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STUDY DESIGN: Basic research. PURPOSE: This finite element (FE) analysis (FEA) aimed to compare the biomechanical parameters in multilevel posterior cervical fixation with the C7 vertebra instrumented by two techniques: lateral mass screw (LMS) vs. transpedicular screw (TPS). OVERVIEW OF LITERATURE: Very few studies have compared the biomechanics of different multilevel posterior cervical fixation constructs. METHODS: Four FE models of multilevel posterior cervical fixation were created and tested by FEA in various permutations and combinations. Generic differences in fixation were determined, and the following parameters were assessed: (1) maximum moment at failure, (2) maximum angulation at failure, (3) maximum stress at failure, (4) point of failure, (5) intervertebral disc stress, and (6) influence of adding a C2 pars screw to the multilevel construct. RESULTS: The maximum moment at failure was higher in the LMS fixation group than in the TPS group. The maximum angulation in flexion allowed by LMS was higher than that by TPS. The maximum strain at failure was higher in the LMS group than in the TPS group. The maximum stress endured before failure was higher in the TPS group than in the LMS group. Intervertebral stress levels at C6-C7 and C7-T1 intervertebral discs were higher in the LMS group than in the TPS group. For both models where C2 fixation was performed, lower von Mises stress was recorded at the C2-C3 intervertebral disc level. CONCLUSIONS: Ending a multilevel posterior cervical fixation construct with TPS fixation rather than LMS fixation at the C7 vertebra provides a stiff and more constrained construct system, with higher stress endurance to compressive force. The constraint and durability of the construct can be further enhanced by adding a C2 pars screw in the fixation system.
ABSTRACT
Thin electroosmotic flow (EOF) micropumps can generate flow in confined spaces such as lab-on-a-chip microsystems and implantable drug delivery devices. However, status quo methods for quantifying flow and other important parameters in EOF micropumps depend on microfluidic interconnects or fluorescent particle tracking: methods that can be complex and error-prone. Here, we present a novel connected droplet shape analysis (CDSA) technique that simplifies flow rate and zeta potential quantification in thin EOF micropumps. We also show that a pair of droplets connected by an EOF pump can function as a tunable convex lens system (TCLS). We developed a biocompatible and all polymer EOF micropump with an SU-8 substrate and poly(3,4-ethylenedioxythiophene) polystyrene sulfonate (PEDOT:PSS) electrodes. We microdrilled a channel through the electrode/SU-8/electrode layers to realize a monolithic EOF micropump. Then, we deposited a pinned droplet on each end of the microchannel so that it connected them. By controlling the EOF between the droplets and measuring the corresponding change in their shape, we quantified the nanoliter EOF rate and zeta potential at the interface of SU-8 with two liquids (deionized water and a l-glutamate neurotransmitter solution). When the droplet pair and pump were used as a TCLS, CDSA successfully predicted how the focal length would change when the pump drove fluid from one droplet to another. In summary, CDSA is a simple low-cost technique for EOF rate and zeta potential measurement, and a pair of droplets connected by an EOF micropump can function as a TCLS without any moving parts.
ABSTRACT
LAMP diagnosis of malaria is simple and cost-effective with acceptable sensitivity and specificity as compared to standard diagnostic modules such as microscopy, RDTs and nested PCR, and thus its deployment for onsite screening of malaria in resource-limited regions is under consideration. However, the requirement of an electricity-operated dry bath and bulky read-out unit is still a major concern. In an effort to simplify this limitation, we have developed a portable LAMP device and fluorescence readout unit which can be used in the rapid point-of-care diagnosis of malaria. We have developed a point-of-care diagnostic LAMP device that is easy to operate by a mobile application, and the results can be quantified with a fluorescent readout unit. The diagnostic performance of the device was evaluated in 90 P. falciparum-infected clinical isolates stored at 4°C for 6-7 years and 10 freshly collected isolates from healthy volunteers. The LOD and quantitative ability of LAMP in estimating parasitemia levels were revealed with laboratory-grown P. falciparum strain (3D7). The LAMP assay performed in our device was exclusive for P. falciparum detection with sensitivity and specificity determined to be 98.89% and 100%, respectively, in clinical isolates. The LOD was documented to be 1 parasite/µl at the cut-off ADC value of 20. Parasite density estimated from ADC values showed concordance with microscopically determined parasite density of the cultured P. falciparum 3D7 strain. The LAMP assay performed in our device provides a possible portable platform for its deployment in the point-of-care diagnosis of malaria. Further validation of the quantitative ability of the assay with freshly collected or properly stored clinical samples of known parasitemia is necessary for field applicability.
