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Vol. 291, Issue 3, 1017-1022, December 1999
Unité mixte Institut Pasteur de Lille-Université d'Artois, Faculté des sciences Jean-Perrin, Lens, France
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Abstract |
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 Top
 Abstract
 Introduction
Materials and Methods
Results
Discussion
References
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A cell culture model of the blood-brain barrier (BBB) consisting of a coculture of bovine brain capillary endothelial cells and rat astrocytes has been used to examine the ability of 60-nm nanoparticles with different physicochemical characteristics to cross the BBB. Neutral, anionic, and cationic nanoparticles were made from crosslinked malto-dextrins derivatized or not (neutral) with phosphates (anionic), quaternary ammoniums (cationic) ligands. Then, these particles were coated or not with a lipid bilayer made of dipalmitoyl phosphatidyl choline and cholesterol. Lipid coating of ionically charged nanoparticles was able to increase BBB crossing 3- or 4-fold compared with uncoated particles, whereas coating of neutral particles did not significantly alter their permeation characteristics across the endothelial cell monolayer. Lipid-coated nanoparticles were nontoxic toward BBB integrity, and crossed the BBB by transcytosis without any degradation. Furthermore, a 27-fold increase in albumin transport was observed when albumin had previously been loaded in the cationic lipid-coated nanoparticles. The influence of red blood cells was studied; a marked inhibition of the transport was observed, probably due to strong interaction between nanoparticles and red blood cells.
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Introduction |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The
discovery and development in the last decade of neuroactive peptides
and proteins with therapeutic potential for a range of neurological
disorders has generated great interest among neuroscientists. Many
growth factors have been shown to support the growth of motor neurons
in laboratory cultures, and so have become candidates for the treatment
of various neurodegenerative diseases (Mobley, 1989
). However, the
clinical utility of these peptides or protein therapeutic agents in the
treatment of neurological disorders is limited by their inability to
penetrate the blood-brain barrier (BBB) efficiently after systemic administration.
The BBB is formed by the endothelial cells (ECs) that make up brain
capillaries. These brain capillary ECs are sealed together by complex
tight junctions and possess few pinocytic vesicles (Reese and
Karnovski, 1967). These characteristics, added to the existence of a
metabolic barrier, restrict the transport of most small polar molecules
and macromolecules from the cerebrovascular circulation into the brain.
One solution is to administer drugs directly into the brain: for
peptide and protein drugs this can be done by 1) i.c.v. infusion of the
compound into the cerebrospinal fluid (Olson et al., 1992), 2)
transplantation into the brain of cells that produce the therapeutic agent (Kordower et al., 1994), 3) implantation in the brain of a
polymer matrix impregnated with the therapeutic compound (Krewson et
al., 1995), or i.v. delivery of the gene encoding the therapeutic agent
to neuronal cells with viral vectors (Suhr and Gage, 1993). However,
all these procedures suffer from the major disadvantage of being
invasive, and requiring neurosurgery.
If the drug is to be administered noninvasively via the bloodstream,
one pathway to the brain is between the cells, by opening tight
junctions. Paracellular transport of compounds across the BBB can be
increased by means of intracarotid infusion of hyperosmotic saccharide
solution (Rapoport, 1988), or with Cereport (RMP-7, receptor mediated
permeabilizer-7), an analog of bradykinin (Inumura et al.,
1994). A potential drawback to all the methods that involve an increase
in BBB permeability is of poor specificity, causing compounds in the
circulating blood such as albumin for example to gain access to the
brain indiscriminately.
The specific endogenous transport mechanisms through brain capillary EC
offer a potential route for the development of brain-specific drug
delivery systems for neuroactive compounds. Several studies have
already shown that OX-26 monoclonal antibody, a receptor-mediated vector, can be successfully used to deliver therapeutic peptides such
as nerve growth factor (Friden et al., 1993) and vasoactive polypeptide
(Bickel et el., 1993) into the brain through the BBB. Despite their
high specificity and affinity, a major problem with such antibodies has
proved to be their failure to reach the target cells in adequate quantities.
To investigate the fundamental mechanisms of BBB transport biology, we
developed an in vitro model of the BBB that closely mimics in vivo
conditions by culturing brain capillary ECs and astrocytes on opposite
sides of a filter (Dehouck et al., 1990, 1992). This model yielded
evidence that macromolecules such as low-density lipoprotein, diferric
transferrin, and lactoferrin undergo transcytosis through the BBB via a
receptor-mediated pathway (Descamps et al., 1996; Dehouck et al., 1997;
Fillebeen et al., 1999).
