ABSTRACT
Humidity plays an important role in many fields, and the realization of high sensitivity and fast response simultaneously for humidity detection is a great challenge in practical application. In this work, we demonstrated a high-performance relative humidity (RH) sensor made by supporting zeolitic imidazolate framework-90 (ZIF-90)-derived porous zinc oxide (ZnO) onto an optical microfiber Sagnac interferometer (OMSI). The ZIF-90-modified OMSI (ZIF-90-OMSI) sensor was in situ heated at different temperatures to obtain porous ZnO, and their humidity-sensing properties were investigated ranging from 25 to 80% RH. The experimental results showed that the porous ZnO fiber sensor prepared at 500 °C (Z500-OMSI) exhibited best humidity-sensing performance with a high sensitivity of 96.2 pm/% RH (25-45% RH) and 521 pm/% RH (50-80% RH) and ultrafast response/recovery time (62.37/206.67 ms) at 22.3% RH. These performances were attributed to the complete transformation of ZIF-90 to ZnO at 500 °C. The obtained Z500 not only retained the high porosity and specific surface area of ZIF-90 but also exhibited the exceptional hydrophilicity of ZnO. In addition, the signals of the proposed Z500-OMSI sensor changed with different breathing patterns, indicating the possibility for human respiration monitoring. This work provided a reliable candidate for an effective RH monitoring system with potential application in medical diagnoses, industrial production, environmental detection, and human health monitoring.
ABSTRACT
Capacitive deionization in environmental decontamination has been widely studied and now requires intensive development to support large-scale deployment. Porous nanomaterials have been demonstrated to play pivotal roles in determining decontamination efficiency and manipulating nanomaterials to form functional architecture has been one of the most exciting challenges. Such nanostructure engineering and environmental applications highlight the importance of observing, recording, and studying basically electrical-assisted charge/ion/particle adsorption and assembly behaviors localized at charged interfaces. In addition, it is generally desirable to increase the sorption capacity and reduce the energy cost, which increase the requirement for recording collective dynamic and performance properties that stem from nanoscale deionization dynamics. Herein, we show how a single optical fiber can serve as an in situ and multifunctional opto-electrochemical platform for addressing these issues. The surface plasmon resonance signals allow the in situ spectral observation of nanoscale dynamic behaviors at the electrode-electrolyte interface. The parallel and complementary optical-electrical sensing signals enable the single probe but multifunctional recording of electrokinetic phenomena and electrosorption processes. As a proof of concept, we experimentally decipher the interfacial adsorption and assembly behaviors of anisotropic metal-organic framework nanoparticles at a charged surface and decouple the interfacial capacitive deionization within an assembled metal-organic framework nanocoating by visualizing its dynamic and energy consumption properties, including the adsorptive capacity, removal efficiency, kinetic properties, charge, specific energy consumption, and charge efficiency. This simple "all-in-fiber" opto-electrochemical platform offers intriguing opportunities to provide in situ and multidimensional insights into interfacial adsorption, assembly, and deionization dynamics information, which may contribute to understanding the underlying assembly rules and the exploring structure-deionization performance correlations for the development of tailor-made nanohybrid electrode coatings for deionization applications.
ABSTRACT
An optical microfiber interferometric biosensor for the low concentration detection of sequence-specific deoxyribonucleic acid (DNA) based on signal amplification technology via oligonucleotides linked to gold nanoparticles (Au-NPs) is proposed and experimentally analyzed. The sensor uses a "sandwich" detection strategy, in which capture probe DNA (DNA-c) is immobilized on the surface of the optical microfiber interferometer, the reporter probe DNA (DNA-r) is immobilized on the surface of Au-NPs, and the DNA-c and DNA-r are hybridized to the target probe DNA (DNA-t) in a sandwich arrangement. The dynamic detection of the DNA-t was found to range from 1.0×10-15 M to 1.0×10-8 M, and the limit of detection (LOD) concentration was 1.32 fM. This sensor exhibited not only a low LOD but also excellent selectivity against mismatched DNA-t, and it can be further developed for application in various sensing platforms.