Subject(s)
Malaria, Falciparum , Malaria , Humans , Malaria/parasitology , Malaria, Falciparum/diagnosis , Malaria, Falciparum/parasitology , Molecular Diagnostic Techniques/methods , Nucleic Acid Amplification Techniques , Parasitemia/diagnosis , Plasmodium falciparum/genetics , Point-of-Care Systems , Sensitivity and SpecificityABSTRACT
The last major review of progress toward a chemical retinal prosthesis was a decade ago. Many important advancements have been made since then with the aim of producing an implantable device for animal testing. We review that work here discussing the potential advantages a chemical retinal prosthesis may possess, the spatial and temporal resolutions it might provide, the materials from which an implant might be constructed and its likely effectiveness in stimulating the retina in a natural fashion. Consideration is also given to implant biocompatibility, excitotoxicity of dispensed glutamate and known changes to photoreceptor degenerate retinas.
ABSTRACT
People afflicted with sickle cell disease (SCD) experience severe deterioration in quality of life. The disease is characterized by debilitating pain, anemia, and increased susceptibility to life threatening infections. This genetic disorder is endemic to many parts of the world. Extensive and accurate screening of individuals with sickle cell trait (SCT) in the population, coupled with genetic counselling can inhibit the propagation of the disease. The gold-standard techniques for the detection of sickle hemoglobin, such as capillary electrophoresis, HPLC, and genetic testing, are prohibitively expensive and time-consuming. Mass screening is usually conducted with a low-cost test called the solubility test, which does not offer high specificity. This study proposes a game-changing single-step low-cost method for rapidly yet accurately screening and diagnosing SCD and SCT. This method relies on the hitherto unexplored differences in the optical absorbance between diseased, trait, and normal blood samples, under deoxygenated conditions. The proposed method was tested in two phases of clinical validation: a pilot study and a blind study. A total of 438 patient samples were tested using the proposed method across the two phases. The proposed method offers an average accuracy, sensitivity, and specificity of 97.6%, 96.9%, and 98.6%, respectively. The proposed test has the potential to obliviate the conventional two-step process of screening and diagnostic tests as it can be used at the point-of-care with minimal training and yet yield results reliable enough to assess disability benefit claims.
Subject(s)
Anemia, Sickle Cell , Sickle Cell Trait , Anemia, Sickle Cell/diagnosis , Anemia, Sickle Cell/genetics , Humans , Pilot Projects , Point-of-Care Systems , Quality of Life , Sickle Cell Trait/diagnosis , Sickle Cell Trait/epidemiologyABSTRACT
Human activity recognition (HAR) is an important task in many applications such as smart homes, sports analysis, healthcare services, etc. Popular modalities for human activity recognition involving computer vision and inertial sensors are in the literature for solving HAR, however, they face serious limitations with respect to different illumination, background, clutter, obtrusiveness, and other factors. In recent years, WiFi channel state information (CSI) based activity recognition is gaining momentum due to its many advantages including easy deployability, and cost-effectiveness. This work proposes CSITime, a modified InceptionTime network architecture, a generic architecture for CSI-based human activity recognition. We perceive CSI activity recognition as a multi-variate time series problem. The methodology of CSITime is threefold. First, we pre-process CSI signals followed by data augmentation using two label-mixing strategies - mixup and cutmix to enhance the neural network's learning. Second, in the basic block of CSITime, features from multiple convolutional kernels are concatenated and passed through a self-attention layer followed by a fully connected layer with Mish activation. CSITime network consists of six such blocks followed by a global average pooling layer and a final fully connected layer for the final classification. Third, in the training of the neural network, instead of adopting general training procedures such as early stopping, we use one-cycle policy and cosine annealing to monitor the learning rate. The proposed model has been tested on publicly available benchmark datasets, i.e., ARIL, StanWiFi, and SignFi datasets. The proposed CSITime has achieved accuracy of 98.20%, 98%, and 95.42% on ARIL, StanWiFi, and SignFi datasets, respectively, for WiFi-based activity recognition. This is an improvement on state-of-the-art accuracies by 3.3%, 0.67%, and 0.82% on ARIL, StanWiFi, and SignFi datasets, respectively. In lab-5 users' scenario of the SignFi dataset, which has the training and testing data from different distributions, our model achieved accuracy was 2.17% higher than state-of-the-art, which shows the comparative robustness of our model.
