JavaScript is disabled in your browser. Please enable JavaScript to view this website.
AB326518

PE Anti-LAMP2 antibody [H4B4]

Be the first to review this product! Submit a review

|

(0 Publication)

Mouse Monoclonal LAMP2 antibody - conjugated to PE. Suitable for Flow Cyt and reacts with Human samples.

View Alternative Names

CD107b, Lysosome-associated membrane glycoprotein 2, LAMP-2, Lysosome-associated membrane protein 2, CD107 antigen-like family member B, LGP-96, LAMP2

8 Images
Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)
  • Flow Cyt

Supplier Data

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)

Flow cytometry surface staining pattern of anti-IgE stimulated human peripheral whole blood stained using ab326518 (concentration in sample 1.67 μg/ml).

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)
  • Flow Cyt

Supplier Data

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)

Analysis of the antibody staining profile was performed on blood leukocytes isolated from buffy coats. HCDM CDMaps standardized procedures (Kuzilkova D et al. Front Immunol. 2022;13 : 827898) were used for cell isolation and surface staining of blood leukocytes, with the modification of staining protocol using cytometry test tubes. ab326518 was used in concentration 5 µg/ml in stained blood sample (2 x 10^6 cells).

Flow Cytometry (Intracellular) - PE Anti-LAMP2 antibody [H4B4] (AB326518)
  • Flow Cyt (Intra)

Supplier Data

Flow Cytometry (Intracellular) - PE Anti-LAMP2 antibody [H4B4] (AB326518)

Expression profiling on peripheral blood subsets using ab326518. Intracellular staining, adaptive panel

Analysis of the antibody staining profile was performed on blood leukocytes isolated from buffy coats and permeabilized using EXCELLYSE XPerm buffer set.
HCDM CDMaps standardized procedures (Kuzilkova D et al. Front Immunol. 2022;13 : 827898) were used for leukocyte isolation.
Suspension of blood leukocytes isolated from buffy coats (2 x 10^6 cells) was added to the mixture of optimized backbone antibody panel (HLDA Adaptive) and Monocyte Blocking Buffer, vortexed and incubated for 20 min.
Next, EXCELLYSE XPerm buffer set was used for leukocytes permeabilization according to the instruction procedure.
ab326518 was used in concentration 5 µg/ml in stained blood sample (2 x 10^6cells).

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)
  • Flow Cyt

Supplier Data

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)

Separation of human CD107b positive CD203c positive basophils (red-filled) from CD107b negative lymphocytes (black-dashed) in flow cytometry analysis (surface staining) of anti-IgE stimulated human peripheral whole blood stained using ab326518 (concentration in sample 1.67 μg/ml).

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)
  • Flow Cyt

Supplier Data

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)

Flow cytometry multicolor surface staining pattern of anti-IgE stimulated human peripheral blood mononuclear cells stained using anti-human CD203c (NP4D6) APC antibody (10 μl reagent / 100 μl of peripheral whole blood) and ab326518 (concentration in sample 1.67 μg/ml).

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)
  • Flow Cyt

Supplier Data

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)

Expression profiling on peripheral blood subsets using ab326518. Adaptive panel

HCDM CDMaps standardized procedures (Kuzilkova D et al. Front Immunol. 2022;13 : 827898) were used for cell isolation and surface staining of blood leukocytes, with the modification of staining protocol using cytometry test tubes.
Suspension of blood leukocytes isolated from buffy coats (2 x 10^6 cells) was added to the mixture of ab326518 (5 µg/ml in stained blood sample) and Monocyte Blocking Buffer, vortexed and incubated for 20 min. Next, optimized backbone antibody panel (HLDA Adaptive) was added to test tubes, vortexed and incubated for 20 min. The residual erythrocytes were lysed with 2 ml of 10X diluted EXCELLYSE Easy solution and incubated for 10 min. Finally, samples were centrifuged (670 g, 5 min.), supernatant removed and the cell pellet was resuspended in 200 µl of PBS for acquisition.

Flow Cytometry (Intracellular) - PE Anti-LAMP2 antibody [H4B4] (AB326518)
  • Flow Cyt (Intra)

Supplier Data

Flow Cytometry (Intracellular) - PE Anti-LAMP2 antibody [H4B4] (AB326518)

Expression profiling on peripheral blood subsets using ab326518. Intracellular staining, innate panel

Analysis of the antibody staining profile was performed on blood leukocytes isolated from buffy coats and permeabilized using EXCELLYSE XPerm buffer set.
HCDM CDMaps standardized procedures (Kuzilkova D et al. Front Immunol. 2022;13 : 827898) were used for leukocyte isolation.
Suspension of blood leukocytes isolated from buffy coats (2 x 10^6cells) was added to the mixture of optimized backbone antibody panel (HLDA Innate) and Monocyte Blocking Buffer, vortexed and incubated for 20 min.
Next, EXCELLYSE XPerm buffer set was used for leukocytes permeabilization according to the instruction procedure.
ab326518 was used in concentration 5 µg/ml in stained blood sample (2 x 10^6 cells).