Subject(s)
Biosensing Techniques/instrumentation , DNA/analysis , Gold/chemistry , Interferometry/instrumentation , Metal Nanoparticles/chemistry , Optical Devices , Equipment Design , Limit of DetectionABSTRACT
Fiber-optic biosensors are of great interest to many bio/chemical sensing applications. In this study, we demonstrate a high-order-diffraction long period grating (HOD-LPG) for the detection of prostate specific antigen (PSA). A HOD-LPG with a period number of less than ten and an elongated grating pitch could realize a temperature-insensitive and bending-independent biosensor. The bio-functionalized HOD-LPG was capable of detecting PSA in phosphate buffered saline with concentrations ranging from 5 to 500 ng/ml and exhibited excellent specificity. A limit of detection of 9.9 ng/ml was achieved, which is promising for analysis of the prostate specific antigen.
Subject(s)
Biosensing Techniques/methods , Fiber Optic Technology/methods , Optical Fibers , Prostate-Specific Antigen/analysis , Prostate-Specific Antigen/immunology , HumansABSTRACT
In this paper, a gas refractometer based on microfiber Sagnac interferometer is demonstrated, which can achieve an ultrahigh sensitivity when operating at the group birefringence turning point. We undertake a theoretical analysis and a simulated calculation to study the device characteristics and obtain the specific parameters of ellipticity and long axis of the elliptic microfiber for the group birefringence turning point. In the experiment, we obtain a positive sensitivity of 0.295 nm/KPa and a negative sensitivity of -0.219 nm/KPa during gas pressure and refractive index (RI) sensing, the obtained highest RI sensitivity can reach 160,938.9 nm/RIU. To further reveal its practical potential in gas detection, we conduct CO2 gas concentration detection and the device also demonstrates ultrahigh sensitivity and good repeatability. Besides, temperature sensing is performed to explore its temperature response wherein it shows a sensitivity of 486.7 pm/ °C. These results show its potential for use in gas- and acoustic-sensing applications.
ABSTRACT
In clinical diagnosis, accurate and reliable measurement technologies for the detection of disease biomarkers at ultralow concentrations can provide guidance for the initiation of treatment and potentially improve survival for patients. Here, we demonstrate an optical microfiber reader for enhanced analytical sensitivity in enzyme-linked immunosorbent assays (ELISA) that enables the detection of tiny changes of the refractive index (RI) induced by the catalyzed oxidation of substrate, owing to the strong interaction between the evanescent field and surrounding medium. By employing the microfiber reader for the C-reaction protein (CRP) and interleukin-6 (IL-6) assays after the enzymatic signal amplification in ELISA, we experimentally investigate the biosensing capacity of the device. As a result, log-linear relations of CRP and IL-6 detection in PBS and human serum between the concentration and spectral response were obtained at both nanogram and picogram levels, respectively, and anti-CRP/HRP detection as low as 9.75 pg/mL was achieved, which was undetectable by the conventional spectrophotometry. With a stable, accurate, and color-free detection capacity, this optical microfiber reader has a promising prospect in early disease diagnosis and clinical treatment.
Subject(s)
Biosensing Techniques , C-Reactive Protein/analysis , Enzyme-Linked Immunosorbent Assay , Fiber Optic Technology , Interleukin-6/analysis , Optical Fibers , Biosensing Techniques/instrumentation , C-Reactive Protein/metabolism , Enzyme-Linked Immunosorbent Assay/instrumentation , Equipment Design , Fiber Optic Technology/instrumentation , Horseradish Peroxidase/chemistry , Horseradish Peroxidase/metabolism , Humans , Interleukin-6/metabolismABSTRACT
We present here a detailed investigation into the sensitivity of the taper-based Mach-Zehnder interferometer as a function of external refractive index, with particular attention to the dispersion turning point (DTP) and possibilities for ultra-sensitive sensors. Our numerical simulation revealed that two DTPs exist with a decrease in the microfiber waist diameter; given this relationship, it is possible to obtain an ultra-sensitive operation. We then conducted experiments with fabricated devices with different waist diameters to achieve both positive and negative sensitivities at two DTPs. In particular, we achieved an ultrahigh refractive index sensitivity of approximately 95,832â nm/RIU at the second DTP when working with a diameter of 1.87 µm around the RI of air. These results show its potential for use in acoustic sensing and biochemical detection.