Subject(s)
Human Activities , Privacy , Algorithms , Humans , Neural Networks, Computer , Recognition, PsychologyABSTRACT
L. donovani is an intracellular protozoan parasite, that causes visceral leishmaniasis (VL), and consequently, post-kala azar dermal leishmaniasis (PKDL). Diagnosis and treatment of leishmaniasis is crucial for decreasing its transmission. Various diagnostic techniques like microscopy, enzyme-linked immunosorbent assays (ELISA) and PCR-based methods are used to detect leishmaniasis infection. More recently, loop-mediated isothermal amplification (LAMP) assay has emerged as an ideal diagnostic measure for leishmaniasis, primarily due to its accuracy, speed and simplicity. However, point-of-care diagnosis is still not been tested with the LAMP assay. We have developed a portable LAMP device for the monitoring of Leishmania infection. The LAMP assay performed using our device can detect and amplify as little as 100 femtograms of L. donovani DNA. In a preliminary study, we have shown that the device can also amplify L. donovani DNA present in VL and PKDL patient samples with high sensitivity (100%), specificity (98%) and accuracy (99%), and can be used both for diagnostic and prognostic analysis. To our knowledge, this is the first report to describe the development and application of a portable LAMP device which has the potential to evolve as a point-of-care diagnostic and prognostic tool for Leishmania infections in future.
Subject(s)
Leishmaniasis/diagnosis , Leishmaniasis/parasitology , Molecular Diagnostic Techniques/instrumentation , Nucleic Acid Amplification Techniques/instrumentation , Case-Control Studies , DNA, Protozoan/genetics , Equipment Design , Fluorescence , Humans , Leishmania donovani/genetics , Leprosy/parasitology , Molecular Diagnostic Techniques/methods , Nucleic Acid Amplification Techniques/methods , Parasite Load , Point-of-Care Systems , Polymerase Chain Reaction/methods , Sensitivity and SpecificityABSTRACT
Fringe projection profilometry (FPP) is a widely used non-contact optical method for 3D profiling of objects. The commonly used linear fringe pattern in FPP has periodic intensity variations along the lateral direction. As a result, the linear fringe pattern used in FPP cannot uniquely represent the lateral shift induced by the objects having surface discontinuities. Thus, unambiguous surface profiling of objects, especially with surface discontinuities, using a single linear fringe image having a single fringe frequency, is unfeasible. This paper proposes using a radially symmetric circular fringe pattern as the structured light pattern for accurate unambiguous surface profiling of sudden height-discontinuous objects. To the best of our knowledge, this is the only method that can reconstruct discontinuous height profiles with the help of a single fringe image having a single frequency. The performance of the proposed algorithm is evaluated on several synthetic and real objects having smooth variations and discontinuities. Compared to the well-known fringe projection methods, the results depict that for a tolerable range of error, the proposed method can be applied for the reconstruction of objects with 4 times higher dynamic range and even at much lower fringe frequencies.
