Multi-scale cellular engineering: From molecules to organ-on-a-chip.

Recent technological advances in cellular and molecular engineering have provided new insights into biology and enabled the design, manufacturing, and manipulation of complex living systems. Here, we summarize the state of advances at the molecular, cellular, and multi-cellular levels using experimental and computational tools. The areas of focus include intrinsically disordered proteins, synthetic proteins, spatiotemporally dynamic extracellular matrices, organ-on-a-chip approaches, and computational modeling, which all have tremendous potential for advancing fundamental and translational science. Perspectives on the current limitations and future directions are also described, with the goal of stimulating interest to overcome these hurdles using multi-disciplinary approaches

Peptide processing via silk-inspired spinning enables assembly of multifunctional protein alloy fibers

Diverse fiber-forming proteins are found in nature that accomplish a wide range of functions including signaling, cell adhesion, and mechanical support. Unique sequence characteristics of these proteins often lead to their specialized roles. However, these proteins also share a common organizational hierarchy in primary and secondary structures that strongly influence both their intramolecular folding and intermolecular interactions. Based on what is known regarding protein fiber assembly of silk peptides, shear-induced elongation of the molecular strands drives interchain secondary structure crystallization via anisotropic alignment, which creates a molecular superstructure that forms the basis a fiber network. In this work, the hypothesis is this type of protein fiber assembly is not unique to silk sequences and that other proteins can be spun into fibers in similar fashion while maintaining unique functionality given by their specialized amino acid sequences such as RGD, GX1X2, and so forth. This was investigated by modeling the manner in which hydrophobic and hydrophilic blocks of amino acids create interacting secondary structures at the chain level when exposed to shear. It was determined computationally and then verified experimentally that fiber spinning success is most likely to occur after shear processing if the protein sequence exhibits a balance of hydrophobic and hydrophilic content and has sufficient length. Applied to the biological scale, both pure and mixed solutions of proteins such as fibronectin, laminin, and silk fibroin were spun into fibers. In particular, alloy protein fibers of silk fibroin mixed with fibronectin exhibited the characteristic mechanical integrity of silk and the bioactivity of fibronectin. This simple method of creating protein fibers with hybrid characteristics is significantly faster, less expensive, and less technically intensive than chimeric protein production, which purports to do the same. This finding also provides insight into a fundamental means by which protein fibers may be assembled in vivo by taking advantage of the thermodynamically favorable assembly of peptide sequences at the chain level under proper molecular orientation. Taken together, a high throughput means of producing a wide-range of pure and hybrid protein fibers has been developed for various biological applications and research investigations into the fibrous elements of biology

Modeling 3D Cell Shape in Structured Environments with the Cellular Potts Model

In this work, we explore the 3D shape of cells and organoids in structured environments. Understanding the physical determinants of cell shape regulation in structured environments is vital as it plays a crucial role in essential biological processes, including migration, division and tissue development. The cellular Potts model (CPM) has emerged as a powerful computational framework for simulating cell behavior and morphodynamics in complex biological systems. Our research focuses on utilizing the CPM to model 3D single cells on 2D micropatterns and in 3D structured environments. We explicitly consider intracellular structures such as the nucleus and stress fibers and model their impact on cell shape. This allows us to predict morphology and trajectories during the single cell spreading process on micropatterns and demonstrates the effect of nucleus and stress fibers on these processes. Through systematic simulations and comparison with surface minimization approaches and experimental data, we demonstrate the ability of our model to accurately predict cell shapes under different spatial constraints. Additionally, we model the optic cup evagination in fish retina organoids with explicit representation of Matrigel at the surface of the organoid. The findings shed light on the mechanistic basis underlying the shape changes observed in multicellular systems

