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LysoBrite™ Blue

Lysosomes are cellular organelles which contain acid hydrolase enzymes to break up waste materials and cellular debris. Lysosomes digest excess or worn-out organelles, food particles, and engulfed viruses or bacteria. The membrane around a lysosome allows the digestive enzymes to work at pH 4.5. The interior of the lysosomes is acidic (pH 4.5-4.8) compared to the slightly alkaline cytosol (pH 7.2). The lysosome maintains this pH differential by pumping protons from the cytosol across the membrane via proton pumps and chloride ion channels. LysoBrite™ Blue selectively accumulates in lysosomes probably via the lysosome pH gradient. The lysotropic indicator is a hydrophobic compound that easily permeates intact live cells, and trapped in lysosomes after it gets into cells. Its fluorescence is significantly enhanced upon entering lysosomes. This key feature significantly reduces its staining background and makes it useful for a variety of studies, including cell adhesion, chemotaxis, multidrug resistance, cell viability, apoptosis and cytotoxicity. It is suitable for proliferating and non-proliferating cells, and can be used for both suspension and adherent cells.

Example protocol

AT A GLANCE

Assay Protocol with LysoBrite™ Blue
  1. Prepare cells.

  2. Add dye working solution.

  3. Incubate at 37 °C for 30 minutes.

  4. Wash the cells.

  5. Analyze under a fluorescence microscope.

Storage and Handling Conditions

The LysoBrite™ Blue stock solution provided is 500X in DMSO. It should be stable for at least 6 months if stored at -20°C. Protect from light, and avoid freeze/thaw cycles.  

PREPARATION OF WORKING SOLUTION

Prepare LysoBrite™ Blue Working Solution
  1. Warm LysoBrite™ Blue dye to room temperature.

  2. Prepare dye working solution by diluting 20 µL of 500X LysoBrite™ Blue with 10 mL of Hanks and 20 mM HEPES buffer (HBSS) or buffer of your choice.

    Note: 20 µL of LysoBrite™ Blue dye is enough for one 96-well plate. Aliquot and store unused LysoBrite™ dye stock solutions at < -15 °C. Protect it from light and avoid repeated freeze-thaw cycles.

    Note: The optimal concentration of the fluorescent lysosome indicator varies depending on the specific application. The staining conditions may be modified according to the particular cell type and the permeability of the cells or tissues to the probe. 

SAMPLE EXPERIMENTAL PROTOCOL

This protocol only provides a guideline and should be modified according to your specific needs.

Protocol for Preparing and Staining Adherent Cells
  1. Grow cells in a 96-well black wall/clear bottom plate (100 µL/well/96-well plate) or on coverslips inside a petri dish filled with the appropriate culture medium.

  2. When cells reach the desired confluence, add an equal volume of the dye-working solution (from Preparation of Working Solution Step 2). 

  3. Incubate the cells in a 37 °C, 5% CO2 incubator for 30 minutes.

  4. Wash the cells twice with pre-warmed (37 °C) Hanks and 20 mM HEPES buffer (HBSS) or buffer of your choice. Then fill the cell wells with HBSS or growth medium.

  5. Observe the cells using a fluorescence microscope fitted with the desired filter set.

    Note: It is recommended to increase either the labeling concentration or the incubation time to allow the dye to accumulate if the cells do not appear to be sufficiently stained.

Protocol for Preparing and Staining Suspension Cells
  1. Add an equal volume of the dye-working solution (from Preparation of Working Solution Step 2). 

  2. Incubate the cells in a 37 °C, 5% CO2 incubator for 30 minutes.

  3. Wash the cells twice with pre-warmed (37 °C) Hanks and 20 mM HEPES buffer (HBSS) or buffer of your choice. Then fill the cell wells with HBSS or growth medium.

  4. Observe the cells using a fluorescence microscope fitted with the desired filter set.

    Note: It is recommended to increase either the labeling concentration or the incubation time to allow the dye to accumulate if the cells do not appear to be sufficiently stained.

    Note: Suspension cells may be attached to coverslips treated with BD Cell-Tak® (BD Biosciences) and stained as adherent cells (see Protocol for Preparing and Staining Adherent Cells).

