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3. Rolling Circle Amplification in Integrated Microsystems: An Uncut Gem toward Massively Multiplexed Pathogen Diagnostics and Genotyping

Author

Ruben R. G. Soares, Mats Nilsson, and Narayanan Madaboosi

Subjects
Genotype, business.industry, Computer science, SARS-CoV-2, Point-of-Care Systems, Loop-mediated isothermal amplification, COVID-19, Context (language use), General Medicine, General Chemistry, Nucleic acid amplification technique, Biosensing Techniques, Automation, Multiplexing, Article, Workflow, Nucleic Acid Amplification Tests, Humans, Biochemical engineering, business, Throughput (business), Nucleic Acid Amplification Techniques
Abstract

Conspectus The development of robust methods allowing the precise detection of specific nucleic acid sequences is of major societal relevance, paving the way for significant advances in biotechnology and biomedical engineering. These range from a better understanding of human disease at a molecular level, allowing the discovery and development of novel biopharmaceuticals and vaccines, to the improvement of biotechnological processes providing improved food quality and safety, efficient green fuels, and smart textiles. Among these applications, the significance of pathogen diagnostics as the main focus of this Account has become particularly clear during the recent SARS-CoV-2 pandemic. In this context, while RT-PCR is the gold standard method for unambiguous detection of genetic material from pathogens, other isothermal amplification alternatives circumventing rapid heating–cooling cycles up to ∼95 °C are appealing to facilitate the translation of the assay into point-of-care (PoC) analytical platforms. Furthermore, the possibility of routinely multiplexing the detection of tens to hundreds of target sequences with single base pair specificity, currently not met by state-of-the-art methods available in clinical laboratories, would be instrumental along the path to tackle emergent viral variants and antimicrobial resistance genes. Here, we advocate that padlock probes (PLPs), first reported by Nilsson et al. in 1994, coupled with rolling circle amplification (RCA), termed here as PLP-RCA, is an underexploited technology in current arena of isothermal nucleic acid amplification tests (NAATs) providing an unprecedented degree of multiplexing, specificity, versatility, and amenability to integration in miniaturized PoC platforms. Furthermore, the intrinsically digital amplification of PLP-RCA retains spatial information and opens new avenues in the exploration of pathogenesis with spatial multiomics analysis of infected cells and tissue. The Account starts by introducing PLP-RCA in a nutshell focusing individually on the three main assay steps, namely, (1) PLP design and ligation mechanism, (2) RCA after probe ligation, and (3) detection of the RCA products. Each subject is touched upon succinctly but with sufficient detail for the reader to appreciate some assay intricacies and degree of versatility depending on the analytical challenge at hand. After familiarizing the reader with the method, we discuss specific examples of research in our group and others using PLP-RCA for viral, bacterial, and fungal diagnostics in a variety of clinical contexts, including the genotyping of antibiotic resistance genes and viral subtyping. Then, we dissect key developments in the miniaturization and integration of PLP-RCA to minimize user input, maximize analysis throughput, and expedite the time to results, ultimately aiming at PoC applications. These developments include molecular enrichment for maximum sensitivity, spatial arrays to maximize analytical throughput, automation of liquid handling to streamline the analytical workflow in miniaturized devices, and seamless integration of signal transduction to translate RCA product titers (and ideally spatial information) into a readable output. Finally, we position PLP-RCA in the current landscape of NAATs and furnish a systematic Strengths, Weaknesses, Opportunities and Threats analysis to shine light upon unpolished edges to uncover the gem with potential for ubiquitous, precise, and unbiased pathogen diagnostics.

Published
2021

4. Flex Printed Circuit Board Implemented Graphene-Based DNA Sensor for Detection of SARS-CoV-2

Author

Inês F. Pinto, Sindre Søpstad, Martin Peacock, Aman Russom, Ruben R. G. Soares, Samar Damiati, and Ahmad Saleem Akhtar

Subjects
Working electrode, Materials science, business.industry, Graphene, 010401 analytical chemistry, 01 natural sciences, 0104 chemical sciences, law.invention, Printed circuit board, law, Electrode, FLEX, Optoelectronics, Nucleic Acid Amplification Tests, Sensitivity (control systems), Electrical and Electronic Engineering, business, Instrumentation, Biosensor
Abstract

Since the COVID-19 outbreak was declared a pandemic by the World Health Organization (WHO) in March 2020, ongoing efforts have been made to develop sensitive diagnostic platforms. Detection of viral RNA provides the highest sensitivity and specificity for detection of early and asymptomatic infections. Thus, this work aimed at developing a label-free genosensor composed of graphene as a working electrode that could be embedded into a flex printed circuit board (FPCB) for the rapid, sensitive, amplification-free and label-free detection of SARS-CoV-2. To facilitate liquid handling and ease of use, the developed biosensor was embedded with a user-friendly reservoir chamber. As a proof-of-concept, detection of a synthetic DNA strand matching the sequence of ORF1ab was performed as a two-step strategy involving the immobilization of a biotinylated complementary sequence on a streptavidin-modified surface, followed by hybridization with the target sequence recorded by the differential pulse voltammetric (DPV) technique in the presence of a ferro/ferricyanide redox couple. The effective design of the sensing platform improved its selectivity and sensitivity and allowed DNA quantification ranging from 100 fg/mL to $1~\mu \text{g}$ /mL. Combining the electrochemical technique with FPCB enabled rapid detection of the target sequence using a small volume of the sample (5- $20~\mu \text{L}$ ). We achieved a limit-of-detection of 100 fg/mL, whereas the predicted value was ~33 fg/mL, equivalent to approximately $5\times 10^{5}$ copies/mL and comparable to sensitivities provided by isothermal nucleic acid amplification tests. We believe that the developed approach proves the ability of an FPCB-implemented DNA sensor to act as a potentially simpler and more affordable diagnostic assay for viral infections in Point-Of-Care (POC) applications.

Published
2021

5. Sample-to-answer COVID-19 nucleic acid testing using a low-cost centrifugal microfluidic platform with bead-based signal enhancement and smartphone read-out

Author

Aman Russom, Ruben R. G. Soares, Xiushan Yin, Ahmad Saleem Akhtar, Noa Lapins, Donal Barrett, Vicent Pelechano, Gustaf Sandh, and Inês F. Pinto

Subjects
Coronavirus disease 2019 (COVID-19), Computer science, Sample (material), Microfluidics, Biomedical Engineering, Loop-mediated isothermal amplification, Bioengineering, Sensitivity and Specificity, 01 natural sciences, Biochemistry, 03 medical and health sciences, COVID-19 Testing, Primer dimer, Humans, 030304 developmental biology, 0303 health sciences, SARS-CoV-2, 010401 analytical chemistry, COVID-19, General Chemistry, Nucleic acid amplification technique, 0104 chemical sciences, 3. Good health, Molecular Diagnostic Techniques, RNA, Viral, Smartphone, Sample collection, Nucleic Acid Amplification Techniques, Viral load, Biomedical engineering
Abstract

With its origin estimated around December 2019 in Wuhan, China, the ongoing SARS-CoV-2 pandemic is a major global health challenge. The demand for scalable, rapid and sensitive viral diagnostics is thus particularly pressing at present to help contain the rapid spread of infection and prevent overwhelming the capacity of health systems. While high-income countries have managed to rapidly expand diagnostic capacities, such is not the case in resource-limited settings of low- to medium-income countries. Aiming at developing cost-effective viral load detection systems for point-of-care COVID-19 diagnostics in resource-limited and resource-rich settings alike, we report the development of an integrated modular centrifugal microfluidic platform to perform loop-mediated isothermal amplification (LAMP) of viral RNA directly from heat-inactivated nasopharyngeal swab samples. The discs were pre-packed with dried n-benzyl-n-methylethanolamine modified agarose beads used to selectively remove primer dimers, inactivate the reaction post-amplification and allowing enhanced fluorescence detection via a smartphone camera. Sample-to-answer analysis within 1 hour from sample collection and a detection limit of approximately 100 RNA copies in 10 μL reaction volume were achieved. The platform was validated with a panel of 162 nasopharyngeal swab samples collected from patients with COVID-19 symptoms, providing a sensitivity of 96.6% (82.2-99.9%, 95% CI) for samples with Ct values below 26 and a specificity of 100% (90-100%, 95% CI), thus being fit-for-purpose to diagnose patients with a high risk of viral transmission. These results show significant promise towards bringing routine point-of-care COVID-19 diagnostics to resource-limited settings.

Published
2021

7. Evidence of Air and Surface Contamination with SARS-CoV-2 in a Major Hospital in Portugal

Author

Priscilla Gomes da Silva, José Gonçalves, Ariana Isabel Brito Lopes, Nury Alves Esteves, Gustavo Emanuel Enes Bamba, Maria São José Nascimento, Pedro T. B. S. Branco, Ruben R. G. Soares, Sofia I. V. Sousa, and João R. Mesquita

Subjects
environmental contamination, Portugal, SARS-CoV-2, Health, Toxicology and Mutagenesis, Public Health, Environmental and Occupational Health, COVID-19, air samples, Hospitals, Article, surface samples, Communicable Disease Control, Humans, RNA, Viral, Medicine, Pandemics
Abstract

As the third wave of the COVID-19 pandemic hit Portugal, it forced the country to reintroduce lockdown measures due to hospitals reaching their full capacities. Under these circumstances, environmental contamination by SARS-CoV-2 in different areas of one of Portugal’s major Hospitals was assessed between 21 January and 11 February 2021. Air samples (n = 44) were collected from eleven different areas of the Hospital (four COVID-19 and seven non-COVID-19 areas) using Coriolis® μ and Coriolis® Compact cyclone air sampling devices. Surface sampling was also performed (n = 17) on four areas (one COVID-19 and three non-COVID-19 areas). RNA extraction followed by a one-step RT-qPCR adapted for quantitative purposes were performed. Of the 44 air samples, two were positive for SARS-CoV-2 RNA (6575 copies/m3 and 6662.5 copies/m3, respectively). Of the 17 surface samples, three were positive for SARS-CoV-2 RNA (200.6 copies/cm2, 179.2 copies/cm2, and 201.7 copies/cm2, respectively). SARS-CoV-2 environmental contamination was found both in air and on surfaces in both COVID-19 and non-COVID-19 areas. Moreover, our results suggest that longer collection sessions are needed to detect point contaminations. This reinforces the need to remain cautious at all times, not only when in close contact with infected individuals. Hand hygiene and other standard transmission-prevention guidelines should be continuously followed to avoid nosocomial COVID-19.