Herein, we report on the ability of nanoparticle carriers to activate this transcytotic EC pathway. The effect of the particles' charge (anionic, cationic, neutral), and the influence of a phospholipid coating were evaluated. To closely mimic the in vivo conditions, different incubation media were evaluated (sera with and without red blood cells).
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Materials and Methods |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Chemicals and Antibodies
[U-14C]sucrose (677 mCi/mmol) was
obtained from Amersham Laboratories (Les Ulis, France),
1,2-dipalmitoyl-sn-glycero-3-phosphocholine from NOF Corporation
(Hyogo, Japan), 5-([4,6-dichlorotriazin-2-yl]amino) fluorescein from
Sigma Chemical Co. (Saint Louis, MO), 1-chloro-2,3-epoxypropan (epichlorhydrin) and glycidyltrimethylammonium chloride
(hydroxycholine) from Fluka (Saint-Quentin-Fallavier, France), and
phosphoryl chloride from Prolabo (Paris, France). The rabbit polyclonal
antibody against occludin was from Zymed Laboratories Inc. (South San
Francisco, CA). Primary antibody was detected with Bodipy-conjugated
goat anti-rabbit IgG from Molecular Probes, Inc. (Eugene, OR). Albumin (bovine albumin; ICN Biomedicals, Inc., Costa Mesa, CA) was
radiolabeled with reductive methylation and tritiation of albumin
lysine residues with the borohydride method (Tack et al., 1980). The
labeled albumin was checked by capillary electrophoresis. The labeled
albumin behaved like endogenous albumin. The resulting
3H-labeled proteins were at least 97%
trichloroacetic acid precipitable.
Preparation of Light-Biovectors (L-BV)
Polysaccharide particles were prepared from US Pharmacopoeia
maltodextrin (Glucidex, Roquette, Lille, France) as described previously (Betbeder et al., 1996; Prieur et al., 1996). Briefly, 100 g of maltodextrin was dissolved in 2 N sodium hydroxide with magnetic stirring at room temperature. Addition to the crude mixture of
1-chloro-2,3-epoxypropane (epichlorhydrin, neutral) (4.52 ml), or of a
mixture of epichlorhydrin (4.72 ml) and glycidyltrimethylammonium chloride (hydroxycholine, cationic ligand) (31.18 g), or of phosphoryl chloride (anionic ligand:phosphate) (28.46 ml) yielded neutral, cationic, and anionic polysaccharide gels, respectively. The gels were
then neutralized with acetic acid and sheared under high pressure in a
Minilab homogenizer (Rannie; APV Baker, Evreux, France). The 60-nm
neutral, cationic, and anionic polysaccharide nanoparticles obtained
were ultrafiltered on an SGI Hi-flow system (hollow fiber module: 30 UFIB/1 S.6/40 kD; Setric Génie Industriel, Toulouse,
France) to remove low-molecular weight reagents and salts.
L-BVs were prepared in a Minilab homogenizer by mixing polysaccharide
nanoparticles (Major et al., 1997),
1,2-dipalmitoyl-sn-glycero-3-phosphocholine, and cholesterol at a
temperature above the gel-to-liquid phase transition temperature of the
phospholipid (Woodle and Papahadjopoulos, 1989). Polysaccharide and
phospholipid concentrations were 1.0 and 0.3 mg/ml, respectively.
Phospholipid concentration was determined by the method of Bartlett
(1959) for nonionic and cationic L-BVs. Additionally, a
phospholipid enzymatic colorimetric test PL/MRP2 from Boehringer
Mannheim GmBH (Mannheim, Germany) was used for anionic L-BVs.
Cholesterol was analyzed with an enzymatic assay. The mean diameter of
biovectors was determined by laser light scattering with the N4 MD
Coulter nanoparticle analyzer (Coultronics, Margency, France). With
this technique, the mean diameter obtained was 60 ± 15 nm for all
the particles studied (neutral, anionic, and cationic).
