2009, under the supervision
of Prof. F. Albericio. Her
research was focused on the
synthesis of peptides with antitumor properties by Solid Phase
Peptide Synthesis. During 2010–
2011 she worked as a postdoctoral researcher in the group
of Prof. F. Caruso at the
Department of Chemical and
Biomolecular Engineering at the University of Melbourne, Australia. Currently she is a post-doctoral research fellow at iNANO,
Aarhus University, Denmark, where she received a Marie Curie
individual fellowship. Her main interest is the development of
articial cells towards a functional biomedical platform with
potential in enzyme-therapy.
This journal is ª The Royal Society of Chemistry 2013
to copy the agella of bacteria4,5 or the use of motor proteins6
have been considered. In the former case, the self-assembly of
DNA,7,8 peptides,9,10 or lipids11,12 into a variety of nanostructures
has been demonstrated and their complexity is permanently
increasing and functionality is implemented. Conjugates with
biomolecules e.g. cholesterol, have proven to be indispensable
building blocks. Cholesterol, an essential component of
mammalian cells, has been described by Michael S. Brown and
Joseph L. Goldstein as “the most highly decorated small molecule in biology”,13 and this statement could probably be
extended for its application in bionanotechnology as well.
Looking back, the term “cholesterol” was introduced in the
beginning of the 20th century from the term “cholesterine”,
coined by Chevreul in 1816 “Je nommerai cholesterine, de colh,
Yan Zhang is currently a PhD
student in the College of Material Science and Engineering at
Donghua University, China.
Prior to this, she received her MS
degree in Tianjin Polytechnic
University, China. Currently,
she works as an exchange PhD
student in the group of Assistant
Prof. Brigitte Städler at iNANO,
Aarhus University, Denmark.
Her research involves the
assembly of advanced capsules
towards their application in
drug delivery.
Nanoscale, 2013, 5, 89–109 | 89
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
Feature Article
bile, et 23r3o2, solide, la substance cristallisée des calculs biliaires
humains” (I will call cholesterin of colh, bile, and 23r3o2, solid,
crystalline substance of human gallstones).14 However, cholesterol as a substance was already known in the late 1700’s as an
alcohol soluble fraction separated from human gallstones
observed by Poulletier de la Salle. In 1789 De Fourcroy had
prepared a large quantity of this substance, believing that it is
the same as “blanc de baleine” or spermaceti.15 He labeled the
crystalline fraction “adipocire” or fatty wax, a material similar to
that obtained from acid treated grave wax. (Grave was a
substance formed normally in damp areas of cemeteries from
the decomposition of cadavers.) Chevreul later showed that it
differed from these compounds by treatment with potassium
hydroxide and melting point comparisons.16
Initial forays into elucidation of the structure of cholesterol
showed it to be an alcohol17 in the course of the preparation of
esters, and later it was shown to be a secondary alcohol18
through its conversion into the ketone cholesterone. The presence of the double bond was established in 1868. Further
structural elucidation through parallel studies on derivatives of
cholesterol and chemically related bile acids, with verication
Boon M. Teo received her PhD
from The University of Melbourne, Australia in 2010
working on ultrasonic polymer
synthesis. Currently, she is
working as a post-doc in Assistant
Prof. Brigitte Städler’s group at
Aarhus University, Denmark. Her
research interests include emulsion polymerization, anisotropic
polymer colloids and drug
delivery systems.
Almar Postma received his PhD
from The University of New
South Wales, under the supervision of Prof. T. P. Davis and Drs
G. Moad & M. O’Shea (2005) in
the elds of controlled radical
polymerisation and reactive
extrusion. From 2005 to 2008 he
held a postdoctoral fellowship
position with Prof. F. Caruso at
The University of Melbourne
working on both polymer-based
capsular drug delivery vehicles
and with a startup company (iCeutica) in pharmaceutical nanoparticulate reformulations. He re-joined CSIRO as a Research
Scientist in 2008. His current research interests lie at the interface
of polymer design/synthesis and their applications in nanobiomedicine and electoactive materials.
90 | Nanoscale, 2013, 5, 89–109
by X-ray studies,19 allowed the established formula to be arrived
at as described in reviews by Windaus and Neukirchen.20,21
In nature, cholesterol is heterogeneously distributed in
cellular membranes, with the highest content found in the
plasma membrane.22 Most nucleated cells synthesise cholesterol in a regulated process consisting of multiple steps that
mainly take place within the endoplasmic reticulum (ER).23–25
Alternatively, cholesterol can be taken up by the cells from
lipoproteins.26 There are various pathways to traffic cholesterol
to the plasma membrane in order to maintain the high
concentration.27 When the cholesterol level reaches a threshold
level which is regulated by the sphingomyelin content of the
cell, cholesterol is transported to the ER for esterication and
storage.28
The rst link between cholesterol and human health was
discovered in 1843, when Vogel showed that cholesterol was a
major component of arterial plaques,29 and it has since then
been intensively investigated.30,31 Cholesterol was consequently
determined to be widely distributed in the animal kingdom and
its isomeric forms, phytosterol, were shown to frequent the
vegetable kingdom.32 Sterol research in the mid- to late 20th
century progressed to biomimetic chemistry,33 tracer work,34
advanced structural determination of cholesterol using higheld NMR and X-ray diffraction methods,35 with a focus on the
regulation of cholesterol synthesis and human physiology.36,37
Cholesterol’s predominant characteristic is its ability to
modulate the physicochemical properties (e.g. uidity23 and
permeability38) of the cell membrane. Due to this, cholesterol
affects a number of cellular processes. For instance, cholesterol
inuences the behaviour of membrane proteins e.g. too much
cholesterol and ordering will slow down the diffusion of
membrane proteins and increase the bending modulus of the
membrane.39 Cholesterol also acts as a precursor for the
synthesis of bile acids40 (which are stored in the gallbladder and
help to solubilise fats), and is also important for the metabolism of fat soluble vitamins, including vitamins A, D, E, and K.41
Brigitte Städler received her PhD
from ETH Zürich, Switzerland,
followed by over two years as a
post-doc in the group of Prof. F.
Caruso at the University of
Melbourne, Australia. Since
2010, she is Assistant Professor
at iNANO, Aarhus University,
Denmark aer she obtained a
Sapere Aude Starting Grant from
the Danish Council for Independent Research, Technology
and Production Sciences. Her
research group works on the development and characterization of
smart nature-inspired drug delivery vehicles and on the establishment of microuidic platforms to address questions in
biomedicine.
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Feature Article
It is the major precursor for the synthesis of vitamin D and
various steroid hormones.42 Recently, cholesterol has also been
found to play an important role in membrane trafficking, sorting processes, and cell signalling processes, where researchers
have suggested that it is involved in the formation of lipid ras
in the plasma membrane, as represented by G protein-coupled
receptor signalling.39,43,44
The aim of this feature article is to outline the impact that
the small biomolecule cholesterol has made in the eld of
bionanotechnology (Scheme 1). We are reviewing aspects and
progresses in this area made possible and/or considerably
improved and facilitated due to the presence of cholesterol. In
the rst part, we will outline the chemistry of cholesterol,
starting with fundamental aspects, followed by cholesterol
modications and, nally, the synthesis of cholesterol-containing polymers will be discussed. The next section will
address the state-of-the-art and challenges involving the selfassembly of cholesterol and cholesterol-modied polymers into
nanostructures. The last part of this feature article will consider
the effect of cholesterol on liposomes in bionanotechnology
either as a stabiliser in drug delivery and in analytical science,
or as an anchoring unit in engineering of biosensors, for the
decoration of liposomes with polyethylene glycol (PEG), or in
the assembly of capsosomes. The involvement of cholesterol in
each of these aspects will be demonstrated by giving selected
examples. Overall, we hope to demonstrate that the small
molecule cholesterol contributes signicantly to the eld of
bionanotechnology and its many applications.
Nanoscale
both a polar hydroxyl group on one side and a non-polar tetracylic steroidal ring structure with a branched hydrocarbon tail
on the other (Fig. 1a). Further, cholesterol is comprised of a
rigid planar subunit due to the trans-conguration of the rings
and a exible iso-octyl side chain ‘tail’. The combination of this
rigidity and exibility gives cholesterol the property of orientational ordering and display of liquid crystalline behaviour in
combination with amphiphilic lipid membrane binding
capabilities.
Conjugation of cholesterol
Cholesterol is an amphiphatic molecule, a compound possessing both hydrophilic and lipophilic properties. It contains
The majority of conjugation strategies used to conjugate
cholesterol onto molecules, biomolecules, or macromolecules
of interest rely on the hydroxyl group in the 30 position of the
cholesterol ‘A’ ring (Fig. 1b). The most common are esterication, carbamate, and carbonate bond formation using
chloroformate derivatives. These strategies allow common
carboxylic acids, amines, or hydroxyl functional groups which
are found on the most biologically important or other relevant
molecules, to be coupled onto cholesterol. Other strategies
applied to conjugate to cholesterol are illustrated in Scheme 2
and discussed in the next paragraphs.
Of further interest, Achalkumar et al. have recently reviewed
the chemistry and approaches used to make cholesterol
conjugate linkers for tethering onto phospholipid bilayers.45
A practical challenge with any conjugation strategy used for
obtaining amphiphiles based on cholesterol is the choice of
solubilising conditions. The challenge is to nd a solvent that
will dissolve both the hydrophobic cholesterol, and, at the same
time, the hydrophilic material onto which it is conjugated.
Typical solvent choices range from chloroform, dichloromethane, and dioxane, to tetrahydrofuran (THF). Furthermore,
Scheme 1 Schematic illustration of the applications of cholesterol (a small
biomolecule found in biological cell membranes (top left)) in the field of bionanotechnology: self-assembly of cholesterol-containing polymers into nanostructures e.g. polymersomes (top right), cholesterol as a constituent of liposomes
(bottom right), and cholesterol as an anchoring unit for liposomes e.g. for capsosome assembly (bottom left).
Fig. 1 (a) A structural depiction of a cholesterol molecule highlighting the four
domains of functional importance ((A) important for polarity and hydrogen
bonding, (B) sterol rings, its conformation is important as it provides a rigid planar
skeleton, (C) controls the conformation of the side chain, and (D) branched
aliphatic side chain) (left) to function in membranes as a flat elongated
compound. The structure presumed to form in cellular membranes (right).
Reprinted with permission from ref. 37. Copyright (2011) American Chemical
Society. (b) Cholesterol molecule showing the tetracyclic steroid frame (A–D) with
numbering of carbon atoms of the sterol nucleus and side chain based on the
conventional numbering system.17,254
The chemistry of cholesterol
This journal is ª The Royal Society of Chemistry 2013
Nanoscale, 2013, 5, 89–109 | 91
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
Feature Article
methacryloyl chloride,51–53 allow appropriate vinyl esters to be
synthesised in high yields. Further, the acid chloride can be
obtained via reaction of the appropriate carboxylic acid with
thionyl or oxalyl chloride prior to the reaction with cholesterol.54,55 Acid bromides, such as (2-bromoisobutyryl bromide)
can also be efficiently coupled onto.56 Steglich esterication
using N,N0 -dicyclohexylcarbodiimide and DMAP, has been used
successfully to react a carboxylic acid with the alcohol of
cholesterol (Fig. 2a).57,58 Ring opening of succinic anhydride
with cholesterol can also be used to form a cholesterol ester
with a terminal carboxylic acid which can then be used for
further chemical attachments.59
Etherication
Ether formation from the hydroxyl group is a common strategy
for the attachment of PEG and sugars to cholesterol. For
example, cholesterol functionalised monomers containing a
diethyleneglycol60 spacer and tetraethylene glycol10 spacer,
attached via an ether bond, have been synthesised. Williamson
ether synthesis is also a popular synthetic approach which can
Scheme 2 Schematic illustration of synthetic opportunities and conjugation
strategies to the cholesterol alcohol. Clockwise from the top: etherification
through the trichloroacetimidate approach and via Williamson’s ether synthesis,
dioxaphospholane cyclic phosphate functionalisation, carbamate and carbonate
conjugation through a chloroformate, and esterification.
derivatives based on cholesterol oen have a strong tendency to
self-assemble. This oen complicates chemistry isolation
procedures such as water washes during solvent extraction
steps. Nonetheless, chemical synthetic procedures for coupling
cholesterol are well represented in the literature to indicate that
these issues can be overcome.
Chloroformate
A common strategy for cholesterol conjugation is the use of the
chloroformates. Cholesterol chloroformate, a commercially
available compound, is simply combined with the material to be
conjugated onto, which carries an amine, to give a carbamate
cholesterol derivative. The addition of the components is
usually performed under cooled anhydrous conditions and in
the presence of a catalytic amount of a base like triethylamine or
4-dimethylaminopyridine (DMAP). This strategy has been used
for the coupling of cholesterol onto, for example, the primary
amines of 30 -O-(6-aminohexyl)-uridine46 or polyethylenimine
(PEI).47 Also commonly applied, alcohols can be coupled to
cholesterol chloroformate to give the corresponding carbonate.
As an example, the alcohol of hydroxylethyl (meth)acrylate
(HEMA) was coupled to cholesterol, as a way of placing a short
spacer between the cholesterol and the vinyl group.48
Esterication
The hydroxyl group lends itself well for esterication reactions
and, as such, several approaches have been used. Acylation of
the hydroxyl moiety of cholesterol with commercially available,
functional acid chlorides, such as acryloyl chloride49,50 and
92 | Nanoscale, 2013, 5, 89–109
Fig. 2 Schematic examples of cholesteryl-functional polymers: (a) bis-cholesteryl
end-functional P(HPMA),57 (b) ABA triblock copolymer (PNAM-b-PChA-bPNAM),94 and (c) poly(amidoamine)-co-(amidoamine disulfide cholesteryl)
copolymer.102
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Feature Article
be carried out by reaction of the alkoxide of the alcohol with an
alkylating agent carrying the ‘R’ group. Alternatively, to
combine two alcohols together, one of them can be initially
tosylated (using p-toluene sulfonyl chloride) and allowed to
react with the other alcohol to form the corresponding ether.
