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Ligand internalization is a receptor-mediated endocytic process in which the cell will only take in an extracellular molecule if it binds to its specific receptor protein on the cell’s surface. It is an important cell signaling event, and Life Technologies offers a variety of fluorescent ligands targeted to common receptors.
Specific receptor-mediated endocytosis pathways can be investigated with fluorescent ligands including pHrodo dyes targeted to common receptors, including, EGF, LDL, and transferrin.
The most convenient, no-wash assay format uses pHrodo Red or pHrodo Green to allow discrimination of stages in the endocytic pathway from early endosome to lysosome formation with no quench or wash required.
pHrodo dyes are essentially non-fluorescent at neutral pH and exhibit increasing signal with a red or green readout respectively as the pH decreases. The increase in fluorescent signal can be used to monitor progression in the endocytic pathway.
Mouse monocyte/macrophage cells (MMM cells, ATCC) treated with transferrin conjugated with pHrodo Red in Live Cell Imaging Solution and counterstained with NucBlue® Live ReadyProbes Reagent. Punctate red spots are visible where labeled transferrin was internalized.
Specific receptor-mediated endocytosis pathways can be investigated with a variety of fluorescent ligands targeted to common receptors, including, EGF, LDL, and transferrin.
Alexa Fluor® dyes conjugated to a range of ligands provide a choice of wavelength options and single-emission measurement for each. Assays require a wash step to remove unbound conjugates from the cell surface or quenching of the extracellular signal.
Visualization of transferrin and transferrin receptors in A431 cells.
A431 cells incubated with green-fluorescent Alexa Fluor 488 transferrin, then fixed and permeabilized. Transferrin receptors were identified with anti–transferrin receptor, mouse IgG1 monoclonal antibody and visualized with red-fluorescent Alexa Fluor 555 goat anti–mouse IgG antibody. Yellow fluorescence indicates regions of co-localization. Nuclei were stained with DAPI.
Readout |
No-wash assay to image receptor-mediated endocytosis by fluorescence intensity
| |||
---|---|---|---|---|
Range |
Monitors early endosome to early lysosome formation
| |||
Vehicle |
EGF
|
Transferrin
| ||
Common filter set |
TRITC
|
FITC
|
TRITC
| |
Labels |
pHrodo Red
|
pHrodo Green
|
pHrodo Red
| |
Ex/Em (nm) |
560/585
|
509/533
|
560/585
| |
Signal-to-noise ratio | ||||
Photostability | ||||
Multiplexing |
Yes
| |||
Live cells |
Yes
| |||
Fixed cells |
No
| |||
Fixable |
Yes
| |||
Platforms* |
I, M, FC
| |||
Format |
20 µg
|
20 µg
|
1 mg
| |
Cat. No. | ||||
* I = Imaging, M = Microplate, FC = Flow cytometry. |
Readout |
Quench or wash-based assay to image receptor-mediated endocytosis by fluorescence intensity
| |||||
---|---|---|---|---|---|---|
Range |
Fluorescent signal is not modulated by endocytic progress
| |||||
Vehicle |
LDL
|
Transferrin
|
EGF
| |||
Common filter set |
Texas Red
|
FITC
|
FITC
|
Texas Red
|
FITC
|
TRITC
|
Labels |
Alexa Fluor 594
|
Alexa Fluor 488
|
Alexa Fluor 488
|
Alexa Fluor 594
|
Alexa Fluor 488
|
Alexa Fluor 555
|
Ex/Em (nm) |
590/617
|
495/519
|
495/519
|
590/617
|
495/519
|
555/565
|
Signal-to-noise ratio | ||||||
Photostability | ||||||
Bibliography | ||||||
Multiplexing |
Yes
| |||||
Live cells |
Yes
| |||||
Fixed cells |
No
| |||||
Fixable |
Yes
| |||||
Platforms* |
Imaging
| |||||
Format |
200 µL
|
200 µL
|
5 mg
|
5 mg
|
100 µg
|
100 µg
|
Cat. No. |
Readout |
No-wash assay to image receptor-mediated endocytosis by fluorescence intensity
| |||
---|---|---|---|---|
Range |
Monitors early endosome to early lysosome formation
| |||
Vehicle |
EGF
|
Transferrin
| ||
Common filter set |
TRITC
|
FITC
|
TRITC
| |
Labels |
pHrodo Red
|
pHrodo Green
|
pHrodo Red
| |
Ex/Em (nm) |
560/585
|
509/533
|
560/585
| |
Signal-to-noise ratio | ||||
Photostability | ||||
Multiplexing |
Yes
| |||
Live cells |
Yes
| |||
Fixed cells |
No
| |||
Fixable |
Yes
| |||
Platforms* |
I, M, FC
| |||
Format |
20 µg
|
20 µg
|
1 mg
| |
Cat. No. | ||||
* I = Imaging, M = Microplate, FC = Flow cytometry. |
Readout |
Quench or wash-based assay to image receptor-mediated endocytosis by fluorescence intensity
| |||||
---|---|---|---|---|---|---|
Range |
Fluorescent signal is not modulated by endocytic progress
| |||||
Vehicle |
LDL
|
Transferrin
|
EGF
| |||
Common filter set |
Texas Red
|
FITC
|
FITC
|
Texas Red
|
FITC
|
TRITC
|
Labels |
Alexa Fluor 594
|
Alexa Fluor 488
|
Alexa Fluor 488
|
Alexa Fluor 594
|
Alexa Fluor 488
|
Alexa Fluor 555
|
Ex/Em (nm) |
590/617
|
495/519
|
495/519
|
590/617
|
495/519
|
555/565
|
Signal-to-noise ratio | ||||||
Photostability | ||||||
Bibliography | ||||||
Multiplexing |
Yes
| |||||
Live cells |
Yes
| |||||
Fixed cells |
No
| |||||
Fixable |
Yes
| |||||
Platforms* |
Imaging
| |||||
Format |
200 µL
|
200 µL
|
5 mg
|
5 mg
|
100 µg
|
100 µg
|
Cat. No. |