Advanced Fluorescence Microscopy Techniques—FRAP, FLIP, FLAP, FRET and FLIM

Ishikawa-Ankerhold, Hellen; Ankerhold, Richard; Drummen, Gregor P. C.

doi:10.3390/molecules17044047

Cited by 441 publications

(366 citation statements)

References 298 publications

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“…Subsequently, the binding of glucose to GBP induces a conformational change which may apparently bring closer both these two fluorescent proteins and therefore there is an increase in FRET efficiency. Several research workers have reported that FRET is apparently a very complex process when free and immobilized whole-cells or cell-free extracts are involved [19][20][21][22]. Regarding the differences in FRET efficiencies between the free and immobilized nanosensors, there are a number of factors affecting immobilized and soluble proteins such as restricted mobility on immobilization, chemical modification due to the immobilization method used, nature of the microenvironment and diffusion limitation [20].…”

Section: Glucose Assaymentioning

confidence: 99%

Non-enzymatic assay for glucose by using immobilized whole-cells of E. coli containing glucose binding protein fused to fluorescent proteins

Charneca

Karmali

Vieira

2015

Sensors and Actuators B: Chemical

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Genetically encoded nanosensor 3.2 mM High throughput glucose assay Immobilization on 96-well microtiter plates FRET a b s t r a c t Glucose monitoring in vivo is a crucial issue for gaining new understanding of diabetes. Glucose binding protein (GBP) fused to two fluorescent indicator proteins (FLIP) was used in the present study such as FLIP-glu-3.2 mM. Recombinant Escherichia coli whole-cells containing genetically encoded nanosensors as well as cell-free extracts were immobilized either on inner epidermis of onion bulb scale or on 96-well microtiter plates in the presence of glutaraldehyde. Glucose monitoring was carried out by Förster Resonance Energy Transfer (FRET) analysis due the cyano and yellow fluorescent proteins (ECFP and EYFP) immobilized in both these supports.The recovery of these immobilized FLIP nanosensors compared with the free whole-cells and cell-free extract was in the range of 50-90%. Moreover, the data revealed that these FLIP nanosensors can be immobilized in such solid supports with retention of their biological activity. Glucose assay was devised by FRET analysis by using these nanosensors in real samples which detected glucose in the linear range of 0-24 mM with a limit of detection of 0.11 mM glucose. On the other hand, storage and operational stability studies revealed that they are very stable and can be re-used several times (i.e. at least 20 times) without any significant loss of FRET signal. To author's knowledge, this is the first report on the use of such immobilization supports for whole-cells and cell-free extract containing FLIP nanosensor for glucose assay. On the other hand, this is a novel and cheap high throughput method for glucose assay.

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Section: Glucose Assaymentioning

confidence: 99%

Non-enzymatic assay for glucose by using immobilized whole-cells of E. coli containing glucose binding protein fused to fluorescent proteins

Charneca

Karmali

Vieira

2015

Sensors and Actuators B: Chemical

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“…1 Chip-based biomolecular analysis methods, such as DNA chips and protein chips, are also based on fluorescence imaging. The quality of fluorescence imaging and the sensitivity of fluorescence detection are generally evaluated by the signal-to-noise (S/N) ratio, which indicates the ratio between the fluorescence signal from a fluorophore and the background light.…”

Section: Introductionmentioning

confidence: 99%

High-Contrast Fluorescence Imaging Based on the Polarization Dependence of the Fluorescence Enhancement Using an Optical Interference Mirror Slide

Yasuda

Akimoto

2015

ANAL. SCI.

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High-contrast fluorescence imaging using an optical interference mirror (OIM) slide that enhances the fluorescence from a fluorophore located on top of the OIM surface is reported. To enhance the fluorescence and reduce the background light of the OIM, transverse-electric-polarized excitation light was used as incident light, and the transverse-magnetic-polarized fluorescence signal was detected. As a result, an approximate 100-fold improvement in the signal-to-noise ratio was achieved through a 13-fold enhancement of the fluorescence signal and an 8-fold reduction of the background light.

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“…The rapid progress of modern life science depends to a large extent on the use of advanced imaging techniques [1,2]. In particular, the design of fluorescent markers that can be genetically encoded and expressed in vivo have enormously contributed to our understanding of subcellular processes.…”

Section: Introductionmentioning

confidence: 99%

Cell shape recognition and segmentation in fluorescence microscopy images.

Anielski¹,

Beta²

2012

JCIS

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Many cellular processes involve the translocation of proteins from the cytosolic region to the cortex of the cell and vice versa. The dynamics of such processes is typically investigated by fluorescence imaging of GFP-labeled versions of these proteins. Quantitative analysis of the resulting fluorescence images requires image segmentation procedures that identify the cell within the image and subsequently divide the cell into a cytosolic and a cortical region to monitor the temporal evolution of the fluorescence signals within these parts of the cell separately. Here, we present an image segmentation protocol that we have developed for this type of data analysis. It consists of noise reduction, normalization, and thresholding steps to generate masks that define the cytosolic and the cortical regions of a cell. Based on these masks, the desired fluorescence signals can be extracted from the confocal microscopy images.

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Advanced Fluorescence Microscopy Techniques—FRAP, FLIP, FLAP, FRET and FLIM

Cited by 441 publications

References 298 publications

Non-enzymatic assay for glucose by using immobilized whole-cells of E. coli containing glucose binding protein fused to fluorescent proteins

Non-enzymatic assay for glucose by using immobilized whole-cells of E. coli containing glucose binding protein fused to fluorescent proteins

High-Contrast Fluorescence Imaging Based on the Polarization Dependence of the Fluorescence Enhancement Using an Optical Interference Mirror Slide

Cell shape recognition and segmentation in fluorescence microscopy images.

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