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2. Centromeres are maintained by fastening CENP-A to DNA and directing an arginine anchor-dependent nucleosome transition

Author

Lucie Y. Guo, Praveen Kumar Allu, Levani Zandarashvili, Kara L. McKinley, Nikolina Sekulic, Jennine M. Dawicki-McKenna, Daniele Fachinetti, Glennis A. Logsdon, Ryan M. Jamiolkowski, Don W. Cleveland, Iain M. Cheeseman, and Ben E. Black

Subjects
Science
Abstract

Centromere maintenance depends on the persistence of the histone variant CENP-A at the centromeres. Here, the authors characterize the core centromeric nucleosome complex wherein CENP-C confers a stable CENP-A nucleosome conformation and CENP-N fastens CENP-A to the DNA.

Published
2017
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3. Nanoaperture fabrication via colloidal lithography for single molecule fluorescence analysis.

Author

Ryan M Jamiolkowski, Kevin Y Chen, Shane A Fiorenza, Alyssa M Tate, Shawn H Pfeil, and Yale E Goldman

Subjects
Medicine, Science
Abstract

In single molecule fluorescence studies, background emission from labeled substrates often restricts their concentrations to non-physiological nanomolar values. One approach to address this challenge is the use of zero-mode waveguides (ZMWs), nanoscale holes in a thin metal film that physically and optically confine the observation volume allowing much higher concentrations of fluorescent substrates. Standard fabrication of ZMWs utilizes slow and costly E-beam nano-lithography. Herein, ZMWs are made using a self-assembled mask of polystyrene microspheres, enabling fabrication of thousands of ZMWs in parallel without sophisticated equipment. Polystyrene 1 μm dia. microbeads self-assemble on a glass slide into a hexagonal array, forming a mask for the deposition of metallic posts in the inter-bead interstices. The width of those interstices (and subsequent posts) is adjusted within 100-300 nm by partially fusing the beads at the polystyrene glass transition temperature. The beads are dissolved in toluene, aluminum or gold cladding is deposited around the posts, and those are dissolved, leaving behind an array ZMWs. Parameter optimization and the performance of the ZMWs are presented. By using colloidal self-assembly, typical laboratories can make use of sub-wavelength ZMW technology avoiding the availability and expense of sophisticated clean-room environments and equipment.

Published
2019
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4. Multiplexed genome regulation in vivo with hyper-efficient Cas12a

Author

Lucie Y. Guo, Jing Bian, Alexander E. Davis, Pingting Liu, Hannah R. Kempton, Xiaowei Zhang, Augustine Chemparathy, Baokun Gu, Xueqiu Lin, Draven A. Rane, Xiaoshu Xu, Ryan M. Jamiolkowski, Yang Hu, Sui Wang, and Lei S. Qi

Subjects
Gene Editing, Mice, CRISPR-Associated Proteins, Animals, RNA, Cell Biology, CRISPR-Cas Systems
Abstract

Multiplexed modulation of endogenous genes is crucial for sophisticated gene therapy and cell engineering. CRISPR-Cas12a systems enable versatile multiple-genomic-loci targeting by processing numerous CRISPR RNAs (crRNAs) from a single transcript; however, their low efficiency has hindered in vivo applications. Through structure-guided protein engineering, we developed a hyper-efficient Lachnospiraceae bacterium Cas12a variant, termed hyperCas12a, with its catalytically dead version hyperdCas12a showing significantly enhanced efficacy for gene activation, particularly at low concentrations of crRNA. We demonstrate that hyperdCas12a has comparable off-target effects compared with the wild-type system and exhibits enhanced activity for gene editing and repression. Delivery of the hyperdCas12a activator and a single crRNA array simultaneously activating the endogenous Oct4, Sox2 and Klf4 genes in the retina of post-natal mice alters the differentiation of retinal progenitor cells. The hyperCas12a system offers a versatile in vivo tool for a broad range of gene-modulation and gene-therapy applications.

Published
2022

5. Multiplex CRISPR genome regulation in mouse retina with hyper-efficient Cas12a

Author

Lucie Y. Guo, Jing Bian, Alexander E. Davis, Pingting Liu, Hannah R. Kempton, Xiaowei Zhang, Augustine Chemparathy, Baokun Gu, Xueqiu Lin, Draven A. Rane, Ryan M. Jamiolkowski, Yang Hu, Sui Wang, and Lei S. Qi

Abstract

CRISPR-Cas nucleases and their nuclease-deactivated dCas variants have revolutionized the field of genome editing and gene regulation. Cas12a possesses intrinsic RNAse activity and can process multiple functional crRNAs from a single long transcript, making it a powerful tool for multiplex gene targeting. We engineered a dCas12a variant termed hyperCas12a with superior efficacy in gene editing and multiplex gene regulation, especially at restrictive crRNA concentrations. Here, we describe a step-by-step protocol for constructing and validating a crRNA array, and using it with the hyperdCas12a system for multiplex gene regulation in vivo by subretinal delivery in mice.

Published
2022

8. Hybrid Fluoroscopic and Neurophysiological Targeting of Responsive Neurostimulation of the Rolandic Cortex

Author

Scheherazade Le, Jonathon J. Parker, Ryan M Jamiolkowski, Gerald A. Grant, and Casey H. Halpern

Subjects
Neurophysiology, Subdural Space, Somatosensory system, 03 medical and health sciences, 0302 clinical medicine, Cortex (anatomy), Medicine, Fluoroscopy, Humans, Subdural space, medicine.diagnostic_test, business.industry, Motor Cortex, Neuromodulation (medicine), Electrodes, Implanted, medicine.anatomical_structure, 030220 oncology & carcinogenesis, Surgery, Neurology (clinical), business, 030217 neurology & neurosurgery, Motor cortex, Biomedical engineering, Intraoperative neurophysiological monitoring
Abstract

Background Precise targeting of cortical surface electrodes to epileptogenic regions defined by anatomic and electrophysiological guideposts remains a surgical challenge during implantation of responsive neurostimulation (RNS) devices. Objective To describe a hybrid fluoroscopic and neurophysiological technique for targeting of subdural cortical surface electrodes to anatomic regions with limited direct visualization, such as the interhemispheric fissure. Methods Intraoperative two-dimensional (2D) fluoroscopy was used to colocalize and align an electrode for permanent device implantation with a temporary in Situ electrode placed for extraoperative seizure mapping. Intraoperative phase reversal mapping technique was performed to distinguish primary somatosensory and motor cortex. Results We applied these techniques to optimize placement of an interhemispheric strip electrode connected to a responsive neurostimulator system for detection and treatment of seizures arising from a large perirolandic cortical malformation. Intraoperative neuromonitoring (IONM) phase reversal technique facilitated neuroanatomic mapping and electrode placement. Conclusion In challenging-to-access anatomic regions, fluoroscopy and intraoperative neurophysiology can be employed to augment targeting of neuromodulation electrodes to the site of seizure onset zone or specific neurophysiological biomarkers of clinical interest while minimizing brain retraction.