Fluorescence Labeling of L-BVs
Labeling of the polysaccharidic core with fluorescein was
achieved by adding 10 mg of a 5-([4,6-dichlorotriazin-2-yl]amino) fluoresce water solution (2 mg/ml) to 100 mg of polysaccharidic particles at pH 10, with magnetic stirring. These labeled particles were washed and purified by ultrafiltration on an SGI Hi-flow system
(30 UFIB/1S.6/40 kD) with 1 M NaCl, and then with demineralized water
until no fluorescein was detected in the ultrafiltrate. The
fluorescein-labeled polysaccharidic particles (1 mg/ml) were stored in
sterile tubes after filtration through a 0.2-µm filter. This type of
linkage of fluorescein with polysaccharides is classically used for in
vivo studies (Arfors et al., 1973). The stability of the linkage of
fluorescein with the polysaccharide backbone was found to be very high
in solution in the presence of ionic ligands (>1 year at 4°C).
Cell Culture
Bovine Brain Capillary ECs.
ECs were isolated and
characterized as described by Dehouck et al. (1990). The use of cloned
ECs afforded a pure EC population without contamination by pericytes.
The cells were cultured in the presence of Dulbecco's modified
Eagle's medium supplemented with 10% (v/v) heat-inactivated calf
serum and 10% (v/v) horse serum (Gibco Life Technologies, Rockville,
MD), 2 mM glutamine, 50 µg/ml gentamycin, and basic fibroblast growth
factor (1 ng/ml, added every other day).
Rat Astrocytes. Primary cultures of mixed astrocytes were grown from newborn rat cerebral cortex. After removing the meninges, the brain tissue was gently forced through a nylon sieve. Astrocytes were plated on six-well dishes (Nunclon; Nunc A/S, Roskilde, Denmark) at a concentration of 3 × 104 cells/ml in 2 ml of Dulbecco's modified Eagle's medium supplemented with 10% fetal calf serum (Gibco Life Technologies), and the medium was changed twice a week. Three weeks after seeding, the astrocyte cultures were stabilized, and were free of any oligodendrocyte contamination.
Coculture of ECs and Astrocytes.
Filters for coculture were
prepared as follows: culture plate inserts (Millicell PC 3 µm, 30-mm
diameter; Millipore Corp, Bedford, MA) were coated on the upper side
with rat tail collagen prepared by a modification of the method of
Bornstein (1958).
Fluorescence Microscopy
ECs grown on porous filters were fixed and permeabilized with
cold ethanol (
20°C). The samples were washed three times with Tris-buffered saline (20 mM Tris-HCl, 0.5 M NaCl, pH 7) and soaked in
the blocking solution [Tris-buffered saline containing 5% ovalbumin (wt/vol)] for 10 min at room temperature. They were then incubated for
1.5 h in a moist chamber with the rabbit antioccludin pAb in the
blocking solution. After rinsing, the cells were incubated for 1 h
with the secondary antibody, Bodipy-conjugated goat anti-rabbit IgG, in
the blocking solution. Following a final rinse, the filters and their
attached monolayers were mounted on glass microscope slides with Mowiol
mountant (Hoechst, Frankfurt, Germany). The specimens were visualized
and photographed with a Leica fluorescence microscope.
Transendothelial Transport Studies
On the day of the experiment, the inserts containing confluent
EC monolayers and inserts only coated with collagen were washed twice
with buffered Ringer's solution. One insert containing a confluent
monolayer of ECs was transferred to the first well of a six-well plate
filled with 2.5 ml of buffered Ringer's solution in each compartment.
Then, 1.5 ml of buffered Ringer's solution supplemented with 10%
heat-inactivated calf serum (with and without 4-5 million red blood
cells/ml) containing the different fluorescein-labeled L-BVs or
polysaccharide cores (PC) (100 µg/ml), was placed at time zero in the
upper compartment. The incubations were performed for 4 h at
37°C on a rocking platform. Triplicate inserts coated with collagen
seeded and unseeded with ECs were incubated for 12 days with
astrocytes, and used for each compound. At the end of the experiment,
amounts of fluorescein-labeled compounds in the lower compartments were
measured with a Hitachi F-2000 spectrofluorimeter. For the fluorescence
excitation and emission spectra of fluorescein, the wavelengths
ex and em were 495 and 520 nm, respectively. For each test compound, results were
expressed as percentage transport across the brain capillary EC
monolayer alone, obtained from the transport across the inserts coated
with collagen and seeded with ECs, and the transport across the inserts
coated only with collagen. Each point was done in triplicate and the
data are represented as means ± S.E. Sets of data were then
compared with the Mann-Whitney test. At the end of the experiments,
cells incubated with PC and L-BV QAE (cationic) were washed five
times with ice-cold buffered Ringer's solution and fixed in
paraformaldehyde. The filters and their attached monolayers were
mounted on glass microscope slides with Mowiol mountant. The specimens
were visualized and photographed with a Leica fluorescence microscope.