Published
2022

8. A Lab-in-a-Fiber optofluidic device using droplet microfluidics and laser-induced fluorescence for virus detection

Author

Helen E. Parker, Sanghamitra Sengupta, Achar V. Harish, Ruben R. G. Soares, Haakan N. Joensson, Walter Margulis, Aman Russom, and Fredrik Laurell

Subjects
Multidisciplinary, Lab-On-A-Chip Devices, Lasers, Viruses, Fluorescence
Abstract

Microfluidics has emerged rapidly over the past 20 years and has been investigated for a variety of applications from life sciences to environmental monitoring. Although continuous-flow microfluidics is ubiquitous, segmented-flow or droplet microfluidics offers several attractive features. Droplets can be independently manipulated and analyzed with very high throughput. Typically, microfluidics is carried out within planar networks of microchannels, namely, microfluidic chips. We propose that fibers offer an interesting alternative format with key advantages for enhanced optical coupling. Herein, we demonstrate the generation of monodisperse droplets within a uniaxial optofluidic Lab-in-a-Fiber scheme. We combine droplet microfluidics with laser-induced fluorescence (LIF) detection achieved through the development of an optical side-coupling fiber, which we term a periscope fiber. This arrangement provides stable and compact alignment. Laser-induced fluorescence offers high sensitivity and low detection limits with a rapid response time making it an attractive detection method for in situ real-time measurements. We use the well-established fluorophore, fluorescein, to characterize the Lab-in-a-Fiber device and determine the generation of $$\sim$$ ∼ 0.9 nL droplets. We present characterization data of a range of fluorescein concentrations, establishing a limit of detection (LOD) of 10 nM fluorescein. Finally, we show that the device operates within a realistic and relevant fluorescence regime by detecting reverse-transcription loop-mediated isothermal amplification (RT-LAMP) products in the context of COVID-19 diagnostics. The device represents a step towards the development of a point-of-care droplet digital RT-LAMP platform.

Published
2021

9. Digital droplet microfluidic integrated Lab-in-a-fiber detection of SARS-CoV2 viral RNA

Author

Helen E. Parker, Walter Margulis, Achar V. Harish, Fredrik Laurell, Aman Russom, Haakan N. Joensson, Sanghamitra Sengupta, and Ruben R. G. Soares

Subjects
Flexibility (engineering), Software portability, Computer science, law, Microfluidics, Miniaturization, Nanotechnology, Lab-on-a-chip, Multiplexing, Aspect ratio (image), Optofluidics, law.invention
Abstract

Lab-on-a-chip (LOC) is a well-established microfluidic platform that allows the miniaturization of chemical and biological processes onto a single unit. Minimal sample and reagent consumption, the potential for multiplexing, rapid analysis, and portability are some of the key advantages of LOC. However, the chips typically need to be integrated with bulky and expensive external optics. Alternatively, silica fibers and capillaries offer opportunities for more compact integration of optics with microfluidics while adding advantages such as; flexibility within a high aspect ratio format, uniaxial arrangements, and measurement-at-a-distance.

Published
2021

10. Label-Free Detection of Biomolecules in Microfluidic Systems Using On-Chip UV and Impedimetric Sensors

Author

Denis R. Santos, Catarina R.F. Caneira, João Pedro Conde, Virginia Chu, Inês F. Pinto, Rui M. R. Pinto, and Ruben R. G. Soares

Subjects
chemistry.chemical_classification, Detection limit, Analyte, Materials science, Cost effectiveness, Biomolecule, 010401 analytical chemistry, Microfluidics, Molecular biophysics, Nanotechnology, 01 natural sciences, 0104 chemical sciences, Microelectrode, chemistry, Electrical and Electronic Engineering, Instrumentation, Biosensor
Abstract

Label-free approaches to biomolecular detection in microfluidics avoid potential labeling interference, are suitable for the screening of analytes that are not easily tagged, and simplify assay development toward point-of-use applications. In this paper, multimodal label-free detection of biomolecules was performed in a microfluidic system: 1) optically, with an integrated hydrogenated amorphous silicon thin-film photodiode and 2) electrically, using integrated electrochemical impedance interdigitated microelectrodes. Bovine serum albumin, single-stranded DNA, and a mixture of human immunoglobulins G were selected as model biomolecules. The sensitivities of the biomolecular detection were first evaluated in a bare microfluidic channel. The lower limit of detection obtained, for each transducing technique, was 10 nM for the impedimetric detection of ssDNA and 80 nM for the optical detection of a mixture of antibodies. These sensitivities were considered fit-for-purpose when applied to microfluidic systems aimed at monitoring molecular adsorption to different immobilized ligands. To validate the proposed multimodal detection, the model biomolecules were detected in a microfluidic structure packed with ion exchange chromatography agarose microbeads and the target biomolecules were monitored in real time both at bead level and downstream of the packed beads. The application of these label-free sensors ranges from bioprocess optimization to molecular purification and potentially the development of rapid analytics, with the advantages of device compactness, cost effectiveness, high speed of analysis, and multiplexed signal acquisition.

Published
2019

11. Development of a rapid bead-based microfluidic platform for DNA hybridization using single- and multi-mode interactions for probe immobilization

Author

Ana Azevedo, Inês F. Pinto, Ruben R. G. Soares, Virginia Chu, Catarina R.F. Caneira, Hanna S. Mueller-Landau, and João Pedro Conde

Subjects
Detection limit, Chemistry, Nanoporous, DNA–DNA hybridization, Microfluidics, Metals and Alloys, 02 engineering and technology, 010402 general chemistry, 021001 nanoscience & nanotechnology, Condensed Matter Physics, 01 natural sciences, DNA sequencing, 0104 chemical sciences, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, Dissociation constant, Quantum dot, Materials Chemistry, Biophysics, A-DNA, Electrical and Electronic Engineering, 0210 nano-technology, Instrumentation
Abstract

The demand for portable, rapid, sensitive and low-cost DNA detection systems that could be used for rapid diagnostic of disease and infection has greatly motivated the development of new DNA detection platforms in recent years. However, these platforms are often highly complex, requiring an excessively long time of analysis and/or suffer from inadequate sensitivity. Here we report a rapid and simple bead-based microfluidic platform to detect a specific 22-mer DNA sequence via hybridization, serving as a model of a miRNA biomarker for tumor and cardiovascular diseases. Commercial nanoporous chromatography beads were used as solid support for probe DNA immobilization, using either a single-mode electrostatic interaction or multi-mode interactions (electrostatic and hydrophobic). Using a mass balance approach, a probe density of 2.4 × 10 13 ± 18 % ( ± RSD%) molecules/cm2 was quantified in optimized conditions, which was found to provide hybridization efficiencies above 95 % and a hybridization dissociation constant below 1 nM. Comparing targets with different optical labels, namely Atto 430LS, quantum dots and horseradish peroxidase, the lowest limit of detection of 9.5 ± 1.1 pM was achieved with an assay time of 10 min using a quantum dot label coupled with a multi-mode immobilization. These results highlight the potential of the system to be applied as a simple and highly sensitive DNA hybridization platform, achieving low pM sensitivities without the need of a DNA amplification procedure.

Published
2019

12. Viral detection and quantification in a digital droplet microfluidic lab-in-a-fiber device

Author

Helen E. Parker, Sanghamitra Sengupta, Aman Russom, Achar V. Harish, Haakan N. Joensson, Walter Margulis, Ruben R. G. Soares, and Fredrik Laurell

Subjects
Detection limit, Fabrication, Materials science, business.industry, Microfluidics, Loop-mediated isothermal amplification, Optoelectronics, Fiber, business, Fluorescence, Sensitivity (electronics), Optofluidics
Abstract

In this work, we present the design and fabrication of a fiber device that performs digital droplet microfluidics for molecular diagnostics. A variety of fibers and capillaries were used to build three connected modules dedicated to droplet generation, incubation, and fluorescence detection which enables a uniaxial arrangement. This is in contrast to the traditional 2-dimensional lab-on-a-chip architecture. We characterize our fiber device using a fluorescein dilution series. Our observed detection limit is on the order of 10 nM fluorescein. We demonstrate our all-fiber device for the fluorescence readout after loop-mediated isothermal amplification (LAMP) of synthetic SARS-CoV-2. Our results suggest that this fiber device can successfully distinguish between positive and negative samples in molecular diagnostics. We propose that our fiber device offers benefits over microfluidic chip techniques such as easier optical integration, much simpler sample loading, and faster diagnosis with high specificity and sensitivity.

Published
2021

13. Airborne spread of infectious SARS-CoV-2: Moving forward using lessons from SARS-CoV and MERS-CoV

Author

João R. Mesquita, Priscilla Gomes da Silva, Ruben R. G. Soares, Sofia I. V. Sousa, Maria São José Nascimento, and Instituto de Saúde Pública da Universidade do Porto

Subjects
2019-20 coronavirus outbreak, Environmental Engineering, 010504 meteorology & atmospheric sciences, Web of science, Coronavirus disease 2019 (COVID-19), viruses, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), India, Review, 010501 environmental sciences, Biology, 01 natural sciences, law.invention, Genetic similarity, law, Environmental health, Humans, Environmental Chemistry, Waste Management and Disposal, 0105 earth and related environmental sciences, Emerging diseases, SARS-CoV-2, fungi, Infectious, virus diseases, COVID-19, biochemical phenomena, metabolism, and nutrition, Pollution, respiratory tract diseases, Transmission (mechanics), Systematic review, Viability, Airborne, Middle East Respiratory Syndrome Coronavirus, RNA, Viral, Brazil
Abstract

Background Although an increasing body of data reports the detection of SARS-CoV-2 RNA in air, this does not correlate to the presence of infectious viruses, thus not evaluating the risk for airborne COVID-19. Hence there is a marked knowledge gap that requires urgent attention. Therefore, in this systematic review, viability/stability of airborne SARS-CoV-2, SARS-CoV and MERS-CoV viruses is discussed. Methods A systematic literature review was performed on PubMed/MEDLINE, Web of Science and Scopus to assess the stability and viability of SARS-CoV, MERS-CoV and SARS-CoV-2 on air samples. Results and discussion The initial search identified 27 articles. Following screening of titles and abstracts and removing duplicates, 11 articles were considered relevant. Temperatures ranging from 20 °C to 25 °C and relative humidity ranging from 40% to 50% were reported to have a protective effect on viral viability for airborne SARS-CoV and MERS-CoV. As no data is yet available on the conditions influencing viability for airborne SARS-CoV-2, and given the genetic similarity to SARS-CoV and MERS-CoV, one could extrapolate that the same conditions would apply. Nonetheless, the effect of these conditions seems to be residual considering the increasing number of cases in the south of USA, Brazil and India, where high temperatures and humidities have been observed. Conclusion Higher temperatures and high relative humidity can have a modest effect on SARS-CoV-2 viability in the environment, as reported in previous studies to this date. However, these studies are experimental, and do not support the fact that the virus has efficiently spread in the tropical regions of the globe, with other transmission routes such as the contact and droplet ones probably being responsible for the majority of cases reported in these regions, along with other factors such as human mobility patterns and contact rates. Further studies are needed to investigate the extent of aerosol transmission of SARS-CoV-2 as this would have important implications for public health and infection-control policies., Graphical abstract Unlabelled Image, Highlights • Detection of SARS-CoV-2 RNA in the air do not correlate to infectivity. • Virus viability in air is important to understand the aerosol transmission. • SARS-CoV-2 may be less stable in higher temperatures and relative humidity. • The effect of temperature and humidity on SARS-CoV-2 seems to be residual.

