Your search keyword '"Fluorescent Dyes standards"' showing total 88 results

1. Exploratory development of PCR-fluorescent probes in rapid detection of mutations associated with extensively drug-resistant tuberculosis.

Author

Liang J, An H, Zhou J, Liu Y, Xiang G, Liu Y, Xing W, and Gong W

Subjects

Antitubercular Agents pharmacology, Bacterial Proteins genetics, Drug Resistance, Multiple, Bacterial, Fluorescent Dyes metabolism, Fluorescent Dyes pharmacology, Genotype, Humans, Microbial Sensitivity Tests, Mycobacterium tuberculosis drug effects, Polymerase Chain Reaction methods, Sequence Analysis, DNA, Sputum microbiology, Extensively Drug-Resistant Tuberculosis microbiology, Fluorescent Dyes standards, Mutation, Mycobacterium tuberculosis genetics, Polymerase Chain Reaction standards

Abstract

This study aims to evaluate the clinical value of PCR-fluorescent probes for detecting the mutation gene associated with extensively drug-resistant tuberculosis (XDR-TB). The molecular species identification of 900 sputum specimens was performed using polymerase chain reaction (PCR)-fluorescent probe. The mutations of the drug resistance genes rpoB, katG, inhA, embB, rpsL, rrs, and gyrA were detected. The conventional drug susceptibility testing (DST) and PCR-directed sequencing (PCR-DS) were carried out as control. DST demonstrated that there were 501 strains of rifampicin resistance, 451 strains of isoniazid resistance, 293 strains of quinolone resistance, 425 strains of streptomycin resistance, 235 strains of ethambutol resistance, and 204 strains of amikacin resistance. Furthermore, 427 (47.44%) or 146 (16.22%) strains were MDR-TB or XDR-TB, respectively. The mutations of the rpoB, katG, inhA, embB, rpsL, rrs, and gyrA genes were detected in 751 of 900 TB patients by PCR-fluorescent probe method, and the rate of drug resistance was 751/900 (83.44%). No mutant genes were detected in the other 149 patients. Compared with DST, the mutant rates of rpoB, katG/inhA, rpsL, rrs, embB, and gyrA of six drugs were higher than 88%; five of six drugs were higher than 90% except for SM (88.11%). The MDR and XDR mutant gene types were found in 398 (42.22%) and 137 (15.22%) samples. PCR-DS was also employed and confirmed the PCR-fluorescent probe method with the accordance rate of 100%. The PCR-fluorescent probe method is rapid and straightforward in detecting XDR-TB genotypes and is worthy of being applied in hospitals., (© 2021. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published

2021

2. Comparison of the Benzanthrone Luminophores: They Are Not Equal for Rapid Examination of Parafasciolopsis fasciolaemorpha (Trematoda: Digenea).

Author

Rubenina I, Gavarane I, Kirilova E, Mezaraupe L, and Kirjusina M

Subjects

Animals, Fluorescent Dyes standards, Microscopy, Confocal methods, Muscles cytology, Muscles metabolism, Sensitivity and Specificity, Tissue Fixation methods, Benz(a)Anthracenes chemistry, Fluorescent Dyes chemical synthesis, Staining and Labeling methods, Trematoda cytology

Abstract

Luminescent derivatives of benzanthrone are becoming more useful based on their light-absorbing and fluorescent-emitting properties. Our previous studies showed that luminescent staining properties of the same benzanthrone dye differ for variable parasite samples. Therefore, two types of benzanthrone dyes were prepared. One has a strongly basic amidine group and a halogen atom, and the other has an amide moiety and a tertiary amine group. Trematoda Parafasciolopsis fasciolaemorpha is a liver fluke of a moose ( Alces alces ) and has a significant influence on the health and abundance of the moose population. Staining protocols for parasite P. fasciolaemorpha specific organ or organ systems imaging are mostly time-consuming and labor-intensive. The study aimed to compare the fixation technique and the staining protocol by synthesized benzanthrone luminescent dyes to determine detailed morphology, anatomical arrangement of the organ systems and gross organization of the muscle layers of P. fasciolaemorpha using confocal laser scanning microscopy. Luminophores were tested for samples fixed in different fixatives. Developed dyes and staining protocol resulting in imaging of all parts of trematode without additional sample preparation procedures, which usually are required for parasite examination. Obtained results confirmed that the most qualitative results could be reached using 3-N-(2-piperidinylacetamido)benzanthrone dye which has amide moiety and a tertiary amine group. Based on obtained results, 3-N-(2-piperidinylacetamido)benzanthrone gave more qualitative parasite visualization than 2-bromo-3-N-(N',N'-dimethylformamidino)benzanthrone.

Published

2021

3. Progress and challenges in the use of fluorescence-based flow cytometric assays for anti-malarial drug susceptibility tests.

Author

Kulkeaw K

Subjects

Erythrocytes parasitology, Flow Cytometry standards, Fluorescent Dyes standards, Parasitic Sensitivity Tests standards, Staining and Labeling, Antimalarials pharmacology, Flow Cytometry methods, Fluorescence, Parasitic Sensitivity Tests methods, Plasmodium falciparum drug effects

Abstract

Drug-resistant Plasmodium is a frequent global threat in malaria eradication programmes, highlighting the need for new anti-malarial drugs and efficient detection of treatment failure. Plasmodium falciparum culture is essential in drug discovery and resistance surveillance. Microscopy of Giemsa-stained erythrocytes is common for determining anti-malarial effects on the intraerythrocytic development of cultured Plasmodium parasites. Giemsa-based microscopy use is conventional but laborious, and its accuracy depends largely on examiner skill. Given the availability of nucleic acid-binding fluorescent dyes and advances in flow cytometry, the use of various fluorochromes has been frequently attempted for the enumeration of parasitaemia and discrimination of P. falciparum growth in drug susceptibility assays. However, fluorochromes do not meet the requirements of being fast, simple, reliable and sensitive. Thus, this review revisits the utility of fluorochromes, notes previously reported hindrances, and highlights the challenges and opportunities for using fluorochromes in flow cytometer-based drug susceptibility tests. It aims to improve drug discovery and support a resistance surveillance system, an essential feature in combatting malaria.

Published

2021

4. Clinical Validation of an Automated Fluorogenic Factor XIII Activity Assay Based on Isopeptidase Activity.

Author

Leitner M, Büchold C, Pasternack R, Binder NB, and Moore GW

Subjects

Automation, Laboratory standards, Bilirubin metabolism, Blood Coagulation Tests standards, Chromogenic Compounds standards, Factor XIII metabolism, Factor XIII Deficiency blood, Fluorometry methods, Fluorometry standards, Hemolysis, Humans, Immunologic Tests methods, Immunologic Tests standards, Reproducibility of Results, Transglutaminases metabolism, Automation, Laboratory methods, Blood Coagulation Tests methods, Carbon-Nitrogen Lyases metabolism, Factor XIII analysis, Factor XIII Deficiency diagnosis, Fluorescent Dyes standards

Abstract

Hereditary factor XIII (FXIII) deficiency is a rare autosomal bleeding disorder which can cause life-threatening bleeding. Acquired deficiency can be immune-mediated or due to increased consumption or reduced synthesis. The most commonly used screening test is insensitive, and widely used quantitative assays have analytical limitations. The present study sought to validate Technofluor FXIII Activity, the first isopeptidase-based assay available on a routine coagulation analyser, the Ceveron s100. Linearity was evidenced throughout the measuring range, with correlation coefficients of >0.99, and coefficients of variation for repeatability and reproducibility were <5% and <10%, respectively. A normally distributed reference range of 47.0-135.5 IU/dL was derived from 154 normal donors. Clinical samples with Technofluor FXIII Activity results between 0 and 167.0 IU/dL were assayed with Berichrom ® FXIII Activity, a functional ammonia release assay, and the HemosIL ™ FXIII antigen assay, generating correlations of 0.950 and 0.980, respectively. Experiments with a transglutaminase inhibitor showed that Technofluor FXIII Activity can detect inhibition of enzymatic activity. No interference was exhibited by high levels of haemolysis and lipaemia, and interference by bilirubin was evident at 18 mg/dL, a level commensurate with severe liver disease. Technofluor FXIII Activity is a rapid, accurate and precise assay suitable for routine diagnostic use with fewer interferents than ammonia release FXIII activity assays.

Published

2021

5. Supramolecular Assembly of TPE-Based Glycoclusters with Dicyanomethylene-4H-pyran (DM) Fluorescent Probes Improve Their Properties for Peroxynitrite Sensing and Cell Imaging.

Author

Dong L, Fu M, Liu L, Han HH, Zang Y, Chen GR, Li J, He XP, and Vidal S

Subjects

Glycoconjugates chemistry, Fluorescent Dyes chemistry, Fluorescent Dyes standards, Optical Imaging methods, Peroxynitrous Acid analysis, Pyrans chemistry, Stilbenes chemistry

Abstract

Two red-emitting dicyanomethylene-4H-pyran (DM) based fluorescent probes were designed and used for peroxynitrite (ONOO - ) detection. Nevertheless, the aggregation-caused quenching effect diminished the fluorescence and restricted their further applications. To overcome this problem, tetraphenylethylene (TPE) based glycoclusters were used to self-assemble with these DM probes to obtain supramolecular water-soluble glyco-dots. This self-assembly strategy enhanced the fluorescence intensity, leading to an enhanced selectivity and activity of the resulting glyco-dot comparing to DM probes alone in PBS buffer. The glyco-dots also exhibited better results during fluorescence sensing of intracellular ONOO - than the probes alone, thereby offering scope for the development of other similar supramolecular glyco-systems for chemical biological studies., (© 2020 Wiley-VCH GmbH.)