Micro/nanofluidic and lab-on-a-chip devices for biomedical applications

Micro/Nanofluidic and lab-on-a-chip devices have been increasingly used in biomedical research [1]. Because of their adaptability, feasibility, and cost-efficiency, these devices can revolutionize the future of preclinical technologies. Furthermore, they allow insights into the performance and toxic effects of responsive drug delivery nanocarriers to be obtained, which consequently allow the shortcomings of two/three-dimensional static cultures and animal testing to be overcome and help to reduce drug development costs and time [2–4]. With the constant advancements in biomedical technology, the development of enhanced microfluidic devices has accelerated, and numerous models have been reported. Given the multidisciplinary of this Special Issue (SI), papers on different subjects were published making a total of 14 contributions, 10 original research papers, and 4 review papers. The review paper of Ko et al. [1] provides a comprehensive overview of the significant advancements in engineered organ-on-a-chip research in a general way while in the review presented by Kanabekova and colleagues [2], a thorough analysis of microphysiological platforms used for modeling liver diseases can be found. To get a summary of the numerical models of microfluidic organ-on-a-chip devices developed in recent years, the review presented by Carvalho et al. [5] can be read. On the other hand, Maia et al. [6] report a systematic review of the diagnosis methods developed for COVID-19, providing an overview of the advancements made since the start of the pandemic. In the following, a brief summary of the research papers published in this SI will be presented, with organs-on-a-chip, microfluidic devices for detection, and device optimization having been identified as the main topics.info:eu-repo/semantics/publishedVersio

Roadmap for Optical Tweezers 2023

Optical tweezers are tools made of light that enable contactless pushing, trapping, and manipulation of objects ranging from atoms to space light sails. Since the pioneering work by Arthur Ashkin in the 1970s, optical tweezers have evolved into sophisticated instruments and have been employed in a broad range of applications in life sciences, physics, and engineering. These include accurate force and torque measurement at the femtonewton level, microrheology of complex fluids, single micro- and nanoparticle spectroscopy, single-cell analysis, and statistical-physics experiments. This roadmap provides insights into current investigations involving optical forces and optical tweezers from their theoretical foundations to designs and setups. It also offers perspectives for applications to a wide range of research fields, from biophysics to space exploration

Activity Report 2017-18

The Scientific Activity Report you have in your hands summarizes two years of intense and continued efforts by the dedicated group of scientists conforming the Institute of Nanoscience and Nanotechnology of the University of Barcelona (IN2UB). Created in 2006, the Institute aims to harness the multidisciplinary skills of the UB researchers interested in nanotechnology, with a view of favoring ambitious collaborative research. Thus, it integrates members from up to six Faculties of the University, namely Physics, Chemistry, Farmacy, Medicine, Biology and, most recently, Geology. As a Director, it has been to me a huge responsibility and a tremendous challenge to uphold the high standards set out by my predecessors, Prof. Amilcar Labarta and Prof. Jordi Borrell

A Novel Microbial Source Tracking DNA Microarray Used for Pathogen Detection in Environmental Systems

