RESUMO
The efficient development of selective materials for uranium recovery from wastewater and seawater is crucial for the utilization of uranium resources and environmental protection. The potential of graphene oxide (GO) as an effective adsorbent for the removal of environmental contaminants has been extensively investigated. Further modification of the functional groups on the basal surface of GO can significantly enhance its adsorption performance. In this study, a novel poly(amidoxime-hydroxamic acid) functionalized graphene oxide (pAHA-GO) was synthesized via free radical polymerization followed by an oximation reaction, aiming to enhance its adsorption efficiency for U(VI). A variety of characterization techniques, including SEM, Raman spectroscopy, FT-IR, and XPS, were employed to demonstrate the successful decoration of amidoxime and hydroxamic acid functional groups onto GO. Meanwhile, the adsorption of U(VI) on pAHA-GO was studied as a function of contact time, adsorbent dosage, pH, ionic strength, initial U(VI) concentration, and interfering ions by batch-type experiments. The results indicated that the pAHA-GO exhibited excellent reuse capability, high stability, and anti-interference ability. Specially, the U(VI) adsorption reactions were consistent with pseudo-second-order and Langmuir isothermal adsorption models. The maximum U(VI) adsorption capacity was evaluated to be 178.7 mg/g at pH 3.6, displaying a higher U(VI) removal efficiency compared with other GO-based adsorbents in similar conditions. Regeneration of pAHA-GO did not significantly influence the adsorption towards U(VI) for up to four sequential cycles. In addition, pAHA-GO demonstrated good adsorption capacity stability when it was immersed in HNO3 solution at different concentrations (0.1-1.0 mol/L) for 72 h. pAHA-GO was also found to have anti-interference ability for U(VI) adsorption in seawater with high salt content at near-neutral pH condition. In simulated seawater, the adsorption efficiency was above 94% for U(VI) across various initial concentrations. The comprehensive characterization results demonstrated the involvement of oxygen- and nitrogen-containing functional groups in pAHA-GO in the adsorption process of U(VI). Overall, these findings demonstrate the feasibility of the pAHA-GO composite used for the capture of U(VI) from aqueous solutions.
Assuntos
Grafite , Oximas , Urânio , Urânio/análise , Espectroscopia de Infravermelho com Transformada de Fourier , Água , Adsorção , CinéticaRESUMO
Multinuclear U(VI) species may be dominant in aqueous solutions under environmental conditions, while the structures of the multinuclear U(VI) species on mineral surfaces remain unclear. This work reports the structural and bonding properties of the possible surface complexes of three aqueous multinuclear U(VI) species, i.e., (UO2)2(OH)3+, (UO2)2(OH)22+ and (UO2)3(O)(OH)3+, on the hydroxylated α-SiO2(001) surface based on density functional theory (DFT) calculations. The results show that (UO2)2(OH)22+ and (UO2)3(O)(OH)3+ tend to form end-on structures at îSiO(H)SiO(H) sites, whereas (UO2)2(OH)3+ prefers a side-on structure at îSiO(H)O(H)-SiO(H)O(H) sites. The main driving forces for the formation of the multinuclear U(VI) surface complexes are electrostatic interactions and partially covalent chemical bonds. The Os-2p orbital hybridizes strongly with U-5f and U-6d orbitals, with a decreasing binding strength in the sequence of (UO2)2(OH)3+ > (UO2)2(OH)22+ > (UO2)3(O)(OH)3+ for the adsorption at the same type of surface sites. For the adsorption of the same multinuclear U(VI) species, the binding energy increases with the deprotonation extent of the identical sites. In addition, hydrogen bonds between surface hydroxyls and coordination waters as well as the acyl oxygen of uranyl moieties contribute to the formation of the multinuclear U(VI) surface complexes. The U-5f electron delocalization of far-side U atoms in the end-on structures of (UO2)2(OH)22+ and (UO2)3(O)(OH)3+ surface complexes also contributes slightly to the overall binding energy. Overall, this study provides insights into the adsorption behavior of multinuclear U(VI) on silica.
