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Transcript 
Quantifying extracted lipid membrane composition of Gold
Nanoparticles
Julie
1
Phanord ,
Fangda
2
Xu ,
Bjoern
2
REINHARD
Chemistry Department, Boston University2, Boston MA
RESULTS
ABSTRACT
Gold Nanoparticles(Au NPs) have been the object of profound studies regarding their distinctive physical and
biological properties, as well as their promising applications as drug carriers in the field of bio-medical engineering.
Lipid wrapped Au NPs are emerging up as a novel bio-medical tool in the field of bio-imaging and target-delivery
due to their enhanced bio-compatibility and extended lipid based bio-functions. Interestingly, the lipid membrane
behavior supported by the surface of Au NPs could substantially differ from its precursor, liposomes, in which lipid
membrane can flow in a relatively free fashion . This research aims to characterize and validate such difference
and explore the intrinsic reasons behind such difference, such as lipids content variation before and after wrapping.
In this research, lipid membrane behavior was mostly focused on the phase transition of lipid membrane.
Differential Scanning Calorimetry (DSC) strategy was taken to quantify such potential phase transition of lipid
membrane in the free liposomes and on the surface of Au NPs. In addition to the DSC method, a High
Performance Liquid Chromatography Mass-spec method was developed as well to quantify the potential lipids
content variation before and after lipid membrane wrapping.
MASS- SPEC
DSC
GOLD NANOPARTICLES AND MEMBRANE COMPOSITION
5 mM DOPS ------ 1%
1,2-dioleoyl-sn-glycero-3-phospho-L-serine (sodium
salt)
10 mM DPPC ------- 51%
1,2-dipalmitoyl-sn-glycero-3-phosphocholine
10 mM Cholesterol – 40 %
PC Dye---- 8%
METHODS: HPLC-MS
Samples are forced by a solvent (mobile phase)
through a column containing a stationary phase
in which molecules are fragmented and brought
to the mass detector, leading to the removal of
the solvent followed by the ionization of the
fragments. The ions are carried through a
vacuum and scanned by mass by a detector,
recording a spectrum on a monitor for each
sample.
Fig1. Sample of 10mM DPPC; peaks of different molecular
weight were detected
CONCLUSION
Fig1.
-Molecular weight detected is greater than expected: 780 > 733
(DPPC MW)
-Possible presence of other compounds in samples which might
be the peaks we are seeing in the chromatogram.
Fig2.
-If a phase transition happens at 49°C, then human body
temperature 37°C may not be a potential cause of variations of
lipid content in the AuNPs membrane.
Fig2. Sample of liposomes showing a transition at 49°C, close to
that of DPPC 41°C, the primary constituent of the lipid
membrane.
AKNOWLEDGEMENTS
National Science Foundation and BU Photonics Center
EPOSTERBOARDS TEMPLATE
LC-MS METHOD
CONCLUSIONS
REFERENCES
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