Published
2021
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14. Rolling Circle Amplification in Bead-Based Microfluidic Device with Integrated Photodiode for Fluorescence Signal Transduction

Author

Catarina R.F. Caneira, João Pedro Conde, Katerina Nikolaidou, Virginia Chu, Mats Nilsson, Narayanan Madaboosi, and Ruben R. G. Soares

Subjects
Interference filter, Materials science, business.industry, 010401 analytical chemistry, Microfluidics, Loop-mediated isothermal amplification, 02 engineering and technology, 021001 nanoscience & nanotechnology, 01 natural sciences, Signal, 0104 chemical sciences, Photodiode, law.invention, law, Rolling circle replication, Optoelectronics, System on a chip, 0210 nano-technology, business, Sensitivity (electronics)
Abstract

The detection of pathogens in primary care settings is critical, not only for virus detection but also for the detection of antibiotic resistant bacteria. Microfluidic devices can be used to develop point-of-care detection systems, but are usually insufficiently sensitive for the application. An on-chip isothermal amplification technique, such as the padlock probing-based rolling circle amplification technique, could potentially achieve the desired specificity and sensitivity, while keeping the complexity of the microfluidic device low. In this work, we describe an innovative microfluidic rolling circle amplification performed on microbeads using a continuous flow of solutions with the potential to achieve the required clinical demands in fast and sensitive fashion. Moreover, the integration with amorphous-hydrogenated silicon thin film p-i-n photodiode and a high-pass interference filter to allow the acquisition of the fluorescence signal from the amplification product on-chip, demonstrates the capability of performing the full assay on-chip along with the portability potential of the device.

Published
2021

15. Knowing more from less: miniaturization of ligand-binding assays and electrophoresis as new paradigms for at-line monitoring and control of mammalian cell bioprocesses

Author

Aman Russom, Inês F. Pinto, Saara Mikkonen, Meeri Mäkinen, Veronique Chotteau, Ruben R. G. Soares, Leila Josefsson, and Åsa Emmer

Subjects
Electrophoresis, Computer science, Process analytical technology, Microfluidics, Biomedical Engineering, Bioengineering, 02 engineering and technology, Ligands, 01 natural sciences, Capillary electrophoresis, Teknik och teknologier, Miniaturization, Animals, Bioprocess, Bioprocess Technology, Ligand binding assay, 010401 analytical chemistry, Bioprocessteknik, 021001 nanoscience & nanotechnology, 0104 chemical sciences, Engineering and Technology, Biological Assay, Biochemical engineering, 0210 nano-technology, Critical quality attributes, Biotechnology
Abstract

Monitoring technologies for Process Analytical Technology (PAT) in mammalian cell cultures are often focusing on the same hand full parameters although a deeper knowledge and control of a larger panel of culture components would highly benefit process optimization, control and robustness. This short review highlights key advances in microfluidic affinity assays and microchip capillary electrophoresis (MCE). Aiming at the miniaturization and integration of PAT, these can detect at-line a variety of metabolites, proteins and Critical Quality Attributes (CQA’s) in a bioprocess. Furthermore, discrete analytical components, which can potentially support the translation of increasingly mature microfluidic technologies towards this novel application, are also presented as a comprehensive toolbox ranging from sample preparation to signal acquisition.

Published
2021

16. Multiplexed Microfluidic Cartridge for At-Line Protein Monitoring in Mammalian Cell Culture Processes for Biopharmaceutical Production

Author

Ruben R. G. Soares, Veronique Chotteau, Meeri Mäkinen, Aman Russom, and Inês F. Pinto

Subjects
host cell proteins, Microfluidics, Cell Culture Techniques, microfluidics, Bioengineering, Context (language use), 02 engineering and technology, CHO Cells, 01 natural sciences, Article, colorimetric, Cricetulus, Cricetinae, Bioreactor, medicine, Animals, Humans, Viability assay, immunoassay, Instrumentation, Bioprocess Technology, Fluid Flow and Transfer Processes, Biological Products, Downstream processing, medicine.diagnostic_test, Chemistry, Process Chemistry and Technology, Chinese hamster ovary cell, 010401 analytical chemistry, Bioprocessteknik, 021001 nanoscience & nanotechnology, 0104 chemical sciences, Cell biology, Biopharmaceutical, Cell culture, Immunoassay, streptavidin beads, monoclonal antibodies, 0210 nano-technology
Abstract

The biopharmaceutical market has been rapidly growing in recent years, creating a highly competitive arena where R&D is critical to strike a balance between clinical safety and profitability. Toward process optimization, the recent development and adoption of new process analytical technologies (PAT) highlight the dynamic complexity of mammalian/human cell culture processes, as well as the importance of fine-tuning and modeling key metabolites and proteins. In this context, simple, rapid, and cost-effective devices allowing routine at-line monitoring of specific proteins during process development and production are currently lacking. Here, we report the development of a versatile microfluidic protein analysis cartridge allowing the multiplexed bead-based immunodetection of specific proteins directly from complex mixtures with minimal hands-on time. Colorimetric quantification of Chinese hamster ovary (CHO) host cell proteins as key impurities, monoclonal antibodies as target biopharmaceuticals, and lactate dehydrogenase as a marker of cell viability was achieved with limits of detection in the 1-10 ng/mL range and analysis times as short as 30 min. The device was further demonstrated for the monitoring of a Rituximab-producing CHO cell bioreactor over the course of 8 days, providing comparable recoveries to standard enzyme-linked immunosorbent assay (ELISA) kits. The high sensitivity combined with robustness to matrix interference highlights the potential of the device to perform at-line measurements spanning from the bioreactor to the downstream processing. QC 20210507

Published
2021

17. Multi-layer assembly of cellulose nanofibrils in a microfluidic device for the selective capture and release of viable tumor cells from whole blood

Author

Harisha Ramachandraiah, Zenib Aljadi, Leyla Ali Dholey, Torbjörn Pettersson, Negar Abbasi Aval, Ruben R. G. Soares, Tharagan Kumar, and Aman Russom

Subjects
Colorectal cancer, Biomaterialvetenskap, Cell Count, Cell Separation, chemistry.chemical_compound, Circulating tumor cell, Cell Line, Tumor, Lab-On-A-Chip Devices, medicine, Humans, General Materials Science, Viability assay, Cellulose, Whole blood, biology, Cancer, Microfluidic Analytical Techniques, medicine.disease, Neoplastic Cells, Circulating, chemistry, Cell culture, biology.protein, Biomaterials Science, Antibody, Biomedical engineering
Abstract

According to reports by the World Health Organization (WHO), cancer-related deaths reached almost 10 million in 2018. Nearly 65% of these deaths occurred in low- to middle-income countries, a trend that is bound to increase since cancer diagnostics are not currently considered a priority in resource-limited settings (RLS). Thus, cost-effective and specific cancer screening and diagnostics tools are in high demand, particularly in RLS. The selective isolation and up-concentration of rare cells while maintaining cell viability and preventing phenotypic changes is a powerful tool to allow accurate and sensitive downstream analysis. Here, multi-layer cellulose nanofibril-based coatings functionalized with anti-EpCAM antibodies on the surface of disposable microfluidic devices were optimized for specific capture of target cells, followed by efficient release without significant adverse effects. HCT 116 colon cancer cells were captured in a single step with >97% efficiency at 41.25 mu L min(-1) and, when spiked in whole blood, an average enrichment factor of similar to 200-fold relative to white blood cells was achieved. The release of cells was performed by enzymatic digestion of the cellulose nanofibrils which had a negligible impact on cell viability. In particular, >80% of the cells were recovered with at least 97% viability in less than 30 min. Such performance paves the way to expand and improve clinical diagnostic applications by simplifying the isolation of circulating tumor cells (CTCs) and other rare cells directly from whole blood. QC 20201201

Published
2020

18. Capillary-driven microfluidic device with integrated nanoporous microbeads for ultrarapid biosensing assays

Author

Inês F. Pinto, Ruben R. G. Soares, Roberta Epifania, Virginia Chu, and João Pedro Conde

Subjects
Analyte, Materials science, Nanoporous, Capillary action, 010401 analytical chemistry, Microfluidics, Metals and Alloys, Nanotechnology, 02 engineering and technology, 021001 nanoscience & nanotechnology, Condensed Matter Physics, 01 natural sciences, 0104 chemical sciences, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, Robustness (computer science), Materials Chemistry, Competitive immunoassay, Electrical and Electronic Engineering, 0210 nano-technology, Instrumentation, Biosensor
Abstract

For microfluidic devices to achieve a practical point-of-need application, it is necessary to circumvent the often excessive system complexity required, such as external pumps and multi-step operation, in order to provide a rapid and simple, while still robust and fit-for-purpose device. We report a simple capillary-based microfluidic device with integrated microbeads and a no-wash, single-step mode of operation that achieves a sub-minute detection of analytes using a fluorescent competitive immunoassay. In particular, minimum detectable limits of 1.7 ng/mL were obtained for mycotoxin detection within 70 s assay time, using 4.5 μL of sample. Furthermore, an internal control was also included in the microfluidic device to provide additional robustness and result validation. These results support the development of ultra-rapid and simple microfluidic devices, easily extended to other relevant targets within the food safety, biomedical or environmental fields.

Published
2018

19. A regenerable microfluidic device with integrated valves and thin-film photodiodes for rapid optimization of chromatography conditions

Author

João Pedro Conde, Ana Azevedo, Inês F. Pinto, Denis R. Santos, Ruben R. G. Soares, Virginia Chu, and Maria Raquel Aires-Barros

Subjects
Materials science, Microfluidics, Nanotechnology, 02 engineering and technology, 01 natural sciences, law.invention, Adsorption, law, Materials Chemistry, Electrical and Electronic Engineering, Thin film, Instrumentation, Enhanced selectivity, Chromatography, Elution, 010401 analytical chemistry, Metals and Alloys, 021001 nanoscience & nanotechnology, Condensed Matter Physics, 0104 chemical sciences, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, Photodiode, Lower cost, Cell culture supernatant, 0210 nano-technology
Abstract

The optimization of chromatography operating conditions is a lengthy and demanding task that typically requires large volumes of reagents and costly dedicated equipment. In particular, the use of multimodal chromatography, in which multiple interaction groups co-exist in the same ligand, can make the optimization process even more challenging. Nevertheless, the interest in using this emerging type of ligands has been increasing due to the enhanced selectivity and stability demonstrated by multimodal ligands in the purification of several biopharmaceuticals and their lower cost compared to biological affinity ligands. In this work, we report the development of an integrated, regenerable and portable microfluidic platform for performing a rapid screening of chromatography conditions. This platform was tested for the capture of fluorophore-labeled monoclonal antibodies directly from a cell culture supernatant using a multimodal ligand (Capto MMC). Liquid insertion in the microfluidic device was controlled by pneumatically actuated embedded valves and chromatography cycles were monitored via fluorescence measurements using thin-film a-Si:H photodiodes aligned beneath the device. The regeneration of the chromatography micro-column (70 nL) was performed in the end of each cycle, providing repeatable results over several consecutive cycles. Different buffers were successively evaluated in cycles, each cycle having duration of about 3 min, and the different adsorption and elution kinetics were compared, allowing the rapid optimization of conditions to address the capture of the monoclonal antibody from complex media. Overall, a versatile, rapid and relatively inexpensive platform to perform screening studies was developed, providing a high degree of scalability.