RESUMO
To tune the complexation and solvent extraction performance of the ligands with a 1,10-phenanthroline core for trivalent actinides (An3+) and lanthanides (Ln3+), we synthesized two new asymmetric tetradentate ligands with pyrazole and amide groups, i.e., L1 (N,N-diethyl-9-(5-ethyl-1H-pyrazol-3-yl)-1,10-phenanthroline-2-carboxamide) and its analogue L2 with longer alkyl chains (N,N-dihexyl). The complexation of the ligands with Ln3+ was confirmed by 1H NMR titration and X-ray crystallography, and stability constants were measured in methanol by spectrophotometric titration. The asymmetric ligands exhibited an improved performance in terms of selective solvent extraction of Am3+ over Eu3+ in strongly acidic solutions compared to their symmetric analogues. The improved selectivity of the asymmetric ligands was interpreted theoretically by density functional theory simulations. This study implies that combining different functional groups to construct asymmetric ligands may be an efficient way to tune ligand performance with regard to An3+ separation from Ln3+.
RESUMO
High room-temperature ionic conductivities, large Li+ -ion transference numbers, and good compatibility with both Li-metal anodes and high-voltage cathodes of the solid electrolytes are the essential requirements for practical solid-state lithium-metal batteries. Herein, a unique "superconcentrated ionogel-in-ceramic" (SIC) electrolyte prepared by an in situ thermally initiated radical polymerization is reported. Solid-state static 7 Li NMR and molecular dynamics simulation reveal the roles of ceramic in Li+ local environments and transport in the SIC electrolyte. The SIC electrolyte not only exhibits an ultrahigh ionic conductivity of 1.33 × 10-3 S cm-1 at 25 °C, but also a Li+ -ion transference number as high as 0.89, together with a low electronic conductivity of 3.14 × 10-10 S cm-1 and a wide electrochemical stability window of 5.5 V versus Li/Li+ . Applications of the SIC electrolyte in Li||LiNi0.5 Co0.2 Mn0.3 O2 and Li||LiFePO4 batteries further demonstrate the high rate and long cycle life. This study, therefore, provides a promising hybrid electrolyte for safe and high-energy lithium-metal batteries.
RESUMO
Dissolved silicic acid in the environment has strong affinity for actinides (An), but An(III)-silicate colloids have been scarcely investigated. In this study, Eu(III)-silicate colloids, an analogue to An(III)-silicate, were prepared and the aggregation kinetics of the colloids was investigated as a function of Eu content (Si/Eu molar ratio), pH, background electrolyte (NaCl, NaNO3, NaClO4, KCl and CsCl) and fulvic acid (FA). Results indicated that the colloids with higher Si/Eu molar ratio exhibited higher stability under the same conditions. The stability of the colloids increased with increasing aqueous pH (7.1-9.4) and decreasing ionic strength, and the inhibition effect of monovalent electrolytes on the colloid stability followed the order of Na+ < K+ < Cs+ and Cl- < NO3- < ClO4-. In addition, the presence of FA significantly increased the stability of the colloids. The dependence of the stability on the chemical conditions in all cases could be illustrated by DLVO theory. Disaggregation kinetics showed that the aggregation process of the colloids was not fully reversible, because a time-dependent size memory effect led to a bigger mean size of disaggregated colloids as compared to the initial ones. The present work provides detailed insight in the formation and stability of An(III)-silicate colloids under the alkaline conditions relevant to geological disposal of radioactive waste, which is critical for understanding the behavior of this type of colloids in the environment.
RESUMO
Biochar has attracted much attention for remediating the sites contaminated with heavy metals and radionuclides due to its low cost and high adsorption affinity. However, little is known about how colloidal biochar influences U(VI) transport in the environment. In this study, column experiments were conducted to investigate the individual and co-transport of U(VI) and biochar colloids (BC) in quartz sand heterogeneous media. Results showed that the transport of U(VI) in the individual transport system was pH-dependent and insensitive to ionic strength, whereas the individual BC transport was more sensitive to the changes in ionic strength compared to those in pH, indicating that electrostatic interaction plays a major role during BC transport but chemical interaction dominates U(VI) transport. In the presence of BC, the transport of U(VI) was significantly facilitated because of U(VI) adsorption on BC. The existence of low concentration of U(VI) (2.5 × 10-6 M), however, did not affect the breakthrough curves (BTCs) of BC, except for the co-transport at relatively high ionic strength (100 mM) where BC transport was impeded due to the decrease of colloid suspension stability. Colloid size exclusion effect was evidenced by the evolution of particle size and zeta potential of the effluents. The transport of BC in both the individual and co-transport systems could be described by a two-site kinetic attachment/detachment model. This work implies that a risk assessment of BC facilitated heavy metal transport should be carefully considered when biochar is applied to the remediation of heavy metal contaminated sites.