This was successfully carried out for the synthesis of a norbornene based monomer61 and a vinyl monomer containing an
aliphatic spacer.62
A glycolipid library based on acylated cholesteryl-b-galactosides was synthesised for the elucidation and construction of a
vaccine against Lyme disease. Here, the glycosylation of
cholesterol with galactose, essentially an ether bond formation,
was achieved using a trichloroacetimidate approach.63 Several
3-cholesteryl 6-(glycosylthio)hexyl ether glycolipids were also
prepared via thiol alkylation using 3-cholesteryl 6-iodohexyl
ether. The latter was formed from cholesteryl p-toluenesulfonate via three steps.64
Miscellaneous chemistry
An example of the cyclic phosphate functionalisation of
cholesterol was published by Iwasaki and Akiyoshi as a cholesteryl-functional monomer strategy for the synthesis of
biodegradable and biocompatible polyphosphates.65 The
synthesis of this monomer was achieved by the addition of
cholesterol to a cooled solution of 2-chloro-2-oxo-1,3,2-dioxaphospholane in ether. However, only a 33% yield was achieved
aer recrystallisation.
Monomers and polymers
The conjugation techniques previously mentioned are
commonly applied to the synthesis of cholesterol-based (cholesteryl) monomers for the synthesis of polymers. Esterications and carbamate formation are typically used to add the
appropriate polymerisable or polymer initiating group to
cholesterol. These can then be used to create a diversity of
polymer architectures such as end-functional polymers,
homopolymers, copolymers and block copolymers.
Polymer end-functionalisation
Ring opening polymerisation (ROP)66 is one approach that has
been used for adding efficiently cholesteryl end-functionality to
polymers. The polymerisation is simply initiated by an alcohol, in
this case cholesterol, which conveniently ring opens the monomers without the use of a catalyst. This approach has been used
to synthesise polyesters, polylactide (PLA), polyglycolide and their
copolymers, poly(lactide-co-glycolide) (PLGA)67 and, with the
addition of a catalyst Sn(Oct)2, 3-caprolactone, which ring opens
to give poly(3-caprolactone).68 Polycarbonates based on trimethylene carbonate69 or 2,2-dimethyltrimethylene carbonate70
were also easily synthesised without the use of a catalyst.
Klok et al. used ROP to great effect to synthesise L-lactic acid
oligomer linkers initiated by cholesterol and terminated by
cholesterol, or bioactive drugs, uorescent markers,71 and
generation 1, 2 and 3 L-lysine dendrons.72
End-functionalisation of a radical polymer with a
cholesteryl moiety can be performed simply by the use of a
This journal is ª The Royal Society of Chemistry 2013
Nanoscale
cholesteryl-functional initiator. An example is the use of a cholesteryl radical initiator in conjunction with a cholesteryl-functional vinyl monomer. In this case 4,4-azobis(4-cyano-1cholesteryl) pentanoate azo initiator was used to initiate the
polymerisation of sodium 2-(acrylamido)-2-methylpropanesulfonate to give a cholesteryl end-capped and linear poly(sodium 2(acrylamido)-2-methylpropanesulfonate).54 In another report,
poly[N-(2-hydroxypropyl)methacrylamide]s (PHPMAs) with a
terminal cholesteryl moiety either at one or both ends of the
polymer chains have been synthesised (PHPMA-Chol and
PHPMA-2-Chol). These were prepared by the radical polymerisation of N-(2-hydroxypropyl)methacrylamide, initiated with 4,40 azobis-[(3-cholesteryl) 4-cyanopentanoate] in the presence of
2-mercaptoethanol and thiocholesterol chain-transfer reagents,
respectively.73
A cholesteryl functional reversible addition fragmentation
chain transfer (RAFT)74–78 agent with a single cholesteryl functionality placed in the RAFT re-initiating the ‘R’ group was used
for the synthesis of u-cholesteryl functional poly(polyethylene
glycol) acrylate.58 A bis-cholesteryl functional ‘R’ group RAFT
agent was used to place two cholesteryl u-end groups onto
poly(N,N-dimethyl acrylamide) (PDMA), PHPMA and copolymers thereof.57
Atom transfer radical polymerisation (ATRP)79–81 has also
been used as a tool to initiate polymerisations with a cholesteryl-functional initiator.82 Xu et al. applied this technique to
synthesise a biomimetic amphiphile from 2-(methacryloyloxy)
ethyl phosphorylcholine from 10-cholesteryloxydecanyl-2-bromoisobutyrate.83,84 Similarly, cholesteryl-2-bromoisobutyrate
was used to initiate various oligo(ethylene glycol) (meth)acrylates to produce copolymers with u-bromine end-groups. These
bromine end-groups were later transformed to reactive azides
by nucleophilic substitution with sodium azide and, once
assembled into micelles, allowed the azide–alkyne cycloaddition “click” reaction to occur in the corona of the micelle.56
Post-functionalisation of end-groups
The exibility of RAFT agents allows for a symmetrical design of
polymer end-group functionality via the RAFT agent. This can
be achieved by using a RAFT agent that has a central bis-functional radical leaving/reinitiating the ‘R’ group and two thiocarbonylthio ‘Z’ groups on either side. Post-functionalisation
can then be carried out through the aminolysis of the thiocarbonylthio end-groups which transform them into thiols.
Such an approach has been used to react end group thiols with
3-cholesteryl 6-iodohexyl ether via nucleophilic reaction to
make a,u-di(cholest-5-en-3b-yl-6-oxyhexylthio) poly(N-isopropyl
acrylamide) P(NiPAM).85 A pyridyldisulde poly(oligo (ethyleneglycol) acrylate) RAFT polymer with a pre-attached bovine
serum albumin (BSA), was functionalised with a cholesteryl
group through disulde exchange with thiocholesterol.86
Homopolymers
One of the ways of introducing several cholesteryl functionalities
along the length of a polymer chain is by homopolymerising a
cholesteryl-functional monomer. Ruthenium-catalysed ring
Nanoscale, 2013, 5, 89–109 | 93
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
opening metathesis polymerisation (ROMP)87,88 of a monomer
functionalised with both norbornyl and cholesteryl moieties has
been utilised to make pendant cholesteryl-functional homopolymers with a variety of spacers present between the backbone and
the cholesterol.55
A technique that has been used more prolically for introducing cholesteryl-functionality along a polymer chain is the
radical polymerisation of cholesteryl-functionalised acrylate or
methacrylate monomers to give pendant cholesteryl functionality to polymers. This was looked at as early as the late 60’s and
70’s by Hardy et al.89,90 and De Visser et al.49,50 More recently,
cholesteryl polymerisation has seen resurgence when paired
with controlled radical techniques like ATRP and RAFT. For
example, a homopolymer based on cholesteryl acrylate (CA)
using RAFT was synthesised and block extended with styrene.91
Block copolymers
Zhang et al. designed cholesterol monomers with a hydrophilic
tetra(ethylene glycol) (TEG) spacer inserted between the mesogen and the acrylate (or methacrylate) polymerisable group in
order to increase the water solubility of the monomer in their
dispersion polymerisation system.10 From the poly(methacrylic
acid (MAA)-co-PEG methacrylate (PEGMA)) copolymer macroRAFT agent, they synthesised the block copolymer P(MAA-coPEGMA)-b-P(Chol-TEGMA) under dispersion polymerisation
conditions, which allowed the formation of a block copolymer
via self-assembly in minimal steps. In a different report, Liu
et al. used a diethyleneglycol spacer between the cholesterol and
the acrylate and made blocks with (benzyl protected) ascorbate
sections.92 In our own research, we designed an amphiphilic
block copolymer poly(N-vinyl pyrrolidone) P(NVP)-b-P(CA)
which was obtained by polymerising a short CA oligomer
section of, on average, 3 units from a P(NVP) macroRAFT
agent.93 This macroRAFT agent was obtained via the controlled
polymerisation of NVP with a xanthate RAFT agent. Alternatively, diblock copolymers have also been designed by growing
the second block from a cholesteryl methacrylate (CMA) macroRAFT agent with a trimethylsilyl protected hydroxyethyl
methacrylate (HEMA-TMS), giving P(CMA-b-HEMA-TMS). This
block copolymer was further deprotected by the addition of
concentrated HCl in a THF solution resulting in the clean
product copolymer P(CMA-b-HEMA).51 Curiously, the authors
reported problems with controlling of the polymerisation of the
unprotected HEMA. Additionally, they initially observed difficulties polymerising CMA under ATRP conditions with methyl
2-bromopropionate as the initiator and copper(I) chloride as
bipyridine as the catalyst–ligand system at 90 C. Recently, we
have looked at the synthesis of an ABA triblock copolymer in two
steps from a bis ‘Z’ functional RAFT agent to form a CA macroRAFT agent, from which two N-acryloyl morpholine (NAM)
arms can be grown (Fig. 2b).94 We designed the NAM : CA block
ratio to be close to 2.5 : 1 to direct the spatial self-organisation
of the polymer into polymersomes. A bis ‘R’ RAFT agent for the
design of an ABA triblock with the cholesteryl as the ‘B’ block,
for use in liquid crystalline block copolymers, has also been
looked at by Shibaev et al.95
94 | Nanoscale, 2013, 5, 89–109
Feature Article
ROMP can also be successfully used to synthesise well
controlled block copolymers containing a cholesterol rich
section. Here, a norborene functional cholesterol monomer is
polymerised to form the second block from a poly(ethylene
oxide) brush block. These block copolymers are assembled into
nanoparticles for the delivery of doxorubicin and indomethacin, through acid labile carbamate linkers.61
Random or statistical copolymers
Copolymerisation is a convenient method for the introduction
of cholesteryl pendants into the polymer chain at various mole
percentages. Some examples include the free radical copolymerisation of acrylic acid (AA) with 5-acryloyloxypentyl cholesterate (Ch5A) to give P(Ch5A-co-AA),96 NiPAM with CA to give
P(NiPAM-co-CA),97 HPMA terpolymerised with 6-methacrylamido hexanoyl hydrazine and cholest-5en-3b-yl 6-methacrylamido hexanoate,98 and our own work via RAFT mediated
copolymerisation to give P(MAA-co-CMA) with a 7 mol%
cholesterol content.52,99 Researchers at the Australian Centre for
Nanomedicine have also recently looked at the copolymerisation of CMA with MAA.100 They varied the CMA content from
2 mol% to 8 mol% and together with dimethylamino ethyl
methacrylates53 and RAFT mediated control, they were able to
achieve a CMA content ranging from 2 mol% to 20 mol% whilst
keeping their polymer molecular weights around 20–24 kDa
with low molecular weight dispersities throughout. The
amphiphilic copolymers showed pH-induced phase transitions
in aqueous media and are envisioned to be useful for
condensing and transporting siRNA due to their lipid
membrane destabilizing properties.
An example of a polyphosphate terpolymer containing
pendant cholesteryl functionality, pendant ATRP initiating
groups as well as 2-isopropyl-2-oxo-1,3,2-dioxaphospholane units
were synthesised as a biodegradable gra terpolymer, a novel
amphiphilic biomaterial which can function as a nanocarrier.65
Alternatively, post-functionalisation of polymers to introduce
cholesterol has been performed on polymers containing amine or
acid reactive groups, PEI,47 poly(L-lysine) (PLL)52 and sodium
alginate,101 giving random copolymers. An interesting example of
post-functionalisation is the Michael addition polymer poly(amidoamine) (PAA) (Fig. 2c).102 The nanoparticulate polymer
network can be obtained using cystamine as a cross-linking agent
which can be made to react with 2,20 -dithiodipyridine turning
them into linear PAAs with dithiopyridyl side groups that are able
to undergo a thiol exchange reaction with the commercially
available thiocholesterol. The resultant products are examples of
amphiphilic PAA–cholesterol conjugates in which lipophilic
cholesterol moieties are linked to the hydrophilic PAA chain by
disulde bonds. These are relatively stable in blood but are
cleavable under the reductive conditions within cells.
There are many more examples of cholesterol containing
polymers, mostly with a focus on optical, liquid crystal and
some general bioapplications; however, these are beyond the
scope of this review. The reader is directed to reviews by Zhou
et al. and Yusa for a more exhaustive list and description of
these polymers.103,104
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Feature Article
Nanoscale
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Self-assembly of cholesterol
As previously mentioned, cholesterol is structurally composed
of different sections which play a role in its interesting selfassembly behaviour in a variety of multi-component
solutions.105–108
Helical ribbons were rst discovered in human gallbladder
bile, and it was found that these structures form as a precursor
of gallstones upon dilution of bile.107 Konikoff et al. conrmed
that cholesterol is the major constituent of these helical ribbons
by various experimental techniques including density gradient
centrifugation or X-ray diffraction. They also found that the
helical ribbons themselves are precursors of stable cholesterol
monohydrate crystals.106,107 Chung et al. used several model bile
systems which consisted of a mixture of three types of chiral
molecules in water: a bile salt, a phosphatidylcholine, and
cholesterol. They demonstrated that helical ribbons formed
with two distinctive pitch angles, 11.1 0.5 and 53.7 0.8 .105
Zastavker et al. then showed that the self-assembly of the helical
ribbons with these two distinct pitch angles was not unique to
model bile, but was a general phenomenon for a variety of fourcomponent systems composed of a bile salt or surfactants, a
phosphatidylcholine or fatty acids, a steroid analogue of
cholesterol, and water.109 It was found that in undiluted solutions containing cholesterol, surfactants, and fatty acids or
phospholipids, cholesterol is solubilised by micelles, i.e.
cholesterol was contained in the core. These solutions contain
both the free surfactants and the surfactants contained in
micelles in equilibrium. Upon dilution, the equilibrium shis
from primarily micelles to primarily free surfactants. The
micelles break up and release the cholesterol, causing the
solution to become supersaturated with cholesterol. Subsequent dilution leads to the formation of large cholesterol
monohydrate crystals. However, the exact structures that are
formed and the sequence in which they form depend on the
composition of the solution and the concentration of its
components as shown in Fig. 3a.105
In an attempt to assess the properties of helical ribbons,
Starostin and coworkers studied the non-monotonic forceextension properties and predicted hysteresis behaviour for lowpitch ribbons of arbitrary material properties using a new
model for inextensible elastic strips. It explained the rst-order
transition between two different helical states as experimentally
observed. Furthermore, they revealed a new uncoiling scenario
in which a ribbon of very low pitch shears under tension and
successively releases a sequence of almost planar loops. They
considered their results to be relevant for nanoscale devices
such as force probes.110 Also, helical ribbons were thought to
have potential serving as mesoscopic springs to measure or to
exert forces on nanoscale biological objects. The spring
constants of these helices depend on their submicroscopic
thickness. Using quantitative phase microscopy, Khaykovich
et al. discovered a quadratic relationship between the radius R
and the thickness t of helical ribbons that form spontaneously
in multicomponent cholesterol–surfactant mixtures. The
quadratic relationship (R f t2) between radius and thickness is
a consequence of the crystal structure of the ribbons and
This journal is ª The Royal Society of Chemistry 2013
Fig. 3 (a) Sequence and relative stability of metastable intermediates plotted as
a functions of time after supersaturation of bile. Reproduced with permission
from ref. 105. Copyright (1994) National Academy of Sciences, USA. (b) Images of
a helical cholesterol ribbon. Phase images for angle of 0 illumination (i) and for
aperture synthesis (ii). Reproduced with permission from ref. 113.
enables the determination of the spring constant of any helices
solely in terms of its observable geometrical dimensions.111
Choi et al. used high-speed synthetic aperture microscopy to
image helical cholesterol ribbons in surfactant mixtures, as well
as to measure the thickness of a nanoscale cholesterol helical
ribbon (Fig. 3b) which was determined to be 68 nm.112,113 These
fundamental ndings provide the foundation towards applications of the helical ribbons.