Published
2018

20. Circle-to-circle amplification coupled with microfluidic affinity chromatography enrichment for in vitro molecular diagnostics of Zika fever and analysis of anti-flaviviral drug efficacy

Author

Aman Russom, Mats Nilsson, Aleksandra Pettke, Sahar Zeebaree, Agustín Robles-Remacho, Ruben R. G. Soares, Narayanan Madaboosi, Sibel Ciftci, Marianna Tampere, and Marjo-Riitta Puumalainen

Subjects
Diagnostic methods, Metals and Alloys, Loop-mediated isothermal amplification, 02 engineering and technology, Limiting, Biology, 010402 general chemistry, 021001 nanoscience & nanotechnology, Condensed Matter Physics, biology.organism_classification, Molecular diagnostics, 01 natural sciences, Virology, 0104 chemical sciences, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, Zika virus, Rolling circle replication, Materials Chemistry, Electrical and Electronic Engineering, 0210 nano-technology, Instrumentation, Limited resources
Abstract

Sensitive viral diagnostic methods are increasingly in demand to tackle emerging epidemics. The Zika virus (ZIKV) is particularly relevant in tropical resource limited settings (RLS) and is associated with intermittent epidemics such as the recent 2016 ZIKV outbreak in South America, wherein Zika fever was classified by WHO as a public health emergency of international concern. Thus, there is an urgent need for widespread Zika fever diagnostics and efficient drug therapies. ZIKV diagnostics are typically performed using RT-qPCR in centralized laboratories. While extremely sensitive, RT-qPCR requires rapid heating-cooling cycles, combined with continuous fluorescence measurements to allow quantification, implying high costs and limiting availability of molecular diagnostics in RLS. Here, we report isothermal amplification of ZIKV cDNA using padlock probes followed by two rounds of Rolling Circle Amplification (RCA), termed as circle-to-circle amplification (C2CA), combined with a microfluidic affinity chromatography enrichment (μACE) platform. This platform allowed the detection of

Published
2021

21. A multiplexed microfluidic toolbox for the rapid optimization of affinity-driven partition in aqueous two phase systems

Author

Ana Azevedo, Pedro Fernandes, João Pedro Conde, Ruben R. G. Soares, Virginia Chu, Eduardo J. S. Bras, M. Raquel Aires-Barros, and Miguel Arévalo-Rodríguez

Subjects
Liquid-Liquid Extraction, Microfluidics, 02 engineering and technology, Ligands, 01 natural sciences, Biochemistry, Multiplexing, Antibodies, Polyethylene Glycols, Analytical Chemistry, Liquid–liquid extraction, Microfluidic channel, Chromatography, Aqueous solution, Chemistry, 010401 analytical chemistry, Organic Chemistry, General Medicine, 021001 nanoscience & nanotechnology, Fusion protein, Toolbox, 0104 chemical sciences, Partition coefficient, Kinetics, 0210 nano-technology
Abstract

Antibodies and other protein products such as interferons and cytokines are biopharmaceuticals of critical importance which, in order to be safely administered, have to be thoroughly purified in a cost effective and efficient manner. The use of aqueous two-phase extraction (ATPE) is a viable option for this purification, but these systems are difficult to model and optimization procedures require lengthy and expensive screening processes. Here, a methodology for the rapid screening of antibody extraction conditions using a microfluidic channel-based toolbox is presented. A first microfluidic structure allows a simple negative-pressure driven rapid screening of up to 8 extraction conditions simultaneously, using less than 20μL of each phase-forming solution per experiment, while a second microfluidic structure allows the integration of multi-step extraction protocols based on the results obtained with the first device. In this paper, this microfluidic toolbox was used to demonstrate the potential of LYTAG fusion proteins used as affinity tags to optimize the partitioning of antibodies in ATPE processes, where a maximum partition coefficient (K) of 9.2 in a PEG 3350/phosphate system was obtained for the antibody extraction in the presence of the LYTAG-Z dual ligand. This represents an increase of approx. 3.7 fold when compared with the same conditions without the affinity molecule (K=2.5). Overall, this miniaturized and versatile approach allowed the rapid optimization of molecule partition followed by a proof-of-concept demonstration of an integrated back extraction procedure, both of which are critical procedures towards obtaining high purity biopharmaceuticals using ATPE.

Published
2017

22. A point-of-use microfluidic device with integrated photodetector array for immunoassay multiplexing: Detection of a panel of mycotoxins in multiple samples

Author

Ana Azevedo, Maria Raquel Aires-Barros, Denis R. Santos, Ruben R. G. Soares, João Pedro Conde, and Virginia Chu

Subjects
Ochratoxin A, Analyte, Aflatoxin B1, Immunoconjugates, Materials science, Microfluidics, Biomedical Engineering, Biophysics, Photodetector, Food Contamination, Nanotechnology, Biosensing Techniques, 02 engineering and technology, 01 natural sciences, Multiplexing, chemistry.chemical_compound, Limit of Detection, Lab-On-A-Chip Devices, Electrochemistry, medicine, media_common.cataloged_instance, Multiplex, European union, Horseradish Peroxidase, media_common, Immunoassay, Chromatography, medicine.diagnostic_test, 010401 analytical chemistry, Equipment Design, General Medicine, 021001 nanoscience & nanotechnology, Ochratoxins, 0104 chemical sciences, chemistry, Luminescent Measurements, Trichothecenes, 0210 nano-technology, Biotechnology
Abstract

For a point-of-use analytical device to be successful in real-world applications, it needs to be rapid, simple to operate and, ideally, able to multiplex the detection of several analytes and samples. Mycotoxin detection in food and feedstock in particular has become increasingly relevant as these toxins, such as ochratoxin A (OTA), aflatoxin B1 (AFB1) and deoxynivalenol (DON), are subject to strict regulations and recommendations in the European Union. A novel, simple, negative pressure-driven device with manually operated magnetic valves was developed and the simultaneous immunodetection of these three mycotoxins was demonstrated via the laminar flow patterning of probes in an area of ≈0.12mm2 and subsequent chemiluminescence generation via HRP-labeled antibodies. The three mycotoxins were detected in less than 20min at concentrations of 100ng/mL for OTA and DON and 3ng/mL for AFB1, spiked in a sample under analysis and simultaneously compared to a toxin-free reference and a standard contaminated with critical target concentrations. The on-chip optical detection was performed in a single acquisition step by integrating a microfabricated array of 25×25µm2 hydrogenated amorphous silicon (a-Si:H) photosensors below the microfluidic chip. The device presented in this work is simple and effective for point-of-use multiplexing of immunoassays and was applied in this work to the screening of mycotoxins.

Published
2017

23. Applications of Recent Developments in Microfluidics for Rapid Analysis of Food Safety and Quality

Author

João Pedro Conde, Ruben R. G. Soares, and Virginia Chu

Subjects
Scope (project management), business.industry, Computer science, media_common.quotation_subject, Scale (chemistry), Microfluidics, Context (language use), Food safety, Automation, Microfluidic channel, Quality (business), Biochemical engineering, business, media_common
Abstract

Immunoassays performed on the nanolitre scale using microfluidics allow a reduction in reagent volumes and assay times, providing, by design, a high degree of control of mass transport and reaction kinetics. Furthermore, the development of rapid microfluidic prototyping technologies including soft lithography, 3D-printing and micromilling have resulted in a dramatic increase in the reporting of innovative analytic strategies integrating sample preparation, immunodetection and signal transduction in miniaturized portable devices. This degree of integration and automation aims to allow the routine monitoring of target molecules by non-specialized personnel. This is currently in high demand by regulatory agencies, producers and consumers within the scope of food safety and quality. This chapter summarizes recent trends in miniaturized immunoassays, discusses the fundamental concepts of immunoassays performed in microfluidic channels and provides an overview of current design strategies for miniaturization, with an emphasis on the integration of optical, electrochemical and label-free methods to provide signal transduction. In addition, examples of these assays in the context of food safety and quality, namely in the detection of low molecular weight organic and inorganic contaminants, protein toxins or allergens and foodborne pathogens, are described and discussed in detail.

Published
2019

24. Minimizing the Influence of Fluorescent Tags on IgG Partition in PEG-Salt Aqueous Two-Phase Systems for Rapid Screening Applications

Author

Ruben R. G. Soares, Ana Azevedo, Mariana N. São Pedro, and Maria Raquel Aires-Barros

Subjects
Boron Compounds, Fluorophore, Phosphines, Liquid-Liquid Extraction, Context (language use), Polyethylene glycol, Sodium Chloride, Applied Microbiology and Biotechnology, Phosphates, Polyethylene Glycols, Maleimides, chemistry.chemical_compound, Lab-On-A-Chip Devices, Sulfhydryl Compounds, Maleimide, Fluorescent Dyes, Chromatography, General Medicine, Partition coefficient, Molecular Weight, chemistry, Reagent, Immunoglobulin G, TCEP, Molecular Medicine, BODIPY
Abstract

Aqueous two-phase extraction (ATPE) has been showing significant potential in the biopharmaceutical industry, allowing the selective separation of high-value proteins directly from unclarified cell culture supernatants. In this context, effective high-throughput screening tools are critical to perform a rapid empirical optimization of operating conditions. In particular, microfluidic ATPE screening devices, coupled with fluorescence microscopy to continuously monitor the partition of fluorophore-labeled proteins, have been recently demonstrated to provide short diffusion distances and rapid partition, using minimal reagent volumes. Nevertheless, the currently overlooked influence of the labeling procedure on partition must be carefully evaluated to validate the extrapolation of results to the unlabeled molecule. Here, three fluorophores with different global charge and reactivity selected to label immunoglobulin G (IgG) at degrees of labeling (DoL) ranging from 0.5 to 7.6. Labeling with BODIPY FL maleimide (DoL = 0.5), combined with tris(2-carboxyethyl) phosphine (TCEP) to generate free thiol groups, is the most promising strategy to minimize the influence of the fluorophore on partition. In particular, the partition coefficient (Kp ) measured in polyethylene glycol (PEG) 3350-phosphate systems with and without the addition of NaCl using microtubes (batch) or microfluidic devices (continuous) is comparable to those quantified for the native protein.