Assuntos
Quartzo , Areia , Adsorção , Carvão Vegetal , Coloides , PorosidadeRESUMO
For the geological repository of high-level radioactive waste (HLW) built in granitic host rockï¼the control of buffer material (compacted bentonite) erosion and subsequent loss caused by groundwater in granite fissures is an unresolved problem of major concern. We propose here new insight into enhancing the erosion resistance of compacted bentonite by means of its electrostatic interaction with oppositely-charged layered double hydroxide (LDH). The interaction between bentonite and LDH was studied by dropwise addition of colloidal LDH into colloidal bentonite suspension, during which the variation in electrical conductivity, zeta potential and particle size proved a strong interaction between these two materials. Interestingly, in addition to their aggregation, intercalated structures of LDH and montmorillonite were found in the composite (BEN@LDH) by a combined characterization of X-ray diffraction (XRD) and high resolution transmission electron microscopy (HR-TEM), and were confirmed by density functional theory (DFT) calculation. Colloid generation of compacted BEN@LDH under ultrasonic conditions is negligible comparing with that of compacted bentonite, indicating a significantly higher erosion resistance. Besides, a small amount of LDH by mechanically mixing with bentonite (mass ratio 1:99) can also effectively improve the erosion resistance of compacted bentonite. Moreover, BEN@LDH displayed stronger retention performance towards U(VI) and Se(IV) than bentonite under near-neutral/weakly alkaline conditions. Our results indicate that LDH is a promising additive in compacted bentonite, and this approach may be extended to common geotechnical structures built with clays and soils.
Assuntos
Bentonita , Resíduos Radioativos , Argila , Hidróxidos , Resíduos Radioativos/análise , Eletricidade EstáticaRESUMO
Understanding the in-situ transport behavior of U(VI) in granitic formations is of considerable interest for geological disposal of high-level radioactive wastes (HLW). In this context, the co-transport of U(VI) and representative naturally-occurring colloids, i.e., humic acid (HA) and gibbsite colloid (GC), was studied in granite column as a function of pH, U(VI) concentration and HA amount. It was found that, in addition to pH, co-transport of U(VI) and GC was also controlled by U(VI) concentration, the effect of which can be transport-facilitating and transport-impeding for U(VI) at relatively low concentration (2.0â¯×â¯10-6â¯mol/L) and for U(VI) at high concentration (5.0â¯×â¯10-5â¯mol/L), respectively. HA can present opposite effects on GC transport depending on HA amount. The transport-impeding effect by small amount of HA (5â¯mg/L) is due to strong aggregation between GC and HA from electrostatic attraction and complexation, whereas the transport-facilitating effect by big amount of HA (20â¯mg/L) is because of the complete HA coating which stabilizes associated colloids and alters surface charge from positive to negative. In ternary co-transport systems, a similar HA-dependent effect was also observed for both U(VI) and GC regardless of presence of high concentration U(VI). Besides the application of the Derjaguin-Landau-Verwey-Overbeek (DLVO) theory, the mechanisms behind binary and ternary co-transport of U(VI), GC and HA were also analyzed by assessing the evolutions of zeta potential and particle size in the column effluents. Finally, a two-site non-equilibrium model and a two-site kinetic attachment/detachment model were applied to describe the breakthrough curves of U(VI) and individual/combined colloids, respectively. The findings of this study indicated that combined effects of GC and HA on radionuclides transport is dominated by the amount of HA, and a facilitating transport of radionuclide can be expected in the underground environment rich in humic acid.
RESUMO
The release of uranyl from uranium tailing sites is a widely concerned environmental issue, with limited investigations on the effect of coexistence of various colloids. Gibbsite colloids extensively exist, together with ubiquitous humic substances, in uranium polluted waters at tailing sites, due to high concentration of dissolved Al in acid mine drainage. In this context, we investigated the co-transport of U(VI), gibbsite colloids and humic acid (HA) as a function of pH and ionic strength at a U(VI) concentration (5.0â¯×â¯10-5â¯M) relevant within mine tailings and related waste. It was found that, owing to electrostatic attraction, gibbsite colloids and HA associated with each other and transported simultaneously regardless of U(VI) presence. Besides the impact of pH and ionic strength, whether gibbsite colloids facilitated U(VI) transport depended on HA concentration. Gibbsite colloids impeded U(VI) transport at relatively low HA concentration (≤5â¯mgâ¯L-1), because associated colloids loaded with U(VI) were positively charged which favored colloid retention on negatively charged quartz sand in the column. U(VI) together with gibbsite colloids and low concentration HA was completely blocked at natural pH and/or high ionic strength. At relatively high HA concentration (20â¯mgâ¯L-1), however, the associated colloids showed negative zeta potential which facilitated U(VI) transport because of repulsion between negatively charged colloids and quartz sand. Meanwhile, high concentration of HA dramatically accelerated the transport of gibbsite colloids. These results implied that gibbsite colloids might imped U(VI) migration at uranium tailing sites unless the aquifers are enriched with abundant humic substances.