Self-assembly of cholesterol-modified
polymers into nanostructures
Due to its highly hydrophobic sterol skeleton, good biodegradability and biocompatibility, hydrophobic cholesterol is a
good choice for the amphiphilic modication of many watersoluble polymers. Self-assembly of amphiphilic cholesterolmodied polymers has been a subject of great interest for the
past few decades.71,73,101,114–116 Cholesterol units attached onto
macromolecules as pendant(s) or as end-group(s) can induce
formation of structures of well-dened morphology in water as
a result of specic interactions among the cholesterol moieties.103,104 Though cholesterol has been used to modify many
kinds of polymers,84,102,117–120 herein we will focus on cholesterolmodied polymers and their self-assembly behaviour with
potential biomedical applications, e.g. drug delivery.
Cholesterol-modied polysaccharides have attracted the
interest of many researchers. Akiyoshi et al. prepared cholesteryl-bearing mannans (CHM) and cholesteryl pullulan (CHP).
CHM and CHP can self-organise into nanoparticles and gels in
Nanoscale, 2013, 5, 89–109 | 95
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
semi-dilute solution due to the hydrophobic interaction of the
cholesterol moieties.121 Cholesterol-modied chitosan (CS-CH)
can form self-aggregated nanoparticles in physiological saline.
The drug-loading and release behaviour of the CS-CH nanoparticles were investigated using Cyclosporine A (CyA) as a
model drug. CyA was physically entrapped in the nanoparticles
during the dialysis process, and the drug-loading was on the
order of 6.2 wt% of the CS-CH self-aggregated nanoparticles.122
Yu et al. investigated cholesterol-modied glycol chitosan
(CHGC), and used the CHGC self-aggregated nanoparticles for
doxorubicin loading and delivery.123 They found that doxorubicin release from CHGC nanoparticles was dependent on the
pH, with faster release at lower pH. This aspect was considered
important, because the drug would be more efficiently released
in the tumour tissue than in circulation. They reported that the
pharmacokinetic parameters of doxorubicin changed in mice
and more efficient tumor growth inhibition for doxorubicinloaded CHGC compared to free doxorubicin was reported,
making these nanoparticles promising carriers for insoluble
anticancer drugs in cancer therapy. The Zhang group published
a series of reports involving CS-CH124–128 and synthesised
cholesterol-modied O-carboxymethyl chitosan (CCMC),
cholesterol-modied chitosan conjugate with succinyl linkages
(CHCS) and 6-O-cholesterol modied chitosan nanoparticles
(O-CHCS NPs). The self-aggregation behaviour of the modied
chitosan and chitosan nanoparticles due to the strong hydrophobic interaction of the cholesterol moieties was investigated.
It was found that the degrees of substitution (DS) of the
cholesterol moieties played an important role in the size and
the surface property of the self-aggregated nanoparticles.
Comparing the morphology and the stability of self-aggregated
nanoparticles between CCMC and CHCS, the negatively charged
carboxymethyl groups are advantageous for the formation of
well-shaped and stable self-aggregated nanoparticles.126 They
studied the drug loading and release property of CHCS and
CCMC nanoparticles using Epirubicin (EPB) and paclitaxel,
respectively.124,127 The results showed that the release rate
decreased with increasing pH of the media. In PBS, the EPB
release was very slow (24.9% in 48 h), while paclitaxel was
continuously released over 84 h at 37 C. The biodistribution of
paclitaxel-loaded CCMC self-assembled nanoparticles showed
that these nanoparticles seemed to signicantly increase the
uptake of paclitaxel in plasma, liver and spleen, but decreased
the uptake in heart and kidney. Further, the interaction
between BSA and self-aggregated CCMC and O-CHCS NPs with
different DS of cholesterol moieties was assessed.125,129 The
addition of O-CHCS NPs led to the decrease of the a-helical
content of BSA and the increase of the b-strand content. The
unfolding of BSA by a denaturant such as urea was largely
suppressed upon interaction with CCMC self-aggregated
nanoparticles.
Cholesterol is oen used to modify PEG polymers leading to
different self-assembly behaviour.130–137 Jia et al. synthesised
amphiphilic liquid crystal block copolymers consisting of a
cholesterol-based smectic liquid crystalline polymer block
(PAChol) and a PEG block (Fig. 4i).135 They found that PEG45-bPAChol and PEG114-b-PAChol (45 and 114 are the degrees of
96 | Nanoscale, 2013, 5, 89–109
Feature Article
Fig. 4 (i) Molecular structure of the diblock copolymer PEG-b-PAChol. (ii) Selfassembled structures of PEG45-b-PAChol in dioxane/water: cryo-transmission
electron microscopy (TEM) image of vesicles of PEG45-b-PAChol10 (left) and cryoTEM images of vesicles of PEG45-b-PAChol16 (right). (iii) Schematic presentation of
the model for ellipsoidal smectic polymer vesicle (top) and smectic rod-like
micelles (bottom). Reproduced with permission from ref. 135.
polymerisation of the PEG blocks) with different hydrophilic/
hydrophobic weight ratios could self-assemble into polymer
aggregates with different morphologies in THF/water and
dioxane/water (Fig. 4ii). Adding water to a dilute solution of
copolymers in dioxane yielded smectic polymer vesicles and/or
nanobers. By using THF instead, solid spherical aggregates were
obtained upon water addition for the PEG45-b-PAChol copolymer. With proper block sizes and the use of appropriate organic
co-solvents, these biocompatible cholesterol-based copolymers
can self-assembly into aggregates with desirable shapes (e.g.
vesicles or nanobers) (Fig. 4iii), which have potential applications in drug delivery and material science.135 Nagahama et al.
prepared a novel star-shaped copolymer derivative with cholesterol end groups, cholesterol-substituted 8-arm PEG-b-poly(L-lactide) (8-arm PEG-b-PLA-cholesterol). Based on the specic
self-assembly between the cholesterol end groups, the 8-arm
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Feature Article
PEG-b-PLA-cholesterol aqueous solution exhibited instantaneous
temperature-induced gelation at 34 C.131 In addition, PEGylated
poly(N-methyldietheneamine sebacate)-co-((cholesteryl oxocarbonylamido ethyl) methyl bis(ethylene) ammonium bromide)
sebacate) (PEG-P(MDS-co-CES)) were synthesised, which could
self-assemble into stable micelles of small size with a hydrophobic core and hydrophilic shell.136,137 Different cholesterolgraing degrees of the PEG-P(MDS-co-CES) polymer were shown
to have improved stability of micelle/DNA complexes in blood for
systemic in vivo gene delivery. In another report, Manakker et al.
investigated the rheological properties of a self-assembled
hydrogel system composed of b-cyclodextrin (bCD)- and cholesterol-derived 8-arm star-shaped PEG.133 They found that the 8-arm
polymer-based mixtures yielded tight viscoelastic networks, but
their storage and loss moduli signicantly deviated from those
predicted by the Maxwell model. Rheological analysis also
showed that the hydrogels were thermo-reversible. At low
temperatures, the gels showed viscoelastic behaviour due to slow
overall relaxation of the polymer chains. At higher temperatures,
however, a reduced number of bCD–cholesterol complexes and
concomitant faster chain relaxation processes eventually led to
liquid-like behaviour.
Cholesterol-modied compounds can also be mixed with
others, and self-assembled into different macroscopic vesicles.
For example, the nucleoside 20 -deoxy-20 -aminouridine was
modied with cholesterol, and the lipophilic nucleoside 20 -N-(2(cholesteryl)-succinyl)-20-deoxy-20-aminouridine was obtained.
When mixed with the unsaturated phospholipid dioleoylphosphatidylcholine, microtubes were formed. From
confocal uorescence microscopy images, the tubes appeared
as open-ended cylindrical structures with outer diameters
between 2 and 3 mm and lengths between 20 and 40 mm.138 In
another report, the dialysis of a dimethyloxide solution of
cholesterol-modied dextran (Chol-Dex) and PLA against water
yielded hollow polymer nanocapsules with a highly stable
structure and relatively narrow size distribution.139 The hollow
capsules were thought to be formed by anchoring of most of the
amphiphilic polysaccharide onto the surface of swelled aggregates as a result of phase separation of amphiphilic Chol-Dex
from hydrophobic PLA. The capsules obtained have potential
application as drug carriers or as biomembrane models.
We recently reported the self-assembly of an amphiphilic
block copolymers containing cholesterol as the hydrophobic
block into polymersomes (Fig. 5).94 We synthesised an ABA
triblock copolymer with the ‘A’ segment consisting of poly(NAM),
a non-ionic hydrophilic polymer with low-fouling properties
similar to PEG, and the ‘B’ segment of poly(CA) as the hydrophobic part of the triblock copolymer. We demonstrated the
stable, non-aggregated assembly of polymersomes with narrow
polydispersity. We used these polymersomes as reservoirs in
poly(vinyl alcohol) composite hydrogels and showed a signicant
decrease in viability of adhering myoblast cells when a cytotoxic
compound was entrapped in the polymersomes, thus conrming
the potential of this system in surface-mediated drug delivery, a
biomedical approach which aims to deliver therapeutic
compounds from the surface of an implantable device or a tissue
culturing scaffold to adhering cells or to the surrounding media.
This journal is ª The Royal Society of Chemistry 2013
Nanoscale
Fig. 5 Schematic representation of a polymersome (i) assembled from an ABA
triblock copolymer consisting of poly(N-acryloyl morpholine) and poly(cholesteryl
acrylate) with entrapped cargo in the hydrophobic part of its polymer membrane
(ii), and a cryo-TEM image confirming the assembly of polymersomes (iii).
Reproduced with permission from ref. 94.
In summary, based on the hydrophobic interaction, cholesterol-modied polymers can self-assemble into different
micelles, nanoparticles, nanotubes, nanogels, or polymersomes. The size, shape and mechanical properties of these
assemblies are designed for encapsulation, storage, release and
delivery of therapeutics with potential application in biomaterials and biomedicine.
Cholesterol and liposomes
The nal part of this feature article reviews the benets of
cholesterol incorporated into liposomes for biomedical applications. Two different aspects of cholesterol, namely its ability
to act as stabiliser for lipid membranes and its ability to link
lipid and polymeric structures together, are discussed. Examples of applications in drug delivery and biosensing will be
outlined for both aspects.
Cholesterol as a stabiliser
Liposomes are among the prominent candidates for various
biomedical applications in bionanotechnology. Liposomes are
spherical vesicles which consist of one or more lipid bilayer
membrane(s), encapsulating a volume of aqueous medium
(Fig. 6a).140 Glycerophospholipids, sphingolipids, and cholesterol are the predominant components used for their preparation. Their structural similarity to natural cell membranes,141
and their ability to mimic the behaviour of biological cell
membranes make liposomes useful in various applications
ranging from drug delivery,142,143 cosmetic,144 and food
science145 to agriculture.145 However, control over the lipid
bilayer permeability and stability towards solutes or biomolecules is oen a challenge and can compromise their applications in the aforementioned elds. This aspect can be regulated
by adjusting the cholesterol content of the lipid bilayer,146,147
since cholesterol affects the physicochemical properties of the
Nanoscale, 2013, 5, 89–109 | 97
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
Fig. 6 Cholesterol as stabiliser: (a) schematic illustration of the fundamental selfassembly process from individual phospholipid molecules (i) to bilayer membrane
leaflets (ii), followed by transformation into liposomes (iii). A single bilayer consists
of arranged individual lipid molecules with their hydrophobic tails facing each
other and their hydrophilic head-groups facing toward the internal and external
aqueous media (iv). Adapted with permission from ref. 140. (b) Schematic
representation of liposomes with encapsulated enzymes. Substrates diffuse into
the void of the liposome through porin channels, react with the enzymes, and the
product is released back into the solution through diffusion. Reproduced with
permission from ref. 141. (c) Schematic representation of a biosensor assay where
a DNA capture probe is immobilised on a polyethersulfone membrane and a DNA
reporter probe is coupled to the surface of a liposome. When a specific E. coli
mRNA is present, a sandwich is formed between the capture probe, the E. coli
mRNA and the reporter probe, capturing the liposome in the capture/detection
zone. The number of liposomes is directly proportional to the amount of E. coli
mRNA present. Reproduced with permission from ref. 203. (d) Table containing
most common homogeneous complement mediated liposome immunoassays.