Published
2019

25. Optimizing the Performance of Chromatographic Separations Using Microfluidics: Multiplexed and Quantitative Screening of Ligands and Target Molecules

Author

Ana Azevedo, João Pedro Conde, Ruben R. G. Soares, Virginia Chu, Inês F. Pinto, and Maria Raquel Aires-Barros

Subjects
0106 biological sciences, medicine.drug_class, Microfluidics, Context (language use), Monoclonal antibody, Ligands, 01 natural sciences, Applied Microbiology and Biotechnology, Multiplexing, 010608 biotechnology, medicine, Molecule, Bovine serum albumin, Fluorescent Dyes, Chromatography, biology, Chemistry, 010401 analytical chemistry, Serum Albumin, Bovine, General Medicine, Fluorescence, 0104 chemical sciences, Yield (chemistry), Immunoglobulin G, biology.protein, Molecular Medicine
Abstract

The optimization of chromatography ligands for the purification of biopharmaceuticals is highly demanded to meet the needs of the pharmaceutical industry. In the case of monoclonal antibodies (mAbs), synthetic ligands comprising multiple types of interactions (multimodal) provide process and economic advantages compared to protein-based affinity ligands. However, optimizing the operation window of these ligands requires the development of effective high-throughput screening platforms. Here, a novel microfluidics-based methodology to perform rapid and multiplexed screening of various multimodal ligands relative to their ability to bind different target molecules is demonstrated. The microfluidic structure comprises three individual chambers (≈8 nL each) packed with different types of chromatography beads in series with the feed flow. An artificial mixture composed of immunoglobulin G (IgG) and bovine serum albumin, labeled with different thiol-reactive neutral fluorescent dyes, is used as a model to quantitatively optimize the performance (yield and purity) of the separation. This approach can potentially be used as a predictive analytical tool in the context of mAb purification, allowing low consumption of molecules and providing results in

Published
2019

26. Silica bead-based microfluidic device with integrated photodiodes for the rapid capture and detection of rolling circle amplification products in the femtomolar range

Author

Virginia Chu, Aman Russom, Mats Nilsson, Iván Hernández-Neuta, João Pedro Conde, Felix Neumann, Inês F. Pinto, Narayanan Madaboosi, Denis R. Santos, Ruben R. G. Soares, Sibel Ciftci, and Catarina R.F. Caneira

Subjects
Materials science, Point-of-Care Systems, Microfluidics, Biomedical Engineering, Biophysics, Nanotechnology, 02 engineering and technology, Biosensing Techniques, 01 natural sciences, Fluorescence, law.invention, law, Limit of Detection, Lab-On-A-Chip Devices, Electrochemistry, Detection limit, Base Sequence, 010401 analytical chemistry, Ranging, General Medicine, Amplicon, 021001 nanoscience & nanotechnology, Ebolavirus, Silicon Dioxide, 0104 chemical sciences, Photodiode, Transducer, Rolling circle replication, Nucleic acid, RNA, 0210 nano-technology, Nucleic Acid Amplification Techniques, Biotechnology
Abstract

The rapid and sensitive detection of specific nucleic acid sequences at the point-of-care (PoC) is becoming increasingly in demand for a variety of emergent biomedical applications ranging from infectious disease diagnostics to the screening of antimicrobial resistance. To meet such demand, considerable efforts have been invested towards the development of portable and integrated analytical devices combining microfluidics with miniaturized signal transducers. Here, we demonstrate the combination of rolling circle amplification (RCA)-based nucleic acid amplification with an on-chip size-selective trapping of amplicons on silica beads (~8 nL capture chamber) coupled with a thin-film photodiode (200 × 200 µm area) fluorescence readout. Parameters such as the flow rate of the amplicon solution and trapping time were optimized as well as the photodiode measurement settings, providing minimum detection limits below 0.5 fM of targeted nucleic acids and requiring only 5 μL of pre-amplified sample. Finally, we evaluated the analytical performance of our approach by benchmarking it against a commercial instrument for RCA product (RCP) quantification and further investigated the effect of the number of RCA cycles and elongation times (ranging from 10 to 120 min). Moreover, we provide a demonstration of the application for diagnostic purposes by detecting RNA from influenza and Ebola viruses, thus highlighting its suitability for integrated PoC systems.

Published
2019
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27. An ultrarapid and regenerable microfluidic immunoassay coupled with integrated photosensors for point-of-use detection of ochratoxin A

Author

Ruben R. G. Soares, João Pedro Conde, Virginia Chu, Diogo Ramadas, A.C. Cascalheira, Maria Raquel Aires-Barros, and Ana S. Viana

Subjects
Ochratoxin A, Computer science, Microfluidics, Nanotechnology, 02 engineering and technology, 01 natural sciences, chemistry.chemical_compound, Materials Chemistry, medicine, Electrical and Electronic Engineering, Mycotoxin, Process engineering, Instrumentation, Health implications, medicine.diagnostic_test, business.industry, 010401 analytical chemistry, Metals and Alloys, 021001 nanoscience & nanotechnology, Condensed Matter Physics, 0104 chemical sciences, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, chemistry, Immunoassay, 0210 nano-technology, business
Abstract

The assurance of food and feed safety is one of the major challenges in modern society given the increasing pace at which food commodities are demanded, produced and traded across the globe. Ochratoxin A (OTA), a mycotoxin produced either in the field or during storage, has been increasingly associated with detrimental chronic and acute health implications such as carcinogenicity and hepatotoxicity. Currently, standard certified detection methods include complex and time consuming (>1 h) methodologies based on packed-bed chromatography which must be performed by specialized personnel. However, to effectively monitor mycotoxin levels in crops prior to further processing, either after harvest, during transport or during storage, a rapid, simple, portable and sensitive means of screening is in high demand. In order to meet this demand, a novel ultra-rapid, sensitive (limit-of-detection (LoD)

Published
2016

28. Miniaturization of aqueous two-phase extraction for biological applications: From micro-tubes to microchannels

Author

João Pedro Conde, Ruben R. G. Soares, Pedro Fernandes, Ana Azevedo, D.F.C. Silva, M. Raquel Aires-Barros, and Virginia Chu

Subjects
Materials science, Liquid-Liquid Extraction, Microfluidics, Nanotechnology, 02 engineering and technology, 01 natural sciences, Applied Microbiology and Biotechnology, Lab-On-A-Chip Devices, Miniaturization, Animals, Cells, Cultured, Microscale chemistry, chemistry.chemical_classification, Microchannel, Aqueous solution, Biomolecule, 010401 analytical chemistry, Equipment Design, General Medicine, Micro tube, 021001 nanoscience & nanotechnology, 0104 chemical sciences, chemistry, Culture Media, Conditioned, Fermentation, Molecular Medicine, 0210 nano-technology, Biotechnology, Large animal
Abstract

Aqueous two-phase extraction (ATPE) is a biocompatible liquid-liquid (L-L) separation technique that has been under research for several decades towards the purification of biomolecules, ranging from small metabolites to large animal cells. More recently, with the emergence of rapid-prototyping techniques for fabrication of microfluidic structures with intricate designs, ATPE gained an expanded range of applications utilizing physical phenomena occurring exclusively at the microscale. Today, research is being carried simultaneously in two different volume ranges, mL-scale (microtubes) and nL-scale (microchannels). The objective of this review is to give insight into the state of the art at both microtube and microchannel-scale and to analyze whether miniaturization is currently a competing or divergent technology in a field of applications including bioseparation, bioanalytics, enhanced fermentation processes, catalysis, high-throughput screening and physical/chemical compartmentalization. From our perspective, both approaches are worthy of investigation and, depending on the application, it is likely that either (i) one of the approaches will eventually become obsolete in particular research areas such as purification at the preparative scale or high-throughput screening applications; or (ii) both approaches will function as complementing techniques within the bioanalytics field.

Published
2016

29. Lab-on-chip systems for integrated bioanalyses

Author

Virginia Chu, João Pedro Conde, Narayanan Madaboosi, João Tiago S. Fernandes, G. Moulas, P. Novo, and Ruben R. G. Soares

Subjects
Analyte, Computer science, Microfluidics, Nanotechnology, Biosensing Techniques, 02 engineering and technology, Transduction (psychology), fluidic handling, 01 natural sciences, Biochemistry, Signal, Article, law.invention, signal detection, law, Microchip Analytical Procedures, Detection theory, Fluidics, Molecular Biology, business.industry, 010401 analytical chemistry, integrated systems, Lab-on-a-chip, 021001 nanoscience & nanotechnology, Chip, lab-on-chip, 0104 chemical sciences, Molecular Diagnostic Techniques, point-of-care, 0210 nano-technology, business, Computer hardware
Abstract

Biomolecular detection systems based on microfluidics are often called lab-on-chip systems. To fully benefit from the miniaturization resulting from microfluidics, one aims to develop ‘from sample-to-answer’ analytical systems, in which the input is a raw or minimally processed biological, food/feed or environmental sample and the output is a quantitative or qualitative assessment of one or more analytes of interest. In general, such systems will require the integration of several steps or operations to perform their function. This review will discuss these stages of operation, including fluidic handling, which assures that the desired fluid arrives at a specific location at the right time and under the appropriate flow conditions; molecular recognition, which allows the capture of specific analytes at precise locations on the chip; transduction of the molecular recognition event into a measurable signal; sample preparation upstream from analyte capture; and signal amplification procedures to increase sensitivity. Seamless integration of the different stages is required to achieve a point-of-care/point-of-use lab-on-chip device that allows analyte detection at the relevant sensitivity ranges, with a competitive analysis time and cost.

Published
2016

30. DNA aptamer-based sandwich microfluidic assays for dual quantification and multi-glycan profiling of cancer biomarkers

Author

Narayanan Madaboosi, Jaroslav Katrlík, V. Chu, João Pedro Conde, Ruben R. G. Soares, Pavel Damborsky, Pedro Estrela, and Pawan Jolly

Subjects
Male, 0301 basic medicine, Analyte, Glycosylation, Aptamer, Microfluidics, microfluidics, Biomedical Engineering, Biophysics, Enzyme-Linked Immunosorbent Assay, Biosensing Techniques, 01 natural sciences, law.invention, 03 medical and health sciences, Prostate cancer, chemistry.chemical_compound, SDG 3 - Good Health and Well-being, Polysaccharides, law, Biomarkers, Tumor, Electrochemistry, medicine, Humans, Chemiluminescence, sandwich assay, biology, 010401 analytical chemistry, glycoprofiling, Prostatic Neoplasms, General Medicine, DNA aptamers, Aptamers, Nucleotide, Prostate-Specific Antigen, Prognosis, medicine.disease, Primary and secondary antibodies, Molecular biology, 0104 chemical sciences, 030104 developmental biology, chemistry, biology.protein, ELISA, Cancer biomarkers, Antibody, Biotechnology
Abstract

Two novel sandwich-based immunoassays for prostate cancer (PCa) diagnosis are reported, in which the primary antibody for capture is replaced by a DNA aptamer. The assays, which can be performed in parallel, were developed in a microfluidic device and tested for the detection of free Prostate Specific Antigen (fPSA). A secondary antibody (Aptamer–Antibody Assay) or a lectin (Aptamer–Lectin Assay) is used to quantify, by chemiluminescence, both the amount of fPSA and its glycosylation levels. The use of aptamers enables a more reliable, selective and controlled sensing of the analyte. The dual approach provides sensitive detection of fPSA along with selective fPSA glycoprofiling, which is of significant importance in the diagnosis and prognosis of PCa, as tumor progression is associated with changes in fPSA glycosylation. With these approaches, we can potentially detect 0.5 ng/mL of fPSA and 3 ng/mL of glycosylated fPSA using Sambucus nigra (SNA) lectin, both within the relevant clinical range. The approach can be applied to a wide range of biomarkers, thus providing a good alternative to standard antibody-based immunoassays with significant impact in medical diagnosis and prognosis.