Assuntos
Coloides/química , Substâncias Húmicas/análise , Modelos Químicos , Urânio/química , Poluentes Radioativos da Água/química , Adsorção , Água Subterrânea/química , Concentração Osmolar , Porosidade , Quartzo , Dióxido de Silício , Simportadores , Urânio/análise , ÁguaRESUMO
Remediating uranium contamination becomes a worldwide interest because of increasing uranium release from mining activities. Due to ubiquitous presence of pyrite and the application of iron-based technology, colloidal iron oxy-hydroxides such as akaganéite colloid (AKC) extensively exist in uranium polluted water at uranium tailing sites. In this context, we studied individual and co-transport of U(VI) and AKC in water-saturated sand columns at 50â¯mg/L AKC and environmentally relevant U(VI) concentrations (5.0â¯×â¯10-7 â¼ 5.0â¯×â¯10-5â¯M). It was found that, in addition to the impact of pH and ionic strength, whether AKC facilitated U(VI) transport depended on U(VI) concentration as well. The presence of AKC facilitated U(VI) transport at relatively low U(VI) concentration (5.0â¯×â¯10-7 â¼ 5.0â¯×â¯10-6â¯M), which was due to the strong adsorption of U(VI) on AKC and faster transport of AKC than that U(VI) as observed in their individual transport experiments. At relatively high U(VI) concentrations (5.0â¯×â¯10-5â¯M), however, AKC impeded U(VI) transport because U(VI) of high concentration decreased AKC colloidal stability and increased AKC aggregation and attachment. Thus, U(VI) and AKC co-transport was even blocked completely at relatively high pH and ionic strength. The mechanisms behind the co-transport of U(VI) and AKC were also confirmed by assessing the evolutions of aqueous pH and AKC zeta potential and particle size distribution in the column effluents. A two-site non-equilibrium model and a two-site kinetic attachment/detachment model well-described the breakthrough curves of U(VI) and AKC, respectively. Knowledge generated from this study provides a thorough understanding of uranium transport in the absence/presence of AKC, and brings new insights into the influence of contaminant concentration on co-transport in the presence of colloids.
Assuntos
Urânio , Água , Adsorção , Coloides , Compostos Férricos , Concentração de Íons de Hidrogênio , Concentração Osmolar , PorosidadeRESUMO
A microfluidic system consisting of generic single use cartridges which interface with a workstation allows the automatic performance of all necessary sample preparation, PCR analysis and interpretation of multiplex PCR assays. The cartridges contain a DNA array with 20 different 16mer DNA "universal" probes immobilized at defined locations. PCR amplicons can be detected via hybridization of user-defined "reporter" probes that are complementary at their 3' termini to one or more of the universal probes and complementary to the target amplicons at their 5' termini. The system was able to detect single-plex and multiplex PCR amplicons from various infectious agents as well as wild type and mutant alleles of single nucleotide polymorphisms. The system's ease of use was further demonstrated by converting a published PCR assay for the detection of Mycobacterium genitalium in a fully automated manner. Excellent correlation between traditional manual methods and the automated analysis performed by the workstation suggests that the system can provide a means to easily design and implement a variety of customized PCR-based assays. The system will be useful to researchers or clinical investigators seeking to develop their own user defined assays. As the U.S. FDA continues to pursue regulatory oversight of LDTs, the system would also allow labs to continue to develop compliant assays.
