Your search keyword '"Thei, F"' showing total 12 results

1. An automatic offset correction platform for high-throughput ion-channel electrophysiology

Author

Thei, F., Rossi, M., Bennati, M., Crescentini, M., and Tartagni, M.

Published

2010

2. Sub-pA Delta-Sigma Current Amplifier for Single-Molecule Nanosensors

Author

Bennati, M, Thei, F, Rossi, M, Crescentini, M, D'Avino, G, Baschirotto, A, Tartagni, M, Tartagni, M., BASCHIROTTO, ANDREA, Bennati, M, Thei, F, Rossi, M, Crescentini, M, D'Avino, G, Baschirotto, A, Tartagni, M, Tartagni, M., and BASCHIROTTO, ANDREA

Published

2009

3. A nanosensor interface based on delta-sigma Arrays

Author

Crescentini, M., primary, Rossi, M., additional, Bennati, M., additional, Thei, F., additional, Baschirotto, A., additional, and Tartagni, M., additional

Published

2009

4. 20.5 A Sub-pA ΔΣ Current Amplifier for Single-Molecule Nanosensors

Author

Bennati, M., primary, Thei, F., additional, Rossi, M., additional, Crescentini, M., additional, D'Avino, G., additional, Baschirotto, A., additional, and Tartagni, M., additional

Published

2009

5. Concurrent Acquisition Approach for High Resolution Sensor Arrays.

Author

Thei, F., Bennati, M., Rossi, M., Crescentini, M., and Tartagni, M.

Published

2010

6. Parallel Recording of Single Ion Channels: A Heterogeneous System Approach

Author

Michele Rossi, Marco Tartagni, Hywel Morgan, Federico Thei, Marco Bennati, Francesco Lodesani, Marco Crescentini, Thei F., Rossi M., Bennati M., Crescentini M., Lodesani F., Morgan H., and Tartagni M.

Subjects

Materials science, business.industry, Amplifier, NANOTECNOLOGIE, Noise (electronics), Computer Science Applications, BIOSENSORI, Printed circuit board, Nanosensor, Electronic engineering, Miniaturization, Microelectronics, Fluidics, Electronics, Electrical and Electronic Engineering, business

Abstract

The convergence of integrated electronic devices with nanotechnology structures on heterogeneous systems presents promising opportunities for the development of new classes of rapid, sensitive, and reliable sensors. The main advantage of em- bedding microelectronic readout structures with sensing elements is twofold. On the one hand, the SNR is increased as a result of scal- ing. On the other, readout miniaturization allows organization of sensors into arrays. The latter point will improve sensing accuracy by using statistical methods. However, accurate interface design is required to establish efficient communication between ionic-based and electronic-based signals. This paper shows a first example of a concurrent readout system with single-ion channel resolution, using a compact and scalable architecture. An array of biological nanosensors is organized on different layers stacked together in a mixed structure: fluidics, printed circuit board, and microelec- tronic readout. More specifically, an array of microholes machined into a polyoxymethylene homopolymer (POMH or Delrin) device coupled with ultralow noise sigma–delta converters current ampli- fiers, is used to form bilayer membranes within which ion channels are embedded. It is shown how formation of multiple artificial bi- layer lipid membranes (BLMs) is automatically monitored by the interface. The system is used to detect current signals in the pA range, from noncovalent binding between single, BLM-embedded α-hemolysin pores and β-cyclodextrin molecules. The current sig- nals are concurrently processed by the readout structure.

Published

2010

7. A nanosensor interface based on delta-sigma Arrays

Author

Michele Rossi, Marco Crescentini, Andrea Baschirotto, Marco Bennati, Federico Thei, Marco Tartagni, M. Crescentini, M. Rossi, M. Bennati, F. Thei, A. Baschirotto, M. Tartagni, Crescentini, M, Rossi, M, Bennati, M, Thei, F, Baschirotto, A, and Tartagni, M

Subjects

Materials science, electronic readout, Interface (computing), Microfluidics, readout electronics, Nanotechnology, NANOSENSORS, biosensor, digital signal processing chip, Delta-sigma modulation, nanobiotechnology, beta-cyclodextrin, Nanosensor, DNA sequencing, nanopore, nanosensor interface, Digital signal processing, Current-feedback operational amplifier, data storage, delta sigma array, business.industry, USB interface, DNA, artificial lipid bilayer, nanowire, ion channel, Computer data storage, nanotube, business, Biosensor, data processing