Published

2020

6. Evaluation of a six-dye multiplex composed of 27 markers for forensic analysis and databasing.

Author

Wang S, Song F, Xie M, Zhang K, Xie B, Huang Z, and Luo H

Subjects

Chromosomes, Human genetics, Female, Fluorescent Dyes chemistry, Fluorescent Dyes standards, Forensic Genetics standards, Genetic Markers, Humans, Male, Multiplex Polymerase Chain Reaction standards, Reference Standards, Sensitivity and Specificity, Databases, Genetic, Forensic Genetics methods, Microsatellite Repeats, Multiplex Polymerase Chain Reaction methods, Population genetics

Abstract

Background: Short tandem repeat (STR) markers play a significant role in genetic applications and have proved to be effective for the personal identification in forensic medicine. In this study, a six-dye multiplex composed of 23 autosomal STR loci (TH01, D3S1358, Penta D, D6S1043, D21S11, TPOX, D1S1656, D12S391, Penta E, D10S1248, D22S1045, D19S433, D8S1179, D2S1338, D2S441, D18S51, vWA, FGA, D16S539, CSF1PO, D13S317, D5S818, D7S820), one Y chromosome STR (DYS391), two internal quality control markers (Quality Sensor QS1 and QS2), and Amelogenin was evaluated., Methods: Evaluation studies, including PCR-based studies, sensitivity studies, species specificity studies, stability studies, DNA mixture studies, concordance studies, and precision evaluations were performed according to the guidelines of "Validation Guidelines for Forensic DNA Analysis Methods (2016)" by the Scientific Working Group on DNA Analysis Methods (SWGDAM). In addition, the forensic characteristics of 357 unrelated male samples from Han and Hui populations in China were investigated using 27 markers., Results: Full STR profiles were obtained from different reaction volumes (5 ~ 25 μl), cycle numbers (28 ~ 34 cycles) and annealing temperatures (58 ~ 62°C). All STR profiles were obtained at humic acid concentration of up to 200 ng/μl and hematin concentration of up to 500 μM. No peaks were observed in most common animal samples except two innovative internal PCR controls (Quality Sensor QS1 and QS2). The six-dye multiplex showed a notably high value for the combined probability of exclusion (CPE), exhibiting values of with 0.99999999977688 in the Han population and 0.999999999583875 in the Hui population. The values of combined probability of discrimination (CPD) were 0.999999999999999999999999999997453 in the Han population and 0. 999999999999999999999999999994398 in the Hui population. In addition, concordance studies showed that there was no difference with the AGCU Express Marker 22 Kit., Conclusion: The results indicated that the Investigator ® 26plex QS Kit is a robust, reliable, and suitable tool for forensic analysis and databasing., (© 2020 The Authors. Molecular Genetics & Genomic Medicine published by Wiley Periodicals LLC.)

Published

2020

7. Recent progress on the organic and metal complex-based fluorescent probes for monitoring nitric oxide in living biological systems.

Author

Wang L, Zhang J, An X, and Duan H

Subjects

Animals, Cells metabolism, Coordination Complexes chemistry, Fluorescent Dyes standards, Humans, Molecular Imaging methods, Organelles metabolism, Fluorescent Dyes chemistry, Nitric Oxide analysis

Abstract

Nitric oxide (NO) is an important gaseous signaling molecule related to various human diseases. To investigate the biological functions of NO, many strategies have been developed for real-time monitoring the NO levels in biological systems. Among these strategies, fluorescent probes are considered to be one of the most efficient and applicable methods owing to their excellent sensitivity and selectivity, high spatiotemporal resolution, noninvasiveness, and experimental convenience. Therefore, great efforts have been paid to the design, synthesis, and fluorescence investigation of novel NO fluorescent probes in the past several years. However, few of them exhibit practical applications owing to the low concentration, short half-life, and rapid diffusion characteristics of NO in biological systems. Rational design of NO fluorescent probes with excellent selectivity and sensitivity, low cytotoxicity, long-lived fluorescent emission, and low background interference is still a challenge for scientists all over the word. To provide spatial-temporal information, this article focuses on the progress made in the organic and metal complex-based NO fluorescent probes during the past five years. The key structural elements and sensing mechanisms of NO fluorescent probes are discussed. Some novel ratiometric, luminescence, and photoacoustic probes with low background interference and deep tissue penetrating ability are mentioned. All these probes have been used for imaging exogenous and endogenous NO in cells and animal models. More importantly, this article also describes the development of multi-functional NO fluorescent probes, such as organelle targeting probes, dual-analysis probes, and probe-drug conjugates, which will inspire the design of various functional fluorescent probes.

Published

2020

8. Lot-to-lot stability of antibody reagents for flow cytometry.

Author

Böttcher S, van der Velden VHJ, Villamor N, Ritgen M, Flores-Montero J, Escobar HM, Kalina T, Brüggemann M, Grigore G, Martin-Ayuso M, Lecrevisse Q, Pedreira CE, van Dongen JJM, and Orfao A

Subjects

Animals, Mice, Protein Stability, Reproducibility of Results, Antibodies, Monoclonal, Flow Cytometry methods, Flow Cytometry standards, Fluorescent Dyes standards

Abstract

The fluorescence detected using fluorochrome-labelled monoclonal antibodies depends not only on the abundance of the target antigen, but amongst many other factors also on the effective fluorochrome-to-antibody ratio. The diagnostic approach of the EuroFlow consortium relies on reproducible fluorescence intensities over time. A capture bead system for mouse immunoglobulin light chains was utilized to compare the mean fluorescence intensity of 1323 consecutive antibody lots to the currently used lot of the same monoclonal antibody. In total, 157 different monoclonal antibodies were assessed over seven years. Median relative difference between consecutive lots was 3.8% (range: 0.01% to 164.7%, interquartile range: 1.3% to 10.1%). The relative difference exceeded 20% in 8.8% of all comparisons. FITC labelled monoclonal antibodies (median relative difference: 2.1%) showed a significantly smaller variation between lots than antibodies conjugated to PE (3.5%), PECy7 (3.9%), PerCPCy5.5 (5.8%), APC (5.8%), APCH7 (7.4%), and APCC750 (14.5%). Reagents labelled with Pacific Blue (1.4%), Pacific Orange (2.4%), HV450 (0.7%), and HV500 (1.7%) demonstrated more consistent results compared to conjugates of BV421 (4.1%) and BV510 (16.2%). Additionally, significant differences in lot-to-lot fluorescence stability amongst antibodies labelled with the same fluorochrome were observed between manufacturers. These observations might guide future quality recommendations for the production and application of fluorescence-labelled monoclonal antibodies in multicolor flow cytometry., (Copyright © 2017. Published by Elsevier B.V.)

Published

2019

9. Pharmacological control of inflammation in wound healing.

Author

Shukla SK, Sharma AK, Gupta V, and Yashavarddhan MH

Subjects

Administration, Topical, Anti-Inflammatory Agents, Non-Steroidal standards, Anti-Inflammatory Agents, Non-Steroidal therapeutic use, Cyclooxygenase Inhibitors standards, Cyclooxygenase Inhibitors therapeutic use, Fluorescent Dyes standards, Fluorescent Dyes therapeutic use, Humans, Inflammation prevention & control, Insulin administration & dosage, Insulin standards, Insulin therapeutic use, Mesenchymal Stem Cells, MicroRNAs standards, MicroRNAs therapeutic use, Inflammation drug therapy, Wound Healing drug effects

Abstract

Wound inflammation is a rapid and highly orchestrated process that significantly impacts the wound healing cascade. Consequent to injury, a series of events set off that include inflammatory, proliferation and maturation phases leading to wound closure and restoration of normal skin integrity. Stimuli causing stress to host immune system or induce inflammatory response include tissue damage and pathogenic microbial infection.Several evidences points towards the positive role of inflammation as it essential to fight against the attack of invading pathogens and to remove dead tissues from the site of injury. Besides its positive role, prolonged inflammation is injurious and may result in deregulated stages of the wound healing which may lead to excessive scarring. Achieving balance in inflammatory cascade is one of the challenging tasks for development of a wound healing drug. This review mainly focuses on the pharmacological control of inflammation by agents which critically balance the inflammatory cascade. However, none of the agent is available in the healthcare market which exclusively plays a role in wound repair. In this review we shall explore different factors or agents affecting inflammation in wound healing. This information might be helpful in designing and development new process, technologies or drugs for better management of wound care. In addition, understanding the effect of inflammation on the outcome of the healing process will serve as a significant milestone in the area of pathological tissue repair., (Copyright © 2019 Tissue Viability Society. Published by Elsevier Ltd. All rights reserved.)