ABSTRACT
Progranulin (PGRN) is a multi-functional growth factor that mediates cell proliferation, survival, migration, tumorigenesis, wound healing, development, and anti-inflammation activity. A novel alternatively spliced transcript from the short-form PGRN1 gene encoding a novel, secreted GRN peptide composed of 20-a.a. signal peptide and 41-a.a. GRN named GRN-41 was identified to be abundantly expressed in immune-related organs including spleen, head kidney, and intestine of Mozambique tilapia. The expression of GRN-41 and PGRN1 were further induced in the spleen of tilapia challenged with Vibrio vulnificus at 3â¯h post infection (hpi) and 6 hpi, respectively. In this study, we established three transgenic zebrafish lines expressing the secreted GRN-41, GRN-A and PGRN1 of Mozambique tilapia specifically in muscle. The relative percent of survival (RPS) was enhanced in adult transgenic zebrafish expressing tilapia GRN-41 (68%), GRN-A (32%) and PGRN1 (36%) compared with control transgenic zebrafish expressing AcGFP after challenge with V. vulnificus. It indicates tilapia GRN-41 is a potent peptide against V. vulnificus infection. The secreted tilapia GRN-41 can induce the expression of innate immune response-related genes, such as TNFa, TNFb, IL-8, IL-1ß, IL-6, IL-26, IL-21, IL-10, complement C3, lysozyme (Lyz) and the hepatic antimicrobial peptide hepcidin (HAMP), in adult transgenic zebrafish without V. vulnificus infection. The tilapia GRN-41 peptide can enhance the innate immune response by further elevating TNFb, IL-1ß, IL-8, IL-6, and HAMP expression in early responsive time to the V. vulnificus challenge in transgenic zebrafish. Our results suggest that the novel GRN-41 peptide generated from alternative splicing of the tilapia PGRN1 gene is a potent peptide that defends against V. vulnificus in the transgenic zebrafish model by modulation of innate immunity.
Subject(s)
Fish Diseases/immunology , Immunity, Innate , Intercellular Signaling Peptides and Proteins/genetics , Intercellular Signaling Peptides and Proteins/immunology , Tilapia/genetics , Zebrafish/genetics , Zebrafish/immunology , Animals , Animals, Genetically Modified/genetics , Animals, Genetically Modified/immunology , Female , Fish Proteins/genetics , Fish Proteins/immunology , Longevity , Male , Progranulins , Vibrio Infections/immunology , Vibrio vulnificus/physiologyABSTRACT
We investigate the crystallization behavior of isotactic polypropylene (iPP) under the influence of nanoscale confinement templated by the microphase-separated structure of an iPP-based diblock copolymer system, isotactic polypropylene-block-atactic polystyrene (iPP-b-aPS). Three types of iPP microdomains, i.e., lamellae, cylinder, and sphere, were generated by controlling the composition of the diblock. The effect of microdomain morphology on the nucleation mechanism, crystallization kinetics, self-nucleation behavior, the population of the helical sequence of iPP block in the melt state, and crystal orientation have been systematically studied. It was found that the crystallization rate of iPP was predominantly controlled by homogeneous nucleation when the crystallization process was largely confined within the individual cylindrical and spherical microdomains. Such a nucleation mechanism and the highly frustrated crystal growth in the isolated microdomains led to the absence of Domain II and atypical crystallization kinetics in Domain III in the self-nucleation study. The population of the longer helical sequence of iPP block revealed by infrared spectroscopy was found to be affected by temperature but not by the spatial confinement, chain stretching, and junction point constraint imposed by the microdomains. Finally, the orientation of α-form iPP crystals in the lamellae-forming iPP-b-aPS was identified over a broad range of crystallization temperatures (T(c)). Different from other crystalline-amorphous diblocks, a lamellar branching of α-form iPP was observed in the lamellar microdomains at T(c) lying between 15 and 80 °C, where the daughter lamellae developed from the perpendicularly orientated parent iPP crystals with a specific angle of 80° or 100°. Once the sample was crystallized at T(c) ≤ 10 °C, the iPP crystals became randomly oriented.