ABSTRACT
Microscopic observation of biological specimen smears is the mainstay of diagnostic pathology, as defined by the Digital Pathology Association. Though automated systems for this are commercially available, their bulky size and high cost renders them unusable for remote areas. The research community is investing much effort towards building equivalent but portable, low-cost systems. An overview of such research is presented here, including a comparative analysis of recent reports. This paper also reviews recently reported systems for automated staining and smear formation, including microfluidic devices; and optical and computational automated microscopy systems including smartphone-based devices. Image pre-processing and analysis methods for automated diagnosis are also briefly discussed. It concludes with a set of foreseeable research directions that could lead to affordable, integrated and accurate whole slide imaging systems.
Diagnosis of some diseases such as cervical cancer is done using a microscope, and this process still relies heavily on human experts. Since the need for such diagnosis is increasing at a rapid pace, it makes a lot of sense to automate the whole process. This requires automatic microscopes, which should be able to take images of a 'slide' - a glass slab with colorized human cells at its surface. These images should get analyzed by a software, resulting in a fully automated diagnosis. This article reviews recent research into this field, especially the technical advances on the hardware for automated microscopes (also known as slide imagers). It compares research reports and highlights how there's still more effort needed to build low-cost, yet clinically useful systems. It also highlights some of the emerging technologies that can be integrated into slide imagers to enable new kinds of diagnostics.
Subject(s)
Image Processing, Computer-Assisted , Microscopy , Image Processing, Computer-Assisted/instrumentation , Image Processing, Computer-Assisted/methods , Microscopy/instrumentation , Microscopy/methods , Pathology/instrumentation , Pathology/methods , Signal Processing, Computer-Assisted , SmartphoneABSTRACT
Lipopolysaccharides (endotoxins), found on Gram-negative bacteria, can trigger a severe immune response in humans leading to septic shock and in extreme cases, even death. Therefore, the detection and neutralization of lipopolysaccharides (LPS) is of utmost importance in the pharmaceutical and medical industries. The United States Food and Drug Administration (US FDA) recommended detection method for LPS, the Limulus amebocyte lysate (LAL) assay, is expensive, time consuming, complex, and is prone to interference from proteases. As an alternative, this paper proposes a rapid, label-free fluorescence-based assay using LPS-specific aptamers and the SYBR Green DNA stain. The proposed method has a detection limit of 0.1 ng/ml, which is sufficient to detect the permissible levels of LPS in many pharmaceutical drugs and medical products. The fluorescence signal was found to be a linear function of the concentration of LPS in the range from 0.1 ng/ml to 105 ng/ml.
Subject(s)
Endotoxins , Lipopolysaccharides , Benzothiazoles , Biological Assay , Diamines , Humans , Oligonucleotides , Quinolines , United StatesABSTRACT
Pebrine is the most dreaded infectious disease of the silkworm and has devastated sericulture in Europe during the 18th century. Thereafter, if it is detected, the crop is burned to prevent further dissemination. The conventional microscopic examination of moth's body fluid is erroneous and it exacerbates on Metarhizium anisopliae (MA) contaminated test samples. This is due to the resemblance of pebrine and MA spores in the microscopic examination. Therefore, this study aims to demonstrate an efficient pebrine detection technique. In the proposed method, a motorised brightfield microscope is custom-made to acquire focused and defocused images of test spores. These images are used to produce quantitative phase images of the spores by the transport of intensity equation method. The phase images' histogram of oriented gradients feature is used by a machine learning classifier to categorise the spores. This system classified 92 pebrine and 185 MA spores with an accuracy of 97% at 0.04 seconds/spore. The duration taken for image acquisition is 2.5 minutes per sample (10 fields of view covering an area of 302 × 260 µm2 ). The proposed method shows reliable results in pebrine diagnosis and would be an efficient alternative for current approaches.
