Synthesis and Characterization of Lipid Coated Nanoparticles as Drug Delivery Vehicles

Spherical monodisperse nanoparticles composed of gold or silver cores were modified with lipids as part of an ongoing project to utilize functionalized nanoparticles as drug delivery vehicles. A reduction reaction with sodium tri-citrate was used to synthesize nanoparticles that were characterized physically through a NanoSight LM10 HS particle sizer as well as optically with a Shimadzu UV-vis spectrophotometer. The particles were then characterized again after purification of excess ligands through centrifugation. Poly(allylamine hydrochloride) was added to flip the surface charge of the particles from negative to positive as well as to serve as a stabilizing agent. After purification, the particles were coated with lipids and spun to purify them. Characterization data suggest that the particles are successfully coated with both poly(allylamine hydrochloride) and lipids and that monodispersity was maintained, as evidenced by the measured changes in size and optical properties

Site Selective Antibody-Oligonucleotide Conjugation via Microbial Transglutaminase.

Nucleic Acid Therapeutics (NATs), including siRNAs and AntiSense Oligonucleotides (ASOs), have great potential to drug the undruggable genome. Targeting siRNAs and ASOs to specific cell types of interest has driven dramatic improvement in efficacy and reduction in toxicity. Indeed, conjugation of tris-GalNAc to siRNAs and ASOs has shown clinical efficacy in targeting diseases driven by liver hepatocytes. However, targeting non-hepatic diseases with oligonucleotide therapeutics has remained problematic for several reasons, including targeting specific cell types and endosomal escape. Monoclonal antibody (mAb) targeting of siRNAs and ASOs has the potential to deliver these drugs to a variety of specific cell and tissue types. However, most conjugation strategies rely on random chemical conjugation through lysine or cysteine residues resulting in conjugate heterogeneity and a distribution of Drug:Antibody Ratios (DAR). To produce homogeneous DAR-2 conjugates with two siRNAs per mAb, we developed a novel two-step conjugation procedure involving microbial transglutaminase (MTGase) tagging of the antibody C-terminus with an azide-functionalized linker peptide that can be subsequently conjugated to dibenzylcyclooctyne (DBCO) bearing oligonucleotides through azide-alkyne cycloaddition. Antibody-siRNA (and ASO) conjugates (ARCs) produced using this strategy are soluble, chemically defined targeted oligonucleotide therapeutics that have the potential to greatly increase the number of targetable cell types

Application of crossflow ultrafiltration for scaling up the purification of a recombinant ferritin

Ferritin proteins are taking center stage as smart nanocarriers for drug delivery due to their hollow cage-like structures and their unique 24-meric assembly. Among all ferritins, the chimeric Archaeoglobus ferritin (HumFt) is able assemble/disassemble varying the ionic strength of the medium while recognizing human TfR1 receptor overexpressed in cancer cells. In this paper we present a highly efficient, large scale purification protocol mainly based on crossflow ultrafiltration, starting from fermented bacterial paste. This procedure allows one to obtain about 2 g of purified protein starting from 100 g of fermented bacterial paste. The current procedure can easily remove contaminant proteins as well as DNA molecules in the absence of expensive and time consuming chromatographic steps

Label-free enrichment of adrenal cortical progenitor cells using inertial microfluidics.

Passive and label-free isolation of viable target cells based on intrinsic biophysical cellular properties would allow for cost savings in applications where molecular biomarkers are known as well as potentially enable the separation of cells with little-to-no known molecular biomarkers. We have demonstrated the purification of adrenal cortical progenitor cells from digestions of murine adrenal glands utilizing hydrodynamic inertial lift forces that single cells and multicellular clusters differentially experience as they flow through a microchannel. Fluorescence staining, along with gene expression measurements, confirmed that populations of cells collected in different outlets were distinct from one another. Furthermore, primary murine cells processed through the device remained highly viable and could be cultured for 10 days in vitro. The proposed target cell isolation technique can provide a practical means to collect significant quantities of viable intact cells required to translate stem cell biology to regenerative medicine in a simple label-free manner

Structural and biophysical analysis of important biomedical enzymes and nano-architectures