Published
2016

31. Integration of Photosensors in a Nano-liter Scale Chromatography Column for the Online Monitoring of Adsorption/Desorption Kinetics of a Fluorophore-labeled Monoclonal Antibody

Author

Ana Azevedo, João Pedro Conde, Inês F. Pinto, Ruben R. G. Soares, Maria Raquel Aires-Barros, Virginia Chu, and Denis R. Santos

Subjects
0106 biological sciences, Fluorophore, Chromatography, medicine.drug_class, Microfluidics, 02 engineering and technology, General Medicine, 021001 nanoscience & nanotechnology, Monoclonal antibody, 01 natural sciences, Fluorescence, Receptor–ligand kinetics, chemistry.chemical_compound, chemistry, 010608 biotechnology, Reagent, medicine, 0210 nano-technology, Chromatography column, Engineering(all), Conjugate
Abstract

Chromatography is a robust purification technique, but requires time-consuming optimization on a case-by-case basis, particularly for monoclonal antibodies (mAbs). This work presents a novel microfluidic platform that significantly speeds up the optimization process and reduces the amount of reagent needed. Binding kinetics for a fluorescent conjugate mAb-Alexa 430 were measured in real time at resin level by integration of the microfluidic chip with 200×200 μm a-Si:H photodiodes on glass substrates aligned with micro-columns. Screening studies were performed using reduced amounts of reagents (∼50 μL), mAb molecules (∼2.5 μL) and resin (∼70 nL) in a rapid (∼2 min/condition) and simple manner.

Published
2016

32. A Multiplexed Integrated a-Si:H Photosensor for Simultaneous Detection of Mycotoxins for Point-of-use Food Safety Applications

Author

Ruben R. G. Soares, Denis R. Santos, Maria Raquel Aires-Barros, Virginia Chu, and João Pedro Conde

Subjects
Ochratoxin A, Aflatoxin, Materials science, 010401 analytical chemistry, Microfluidics, food and beverages, Photodetector, Nanotechnology, 02 engineering and technology, General Medicine, 021001 nanoscience & nanotechnology, 01 natural sciences, Multiplexing, 0104 chemical sciences, law.invention, chemistry.chemical_compound, chemistry, law, media_common.cataloged_instance, European union, 0210 nano-technology, Mycotoxin, Engineering(all), media_common, Chemiluminescence
Abstract

Food safety can be seriously compromised by the presence of mycotoxins. Their detection becomes increasingly relevant as they are subject to strict regulations in the European Union. To cope with this demand, a novel device with manually operated magnetic valves was developed and applied in a direct competitive immunoassay with multiplexed chemiluminescence detection of ochratoxin A, aflatoxin B1 and deoxynivalenol. The optical detection of chemiluminescence from the enzymatically labelled antibodies is performed with a microfabricated array of 25 μm x 25 μm hydrogenated amorphous silicon (a-Si:H) photoconductors. This strategy provides a simple multiplexing device for mycotoxin screening on the field.

Published
2016

33. Point-of-use Ultrafast Single-step Detection of Food Contaminants: A Novel Microfluidic Fluorescence-based Immunoassay with Integrated Photodetection

Author

Maria Raquel Aires-Barros, João Pedro Conde, Ana Azevedo, Virginia Chu, Denis R. Santos, Ruben R. G. Soares, and Inês F. Pinto

Subjects
Aflatoxin, Materials science, medicine.diagnostic_test, business.industry, 010401 analytical chemistry, Microfluidics, Single step, Nanotechnology, 02 engineering and technology, General Medicine, Photodetection, 021001 nanoscience & nanotechnology, Food safety, 01 natural sciences, Fluorescence, 0104 chemical sciences, Immunoassay, medicine, 0210 nano-technology, business, Engineering(all), Food contaminant
Abstract

The assurance of strict food safety standards is a major challenge in modern society. Mycotoxins, in particular, are produced by fungi during production, storage or transport, posing serious health concerns to humans and animals. Aiming at developing a point-of-use tool for the rapid detection of mycotoxins at the required regulatory levels, we report a microfluidic ultrafast and single-step fluorescence-based immunoassay, using minimal amounts of reagents. This assay was integrated with 200×200 μm thin-film a-Si:H photodiodes towards a compact detection system. Aflatoxin B1 was detected at 1 ng/mL after 2 min assay time, among the fastest reported in the literature.

Published
2016
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34. Sub-attomole detection of HIV-1 using padlock probes and rolling circle amplification combined with microfluidic affinity chromatography

Author

Aman Russom, Manickam Ashokkumar, Mats Nilsson, Ujjwal Neogi, João C. Varela, Narayanan Madaboosi, Inês F. Pinto, Sibel Ciftci, and Ruben R. G. Soares

Subjects
Fluorophore, Computer science, Microfluidics, Biomedical Engineering, Biophysics, Human immunodeficiency virus (HIV), Nanotechnology, Biosensing Techniques, 02 engineering and technology, medicine.disease_cause, 01 natural sciences, Signal, Chromatography, Affinity, chemistry.chemical_compound, Affinity chromatography, Electrochemistry, medicine, Humans, Detection limit, 010401 analytical chemistry, General Medicine, 021001 nanoscience & nanotechnology, Molecular diagnostics, 0104 chemical sciences, chemistry, Rolling circle replication, HIV-1, 0210 nano-technology, Nucleic Acid Amplification Techniques, Biotechnology
Abstract

Despite significant progress in diagnostics and disease management during the past decades, human immunodeficiency virus (HIV) infections are still responsible for nearly 1 million deaths every year, mostly in resource-limited settings. Thus, novel, accurate and cost-effective tools for viral load monitoring become crucial to allow specific diagnostics and the effective monitoring of the associated antiviral therapies. Herein, we report an effective combination of a (1) padlock probe (PLP)-mediated rolling circle amplification (RCA) bioassay and an (2) agarose bead-based microfluidic device for the affinity chromatography-based capture and detection of RCA products (RCPs) pre-labelled simultaneously with biotin and an organic fluorophore. This method allowed the efficient capture of ~1 μm-sized RCPs followed by their quantification either as discrete signals or an average fluorescence signal, thus being compatible with both high-resolution imaging for maximum sensitivity as well as simpler optical detection setups. A limit of detection30 fM was obtained for HIV-1 synthetic target with just a single round of RCA, comparable to recently reported procedures requiring technically complex amplification strategies such as hyperbranching and/or enzymatic digestion/amplification. Furthermore, targeting a set of five conserved regions in the HIV-1 gag gene, the method could specifically detect HIV-1 in 293T cell culture supernatants, as well as a set of 11 HIV-1 NIH reference samples with four different subtypes. The reported method provides simplicity of operation, unique versatility of signal transduction (i.e. average or discrete signals), and potential coupling with previously reported miniaturized photodetectors. These combined features hold promise for bringing RCA-based molecular diagnostics closer to the point-of-care.

Published
2020

35. Multiplexed microfluidic fluorescence immunoassay with photodiode array signal acquisition for sub-minute and point-of-need detection of mycotoxins

Author

Ruben R. G. Soares, Ana Azevedo, M. Raquel Aires-Barros, Inês F. Pinto, Denis R. Santos, Virginia Chu, and João Pedro Conde

Subjects
Ochratoxin A, Aflatoxin, Analyte, Materials science, Microfluidics, Biomedical Engineering, Fluorescent Antibody Technique, Bioengineering, 02 engineering and technology, 01 natural sciences, Biochemistry, Multiplexing, Zea mays, law.invention, chemistry.chemical_compound, law, Limit of Detection, Sample preparation, Detection limit, Chromatography, 010401 analytical chemistry, food and beverages, Reproducibility of Results, General Chemistry, Equipment Design, Microfluidic Analytical Techniques, Mycotoxins, 021001 nanoscience & nanotechnology, 0104 chemical sciences, Photodiode, chemistry, Linear Models, 0210 nano-technology, Protein Binding
Abstract

Portable, rapid, cost effective and simple analytical tools are in increasing demand to facilitate the routine monitoring of target chemical/biological compounds at the point-of-need. Such devices are highly relevant within the context of food safety, particularly concerning the screening of highly toxic and strictly regulated mycotoxins. To achieve ultrarapid detection of mycotoxins, namely aflatoxin B1, ochratoxin A and deoxynivalenol, at the point-of-need, a novel multiplexed bead-based microfluidic competitive immunosensor, coupled with an array of a-Si:H thin-film photodiodes for integrated fluorescence signal acquisition, is reported. Simultaneously measuring the initial binding rate for each analyte of the sample under analysis against an internal reference, this device provided limits of detection below 1 ng mL−1 for all mycotoxins in a single-step assay and within 1 minute after mixing the sample under analysis with a fluorescent conjugate. The compatibility of the device with the analysis of mycotoxins spiked in corn samples was further demonstrated after performing a sample preparation procedure based on aqueous two-phase extraction. The short times of analysis and sensitivities in the low ng mL−1 range make these devices potentially competitive with the lateral flow devices that are currently the standard for this application. Furthermore, this device architecture and concept is amenable of being expanded to other analytes in food safety, biomedical and other applications.

Published
2018

36. Advances, challenges and opportunities for point-of-need screening of mycotoxins in foods and feeds

Author

Giampiero de Cesare, Alessandra Ricelli, M. Raquel Aires-Barros, João Pedro Conde, Virginia Chu, Corrado Fanelli, Ruben R. G. Soares, and Domenico Caputo

Subjects
mycotoxin, detection, lab-on-chip, point-of-need, ELISA, Context (language use), Food Contamination, 02 engineering and technology, 01 natural sciences, Biochemistry, Analytical Chemistry, chemistry.chemical_compound, Electrochemistry, Environmental Chemistry, media_common.cataloged_instance, Animals, Humans, European union, Mycotoxin, Spectroscopy, media_common, Animal health, 010401 analytical chemistry, Fungi, food and beverages, LABEL-FREE DETECTION, CHROMATOGRAPHY-MASS-SPECTROMETRY, LATERAL FLOW IMMUNOASSAY, AQUEOUS 2-PHASE SYSTEMS, TESTING SHELLED CORN, QUANTUM-DOT BEADS, AFLATOXIN B-1, CARBON ELECTRODE, OCHRATOXIN-A, MICROFLUIDIC IMMUNOASSAY, Mycotoxins, 021001 nanoscience & nanotechnology, Animal Feed, 0104 chemical sciences, Risk analysis (engineering), chemistry, Food Microbiology, Business, 0210 nano-technology
Abstract

The assurance of food and feed safety, including the identification and effective monitoring of multiple biological and chemical hazards, is a major societal challenge, given the increasing pace at which food commodities are demanded, produced and traded across the globe. Within this context, mycotoxins are globally widespread secondary fungal metabolites, which can contaminate crops either in the field or during storage and have serious human and animal health impacts such as carcinogenic, teratogenic and hepatotoxic effects. Therefore, their presence in a wide range of foods and feeds is strictly regulated, particularly in the European Union. In order to perform effective and routine monitoring of mycotoxin levels in the field prior to further processing, during transport or during processing, rapid, simple, portable and sensitive means of screening of regulated mycotoxins are in high demand. This review focuses on (1) discussing the relevance of mycotoxins and the standard approaches for their sampling and monitoring; and (2) compiling and discussing recent advances in miniaturized analytical tools for mycotoxin detection. This provides insights into current research efforts and opportunities to develop a truly integrated and fit-for-purpose analytical tool, suitable for use at critical points of the food, feed and raw material processing and distribution chains.