Subject(s)
Bombyx , Machine Learning , Animals , Diagnostic ImagingABSTRACT
Objective.Our laboratory has proposed chemical stimulation of retinal neurons using exogenous glutamate as a biomimetic strategy for treating vision loss caused by photoreceptor (PR) degenerative diseases. Although our previousin-vitrostudies using pneumatic actuation indicate that chemical retinal stimulation is achievable, an actuation technology that is amenable to microfabrication, as needed for anin-vivoimplantable device, has yet to be realized. In this study, we sought to evaluate electroosmotic flow (EOF) as a mechanism for delivering small quantities of glutamate to the retina. EOF has great potential for miniaturization.Approach.An EOF device to dispense small quantities of glutamate was constructed and its ability to drive retinal output tested in anin-vitropreparation of PR degenerate rat retina.Main results.We built and tested an EOF microfluidic system, with 3D printed and off-the-shelf components, capable of injecting small volumes of glutamate in a pulsatile fashion when a low voltage control signal was applied. With this device, we produced excitatory and inhibitory spike rate responses in PR degenerate rat retinae. Glutamate evoked spike rate responses were also observed to be voltage-dependent and localized to the site of injection.Significance.The EOF device performed similarly to a previously tested conventional pneumatic microinjector as a means of chemically stimulating the retina while eliminating the moving plunger of the pneumatic microinjector that would be difficult to miniaturize and parallelize. Although not implantable, the prototype device presented here as a proof of concept indicates that a retinal prosthetic based on EOF-driven chemical stimulation is a viable and worthwhile goal. EOF should have similar advantages for controlled dispensing of charged neurochemicals at any neural interface.
Subject(s)
Electroosmosis , Retina , Animals , Biomimetics , Glutamic Acid , Photoreceptor Cells , RatsABSTRACT
Photocatalysis is an effective way for treatment of wastewater and degradation of dyes. It is important to assess the reusability of photocatalyst and treated water after the treatment process. In this study, the photocatalytic activity of TiO2 (titanium dioxide) and TiO2-TMAOH (titanium dioxide-tetramethylammonium hydroxide) was analyzed for degradation of methylene blue dye. Enhanced degradation of methylene blue is observed while treated with TiO2-TMAOH with photodegradation efficiency (PDE) 80% within 20 min. A further study shows the reusability of TiO2 for degradation of dye for six cycles with a decrease in photodegradation efficiency from 90% (cycle-1) to 50% (cycle-2). Fourier transform infrared spectroscopy (FTIR), energy-dispersive X-ray spectroscopy (EDX), and cyclic voltammetry (CV) analysis were carried out to identify the functional groups in treated water, traces of titanium, and TMAOH, respectively. Seed germination of Vigna radiata using TiO2- and TiO2-TMAOH-treated water shows equivalent and consistent growth. Water quality analysis of treated water shows improved biochemical oxygen demand (BOD) level (1.5 mg L-1), which is suitable for reusability of water for many applications. The outcomes suggest treated water can be used for irrigation and plantation purposes.
Subject(s)
Germination , Water , Catalysis , Seeds , TitaniumABSTRACT
The detection of food adulterants and toxicants can prevent a large variety of adverse health conditions for the global population. Through the process of rapid sensing enabled by deploying novel and robust sensors, the food industry can assist in the detection of adulterants and toxicants at trace levels. Sensor platforms which exploit graphene-based nanomaterials satisfy this requirement due to outstanding electrical, optical and thermal properties. The materials' facile conjugation with linkers and biomolecules along with the option for further enhancement using nanoparticles results in highly sensitive and selective sensing characteristics. This review highlights novel applications of graphene derivatives for detection covering three important approaches; optical, electrical (field-effect) and electrochemical sensing. Suitable graphene-based sensors for portable devices as point-of-need platforms are also presented. The future scope of these sensors is discussed to showcase how these emerging techniques will disrupt the food detection sector for years to come.