Published
2020

9. Fabrication of Zero Mode Waveguides for High Concentration Single Molecule Microscopy

Author

Shawn H. Pfeil, Kevin Y Chen, Ryan M. Jamiolkowski, Shane A. Fiorenza, Yale E. Goldman, and Alyssa M. Tate

Subjects
Fluorophore, Materials science, General Chemical Engineering, Finite Element Analysis, Article, General Biochemistry, Genetics and Molecular Biology, law.invention, chemistry.chemical_compound, law, Fluorescence Resonance Energy Transfer, Colloids, Lithography, Fluorescent Dyes, General Immunology and Microbiology, business.industry, General Neuroscience, Colloidal crystal, Single-molecule experiment, Microspheres, Single Molecule Imaging, Nanostructures, Nanolithography, chemistry, Microscopy, Fluorescence, Optoelectronics, Nanosphere lithography, Microtechnology, Polystyrenes, Gold, business, Crystallization, Waveguide, Porosity, Electron-beam lithography, Copper, Aluminum
Abstract

In single molecule fluorescence enzymology, background fluorescence from labeled substrates in solution often limits fluorophore concentration to pico- to nanomolar ranges, several orders of magnitude less than many physiological ligand concentrations. Optical nanostructures called zero mode waveguides (ZMWs), which are 100-200 nm in diameter apertures fabricated in a thin conducting metal such as aluminum or gold, allow imaging of individual molecules at micromolar concentrations of fluorophores by confining visible light excitation to zeptoliter effective volumes. However, the need for expensive and specialized nanofabrication equipment has precluded the widespread use of ZMWs. Typically, nanostructures such as ZMWs are obtained by direct writing using electron beam lithography, which is sequential and slow. Here, colloidal, or nanosphere, lithography is used as an alternative strategy to create nanometer-scale masks for waveguide fabrication. This report describes the approach in detail, with practical considerations for each phase. The method allows thousands of aluminum or gold ZMWs to be made in parallel, with final waveguide diameters and depths of 100-200 nm. Only common lab equipment and a thermal evaporator for metal deposition are required. By making ZMWs more accessible to the biochemical community, this method can facilitate the study of molecular processes at cellular concentrations and rates.

Published
2020

10. New in Vitro Assay Measuring Direct Interaction of Nonsense Suppressors with the Eukaryotic Protein Synthesis Machinery

Author

Barry S. Cooperman, Amy Weil, Allan Jacobson, Haibo Zhang, Martin Y. Ng, Alireza Baradaran-Heravi, Michel Roberge, Ellen Welch, Westley J. Friesen, Ryan M. Jamiolkowski, Yale E. Goldman, and Vijay Singh

Subjects
0301 basic medicine, chemistry.chemical_classification, viruses, media_common.quotation_subject, fungi, Organic Chemistry, Nonsense, Single-molecule FRET, Biochemistry, Ribosome, In vitro, law.invention, Cell biology, Amino acid, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Eukaryotic translation, chemistry, law, 030220 oncology & carcinogenesis, Drug Discovery, Protein biosynthesis, Suppressor, media_common
Abstract

Nonsense suppressors (NonSups) induce "readthrough", i.e., the selection of near cognate tRNAs at premature termination codons and insertion of the corresponding amino acid into nascent polypeptide. Prior readthrough measurements utilized contexts in which NonSups can promote readthrough directly, by binding to one or more of the components of the protein synthesis machinery, or indirectly, by several other mechanisms. Here we utilize a new, highly purified in vitro assay to measure exclusively direct nonsense suppressor-induced readthrough. Of 16 NonSups tested, 12 display direct readthrough, with results suggesting that such NonSups act by at least two different mechanisms. In preliminary work we demonstrate the potential of single molecule fluorescence energy transfer measurements to elucidate mechanisms of NonSup-induced direct readthrough, which will aid efforts to identify NonSups having improved clinical efficacy.

Published
2018

11. The Antiparallel Dimerization of Myosin X Imparts Bundle Selectivity for Processive Motility

Author

Mitsuo Ikebe, Osamu Sato, Yale E. Goldman, Ryan M. Jamiolkowski, Claire E. Fishman, and Matthew A. Caporizzo

Subjects
Models, Molecular, 0301 basic medicine, Biophysics, macromolecular substances, Myosins, Antiparallel (biochemistry), Protein filament, 03 medical and health sciences, Protein structure, Myosin, Molecular motor, Animals, Molecular Machines, Motors, and Nanoscale Biophysics, Protein Structure, Quaternary, Actin, Chemistry, Processivity, Actin Cytoskeleton, Kinetics, 030104 developmental biology, Cattle, Protein Multimerization, Monte Carlo Method, Filopodia, Protein Binding
Abstract

Myosin X is an unconventional actin-based molecular motor involved in filopodial formation, microtubule-actin filament interaction, and cell migration. Myosin X is an important component of filopodia regulation, localizing to tips of growing filopodia by an unclear targeting mechanism. The native α-helical dimerization domain of myosin X is thought to associate with antiparallel polarity of the two amino acid chains, making myosin X the only myosin that is currently considered to form antiparallel dimers. This study aims to determine if antiparallel dimerization of myosin X imparts selectivity toward actin bundles by comparing the motility of parallel and antiparallel dimers of myosin X on single and fascin-bundled actin filaments. Antiparallel myosin X dimers exhibit selective processivity on fascin-bundled actin and are only weakly processive on single actin filaments below saturating [ATP]. Artificial forced parallel dimers of myosin X are robustly processive on both single and bundled actin, exhibiting no selectivity. To determine the relationship between gating of the reaction steps and observed differences in motility, a mathematical model was developed to correlate the parameters of motility with the biochemical and mechanical kinetics of the dimer. Results from the model, constrained by experimental data, suggest that the probability of binding forward, toward the barbed end of the actin filament, is lower in antiparallel myosin X on single actin filaments compared to fascin-actin bundles and compared to constructs of myosin X with parallel dimerization.