RESUMO
OBJECTIVE: We developed a microfluidic system to simultaneously detect host anti-HIV antibodies and viral RNA in the same specimen in order to satisfy two important diagnostic criteria, especially within resource-limited settings. First, the system can detect acute HIV infection and allow immediate confirmation of a seropositive screening result by detection of HIV RNA. It also addresses the well-known "seroconversion window" during early HIV infection when antibodies are not yet detectable and viral loads are at their highest. METHODS: We first developed and optimized two separate manual assays for the detection of host anti-HIV antibodies and viral RNA and then converted them to the microfluidic system. We optimized a commercially available serologic assay to run within the microfluidic device while we incorporated the isothermal LAMP assay to detect the presence of viral RNA. The microfluidic device and instrumentation were developed to simultaneously perform both assays without any user intervention. RESULTS: The finalized system consists of a disposable injection molded and film-laminated microfluidic CARD disposable device and a portable, software controlled instrument, which together can automatically perform all steps of both assays without any user intervention after the initial loading of samples and reagents. The microfluidic CARD cartridge has multiple microchannels, valves, pumps and reservoirs, which perform the immunoassay, isolates viral RNA for detection by magnetic bead based purification, and Reverse Transcriptase loop-mediated isothermal amplification (RT-LAMP). The microfluidic system was able to detect host anti-HIV antibodies and viral RNA in either a blood or saliva sample. CONCLUSION: The ability to detect antibodies and simultaneously confirm a seropositive HIV-RNA result provides healthcare workers with a complete and accurate appraisal of a patient's infection status in the earliest stages of the disease and represents an important tool for the "Test and Treat" and "Treatment as Prevention" approaches for controlling the HIV epidemic.
RESUMO
CONTEXT: Although the value of pharmacogenomics to improve patient outcomes has become increasingly clear, adoption in medical practice has been slow, which can be attributed to several factors, including complicated and expensive testing procedures and required equipment, lack of training by private practice physicians, and reluctance of both private and commercial payers to reimburse for such testing. OBJECTIVES: To evaluate a fully automated molecular detection system for human genotyping assays, starting with anticoagulated whole blood samples, and to perform all sample preparation, assay, and analysis steps automatically with actionable results reported by the system's software. DESIGN: The genotypes of 254 random individuals were determined by performing bidirectional DNA sequencing, and that information was used to statistically train the imaging software of the automated molecular detection system to distinguish the 3 possible genotypes (ie, homozygous wild type, heterozygous, and homozygous mutant) at each of 3 different loci (CYP2C9*2, CYP2C9*3, and VKORC1). RESULTS: The resulting software algorithm was able to correctly identify the genotypes of all 254 individuals (100%) evaluated without any further user analysis. CONCLUSIONS: The EncompassMDx workstation (Rheonix, Inc, Ithaca, New York) is a molecular detection system that can automatically determine the genotypes of individuals in an unattended manner. Considerably less technical expertise was required to achieve results identical to those obtained using more complex, time-consuming, and expensive bidirectional DNA sequencing. This optimized system may dramatically simplify and reduce the costs of pharmacogenomics testing, thus leading to more-widespread use.
Assuntos
Técnicas de Genotipagem/instrumentação , Técnicas de Genotipagem/métodos , Reação em Cadeia da Polimerase/métodos , Polimorfismo de Nucleotídeo Único , Análise de Sequência de DNA/métodos , Citocromo P-450 CYP2C9/genética , Genótipo , Humanos , Isoenzimas/genética , Reprodutibilidade dos Testes , Software , Vitamina K Epóxido Redutases/genéticaRESUMO
A prototype dual-path microfluidic device (Rheonix CARD) capable of performing simultaneously screening (antigen or antibody) and confirmatory (nucleic acid) detection of pathogens is described. The device fully integrates sample processing, antigen or antibody detection, and nucleic acid amplification and detection, demonstrating rapid and inexpensive "sample-to-result" diagnosis with performance comparable to benchtop analysis. For the chip design, a modular approach was followed allowing the optimization of individual steps in the sample processing process. This modular design provides great versatility accommodating different disease targets independently of the production method. In the detection module, a lateral flow (LF) protocol utilizing upconverting phosphor (UCP) reporters was employed. The nucleic acid (NA) module incorporates a generic microtube containing dry reagents. Lateral flow strips and PCR primers determine the target or disease that is diagnosed. Diagnosis of HIV infection was used as a model to investigate the simultaneous detection of both human antibodies against the virus and viral RNA. The serological result is available in less than 30 min, and the confirmation by RNA amplification takes another 60 min. This approach combines a core serological portable diagnostic with a nucleic acid-based confirmatory test.