Using the same procedure, the integrity of the brain EC monolayers was
checked by adding [14C]sucrose in the upper
compartment containing the different test compounds. Amounts of
radiotracers in the lower compartment were measured in a liquid
scintillation counter (Wallac 14110; Pharmacia, Piscataway, NJ). The
endothelial permeability coefficient (Pe in cm/min) was calculated as
previously described (Dehouck et al., 1992).
The same experiments were performed with [3H]albumin and biovectors loaded with [3H]albumin. The formulations were made up by simple mixing of [3H]albumin with premade L-BV with stirring. The albumin/liter-BV ratio was 1:10 (w/w). The rate of adsorption was analyzed with a plasmon resonance experiment (BIACORE, Uppsala, Sweden).
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Results |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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EC Characterization.
Fig. 1A
depicts the typical structure of confluent brain capillary ECs
cocultured for 12 days with astrocytes on an insert coated with rat
tail collagen. The cells form a monolayer of nonoverlapping and
contact-inhibited cells. The monolayer was homogeneous; no contamination by pericytes was observed. Immunofluorescent staining of
the tight-junction integral protein occludin showed preferential cortical membrane localization (Fig. 1B). This continuous network of
occludin labeling suggests that the tight junction barrier is well
established. This and numerous previous results concerning the high
electrical resistance (500-800 
· cm2), low
permeability for sucrose and inulin (Dehouck et al., 1990), and
particularly the correlation between drug permeabilities obtained in
vitro with our model and in vivo with the Oldendorf technique (Dehouck
et al., 1992) support this coculture model as a legitimate model of the
BBB.
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Transendothelial Transport Studies.
L-BVs were prepared from
60-nm PCs enveloped in a lipid bilayer (Major et al.,1997). These PCs
were neutral (N), cationic (QAE), or anionic (P), depending on the
meshing agent and on additional groups used for the synthesis.
Transport studies of the different PCs (neutral and ionically charged)
and their corresponding L-BVs across the brain capillary EC monolayer
were performed as described in Materials and Methods. To
study the luminal-to-abluminal transport, fluorescein-labeled PCs or
L-BVs were added to the luminal chamber of the coculture system and the
transfer of these nanoparticles across the cell monolayer was observed
after a 4-h incubation.
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, 1995), and is used as an indicator of the functional integrity of tight junctions. The permeability coefficients of ECs for sucrose coincubated with and without the tested
compounds were not significantly different (Pe sucrose = 0.42 ± 0.03 × 10
3 cm/min alone; Pe
sucrose = 0.58 ± 0.01 × 103
cm/min with PC P; Pe sucrose = 0.45 ± 0.06 × 103 cm/min with L-BV P). The same results were
obtained with the cationic and neutral PC or L-BV (Pe sucrose = 0.51 ± 0.02 × 103 cm/min with PC
QAE; Pe sucrose = 0.48 ± 0.04 × 103 cm/min with L-BV QAE; Pe sucrose = 0.56 ± 0.03 × 103 cm/min with PC N;
Pe sucrose = 0.53 ± 0.04 × 103
cm/min with L-BV N), demonstrating that EC monolayer integrity was
maintained during the transport experiments, and that the concentration
used (100 µg/ml for all compounds) was nontoxic for the ECs.
The results of the above-mentioned experiments indicate that PCs and
L-BVs were transported across the in vitro BBB directly through the
cells. Figure 3 shows the staining
obtained with an immunofluorescent microscope after a 4-h incubation of
the cells with fluorescein-labeled PC QAE and L-BV QAE at 37°C. As
shown in Fig. 3A, fluorescein-labeled PC QAE shows a perinuclear
localization characteristic of its lysosomal accumulation. This
observation agrees with the low transendothelial transport values
obtained for this PC QAE vector. In contrast, fluorescein-labeled L-BV QAE was found as small individual vesicles throughout the cells (Fig.