Subject(s)
Food Analysis/methods , Food Contamination/analysis , Graphite/chemistry , Electricity , NanotechnologyABSTRACT
Microporous SAPO-35 molecular sieves (Levyne type) were synthesized in non-aqueous media by using different inorganic promoters (HClO4 -, HF, H3PO4, and NaNO3) to enhance the rate of crystallization, and the as-synthesized materials were characterized by using different methods such as powder X-ray diffraction spectroscopy (PXRD), scanning electron microscopy (SEM), Fourier transform infrared spectroscopy (FT-IR), magic angle spinning-nuclear magnetic resonance spectroscopy (MAS-NMR), Brunauer-Emmett-Teller (BET) analysis, and X-ray photoelectron spectroscopy (XPS). From PXRD patterns, it was found that all the materials have a highly crystalline nature without any other impurities. SEM images reveal rhombohedral particles in all synthesis conditions. The framework structure of the synthesized materials was identified by FT-IR spectroscopy, and it reveals that all materials gave a similar framework structure. From BET and XPS, we have confirmed that the pore size and pore diameters along with the elemental compositions have a minor change. The 27Al, 31P, and 29Si MAS-NMR spectra of all the promoter-based SAPO-35 materials are close to those of the standard SAPO-35 material. All the above characterization studies reveal the formation of SAPO-35 in a short time with promoters. The catalytic application studies of these synthesized materials for a methanol-to-olefin conversion reaction were performed, and the efficiency of these materials was found to be similar to that of standard materials.
ABSTRACT
The introduction of lipopolysaccharides (LPS) or endotoxins that originate from Gram-negative bacteria into the human blood stream induces a severe immune response that can lead to septic shock, and even death. Hence, the accurate detection of LPS is of great importance in the medical and pharmaceutical sectors. This paper proposes a novel label-free fluorescence assay for the detection of LPS utilizing aptamers and the interference synthesis of dsDNA-templated copper nanoparticles. The assay can be performed at room temperature and does not require expensive reagents. The proposed assay has a limit of detection of 0.95 ng ml-1 of LPS, and the fluorescence emission from the copper nanoparticles was found to vary linearly with the concentration of LPS over a wide range (1 to 105 ng ml-1) with R2 = 0.9877.
Subject(s)
Copper , Metal Nanoparticles , DNA , Fluorescent Dyes , Humans , LipopolysaccharidesABSTRACT
Opportunistic skin pathogens and their resistance to pre-existing therapeutics are a challenge to normal physiological wound healing processes. Consistent development of antimicrobial agents is required to overcome the complications raised by antimicrobial resistance. An effective alternative proposed in recent research includes the use of antimicrobial nanoparticles or nanobiopolymers. Unfortunately, metallic nanoparticles that have been proven as antimicrobial agents also possess a certain level of toxicity. In this work, we demonstrate the use of a cationic polymer, branched polyethyleneimine (B-PEI), that has been electrospun to obtain a scaffold/fiber (B-PEI NF) mat resulting in a large surface area-to-volume ratio. SEM analysis revealed that the average diameter of the obtained fibers is 240 nm. The formation of nanoscaffold modulates the controlled release of the polymer from the matrix resulting in long-term effects. The antimicrobial and antibiofilm activity of the B-PEI nanofiber (B-PEI NF) was evaluated against ESKAPE pathogens (Pseudomonas aeruginosa and Staphylococcus aureus) and also against Candida albicans. Dose-dependent inhibition was observed for microbial growth and biofilm for all three test organisms, the minimum inhibitory concentration required for inhibiting P. aeruginosa, S. aureus, and C. albicans is 33.125, 26.5, and 19.875 µM, respectively, in 2 mL of bacterial/fungal broth. Crystal violet and 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide assays showed significant reduction in biomass and cell viability of sessile cells, respectively, within the biofilm after treatment using B-PEI NFs. A B-PEI NF matrix promotes cell migration and wound healing processes by mimicking the extracellular matrix. In vitro wound healing studies showed a fivefold increase in cell migration and wound healing by B-PEI NFs (97% wound coverage in 17 h) when compared to B-PEI (15% wound coverage in 17 h). The in vitro wound healing assays confirmed the biocompatibility and better wound healing activity of B-PEI NF mats.
