Concerning the outer sphere relaxation theory, the sensitivity of a T(2) MRI contrast agent, expressed by the transverse relaxivity r(2), depends on the diffusion length of water molecules relative to the particle size. For T(2)-weighted spin-echo imaging, theoretical concepts reveal three regimes regarding the r(2) relaxivity depending on the nanocrystal size: the motional averaging regime (MAR), the static dephasing regime (SDR), and the echo-limiting regime (ELR). The r(2) maximum corresponds to the SDR, which represents a small size regime. To verify the theoretical concepts and to adjust the SDR, tailor-made T(2) contrast agents were synthesized by controlled self-assembly of superparamagnetic iron oxide nanocrystals (SPIOs) into raspberry-like nanoclusters with diameters of 30-200 nm using a PEG-based ligand. The results highlight an opportunity to optimize the relaxivity of T(2) contrast agents by tuning the cluster size of SPIO nanocrystals.
The biofunctionalization of CdSe/CdS/ZnS quantum dots and Fe(3)O(4) nanocrystals using a novel ligand system based on polyisoprene-block-poly(ethylene oxide) ligands is described. The synthesis includes a partial ligand exchange of the hydrophobic nanocrystals with amino-functionalized polyisoprene ligands, followed by seeded micelle formation of the diblock-copolymers in water. The resulting water-soluble quantum dots showed fluorescence quantum efficiencies in the 40 to 50% range and extraordinary fluorescence stability in the biological environment after cross-linking of the polyisoprene moiety of the ligand shell. No toxicity was detected by water-soluble tetrazolium (WST8) and lactate dehydrogenase (LDH) assays, even at very high nanoparticle concentrations, and almost no nonspecific cell adhesion was detected. The ligand shell was further coupled to the antigen-related cell adhesion molecule (CEACAM) specific monoclonal antibody T84.1. The so-conjugated Fe(3)O(4) nanocrystals allowed in vitro and in vivo tumor targeting by magnetic resonance imaging.
It is demonstrated that the melting
behavior and the morphology
of three segmented thermoplastic polyurethane elastomers (TPUs) can
be tailored by applying self-nucleation (SN) procedures. The self-nucleating
temperature ranges for each of the TPU have been first determined
by differential scanning calorimetry (DSC), while their morphology
was studied by polarized light optical microscopy (PLOM), atomic force
microscopy (AFM), and small-angle X-ray scattering (SAXS). When the
samples are cooled at slow to moderate rates after SN, the crystallization
temperature of the TPUs increases by up to 45 °C, when the samples
are ideally self-nucleated. This large reduction in supercooling increases
the melting points of the samples by approximately 20 °C. At
the same time, SAXS and AFM experiments demonstrate the growth of
thicker lamellae under these slow to moderate cooling conditions as
compared to untreated samples. When ideally self-nucleated samples
are rapidly quenched (e.g., at rates of 100 °C min–1 or larger) from their self-nucleation temperature to room temperature,
the effects of SN described above on the morphology and melting points
of the samples disappear for the TPUs that do not crystallize fast
enough.
Nanoparticles (NPs) play an increasingly important role in biological labeling and imaging applications. However, preserving their useful properties in an aqueous biological environment remains challenging, even more as NPs therein have to be long-time stable, biocompatible and nontoxic. For in vivo applications, size control is crucial in order to route excretion pathways, e.g. renal clearance vs. hepato-biliary accumulation. Equally necessary, cellular and tissue specific targeting demands suitable linker chemistry for surface functionalization with affinity molecules, like peptides, proteins, carbohydrates and nucleotides. Herein, we report a three stage encapsulation process for NPs comprised of (1) a partial ligand exchange by a multidentate polyolefinic amine ligand, PI-N3, (2) micellar encapsulation with a precisely tuned amphiphilic diblock PI-b-PEG copolymer, in which the PI chains intercalate to the PI-N3 prepolymer and (3) radical cross-linking of the adjacent alkenyl bonds. As a result, water-soluble NPs were obtained, which virtually maintained their primal physical properties and were exceptionally stable in biological media. PEG-terminal functionalization of the diblock PI-b-PEG copolymer with numerous functional groups was mostly straightforward by chain termination of the living anionic polymerization (LAP) with the respective reagents. More complex affinity ligands, e.g. carbohydrates or biotin, were introduced in a two-step process, prior to micellar encapsulation. Advantageously, this pre-assembly approach opens up rapid access to precisely tuned multifunctional NPs, just by using mixtures of diverse functional PI-b-PEG polymers in a combinatorial manner. All constructs showed no toxicity from 0.001 to 1 μM (particle concentration) in standard WST and LDH assays on A549 cells, as well as only marginal unspecific cellular uptake, even in serum-free medium.
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