Published

2019

10. Green-Emitting Rhodamine Dyes for Vital Labeling of Cell Organelles Using STED Super-Resolution Microscopy.

Author

Grimm F, Nizamov S, and Belov VN

Subjects

Color, Fibroblasts ultrastructure, Fluorescent Dyes standards, Humans, Microscopy, Fluorescence methods, Fluorescent Dyes chemistry, Microscopy, Fluorescence instrumentation, Organelles, Rhodamines, Staining and Labeling methods

Abstract

Fluorescence microscopy reveals the localization, spatial distribution, and temporal dynamics of the specifically labeled organelles in living cells. Labeling with exogenous conjugates prepared from fluorescent dyes and small molecules (ligands) is an attractive alternative to the use of fluorescent proteins, but proved to be challenging due to insufficient cell-permeability of the probes, unspecific staining, or low dye brightness. We evaluated four green-emitting rhodamine dyes and their conjugates intended for the specific labeling of lysosomes, mitochondria, tubulin, and actin in living cells. The imaging performance of the probes in living human fibroblasts has been studied by using confocal and stimulated emission depletion (STED) super-resolution microscopy with a commercial 595 nm STED laser. Two bright and photostable dyes (LIVE 510 and LIVE 515) provide specific and versatile staining., (© 2019 Wiley-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2019

11. Comparative study of two near-infrared coumarin-BODIPY dyes for bioimaging and photothermal therapy of cancer.

Author

Zhang Y, Song N, Li Y, Yang Z, Chen L, Sun T, and Xie Z

Subjects

Cell Proliferation drug effects, Cell Proliferation radiation effects, Fluorescent Dyes chemistry, HeLa Cells, Humans, Infrared Rays, Nanoparticles, Boron Compounds chemistry, Coumarins chemistry, Fluorescent Dyes standards, Neoplasms diagnostic imaging, Neoplasms therapy, Optical Imaging methods, Phototherapy methods

Abstract

Near-infrared (NIR) responsive agents for cancer bioimaging and photothermal therapy are available and significant. Herein, we employed two easily available dyes, boron-dipyrromethane and coumarin, to synthesize a pair of coumarin-borondipyrromethane dyes with different conjugate degrees (BDC and BSC). The difference in conjugate degree made their photophysical properties poles apart. After the self-assembling of BDC and BSC, the newly constructed nanoparticles (BDC NPs and BSC NPs) demonstrated good biocompatibility. Moreover, BDC NPs exhibited a good photothermal effect under irradiation of 808 nm laser, which could effectively inhibit the growth of HeLa cells, and BSC NPs could quickly show a conspicuous fluorescence in the HeLa cells. The exploration demonstrates that the two organic dyes prepared with different conjugation degrees could provide new options for photothermal therapy of cancer and rapid bioimaging.

Published

2019

12. Development of a near-infrared ratiometric fluorescent probe for glutathione using an intramolecular charge transfer signaling mechanism and its bioimaging application in living cells.

Author

Zhou Y, Zhang L, Zhang X, and Zhu ZJ

Subjects

Fluorescent Dyes pharmacology, Fluorescent Dyes standards, HeLa Cells, Humans, Infrared Rays, Limit of Detection, Signal Transduction, Fluorescent Dyes chemistry, Glutathione analysis, Optical Imaging methods

Abstract

A novel near-infrared (NIR) ratiometric fluorescent probe HBT-GSH derived from conjugated benzothiazole was developed for the selective detection of glutathione (GSH) over cysteine (Cys) and homocysteine (Hcy). The probe was sophisticatedly designed based on the GSH selectively induced enhancement of intramolecular charge transfer (ICT) fluorescence. It was synthesized by masking the active phenol group of 2,6-bis(2-vinylbenzothiazolyl)-4-fluorophenol through an acetyl group that acts both as a trigger of the ICT fluorescence and as a recognition moiety for GSH. On its own, the probe HBT-GSH exhibited strong blue fluorescence emission at 426 nm and weak NIR fluorescence emission at 665 nm in aqueous solution, whereas the NIR fluorescence was significantly enhanced and the short emission decreased upon the addition of GSH. Thus an NIR ratiometric fluorescent probe for GSH was developed based on the GSH-selective removal of the acetyl group, therefore switching on the ICT in HBT-GSH. The fluorescence intensity ratio (I 665 nm /I 426 nm ) showed a linear relationship with a GSH concentration of 0-100 μM with a detection limit of 0.35 μM. Moreover, the fluorescent probe was successfully used for the ratiometric fluorescence bioimaging of GSH in living cells.

Published

2019

13. Yellow-emissive carbon dots with a large Stokes shift are viable fluorescent probes for detection and cellular imaging of silver ions and glutathione.

Author

Yan F, Bai Z, Zu F, Zhang Y, Sun X, Ma T, and Chen L

Subjects

Cell Line, Diagnostic Imaging standards, Fluorescent Dyes standards, Humans, Ions, Solanum lycopersicum cytology, Microscopy, Fluorescence methods, Microscopy, Fluorescence standards, Molecular Probes chemistry, Molecular Probes standards, Spectrometry, Fluorescence methods, Spectrometry, Fluorescence standards, Vitis cytology, Diagnostic Imaging methods, Fluorescent Dyes chemistry, Glutathione analysis, Silver analysis

Abstract

Yellow-emissive carbon dots (Y-CDs) were prepared by a solvothermal method using anhydrous citric acid and 2,3-phenazinediamine as the starting materials. The Y-CDs display a 24% fluorescence quantum yield, a 188-nm Stokes' shift and excellent stability. They are shown here to be excellent fluorescent probes for the determination of Ag(I) ion and glutathione (GSH). If exposed to Ag(I) ions, they are bound by the carboxy groups of the Y-CDs, and this causes quenching of fluorescence (with excitation/emission maxima at 380/568 nm) via a static quenching mechanism. This effect was used to design a fluorometric assay for Ag(I). The quenched fluorescence of the Y-CDs can be restored by adding GSH due to the high affinity of GSH for Ag(I). The calibration plot for Ag(I) is linear in the 1-4 μM Ag(I) concentration range, and the limit of detection is 31 nM. The respective values for GSH are 5-32 μM, and 76 nM, respectively. The method was applied to the detection of Ag(I) in spiked environmental water samples and gave recoveries ranging from 93 to 107%. It was also applied to the determination of GSH in tomatoes and purple grapes and gave satisfactory recoveries. The Y-CDs display low cytotoxicity and were successfully used to image Ag(I) and GSH in H1299 cells. Graphical abstract Schematic presentation of the mechanism of yellow fluorescent CDs for the detection of Ag + and glutathione.

Published

2019

14. A turn-on fluorescent probe for vitamin C based on the use of a silicon/CoOOH nanoparticle system.

Author

Lu Q, Chen X, Liu D, Wu C, Liu M, Li H, Zhang Y, and Yao S

Subjects

Cobalt chemistry, Fluorescence Resonance Energy Transfer, Fluorescent Dyes standards, Fluorometry methods, Fluorometry standards, Oxidation-Reduction, Oxides chemistry, Silicon chemistry, Ascorbic Acid analysis, Fluorescent Dyes chemistry, Nanoparticles chemistry

Abstract

The authors describe a fluorometric method for the turn-on determination of vitamin C (ascorbic acid). The blue fluorescence of silicon nanoparticles (SiNPs; with excitation/emission maxima at 350/450 nm) is found to be quenched by CoOOH nanoparticles (NPs). In the presence of vitamin C, the CoOOH NPs are decomposed by a redox reaction between the diol group of vitamin C and CoOOH NPs. As a result, fluorescence recovers. On the basis of this finding, a fluorometric method was designed for the turn-on detection of vitamin C. Under optimal conditions, the method has a low detection limit (0.47 μM) and a linear response in the 0.5 μM to 20 μM a concentration range. It was successfully applied to the determination of vitamin C in spiked red grape and orange juice, and in vitamin C tablets. Graphical abstract A target-triggered dissociation of quencher-based strategy for the fluorescence "turn-on" detection of vitamin C was developed. It is based on surface energy transfer (SET) and an inner filter effect (IFE) between silicon nanoparticles and CoOOH nanoparticles as well as the redox reaction between vitamin C and CoOOH nanoparticles.

Published

2019

15. Reconsidering the H&E stain as the gold standard in assessing the depth of burn wounds.

Author

Rosenberg AS

Subjects

Burns diagnosis, Fluorescent Dyes economics, Fluorescent Dyes standards, Humans, L-Lactate Dehydrogenase standards, Molecular Imaging methods, Reproducibility of Results, Skin pathology, Staining and Labeling methods, Tissue Survival immunology, Burns pathology, Coloring Agents standards, Staining and Labeling standards

Abstract

While histological examination is considered by most as the gold standard for burn depth assessment, it has no practical use in the clinical setting. It has, however, been used in the research setting, as a mean for evaluating emerging techniques of depth measurement. Due to the limitations of the H&E stain, other stains have also been explored, such as lactate dehydrogenase (LDH), as presented in this issue, in "Improving the Histologic Characterization of Burn Depth." As the determination of burn depth is not a typical subject in dermatopathology, a summary of selected techniques and the possible role for the LDH stain in future research, is described herein., (© 2017 John Wiley & Sons A/S. Published by John Wiley & Sons Ltd.)