Reprinted with permission from ref. 205. (ab, antibody; ag, antigen; BSA, bovine
serum albumin; CF, carboxyfluorescein; chol., cholesterol; DCP, dicetylphosphate;
DMPC, dimyristoylphosphatidylcholine; DMPG, 1,2-dimyristoyl-sn-glycero-3phospho-(10 -rac-glycerol); DNP, dinitripheno(y)l(ated); DPPC, dipalmitoylphosphatidylcholine; DPPE, dipalmitoylphosphatidylethanolamine; DSPC, distearoylphosphatidylcholine; EA, egg albumin; HSA, human serum albumin; PA,
palmitic acid; PC, phosphatidylcholine; PE, phosphatidylethanolamine; SA, stearylamine; and SPH, sphingomyeline).
lipid membrane. For an in-depth discussion, the reader is
referred to the reviews by Ohvo-Rekilä et al. or Rog et al.148,149
The amphiphilic cholesterol is arranged in the lipid membrane
by orienting the steroid ring parallel to the hydrocarbon chains
of the lipids (phospholipids or sphingolipids) and the hydroxyl
group encountering the aqueous phase. There are two physical
98 | Nanoscale, 2013, 5, 89–109
Feature Article
states of a lipid bilayer in the absence of cholesterol: the gel
state at lower temperatures and the liquid-crystalline state at
higher temperatures. The individual lipid molecules of a lipid
bilayer have temperature-dependent mobility (uidity). All
lipids have a characteristic temperature in which they undergo a
transition from the gel to the liquid-crystalline phase, which is
known as phase transition temperature (Tm). The phase
behaviour of the lipid bilayer and thus Tm is determined by the
van der Waals (VDW) interactions between adjacent lipid
molecules. The interaction between the acyl chains of the lipids
is mainly governed by two factors: the length of the chain and
the packing of the lipids in the bilayer, i.e. longer tail lipids have
more area to interact, which will, in turn, increase the strength
of the interaction and, consequently, decrease the mobility of
the lipid. The type of acyl chain (degree of saturation) plays an
important role in how the lipids bind in the bilayer, since an
unsaturated double bond can produce a kink in the alkane
chain which will create extra free space within the bilayer, thus
allowing for additional exibility in the adjacent chains.
Therefore, unsaturated lipids have a signicantly lower Tm
compared to saturated lipids. Incorporation of increasing
amounts of cholesterol into the lipid bilayer induces an
“intermediate” state by increasing and decreasing the uidity of
the hydrocarbon chain below and above Tm, respectively, and
eventually eliminating Tm entirely. In the gel phase, the presence of cholesterol in the membrane weakens the VDW interactions between the hydrocarbon chains of the fatty acids and
prevents lipid crystallisation, while in the liquid-crystalline
phase, the hydrocarbon chains of the lipids which interact with
the rigid, planar rings of the cholesterol, are partly immobilised. Specically, cholesterol increases the degree of orientation and reduces the rate of motion in the liquid-crystalline
phase of the lipid membrane. This leads to a laterally
condensed membrane with increased packing density and, as a
consequence, higher mechanical strength and lower permeability. Nature makes use of this aspect in many ways, but
nanotechnological applications also rely strongly on this effect
as outlined in the subsequent paragraphs.
Drug delivery
Liposomes have been considered as drug delivery vehicles due
to their colloidal size, ease of preparation, controllable surface
and membrane properties, large carrying capacity, and
biocompatibility for over 30 years.150 Since the liposomal shell
can enclose or bind many different classes of substances, liposomes are successfully employed as therapeutic agents for the
delivery of antibacterial,151 antiviral,152 and anticancer drugs,153
as well as hormones,154 enzymes,155 and nucleotides.153,156
However, two of the major drawbacks of liposomes as drug
carriers are their oen poor stability in blood circulation upon
systemic application and the sometimes suboptimal control
over cargo retention and release.157 In the latter case, drugs have
to be transported to their site of action quantitatively, or the
therapeutic cargo has to be gradually released.146,147
Cholesterol has served to overcome both of the abovementioned challenges. Since the addition of cholesterol reduces
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Feature Article
the uidity of the lipid bilayer and increases the stability of the
liposomal membrane,158 adjusting the cholesterol content of
liposomes has been one of the prime ways to control the
permeability to solutes both in vivo and in vitro. Typically, halflives of passively encapsulated drugs range from minutes, in egg
phosphocholine liposomes, to a dozen hours for cholesterolcontaining liposomes.159 Owing to this increased cargo retention, the rst liposomal formulation of the antitumor drug
Doxorubicin (Doxil) was approved in 1995 by the Food and
Drug Administration (FDA) for medical use in oncology.160,161
Other cholesterol-containing liposomal formulations of drugs,
i.e. Daunorubicin (DaunoXome) used for the treatment of
advanced HIV-associated Kaposi’s sarcoma,162 Amphotericin B
(AmBisome, Amphotec, and Ableet) for the treatment of
fungal infections in febrile neutropenic patients as well as for
the treatment of aspergillosis, candidiasis, and cryptococcosis
infections refractory to Amphotericin B,163,164 and cytarabine
(DepoCyt) for the treatment of lymphomatous meningitis,165
were FDA approved in 1996 (DaunoXome), 1997 (AmBisome), and 1999 (DepoCyt), respectively, and are still on the
market.164,166–168
Liposomal formulations containing cholesterol of different
drugs, such as vincristine sulfate169 or cisplatin (Lipoplatin),170
have not been FDA approved yet but are on Phase II and Phase
III clinical trials, respectively.
Analytical science
Interest in liposome technologies and applications for analytical purposes is constantly growing, and four major areas of
activity can be identied, namely liquid chromatography (LC),
capillary electrophoresis (CE), biosensors, and immunoassays.140 In all four analytical techniques, cholesterol plays an
important role in liposome stabilisation.
LIQUID CHROMATOGRAPHY. The understanding of the interaction between cell membranes and different molecules (e.g.
drugs, proteins, and peptides) is of great importance in predicting the behaviour of the drug in the organism. In vivo
investigations of the fraction of the drug adsorbed in humans
and animals are time-consuming and difficult to perform. Since
liposomes structurally closely resemble natural membranes,
they are extensively used in medical and pharmaceutical
research as models for mimicking the structure and the function of biological cell membranes.171,172 The use of liposomes
immobilised within the pores of carrier gel beads as a stationary
phase for column chromatography with an aqueous mobile
phase is known as immobilised liposome chromatography
(ILC),173 a method that emerged in the 1990s171 and has proven
successful in studying solute–membrane interactions.174 In ILC,
variations in the retention volume depend on the extent of
solute–membrane interaction and can be precisely measured.175
Liposomes can be immobilised in these columns by several
ways173,176–178 including avidin–biotin interaction.140,171,179 This
specic binding pioneered by Yang et al. allowed prolonging the
column lifetime for over a year.175,179,180 Further, these liposome
columns have successfully been used to predict the drug
absorption in vivo by estimating the membrane partitioning
This journal is ª The Royal Society of Chemistry 2013
Nanoscale
coefficient of the diverse drugs. The results showed that, for
drugs that follow the transcellular passive transport route, the
liposome column could be used for a preliminary drug
screening, offering an alternative to the high throughput drug
screening system based on Caco-2 cells used by pharmaceutical
companies.175,181 In this context, cholesterol has been important
as a component of the small-intestine brush-border membranes
which are composed of egg phosphatidylcholine, phosphatidylserine (PS), phosphatidylethanolamine, and cholesterol.182
Liu et al. reported retention data of numerous drugs utilising
ILC and liposomes made of these components to mimic the
intestinal membranes. The aim was to predict drug intestinal
adsorption, since absorption of orally administered drugs in the
intestine (i.e. uptake of the drug through the cell membrane) is
the rst step of the drug’s action.175,181,183
CAPILLARY ELECTROPHORESIS. CE is an analytical technique
that separates ions based on their electrophoretic mobility with
the use of an applied voltage. Liposome capillary electrophoresis (LCE) is a recent approach that involves the use of liposomes as coating material184,185 or carrier.171,172 The details of the
technique are beyond of the scope of this review and for a more
detailed overview, the reader is referred to other reports.171,172
Here, just two examples to illustrate the importance of
cholesterol are discussed. Wiedmer et al. employed 1-palmitoyl2-oleyl-sn-glycero-3-phosphocholine (POPC) and POPC/PS liposomes with various amounts of cholesterol as carriers and
steroidal sex hormones as model analytes. The study investigated the inuence of cholesterol on the sizes and electrophoretic mobility of POPC and POPC/PS liposomes with special
focus on the inuence of cholesterol on possible selective
interactions between the steroids and the liposomal
membranes. Their results showed that the presence of cholesterol slightly increased the liposomal diameter, and signicant
differences in selectivity between the steroids and the liposomal
membranes were achieved through the addition of cholesterol.186 Alternatively, liposomes have been used as coating
materials in CE in order to mimic biological cell membranes,
since cell membranes are mainly composed of phospholipids
and cholesterol, and the interaction between the liposomes and
the analytes has been studied.185,187 As an example, Hautala and
collaborators showed the coating of silica capillaries with
anionic liposomes comprising POPC, bovine brain PS, and
cholesterol, and evaluated the coating effectiveness by examining the interactions of steroids with the coated capillaries.
Their results show that the capillaries can be successfully
coated with liposomes and those coated capillaries can be used
to study the interactions between phospholipid bilayers and
uncharged steroids. Since the steroids are neutral under the
applied conditions, the separation is based on hydrophobic
interactions with the liposome coating.187
BIOSENSORS. Biosensors show promise in many aspects of
medical care from drug development over early detection of
diseases to monitoring the progress of a treatment. All these
applications require sensitive, rapid, cheap, and reproducible
detection and recent advances in nano- and biotechnology as
well as chemistry, biochemistry, physics, and biology have made
outstanding contributions141 for the development of biosensors
Nanoscale, 2013, 5, 89–109 | 99
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
in medicine,188–190 for environmental applications,191 and in the
food industry.192,193 However, ways to immobilise biological
molecules while preserving their activity remains one of the
major challenges in the development of advanced biosensors.
Encapsulation techniques are among the most favourable
approaches to entrap biological molecules while preserving
their functionality for an extended period of time. Various
approaches have been employed for the encapsulation of biological material including polymeric vesicles,194 biomolecule–
nanoparticle hybrid systems,195 capsules assembled via the
Layer-by-Layer (LbL) technique,196,197 or single-enzyme nanoparticles where each enzyme molecule is surrounded by a
porous composite organic/inorganic network.198,199 However,
liposomes have emerged as lead candidates by providing a
comfortable cage which can preserve the biomolecule activity in
a three dimensional space, which is particular important for
enzymes.141 Fig. 6b shows a representation of a liposome
encapsulating enzymes. The substrate can diffuse across the
membrane through channel gates, react with the enzymes, and
the products can be released back in solution.141 In addition,
encapsulation offers other benecial properties e.g. amplication since liposomes concentrate the enzymes in a conned
space, thus, the enzymes are able to convert a higher amount of
substrate molecules into their corresponding products.172 This
feature is benecial in a number of biosensor applications such
as the determination of pH200 and oxygen,201 or the detection of
bacteria202,203 and other agents.204 For the creation of liposomes
in biosensing applications, cholesterol plays a crucial role in
controlling the uidity and, in particular, the permeability of
the lipid membrane in order to ensure stable entrapment of
molecules required for detection.172
An interesting example of cholesterol-containing liposomes
in this context was reported by McNamara and co-workers, who
developed a uorescence-based oxygen nanosensor by encapsulating an oxygen-sensitive dye in the internal compartment of
the liposomes.201 A major concern when developing liposomal
uorescence-based sensors is leaking of the dye molecules from
the supportive matrix. To this end, McNamara and collaborators prepared liposomes with a lipid composition consisting of
dimyristoylphosphatidylcholine, cholesterol, and dihexadecyl
phosphate and showed high stability toward dye leaking at
room temperature for 8 days, a fact which could be attributed to
the addition of cholesterol to the lipid membrane.
Since safety of water and food supplies has to be ensured to
avoid contamination of infectious agents, the detection of pathogenic organisms remains a crucial aspect. With the aim to
address this issue, Baeumner et al. developed a nucleic acid based
sensor, also known as a genosensor or gene probe, which is a
highly sensitive and specic RNA biosensor for the rapid detection of viable Escherichia coli (E. coli) as an indicator of pathogenic
organisms in water.203 Briey, the mRNA from E. coli was extracted, puried, amplied, and then quantied with the biosensor.
The biosensor is a membrane-based DNA/RNA hybridisation
system and cholesterol-containing liposomes (a mixture
composed of dipalmitoyl phosphatidyl choline (DPPC), cholesterol, dipalmitoyl phosphatidyl glycerol, and dipalmitoyl phosphatidyl ethanolamine) encapsulating sulphorhodamine for
100 | Nanoscale, 2013, 5, 89–109
Feature Article
signal amplication. The method is based on the formation of a
sandwich between a DNA-capture probe immobilised on a polyethersulfonate membrane, the target mRNA sequence, and a
DNA-reported probe coupled to the surface of a liposome (Fig. 6c).