Published
2018

12. tRNA Fluctuations Observed on Stalled Ribosomes Are Suppressed during Ongoing Protein Synthesis

Author

Barry S. Cooperman, Ryan M. Jamiolkowski, Yale E. Goldman, and Chunlai Chen

Subjects
Ribosomal Proteins, 0301 basic medicine, Messenger RNA, 030102 biochemistry & molecular biology, GTP', Chemistry, Biophysics, RNA, Peptide Elongation Factor G, Ribosome, 03 medical and health sciences, 030104 developmental biology, Förster resonance energy transfer, RNA, Transfer, Ribosomal protein, Protein Biosynthesis, Transfer RNA, Fluorescence Resonance Energy Transfer, Protein biosynthesis, Nucleic Acids and GenomeBiophysics, Ribosomes
Abstract

The pretranslocation complex of the ribosome can undergo spontaneous fluctuations of messenger RNA and transfer RNAs (tRNAs) between classical and hybrid states, and occupation of the hybrid tRNA positions has been proposed to precede translocation. The classical and hybrid state tRNA positions have been extensively characterized when the ribosome is stalled along the messenger RNA by either the absence or delayed addition of elongation factor G (EF-G), or by the presence of antibiotics or GTP analogs that block translocation. However, during multiple ongoing elongation cycles when both EF-G and ternary complexes are present, EF-G can bind to the pretranslocation complex much faster than the timescale of the classic-hybrid transitions. Using single-molecule fluorescence resonance energy transfer between adjacent tRNAs and between A-site tRNA and ribosomal protein L11, we found that the tRNAs do not fluctuate between the hybrid and classical states, but instead adopt a position with fluorescence resonance energy transfer efficiencies between those of the stalled classical and hybrid states.

Published
2017

13. Deconvolution of Camera Instrument Response Functions

Author

E. Michael Ostap, Yale E. Goldman, Ryan M. Jamiolkowski, John H. Lewis, and Michael S. Woody

Subjects
0301 basic medicine, Physics, Macromolecular Substances, business.industry, Biophysics, Time resolution, Models, Theoretical, Frame rate, Kinetic energy, Temporal database, Kinetics, 03 medical and health sciences, Dwell time, 030104 developmental biology, 0302 clinical medicine, Optics, Fluorescence Resonance Energy Transfer, Molecular Machines, Motors, and Nanoscale Biophysics, Deconvolution, Discrete sampling, business, 030217 neurology & neurosurgery, Probability
Abstract

Temporal sequences of fluorescence intensities in single-molecule experiments are often obtained from stacks of camera images. The dwell times of different macromolecular structural or functional states, correlated with characteristic fluorescence intensities, are extracted from the images and combined into dwell time distributions that are fitted by kinetic functions to extract corresponding rate constants. The frame rate of the camera limits the time resolution of the experiment and thus the fastest rate processes that can be reliably detected and quantified. However, including the influence of discrete sampling (framing) on the detected time series in the fitted model enables rate processes near to the frame rate to be reliably estimated. This influence, similar to the instrument response function in other types of instruments, such as pulsed emission decay fluorometers, is easily incorporated into the fitted model. The same concept applies to any temporal data that is low-pass filtered or decimated to improve signal to noise ratio.

Published
2017

14. Nanoaperture fabrication via colloidal lithography for single molecule fluorescence imaging

Author

Yale E. Goldman, Shane A. Fiorenza, Ryan M. Jamiolkowski, Shawn H. Pfeil, Alyssa M. Tate, and Kevin Y Chen

Subjects
0303 health sciences, Fabrication, Materials science, business.industry, 02 engineering and technology, 021001 nanoscience & nanotechnology, Single-molecule experiment, Cladding (fiber optics), Fluorescence, 03 medical and health sciences, chemistry.chemical_compound, chemistry, Optoelectronics, Polystyrene, 0210 nano-technology, business, Glass transition, Nanoscopic scale, Deposition (law), 030304 developmental biology
Abstract

In single molecule fluorescence studies, background emission from labeled substrates often restricts their concentrations to non-physiological nanomolar values. One approach to address this challenge is the use of zero-mode waveguides (ZMWs), nanoscale holes in a thin metal film that physically and optically confine the observation volume allowing much higher concentrations of fluorescent substrates. Standard fabrication of ZMWs utilizes slow and costly E-beam nano-lithography. Herein, ZMWs are made using a self-assembled mask of polystyrene microspheres, enabling fabrication of thousands of ZMWs in parallel without sophisticated equipment. Polystyrene 1 μm dia. microbeads self-assemble on a glass slide into a hexagonal array, forming a mask for the deposition of metallic posts in the inter-bead interstices. The width of those interstices (and subsequent posts) is adjusted within 100-300 nm by partially fusing the beads at the polystyrene glass transition temperature. The beads are dissolved in toluene, aluminum or gold cladding is deposited around the posts, and those are dissolved, leaving behind an array ZMWs. Parameter optimization and the performance of the ZMWs are presented. By using colloidal self-assembly, typical laboratories can make use of sub-wavelength ZMW technology avoiding the availability and expense of sophisticated clean-room environments and equipment.