3B), as previously demonstrated with fluorescent-labeled low-density
lipoproteins (LDL) (Dehouck et al., 1997), suggesting that L-BV QAE is
transported through the ECs without any degradation.
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3 versus 0.43 × 103 cm/min, respectively). However, a 27-fold
increase in albumin transport was observed when albumin had previously
been loaded in the L-BV QAE (0.81 × 103
versus 0.03 × 103 cm/min). The increase
in albumin transport is not due to a breakdown of the BBB because no
toxic effect was detected in sucrose transport during the 4-h
incubation experiments with albumin alone or with albumin loaded on the
L-BV QAE at the concentration used (Pe sucrose = 0.43 ± 0.05 × 103 cm/min alone; Pe sucrose = 0.48 ± 0.05 × 103 cm/min with
albumin; Pe = 0.45 ± 0.06 × 103 cm/min with albumin loaded on L-BV QAE).
These results clearly demonstrate that this increase in albumin
transport was not due to tight junction opening of the BBB.
To mimic the in vivo conditions more closely, the luminal-abluminal
transport experiments were performed in the presence of serum and red
blood cells (4 to 5 million cells/ml) in the luminal compartment of our
coculture model. As shown in Fig. 4,
addition of red blood cells on the EC luminal face induced a huge
decrease in all vector transport with the exception that of PC P and
L-BV N. The transport decreased 2.4- to 8-fold depending on the studied vector.
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Discussion |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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By growing primary ECs on one side of a porous filter and
astrocytes on the other, we can reconstruct the environment that exists
in vivo and so induce most of the BBB characteristics (Dehouck et al.,
1992). Of these characteristics, one is of major importance for
studying drug transport to the brain; in vivo, brain capillary ECs
connected by tight junctions form a continuous lining in the capillary
wall that prevents paracellular flux of solutes. Occludin expression
can be a determinant of tight junction permeability (McCarthy et al.,
1996). Our immunofluorescent studies clearly demonstrate that brain
capillary ECs in these culture conditions express occludin continuously
at cell-to-cell contacts. As described by Hirase et al. (1997), this
continuous staining of occludin at the cell border indicates that these
cells are highly differentiated ECs of cerebral origin. These and
previously published results demonstrating high electrical resistance
(500-800 · cm2) and low permeability
(Dehouck et al., 1990), indicate that we have a highly differentiated
BBB model that is suited to the study of drug transport. Furthermore,
with this in vitro model, we found evidence for an endogenous
transcytotic pathway in ECs for the transport of different
receptor-mediated proteins. Such a pathway seems to be a feature of
capillary ECs of cerebral origin because it has already been described
for three blood-borne molecules: LDL, transferrin, and lactotransferrin
(Descamps et al., 1996; Dehouck et al., 1997; Fillebeen et al., 1999).
All these macromolecules follow an intracellular pathway bypassing the
lysosomal compartment, and thus are not degraded within the cells to be
delivered to the abluminal side of the barrier. This endogenous pathway
is therefore a potential route for molecule delivery to the brain. We
set out to evaluate whether 60-nm L-BV nanoparticles could cross the
BBB. We evaluated the effects of core charge and coating with a lipid
bilayer. We observed that by enveloping a charged PC with a
phospholipid bilayer, it was possible to increase its transport through
the EC monolayer. No modification of the paracellular permeability was
observed during the incubation of cells with L-BV, so this increase was
not due to a breakdown of the barrier. These results are confirmed by
the immunofluorescent study demonstrating that fluorescein-labeled
L-BVs are distributed throughout the cytoplasm. This intracellular
localization is characteristic of transcellular transport, as described
for LDL and transferrin (Descamps et al., 1996; Dehouck et al., 1997).
In contrast, the perinuclear localization of fluorescein PCs shows an
intracellular accumulation of these nanoparticles in a degradation
compartment, as already observed for acetylated LDL. Taken together,
these results demonstrate that the intracellular pathway of PCs differs according to whether the phospholipid bilayer is present, with coated
PCs being transcytosed through the ECs.