When a specic E. coli mRNA is present, a sandwich is formed
between the DNA capture probe attached onto the polyethersulfonate membrane, the E. coli mRNA, and the reporter
probe attached to the liposomes, thus the liposomes being
captured in the capture/detection zone. Since the number of
liposomes is directly proportional to the amount of E. coli mRNA,
when non-specic RNA is present instead of E. coli mRNA, the
liposomes are not captured in the capture/detection zone, and no
signal is reported in the detection zone.203
IMMUNOASSAYS. Immunoassay formats rely on a directly or
indirectly detectable label. The label can be an easily detectable
molecule (e.g. radioactive or uorescent) or, alternatively, an
enzyme. In an enzyme linked immunosorbent assay (ELISA) the
enzyme label generates a measurable amount of product which
is (inversely) proportional to the unknown concentration of
analyte (usually an antigen).205 The technique essentially
requires any ligating reagent which can be immobilised, a
detection reagent that will bind specically, and an enzyme that
will generate a signal that can be quantied. LISA, liposome
immunosorbent assay, is the counterpart of ELISA, with the
enzymes replaced by liposomes encapsulating a large amount of
marker and receptor molecules. The sensitivity of the system is
high and the additional advantage is that, by lysing the liposomes, the detectable markers are released immediately, thus
avoiding the ELISA incubation step in which the substrate is
converted into the product.172 Similar to an ELISA, the encapsulated marker can be colorimetrically, uorimetrically, chemiluminometrically, or electrochemically detected upon lysis of
the immobilised liposomes.205 Additionally, most formats
applied in enzyme immunoassays can be used in combination
with liposomes.205 The stability of the liposomes is of paramount importance for successful LISA performance e.g. in
terms of sensitivity and selectivity. To increase the stability of
the liposome membrane, cholesterol in combination with
saturated lipids has been employed.205
Fig. 6d depicts a table with the most commonly used liposomal compositions and the markers used to detect different
analytes. As shown in the table, most liposomal compositions
contain cholesterol to equip the lipid bilayer with additional
stability.205 For instance, Kim and collaborators reported the
creation of a liposome immunoassay for the detection of gentamicin using phospholipase C to release the uorescent marker
from the liposomes.206,207 Gentamicin, a drug frequently used for
the treatment of serious Gram-negative microbial infections, was
chosen as a model analyte.206 The liposomes were composed of a
mixture of DPPC and cholesterol, since it was previously
demonstrated that this composition allows the lysis of the liposomes by the lowest concentration of phospholipase C.206,207
Cholesterol as anchor
So far, the aspect of the cholesterol’s ability to affect the
membrane properties of the liposomes and the consequences
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Feature Article
for different biomedical applications have been discussed. This
section considers the use of cholesterol for a different purpose,
namely as an anchor either to immobilise the liposomes to a
surface for biosensing applications, or to coat liposomes with
specic molecules.
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Biosensors
Liposomes hold enormous potential for biosensing applications, not only as labels as discussed previously, but also for the
establishment of a successful platform for high-throughput
(membrane) protein sensing.208 Immobilised liposomes in an
array format can act as supports for (membrane) proteins since
the lipid bilayer provides a favorable environment that allows
protein exibility and movement while avoiding their denaturation and loss of function. These sensors are of paramount
importance since proteins play a major role in disease developments and 60–70% of the drug targets are (membrane)
proteins.209
Approaches to immobilise intact liposomes include linkages
such as avidin–biotin,210,211 interaction between antibody and
antigen,212,213 disulde bonds,214 or the chemical linkage
between histidines,215 but also the chemisorption of vesicles
onto gold lms.214 However, when these types of linkages are
used, the controlled immobilisation of different types of liposomes to predened spots on the surface is impossible. This
challenge has been addressed by tethering liposomes to solid
supports via DNA-directed coupling, an approach that was rst
introduced by Niemeyer and co-workers.216
Several strategies have been developed for the DNA-labeling
of intact vesicles by using functionalised lipids such as thiolreactive maleimido-lipids217,218 and thiol derivatives of DNA.219
Alternately, several approaches which make use of cholesterolmodied DNA for spontaneous anchoring of liposomes to
(patterned) substrates with immobilized complementary
strands have been reported (Fig. 7ai).220–223 This non-covalent
approach is advantageous compared to the previously
mentioned concepts since it is largely independent of the lipid
composition of the liposomes, does not require chemical
modication of a lipid, has fast coupling rates, and there is noneed of introducing functionalised lipids. Therefore, by making
use of a naturally occurring membrane constituent, unwanted
side reactions between the functional groups and other
membrane constituents are eradicated. However, cholesterolbased anchoring of DNA is relatively weak, i.e. it is reversible. In
order to allow tagging of a type of liposomes with a specic DNA
sequence, the cholesterol anchor has to be strengthened by
using bivalent cholesterol DNA coupling.224 This approach
allows sorting of red and green liposomes from a mixture
(Fig. 7aii). In a continuation of this approach, ligand binding to
liposome arrays equipped with G-protein coupled receptors has
been demonstrated on the way to develop this platform into a
heterogeneous, self-sorting biosensing platform (Fig. 7b).225
PEGylation
One of the main drawbacks of liposomes in drug delivery is
their low stability in systemic circulation. Stealth liposomes
This journal is ª The Royal Society of Chemistry 2013
Nanoscale
were created when it was realised that neither mechanical nor
electrostatic stabilisation could improve their performance
signicantly enough.157 It has been widely demonstrated that
the incorporation of glycolipids such as monosialoganglioside
GM1226 into the lipid bilayer or the coating of liposomes with
hydrophilic polymer chains like polysaccharides226 or, preferentially, PEG226,227 becomes an efficient stabilisation tool by
providing a steric barrier. The particular efficiency of surfaceattached PEG chains has been explained by the combination of
their water solubility and exibility, which sterically stabilises
the liposomes by preventing them from self-aggregation and
fusion, as well as from opsonin adsorption, the rst step
towards clearance by the reticuloendothelial system.226–228 PEG
coated liposomes remain in the blood for up to 100 longer
than ordinary liposomes, thus increasing the pharmacological
efficacy of the encapsulated agents,157 and passive targeting to
tumors has been reported.227 The reader is referred to recent
reviews229–232 for a more detailed discussion on the topic of
PEGylated liposomes.
There are different ways to coat liposomes with PEG such as
by graing it to the lipids by covalent bonding.226 Alternatively,
cholesterol or phospholipids have been employed to anchor
PEG to the liposome membrane, and it has been shown that
cholesterol-PEG was easily incorporated, making cholesterol
the more successful anchor moiety.104,158,226–228,233–235 They speculated that long anchor units are difficult to insert into the
liposomal membranes or that there is a higher affinity between
cholesterol and the constituent lipids.227 PEG-cholesterol has
the added benet that it confers cohesion on lipid bilayers by
inducing tighter molecular packing and restricting the motions
of the hydrocarbon chains, thus improving the cargo retention.226 Long-circulating liposomes containing cholesterol–PEG
have already been successfully used in the cisplatin delivery in
vitro and in vivo.158 Fig. 7ci depicts a schematic illustration of
liposomes containing a mixture of cholesterol-PEG and thiolated cholesterol for cisplatin encapsulation. The in vivo
cisplatin concentrations in the kidney tissue of Chinese Kun
Ming mice aer injection of the liposome formulation and free
cisplatin were compared (Fig. 7cii). The results showed that
PEGylated liposomes could successfully avoid the peakconcentration in kidney aroused from free cisplatin, reducing
the in vivo acute nephrotoxicity.158
Capsosomes
Sub-compartmentalised systems hold tremendous potential as
cell mimics, which is an approach that aims to substitute for
lost or missing cellular function.236 Articial multi-compartment systems do not need to possess the entire complexity of
biological cells, but a specic key feature, which will mostly
depend on the application in mind (e.g. enzyme encapsulation
for enzyme replacement therapy to provide a biological-inspired
long term solution for patients with chronic diseases).
Mimicking the hierarchical sub-compartmentalised structure of
cells is essential to perform triggered, spatially separated,
encapsulated (enzymatic cascade) reactions.52,237 Among the
reported multi-compartment systems (e.g. vesosomes,238
Nanoscale, 2013, 5, 89–109 | 101
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
Fig. 7 Cholesterol as anchor: (a) (i) schematic illustration of a tethered vesicle–
DNA assembly, showing how the hybridisation of complementary cholesterol–
DNA pairs forms the (mobile) tether. The DNA array was produced by preferential
adsorption of biotin–BSA to Au spots, leaving the surrounding SiO2 substrate
available for spontaneous supported phospholipid bilayer (SPB) formation, followed by the addition of NeutrAvidin, which binds to biotin–BSA-modified Au
only. Biotin–DNAB and chol–DNAA specifically binds to NeutrAvidin/biotin–BSA/
Au and SPB/SiO2, respectively, followed by the immobilization of liposomes
tagged with the complementary DNA. (ii) Micrographs illustrating sorting of
liposomes tagged with different DNA. Micrographs (1) and (2) were obtained by
exposing the DNA-modified substrate to a mixture of red-labelled and greenlabelled liposomes tagged with different monovalent coupled chol–DNA. (3) and
102 | Nanoscale, 2013, 5, 89–109
Feature Article
liposomes within a liposome carrier, polymersomes within a
polymersome,239 polymer capsule within a polymer
capsule,240,241 polymer hydrogel capsules containing cubosomes242 or polymersomes243 and cellosomes,244 yeast cells
associated with a polymer membrane)245,246 capsosomes, intact
liposomes embedded into a polymer carrier capsule,52 are a
novel, well-characterised system with potential in therapeutic
cell mimicry. Capsosomes, as a dual composition system, can
take advantage of the different properties of the sub-compartments and the carrier capsule. Liposomes, due to the inherently
high impermeability of their lipid membranes, are ideal to
encapsulate small or fragile cargo. The polymeric carriers, due
to their semi-permeable nature, permit the interaction between
the internal and the external environment while providing the
structural integrity and help to overcome some of the limitations of liposomes such as instability under in vivo conditions
and the lack of control over their degradation. Capsosomes are
assembled via the LbL technique,247 by alternatingly depositing
polymer and liposomes onto silica particles, followed by the
assembly of the polymer carrier capsule and core dissolution
(Fig. 8a).
With the aim of stably anchoring the liposomes into the
polymer membrane, we employed cholesterol-modied polymers, i.e. cholesterol-containing PLL (PLLc),52,99 poly(methacrylic acid-co-cholesteryl methacrylate) (PMAc),52,99 and
poly(N-vinyl pyrrolidone-block-cholesteryl acrylate) (P(NVPc)).93
We also showed that PMAc was the more successful polymer to
anchor liposomes than PMA containing oleic acid (PMAoa).248
Interestingly, while PMAc, PMAoa, and PLLc led to the formation
of capsosomes with the liposomal units associated with the
polymer carrier capsule (Fig. 8b1), P(NVPc) promoted the “freeoating” of the liposomal sub-units in the void of the carrier
capsule (Fig. 8b2).93 Since P(NVPc) is a cholesterol-containing
uncharged block copolymer and contains the cholesterol
moieties in a short block, while the others are copolymers, we
speculated that in the former case the entanglement of the
liposome-anchoring polymer with the carrier capsule is minimised and, therefore, allows for the detachment of the liposomes from the polymer membrane. The cholesterol-modied
polymers allowed us to assemble capsosomes with up to
160 000 liposomes within a 3 mm diameter carrier capsule.249
Further, P(NVPc), PMAc, or PMAoa, allowed for the subsequent
assembly of the carrier capsule using the polymer pair P(NVP)
and thiol-modied poly(methacrylic acid) PMASH via hydrogen
bonding, followed by crosslinking of the thiols in the lm250 and
P(NVP) release at physiological conditions upon disruption of
the hydrogen bonds.251 Their functionality and their potential
(4) shows an identical experiment, but for a liposome mixture using bivalent
coupled chol–DNA. Reprinted with permission from ref. 224. Copyright (2005)
American Chemical Society. (b) Site-specific immobilisation of liposomes containing GPCRs is shown using ZeptoREADER imaging. Reprinted with permission
from ref. 225. (c) (i) Schematic illustration of the preparation of cisplatin, (cisdiammine dichloroplatinum(II); CDDP) liposomes. Adapted with permission from
ref. 158. (ii) In vivo CDDP concentration in kidney tissue of normal male Chinese
Kun Ming (KM) mice, at predetermined time intervals after injection of CDDP
loaded liposomes and free CDDP. Reprinted with permission from ref. 158.
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Feature Article
Nanoscale
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
for biomedical applications were conrmed by encapsulating
both hydrophilic52,93,99,249 and hydrophobic248,252 cargo within the
liposomal sub-compartments and the demonstration of the
payload activity in cell viability assays248,252 and for encapsulated
enzymatic catalysis.52,93,253 A particularly interesting example is a
two-step catalytic reaction in which the production of a
substrate was employed to subsequently trigger cargo release by
co-encapsulating glutathione reductase (GR) within cholesterolcontaining liposomes and a disulde-linked polymer–oligopeptide conjugate within the polymer carrier capsule
(Fig. 8ci).253 By incubating these capsosomes with oxidised
glutathione (GSSG) and by increasing the temperature above the
Tm of the liposomal subunits, the entrapped enzyme was
allowed to interact with the substrate GSSG and converted it
into its reduced product (GSH) which subsequently induced
the release of the encapsulated uorescent oligopeptides from
the capsosomes by reducing the disulde bond, as shown by the
decrease in uorescence intensity over time (Fig. 8cii). This
result brings capsosomes a step closer to potentially address a
real medical problem by continuously generating a potent
antioxidant while releasing a small molecule with therapeutic
relevance.
Conclusions and future perspectives
This feature article gives an overview over the current use of
cholesterol in bionanotechnology, including some fundamental
aspects in cholesterol chemistry and polymer chemistry, the
application of these polymeric materials into self-assembled
structures, and the development of higher order nano-structures, along with their use in biosensing, analytical sciences,
drug delivery, and cell mimicry.
In terms of cholesterol chemistry, cholesterol chloroformate
is commonly used to conjugate cholesterol. Further, esterication and etherication of the cholesterol’s hydroxyl group are
common ways to conjugate this molecule. A variety of cholesterol-containing end-functional polymers, homopolymers, and
co- and block copolymers have been synthesised and used for
the self-assembly of different micelles, nanoparticles, nanotubes, nanogels, or polymersomes. An interesting avenue that
has not been investigated is conjugation onto cholesterol in
other positions, besides the obvious hydroxyl, and how this
effects its self-assembly and function. Also, the ne-tuning of
Fig. 8 Capsosomes: (a) schematic illustration of the capsosome assembly. A silica
particle (i) is coated with a cholesterol-functionalised polymer precursor layer (ii),
liposomes (iii), and a cholesterol-functionalised polymer capping layer (iv), followed by subsequent polymer multilayer deposition (v), and removal of the silica
template core (vi). Liposomes are adsorbed onto the polymer surface non-covalently with cholesterol-modified polymers (iva). Cholesterol is spontaneously
incorporated into the lipid membrane (ivb). Reprinted with permission from ref.
This journal is ª The Royal Society of Chemistry 2013
99. (b) Fluorescence microscopy images of capsosomes containing fluorescently
labelled liposomes using PMAc (1) or PVPc (2) as precursor and capping layers.
While capsosomes assembled using PMAc contain the liposomal sub-units
attached onto the carrier membrane, PVPc promotes the free-floating of the
liposomes. Reprinted with permission from ref. 93. (c) (i) Release of encapsulated
oligopeptide KP9 from capsosomes triggered by glutathione reductase (GR).