Dopa decarboxylase (DDC) is an important enzyme in the catecholamine biosynthesis pathways. Catecholamines, e.g., dopamine, serotonin, etc. often are the major neuromodulators or neurotransmitters. Hence, DDC plays a key role in regulation of neurodegenerative diseases like Parkinson’s disease (PD). In order to achieve a medicine for PD, a successful inhibitor for DDC, that could reduce the activity of DDC in the blood while making it more effective in brain, is required. An effective design of an inhibitor requires a detailed structural study of human DDC. It was aimed to solve the DDC structure by X-ray crystallography. In order to have enough protein the DDC encoding gene has been cloned in the pET21d vector which was later termed as pET-DDC-His. However, it required numerous trials and errors until a suitable condition for soluble DDC expression was found. Addition of additives like PLP, ethanol, a complex of sorbitol and betaine in the growth medium of the bacteria did not help bring the protein in the soluble part as it formed inclusion bodies. Several soluble protein fusions with DDC, like Thioredoxin and Glutathione-S-transferase were also not quite helpful towards achieving soluble expression of DDC. Finally, a coexpression of DDC along with bacterial chaperone proteins, e.g., GroEL and GroES (after cotransforming both the DDC and Chaperone protein encoding plasmid in the same E.coli cell, used for expression) lead to solubilization of recombinant human DDC. This enzyme was then purified to homogeneity by successively passing the crude bacterial proteins through Ni-chelate-affinity chromatography and Size Exclusion Chromatography. The purified protein (>90 % purity) did not produce a good yield (4mg/ 8L culture), but this was enough to start the initial crystallization trial. Using a scale up to a 50 L culture, quite a good amount of protein was achieved. The homogeneity of DDC was further confirmed by using Multi-Angle Light Scattering and Blue Native PAGE. The dimeric enzyme preparation was then utilized for crystallization using the Hanging Drop Vapor Diffusion method. In a particular condition of the crystal screens trigonal bipyramidal crystals formed. However, these crystals did not show good diffraction when bombarded with X-ray beams. Later, this particular crystallization condition remained irreproducible. The peptide nanoparticle, designed and produced in our lab, could possibly be a very valuable tool in biomedical applications, e.g., in designing vaccines, delivering drugs, bioimaging, serodiagnosis, etc. The design of the peptide nanoparticles is based on the application of the symmetry elements of virus icosahedral capsid on a specially designed building block peptide. The designed peptide building block contains two oligomerization motifs, i.e., a trimeric coiled coil and a pentameric coiled coil joined by a linker region. Sixty such peptide units, upon self-assembly, would produce peptide nanoparticle mimicking a small icosahedral virus particle. The peptide chains in the building block provide flexibility in the design so that an additional peptide could be attached to it at the C-terminus in order to functionalize the peptide nanoparticle for various biomedical applications. First of all, the functional peptide at the C-terminus could be an epitope for the antibody of a life threatening disease like HIV. These peptide nanoparticles can then function as the potent vaccine candidate for that particular disease. In this thesis work, I have attached the two epitopes against the two broadly neutralizing classes of antibody for HIV infection, 2F5 and 4E10, to the peptide nanoparticle. Secondly, another sequence of peptide, which proved to have the capacity of seeding gold on its surface, was attached to the building block peptide unit. The nanoparticle, functionalized with such a peptide, can decorate a gold layer surrounding it. Gold coating on the peptide nanoparticle scaffold can provide a nanostructure, called ‘nanoshells’, which could be very important in the field of therapeutics because of its ability in easy detection and quick treatment of cancer cells. Lastly, I added three peptides; those are recognized in the culture filtrates of M.tuberculosis isolated from TB patients, separately, to the basic peptide construct to form three different nanoparticles. Also, I tried to make a single nanoparticle that displays all the three peptides on its surface. Such a nanoparticle could be a very useful tool in the serodiagnosis or the antibody-based rapid detection of the deadly disease- Tuberculosis. The nanoparticle formation in each of the above-mentioned cases was more or less successful. One of the constructs could successfully even produce gold shells on the peptide nanoparticle

Measuring ligand efficacy at the mu-opioid receptor using a conformational biosensor.