Published

2017

16. An ultrasensitive stain for negative protein detection in SDS-PAGE via 4',5'-Dibromofluorescein.

Author

Yu D, Wang Y, Zhang S, Chen Z, Xue M, Wang Y, Cong W, Jin L, and Zhu Z

Subjects

Fluoresceins chemistry, Fluorescent Dyes chemistry, Molecular Docking Simulation, Time Factors, Electrophoresis, Polyacrylamide Gel methods, Fluoresceins standards, Fluorescent Dyes standards, Proteins analysis, Staining and Labeling standards

Abstract

A highly sensitive method for brief and economical staining of proteins in 1-D and 2-D sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) by 4',5'-Dibromofluorescein (DBF) was developed in this study. Down to 0.025-0.05ng protein could be detected within 10min (only 2 steps) by DBF stain, which is approximately 10-fold more sensitive than those of Eosin Y (EY) and SYPRO Ruby stains, and 20-fold more sensitive than that of imidazole-zinc (IZ) negative stain. In addition, the LC-MS/MS results indicated that the newly developed staining method is compatible with the downstream protein identification. Moreover, the mechanism of DBF stain was investigated by molecular docking., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

17. Design, installation, and performance evaluation of a custom dye matrix standard for automated capillary electrophoresis.

Author

Cloete KW, Ristow PG, Kasu M, and D'Amato ME

Subjects

Automation, Laboratory methods, Electrophoresis, Capillary methods, Fluorescent Dyes chemistry, Genotyping Techniques methods, Research Design, Automation, Laboratory standards, Electrophoresis, Capillary standards, Fluorescent Dyes analysis, Fluorescent Dyes standards, Genotyping Techniques standards

Abstract

CE equipment detects and deconvolutes mixtures containing up to six fluorescently labeled DNA fragments. This deconvolution is done by the collection software that requires a spectral calibration file. The calibration file is used to adjust for the overlap that occurs between the emission spectra of fluorescence dyes. All commercial genotyping and sequencing kits require the installation of a corresponding matrix standard to generate a calibration file. Due to the differences in emission spectrum overlap between fluorescent dyes, the application of existing commercial matrix standards to the electrophoretic separation of DNA labeled with other fluorescent dyes can yield undesirable results. Currently, the number of fluorescent dyes available for oligonucleotide labeling surpasses the availability of commercial matrix standards. Therefore, in this study we developed and evaluated a customized matrix standard using ATTO 633, ATTO 565, ATTO 550, ATTO Rho6G, and 6-FAM dyes for which no commercial matrix standard is available. We highlighted the potential genotyping errors of using an incorrect matrix standard by evaluating the relative performance of our custom dye set using six matrix standards. The specific performance of two genotyping kits (UniQTyper™ Y-10 version 1.0 and PowerPlex® Y23 System) was also evaluated using their specific matrix standards. The procedure we followed for the construction of our custom dye matrix standard can be extended to other fluorescent dyes., (© 2016 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2017

18. Optimizing probes to image cleared tissue.

Author

Marx V

Subjects

Animals, Fluorescent Dyes chemistry, Humans, Molecular Probes chemistry, Brain diagnostic imaging, Cell Physiological Phenomena, Fluorescent Dyes standards, Molecular Imaging methods, Molecular Probes standards

Published

2016

19. Development of real-time PCR for detection and quantitation of Streptococcus parauberis.

Author

Nguyen TL, Lim YJ, Kim DH, and Austin B

Subjects

Animals, DNA Gyrase genetics, DNA Primers standards, DNA, Bacterial analysis, Fisheries, Fluorescent Dyes standards, Gene Dosage, Intestinal Mucosa microbiology, Kidney microbiology, Real-Time Polymerase Chain Reaction standards, Reproducibility of Results, Sensitivity and Specificity, Spleen microbiology, Streptococcal Infections microbiology, Streptococcus genetics, Streptococcus growth & development, Fish Diseases microbiology, Flounder, Real-Time Polymerase Chain Reaction veterinary, Streptococcal Infections veterinary, Streptococcus isolation & purification

Abstract

Streptococcus parauberis is an increasing threat to aquaculture of olive flounder, Paralichthys olivaceus Temminck & Schlegel, in South Korea. We developed a real-time polymerase chain reaction (PCR) method using the TaqMan probe assay to detect and quantify S. parauberis by targeting the gyrB gene sequences, which are effective for molecular analysis of the genus Streptococcus. Our real-time PCR assay is capable of detecting 10 fg of genomic DNA per reaction. The intra- and interassay coefficient of variation (CV) values ranged from 0.42-1.95%, demonstrating that the assay has good reproducibility. There was not any cross-reactivity to Streptococcus iniae or to other streptococcal/lactococcal fish pathogens, such as S. agalactiae and Lactococcus garvieae, indicating that the assay is highly specific to S. parauberis. The results of the real-time PCR assay corresponded well to those of conventional culture assays for S. parauberis from inoculated tissue homogenates (r = 0.957; P < 0.05). Hence, this sensitive and specific real-time PCR is a valuable tool for diagnostic quantitation of S. parauberis in clinical samples., (© 2014 John Wiley & Sons Ltd.)

Published

2016

20. Using the Peggy Simple Western system for fine needle aspirate analysis.

Author

Gentalen ET and Proctor JM

Subjects

Animals, Automation, Electrophoresis, Capillary, Equipment Design, Fluorescent Dyes standards, Humans, Mice, Neoplasms, Experimental pathology, Biopsy, Fine-Needle, Blotting, Western instrumentation, Blotting, Western methods

Abstract

Simple Western™ assays are capillary-based electrophoretic immunoassays, similar in scope to SDS-PAGE (molecular weight separation, "size") and IEF (isoelectric focusing, "charge") immunoblotting. The enhanced sensitivity and automation of the Simple Western makes it better suited to cancer diagnostics and research than the traditional Western platform. Because of its smaller sample volume requirements, primary cells, such as those obtained from fine needle aspirates (FNAs), and solid tumor slices may be used to generate quantitative comparable data. The Peggy™ instrument is capable of performing either size or charge assays on up to 96 samples in a single unattended run.

Published

2015

21. Tailor made plasmin substrates as potential diagnostic tool to test for mastitis.

Author

Bikker FJ, Koop G, Leusink NB, Nazmi K, Kaman WE, Brand HS, and Veerman EC

Subjects

Animals, Cattle, Female, Fluorescent Dyes metabolism, Milk enzymology, Sensitivity and Specificity, Fibrinolysin metabolism, Fluorescent Dyes standards, Mastitis, Bovine diagnosis

Abstract

Plasmin is a protease in milk, which concentration is increased during mastitis. The aim of the study was design and characterize short, tailor made fluorogenic substrates for plasmin to see differences in plasmin activity in healthy milk compared to mastitic milk. According to the specificity matrix of plasmin, containing 125 currently known plasmin substrates, six novel plasmin specific substrates were designed and characterized. Eight other substrates were insensitive for plasmin, which was in line with our expectations. The plasmin-sensitive substrates showed no cross-reactivity with proteases from mastitogenic bacteria in vitro. A proof of concept to distinguish healthy milk from mastitic milk is described. Potentially, these substrates present a rapid alternative to the currently established methodologies to detect mastitis in milk.

Published

2014

22. Measuring the steady-state properties of Ca²⁺ indicators with a set of calibrated [Ca²⁺] solutions.

Author

Faas GC and Mody I

Subjects

Calibration, Solutions, Calcium analysis, Chemistry Techniques, Analytical methods, Fluorescent Dyes standards

Abstract

Fluorescent Ca(2+) indicators are widely used to measure the concentration of free Ca(2+) ([Ca(2+)]free) in biological processes. By calibrating the dye under the same experimental conditions as employed during its planned use, the actual [Ca(2+)] can be calculated from the measured fluorescence. When using non ratiometric dyes, such as the Oregon Green BAPTA (OGB) family of dyes or the Fluo dyes, the steady-state affinity (K(d)) and the ratio between the maximal and minimal fluorescence (F(ratio) = F(max)/F(min)) of the particular dye are needed for this conversion. Although these values are usually given by the manufacturer, we consistently find that the actual values can differ between various batches delivered by the companies that make the dyes. In this protocol, we provide the recipe for a series of solutions with a known and tightly buffered [Ca(2+)](free) and describe how to use these mixtures to determine the exact K(d) and F(ratio) of a fluorescent Ca(2+) dye., (© 2014 Cold Spring Harbor Laboratory Press.)

Published

2014

23. A highly sensitive fluorescent indicator dye for calcium imaging of neural activity in vitro and in vivo.

Author

Tada M, Takeuchi A, Hashizume M, Kitamura K, and Kano M

Subjects

Action Potentials, Aniline Compounds pharmacology, Aniline Compounds standards, Animals, Calcium Signaling, Cells, Cultured, Fluoresceins pharmacology, Fluoresceins standards, Fluorescent Dyes pharmacology, Male, Mice, Mice, Inbred C57BL, Neocortex cytology, Neocortex metabolism, Purkinje Cells drug effects, Purkinje Cells physiology, Pyramidal Cells drug effects, Pyramidal Cells physiology, Signal-To-Noise Ratio, Calcium metabolism, Fluorescent Dyes standards, Microscopy, Fluorescence methods, Purkinje Cells metabolism, Pyramidal Cells metabolism

Abstract

Calcium imaging of individual neurons is widely used for monitoring their activity in vitro and in vivo. Synthetic fluorescent calcium indicator dyes are commonly used, but the resulting calcium signals sometimes suffer from a low signal-to-noise ratio (SNR). Therefore, it is difficult to detect signals caused by single action potentials (APs) particularly from neurons in vivo. Here we showed that a recently developed calcium indicator dye, Cal-520, is sufficiently sensitive to reliably detect single APs both in vitro and in vivo. In neocortical neurons, calcium signals were linearly correlated with the number of APs, and the SNR was > 6 for in vitro slice preparations and > 1.6 for in vivo anesthetised mice. In cerebellar Purkinje cells, dendritic calcium transients evoked by climbing fiber inputs were clearly observed in anesthetised mice with a high SNR and fast decay time. These characteristics of Cal-520 are a great advantage over those of Oregon Green BAPTA-1, the most commonly used calcium indicator dye, for monitoring the activity of individual neurons both in vitro and in vivo., (© 2014 The Authors. European Journal of Neuroscience published by Federation of European Neuroscience Societies and John Wiley & Sons Ltd.)