Upon increasing the T above the Tm of the liposomal subunits, the entrapped GR
interacts with the oxidised substrate glutathione (GSSG) and it is converted into
its reduced product (GSH) which, in turn, induces the release of KP9 by reducing
the disulfide bond. (ii) Normalised fluorescence intensity of capsosomes encapsulating GR within the liposomal subcompartments and fluorescently labelled
KP9 upon incubation with GSSG and NADPH as a function of time. A decrease in
the fluorescence intensity indicates a release of KP9. Reprinted with permission
from ref. 253.
Nanoscale, 2013, 5, 89–109 | 103
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
the self-assembly process of cholesterol-modied polymers to
yield structures with increased complexity would be another
aspect to consider in the future. Although there are a few
examples where the self-assembled nanostructures have been
used in vivo, many of them were only examined in vitro using a
model drug, if at all. A future challenge will be to consider
specic medical conditions which require therapeutic
compounds to be delivered and to assess the pharmacokinetics
and pharmacodynamics of the cholesterol based delivery
vehicle under biologically relevant conditions. An important
question to address would be if the cholesterol-based delivery
vehicles would inherently have an impact on cells or the health
of animals in vivo.
Cholesterol has the ability to self-assemble from multicomponent solutions. Many fundamental aspects are being
understood and many applications are being thought of. The
future challenge here will be the stabilization and post-modication of helical ribbons in order to integrate them in devices
and use them as a tool in nanotechnology e.g. as nano-springs.
Cholesterol incorporated into liposomes also plays an
important role in biomedical applications. Its ability to modulate the physicochemical properties of lipid bilayer has been
employed to stabilise liposomes for their application in drug
delivery or analytical science. In the former case, in order to
make more liposome-based formulations commercially available for clinical applications, alternative concepts for stabilization and functionalization will have to be conceived. While
cholesterol will remain an integral building block, cholesterolmodied polymers, instead of (cholesterol-)modied lipids, as a
way to improve the stability and control over cargo retention
and release, should be considered more. In analytical science,
the use of cholesterol has a well-dened task, i.e. to stabilize the
membrane. The future challenge in this context remains to
successfully move from proof of concepts in research lab to
commercially available products.
Further, cholesterol can be used to anchor other molecules
such as PEG or DNA to the liposomes for their application in
biosensing or as “stealth” drug carriers. In the latter case, the
challenges are similar to the ones outlined above. One of the
aims when using DNA-tagged liposomes in biosensing is to
assemble a single-liposome array with the liposomes carrying
different membrane proteins, and to nd a means to analyse
the protein–analyte interaction in a fast, quantitative and
sensitive way. This would contribute considerably to the early
detection of disease and identication of suitable drug
candidates.
Cholesterol-modied polymers were found to be essential in
the assembly of capsosomes as simple cell mimics. These have
been well-characterized from a material point of view and
diverse functionality has been demonstrated. In our research,
we are convinced that capsosomes have the potential to
address clinical issues, when the proper route of administration and the suitable cell type to mimic is chosen. However, we
have yet to perform in vivo experiments and to consider actual
medical conditions. These are major future challenges to be
considered for further development of capsosomes in
biomedicine.
104 | Nanoscale, 2013, 5, 89–109
Feature Article
Overall, cholesterol is a small molecule which has had a
great impact in all the elds presented, and it will remain an
indispensable player in various areas of bionanotechnology.
Acknowledgements
This work was supported by a Sapere Aude Starting Grant from
the Danish Council for Independent Research, Technology and
Production Sciences, Denmark.
Notes and references
1 D. S. Goodsell, Bionanotechnology: Lessons from Nature,
Wiley, 2004.
2 J. Wang, ACS Nano, 2009, 3, 4–9.
3 S. J. Ebbens and J. R. Howse, So Matter, 2010, 6, 726–738.
4 R. Dreyfus, J. Baudry, M. L. Roper, M. Fermigier, H. A. Stone
and J. Bibette, Nature, 2005, 437, 862–865.
5 L. Zhang, K. E. Peyer and B. J. Nelson, Lab Chip, 2010, 10,
2203–2215.
6 H. Hess, in Annual Review of Biomedical Engineering, ed. M.
L. Yarmush, J. S. Duncan and M. L. Gray, 2011, vol. 13, pp.
429–450.
7 N. Michelotti, A. Johnson-Buck, A. J. Manzo and
N. G. Walter, Wiley Interdiscip. Rev.: Nanomed.
Nanobiotechnol., 2012, 4, 139–152.
8 R. M. Zadegan and M. L. Norton, Int. J. Mol. Sci., 2012, 13,
7149–7162.
9 A. Lakshmanan, S. G. Zhang and C. A. E. Hauser, Trends
Biotechnol., 2012, 30, 155–165.
10 X. Zhang, S. Boisse, C. Bui, P.-A. Albouy, A. Brulet, M.-H. Li,
J. Rieger and B. Charleux, So Matter, 2012, 8, 1130–1141.
11 J. M. Schnur, Science, 1993, 262, 1669–1676.
12 D. Landesman-Milo and D. Peer, J. Controlled Release, 2012,
161, 600–608.
13 M. S. Brown and J. L. Goldstein, Science, 1986, 232, 34–47.
14 M. E. Chevreul, Ann. Chim. Phys., 1816, 2, 339–372.
15 A. de Fourcroy, Ann. Chim., 1789, 3, 242–252.
16 M. E. Chevreul, Ann. Chim., 1815, 95, 5–50.
17 M. Berthelot, Ann. Chim. Phys., 1859, 56, 51–98.
18 O. Diels and E. Abderhalden, Ber. Dtsch. Chem. Ges., 1904,
37, 3092–3103.
19 J. D. Bernal, Nature, 1932, 129, 277–278.
20 A. Windaus and K. Neukirchen, Ber. Dtsch. Chem. Ges.,
1919, 52, 1915–1919.
21 A. Windaus, Hoppe-Seyler’s Z. Physiol. Chem., 1932, 213,
147–187.
22 P. L. Yeagle, The Membranes of Cells, Academic Press, 1993.
23 P. L. Yeagle, Biochim. Biophys. Acta, 1985, 822, 267–287.
24 P. L. Yeagle, The Structure of Biological Membranes, CRC
Press, Boca Raton, 2005.
25 D. M. Medeiros and R. E. C. Wildman, Advanced Human
Nutrition, Jones & Bartlett Publishers, 2011.
26 C. J. Fielding and P. E. Fielding, J. Lipid Res., 1995, 36, 211–
228.
27 F. R. Maxeld and D. Wustner, J. Clin. Invest., 2002, 110,
891–898.
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Feature Article
28 F. J. Field, E. Born, S. Murthy and S. N. Mathur, J. Lipid Res.,
1998, 39, 333–343.
29 J. Vogel, The Pathological Anatomy of the Human Body, H.
Bailliere, 1847.
30 M. R. Hayden and S. C. Tyagi, Cardiovasc. Diabetol., 2004,
3, 1.
31 P. R. Moreno, J. Sanz and V. Fuster, J. Am. Coll. Cardiol.,
2009, 53, 2315–2323.
32 C. Doree, Biochem. J., 1909, 4, 72–106.
33 W. S. Johnson, Bioorg. Chem., 1976, 5, 51–98.
34 R. E. Ostlund and D. E. Matthews, J. Lipid Res., 1993, 34,
1825–1831.
35 L. J. Goad and T. Akihisa, Analysis of Sterols, Blackie
Academic & Professional, 1997.
36 J. L. Goldstein and M. S. Brown, Nature, 1990, 343, 425–430.
37 W. D. Nes, Chem. Rev., 2011, 111, 6423–6451.
38 K. Simons and W. L. C. Vaz, Annu. Rev. Biophys. Biomol.
Struct., 2004, 33, 269–295.
39 E. Ikonen, Nat. Rev. Mol. Cell Biol., 2008, 9, 125–138.
40 N. B. Javitt, FASEB J., 1994, 8, 1308–1311.
41 D. R. Schmidt, S. R. Holmstrom, K. F. Tacer, A. L. Bookout,
S. A. Kliewer and D. J. Mangelsdorf, J. Biol. Chem., 2010, 285,
14486–14494.
42 P. Insel, D. Ross, K. McMahon and M. Bernstein, Nutrition,
Jones and Bartlett Publishers, 2004.
43 G. Vanmeer, Annu. Rev. Cell Biol., 1989, 5, 247–275.
44 V. Cherezov, D. M. Rosenbaum, M. A. Hanson,
S. G. F. Rasmussen, F. S. Thian, T. S. Kobilka, H.-J. Choi,
P. Kuhn, W. I. Weis, B. K. Kobilka and R. C. Stevens,
Science, 2007, 318, 1258–1265.
45 A. S. Achalkumar, R. J. Bushby and S. D. Evans, So Matter,
2010, 6, 6036–6051.
46 M. K. Bijsterbosch, E. T. Rump, R. L. A. D. Vrueh,
R. Dorland, R. van Veghel, K. L. Tivel, E. A. L. Biessen,
T. J. C. van Berkel and M. Manoharan, Nucleic Acids Res.,
2000, 28, 2717–2725.
47 S.-O. Han, R. I. Mahato and S. W. Kim, Bioconjugate Chem.,
2001, 12, 337–345.
48 S. Boisse, J. Rieger, A. Di-Cicco, P. A. Albouy, C. Bui, M. H. Li
and B. Charleux, Macromolecules, 2009, 42, 8688–8696.
49 A. C. De Visser, K. De Groot, J. Feyen and A. Bantjes,
J. Polym. Sci., Part A-1: Polym. Chem., 1971, 9, 1893–1899.
50 A. C. De Visser, J. Feyen, K. De Groot and A. Bantjes,
J. Polym. Sci., Part B: Polym. Lett., 1970, 8, 805–808.
51 Y. Zhou and R. M. Kasi, J. Polym. Sci., Part A: Polym. Chem.,
2008, 46, 6801–6809.
52 B. Städler, R. Chandrawati, A. D. Price, S.-F. Chong,
K. Breheney, A. Postma, L. A. Connal, A. N. Zelikin and
F. Caruso, Angew. Chem., Int. Ed., 2009, 48, 4359–4362.
53 S. Sevimli, S. Sagnella, M. Kavallaris, V. Bulmus and
T. P. Davis, Polym. Chem., 2012, 3, 2057–2069.
54 S. Yusa, M. Kamachi and Y. Morishima, Macromolecules,
2000, 33, 1224–1231.
55 S.-K. Ahn, L. T. Nguyen Le and R. M. Kasi, J. Polym. Sci., Part
A: Polym. Chem., 2009, 47, 2690–2701.
56 J.-F. Lutz, S. Pfeifer and Z. Zarafshani, QSAR Comb. Sci.,
2007, 26, 1151–1158.
This journal is ª The Royal Society of Chemistry 2013
Nanoscale
57 J. T. Xu, L. Tao, C. Boyer, A. B. Lowe and T. P. Davis,
Macromolecules, 2011, 44, 299–312.
58 J. Q. Liu, E. Setijadi, Y. K. Liu, M. R. Whittaker, C. Boyer and
T. P. Davis, Aust. J. Chem., 2010, 63, 1245–1250.
59 Y. Zhu, Y. Zhou, Z. Chen, R. Lin and X. Wang, Polymer, 2012,
53, 3566–3576.
60 Y. Liu, Y. Wang, D. Zhuang, J. Yang and J. Yang, J. Colloid
Interface Sci., 2012, 377, 197–206.
61 D. Smith, S. H. Clark, P. A. Bertin, B. L. Mirkin and
S. T. Nguyen, J. Mater. Chem., 2009, 19, 2159–2165.
62 Y. Zhou, S.-k. Ahn, R. K. Lakhman, M. Gopinadhan,
C. O. Osuji and R. M. Kasi, Macromolecules, 2011, 44,
3924–3934.
63 G. Stübs, B. Rupp, R. R. Schumann, N. W. J. Schröder and
J. Rademann, Chem.–Eur. J., 2010, 16, 3536–3544.
64 J. C. Chabala and T. Y. Shen, Carbohydr. Res., 1978, 67, 55–
63.
65 Y. Iwasaki and K. Akiyoshi, Biomacromolecules, 2006, 7,
1433–1438.
66 A.-C. Albertsson and I. K. Varma, Biomacromolecules, 2003,
4, 1466–1486.
67 T. Zou, S.-X. Cheng and R.-X. Zhuo, Colloid Polym. Sci.,
2005, 283, 1091–1099.
68 L. Zhang, Q.-R. Wang, X.-S. Jiang, S.-X. Cheng and
R.-X. Zhuo, J. Biomater. Sci., Polym. Ed., 2005, 16, 1095–1108.
69 T. Zou, F. Li, S.-X. Cheng and R.-X. Zhuo, J. Biomater. Sci.,
Polym. Ed., 2006, 17, 1093–1106.
70 T. Wan, T. Zou, S.-X. Cheng and R.-X. Zhuo,
Biomacromolecules, 2005, 6, 524–529.
71 H. A. Klok, J. J. Hwang, S. N. Iyer and S. I. Stupp,
Macromolecules, 2002, 35, 746–759.
72 H. A. Klok, J. J. Hwang, J. D. Hartgerink and S. I. Stupp,
Macromolecules, 2002, 35, 6101–6111.
73 K. Sugiyama, R. Hanamura and M. Sugiyama, J. Polym. Sci.,
Part A: Polym. Chem., 2000, 38, 3369–3377.
74 J. Chiefari, Y. K. Chong, F. Ercole, J. Krstina, J. Jeffery,
T. P. T. Le, R. T. A. Mayadunne, G. F. Meijs, C. L. Moad,
G. Moad, E. Rizzardo and S. H. Thang, Macromolecules,
1998, 31, 5559–5562.
75 G. Moad, E. Rizzardo and S. H. Thang, Acc. Chem. Res., 2008,
41, 1133–1142.
76 G. Moad, E. Rizzardo and S. H. Thang, Polymer, 2008, 49,
1079–1131.
77 G. Moad, E. Rizzardo and S. H. Thang, Aust. J. Chem., 2009,
62, 1402–1472.