Published
2019

15. Nanoaperture fabrication via colloidal lithography for single molecule fluorescence analysis

Author

Alyssa M. Tate, Kevin Y Chen, Shane A. Fiorenza, Ryan M. Jamiolkowski, Shawn H. Pfeil, and Yale E. Goldman

Subjects
Optics and Photonics, Light, Polymers, 02 engineering and technology, Glass Science, Biochemistry, Fluorophotometry, law.invention, chemistry.chemical_compound, Spectrum Analysis Techniques, Fluorescence Microscopy, law, Fluorescence Resonance Energy Transfer, Nanotechnology, Materials, 0303 health sciences, Microscopy, Multidisciplinary, Physics, Electromagnetic Radiation, Light Microscopy, 021001 nanoscience & nanotechnology, Single-molecule experiment, Single Molecule Imaging, Chemistry, Macromolecules, Spectrophotometry, Physical Sciences, Optoelectronics, Engineering and Technology, Medicine, Cellular Structures and Organelles, 0210 nano-technology, Glass transition, Research Article, Chemical Elements, Heat Treatment, Materials science, Fabrication, Science, Materials Science, Research and Analysis Methods, 03 medical and health sciences, Colloids, Nanoscopic scale, Polystyrene, 030304 developmental biology, business.industry, Biology and Life Sciences, Cell Biology, Cladding (fiber optics), Laser, Polymer Chemistry, Nanostructures, Spectrometry, Fluorescence, chemistry, Manufacturing Processes, Nanosphere lithography, Glass, Gold, business, Ribosomes, Aluminum
Abstract

In single molecule fluorescence studies, background emission from labeled substrates often restricts their concentrations to non-physiological nanomolar values. One approach to address this challenge is the use of zero-mode waveguides (ZMWs), nanoscale holes in a thin metal film that physically and optically confine the observation volume allowing much higher concentrations of fluorescent substrates. Standard fabrication of ZMWs utilizes slow and costly E-beam nano-lithography. Herein, ZMWs are made using a self-assembled mask of polystyrene microspheres, enabling fabrication of thousands of ZMWs in parallel without sophisticated equipment. Polystyrene 1 μm dia. microbeads self-assemble on a glass slide into a hexagonal array, forming a mask for the deposition of metallic posts in the inter-bead interstices. The width of those interstices (and subsequent posts) is adjusted within 100-300 nm by partially fusing the beads at the polystyrene glass transition temperature. The beads are dissolved in toluene, aluminum or gold cladding is deposited around the posts, and those are dissolved, leaving behind an array ZMWs. Parameter optimization and the performance of the ZMWs are presented. By using colloidal self-assembly, typical laboratories can make use of sub-wavelength ZMW technology avoiding the availability and expense of sophisticated clean-room environments and equipment.

Published
2019

16. Point-of-Care Rapid-Seeding Ventricular Assist Device with Blood-Derived Endothelial Cells to Create a Living Antithrombotic Coating

Author

Justin E. Grenet, Carmelo A. Milano, Hardean E. Achneck, Ryan M. Jamiolkowski, George A. Truskey, Tim A. Carlon, Qiuyu Lin, Alexandra E. Jantzen, Maria Noviani, and Le Qi

Subjects
Point-of-Care Systems, medicine.medical_treatment, 0206 medical engineering, Cell, Biomedical Engineering, Biophysics, Bioengineering, 02 engineering and technology, 030204 cardiovascular system & hematology, Thrombomodulin, Article, Nitric oxide, Biomaterials, 03 medical and health sciences, chemistry.chemical_compound, Platelet Adhesiveness, 0302 clinical medicine, Antithrombotic, medicine, Humans, Cells, Cultured, Titanium, Heart transplantation, business.industry, technology, industry, and agriculture, Endothelial Cells, Thrombosis, General Medicine, Fetal Blood, equipment and supplies, medicine.disease, 020601 biomedical engineering, Endothelial stem cell, medicine.anatomical_structure, chemistry, Heart-Assist Devices, business, Ex vivo, Biomedical engineering
Abstract

The most promising alternatives to heart transplantation are left ventricular assist devices and artificial hearts; however, their use has been limited by thrombotic complications. To reduce these, sintered titanium (Ti) surfaces were developed, but thrombosis still occurs in approximately 7.5% of patients. We have invented a rapid-seeding technology to minimize the risk of thrombosis by rapid endothelialization of sintered Ti with human cord blood-derived endothelial cells (hCB-ECs). Human cord blood-derived endothelial cells were seeded within minutes onto sintered Ti and exposed to thrombosis-prone low fluid flow shear stresses. The hCB-ECs adhered and formed a confluent endothelial monolayer on sintered Ti. The exposure of sintered Ti to 4.4 dynes/cm2 for 20 hr immediately after rapid seeding resulted in approximately 70% cell adherence. The cell adherence was not significantly increased by additional ex vivo static culture of rapid-seeded sintered Ti before flow exposure. In addition, adherent hCB-ECs remained functional on sintered Ti, as indicated by flow-induced increase in nitric oxide secretion and reduction in platelet adhesion. After 15 day ex vivo static culture, the adherent hCB-ECs remained metabolically active, expressed endothelial cell functional marker thrombomodulin, and reduced platelet adhesion. In conclusion, our results demonstrate the feasibility of rapid-seeding sintered Ti with blood-derived hCB-ECs to generate a living antithrombotic surface.

Published
2016

17. A new in vitro assay measuring direct interaction of nonsense suppressors with the eukaryotic protein synthesis machinery

Author

Barry S. Cooperman, Yale E. Goldman, Vijay Singh, Alireza Baradaran-Heravi, Ellen Welch, Amy Weil, Ryan M. Jamiolkowski, Haibo Zhang, Michel Roberge, Martin Y. Ng, Allan Jacobson, and Westley J. Friesen

Subjects
0303 health sciences, Chemistry, media_common.quotation_subject, viruses, Cell, Nonsense, fungi, MRNA Decay, Single-molecule FRET, In vitro, law.invention, Cell biology, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, law, 030220 oncology & carcinogenesis, medicine, Protein biosynthesis, Suppressor, Premature Termination Codon, 030304 developmental biology, media_common
Abstract

Nonsense suppressors (NonSups) induce “readthrough”, i.e., the selection of near cognate tRNAs at premature termination codons and insertion of the corresponding amino acid into nascent polypeptide. Prior readthrough measurements utilized contexts in which NonSups can promote readthrough directly, by binding to one or more of the components of the protein synthesis machinery, or indirectly, by several other mechanisms. Here we utilize a new, highly-purified in vitro assay to measure exclusively direct nonsense suppressor-induced readthrough. Of 16 NonSups tested, 12 display direct readthrough, with results suggesting that such NonSups act by at least two different mechanisms. In preliminary work we demonstrate the potential of single molecule fluorescence energy transfer measurements to elucidate mechanisms of NonSup-induced direct readthrough, which will aid efforts to identify NonSups having improved clinical efficacy.Table of Contents artwork