Published

2014

24. Guidelines on the use of multicolour flow cytometry in the diagnosis of haematological neoplasms. British Committee for Standards in Haematology.

Author

Johansson U, Bloxham D, Couzens S, Jesson J, Morilla R, Erber W, and Macey M

Subjects

Humans, Antibodies, Neoplasm immunology, Antigen-Antibody Reactions, Antigens, Neoplasm immunology, Blood Cells pathology, Bone Marrow Examination, Calibration standards, Color, Drug Storage standards, Equipment Design standards, Fluorescent Dyes standards, Forms and Records Control, Indicators and Reagents, Lasers standards, Medical Laboratory Personnel education, Quality Control, Reproducibility of Results, Specimen Handling standards, United Kingdom, Flow Cytometry instrumentation, Flow Cytometry methods, Flow Cytometry standards, Hematologic Neoplasms diagnosis, Hematologic Neoplasms pathology, Immunophenotyping methods, Immunophenotyping standards

Published

2014

25. Tandem dyes: Stability in cocktails and compensation considerations.

Author

Johansson U and Macey M

Subjects

Antibodies, Monoclonal chemistry, Color, Cryopreservation, Freeze Drying, Humans, Immunoconjugates chemistry, Signal-To-Noise Ratio, Bone Marrow Cells cytology, Carbocyanines standards, Flow Cytometry standards, Fluorescent Dyes standards, Phycoerythrin standards

Abstract

Background: The stability and performance of tandem-conjugated antibodies can be impaired when stored in antisera cocktails (Biancotto et al., J Immunol Methods 2011;363:245-261; Rawstron et al., Leukemia 2013;27:142-149). This, and the need for frequent re-compensation due to the possible spectral spillover variation between tandem lots, reduces the robustness of clinical flow cytometry panels that include tandems. Since tandems are required for standard 8-10 color screens, further studies of the stability of tandems in cocktails and their spillover variability are warranted., Methods: The performance of PE- and APC-tandems stored in cocktails was tested on fresh bone marrow, preserved blood and lyophilized cell samples over 1-, 6-, or 8-week periods, respectively, and their spillover matrices were compared. The observed correction factor differences were used as the basis for analyzing how the application of an incorrect compensation matrix could influence data interpretation., Results: Signal intensities and background fluorescence remained constant for all fluorochromes in the cocktails tested. Spillover correction factors for different PE-Cy7 mAbs did not exceed or were only marginally higher than those for non-tandem organic dye-conjugated mAb. By applying the correction factor differences observed between tandem mAb lots to clinical data, it was found that the over and under compensation would not alter the clinical interpretation., Conclusions: Tandems can be safely stored and used in cocktails. However, each cocktail should be tested on relevant material prior to use. Exact compensation settings are a requirement for accurate data. Provided that careful evaluation of tandem compensation requirements is carried out, certain tandems may use a generic compensation matrix., (© 2013 Clinical Cytometry Society.)

Published

2014

26. Improving the sensitivity of confocal laser induced fluorescence detection to the sub-picomolar scale for round capillaries by laterally shifting the laser focus point.

Author

Zhu Y, Chen N, Li Q, and Fang Q

Subjects

Electrophoresis, Capillary methods, Electrophoresis, Capillary standards, Fluorescent Dyes chemistry, Microscopy, Confocal methods, Microscopy, Confocal standards, Microscopy, Fluorescence methods, Microscopy, Fluorescence standards, Fluorescent Dyes standards, Lasers standards, Nanotechnology methods, Nanotechnology standards

Abstract

This paper describes a simple and efficient approach to reduce the background level of confocal laser induced fluorescence (LIF) detection for round capillaries by laterally shifting the laser focus point. A phenomenon of spontaneous separation of the fluorescence and reflected laser beams at the pinhole of a confocal LIF system when the laser focus point deviates from the center of a capillary channel to the sides was observed for the first time. On the basis of this phenomenon, the reflected laser light from the capillary-air interfaces could be mostly eliminated with a spatial filtering pinhole. A comprehensive study on the phenomenon and optimization of the shift distance was carried out using both experimental and simulation methods. A best shift distance of ±20 μm was obtained, with which background intensity could be significantly reduced by 98.9%, while fluorescence intensity was only reduced by 25.7%, resulting in an improvement of signal-to-noise ratio of 8.3 times, compared with that at a shift distance of 0 μm usually used in most of the confocal LIF systems for round capillaries. A limit of detection of 66 fM was obtained for sodium fluorescein. To demonstrate its potential as an on-column sensitive detector for microscale separation systems, the present system was coupled with a capillary electrophoresis system for separation of four fluorescein isothiocyanate labeled amino acids with concentrations of 100 pM.

Published

2013

27. Terbium fluorescence as a sensitive, inexpensive probe for UV-induced damage in nucleic acids.

Author

El-Yazbi AF and Loppnow GR

Subjects

Fluorescence, Fluorescent Dyes economics, Fluorescent Dyes standards, Nucleic Acids analysis, Nucleic Acids radiation effects, Terbium economics, Terbium standards, DNA Damage radiation effects, Fluorescent Dyes chemistry, Oligonucleotides analysis, Oligonucleotides radiation effects, Terbium chemistry, Ultraviolet Rays adverse effects

Abstract

Much effort has been focused on developing methods for detecting damaged nucleic acids. However, almost all of the proposed methods consist of multi-step procedures, are limited, require expensive instruments, or suffer from a high level of interferences. In this paper, we present a novel simple, inexpensive, mix-and-read assay that is generally applicable to nucleic acid damage and uses the enhanced luminescence due to energy transfer from nucleic acids to terbium(III) (Tb(3+)). Single-stranded oligonucleotides greatly enhance the Tb(3+) emission, but duplex DNA does not. With the use of a DNA hairpin probe complementary to the oligonucleotide of interest, the Tb(3+)/hairpin probe is applied to detect ultraviolet (UV)-induced DNA damage. The hairpin probe hybridizes only with the undamaged DNA. However, the damaged DNA remains single-stranded and enhances the intrinsic fluorescence of Tb(3+), producing a detectable signal directly proportional to the amount of DNA damage. This allows the Tb(3+)/hairpin probe to be used for sensitive quantification of UV-induced DNA damage. The Tb(3+)/hairpin probe showed superior selectivity to DNA damage compared to conventional molecular beacons probes (MBs) and its sensitivity is more than 2.5 times higher than MBs with a limit of detection of 4.36±1.2 nM. In addition, this probe is easier to synthesize and more than eight times cheaper than MBs, which makes its use recommended for high-throughput, quantitative analysis of DNA damage., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013

28. [Another discussion of membrane voltage alterations in growing pollen tube].

Author

Breĭgina MA, Smirnova AV, Matveeva NP, and Ermakov IP

Subjects

Barbiturates standards, Fluorescent Dyes standards, Ion Transport, Isoxazoles standards, Pollen physiology, Pollen Tube growth & development, Pyridinium Compounds standards, Cell Membrane metabolism, Membrane Potentials physiology, Pollen Tube metabolism, Nicotiana physiology

Abstract

Here we give a critical analysis of the opinion of Andreev (2011) on membrane potential distribution along the pollen tube plasmalemma. He assumes that a lateral gradient of dipole potential exists, but suggests a lateral gradient of transmembrane potential impossible. We demonstrate by concrete examples that the argumentation of the initiator of discussion is based on inaccurate citation of our experimental data (Breygina et al., 2009) and incomplete analysis of previously published articles. Speaking about transmembrane potential, he doesn't consider numerous facts demonstrating the uneven distribution of transmembrane ion fluxes and ion-transport proteins in the pollen tube plasmalemma, as well as data obtained by modeling of transmembrane potential distribution in objects of different shape. In addition, the assumption on the uneven distribution of dipole potential doesn't have an experimental basis neither in studies of the pollen tube, nor in the practice of using fluorescent voltage-sensitive dyes DiBAC4(3) and Di-4-ANEPPS. We are expecting the author to obtain experimental data in support of his position.