78 G. Moad, E. Rizzardo and S. H. Thang, Aust. J. Chem., 2012,
65, 985–1076.
79 M. Kato, M. Kamigaito, M. Sawamoto and T. Higashimura,
Macromolecules, 1995, 28, 1721–1723.
80 V. Percec and B. Barboiu, Macromolecules, 1995, 28, 7970–
7972.
81 J.-S. Wang and K. Matyjaszewski, J. Am. Chem. Soc., 1995,
117, 5614–5615.
82 D. M. Haddleton, R. Edmonds, A. M. Heming, E. J. Kelly and
D. Kukulj, New J. Chem., 1999, 23, 477–479.
83 J. P. Xu, J. Ji, W. D. Chen and J. C. Shen, Macromol. Biosci.,
2005, 5, 164–171.
Nanoscale, 2013, 5, 89–109 | 105
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
84 J. P. Xu, J. Ji, W. D. Chen and J. C. Shen, J. Controlled Release,
2005, 107, 502–512.
85 F. Segui, X. P. Qiu and F. M. Winnik, J. Polym. Sci., Part A:
Polym. Chem., 2008, 46, 314–326.
86 J. Liu, H. Liu, V. Bulmus, L. Tao, C. Boyer and T. P. Davis,
J. Polym. Sci., Part A: Polym. Chem., 2010, 48, 1399–1405.
87 C. W. Bielawski and R. H. Grubbs, Prog. Polym. Sci., 2007,
32, 1–29.
88 S. Sutthasupa, M. Shiotsuki and F. Sanda, Polym. J., 2010,
42, 905–915.
89 G. Hardy and K. Nyitrai, Acta Chim. Hung., 1970, 65, 301–
310.
90 G. Hardy, K. Nyitrai and F. Cser, Polymerization of
Cholesteryl Acrylate in its Smectic Liquid Crystalline State,
1969.
91 S. J. He, Y. Zhang, Z. H. Cui, Y. Z. Tao and B. L. Zhang, Eur.
Polym. J., 2009, 45, 2395–2401.
92 Y. J. Liu, Y. Z. Wang, D. Q. Zhuang, J. J. Yang and J. Yang, J.
Colloid Interface Sci., 2012, 377, 197–206.
93 L. Hosta-Rigau, S. F. Chung, A. Postma, R. Chandrawati,
B. Städler and F. Caruso, Adv. Mater., 2011, 23, 4082–
4087.
94 L. Hosta-Rigau, B. E. B. Jensen, K. S. Fjeldsø, A. Postma,
G. Li, K. N. Goldie, F. Albericio, A. N. Zelikin and
B. Städler, Adv. Healthcare Mater., 2012, 1, 791–795.
95 V. Shibaev, M. Ivanov, N. Boiko and E. Chernikova, Dokl.
Chem., 2009, 427, 183–185.
96 T. Kaneko, H. Nagasawa, J. P. Gong and Y. Osada,
Macromolecules, 2003, 37, 187–191.
97 Z. Hongbo, L. Yaobang, Z. Haoyu and W. Xiaogong, Acta
Polym. Sin., 2004, 1, 327–332.
98 S. K. Filippov, P. Chytil, P. V. Konarev, M. Dyakonova,
C. Papadakis, A. Zhigunov, J. Plestil, P. Stepanek,
T.
Etrych,
K.
Ulbrich
and
D.
I.
Svergun,
Biomacromolecules, 2012, 13, 2594–2604.
99 R. Chandrawati, B. Städler, A. Postma, L. A. Connal,
S.-F. Chong, A. N. Zelikin and F. Caruso, Biomaterials,
2009, 30, 5988–5998.
100 S. Sevimli, F. Inci, H. M. Zareie and V. Bulmus,
Biomacromolecules, 2012, 13, 3064–3075.
101 L. Yang, B. Zhang, L. Wen, Q. Liang and L.-M. Zhang,
Carbohydr. Polym., 2007, 68, 218–225.
102 E. Ranucci, M. A. Suardi, R. Annunziata, P. Ferruti,
F. Chiellini and C. Bartoli, Biomacromolecules, 2008, 9,
2693–2704.
103 Y. Zhou, V. A. Briand, N. Sharma, S.-k. Ahn and R. M. Kasi,
Materials, 2009, 2, 636–660.
104 S.-I. Yusa, Int. J. Polym. Sci., 2012, 2012, 609767–609777.
105 D. S. Chung, G. B. Benedek, F. M. Konikoff and
J. M. Donovan, Proc. Natl. Acad. Sci. U. S. A., 1993, 90,
11341–11345.
106 F. M. Konikoff, D. S. Chung, J. M. Donovan, D. M. Small and
M. C. Carey, J. Clin. Invest., 1992, 90, 1155–1160.
107 F. M. Konikoff, D. E. Cohen and M. C. Carey, Mol. Cryst. Liq.
Cryst. Sci. Technol., Sect. A, 1994, 248, 291–296.
108 B. Smith, Y. Zastavker and G. Benedek, Phys. Rev. Lett.,
2001, 87, 2781011–2781014.
106 | Nanoscale, 2013, 5, 89–109
Feature Article
109 Y. V. Zastavker, N. Asherie, A. Lomakin, J. Pande,
M. Donovan, J. M. Schnur and J. B. Benedek, Proc. Natl.
Acad. Sci. U. S. A., 1999, 96, 7883–7887.
110 G. H. M. van der Heijden and E. L. Starostin, Phys. Rev. Lett.,
2008, 101, 4.
111 B. Khaykovich, N. Kozlova, W. Choi, A. Lomakin,
C. Hossain, Y. Sung, R. R. Dasari, M. S. Feld and
G. B. Benedek, Proc. Natl. Acad. Sci. U. S. A., 2009, 106,
15663–15666.
112 W. Choi, C. Fang-Yen, K. Badizadegan, S. Oh, N. Lue,
R. R. Dasari and M. S. Feld, Nat. Methods, 2007, 717–
719.
113 M. Kim, Y. Choi, C. Fang-Yen, Y. Sung, R. R. Dasari,
M. S. Feld and W. Choi, Opt. Lett., 2011, 36, 148–150.
114 S.-I. Yusa, M. Kamachi and Y. Morishima, Langmuir, 1998,
14, 6059–6067.
115 Y. Jin, R. Xin, P. Ai and D. Chen, Int. J. Pharm., 2008, 350,
330–337.
116 Q. V. Bach, J. R. Moon, Y. S. Jeon, W.-S. Choe and J.-H. Kim,
J. Appl. Polym. Sci., 2011, 120, 1685–1693.
117 X. Zhu and M. Nichifor, Acc. Chem. Res., 2002, 35, 539–546.
118 C.-S. Chaw, K.-W. Chooi, X.-M. Liu, C.-w. Tan, L. Wang and
Y.-Y. Yang, Biomaterials, 2004, 25, 4297–4308.
119 X. Liu, K. P. Pramoda, Y. Yang, S. Y. Chow and C. He,
Biomaterials, 2004, 25, 2619–2628.
120 H. Zeng, Y. Li, H. Zhang and X. Wang, Acta Polym. Sin.,
2004, 1, 327–332.
121 E. Akiyama, N. Morimoto, P. Kujawa, Y. Ozawa,
F. M. Winnik and K. Akiyoshi, Biomacromolecules, 2007, 8,
2366–2373.
122 X. Yuan, H. Li and Y. Yuan, Carbohydr. Polym., 2006, 65,
337–345.
123 J. Yu, Y. Li, L. Qiu and Y. Jin, J. Pharm. Pharmacol., 2009, 61,
713–719.
124 Y.-S. Wang, Q. Jiang, R.-S. Li, L.-L. Liu, Q.-Q. Zhang,
Y.-M. Wang and J. Zhao, Nanotechnology, 2008, 19,
145101–145109.
125 Y. Wang, Q. Jiang, L. R. Liu and Q. Zhang, Polymer, 2007, 48,
4135–4142.
126 Y. Wang, L. Liu, J. Weng and Q. Zhang, Carbohydr. Polym.,
2007, 69, 597–606.
127 Y.-S. Wang, L.-R. Liu, Q. Jiang and Q.-Q. Zhang, Eur. Polym.
J., 2007, 43, 43–51.
128 X. Li, M. Chen, z. Zhou, L. Liu and Q. Zhang, Colloids Surf.,
B, 2012, 1, 136–141.
129 X. Li, M. Chen, W. Yang, Z. Zhou, L. Liu and Q. Zhang,
Colloids Surf., B, 2012, 92, 136–141.
130 C.-S. Chern, H.-C. Chiu and Y.-C. Chuang, Polym. Int., 2004,
53, 420–429.
131 K. Nagahama, T. Ouchi and Y. Ohya, Adv. Funct. Mater.,
2008, 18, 1220–1231.
132 C. J. Thompson, C. Ding, X. Qu, Z. Yang, I. F. Uchegbu,
L. Tetley and W. P. Cheng, Colloid Polym. Sci., 2008, 286,
1511–1526.
133 F. van de Manakker, T. Vermonden, N. el Morabit, C. F. van
Nostrum and W. E. Hennink, Langmuir, 2008, 24, 12559–
12567.
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Feature Article
134 D. Yang, J. Zhu, Z. Huang, H. Ren and Z. Zheng, Colloids
Surf., B, 2008, 63, 192–199.
135 L. Jia, P.-A. Albouy, A. Di Cicco, A. Cao and M. Li, Polymer,
2011, 52, 2565–2575.
136 Y. Wang, C.-Y. Ke, C. W. Beh, S.-Q. Liu, S.-H. Goh and
Y.-Y. Yang, Biomaterials, 2007, 28, 5358–5368.
137 J. P. Xu, J. Ji, W. D. Chen and J. C. Shen, in Asbm6: Advanced
Biomaterials Vi, ed. X. Zhang, J. Tanaka, Y. Yu and Y.
Tabata, 2005, vol. 288–289, pp. 465–468.
138 P. Pescador, N. Brodersen, H. A. Scheidt, M. Loew,
G. Holland, N. Bannert, J. Liebscher, A. Herrmann,
D. Huster and A. Arbuzova, Chem. Commun., 2010, 46,
5358.
139 L. Long, X. Yuan, J. Chang, Z. Zhang, M. Gu, T. Song,
Y. Xing, X. Yuan, S. Jiang and J. Sheng, Carbohydr. Polym.,
2012, 87, 2630–2637.
140 A. Jesorka and O. Orwar, Annu. Rev. Anal. Chem., 2008, 1,
801–832.
141 B.-W. Park, D.-Y. Yoon and D.-S. Kim, Biosens. Bioelectron.,
2010, 26, 1–10.
142 J. Thongborisute, A. Tsuruta, Y. Kawabata and H. Takeuchi,
J. Drug Targeting, 2006, 14, 147–154.
143 Y. Gerelli, S. Barbieri, M. T. Di Bari, A. Deriu, L. Cantu,
P. Brocca, F. Sonvico, P. Colombo, R. May and S. Motta,
Langmuir, 2008, 24, 11378–11384.
144 P. M. B. Goncalves Maia Campos, F. B. de Camargo Junior,
J. P. de Andrade and L. R. Gaspar, Photochem. Photobiol.,
2012, 88, 748–752.
145 T. M. Taylor, P. M. Davidson, B. D. Bruce and J. Weiss, Crit.
Rev. Food Sci. Nutr., 2005, 45, 587–605.
146 C. Kirby, J. Clarke and G. Gregoriadis, Biochem. J., 1980,
186, 591–598.
147 C. Kirby, J. Clarke and G. Gregoriadis, FEBS Lett., 1980, 111,
324–328.
148 H. Ohvo-Rekilä, B. Ramstedt, P. Leppimaki and J. P. Slotte,
Prog. Lipid Res., 2002, 41, 66–97.
149 T. Rog, M. Pasenkiewicz-Gierula, I. Vattulainen and
M. Karttunen, Biochim. Biophys. Acta, Biomembr., 2009,
1788, 97–121.
150 B. J. Boyd, Expert Opin. Drug Delivery, 2008, 5, 69–85.
151 E. A. Trafny, M. Antos-Bielska and J. Grzybowski, J.
Microencapsulation, 1999, 16, 419–429.
152 B. Ludewig, F. Barchiesi, M. Pericin, R. M. Zinkernagel,
H. Hengartner and R. A. Schwendener, Vaccine, 2000, 19,
23–32.
153 D. D. Lasic, J. J. Vallner and P. K. Working, Curr. Opin. Mol.
Ther., 1999, 1, 177–185.
154 M. A. Kisel, L. N. Kulik, I. S. Tsybovsky, A. P. Vlasov,
M. S. Vorob’yov, E. A. Kholodova and Z. V. Zabarovskaya,
Int. J. Pharm., 2001, 216, 105–114.
155 M. M. Gaspar, R. PerezSoler and M. E. M. Cruz, Cancer
Chemother. Pharmacol., 1996, 38, 373–377.
156 F. Eckstein, Expert Opin. Biol. Ther., 2007, 7, 1021–1034.
157 D. D. Lasic and D. Papahadjopoulos, Science, 1995, 267,
1275–1276.
158 Y. Kuang, J. Liu, Z. Liu and R. Zhuo, Biomaterials, 2012, 33,
1596–1606.
This journal is ª The Royal Society of Chemistry 2013
Nanoscale
159 B. Ceh, M. Winterhalter, P. M. Frederik, J. J. Vallner and
D. D. Lasic, Adv. Drug Delivery Rev., 1997, 24, 165–177.
160 Y. C. Barenholz, J. Controlled Release, 2012, 160, 117–134.
161 D. C. Drummond, O. Meyer, K. L. Hong, D. B. Kirpotin and
D. Papahadjopoulos, Pharmacol. Rev., 1999, 51, 691–
743.
162 Anonymous, J. Int. Assoc. Phys. AIDS Care, 1996, 2, 50–51.
163 G. W. Boswell, D. Buell and I. Bekersky, J. Clin. Pharmacol.,
1998, 38, 583–592.
164 K. V. Clemons and D. A. Stevens, Antimicrob. Agents
Chemother., 2004, 48, 1047–1050.