Subject(s)
Anti-Infective Agents , Nanofibers , Anti-Bacterial Agents/chemistry , Anti-Infective Agents/pharmacology , Candida albicans , Nanofibers/therapeutic use , Polyethyleneimine/pharmacology , Staphylococcus aureus , Wound HealingABSTRACT
Low-cost automated histopathology microscopy systems usually suffer from optical imperfections, producing images that are slightly Out of Focus (OoF). In this work, a guided filter (GF) based image preprocessing is proposed for compensating focal errors and its efficacy is demonstrated on images of healthy and malaria infected red blood cells (h-RBCs and i-RBCs), and PAP smears. Since contrast enhancement has been widely used as an image preprocessing step for the analysis of histopathology images, a systematic comparison is made with six such prominently used methods, namely Contrast Limited Adaptive Histogram Equalization (CLAHE), RIQMC-based optimal histogram matching (ROHIM), modified L0, Morphological Varying(MV)-Bitonic filter, unsharp mask filter and joint bilateral filter. The images enhanced using GF approach lead to better segmentation accuracy (upto 50% improvement over native images) and visual quality compared to other approaches, without any change in the color tones. Thus, the proposed GF approach is a viable solution for rectifying the OoF microscopy images without the loss of the valuable diagnostic information presented by the color tone.
Subject(s)
Algorithms , Image Enhancement , Female , HumansABSTRACT
INTRODUCTION: Though the oral health status of workers from different industries was reported in literature, there is little information with regard to spinning mill workers. The aim of this study was to document the oral health status, oral hygiene routine, and frequency of utilization of oral health care services among spinning mill workers in Guntur district. MATERIALS AND METHODS: 458 spinning mill workers in Guntur district participated in this study. Data on hygiene practices, self-reported dental problems, past dental visits, type and place of availed treatments, and barriers for utilizing dental services were recorded. Oral health status was examined using Simplified Oral Hygiene Index, DMFT index, and Community Periodontal Index. RESULTS: Female participants were found to have better oral hygiene status compared to males, which is partially significant. Similar was the scenario when caries experience was considered. Majority of the study subjects (74%) have a DMFT score of 1-6. There were 86 participants without any coronal caries experience. The mean coronal caries experience was more among older spinning mill workers compared to the younger workers. The difference in DMFT scores between males and females was not significant. Majority of the participants (46.3%) were with CPI score 2, while only 10.2% were observed to have all healthy sextants. 136 subjects (30.15%) demonstrated loss of attachment of some severity. CONCLUSION: Though the oral hygiene habits reported by the spinning mill workers were fair, oral health care seeking behaviors were found to be less informed. There is a serious need to improve the oral health awareness and care seeking behaviors among these workers.
ABSTRACT
Fluorescent copper nanoparticles templated by dsDNA have gained significant research interest as they are inexpensive and easy to synthesize, and have found applications in the detection of a wide range of analytes. The presence of the analyte in the reaction mixture interferes with the synthesis of the copper nanoparticles and the subsequent drop in fluorescence can be correlated to the concentration of the analyte present in the solution. Analyte detection using copper nanoparticle-based assays is amenable for in-situ applications as the test does not require expensive reagents and can be performed at room temperature. However, expensive and sophisticated detection systems are required for the detection of copper nanoparticles due to the low fluorescence emission signal from these nanoparticles. This restricts the use of the technology to centralized labs. Utilizing a recently developed chemical technique for fluorescence enhancement, this paper presents the first report of a handheld fluorometer capable of detecting DNA-templated copper nanoparticles. The fluorometer is portable and constructed with low-cost, off-the-shelf components like a UV-LED and a PIN photodiode. The performance of the developed system is demonstrated through the detection of melamine in milk samples via the interference synthesis of copper nanoparticles. Melamine is an adulterant used in dairy products that is harmful to human health if present in levels above 1 ppm. The developed system is capable of detecting up to 0.1 ppm of melamine in milk samples with a linear relationship observed between the detector output and concentration of melamine in the range from 0.1 ppm to 100 ppm (R2 = 0.9979).