The intrinsic efficacy of orthosteric ligands acting at G-protein-coupled receptors (GPCRs) reflects their ability to stabilize active receptor states (R*) and is a major determinant of their physiological effects. Here, we present a direct way to quantify the efficacy of ligands by measuring the binding of a R*-specific biosensor to purified receptor employing interferometry. As an example, we use the mu-opioid receptor (µ-OR), a prototypic class A GPCR, and its active state sensor, nanobody-39 (Nb39). We demonstrate that ligands vary in their ability to recruit Nb39 to µ-OR and describe methadone, loperamide, and PZM21 as ligands that support unique R* conformation(s) of µ-OR. We further show that positive allosteric modulators of µ-OR promote formation of R* in addition to enhancing promotion by orthosteric agonists. Finally, we demonstrate that the technique can be utilized with heterotrimeric G protein. The method is cell-free, signal transduction-independent and is generally applicable to GPCRs

Site-Directed Mutagenesis and Site-Specific Binding Analysis of Calmodulin (CaM)

Calcium signaling is a major regulatory system in cells and a crucial part of cell biology. An important element in the decoding of intracellular calcium concentration into downstream processes is the ubiquitous and highly conserved calcium binding protein calmodulin (CaM) which can bind to and modulate the function of hundreds of different target proteins, regulating such processes as synaptic plasticity, gene expression and electrical signaling. The biophysical characterization of binding affinity and cooperative interactions between each of calmodulin’s four EF-hand calcium binding sites is essential for understanding calcium signaling. Highly conserved amino acid sequence differences in the ion binding loops of the EF-hands give each site unique affinity for calcium. EF-hands are almost always found in pairs, where binding to one of the sites affects the affinity of the paired site. We have used spectroscopy to measure site-specific binding in each of the paired binding sites in the CaM N-lobe, along with site-directed mutagenesis, to study the contributions of individual amino acids to the ion binding affinity in the mutated site (cis effects) and in the neighboring site (trans effects). Of the twelve amino acids in the binding loops, five are different between Site 1 and Site 2. We constructed proteins with substituted individual residues from Site 1 to Site 2. CaM with the full Site 1 sequence in both Site 1 and Site 2 shows significant changes in affinity and binding characteristics in both sites. To investigate the contributions of the individual amino acid differences, we made intermediate mutants containing individual amino acid changes in Site 2. The cis-effects of the intermediate mutations on the mutated site, Site 2, seem to be independent and additive, whereas the trans-effects on the non-mutated Site 1 showed unexpected dependence on combinations of amino acid changes in Site 2.Neuroscienc

Target identification strategies in plant chemical biology

The current needs to understand gene function in plant biology increasingly require more dynamic and conditional approaches opposed to classic genetic strategies. Gene redundancy and lethality can substantially complicate research, which might be solved by applying a chemical genetics approach. Now understood as the study of small molecules and their effect on biological systems with subsequent target identification, chemical genetics is a fast developing field with a strong history in pharmaceutical research and drug discovery. In plant biology however, chemical genetics is still largely in the starting blocks, with most studies relying on forward genetics and phenotypic analysis for target identification, whereas studies including direct target identification are limited. Here, we provide an overview of recent advances in chemical genetics in plant biology with a focus on target identification. Furthermore, we discuss different strategies for direct target identification and the possibilities and challenges for plant biology

Microwave-assisted synthesis of a MK2 inhibitor by Suzuki-Miyaura coupling for study in Werner syndrome cells

Microwave-assisted Suzuki-Miyaura cross-coupling reactions have been employed towards the synthesis of three different MAPKAPK2 (MK2) inhibitors to study accelerated aging in Werner syndrome (WS) cells, including the cross-coupling of a 2-chloroquinoline with a 3-pyridinylboronic acid, the coupling of an aryl bromide with an indolylboronic acid and the reaction of a 3-amino-4-bromopyrazole with 4-carbamoylphenylboronic acid. In all of these processes, the Suzuki-Miyaura reaction was fast and relatively efficient using a palladium catalyst under microwave irradiation. The process was incorporated into a rapid 3-step microwave-assisted method for the synthesis of a MK2 inhibitor involving 3-aminopyrazole formation, pyrazole C-4 bromination using N-bromosuccinimide (NBS), and Suzuki-Miyaura cross-coupling of the pyrazolyl bromide with 4-carbamoylphenylboronic acid to give the target 4-arylpyrazole in 35% overall yield, suitable for study in WS cells