Abstract

An emerging area of biosensors is based on the use of structures provided by recent advances of Nanotechnology such as nanowires, nanotubes and nanopores. Among them, the integration of natural nanopores such as ion channels with electronics is a promising approach to develop rapid, sensitive and reliable biosensors able to detect low concentration of target molecules or DNA sequencing. This paper presents a compact and low-cost system able to readout, process and record current in the pA range, provided by biological or synthetic nanopores. The approach is based on the idea that by processing the outputs of a large amount of single- molecule nanosensors would result in a significant increase of resolution and signal-to-noise ratio. The approach consists of an electronic interface able to detect current-based array of nanosensors, where the management of very large amount of data is critical for the readout process. As working example, we acquired the single molecule signals derived from non-covalent bindings between single α-hemolysin pores, embedded into an artificial lipid bilayer, and β-cyclodextrin molecules. The system embeds the electronic readout with the microfluidic where is placed the nanosensor array. The electronic interface is a 0.5mm2 current amplifier based on an array of ΣΔ converters. Then the high rate data streams are processed and downsampled by a DSP that communicates with a PC via a USB interface for data processing and storage.

Published

2009

8. In-situ PLL-g-PEG Functionalized Nanopore for Enhancing Protein Characterization.

Author

Salehirozveh M, Kure Larsen AK, Stojmenovic M, Thei F, and Dong M

Subjects

Polyethylene Glycols, Nanotechnology methods, Polylysine, Nanopores

Abstract

Single-molecule nanopore detection technology has revolutionized proteomics research by enabling highly sensitive and label-free detection of individual proteins. Herein, we designed a small, portable, and leak-free flowcell made of PMMA for nanopore experiments. In addition, we developed an in situ functionalizing PLL-g-PEG approach to produce non-sticky nanopores for measuring the volume of diseases-relevant biomarker, such as the Alpha-1 antitrypsin (AAT) protein. The in situ functionalization method allows continuous monitoring, ensuring adequate functionalization, which can be directly used for translocation experiments. The functionalized nanopores exhibit improved characteristics, including an increased nanopore lifetime and enhanced translocation events of the AAT proteins. Furthermore, we demonstrated the reduction in the translocation event's dwell time, along with an increase in current blockade amplitudes and translocation numbers under different voltage stimuli. The study also successfully measures the single AAT protein volume (253 nm 3 ), which closely aligns with the previously reported hydrodynamic volume. The real-time in situ PLL-g-PEG functionalizing method and the developed nanopore flowcell hold great promise for various nanopores applications involving non-sticky single-molecule characterization., (© 2023 The Authors. Chemistry - An Asian Journal published by Wiley-VCH GmbH.)

Published

2023

9. Large-scale production of polyimide micropore-based flow cells for detecting nano-sized particles in fluids.

Author

Salehirozveh M, Porro A, and Thei F

Abstract

In diagnostic and sequencing applications, solid-state nanopores hold significant promise as a single-molecule sensing platform. The fabrication of precisely sized pores has traditionally been challenging, laborious, expensive, and inefficient, which has limited its applications until recently. To overcome this problem, this paper proposes a novel, reliable, cost-effective, portable, mass-productive, robust, and ease-of-use micropore flow cell that works based on the resistive pulse sensor (RPS) technique in order to distinguish the different sizes of c nanoparticles. RPS is a robust and informative technique that can provide valuable details of the size, shape, charge, and individual particle concentrations in the media. By femtosecond laser drilling of a polyimide substrate as an alternate material, translocation of 100, 300, and 350 nm polystyrene nanoparticles in PBS buffer was distinguished by 0.1, 1, and 2 nA current blockade levels, respectively. This is the first time a micropore has been opened in a polyimide membrane using a femtosecond laser in a single step. The experimental and theoretical investigation, scanning electron microscopy and focused ion beam spectroscopy were performed to comprehensively explain the micropore's performance. We showed that our innovative micropore-based flow cell could distinguish nano-sized particles in fluids, and it can be used in large-scale production because of its simplicity and cost-effectiveness., Competing Interests: There are no conflicts of interest to declare., (This journal is © The Royal Society of Chemistry.)