Published
2018

37. Multiplexed microfluidic platform coupled with photodetector array for point-of-need and sub-minute detection of food contaminants

Author

Denis R. Santos, Ana Azevedo, M. Raquel Aires-Barros, Ruben R. G. Soares, Inês F. Pinto, Virginia Chu, and João Pedro Conde

Subjects
Materials science, Mycotoxin contamination, business.industry, Microfluidics, Photodetector, Single step, 02 engineering and technology, 010402 general chemistry, 021001 nanoscience & nanotechnology, 01 natural sciences, Multiplexing, 0104 chemical sciences, 0210 nano-technology, business, Computer hardware
Abstract

This paper presents an innovative integrated microfluidic platform which allows an ultrarapid detection of mycotoxins, a prevalent and increasingly monitored class of food contaminants. The simultaneous detection of aflatoxin B1 (AFB1), deoxynivalenol (DON) and ochratoxin A (OTA), within their respective regulatory limits is achieved in a single step within 60 s, by combining an array of thin-film photosensors and a disposable microfluidic device. This platform can potentially be the basis of portable tools allowing routine and cost-effective on-site screening of mycotoxin contamination by non-specialized personnel and be extended to other applications such as biomedical and environmental.

Published
2018

38. Quantitative analysis of optical transduction in microfluidic biosensing platforms: Nanoporous microbeads coupled with thin-film photodiodes

Author

Virginia Chu, João Pedro Conde, Ruben R. G. Soares, Catarina R.F. Caneira, Inês F. Pinto, and Denis R. Santos

Subjects
0301 basic medicine, Materials science, Nanoporous, Microfluidics, Photodetector, Nanotechnology, 02 engineering and technology, 021001 nanoscience & nanotechnology, Fluorescence, Photodiode, law.invention, 03 medical and health sciences, 030104 developmental biology, law, Thin film, 0210 nano-technology, Biosensor, Chemiluminescence
Abstract

This work presents a simple and innovative approach for the quantitative analysis of optical transduction signals from fluorescence, chemiluminescence and colorimetry coupled to a model affinity interaction inside a microfluidic device. By coupling nanoporous microbeads packed inside a microfluidic channel with an integrated photodetector, it was possible to quantify (i) the specific number of antibody-label conjugates bound to protein A coated beads at increasing concentrations and (ii) the emitted/absorbed photon flux involved in each of the transduction mechanisms. The measurement of (i) and (ii) allows a full quantitative understanding of a biosensing mechanism in general, providing a generic methodology to design a microfluidic point-of-need device with the appropriate label and probe dissociation constant (Kd) to achieve the required sensitivity.

Published
2018

39. Optimization and miniaturization of aqueous two phase systems for the purification of recombinant human immunodeficiency virus-like particles from a CHO cell supernatant

Author

A. Tover, Ana Azevedo, Ruben R. G. Soares, Virginia Chu, Maria João Jacinto, João Pedro Conde, and Maria Raquel Aires-Barros

Subjects
Ammonium sulfate, chemistry.chemical_compound, Chromatography, Downstream processing, Aqueous solution, Biocompatibility, Chemistry, Extraction (chemistry), Filtration and Separation, Polyethylene glycol, Bioprocess, Analytical Chemistry, Trisodium citrate
Abstract

Virus-like particles (VLPs) are promising candidates for a new generation of biopharmaceuticals, with a high impact in gene therapy, vaccination and also in the construction of delivery vehicles. Despite the growing interest in these particles, their production is currently limited by the low capacities and throughputs of classical downstream processing technologies. Aqueous two-phase extraction (ATPE) is a promising bioprocessing technique allowing clarification, concentration and purification to be accomplished in a single step. ATPE also combines a high biocompatibility with a simple and reliable scale-up and can also be performed in a continuous mode of operation. In this work, ATPE conditions for the purification of a Human Immunodeficiency Virus (HIV) VLP were screened and optimized in mL scale batch conditions. Polyethylene glycol (PEG)–salt (potassium phosphate, ammonium sulfate and trisodium citrate) and polymer–polymer (PEG–dextran) systems were investigated, among which the PEG–ammonium sulfate system demonstrated the higher partition coefficient ( K = 4.4). This parameter was then compared with the obtained in a continuous microfluidic setting, performed by flowing both immiscible phases through a 100 width × 20 μm wide microchannel. The batch optimization results showed good agreement with the continuous miniaturized extraction, both in terms of K ( K = 3.9 in microfluidic scale) and protein purity. These novel findings show that PEG–ammonium sulfate ATPE is a promising system for primary HIV-VLP recovery and demonstrate the potential of a miniaturized ATPE for massive parallelization (scale-out) at the preparative scale or integrated in analytical miniaturized systems.

Published
2015

40. Partitioning in aqueous two-phase systems: Analysis of strengths, weaknesses, opportunities and threats

Author

Ana Azevedo, Ruben R. G. Soares, M. Raquel Aires-Barros, and James M. Van Alstine

Subjects
Computer science, Liquid-Liquid Extraction, Industrial scale, Proteins, Nanotechnology, General Medicine, Applied Microbiology and Biotechnology, Economic benefits, Systems analysis, Nucleic Acids, SCALE-UP, Molecular Medicine, Biomanufacturing, Biochemical engineering, Bioprocess, SWOT analysis, Biotechnology
Abstract

For half a century aqueous two-phase systems (ATPSs) have been applied for the extraction and purification of biomolecules. In spite of their simplicity, selectivity, and relatively low cost they have not been significantly employed for industrial scale bioprocessing. Recently their ability to be readily scaled and interface easily in single-use, flexible biomanufacturing has led to industrial re-evaluation of ATPSs. The purpose of this review is to perform a SWOT analysis that includes a discussion of: (i) strengths of ATPS partitioning as an effective and simple platform for biomolecule purification; (ii) weaknesses of ATPS partitioning in regard to intrinsic problems and possible solutions; (iii) opportunities related to biotechnological challenges that ATPS partitioning may solve; and (iv) threats related to alternative techniques that may compete with ATPS in performance, economic benefits, scale up and reliability. This approach provides insight into the current status of ATPS as a bioprocessing technique and it can be concluded that most of the perceived weakness towards industrial implementation have now been largely overcome, thus paving the way for opportunities in fermentation feed clarification, integration in multi-stage operations and in single-step purification processes.

Published
2015

41. Multiplexed capillary microfluidic immunoassay with smartphone data acquisition for parallel mycotoxin detection

Author

Jessica M.D. Machado, Ruben R. G. Soares, Virginia Chu, and João Pedro Conde

Subjects
Ochratoxin A, Aflatoxin B1, Capillary action, Computer science, Microfluidics, Biomedical Engineering, Biophysics, Nanotechnology, 02 engineering and technology, Biosensing Techniques, 01 natural sciences, Multiplexing, chemistry.chemical_compound, Data acquisition, Lab-On-A-Chip Devices, Electrochemistry, medicine, Humans, Mycotoxin, Immunoassay, Chromatography, Animal health, medicine.diagnostic_test, 010401 analytical chemistry, General Medicine, 021001 nanoscience & nanotechnology, Ochratoxins, 0104 chemical sciences, chemistry, Smartphone, 0210 nano-technology, Trichothecenes, Biotechnology
Abstract

The field of microfluidics holds great promise for the development of simple and portable lab-on-a-chip systems. The use of capillarity as a means of fluidic manipulation in lab-on-a-chip systems can potentially reduce the complexity of the instrumentation and allow the development of user-friendly devices for point-of-need analyses. In this work, a PDMS microchannel-based, colorimetric, autonomous capillary chip provides a multiplexed and semi-quantitative immunodetection assay. Results are acquired using a standard smartphone camera and analyzed with a simple gray scale quantification procedure. The performance of this device was tested for the simultaneous detection of the mycotoxins ochratoxin A (OTA), aflatoxin B1 (AFB1) and deoxynivalenol (DON) which are strictly regulated food contaminants with severe detrimental effects on human and animal health. The multiplexed assay was performed approximately within 10min and the achieved sensitivities of

Published
2017

42. A simple method for point-of-need extraction, concentration and rapid multi-mycotoxin immunodetection in feeds using aqueous two-phase systems

Author

Pedro Fernandes, Ana Azevedo, Ruben R. G. Soares, Virginia Chu, João Pedro Conde, and M. Raquel Aires-Barros

Subjects
Ochratoxin A, Aflatoxin, Aflatoxin B1, Animal feed, Food Contamination, 02 engineering and technology, Sodium Citrate, 01 natural sciences, Biochemistry, Zea mays, Analytical Chemistry, Polyethylene Glycols, chemistry.chemical_compound, Vomitoxin, Animals, Sample preparation, Citrates, Mycotoxin, Detection limit, Immunoassay, Chromatography, Chemistry, 010401 analytical chemistry, Organic Chemistry, Extraction (chemistry), food and beverages, General Medicine, Microfluidic Analytical Techniques, 021001 nanoscience & nanotechnology, Animal Feed, Ochratoxins, Cicer, 0104 chemical sciences, Spectrophotometry, Soybeans, 0210 nano-technology, Trichothecenes
Abstract

The rapid detection of mycotoxins in feed samples is becoming an increasingly relevant challenge for the food production sector, in order to effectively enforce current regulations and assure food and feed safety. To achieve rapid mycotoxin detection, several biosensing strategies have been published, many reaching assay times of the order of a few minutes. However, the vast majority of these rely on sample preparation based on volatile organic solvents, often comprising complex multi-step procedures and devoid of clean-up and/or concentration effects. Here, a novel sample preparation methodology based on a green, non-toxic and inexpensive polyethylene glycol-sodium citrate aqueous two-phase system is reported, providing single-step extraction and concentration of three target mycotoxins within 20min: aflatoxin B1 (AFB1), ochratoxin A (OTA) and deoxynivalenol (DON). With point-of-need applications in mind, the extraction procedure was optimized and validated using a rapid multi-toxin microfluidic competitive immunoassay. The assay was successfully tested with spiked complex solid matrices including corn, soy, chickpea and sunflower-based feeds and limits of detection of 4.6ngg-1±15.8%, 24.1ngg-1±8.1% and 129.7ngg-1±53.1% (±CV) were obtained in corn for AFB1, OTA and DON, respectively. These sensitivities are fit-for-purpose at the required regulatory and recommended limits for animal feed, providing an effective and safe semi-quantitative mycotoxin analysis that can be performed in the field.

Published
2017

43. The application of microbeads to microfluidic systems for enhanced detection and purification of biomolecules

Author

Virginia Chu, Ruben R. G. Soares, Ana Azevedo, Inês F. Pinto, João Pedro Conde, Catarina R.F. Caneira, Narayanan Madaboosi, and Maria Raquel Aires-Barros

Subjects
Materials science, Microfluidics, Nanotechnology, 02 engineering and technology, Biosensing Techniques, 01 natural sciences, General Biochemistry, Genetics and Molecular Biology, Antibodies, Molecular recognition, Nucleic Acids, Humans, Dimethylpolysiloxanes, Molecular Biology, Fluorescent Dyes, chemistry.chemical_classification, Biomolecule, 010401 analytical chemistry, Microbead (research), Equipment Design, Microfluidic Analytical Techniques, Mycotoxins, 021001 nanoscience & nanotechnology, Microspheres, 0104 chemical sciences, chemistry, Surface modification, 0210 nano-technology, Biosensor
Abstract

This paper describes microbead-based microfluidic systems. Several aspects of bead assays in microfluidics make them advantageous for bioassays in simple microchannels, including enhanced surface-to-volume ratio, improved molecular recognition reaction efficiency, and the wide range of surface functionalization available with commercial microbeads. Two-level SU-8 molds are used to fabricate PDMS microchannels that can hydrodynamically trap different types of microbeads, with characteristic dimensions of tens of microns. The use of these microbead-based microfluidic systems in the biosensing of antibodies, toxins and nucleic acids, as well as in antibody purification will be presented and discussed in this paper.