165 Anonymous, Biotechnol. Law Rep., 1999, 18, 257.
166 Relevant homepages, http://www.daunoxome.com/, http://
www.multivu.com/mnr/54292-galen-chemotherapy-agentdaunoxome-liposomal-daunorubicin-kaposi-s-sarcoma.
167 J. R. Azanza Perea and J. Barberan, Rev. Esp. Quimioter.,
2012, 25, 17–24.
168 M. C. Chamberlain, J. Neuro-Oncol., 2012, 109, 143–
148.
169 D. A. Thomas, H. M. Kantarjian, W. Stock, L. T. Heffner,
S. Faderl, G. Garcia-Manero, A. Ferrajoli, W. Wierda,
S. Pierce, B. Lu, S. R. Deitcher and S. O’Brien, Cancer,
2009, 115, 5490–5498.
170 G. P. Stathopoulos and T. Boulikas, J. Drug Delivery, 2012,
2012, 581363–581373.
171 S. K. Wiedmer, M. S. Jussila and M. L. Riekkola, TrAC,
Trends Anal. Chem., 2004, 23, 562–582.
172 A. Gomez-Hens and J. M. Fernandez-Romero, TrAC, Trends
Anal. Chem., 2005, 24, 9–19.
173 P. Lundahl and Q. Yang, J. Chromatogr., A, 1991, 544, 283–
304.
174 P. Lundahl and F. Beigi, Adv. Drug Delivery Rev., 1997, 23,
221–227.
175 X. Y. Liu, C. Nakamura, Q. Yang, N. Kamo and J. Miyake, J.
Chromatogr., A, 2002, 961, 113–118.
176 M. Sandberg, P. Lundahl, E. Greijer and M. Belew, Biochim.
Biophys. Acta, Gen. Subj., 1987, 924, 185–192.
177 E. Krause, M. Dathe, T. Wieprecht and M. Bienert, J.
Chromatogr., A, 1999, 849, 125–133.
178 Q. Yang, X. Y. Liu, M. Yoshimoto, R. Kuboi and J. Miyake,
Anal. Biochem., 1999, 268, 354–362.
179 Q. Yang, X. Y. Liu, S. Ajiki, M. Hara, P. Lundahl and
J. Miyake, J. Chromatogr., Biomed. Appl., 1998, 707, 131–141.
180 X. Y. Liu, Q. Yang, C. Nakamura and J. Miyake, J.
Chromatogr., Biomed. Appl., 2001, 750, 51–60.
181 X. Liu, B. Testa and A. Fahr, Pharm. Res., 2011, 28, 962–977.
182 S. Chapelle and M. Gillesbaillien, Biochim. Biophys. Acta,
Lipids Lipid Metab., 1983, 753, 269–271.
183 X. Liu, P. Fan, M. Chen, H. Hefesha, G. K. E. Scriba,
D. Gabel and A. Fahr, Helv. Chim. Acta, 2010, 93, 203–211.
184 Y. X. Zhang, R. Zhang, S. Hjerten and P. Lundahl,
Electrophoresis, 1995, 16, 1519–1523.
185 J. M. Cunliffe, N. E. Baryla and C. A. Lucy, Anal. Chem.,
2002, 74, 776–783.
186 S. K. Wiedmer, M. S. Jussila, J. M. Holopainen,
J. M. Alakoskela, P. K. J. Kinnunen and M. L. Riekkola, J.
Sep. Sci., 2002, 25, 427–437.
Nanoscale, 2013, 5, 89–109 | 107
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Nanoscale
187 J. T. Hautala, M. V. Linden, S. K. Wiedmer, S. J. Ryhanen,
M. J. Saily, P. K. J. Kinnunen and M. L. Riekkola, J.
Chromatogr., A, 2003, 1004, 81–90.
188 N. Dale, S. Hatz, F. M. Tian and E. Llaudet, Trends
Biotechnol., 2005, 23, 420–428.
189 A. Mueller, Mini-Rev. Med. Chem., 2005, 5, 231–239.
190 S. K. Arya, M. Datta and B. D. Malhotra, Biosens.
Bioelectron., 2008, 23, 1083–1100.
191 M. Badihi-Mossberg, V. Buchner and J. Rishpon,
Electroanalysis, 2007, 19, 2015–2028.
192 H. Nakamura and I. Karube, Anal. Bioanal. Chem., 2003,
377, 446–468.
193 S. Andreescu and J. L. Marty, Biomol. Eng., 2006, 23, 1–15.
194 G. B. Sukhorukov, A. L. Rogach, B. Zebli, T. Liedl,
A. G. Skirtach, K. Kohler, A. A. Antipov, N. Gaponik,
A. S. Susha, M. Winterhalter and W. J. Parak, Small, 2005,
1, 194–200.
195 I. Willner, R. Baron and B. Willner, Biosens. Bioelectron.,
2007, 22, 1841–1852.
196 D. Trau and R. Renneberg, Biosens. Bioelectron., 2003, 18,
1491–1499.
197 B. M. Wohl and J. F. J. Engbersen, J. Controlled Release,
2012, 158, 2–14.
198 J. Kim, J. W. Grate and P. Wang, Chem. Eng. Sci., 2006, 61,
1017–1026.
199 J. Kim, J. W. Grate and P. Wang, Trends Biotechnol., 2008,
26, 639–646.
200 T. Nguyen, K. P. McNamara and Z. Rosenzweig, Anal. Chim.
Acta, 1999, 400, 45–54.
201 K. P. McNamara and Z. Rosenzweig, Anal. Chem., 1998, 70,
4853–4859.
202 R. Jelinek and S. Kolusheva, Biotechnol. Adv., 2001, 19, 109–
118.
203 A. J. Baeumner, R. N. Cohen, V. Miksic and J. H. Min,
Biosens. Bioelectron., 2003, 18, 405–413.
204 J. R. Chen, Y. Q. Miao, N. Y. He, X. H. Wu and S. J. Li,
Biotechnol. Adv., 2004, 22, 505–518.
205 H. A. H. Rongen, A. Bult and W. P. vanBennekom, J.
Immunol. Methods, 1997, 204, 105–133.
206 C. K. Kim and K. M. Park, J. Immunol. Methods, 1994, 170,
225–231.
207 S. J. Lim and C. K. Kim, Anal. Biochem., 1997, 247, 89–95.
208 M. Bally, K. Bailey, K. Sugihara, D. Grieshaber, J. Voeroes
and B. Stadler, Small, 2010, 6, 2481–2497.
209 K. Lundstrom, Cell. Mol. Life Sci., 2006, 63, 2597–2607.
210 Y. Barenholz, Curr. Opin. Colloid Interface Sci., 2001, 6, 66–
77.
211 L. S. Jung, J. S. Shumaker-Parry, C. T. Campbell, S. S. Yee
and M. H. Gelb, J. Am. Chem. Soc., 2000, 122, 4177–4184.
212 T. ShibataSeki, J. Masai, T. Tagawa, T. Sorin and S. Kondo,
Thin Solid Films, 1996, 273, 297–303.
213 C. R. MacKenzie, T. Hirama, K. K. Lee, E. Altman and
N. M. Young, J. Biol. Chem., 1997, 272, 5533–5538.
214 I. Stanish, J. P. Santos and A. Singh, J. Am. Chem. Soc., 2001,
123, 1008–1009.
215 T. Stora, Z. Dienes, H. Vogel and C. Duschl, Langmuir, 2000,
16, 5471–5478.
108 | Nanoscale, 2013, 5, 89–109
Feature Article
216 C. M. Niemeyer, T. Sano, C. L. Smith and C. R. Cantor,
Nucleic Acids Res., 1994, 22, 5530–5539.
217 B. Chaize, M. Nguyen, T. Ruysschaert, V. le Berre,
E. Trevisiol, A. M. Caminade, J. P. Majoral, G. Pratviel,
B. Meunier, M. Winterhalter and D. Fournier,
Bioconjugate Chem., 2006, 17, 245–247.
218 B. Städler, M. Bally, D. Grieshaber, J. Voeroes, A. Brisson
and H. M. Grandin, Biointerphases, 2006, 1, 142–145.
219 C. Yoshina-Ishii and S. G. Boxer, J. Am. Chem. Soc., 2003,
125, 3696–3697.
220 S. Svedhem, I. Pfeiffer, C. Larsson, C. Wingren,
C. Borrebaeck and F. Hook, ChemBioChem, 2003, 4, 339–
343.
221 B. Städler, D. Falconnet, I. Pfeiffer, F. Hook and J. Voros,
Langmuir, 2004, 20, 11348–11354.
222 J. J. Benkoski and F. Hook, J. Phys. Chem. B, 2005, 109,
9773–9779.
223 M. R. Dusseiller, B. Niederberger, B. Stadler, D. Falconnet,
M. Textor and J. Voros, Lab Chip, 2005, 5, 1387–1392.
224 I. Pfeiffer and F. Hook, J. Am. Chem. Soc., 2004, 126, 10224–
10225.
225 K. Bailey, M. Bally, W. Leifert, J. Voeroes and T. McMurchie,
Proteomics, 2009, 9, 2052–2063.
226 S. Beugin, K. Edwards, G. Karlsson, M. Ollivon and
S. Lesieur, Biophys. J., 1998, 74, 3198–3210.
227 I. Sugiyama and Y. Sadzuka, Biol. Pharm. Bull., 2007, 30,
208–211.
228 S. Beugin-Deroo, M. Ollivon and S. Lesieur, J. Colloid
Interface Sci., 1998, 202, 324–333.
229 V. P. Torchilin, Nat. Rev. Drug Discovery, 2005, 4, 145–160.
230 Y. Ikeda and Y. Nagasaki, in Polymers in Nanomedicine, ed.
S. Y. T. Kunugi, 2012, vol. 247, pp. 115–140.
231 S. Qian, C. Li and Z. Zuo, Curr. Drug Metab., 2012, 13, 372–
395.
232 R. R. Sawant and V. P. Torchilin, AAPS J., 2012, 14, 303–315.
233 C. Carrion, J. C. Domingo and M. A. de Madariaga, Chem.
Phys. Lipids, 2001, 113, 97–110.
234 X. B. Zhao, N. Muthusamy, J. C. Byrd and R. J. Lee, J. Pharm.
Sci., 2007, 96, 2424–2435.
235 C. Li, J. Cui, C. Wang, L. Zhang, X. Xiu, Y. Li, N. Wei, Y. Li
and L. Zhang, J. Pharm. Pharmacol., 2011, 63, 376–384.
236 Y. Zhang, W. C. Ruder and P. R. LeDuc, Trends Biotechnol.,
2008, 26, 14–20.
237 B. Städler, A. D. Price and A. N. Zelikin, Adv. Funct. Mater.,
2011, 21, 14–28.
238 E. T. Kisak, B. Coldren, C. A. Evans, C. Boyer and
J. A. Zasadzinski, Curr. Med. Chem., 2004, 11, 199–219.
239 H. C. Chiu, Y. W. Lin, Y. F. Huang, C. K. Chuang and
C. S. Chern, Angew. Chem., Int. Ed., 2008, 47, 1875–1878.
240 B. G. De Geest, S. De Koker, K. Immesoete, J. Demeester,
S. C. De Smedt and W. E. Hennink, Adv. Mater., 2008, 20,
3687–3691.
241 O. Kulygin, A. D. Price, S. F. Chong, B. Stadler, A. N. Zelikin
and F. Caruso, Small, 2010, 6, 1558–1564.
242 C. D. Driever, X. Mulet, A. P. R. Johnston, L. J. Waddington,
H. Thissen, F. Caruso and C. J. Drummond, So Matter,
2011, 7, 4257–4266.
This journal is ª The Royal Society of Chemistry 2013
View Article Online
Downloaded on 24/04/2013 13:43:56.
Published on 05 November 2012 on http://pubs.rsc.org | doi:10.1039/C2NR32923A
Feature Article
243 H. Lomas, A. P. R. Johnston, G. K. Such, Z. Zhu, K. Liang,
M. P. Van Koeverden, S. Alongkornchotikul and
F. Caruso, Small, 2011, 7, 2109–2119.
244 R. F. Fakhrullin and V. N. Paunov, Chem. Commun., 2009,
2511–2513.
245 R. Chandrawati, M. P. van Koeverden, H. Lomas and
F. Caruso, J. Phys. Chem. Lett., 2011, 2, 2639–2649.
246 Y. Wang, L. Hosta-Rigau, H. Lomas and F. Caruso, Phys.
Chem. Chem. Phys., 2011, 13, 4782–4801.
247 M.-L. De Temmerman, J. Demeester, S. C. De Smedt and
J. Rejman, Nanomedicine, 2012, 7, 771–788.
248 L. Hosta-Rigau, R. Chandrawati, E. Saveriades,
P. D. Odermatt, A. Postma, F. Ercole, K. Breheney,
K. L. Wark, B. Städler and F. Caruso, Biomacromolecules,
2010, 11, 3548–3555.
This journal is ª The Royal Society of Chemistry 2013
Nanoscale
249 R. Chandrawati, L. Hosta-Rigau, D. Vanderstraaten,
S. A. Lokuliyana, B. Städler, F. Albericio and F. Caruso,
ACS Nano, 2010, 4, 1351–1361.
250 S.-F. Chong, R. Chandrawati, B. Staedler, J. Park, J. Cho,
Y. Wang, Z. Jia, V. Bulmus, T. P. Davis, A. N. Zelikin and
F. Caruso, Small, 2009, 5, 2601–2610.
251 A. N. Zelikin, J. F. Quinn and F. Caruso, Biomacromolecules,
2006, 7, 27–30.
252 L. Hosta-Rigau, B. Städler, Y. Yan, E. C. Nice, J. K. Heath,
F. Albericio and F. Caruso, Adv. Funct. Mater., 2010, 20, 59–66.
253 R. Chandrawati, P. D. Odermatt, S.-F. Chong, A. D. Price,
B. Städler and F. Caruso, Nano Lett., 2011, 11, 4958–4963.
254 P. Blandon, in Cholesterol: Chemistry, Biochemistry and
Pathology, ed. R. P. Cook, Academic Press. Inc., New York,
1958, ch. 2.
Nanoscale, 2013, 5, 89–109 | 109