Assuntos
Anticorpos/análise , Técnicas Analíticas Microfluídicas/instrumentação , Ácidos Nucleicos/análise , Saliva/metabolismo , Anticorpos/química , Anticorpos Antivirais/análise , Desenho de Equipamento , Infecções por HIV/diagnóstico , Humanos , Fósforo/química , Reação em Cadeia da Polimerase , RNA Viral/análiseRESUMO
A versatile microfluidic platform for the evolving molecular diagnostics industry is described. It incorporates low cost Rheonix CARD(®) (Chemistry and Reagent Device) technology to analyze a variety of clinical specimens. A patented lamination process incorporates all pumps, valves, microchannels and reaction compartments into an inexpensive disposable plastic device. Once an untreated clinical specimen is introduced, all assay steps, including cell lysis, nucleic acid purification, multiplex PCR, and end-point analysis, are automatically performed. Three distinct CARD assays are described which utilize either a low density microarray for multiplex detection of amplicons or an integrated primer extension assay to detect single nucleotide polymorphisms of interest. The STI (Sexually Transmitted Infections) CARD(®) is able to simultaneously detect four sexually transmitted infectious agents (N. gonorrhoeae, C.trachomatis, T. pallidum and T. vaginalis). Human C33A cervical epithelial cells were spiked with different levels of genomic DNA from the four species of interest, singly or in combination, and applied to the CARD device. Using multiplex PCR amplification of the targets followed by microarray detection, the CARD device was able to correctly detect a minimum of 10 copies of each of the four pathogens. The HPV (Human Papillomavirus) CARD(®) was able to detect and distinguish 20 different clinically relevant HPV types using cloned HPV DNA. In addition, the HPV CARD could identify HPV types in vaginal specimens previously demonstrated to contain high or low risk HPV using a currently commercially available testing method. Finally, the detection of specific single nucleotide polymorphisms (SNP) associated with warfarin dosing sensitivity was achieved on the Warfarin Genotyping CARD(®) by analyzing human buccal swabs. Once multiplex PCR was completed, the SNPs were detected using a primer extension assay.
RESUMO
Using polystyrene as a fabrication material and pure acetonitrile as a bonding solvent, we have developed an innovative and inexpensive weak-solvent-based chip lamination process to produce highly functional, completely plastic, microfluidic chips with a 3-layer structure. This simple, scalable and rapid method allows active components, such as multiple valves and pumps, to be constructed on chip with a thin, deflectable film as the middle layer sandwiched between two polystyrene layers. Our irreversible bonding method achieves uniform lamination under mild conditions (35-45 degrees C and 10-50 KPa) without damage to the underlying micro-features. The on-chip valve and pump structures have been systematically characterized and the pumping rate has been compared against theoretical rates predicted by mathematical modeling studies. A wide range of pumping rates (0.33-10 microL/s) can be achieved, with the integral pumps maintaining a constant pumping rate and depending on pumping frequency and pump diaphragm size. Valve leakage of less than 0.02 microL/min is noted under pressures of 41 kPa. Utilizing various configurations of on-chip valves and pumps, the fully automated flow control of an integrated chip for sample lysis, nucleic acid purification and PCR is demonstrated. The present technology and chip have been heavily evaluated internally and externally for rapid biomedical diagnosis of HPV, HIV, etc., and they are currently in the process of commercialization.
Assuntos
Acetonitrilas/química , Técnicas Analíticas Microfluídicas/instrumentação , Microtecnologia/métodos , Solventes/química , Desenho de Equipamento , Poliestirenos/químicaRESUMO
The building blocks for an inexpensive, disposable, luminescence-based microfluidic immunoassay cassette are described, and their integration in a point-of-care diagnostic system is demonstrated. Fluid motion in the cassette is driven by depressing finger-actuated pouches. All reagents needed for the immunoassay can be stored in the cassette in liquid form. Prior to use, the cassette consists of two separate parts. A top storage component contains pouches, sealed storage chambers, a metering chamber, and needle seats. The bottom processing component contains connection needles, a mixing chamber, and a detection chamber with immobilized proteins. Subsequent to sample introduction, the storage and processing components are mated. The needles form hydraulic connections between the two parts and, in some cases, close valves. The pouches are then actuated sequentially to induce flow of various reagents and facilitate process operations. The cassette is compatible with different detection modalities. Both a cassette with immunochromatographic-based detection and a cassette with microbead-based detection were constructed and evaluated. The immunochromatographic cassette was used to detect antibodies to HIV in saliva samples. The bead-based cassette was used to detect the proinflammatory chemokine IL-8. The experimental data demonstrates good repeatability and reasonable sensitivity.