Published
2018
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18. Centromeres are maintained by fastening CENP-A to DNA and directing an arginine anchor-dependent nucleosome transition

Author

Don W. Cleveland, Nikolina Sekulic, Praveen Kumar Allu, Kara L. McKinley, Glennis A. Logsdon, Ben E. Black, Ryan M. Jamiolkowski, Iain M. Cheeseman, Jennine M. Dawicki-McKenna, Lucie Y. Guo, Levani Zandarashvili, and Daniele Fachinetti

Subjects
0301 basic medicine, Male, Chromosomal Proteins, Non-Histone, Science, Protein domain, Centromere, General Physics and Astronomy, macromolecular substances, Biology, Protein degradation, Arginine, Article, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Histone H3, Mice, Protein Domains, Centromere Protein A, Genetics, Nucleosome, Animals, Humans, Cancer, Multidisciplinary, General Chemistry, Non-Histone, DNA, Linker DNA, Cell biology, Nucleosomes, Chromosomal Proteins, 030104 developmental biology, Biochemistry, Chromatosome, Female, Generic health relevance, Protein Binding
Abstract

Maintaining centromere identity relies upon the persistence of the epigenetic mark provided by the histone H3 variant, centromere protein A (CENP-A), but the molecular mechanisms that underlie its remarkable stability remain unclear. Here, we define the contributions of each of the three candidate CENP-A nucleosome-binding domains (two on CENP-C and one on CENP-N) to CENP-A stability using gene replacement and rapid protein degradation. Surprisingly, the most conserved domain, the CENP-C motif, is dispensable. Instead, the stability is conferred by the unfolded central domain of CENP-C and the folded N-terminal domain of CENP-N that becomes rigidified 1,000-fold upon crossbridging CENP-A and its adjacent nucleosomal DNA. Disrupting the ‘arginine anchor' on CENP-C for the nucleosomal acidic patch disrupts the CENP-A nucleosome structural transition and removes CENP-A nucleosomes from centromeres. CENP-A nucleosome retention at centromeres requires a core centromeric nucleosome complex where CENP-C clamps down a stable nucleosome conformation and CENP-N fastens CENP-A to the DNA., Centromere maintenance depends on the persistence of the histone variant CENP-A at the centromeres. Here, the authors characterize the core centromeric nucleosome complex wherein CENP-C confers a stable CENP-A nucleosome conformation and CENP-N fastens CENP-A to the DNA.

Published
2017

19. The biocompatibility of titanium cardiovascular devices seeded with autologous blood-derived endothelial progenitor cells

Author

Fu-Hsiung Lin, Liqiao Ma, Jason D. Allen, Amar Parikh, Tao Chen, Jessica K. Huang, Jeffrey H. Lawson, Madison Li, Lauren J. Galinat, Justin M. Haseltine, Bantayehu Sileshi, Whitney O. Lane, Michael J. Serpe, Charles S. Wallace, Hardean E. Achneck, Ryan M. Jamiolkowski, George A. Truskey, Carmelo A. Milano, Alexandra E. Jantzen, and Thomas Stabler

Subjects
Materials science, Biocompatibility, Biophysics, chemistry.chemical_element, Thrombogenicity, Bioengineering, Biomaterials, chemistry, Mechanics of Materials, Platelet adhesiveness, Circulatory system, cardiovascular system, Ceramics and Composites, Platelet activation, Progenitor cell, Fibrinolytic agent, Biomedical engineering, Titanium
Abstract

Implantable and extracorporeal cardiovascular devices are commonly made from titanium (Ti) (e.g. Ti-coated Nitinol stents and mechanical circulatory assist devices). Endothelializing the blood-contacting Ti surfaces of these devices would provide them with an antithrombogenic coating that mimics the native lining of blood vessels and the heart. We evaluated the viability and adherence of peripheral blood-derived porcine endothelial progenitor cells (EPCs), seeded onto thin Ti layers on glass slides under static conditions and after exposure to fluid shear stresses. EPCs attached and grew to confluence on Ti in serum-free medium, without preadsorption of proteins. After attachment to Ti for 15 min, less than 5% of the cells detached at a shear stress of 100 dyne / cm2. Confluent monolayers of EPCs on smooth Ti surfaces (Rq of 10 nm), exposed to 15 or 100 dyne / cm2 for 48 h, aligned and elongated in the direction of flow and produced nitric oxide dependent on the level of shear stress. EPC-coated Ti surfaces had dramatically reduced platelet adhesion when compared to uncoated Ti surfaces. These results indicate that peripheral blood-derived EPCs adhere and function normally on Ti surfaces. Therefore EPCs may be used to seed cardiovascular devices prior to implantation to ameliorate platelet activation and thrombus formation.

Published
2011

20. Anion Binding of Short, Flexible Aryl Triazole Oligomers

Author

Stephen L. Craig, José C Castillo, Ryan M. Jamiolkowski, Emily Zhao, Hemraj Juwarker, Sibi Krishnamurthy, Ki-Hyon Kim, and Jeremy M. Lenhardt

Subjects
Anions, Binding Sites, Macrocyclic Compounds, Magnetic Resonance Spectroscopy, Ionic radius, Polymers, Stereochemistry, Organic Chemistry, Molecular Conformation, Solvation, Nuclear magnetic resonance spectroscopy, Triazoles, Oligomer, Inclusion compound, Solvent, chemistry.chemical_compound, Crystallography, chemistry, Solvents, Solvent effects, Anion binding
Abstract

The flexible, electropositive cavity of linear 1,4-diaryl-1,2,3-triazole oligomers provides a suitable host for complexation of various anions. The binding affinities for various combinations of oligomer and anion were determined by (1)H NMR titrations. Effective ionic radius is found to be a primary determinant of the relative binding interactions of various guests, with small but measurable deviations in the case of nonspherical anions. Solvent effects are significant, and the strength of the binding interaction is found to depend directly on the donor ability of the solvent. A picture emerges in which anion binding can be effectively interpreted in terms of a competition between two solvation spheres: one provided by the solvent and a second dominated by a folded cavity lined with electropositive 1,2,3-triazole CH protons. Implications for rigid macrocycles and other multivalent hosts are discussed.

