4 research outputs found
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Cationic HDL mimetics enhance in vivo delivery of self-replicating mRNA
In vivo delivery of large RNA molecules has significant implications for novel gene therapy, biologics delivery, and vaccine applications. We have developed cationic nanolipoprotein particles (NLPs) to enhance the complexation and delivery of large self-amplifying mRNAs (replicons) in vivo. NLPs are high-density lipoprotein (HDL) mimetics, comprised of a discoidal lipid bilayer stabilized by apolipoproteins that are readily functionalized to provide a versatile delivery platform. Herein, we systematically screened NLP assembly with a wide range of lipidic and apolipoprotein constituents, using biophysical metrics to identify lead candidates for in vivo RNA delivery. NLPs formulated with cationic lipids successfully complexed with RNA replicons encoding luciferase, provided measurable protection from RNase degradation, and promoted replicon in vivo expression. The NLP complexation of the replicon and in vivo transfection efficiency were further enhanced by modulating the type and percentage of cationic lipid, the ratio of cationic NLP to replicon, and by incorporating additive molecules
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Producing Membrane Bound Proteins as Countermeasures to Infectious Diseases
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Cell-free production of a functional oligomeric form of a Chlamydia major outer-membrane protein (MOMP) for vaccine development.
Chlamydia is a prevalent sexually transmitted disease that infects more than 100 million people worldwide. Although most individuals infected with Chlamydia trachomatis are initially asymptomatic, symptoms can arise if left undiagnosed. Long-term infection can result in debilitating conditions such as pelvic inflammatory disease, infertility, and blindness. Chlamydia infection, therefore, constitutes a significant public health threat, underscoring the need for a Chlamydia-specific vaccine. Chlamydia strains express a major outer-membrane protein (MOMP) that has been shown to be an effective vaccine antigen. However, approaches to produce a functional recombinant MOMP protein for vaccine development are limited by poor solubility, low yield, and protein misfolding. Here, we used an Escherichia coli-based cell-free system to express a MOMP protein from the mouse-specific species Chlamydia muridarum (MoPn-MOMP or mMOMP). The codon-optimized mMOMP gene was co-translated with Δ49apolipoprotein A1 (Δ49ApoA1), a truncated version of mouse ApoA1 in which the N-terminal 49 amino acids were removed. This co-translation process produced mMOMP supported within a telodendrimer nanolipoprotein particle (mMOMP-tNLP). The cell-free expressed mMOMP-tNLPs contain mMOMP multimers similar to the native MOMP protein. This cell-free process produced on average 1.5 mg of purified, water-soluble mMOMP-tNLP complex in a 1-ml cell-free reaction. The mMOMP-tNLP particle also accommodated the co-localization of CpG oligodeoxynucleotide 1826, a single-stranded synthetic DNA adjuvant, eliciting an enhanced humoral immune response in vaccinated mice. Using our mMOMP-tNLP formulation, we demonstrate a unique approach to solubilizing and administering membrane-bound proteins for future vaccine development. This method can be applied to other previously difficult-to-obtain antigens while maintaining full functionality and immunogenicity
CRISPR-Cas Systems Impact Pseudomonas aeruginosa Genome Structure
<i>Pseudomonas
aeruginosa</i> is both an antibiotic-resistant opportunistic
pathogen and an important model of type I clustered regularly interspaced short
palindromic repeat (CRISPR) and CRISPR-associated protein (CRISPR-Cas) systems.
Comparative genomics has identified several CRISPR-Cas subtypes, and it was
previously unclear how these immune modules might influence the genome content
of <i>P. aeruginosa</i>. To better
understand the distribution of CRISPR-Cas subtypes and their impact on genome
composition, we annotated 672 <i>P.
aeruginosa</i> clinical isolates. We found that CRISPR-Cas systems modulate
genome size and accessory elements. In addition, we identified a novel,
putatively mobile type I-C CRISPR-Cas system. In the process, we also created a
global spacer library that provides a new means of identifying accessory
fragments, and facilitates CRISPR typing of many <i>P. aeruginosa</i> strains. Finally, we have made the assemblies of 282
newly-sequenced <i>P. aeruginosa</i>
isolates public as an NCBI BioProject (ID: PRJNA297679)