Published

2012

29. Calibration of fluorescent calcium indicators.

Author

Helmchen F

Subjects

Fluorescent Dyes metabolism, Indicators and Reagents metabolism, Calcium analysis, Cytological Techniques methods, Cytological Techniques standards, Fluorescent Dyes standards, Indicators and Reagents standards

Published

2011

30. Calibration protocols for fluorescent calcium indicators.

Author

Helmchen F

Subjects

Fluorescent Dyes metabolism, Indicators and Reagents metabolism, Calcium analysis, Cytological Techniques methods, Cytological Techniques standards, Fluorescent Dyes standards, Indicators and Reagents standards

Published

2011

31. Quantification and calibration of images in fluorescence microscopy.

Author

Baskin DS, Widmayer MA, and Sharpe MA

Subjects

Animals, Calibration, Cell Line, Tumor, DNA analysis, DNA standards, Fluorescent Dyes analysis, Fluorescent Dyes standards, Gelatin chemistry, Humans, Microscopy, Fluorescence instrumentation, Microscopy, Fluorescence standards, Oligonucleotides analysis, Oligonucleotides standards, Phantoms, Imaging, Proteins analysis, Proteins standards, Swine, Temperature, Microscopy, Fluorescence methods

Abstract

Fluorescence microscopy is a method widely used in life sciences to image biological processes in living and fixed cells or in fixed tissues. Quantification and calibration of images in fluorescence microscopy is notoriously difficult. We have developed a new methodology to prepare tissue "phantoms" that contain known amounts of (i) fluorophore, (ii) DNA, (iii) proteins, and (iv) DNA oligonucleotide standards. The basis of the phantoms is the ability of gelatin to act as a matrix for the conjugation of fluorophores as either a free-flowing liquid or a gelatinous solid depending on temperature (> or = 40 and < or = 4 degrees C)., (2010 Elsevier Inc. All rights reserved.)

Published

2010

32. In-depth validation of acridine orange staining for flow cytometric parasite and reticulocyte enumeration in an experimental model using Plasmodium berghei.

Author

Hein-Kristensen L, Wiese L, Kurtzhals JA, and Staalsoe T

Subjects

Animals, Blood Preservation methods, Female, Malaria blood, Male, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Parasitemia parasitology, Plasmodium berghei isolation & purification, Rats, Rats, Sprague-Dawley, Rats, Wistar, Reticulocytes parasitology, Time Factors, Acridine Orange standards, Flow Cytometry standards, Fluorescent Dyes standards, Malaria parasitology, Plasmodium berghei growth & development, Reticulocyte Count standards

Abstract

Flow cytometry is potentially an effective method for counting malaria parasites, but inconsistent results have hampered its routine use in rodent models. A published two-channel method using acridine orange offers clear discrimination between the infected and uninfected erythrocytes. However, preliminary studies showed concerns when dealing with Plasmodium berghei-infected blood samples with high numbers of reticulocytes. In hyperparasitemic or chronic P. berghei infection, enhanced erythropoietic activity results in high numbers of circulating immature reticulocytes. We show that even though the protocol offered good discrimination in newly infected animals, discrimination between infected erythrocytes and uninfected reticulocytes became difficult in animals with hyperparasitemia or chronic infections maintained with subcurative treatment. Discrimination was especially hampered by increased nucleic acid content in immature uninfected reticulocytes. Our data confirms that though flow cytometry is a promising analytical tool in malaria research, care should still be taken when analysing samples from anemic or chronically infected animals.

Published

2009

33. Collisional quenching of erythrosine B as a potential reference dye for impulse response function evaluation.

Author

Szabelski M, Ilijev D, Sarkar P, Luchowski R, Gryczynski Z, Kapusta P, Erdmann R, and Gryczynski I

Subjects

Erythrosine standards, Feasibility Studies, Fluorescent Dyes standards, Reference Values, Reproducibility of Results, Sensitivity and Specificity, Spectrometry, Fluorescence standards, Algorithms, Erythrosine analysis, Erythrosine chemistry, Fluorescent Dyes analysis, Fluorescent Dyes chemistry, Potassium Iodide chemistry, Spectrometry, Fluorescence methods

Abstract

We studied the collisional quenching of the erythrosine B fluorophore by potassium iodide. The quenching follows a Stern-Volmer dependence up to the highest quencher concentration. The lifetime of erythrosine B decreases to 24 ps in 5.02 M of potassium iodide. The quantum yield of erythrosine B in the presence of 5.02 M KI is 0.0035. The relatively high brightness makes this compound attractive as an ultrashort reference in time-resolved measurements. In both frequency- and time-domain fluorescence techniques, there is a need for lifetime standards with extremely short decay times. Mimicking the instantaneous scattering at longer wavelengths allows color-effect-free measurements in the emission region. Another motivation is the problem of obtaining the impulse response function in the case of two-photon excitation. Time-resolved microscopy also benefits from fast-decaying dyes because the impulse response function can be evaluated at the emission wavelength of the investigated specimen without changing filters. We demonstrated that impulse response functions for commonly used detectors are practically the same for scattering as for quenched erythrosine B emission. We also analyzed a complex fluorescence decay using both elastic scattering and quenched erythrosine B emission as a response function.

Published

2009

34. Performance of fluorescent labels in sedimentation bead arrays--a comparison study.

Author

Mayr T, Moser C, and Klimant I

Subjects

Magnetics, Microspheres, Molecular Probe Techniques, Fluorescent Dyes standards, Nucleic Acid Hybridization methods, Oligonucleotides analysis

Abstract

An extensive study is described to identify the most suitable fluorescent label in magnetic microsphere sedimentation arrays. The investigated fluorescent labels, commonly used in multiplex analysis, include organic dyes, (fluorescein, Alexa488, Cy5) fluorescent proteins (R-Phycoerythrin, Allophycocyanine, PBXL-3) polymer nanoparticles (FluoSpheres, PD-Pt) and semiconductor nanocrystals (Quantum dots). DNA hybridization assays on magnetic microspheres were applied as model systems to reveal label performance. The fluorescent labels were characterized under optimized conditions regarding signal intensity, non-specific binding and photo-stability. The advantages and drawbacks of individual labels are discussed. The limit of detection and dynamic ranges are determined to compare the performance of selected labels. Detection limits of 2 x 10(-10) mol/L are found for the determination of oligonucleotides using PBXl-3 as label, which is comparable with typical flow cytometer systems. The results and protocols are highly valuable for any type of bead based assays and can be easily transferred.

Published

2009

35. Frequency-domain fluorescence lifetime measurements via frequency segmentation and recombination as applied to pyrene with dissolved humic materials.

Author

Marwani HM, Lowry M, Xing B, Warner IM, and Cook RL

Subjects

Adsorption, Fluorescent Dyes standards, Oxygen chemistry, Pyrenes standards, Solubility, Surface Properties, Time Factors, Fluorescence, Fluorescent Dyes chemistry, Humic Substances, Luminescent Measurements methods, Pyrenes chemistry

Abstract

In this study, the association behavior of pyrene with different dissolved humic materials (DHM) was investigated utilizing the recently developed segmented frequency-domain fluorescence lifetime method. The humic materials involved in this study consisted of three commercially available International Humic Substances Society standards (Suwannee River fulvic acid reference, SRFAR, Leonardite humic acid standard, LHAS, and Florida peat humic acid standard, FPHAS), the peat derived Amherst humic acid (AHA), and a chemically bleached Amherst humic acid (BAHA). It was found that the three commercial humic materials displayed three lifetime components, while both Amherst samples displayed only two lifetime components. In addition, it was found that the chemical bleaching procedure preferentially removed red wavelength emitting fluorophores from AHA. In regards to pyrene association with the DHM, different behavior was found for all commercially available humics, while AHA and BAHA, which displayed strikingly similar behavior in terms of fluorescence lifetimes. It was also found that there was an enhancement of pyrene's measured lifetime (combined with a decrease in pyrene emission) in the presence of FPHAS. The implications of this long lifetime are discussed in terms of (1) quenching mechanism and (2) use of the fluorescence quenching method used to determine the binding of compounds to DHM.

Published

2009

36. Optical monitoring of neuronal activity at high frame rate with a digital random-access multiphoton (RAMP) microscope.

Author

Otsu Y, Bormuth V, Wong J, Mathieu B, Dugué GP, Feltz A, and Dieudonné S

Subjects

Animals, Brain cytology, Calcium Signaling physiology, Cerebellar Cortex cytology, Cerebellar Cortex physiology, Cerebral Cortex cytology, Cerebral Cortex physiology, Dendritic Spines physiology, Dendritic Spines ultrastructure, Fluorescent Dyes standards, Image Cytometry instrumentation, Image Cytometry methods, Microscopy, Fluorescence, Multiphoton instrumentation, Neurons cytology, Neurophysiology instrumentation, Organ Culture Techniques, Purkinje Cells cytology, Purkinje Cells physiology, Pyramidal Cells cytology, Pyramidal Cells physiology, Rats, Rats, Wistar, Staining and Labeling methods, Synaptic Transmission physiology, Action Potentials physiology, Brain physiology, Microscopy, Fluorescence, Multiphoton methods, Neurons physiology, Neurophysiology methods, Optics and Photonics instrumentation

Abstract

Two-photon microscopy offers the promise of monitoring brain activity at multiple locations within intact tissue. However, serial sampling of voxels has been difficult to reconcile with millisecond timescales characteristic of neuronal activity. This is due to the conflicting constraints of scanning speed and signal amplitude. The recent use of acousto-optic deflector scanning to implement random-access multiphoton microscopy (RAMP) potentially allows to preserve long illumination dwell times while sampling multiple points-of-interest at high rates. However, the real-life abilities of RAMP microscopy regarding sensitivity and phototoxicity issues, which have so far impeded prolonged optical recordings at high frame rates, have not been assessed. Here, we describe the design, implementation and characterisation of an optimised RAMP microscope. We demonstrate the application of the microscope by monitoring calcium transients in Purkinje cells and cortical pyramidal cell dendrites and spines. We quantify the illumination constraints imposed by phototoxicity and show that stable continuous high-rate recordings can be obtained. During these recordings the fluorescence signal is large enough to detect spikes with a temporal resolution limited only by the calcium dye dynamics, improving upon previous techniques by at least an order of magnitude.