Published
2016

44. High-Throughput Nanoliter-Scale Analysis and Optimization of Multimodal Chromatography for the Capture of Monoclonal Antibodies

Author

Ana Azevedo, Sara A.S.L. Rosa, Virginia Chu, Maria Raquel Aires-Barros, João Pedro Conde, Ruben R. G. Soares, and Inês F. Pinto

Subjects
medicine.drug_class, Microfluidics, 02 engineering and technology, Monoclonal antibody, Ligands, 01 natural sciences, Analytical Chemistry, High-Throughput Screening Assays, medicine, Fluorescence microscope, Molecule, Dimethylpolysiloxanes, Particle Size, Chromatography, Molecular Structure, Chemistry, Ligand, 010401 analytical chemistry, Antibodies, Monoclonal, Microfluidic Analytical Techniques, 021001 nanoscience & nanotechnology, 0104 chemical sciences, Reagent, Yield (chemistry), Adsorption, 0210 nano-technology
Abstract

Multimodal ligands are synthetic molecules comprising multiple types of interactions that have been increasingly used for the capture of different biopharmaceutical compounds within complex biological mixtures. For monoclonal antibodies (mAbs) in particular, these ligands have shown the possibility of direct capture from cell culture supernatants in native conditions, as well as enhanced selectivity and affinity compared to traditional single-mode ligands. However, performing the capture of a target mAb using multimodal chromatography comes with the need for extensive optimization of the operating conditions, due to the multitude of interactions that can be promoted in parallel. In this work, a high-throughput microfluidic platform was developed for the optimization of chromatographic conditions regarding the capture of an anti-interleukin 8 mAb, using a multimodal ligand (2-benzamido-4-mercaptobutanoic acid), under a wide range of buffer pH and conductivities. The interaction of the ligand with the fluorescently labeled target mAb was also analyzed with respect to the individual contribution of the hydrophobic (phenyl) and electrostatic (carboxyl) moieties using fluorescence microscopy. The results were further validated at the macroscale using prepacked columns in standard chromatography assays, and recovery yield values of 94.6% ± 5.2% and 97.7% ± 1.5% were obtained under optimal conditions for the miniaturized and conventional approaches, respectively. In summary, this study highlights that a microfluidic-based approach is a powerful analytical tool to expedite the optimization process while using reduced reagent volumes (

Published
2016

45. 'Bio-functionalization study of Memristive-Biosensors for early detection of prostate cancer'

Author

Sandro Carrara, V. Chu, João Pedro Conde, G. De Micheli, N. Madaboosi, Ioulia Tzouvadaki, and Ruben R. G. Soares

Subjects
chemistry.chemical_classification, Materials science, Nanostructure, chemistry, Biomolecule, Femto, technology, industry, and agriculture, Early detection, Surface modification, Nanotechnology, Silicon nanowires, Biosensor
Abstract

Silicon nanowires are reported for their application in bio sensing area and their potential in the detection of various biomolecules. In the present work, freestanding two-terminal Schottky-barrier silicon nanowire arrays exhibiting memristive behavior are fabricated to obtain Memristive-Biosensors. Scanning electron microscopy reveal details on the morphology of the fabricated structures. The memristive devices are functionalized with anti-free-Prostate Specific Antigen (PSA) antibody by two strategies: a) direct passive adsorption on the device surface, and b) bio-affinity approach using Biotin-Streptavidin combination. The electrical behavior of the so-obtained Memristive-Biosensors is examined dealing with the two systems of bio-functionalization. The presence of biomolecules linked to the surface of the nanostructures is detected by a voltage gap appearing in the memristive electrical characteristics. The system shows the potential for applications in molecular diagnostics especially due to possibilities for detection in the femto molar ranges that allow early detection of the cancer disease.

Published
2015

46. Performance of hydrogenated amorphous silicon thin film photosensors at ultra-low light levels: towards attomole sensitivities in labon- chip biosensing applications

Author

Ruben R. G. Soares, Denis R. Santos, Virginia Chu, and João Pedro Conde

Subjects
Photomultiplier, Materials science, business.industry, 010401 analytical chemistry, Photodetector, 02 engineering and technology, Lab-on-a-chip, 021001 nanoscience & nanotechnology, 01 natural sciences, 0104 chemical sciences, law.invention, Photodiode, Light intensity, law, Miniaturization, Optoelectronics, Crystalline silicon, Electrical and Electronic Engineering, 0210 nano-technology, business, Instrumentation, Dark current
Abstract

Thin-film optical transducers integrated in lab-on-a-chip (LoC) devices have the potential to facilitate miniaturization, multiplexing capabilities, portability, and sensitivity. However, there are few systematic studies that provide detailed characterization of these photosensors to particular miniaturized bioassays at reduced light intensities. A more detailed representation of the photosensors performance at low light levels is thus needed in order to improve the engineering of integrated detectors for the next generation of portable biosensors. Here, an assessment of the performance of hydrogenated amorphous silicon (a-Si:H) photosensors, at ultra-low light intensity, based on two different device configurations for integration in a microfluidic platform for biomolecular detection is presented. Both p-i-n photodiodes and parallel contact photoconductors show low dark current density (~10−10 A.cm−2) and photosensitivity comparable with high performing crystalline silicon photosensors. The a-Si:H photosensors were integrated in microfluidic devices for the detection of antibody-horseradish peroxidase conjugates (Ab-HRP) in a chemiluminescence-based assay. Surface concentrations of Ab-HRP as low as ~26 amol.cm−2 and ~9 fmol.cm−2 (corresponding to ~103 and ~106 HRP molecules) were detected with detectors in photodiode and photoconductor configurations, respectively, with the sensitivity of the former being comparable with that of bulky and ultra-sensitive photomultiplier tubes. The excellent sensitivity and dynamic range obtained, together with the miniaturization and arraying potential, highlight the potential of a-Si:H photosensors as an effective means of integrating the multiplexed acquisition of optical data in real time in point-of-need LoC systems.

Published
2017

48. On-chip sample preparation and analyte quantification using a microfluidic aqueous two-phase extraction coupled with an immunoassay

Author

Maria Raquel Aires-Barros, Pedro Fernandes, Virginia Chu, Ruben R. G. Soares, João Pedro Conde, P. Novo, and Ana Azevedo

Subjects
Detection limit, Wine, Analyte, Materials science, Chromatography, medicine.diagnostic_test, Extraction (chemistry), Liquid-Liquid Extraction, Biomedical Engineering, Fluorescent Antibody Technique, Bioengineering, General Chemistry, Equipment Design, Microfluidic Analytical Techniques, Biochemistry, Ochratoxins, Matrix (chemical analysis), Models, Chemical, Limit of Detection, Immunoassay, medicine, media_common.cataloged_instance, Sample preparation, European union, media_common
Abstract

Immunoassays are fast and sensitive techniques for analyte quantification, and their use in point-of-care devices for medical, environmental, and food safety applications has potential benefits of cost, portability, and multiplexing. However, immunoassays are often affected by matrix interference effects, requiring the use of complex laboratory extraction and concentration procedures in order to achieve the required sensitivity. In this paper we propose an integrated microfluidic device for the simultaneous matrix clean-up, concentration and detection. This device consists of two modules in series, the first performing an aqueous two-phase extraction (ATPE) for matrix extraction and analyte pre-concentration, and the second an immunoassay for quantification. The model analyte was the mycotoxin ochratoxin A (OTA) in a wine matrix. Using this strategy, a limit of detection (LoD) of 0.26 ng mL(-1) was obtained for red wine spiked with OTA, well below the regulatory limit for OTA in wines of 2 ng mL(-1) set by the European Union. Furthermore, the linear response on the logarithmic concentration scale was observed to span 3 orders of magnitude (0.1-100 ng mL(-1)). These results are comparable to those obtained for the quantification of OTA in plain buffer without an integrated ATPE (LoD = 0.15 ng mL(-1)). The proposed method was also found to provide similar results for markedly different matrices, such as red and white wines. This novel approach based on aqueous two-phase systems can help the development of point-of-care devices that can directly deal with real samples in complex matrices without the need for extra extraction processes and equipment.

Published
2014

49. Aqueous two-phase systems for enhancing immunoassay sensitivity: simultaneous concentration of mycotoxins and neutralization of matrix interference

Author

P. Novo, Ruben R. G. Soares, Pedro Fernandes, Virginia Chu, Ana Azevedo, Maria Raquel Aires-Barros, and João Pedro Conde

Subjects
Ochratoxin A, Aflatoxin, Analyte, Chromatography, Aqueous solution, Aflatoxin B1, medicine.diagnostic_test, Organic Chemistry, Aqueous two-phase system, food and beverages, Beer, Enzyme-Linked Immunosorbent Assay, Wine, General Medicine, Polyethylene glycol, Hydrogen-Ion Concentration, Biochemistry, Ochratoxins, Analytical Chemistry, Matrix (chemical analysis), chemistry.chemical_compound, chemistry, Limit of Detection, Immunoassay, medicine
Abstract

Immunoassays have a broad application range, from environmental and food toxicology to biomedical analysis, providing rapid and simple methods for analyte quantification. Immunoassays, however, are often challenging at nM and sub nM concentrations and are affected by detrimental matrix interference effects, as is the case of the detection of ochratoxin A (OTA) and Aflatoxin B1 (AFB1). These are widespread mycotoxins found in food and feed, with serious potential implications for human health. This work demonstrates the use of polymer–salt aqueous two phase systems (ATPSs) for the simultaneous concentration of mycotoxins and neutralization of matrix interference. In particular, polyethylene glycol (PEG)-phosphate salt ATPSs were used to enhance the detection sensitivity of OTA and AFB1 in wines and beer by an indirect competitive ELISA. Using this methodology it was possible to quantify both analytes spiked in red wine with limits-of-detection (LoD) down to 0.19 ng/mL and 0.035 ng/mL, respectively, with results comparable to those obtained using solutions of toxins in phosphate buffered saline (PBS) buffer (0.7 ng/mL and 0.009 ng/mL, respectively). Furthermore, a very low matrix-to matrix variability was observed, with LoD and half inhibitory concentration (IC50) values of 5.17 ± 1.08 and 33.2 ± 3.5 ng/mL (±SD) obtained in the detection of OTA spiked in red and white wines, beer or PBS buffer. These results indicate the potential of ATPS as a fast and simple concentration step and in providing matrix-independent analyte quantification for enhanced immunoassay sensitivity below regulatory levels.

Published
2014

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