Published
2009

21. Increased yield of endothelial cells from peripheral blood for cell therapies and tissue engineering

Author

Fu-Hsiung Lin, Oscar Alzate, AnnMarie K Rodriguez, Ryan M. Jamiolkowski, James Frederiksen, George A. Truskey, Sa Do Kang, Siyao Liu, Lukas G. Keil, Alexandra E. Jantzen, Thomas Stabler, Hardean E. Achneck, Marcus D. Darrabie, Jose G. Mantilla, N. Rebecca Haley, Lauren J. Galinat, Justin M. Haseltine, Tim A. Carlon, Jason D. Allen, Maria Noviani, and Antonio J. Arciniegas

Subjects
Embryology, Benzylamines, Cell Transplantation, Cell, Sus scrofa, Biomedical Engineering, Vena Cava, Inferior, Cell Separation, Pharmacology, Cyclams, behavioral disciplines and activities, Transplantation, Autologous, Article, Flow cytometry, Nitric oxide, Cell therapy, chemistry.chemical_compound, Chemokine receptor, Tissue engineering, Heterocyclic Compounds, medicine, Animals, Whole blood, medicine.diagnostic_test, Tissue Engineering, Antagonist, Endothelial Cells, Flow Cytometry, medicine.anatomical_structure, chemistry, Immunology, Models, Animal, Stress, Mechanical, Rheology
Abstract

Aim: Peripheral blood-derived endothelial cells (pBD-ECs) are an attractive tool for cell therapies and tissue engineering, but have been limited by their low isolation yield. We increase pBD-EC yield via administration of the chemokine receptor type 4 antagonist AMD3100, as well as via a diluted whole blood incubation (DWBI). Materials & Methods: Porcine pBD-ECs were isolated using AMD3100 and DWBI and tested for EC markers, acetylated LDL uptake, growth kinetics, metabolic activity, flow-mediated nitric oxide production and seeded onto titanium tubes implanted into vessels of pigs. Results: DWBI increased the yield of porcine pBD-ECs 6.6-fold, and AMD3100 increased the yield 4.5-fold. AMD3100-mobilized ECs were phenotypically indistinguishable from nonmobilized ECs. In porcine implants, the cells expressed endothelial nitric oxide synthase, reduced thrombin-antithrombin complex systemically and prevented thrombosis. Conclusion: Administration of AMD3100 and the DWBI method both increase pBD-EC yield.

Published
2015

22. Islet transplantation in type I diabetes mellitus

Author

Ryan M, Jamiolkowski, Lucie Y, Guo, Yun Rose, Li, Sydney M, Shaffer, and Ali, Naji

Subjects
endocrine system, immunosuppression, endocrine system diseases, diabetes, islet transplantation, Islets of Langerhans Transplantation, surgical procedures, operative, Diabetes Mellitus, Type 1, Animals, Humans, Insulin, Pancreas Transplantation, pancreas, cell therapy, Focus: Translational Medicine
Abstract

For most patients with type I diabetes, insulin therapy and glucose monitoring are sufficient to maintain glycemic control. However, hypoglycemia is a potentially lethal side effect of insulin treatment in patients who are glycemically labile or have hypoglycemia-associated autonomic failure [1]. For those patients, an alternative therapy is beta cell replacement via pancreas or islet transplantation. Pancreas transplants using cadaveric donor organs reduce insulin dependence but carry risks involved in major surgery and chronic immunosuppression. Islet transplantation, in which islets are isolated from donor pancreases and intravenously infused, require no surgery and can utilize islets isolated from pancreases unsuitable for whole organ transplantation. However, islet transplantation also requires immunosuppression, and standard steroid regimens may be toxic to beta cells [2]. The 2000 Edmonton Trial demonstrated the first long-term successful islet transplantation by using a glucocorticoid-free immunosuppressive regimen (sirolimus and tacrolimus). The Clinical Islet Transplantation (CIT) Consortium seeks to improve upon the Edmonton Protocol by using anti-thymocyte globulin (ATG) and TNFα antagonist (etanercept). The trials currently in progress, in addition to research efforts to find new sources of islet cells, reflect enormous potential for islet transplantation in treatment of type I diabetes.

Published
2012

23. Parallel-plate flow chamber and continuous flow circuit to evaluate endothelial progenitor cells under laminar flow shear stress

Author

Lauren J. Galinat, Justin E. Grenet, Fu-Hsiung Lin, Ryan M. Jamiolkowski, Tim A. Carlon, George A. Truskey, Hardean E. Achneck, Melissa M. Ley, Alexandra E. Jantzen, Whitney O. Lane, Justin M. Haseltine, and Jason D. Allen

Subjects
Materials science, General Immunology and Microbiology, Parallel-plate flow chamber, Viscosity, General Chemical Engineering, General Neuroscience, Stem Cells, Shear force, Cytological Techniques, Endothelial Cells, Laminar flow, Bioengineering, Cell morphology, General Biochemistry, Genetics and Molecular Biology, Fractionation, Field Flow, Volumetric flow rate, Shear stress, Shear strength, Animals, Humans, Shear Strength, Biomedical engineering
Abstract

The overall goal of this method is to describe a technique to subject adherent cells to laminar flow conditions and evaluate their response to well quantifiable fluid shear stresses. Our flow chamber design and flow circuit (Fig. 1) contains a transparent viewing region that enables testing of cell adhesion and imaging of cell morphology immediately before flow (Fig. 11A, B), at various time points during flow (Fig. 11C), and after flow (Fig. 11D). These experiments are illustrated with human umbilical cord blood-derived endothelial progenitor cells (EPCs) and porcine EPCs. This method is also applicable to other adherent cell types, e.g. smooth muscle cells (SMCs) or fibroblasts. The chamber and all parts of the circuit are easily sterilized with steam autoclaving. In contrast to other chambers, e.g. microfluidic chambers, large numbers of cells (> 1 million depending on cell size) can be recovered after the flow experiment under sterile conditions for cell culture or other experiments, e.g. DNA or RNA extraction, or immunohistochemistry (Fig. 11E), or scanning electron microscopy. The shear stress can be adjusted by varying the flow rate of the perfusate, the fluid viscosity, or the channel height and width. The latter can reduce fluid volume or cell needs while ensuring that one-dimensional flow is maintained. It is not necessary to measure chamber height between experiments, since the chamber height does not depend on the use of gaskets, which greatly increases the ease of multiple experiments. Furthermore, the circuit design easily enables the collection of perfusate samples for analysis and/or quantification of metabolites secreted by cells under fluid shear stress exposure, e.g. nitric oxide (Fig. 12).

