Human neural stem cell growth and differentiation in a gradient-generating microfluidic device

This paper describes a gradient-generating microfluidic platform for optimizing proliferation and differentiation of neural stem cells (NSCs) in culture. Microfluidic technology has great potential to improve stem cell (SC) cultures, whose promise in cell-based therapies is limited by the inability to precisely control their behavior in culture. Compared to traditional culture tools, microfluidic platforms should provide much greater control over cell microenvironment and rapid optimization of media composition using relatively small numbers of cells. Our platform exposes cells to a concentration gradient of growth factors under continuous flow, thus minimizing autocrine and paracrine signaling. Human NSCs (hNSCs) from the developing cerebral cortex were cultured for more than 1 week in the microfluidic device while constantly exposed to a continuous gradient of a growth factor (GF) mixture containing epidermal growth factor (EGF), fibroblast growth factor 2 (FGF2) and platelet-derived growth factor (PDGF). Proliferation and differentiation of NSCs into astrocytes were monitored by time-lapse microscopy and immunocytochemistry. The NSCs remained healthy throughout the entire culture period, and importantly, proliferated and differentiated in a graded and proportional fashion that varied directly with GF concentration. These concentration-dependent cellular responses were quantitatively similar to those measured in control chambers built into the device and in parallel cultures using traditional 6-well plates. This gradient-generating microfluidic platform should be useful for a wide range of basic and applied studies on cultured cells, including SCs.     

Stabilization of an excess electron on molecular surfaces by a pair of HF molecules

This work presents the results of solvation of electrons on several hypothetical cyclooctane and cyclohexane molecular surfaces, using the hydrogen fluoride (HF) dimer. These complexes were constructed with extensive OH groups on one side of a hydrocarbon surface (i.e., cyclohexane sheets), which creates hydrogen‐bonded networks that can form, increasing the dipole moment of the system. Concurrently, the hydrogen atoms on the opposite side of the surface form a pocket of positive charge that can attract excess electrons. Two possible orientations for HF dimer solvation on eight molecular surfaces that have been demonstrated to be stable toward electron detachment are examined. © 2006 Wiley Periodicals, Inc. Int J Quantum Chem, 2007     

Relative retention of the fibroblast growth factors FGF-1 and FGF-2 on strong cation-exchange sorbents

The isocratic retention of two heparin-binding fibroblast growth factors, FGF-1 (acidic FGF) and FGF-2 (basic FGF), was compared on a set of six preparative strong cation-exchange adsorbents. The FGFs comprise a solute pair that are structurally equivalent, yet differ in protein parameters of potential importance in cation-exchange chromatography, such as isoelectric point, net charge, and the number and distribution of basic amino acids. The cation-exchange adsorbents comprise a diverse set of materials in common use for protein purification, with physical and chemical properties that have been characterized and described previously. Isocratic k' values for the two proteins obtained on each adsorbent at several different [NaCl] are compared with one another and with corresponding data for hen egg lysozyme, which is also strongly retained on cation-exchangers. Of the six adsorbents examined, three showed strong retention of both FGFs, with equivalent k' values for FGF-1 and FGF-2. Three others, which showed weaker overall retention for the FGF pair, showed much larger retention differences between FGF-1 and FGF-2. The trends in retention order among the stationary phases are very similar to those seen previously with other unrelated proteins. However, retention differences between the two FGFs, and between the FGFs and lysozyme, do not correlate well with simple charge properties such as net charge, indicating, as in some previous studies, the importance of local regions on the protein surface in determining retention. These observations are interpreted in terms of the structural features of the proteins and the physicochemical properties of the adsorbents.     

Phospholipid coated poly(lactic acid) microspheres for the delivery of LHRH analogues

The aim of this work was to develop alternative peptide‐loaded microspheres using liposphere formulation—a lipid based microdispersion system. This formulation represents a new type of lipid or polymer‐based encapsulation system developed for parenteral and topical drug delivery of bioactive compounds. Our strategy was to utilize the liposphere formulation to improve the entrapment efficiency and release profile of triptorelin and leuprolide [luteinizing hormone–releasing hormone (LHRH) analogues] in vitro. Peptides (2% w/w) were loaded into lipospheres contained of polylactic acid (PLA) or poly(lactic‐co‐glycolic acid) (PLGA) with several types of phospholipids. The effects of polymer and phospholipid type and concentration, method of preparation and solvents on the liposphere characteristics, particle size, surface and bulk structure, drug diffusion rate, and erosion rate of the polymeric matrix were studied. The use of L ‐PLA (M_w = 2000) and hydrogenated soybean phosphatidylcholine (HSPC) with phospholipid–polymer ratio of 1 : 6 w/w, was the most efficient composition that formed lipospheres of particle size in the range of 10 µm with most of the phospholipid embedded on the particles surface. In a typical procedure, peptides were dissolved in N‐methyl‐2‐pyrrolidone (NMP), and dispersed in a solution of polymer and phospholipids in a mixture of NMP and chloroform with the use of 0.1% poly(vinyl alcohol) (PVA) as the emulsified aqueous medium. Uniform microspheres were prepared after solution was mixed at 2000 rpm at room temperature for 30 min. Using this formulation, the entrapment efficiency of LHRH analogues in lipospheres was up to 80%, and the peptides were released for more than 30 days. Copyright © 2002 John Wiley & Sons, Ltd.     

La3Os2O10, a new compound containing isolated clusters Os2O10 with metal-metal bonds

The formula of a new compound isolated in the LaOsO system has been established by means of crystal structure determination. There are two La₃Os₂O₁₀ units in a face-centered monoclinic unit cell (S.G. $\text{C2}\text{m}$); a = 7.911(2) Å, b = 7.963(2) Å, c = 6.966(2)Å, β = 115.76(2)°;. For 1082 intensities, collected on an automated single-crystal diffractometer, the final R value was 0.025 after absorption corrections. The structure consists of isolated Os₂O₁₀ clusters composed of two edge-shared OsO₆ octahedra. These dimeric units are connected together by two types of La³⁺ ions in eightfold coordination. In view of the OsOs distance inside the pair (2.462 Å), La₃Os₂O₁₀ provides an example of metal-metal bonding involving a transition metal in a half-integral formal oxidation state of 5.5.     

A Convenient Synthesis of Chiral Oxazolidin-2-Ones and Thiazolidin-2-Ones and an Improved Preparation of Triphosgene

Oxazolidin-2-ones and thiazolidin-2-one are conveniently prepared by condensation of L-serine, L-threonine and L-cysteine, respectively with triphosgene. The corresponding methyl esters may be subsequently obtained by quenching the reaction mixture with methanol, without prior need for the isolation of the free acids. An improved procedure for preparation of triphosgene using an internal cooling system is described.