Published

2008

37. Two-photon absorption standards in the 550-1600 nm excitation wavelength range.

Author

Makarov NS, Drobizhev M, and Rebane A

Subjects

Internationality, Light, Photons, Reference Values, Algorithms, Fluorescent Dyes chemistry, Fluorescent Dyes standards, Microscopy, Fluorescence, Multiphoton standards, Spectrometry, Fluorescence standards

Abstract

We present absolute two-photon absorption (2PA) spectra of 15 commercial organic dyes covering an extended range of excitation wavelengths, 550-1600 nm. The 2PA is measured with an estimated accuracy +/-10% using a femtosecond fluorescence excitation method. The data are corrected for the variations of the pulse duration and the beam profile with the excitation wavelength, and are applicable as reference standards for 2PA measurements.

Published

2008

38. Single nucleotide specific detection of DNA by native chemical ligation of fluorescence labeled PNA-probes.

Author

Dose C and Seitz O

Subjects

Base Sequence, Fluorescence Resonance Energy Transfer, Fluorescent Dyes standards, DNA analysis, Fluorescent Dyes chemistry, Molecular Probe Techniques standards, Peptide Nucleic Acids

Abstract

DNA-directed chemical ligations provide the opportunity to diagnose DNA sequences with very high sequence specificity. Fluorescent labels have been attached to reactive probes to enable the homogeneous detection of DNA and RNA. However, it has frequently been found that the attachment of fluorescent labels results in decreases of ligation fidelity. Herein we describe the development of a fluorogenic ligation reaction that provides for 10(2)-fold to perfect sequence selectivity. The reaction is based on the isocysteine-mediated native chemical PNA ligation. It is shown that DNA-induced rate accelerations of approximately 43.000-fold can be obtained through subtle variations of the ligation conditions. PNA-thioesters and isocysteine-PNA conjugates were labeled with FAM and TMR fluorophores, respectively. For gaining rapid synthetic access, a convenient on-resin labeling approach was developed. A new PNA monomer featuring an Alloc-protected lysine side chain was synthesized and coupled in solid-phase PNA synthesis. In the event of a ligation reaction the two fluorophores are brought into proximity. It is shown that fluorescence resonance energy transfer provides a positive fluorescence signal which is specific for product formation rather than for loss of starting materials. Single base mutations can be detected within minutes and with very high sequence selectivity at optimized conditions.

Published

2008

39. Increased efficiency of genetic profiling through quantity and quality assessment of fluorescently labeled oligonucleotide primers.

Author

Frasier TR and White BN

Subjects

Quality Control, Reference Standards, DNA Primers metabolism, DNA Primers standards, Fluorescent Dyes metabolism, Fluorescent Dyes standards, Gene Expression Profiling methods, Gene Expression Profiling standards

Abstract

Optimizing the amount of primer to use in PCR amplification is one of the most important steps when developing protocols for genetic profiling, where subtle changes in primer concentration result in major impacts on the amount of desired product that is amplified. However; there are frequently discrepancies between the reported and actual quantity of primers delivered by suppliers, resulting in a need for re-optimization of conditions between primer orders and limiting the ability to standardize conditions between laboratories. To increase the consistency of genetic profiling protocols, we have developed a simple method to assess the quantity and quality of fluorescently labeled primers and therefore standardize reaction conditions through time and across laboratories. The method is based on analysis by electrophoresis with an automated fluorescent DNA analyzer.

Published

2008

40. Surface trafficking of neurotransmitter receptor: comparison between single-molecule/quantum dot strategies.

Author

Groc L, Lafourcade M, Heine M, Renner M, Racine V, Sibarita JB, Lounis B, Choquet D, and Cognet L

Subjects

Animals, Diffusion, Fluorescent Dyes standards, Humans, Microscopy methods, Protein Transport physiology, Quantum Dots, Cell Membrane metabolism, Receptors, Neurotransmitter metabolism, Staining and Labeling methods, Synaptic Transmission physiology

Published

2007

41. Analyzing B cell chronic lymphocytic leukemia with Oncomark tubes on a FACSCanto.

Author

Warzynski MJ and Rawlings PL Jr

Subjects

Antibodies immunology, Antibody Specificity immunology, Flow Cytometry standards, Fluorescent Antibody Technique standards, Fluorescent Dyes standards, Humans, Leukemia, Lymphocytic, Chronic, B-Cell blood, Leukemia, Lymphocytic, Chronic, B-Cell immunology, Predictive Value of Tests, Quality Control, Reproducibility of Results, User-Computer Interface, Flow Cytometry instrumentation, Flow Cytometry methods, Leukemia, Lymphocytic, Chronic, B-Cell diagnosis

Published

2007

42. Fluorescence imaging study of extracellular zinc at the hippocampal mossy fiber synapse.

Author

Bastian C and Li YV

Subjects

Animals, Calcium analysis, Calcium metabolism, Extracellular Space metabolism, Fluoresceins standards, Hippocampus cytology, Indicators and Reagents standards, Male, Membrane Potentials drug effects, Membrane Potentials physiology, Mossy Fibers, Hippocampal drug effects, Mossy Fibers, Hippocampal ultrastructure, Organ Culture Techniques, Polycyclic Compounds standards, Potassium Chloride pharmacology, Rats, Rats, Sprague-Dawley, Synapses drug effects, Synapses ultrastructure, Synaptic Transmission physiology, Zinc analysis, Fluorescent Dyes standards, Hippocampus metabolism, Microscopy, Fluorescence methods, Mossy Fibers, Hippocampal metabolism, Synapses metabolism, Zinc metabolism

Abstract

Although synaptically released, vesicular Zn(2+) has been proposed to play a neuromodulatory or neuronal signaling role at the mossy fiber-CA3 synapse, Zn(2+) release remains controversial, especially when detected using fluorescent imaging. In the present study, we investigated synaptically released Zn(2+) at the mossy fiber (MF) synapse in rat hippocampal slices using three chemically distinct, fluorescent Zn(2+) indicators. The indicators employed for this study were cell membrane impermeable (or extracellular) Newport Green [K(DZn2+) approximatelly 1 microM] , Zinpyr-4 K(DZn2+) approximately 1 nM and FluoZin-3 K(DZn2+) approximately 15 nM, chosen, in part, for their distinct dissociation constants. Among the three indicators, FluoZin-3 was also sensitive to Ca(2+) K(DCa2+) approximately 200-300 microM which was present in the extracellular medium ([Ca(2+)](o)>2mM). Hippocampal slices loaded with either Newport Green or FluoZin-3 showed increases in fluorescence after electrical stimulation of the mossy fiber pathway. These results are consistent with previous studies suggesting the presence of synaptically released Zn(2+) in the extracellular space during neuronal activities; however, the rise in FluoZin-3 fluorescence observed was complicated by the data that the addition of exogenous Zn(2+) onto FluoZin-3 loaded slices gave little change in fluorescence. In the slices loaded with the high-affinity indicator Zinpyr-4, there was little change in fluorescence after mossy fiber activation by electrical stimulation. Further study revealed that the sensitivity of Zinpyr-4 was mitigated by saturation with Zn(2+) contamination from the slice. These data suggest that the sensitivity and selectivity of a probe may affect individual outcomes in a given experimental system.

Published

2007

43. Fluorescence microscopy--avoiding the pitfalls.

Author

Brown CM

Subjects

Animals, Artifacts, Cytological Techniques methods, Cytological Techniques standards, Cytological Techniques trends, Humans, Image Cytometry instrumentation, Image Cytometry methods, Image Cytometry standards, Microscopy, Confocal instrumentation, Microscopy, Confocal methods, Microscopy, Confocal standards, Microscopy, Fluorescence instrumentation, Software standards, Software trends, Fluorescent Dyes standards, Microscopy, Fluorescence methods, Microscopy, Fluorescence standards

Published

2007

44. The development of quantum dot calibration beads and quantitative multicolor bioassays in flow cytometry and microscopy.