Published
2012

24. Autologous endothelial progenitor cell-seeding technology and biocompatibility testing for cardiovascular devices in large animal model

Author

Lauren J. Galinat, Whitney O. Lane, Alexandra E. Jantzen, Shawn M. Gage, Justin M. Haseltine, Hardean E. Achneck, Fu-Hsiung Lin, Ryan M. Jamiolkowski, and George A. Truskey

Subjects
Issue 55, medicine.medical_specialty, Materials science, Biocompatibility, Swine, Porcine, General Chemical Engineering, Bioengineering, Vascular Surgery, 030204 cardiovascular system & hematology, Inferior vena cava, General Biochemistry, Genetics and Molecular Biology, Cardiovascular Physiological Phenomena, 03 medical and health sciences, 0302 clinical medicine, Blunt dissection, Suture (anatomy), Thromboembolism, Materials Testing, medicine, Stent, Animals, Endothelium, Vicryl, Prolene, 030304 developmental biology, Titanium, 0303 health sciences, General Immunology and Microbiology, General Neuroscience, Stem Cells, Endothelial Cells, Thrombosis, Heparin, Prostheses and Implants, Endothelial Progenitor Cell, Biomaterial, 3. Good health, Surgery, Clamp, medicine.vein, cardiovascular system, Female, medicine.drug, Biomedical engineering, Translational Medicine
Abstract

Implantable cardiovascular devices are manufactured from artificial materials (e.g. titanium (Ti), expanded polytetrafluoroethylene), which pose the risk of thromboemboli formation1,2,3. We have developed a method to line the inside surface of Ti tubes with autologous blood-derived human or porcine endothelial progenitor cells (EPCs)4. By implanting Ti tubes containing a confluent layer of porcine EPCs in the inferior vena cava (IVC) of pigs, we tested the improved biocompatibility of the cell-seeded surface in the prothrombotic environment of a large animal model and compared it to unmodified bare metal surfaces5,6,7 (Figure 1). This method can be used to endothelialize devices within minutes of implantation and test their antithrombotic function in vivo. Peripheral blood was obtained from 50 kg Yorkshire swine and its mononuclear cell fraction cultured to isolate EPCs4,8. Ti tubes (9.4 mm ID) were pre-cut into three 4.5 cm longitudinal sections and reassembled with heat-shrink tubing. A seeding device was built, which allows for slow rotation of the Ti tubes. We performed a laparotomy on the pigs and externalized the intestine and urinary bladder. Sharp and blunt dissection was used to skeletonize the IVC from its bifurcation distal to the right renal artery proximal. The Ti tubes were then filled with fluorescently-labeled autologous EPC suspension and rotated at 10 RPH x 30 min to achieve uniform cell-coating9. After administration of 100 USP/ kg heparin, both ends of the IVC and a lumbar vein were clamped. A 4 cm veinotomy was performed and the device inserted and filled with phosphate-buffered saline. As the veinotomy was closed with a 4-0 Prolene running suture, one clamp was removed to de-air the IVC. At the end of the procedure, the fascia was approximated with 0-PDS (polydioxanone suture), the subcutaneous space closed with 2-0 Vicryl and the skin stapled closed. After 3 - 21 days, pigs were euthanized, the device explanted en-block and fixed. The Ti tubes were disassembled and the inner surfaces imaged with a fluorescent microscope. We found that the bare metal Ti tubes fully occluded whereas the EPC-seeded tubes remained patent. Further, we were able to demonstrate a confluent layer of EPCs on the inside blood-contacting surface. Concluding, our technology can be used to endothelialize Ti tubes within minutes of implantation with autologous EPCs to prevent thrombosis of the device. Our surgical method allows for testing the improved biocompatibility of such modified devices with minimal blood loss and EPC-seeded surface disruption.

Published
2011

25. Use of autologous blood-derived endothelial progenitor cells at point-of-care to protect against implant thrombosis in a large animal model

Author

Ryan M. Jamiolkowski, George A. Truskey, Hardean E. Achneck, Lauren J. Galinat, Jeffrey H. Lawson, Fu-Hsiung Lin, Shawn M. Gage, Justin M. Haseltine, Whitney O. Lane, and Alexandra E. Jantzen

Subjects
Endothelium, Swine, Biophysics, Bioengineering, Inferior vena cava, Article, Biomaterials, Blood vessel prosthesis, medicine, Animals, Humans, Progenitor cell, Titanium, business.industry, Stem Cells, Endothelial Cells, Thrombosis, medicine.disease, Flow Cytometry, Immunohistochemistry, Blood Vessel Prosthesis, Disease Models, Animal, medicine.anatomical_structure, Blood, medicine.vein, Mechanics of Materials, Ceramics and Composites, cardiovascular system, Implant, Stem cell, business, Ex vivo, Biomedical engineering
Abstract

Titanium (Ti) is commonly utilized in many cardiovascular devices, e.g. as a component of Nitinol stents, intra- and extracorporeal mechanical circulatory assist devices, but is associated with the risk of thromboemboli formation. We propose to solve this problem by lining the Ti blood-contacting surfaces with autologous peripheral blood-derived late outgrowth endothelial progenitor cells (EPCs) after having previously demonstrated that these EPCs adhere to and grow on Ti under physiological shear stresses and functionally adapt to their environment under flow conditions ex vivo. Autologous fluorescently-labeled porcine EPCs were seeded at the point-of-care in the operating room onto Ti tubes for 30 minutes and implanted into the pro-thrombotic environment of the inferior vena cava of swine (n = 8). After 3 days, Ti tubes were explanted, disassembled, and the blood-contacting surface was imaged. A blinded analysis found all 4 cell-seeded implants to be free of clot, whereas 4 controls without EPCs were either entirely occluded or partially thrombosed. Pre-labeled EPCs had spread and were present on all 4 cell-seeded implants while no endothelial cells were observed on control implants. These results suggest that late outgrowth autologous EPCs represent a promising source of lining Ti implants to reduce thrombosis in vivo.