We demonstrated previously that this pathway was induced by the binding
of a ligand to its receptor (apoB-LDL receptor;
ferrotransferrin-transferrin receptor). The degradative pathway also
was induced by the binding of the degraded apoB to the scavenger
receptor. In contrast, the results with L-BVs indicated that the lipid
bilayer could activate the transcytotic pathway by a nonspecific
process that does not involve their binding to a receptor. Because
cationic lipid-coated nanoparticles were found to best cross the BBB,
we loaded BSA onto these particles, assuming BSA loading would not
interfere with their membrane properties. Unlike the ECs of peripheral
endothelium, ECs from brain capillaries do not express albumin
receptors in vivo or in vitro (Pardridge et al., 1985). Consequently,
albumin transport through the ECs was extremely low, consistent with
the results of Smith and Borchardt (1989), as indicated by the
calculated Pe (0.03 × 103 cm/min). By
loading albumin on L-BV QAE, we were able to increase its transport
27-fold. Recent studies have demonstrated that caveolae are involved in
the first steps of LDL and transferrin transcytotic pathways (L.F.,
R.C., G. Torpier, unpublished data). Caveolae are small
noncoated plasmalemmal vesicles that are particularly abundantly
expressed in many endothelia. All recent studies suggest these vesicles
are involved in both endocytosis and transcytosis (Ghitescu and
Bendayan, 1992). Moreover, endothelial caveolae have key proteins that
mediate different aspects of vesicle formation, docking, and fusion,
including vesicular soluble NSF attachment receptor, vesicle-associated
membrane protein, and cellubrevin; small and large GTP-binding
proteins; the calcium-dependent lipid-binding proteins annexin II and
VI; and the N-ethylmaleimide-sensitive factor
N-ethylmaleimide-sensitive fusion protein along with
S-nitroso-N-aceytlpenicillamine (Schnitzer
et al., 1995). All these results demonstrate that caveolae are
indeed genuine trafficking organelles capable of budding from the
plasmalemma to form discrete carrier vesicles containing the molecular
machinery necessary for regulated specific transport.
From our previously published results (Dehouck et al., 1997; Fenart et
al., submitted), which agree with those of Schnitzer and Oh (1994),
caveolae can be divided into subpopulations depending on their cellular
destination. Similar results were obtained in this study with PCs and
L-BVs; PCs are delivered to the degradative compartment, whereas L-BVs
are directed to the abluminal side of the cell. Different signaling
molecules have to be activated to induce each of these pathways.
Although kinase and phosphatase have been reported to regulate caveolae
internalization (Smart et al., 1995), nothing is known about the
different intracellular traffic pathway regulation. These two different
vectors could be used to discriminate between the intracellular signals
leading to the transcytotic or degradative pathway.
We studied the influence of red blood cells on the ability of these
nanoparticles to cross the BBB model. We observed a strong inhibition
of the crossing, probably due to nanoparticle-red blood cell
interactions. Red blood cells particles interactions are well described
in the literature. Cationic particles were found to strongly bind to
human erythrocytes (Weiss et al. 1972) Liposomes also were found to
bind to erythrocytes and their lipid content to be incorporated in the
cell membrane (Eytan et al. 1982). These interactions could explain why
the transcytosis of BV nanoparticles is inhibited in the presence of
red blood cells. To decrease the nonspecific binding to red blood
cells, the principle of steric stabilization of colloid particles was
first introduced by Napper and Netchey (1971); it was later found
(Illum and Davies, 1983) that i.v administration of nanoparticles could
be improved by coating them with poloxamer. On the basis of these
results, we expect to improve the ability of BV particles to cross the
BBB in the presence of red blood cells.
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Footnotes |
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Accepted for publication August 17, 1999.
Received for publication June 7, 1999.
1 Current address: Biovector Therapeutics, Chemin du Chêne vert, BP 169, 31676 Labège cedex, France.
2 Current address: Institut National de la Santé et de la Recherche Médicale U325, Département d'Athérosclérose, Institut Pasteur de Lille, 59019 Lille, France.
Send reprint requests to: Roméo Cecchelli, Unité mixte Institut Pasteur-Université d'Artois, Faculté des sciences Jean-Perrin, 62307 Lens, France. E-mail: romeo.cecchelli{at}pasteur-lille.fr
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Abbreviations |
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BBB, blood-brain barrier; EC, endothelial cell; L-BV, light biovector; PC, polysaccharide core; QAE, cationic; N, neutral; P, anionic; LDL, low-density lipoprotein.
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References |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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