Spectrum

Product family

NameExcitation (nm)Emission (nm)
LysoBrite™ Green501510
LysoBrite™ Orange543565
LysoBrite™ Red576596
LysoBrite™ Deep Red597619
LysoBrite™ NIR636651

Citations

View all 9 citations: Citation Explorer
Identification of natural compound garcinone E as a novel autophagic flux inhibitor with anticancer effect in nasopharyngeal carcinoma cells
Authors: Wei, Dan and Wang, Luolin and Lei, Shunmei and Zhang, Han and Dong, Caihua and Ke, Yao and Su, Yuting and Chen, Xiaoying and Xia, Lianping and Kong, Xiaoyang and others,
Journal: Pharmaceutical Biology (2023): 839--857
LDHB inhibition induces mitophagy and facilitates the progression of CSFV infection
Authors: Fan, Shuangqi and Wu, Keke and Zhao, Mingqiu and Yuan, Jin and Ma, Shengming and Zhu, Erpeng and Chen, Yuming and Ding, Hongxing and Yi, Lin and Chen, Jinding
Journal: Autophagy (2020): 1--20
Apatite-Binding Nanoparticulate Agonist of Hedgehog Signaling for Bone Repair
Authors: Zhang, Xiao and Fan, Jiabing and Lee, Chung-Sung and Kim, Soyon and Chen, Chen and Aghaloo, Tara and Lee, Min
Journal: Advanced Functional Materials (2020): 1909218
A ratiometric fluorescent probe for detecting hypochlorite in the endoplasmic reticulum
Authors: Hou, Ji-Ting and Kim, Hyeong Seok and Duan, Chong and Ji, Myung Sun and Wang, Shan and Zeng, Lintao and Ren, Wen Xiu and Kim, Jong Seung
Journal: Chemical communications (2019): 2533--2536
Redox/ATP switchable theranostic nanoparticles for real-time fluorescence monitoring of doxorubicin delivery
Authors: Lin, Yi and Yang, Yidi and Yan, Jianqin and Chen, Jun and Cao, Jun and Pu, Yuji and Li, Li and He, Bin
Journal: Journal of Materials Chemistry B (2018): 2089--2103

References

View all 26 references: Citation Explorer
Requirements, features, and performance of high content screening platforms
Authors: Gough AH, Johnston PA.
Journal: Methods Mol Biol (2007): 41
A pharmaceutical company user's perspective on the potential of high content screening in drug discovery
Authors: Hoffman AF, Garippa RJ.
Journal: Methods Mol Biol (2007): 19
Optimizing the integration of immunoreagents and fluorescent probes for multiplexed high content screening assays
Authors: Giuliano KA., undefined
Journal: Methods Mol Biol (2007): 189
Past, present, and future of high content screening and the field of cellomics
Authors: Taylor DL., undefined
Journal: Methods Mol Biol (2007): 3
Automated high content screening for phosphoinositide 3 kinase inhibition using an AKT 1 redistribution assay
Authors: Wolff M, Haasen D, Merk S, Kroner M, Maier U, Bordel S, Wiedenmann J, Nienhaus GU, Valler M, Heilker R.
Journal: Comb Chem High Throughput Screen (2006): 339
Page updated on November 25, 2024

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Catalog Number22642
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Physical properties

Molecular weight

331.42

Solvent

DMSO

Spectral properties

Excitation (nm)

434

Emission (nm)

480

Storage, safety and handling

Certificate of OriginDownload PDF
H-phraseH303, H313, H333
Hazard symbolXN
Intended useResearch Use Only (RUO)
R-phraseR20, R21, R22

Storage

Freeze (< -15 °C); Minimize light exposure
UNSPSC12352200

Platform

Flow cytometer

Excitation405 nm laser
Emission450, 40 nm filter
Instrument specification(s)Pacific Blue channel

Fluorescence microscope

ExcitationDAPI filter set
EmissionDAPI filter set
Recommended plateBlack wall, clear bottom
Image of HeLa cells stained with LysoBrite™ Blue in a Costar black wall/clear bottom 96-well plate.
Image of HeLa cells stained with LysoBrite™ Blue in a Costar black wall/clear bottom 96-well plate.
Image of HeLa cells stained with LysoBrite™ Blue in a Costar black wall/clear bottom 96-well plate.