Author

Wu Y, Campos SK, Lopez GP, Ozbun MA, Sklar LA, and Buranda T

Subjects

Biotin chemistry, Calibration standards, Evaluation Studies as Topic, Flow Cytometry methods, Fluorescent Antibody Technique standards, Fluorescent Dyes chemistry, Fluorescent Dyes standards, Humans, Microscopy, Fluorescence methods, Molecular Probe Techniques, Reference Standards, Streptavidin chemistry, Tumor Cells, Cultured, Biosensing Techniques methods, Flow Cytometry standards, Microscopy, Fluorescence standards, Microspheres, Nanotechnology methods, Quantum Dots

Abstract

The use of fluorescence calibration beads has been the hallmark of quantitative flow cytometry. It has enabled the direct comparison of interlaboratory data as well as quality control in clinical flow cytometry. In this article, we describe a simple method for producing color-generalizable calibration beads based on streptavidin functionalized quantum dots. Based on their broad absorption spectra and relatively narrow emission, which is tunable on the basis of dot size, quantum dot calibration beads can be made for any fluorophore that matches their emission color. In an earlier publication, we characterized the spectroscopic properties of commercial streptavidin functionalized dots (Invitrogen). Here we describe the molecular assembly of these dots on biotinylated beads. The law of mass action is used to readily define the site densities of the dots on the beads. The applicability of these beads is tested against the industry standard, namely commercial fluorescein calibration beads. The utility of the calibration beads is also extended to the characterization surface densities of dot-labeled epidermal growth factor ligands as well as quantitative indicators of the binding of dot-labeled virus particles to cells.

Published

2007

45. Flow cytometric CD34+ stem cell enumeration: lessons from nine years' external quality assessment within the Benelux countries.

Author

Levering WH, Preijers FW, van Wieringen WN, Kraan J, van Beers WA, Sintnicolaas K, van Rhenen DJ, and Gratama JW

Subjects

Belgium, Blood Cell Count instrumentation, Blood Cell Count methods, Flow Cytometry instrumentation, Fluorescent Dyes standards, Humans, Luxembourg, Netherlands, Quality Control, Reagent Kits, Diagnostic standards, Reference Values, Retrospective Studies, Time Factors, Antigens, CD34 analysis, Blood Cell Count standards, Flow Cytometry methods, Hematopoietic Stem Cells cytology

Abstract

Background: A biannual external quality assurance (EQA) scheme for flow cytometric CD34+ haematopoietic stem cell enumeration has been operational in the Benelux countries since 1996. In an evaluation of the results of 16 send-outs, we studied the effects of the methods used on assay outcome and whether or not this exercise was effective in reducing between-laboratory variation., Methods: Data were analyzed using robust multivariate regression. This approach is relatively insensitive to outliers and is used to assess the effect of methodological aspects of CD34+ cell counting on the bias and variability., Results: Five variables were associated with significant bias of absolute CD34+ cell counts: (i) unique laboratory number (ULN), (ii) gating strategy; (iii) CD34 mAb fluorochrome; (iv) type of flow cytometer, and (v) method of sample preparation. In addition, ULN and platform methodology (i.e., single vs. dual) contributed significantly to the variability of this assay. Overall, the variability in results of CD34+ cell enumeration has declined with time; in particular, after a practical workshop in which participants were trained to use the "single platform ISHAGE protocol.", Conclusions: Between-laboratory variation in CD34+ cell enumeration can be reduced by standardization of methodologies between centres. Our approach, i.e., EQA with targeted training and feedback in response to reported results, has been successful in reducing the variability of CD34+ cell enumeration between participants., (Copyright 2007 Clinical Cytometry Society.)

Published

2007

46. Assessing detection methods for gel-based proteomic analyses.

Author

Harris LR, Churchward MA, Butt RH, and Coorssen JR

Subjects

Animals, Coloring Agents chemistry, Fluorescent Dyes chemistry, Mice, Sensitivity and Specificity, Coloring Agents standards, Electrophoresis, Gel, Two-Dimensional standards, Fluorescent Dyes standards, Proteins analysis, Proteomics standards

Abstract

Proteomic analyses using two-dimensional gel electrophoresis (2DE) depend heavily upon the quality of protein stains for sensitive detection. Indeed, detection rather than protein resolution is likely a current limiting factor in 2DE. The recent development of fluorescent protein stains has dramatically improved the sensitivity of in-gel protein detection and has enabled more accurate protein quantification. Here, we have evaluated the overall quality and relative cost of five commercially available fluorescent stains, Krypton, Deep Purple, Rubeo, Flamingo, and the most commonly used stain, Sypro Ruby (SR). All stains were found to be statistically comparable with regard to number of protein spots detected, but SR was superior with regard to fluorophore stability (e.g., capacity for repeated use of the stain solution). Notably, colloidal Coomassie Blue was also found to be comparable to SR when detected using an infrared fluorescence imaging system rather than standard densitometry. Thus, depending on available equipment and operating budgets, there are at least two high-sensitivity alternatives to achieve the best currently available in-gel protein detection: Sypro Ruby or Coomassie Blue.

Published

2007

47. From imaging to understanding: Frontiers in Live Cell Imaging, Bethesda, MD, April 19-21, 2006.

Author

Wang YL, Hahn KM, Murphy RF, and Horwitz AF

Subjects

Animals, Biosensing Techniques instrumentation, Biosensing Techniques methods, Biosensing Techniques standards, Biosensing Techniques trends, Computational Biology instrumentation, Computational Biology methods, Computational Biology trends, Eukaryotic Cells physiology, Fluorescent Dyes standards, Humans, Image Cytometry instrumentation, Image Cytometry trends, Microscopy instrumentation, Microscopy trends, Molecular Biology instrumentation, Molecular Biology trends, Organelles physiology, Organelles ultrastructure, Eukaryotic Cells cytology, Image Cytometry methods, Microscopy methods, Molecular Biology methods, Optics and Photonics instrumentation

Abstract

A recent meeting entitled Frontiers in Live Cell Imaging was attended by more than 400 cell biologists, physicists, chemists, mathematicians, and engineers. Unlike typical special topics meetings, which bring together investigators in a defined field primarily to review recent progress, the purpose of this meeting was to promote cross-disciplinary interactions by introducing emerging methods on the one hand and important biological applications on the other. The goal was to turn live cell imaging from a "technique" used in cell biology into a new exploratory science that combines a number of research fields.

Published

2006

48. The Calibration Kit Spectral Fluorescence Standards--a simple and certified tool for the standardization of the spectral characteristics of fluorescence instruments.

Author

Pfeifer D, Hoffmann K, Hoffmann A, Monte C, and Resch-Genger U

Subjects

Reference Standards, Spectrometry, Fluorescence methods, Temperature, Calibration standards, Fluorescence, Fluorescent Dyes standards, Spectrometry, Fluorescence instrumentation

Abstract

With the Calibration Kit Spectral Fluorescence Standards BAM-F001-BAM-F005, we developed a simple tool for the characterization of the relative spectral responsivity and the long-term stability of the emission channel of fluorescence instruments under routine measurement conditions thereby providing the basis for an improved comparability of fluorescence measurements and eventually standardization. This first set of traceable fluorescence standards, which links fluorescence measurements to the spectral radiance scale in the spectral range of 300-770 nm and has been optimized for spectrofluorometers, can be employed for different measurement geometries and can be adapted to different fluorescence techniques with proper consideration of the underlying measurement principles.

Published

2006

49. Calibration standards for multicenter clinical trials of fluorescence spectroscopy for in vivo diagnosis.

Author

Marín NM, MacKinnon N, MacAulay C, Chang SK, Atkinson EN, Cox D, Serachitopol D, Pikkula B, Follen M, and Richards-Kortum R

Subjects

Calibration standards, Diagnostic Imaging instrumentation, Equipment Failure Analysis standards, Multicenter Studies as Topic instrumentation, Quality Assurance, Health Care methods, Reference Standards, Reproducibility of Results, Sensitivity and Specificity, Spectrometry, Fluorescence instrumentation, United States, Diagnostic Imaging standards, Fluorescent Dyes analysis, Fluorescent Dyes standards, Multicenter Studies as Topic standards, Quality Assurance, Health Care standards, Spectrometry, Fluorescence standards

Abstract

In the context of clinical trials, calibration protocols for optical instruments that ensure measurement accuracy and the ability to carry out meaningful comparisons of data acquired from multiple instruments are required. A series of calibration standards and procedures are presented to assess technical feasibility of optical devices for cervical precancer detection. Measurements of positive and negative standards, and tissue are made with two generations of research grade spectrometers. Calibration accuracy, ability of standards to correct and account for changes in experimental conditions, and device components are analyzed. The relative frequency of measured calibration standards is investigated retrospectively using statistical analysis of trends in instrument performance. Fluorescence measurements of standards and tissue made with completely different spectrometers show good agreement in intensity and lineshape. Frequency of wavelength calibration standards is increased to every 2 h to compensate for thermal drifts in grating mount. Variations in illumination energy detected between standards and patient measurements require probe redesign to allow for simultaneous acquisition of illumination power with every patient measurement. The use of frequent and well-characterized standards enables meaningful comparison of data from multiple devices and unambiguous interpretation of experiments among the biomedical optics community.

Published

2006

50. Simultaneous analysis of intracellular pH and Ca2+ from cell populations.

Author

Martinez-Zaguilan R, Tompkins LS, Gillies RJ, and Lynch RM

Subjects

Benzopyrans standards, Calibration, Cell Line, Fluorescent Dyes standards, Fura-2 standards, Humans, Naphthols standards, Rhodamines standards, Spectrometry, Fluorescence, Benzopyrans analysis, Calcium analysis, Calcium Signaling, Fluorescent Dyes analysis, Fura-2 analysis, Hydrogen-Ion Concentration, Intracellular Space chemistry, Naphthols analysis, Rhodamines analysis

Published

2006