Pathogen detection and the identification of fecal contamination sources can be challenging in environmental and engineered treatment systems. Factors including pathogen diversity and ubiquity of fecal indicator bacteria hamper risk assessment and remediation of contamination sources. Therefore, a quick method that can detect and identify waterborne pathogens in environmental systems is needed. In this work, a custom microarray targeting pathogens (viruses, bacteria, protozoa), microbial source tracking (MST) markers, mitochondria DNA (mtDNA) and antibiotic resistance genes was used to detect over 430 selected gene targets in whole genome amplification (WGA) DNA and complementary DNA (cDNA) isolated from sewage and animal (avian, cattle, poultry and swine) feces, freshwater and marine water samples, sewage spiked surface water samples, treated wastewater and sewage contaminated produce.;A combination of perfect match and mismatch probes on the microarray reduced the likelihood of false positive detections, thus increasing the specificity of the microarray for various gene targets. A linear decrease in fluorescence of positive probes over a 1:10 dilution series demonstrated a semi-quantitative relationship between gene concentrations in a sample and microarray fluorescence. Various pathogens, including norovirus, Campylobacter fetus, Helicobacter pylori, Salmonella enterica, and Giardia lamblia were detected in sewage via the microarray, as well as MST markers and resistance genes to aminoglycosides, beta-lactams, and tetracycline. Sensitivity (percentage true positives) of MST results in sewage and animal waste samples (21--33%) was lower than specificity (83--90%, percentage of true negatives). Next generation sequencing (NGS) of DNA from the fecal samples revealed two dominant bacterial families that were common to all sample types: Ruminococcaceae and Lachnospiraceae. Five dominant phyla and 15 dominant families comprised 97% and 74%, respectively, of sequences from all fecal sources.;Waterborne pathogens were also detectable via the microarray in freshwater, marine water and sewage spiked surface water samples as well as treated wastewater. Ultrafiltration was used to concentrate microorganisms (bacteria, viruses, protozoa and parasites) from several liters of environmental and treated water samples. Dead-end ultrafiltration (DEUF) was shown to have a 61.4 +/- 47.8 % recovery efficiency and 46-fold concentration increasing ability. Then WGA was utilized to increase gene copies and lower the microarray detection limit. Viruses, including adenovirus, bocavirus, Hepatitis A virus, and polyomavirus were detected in human associated water samples as well as pathogens like Legionella pneumophila, Shigella flexneri, C. fetus and genes coding for resistance to aminoglycosides, beta-lactams, tetracycline. Microbial source tracking results indicate that sewage spiked freshwater and marine samples clustered separately from other fecal sources including wild and domestic animals via non-metric dimensional scaling. A linear relationship between qPCR and microarray fluorescence was found, indicating the semi-quantitative nature of the MST microarray.;Multiple displacement amplification (MDA), which is an important type of WGA, is a widely used tool to amplify genomic nucleic acids. The strong amplification efficiency of MDA and low initial template requirement make MDA an attractive method for environmental molecular and NGS studies. However, like other nucleic acid amplification techniques, various factors may influence MDA efficiency including template concentration (e.g. rare species swamping out), GC amplification bias and genome length favoring amplification of longer genomes. It was found that MDA increased nucleic acids in mixed environmental samples approximately 4.24 +/- 1.40 (log, average +/- standard deviation) for 16S rRNA gene of Enterococcus faecalis, 1.90 +/- 1.70 for RNA polymerase gene of human norovirus, 8.83 +/- 2.88 for T antigen gene of human polyomavirus, 3.83 +/- 0.93 for uidA gene of Escherichia coli, 4.96 +/- 0.32 for invA gene of S. enterica and 8.77 +/- 2.85 for 16S rRNA gene of human Bacteroidales. The template length, concentration and GC content were found to influence MDA efficiency. The results mainly show that the MDA will be more efficient the longer the template length, the greater the initial concentration of nucleic acids and the lower the GC content of the template.;Overall, the results of this work show that 1) the microarray and sample handling technique is suitable for pathogen detection from feces and sewage; 2) when combined with ultrafiltration techniques, the microarray can also be used as a pathogen detection tool in environmental waters; 3) template length, and initial concentration increase MDA efficiency, but higher GC content template negatively effects MDA efficiency. The proposed microarray can be used for pathogen detection in feces, wastewater treatment plant sewage, treated wastewater and environmental waters. Further the proposed method is potentially applicable to pathogen/microorganism detections on vegetables, seafood, in hospital settings, industrial wastewater, and aquaculture settings

Structural insights into phosphoprotein chaperoning of nucleoprotein in measles virus

Instruct Biennial Structural Biology Conference Abstract BookletMeasles virus is an important, highly contagious, human pathogen. The nucleoprotein N binds only to viral genomic RNA and forms the helical ribonucleocapsid that serves as a template for viral replication. We address how N is regulated by another protein, the phosphoprotein, P, to prevent newly synthesized N from binding to cellular RNA. Here, we pulled down an N01-408 fragment lacking most of its C-terminal tail domain by several affinity-tagged, N-terminal, P fragments to map the N0-binding region of P to the first 48 amino acids. We showed biochemically and using P mutants the importance of the hydrophobic interactions for the binding. We fused an N0 binding peptide, P1-48, to the C-terminus of an N021-408 fragment lacking both the N-terminal peptide and the C-terminal tail of N protein to reconstitute and crystallize the N0-P complex. We solved the X-ray structure of the resulting N0-P chimeric protein at 2.7 Å resolution. The structure reveals the molecular details of the conserved N0-P interface and explains how P chaperones N0 preventing both self-assembly of N0 and its binding to RNA. We compare the structure of an N0-P complex to atomic model of helical ribonucleocapsid. We thus propose a model how P may help to start viral RNA synthesis. Our results provide a new insight into mechanisms of paramyxovirus replication. New data on the mechanisms of phosphoprotein chaperone action allows better understanding of the virus genome replication and nucleocapsid assembly. We describe a conserved structural interface for the N-P interaction which could be a target for drug development not only to treat measles but also potentially other paramyxovirus diseases.Non peer reviewe

Aerospace Medicine and Biology - A continuing bibliography with indexes

Annotated bibliography and indexes on Aerospace Medicine and Biology - Dec. 196