Published
2011

26. A comprehensive review of topical hemostatic agents: efficacy and recommendations for use

Author

David M. Albala, Mark L. Shapiro, Jeffrey H. Lawson, Ryan M. Jamiolkowski, Hardean E. Achneck, and Bantayehu Sileshi

Subjects
medicine.medical_specialty, Hemostatic Agent, Biological Products, Physical agents, business.industry, Bandages, Hemostatics, Surgery, Biologic Agents, Topical agents, Expert opinion, Practice Guidelines as Topic, medicine, Cost analysis, Humans, Intensive care medicine, business
Abstract

Since ancient times we have attempted to facilitate hemostasis by application of topical agents. In the last decade, the number of different effective hemostatic agents has increased drastically. In order for the modern surgeon to successfully choose the right agent at the right time, it is essential to understand the mechanism of action, efficacy and possible adverse events as they relate to each agent. In this article we provide a comprehensive review of the most commonly used hemostatic agents, subcategorized as physical agents, absorbable agents, biologic agents, and synthetic agents. We also evaluate novel hemostatic dressings and their application in the current era. Furthermore, wholesale acquisition prices for hospitals in the United States are provided to aid in cost analysis. We conclude with an expert opinion on which agent to use under different scenarios.

Published
2009

27. Regenerating titanium ventricular assist device surfaces after gold/palladium coating for scanning electron microscopy

Author

Jeffrey H. Lawson, Hardean E. Achneck, Stephen L. Craig, Michael J. Serpe, Leslie M. Eibest, and Ryan M. Jamiolkowski

Subjects
Histology, Materials science, Scanning electron microscope, chemistry.chemical_element, Nanotechnology, engineering.material, Microscopy, Atomic Force, Article, Specimen Handling, chemistry.chemical_compound, Coating, X-ray photoelectron spectroscopy, Microscopy, Animals, Humans, Aqua regia, Instrumentation, Staining and Labeling, Photoelectron Spectroscopy, technology, industry, and agriculture, Titanium alloy, Prostheses and Implants, respiratory system, equipment and supplies, Medical Laboratory Technology, chemistry, Microscopy, Electron, Scanning, engineering, Gold, Anatomy, Palladium, Titanium
Abstract

Titanium is one of the most commonly used materials for implantable devices in humans. Scanning electron microscopy (SEM) serves as an important tool for imaging titanium surfaces and analyzing cells and other organic matter adhering to titanium implants. However, high-vacuum SEM imaging of a nonconductive sample requires a conductive coating on the surface. A gold/palladium coating is commonly used and to date no method has been described to "clean" such gold/palladium covered surfaces for repeated experiments without etching the titanium itself. This constitutes a major problem with titanium-based implantable devices which are very expensive and thus in short supply. Our objective was to devise a protocol to regenerate titaniumsurfaces after SEM analysis. In a series of experiments, titanium samples from implantable cardiac assist devices were coated with fibronectin, seeded with cells and then coated with gold/palladium for SEM analysis. X-ray photoelectron spectroscopy spectra were obtained before and after five different cleaning protocols. Treatment with aqua regia (a 1:3 solution of concentrated nitric and hydrochloric acid), with or without ozonolysis, followed by sonication in soap solution and sonication in deionized water, allowed regenerating titanium surfaces to their original state. Atomic force microscopy confirmed that the established protocol did not alter the titanium microstructure. The protocol described herein is applicable to almost all titanium surfaces used in biomedical sciences and because of its short exposure time to aqua regia, will likely work for many titanium alloys as well.

Published
2009

28. The Ribosomal Pre State in Stalled vs. Actively Translating Ribosomes

Author

Yale E. Goldman, Chunlai Chen, Barry S. Cooperman, and Ryan M. Jamiolkowski

Subjects
Crystallography, Stereochemistry, Protein subunit, Transfer RNA, Biophysics, Protein biosynthesis, Translation (biology), Single-molecule FRET, Biology, Ribosomal RNA, Eukaryotic Ribosome, Ribosome
Abstract

During protein synthesis, tRNAs successively occupy three sites on the ribosome: A (aminoacyl), P (peptidyl), and E (exit). A proposed model based on observations of stalled ribosomes describes two distinct states before mRNA and tRNA translocation (PRE-translocation): a classical state in which the tRNAs occupy the same sites in the large and small ribosomal subunits (A/A and P/P), and a hybrid state in which the tRNAs occupy different sites in each subunit (A/P and P/E). To determine whether the exchange and partition between the classical and hybrid PRE states of stalled ribosomes is important for actively translating ribosomes, we conducted single molecule FRET experiments using ribosomes containing Cy5-labeled large subunit protein L11, and Val-tRNAVal(Cy3) or Phe-tRNAPhe(Cy3) in the A-site. We monitored FRET in stalled PRE complexes in the absence of EF-G•GTP, and during ongoing translation in the presence of EF-G•GTP. The mRNA contained a variable number (0, 4, or 8) of Tyr codons preceding Phe and Val codons. In stalled ribosomes, the histogram of L11-tRNA FRET values showed two peaks corresponding to the classical and hybrid states. In contrast, in actively translating ribosomes, the FRET histogram showed only one major peak, with a FRET efficiency that was intermediate between the two values for the stalled complexes. This distribution could correspond to an intermediate structure unique to active turnover, or to a transient state that, in the presence of EF-G, undergoes translocation more rapidly than it converts into the canonical classical and hybrid states. These results suggest that the PRE-translocation ribosomal state during active translation is distinct from the classical and hybrid states observed in stalled ribosomes, consistent with earlier results reported by our group (Rosenblum et al., JACS 2013). Supported by NIH grant GM080376 and AHA fellowship 12POST8910014 to CC.

Published
2014

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