Assuntos
Imunoensaio/instrumentação , Microfluídica/métodos , Cromatografia , Interleucina-8/análise , Microesferas , AgulhasRESUMO
An inexpensive, hand-held, point-of-care, disposable, self-contained immunoassay cassette comprised of air pouches for pumping, a metering chamber, reagents storage chambers, a mixer, and a lateral flow strip was designed, constructed, and tested. The assay was carried out in a consecutive flow format. The detection was facilitated with up-converting phosphor (UCP) reporter particles. The automated, timely pumping of the various reagents was driven by a spring-loaded timer. The utility of the cassette was demonstrated by detecting antibodies to HIV in saliva samples and further evaluated with a non-contagious, haptenized DNA assay. The cassette has several advantages over dip sticks such as sample preprocessing, integrated storage of reagents, and automated operation that reduces operator errors and training. The cassette and actuator described herein can readily be extended to detect biomarkers of other diseases in body fluids and other fluids at the point of care. The system is particularly suitable for resource-poor countries, where funds and trained personnel are in short supply.
Assuntos
Biomarcadores/química , Infecções por HIV/diagnóstico , Imunoensaio/instrumentação , Kit de Reagentes para Diagnóstico , Saliva/química , Humanos , Imunoensaio/economia , Imunoensaio/métodosRESUMO
Oral squamous cell carcinoma (OSCC) is a disfiguring and deadly cancer. Despite advances in therapy, many patients continue to face a poor prognosis. Early detection is an important factor in determining the survival of patients with OSCC. No accurate, cost-efficient, and reproducible method exists to screen patients for OSCC. As a result, many patients are diagnosed at advanced stages of the disease. Early detection would identify patients, facilitating timely treatment and close monitoring. Mass screening requires a rapid oral cancer diagnostic test that can be used in a clinical setting. Current diagnostic techniques for OSCC require modern laboratory facilities, sophisticated equipment, and elaborate and lengthy processing by skilled personnel. The lab-on-chip technology holds the promise of replacing these techniques with miniaturized, integrated, automated, inexpensive diagnostic devices. This article describes lab-on-chip devices for biomarker-based identification of oral cancer. Similar methods can be employed for the screening of other types of cancers.
Assuntos
Carcinoma de Células Escamosas/diagnóstico , Programas de Rastreamento/instrumentação , Técnicas Analíticas Microfluídicas , Neoplasias Bucais/diagnóstico , Antígenos de Neoplasias/metabolismo , Biomarcadores Tumorais , Carcinoma de Células Escamosas/genética , Carcinoma de Células Escamosas/metabolismo , Proteínas de Transporte/metabolismo , Moléculas de Adesão Celular/metabolismo , Molécula de Adesão da Célula Epitelial , Perfilação da Expressão Gênica , Glicoproteínas , Humanos , Programas de Rastreamento/métodos , Neoplasias Bucais/genética , Neoplasias Bucais/metabolismo , RNA Mensageiro/metabolismo , Reação em Cadeia da Polimerase Via Transcriptase Reversa , Software , Transcrição GênicaRESUMO
Confirmatory detection of diseases, such as HIV and HIV-associated pathogens in a rapid point-of-care (POC) diagnostic remains a goal for disease control, prevention, and therapy. If a sample could be analyzed onsite with a verified result, the individual could be counseled immediately and appropriate therapy initiated. Our group is focused on developing a microfluidic "lab-on-a-chip" that will simultaneously identify antigens, antibodies, RNA, and DNA using a single oral sample. The approach has been to design individual modules for each assay that uses similar components (e.g., valves, heaters, metering chambers, mixers) installed on a polycarbonate base with a common reporter system. Assay miniaturization reduces the overall analysis time, increases accuracy by simultaneously identifying multiple targets, and enhances detector sensitivity by upconverting phosphor technology (UPT). Our microfluidic approach employs four interrelated components: (1) sample acquisition-OraSure UPlink collectors that pick-up and release bacteria, soluble analytes, and viruses from an oral sample; (2) microfluidic processing-movement of microliter volumes of analyte, target analyte extraction and amplification; (3) detection of analytes using UPT particles in a lateral flow system; and (4) software for processing the results. Ultimately, the oral-based microscale diagnostic system will detect viruses and bacteria, associated pathogen antigens and nucleic acids, and antibodies to these pathogens.