Published

2023

10. Ultrafast Polymer Dynamics through a Nanopore.

Author

Lin CY, Fotis R, Xia Z, Kavetsky K, Chou YC, Niedzwiecki DJ, Biondi M, Thei F, and Drndić M

Subjects

Polymers, Nanotechnology methods, DNA analysis, Nanopores

Abstract

Ultrathin nanopore sensors allow single-molecule and polymer measurements at sub-microsecond time resolution enabled by high current signals (∼10-30 nA). We demonstrate for the first time the experimental probing of the ultrafast translocation and folded dynamics of double-stranded DNA (dsDNA) through a nanopore at 10 MHz bandwidth with acquisition of data points per 25 ns (150 MB/s). By introducing a rigorous algorithm, we are able to accurately identify each current level present within translocation events and elucidate the dynamic folded and unfolded behaviors. The remarkable sensitivity of this system reveals distortions of short-lived folded states at a lower bandwidth. This work revisits probing of dsDNA as a model polymer and develops broadly applicable methods. The combined improvements in sensor signals, instrumentation, and large data analysis methods uncover biomolecular dynamics at unprecedentedly small time scales.

Published

2022

11. Detection of single analyte and environmental samples with silicon nitride nanopores: Antarctic dirt particulates and DNA in artificial seawater.

Author

Niedzwiecki DJ, Chou YC, Xia Z, Thei F, and Drndić M

Subjects

Antarctic Regions, DNA chemistry, Seawater chemistry, DNA analysis, Membranes, Artificial, Nanopores, Seawater analysis, Silicon Compounds chemistry

Abstract

Nanopore sensing is a powerful tool for the detection of biomolecules. Solid-state nanopores act as single-molecule sensors that can function in harsh conditions. Their resilient nature makes them attractive candidates for taking this technology into the field to measure environmental samples for life detection in space and water quality monitoring. Here, we discuss the fabrication of silicon nitride pores from ∼1.6 to 20 nm in diameter in 20-nm-thick silicon nitride membranes suspended on glass chips and their performance. We detect pure laboratory samples containing a single analyte including DNA, BSA, microRNA, TAT, and poly-D-lys-hydrobromide. We also measured an environmental (mixed-analyte) sample, containing Antarctic dirt provided by NASA Ames. For DNA measurements, in addition to using KCl and NaCl solutions, we used the artificial (synthetic) seawater, which is a mixture of different salts mimicking the composition of natural seawater. These samples were spiked with double-stranded DNA (dsDNA) fragments at different concentrations to establish the limits of nanopore sensitivity in candidate environment conditions. Nanopore chips were cleaned and reused for successive measurements. A stand-alone, 1-MHz-bandwidth Chimera amplifier was used to determine the DNA concentration in artificial seawater that we can detect in a practical time scale of a few minutes. We also designed and developed a new compact nanopore reader, a portable read-out device with miniaturized fluidic cells, which can obtain translocation data at bandwidths up to 100 kHz. Using this new instrument, we record translocations of 400 bp, 1000 bp, and 15000 bp dsDNA fragments and show discrimination by analysis of current amplitude and event duration histograms.

Published

2020

12. A Distributed Amplifier System for Bilayer Lipid Membrane (BLM) Arrays With Noise and Individual Offset Cancellation.

Author

Crescentini M, Thei F, Bennati M, Saha S, de Planque MR, Morgan H, and Tartagni M

Subjects

Amplifiers, Electronic, Computer Communication Networks, Electrochemistry methods, Equipment Design, Ion Channels, Lab-On-A-Chip Devices economics, Electrochemistry instrumentation, Lipid Bilayers chemistry, Microfluidic Analytical Techniques instrumentation

Abstract

Lipid bilayer membrane (BLM) arrays are required for high throughput analysis, for example drug screening or advanced DNA sequencing. Complex microfluidic devices are being developed but these are restricted in terms of array size and structure or have integrated electronic sensing with limited noise performance. We present a compact and scalable multichannel electrophysiology platform based on a hybrid approach that combines integrated state-of-the-art microelectronics with low-cost disposable fluidics providing a platform for high-quality parallel single ion channel recording. Specifically, we have developed a new integrated circuit amplifier based on a novel noise cancellation scheme that eliminates flicker noise derived from devices under test and amplifiers. The system is demonstrated through the simultaneous recording of ion channel activity from eight bilayer membranes. The platform is scalable and could be extended to much larger array sizes, limited only by electronic data decimation and communication capabilities.

Published

2015