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)
  • Flow Cyt

Supplier Data

Flow Cytometry - PE Anti-LAMP2 antibody [H4B4] (AB326518)

Expression profiling on peripheral blood subsets using ab326518. Innate panel

HCDM CDMaps standardized procedures (Kuzilkova D et al. Front Immunol. 2022;13 : 827898) were used for cell isolation and surface staining of blood leukocytes, with the modification of staining protocol using cytometry test tubes.
Suspension of blood leukocytes isolated from buffy coats (2 x 10^6 cells) was added to the mixture of ab326518 (5 µg/ml in stained blood sample) and Monocyte Blocking Buffer, vortexed and incubated for 20 min. Next, optimized backbone antibody panel (HLDA Innate) was added to test tubes, vortexed and incubated for 20 min. The residual erythrocytes were lysed with 2 ml of 10X diluted EXCELLYSE Easy solution and incubated for 10 min. Finally, samples were centrifuged (670 g, 5 min.), supernatant removed and the cell pellet was resuspended in 200 µl of PBS for acquisition.

  • Unconjugated

    Anti-LAMP2 antibody [H4B4] - Lysosome Marker

  • 660 APC

    APC Anti-LAMP2 antibody [H4B4]

  • 519 Alexa Fluor® 488

    Alexa Fluor® 488 Anti-LAMP2 antibody [H4B4] - Lysosome Marker

  • Biotin

    Biotin Anti-LAMP2 antibody [H4B4] - Lysosome Marker

  • 578 PE

    PE Anti-LAMP2 antibody [H4B4] - Lysosome Marker

  • 667 PE/Cy5®

    PE/Cy5® Anti-LAMP2 antibody [H4B4] - Lysosome Marker

  • 387 mFluor™ UV375

    mFluor™ UV375 Anti-CD107b antibody [H4B4]

  • 454 mFluor™ Violet 450

    mFluor™ Violet 450 Anti-CD107b antibody [H4B4]

Key facts

Host species

Mouse

Clonality

Monoclonal

Clone number

H4B4

Isotype

IgG1

Light chain type

kappa

Conjugation

PE

Excitation/Emission

Ex: 480;565nm, Em: 578nm

Carrier free

No

Reacts with

Human

Applications

Flow Cyt

applications

Specificity

The mouse monoclonal antibody H4B4 recognizes an extracellular/luminal epitope of CD107b / LAMP-2, an extensively glycosylated 100-120 kDa widely expressed lysosome-associated protein.

style
left-column

Reactivity data

{ "title": "Reactivity Data", "filters": { "stats": ["", "Species", "Dilution Info", "Notes"], "tabs": { "all-applications": {"fullname" : "All Applications", "shortname": "All Applications"}, "FlowCyt" : {"fullname" : "Flow Cytometry", "shortname":"Flow Cyt"} }, "product-promise": { "all": "all", "testedAndGuaranteed": "tested", "guaranteed": "expected", "predicted": "predicted", "notRecommended": "not-recommended" } }, "values": { "Human": { "FlowCyt-species-checked": "testedAndGuaranteed", "FlowCyt-species-dilution-info": "", "FlowCyt-species-notes": "<p>Flow cytometry: The reagent is designed for analysis of human blood cells using 10 μl reagent / 100 μl of whole blood or 10^6 cells in a suspension. The content of a vial (1 ml) is sufficient for 100 tests. Intracellular and extracellular staining.</p>" } } }
style
left-column
style
left-column

Properties and storage information

Form
Liquid
Purification technique
Size-exclusion chromatography
Purification notes
Purified antibody is conjugated with R-phycoerythrin (PE) under optimum conditions. Unconjugated antibody and free fluorochrome are removed by size-exclusion chromatography.
Storage buffer
pH: 7.4 Preservative: 0.098% Sodium azide Constituents: PBS, 0.2% BSA
Shipped at conditions
Ambient - Can Ship with Ice
Appropriate short-term storage conditions
+4°C
Appropriate long-term storage conditions
+4°C
Storage information
Do Not Freeze|Store in the dark
style
left-column
style
left-column
style
left-column

Product protocols

For this product, it's our understanding that no specific protocols are required. You can visit:
style
left-column

Target data

Lysosomal membrane glycoprotein which plays an important role in lysosome biogenesis, lysosomal pH regulation and autophagy (PubMed : 11082038, PubMed : 18644871, PubMed : 24880125, PubMed : 27628032, PubMed : 36586411, PubMed : 37390818, PubMed : 8662539). Acts as an important regulator of lysosomal lumen pH regulation by acting as a direct inhibitor of the proton channel TMEM175, facilitating lysosomal acidification for optimal hydrolase activity (PubMed : 37390818). Plays an important role in chaperone-mediated autophagy, a process that mediates lysosomal degradation of proteins in response to various stresses and as part of the normal turnover of proteins with a long biological half-live (PubMed : 11082038, PubMed : 18644871, PubMed : 24880125, PubMed : 27628032, PubMed : 36586411, PubMed : 8662539). Functions by binding target proteins, such as GAPDH, GPX4, NLRP3 and MLLT11, and targeting them for lysosomal degradation (PubMed : 11082038, PubMed : 18644871, PubMed : 24880125, PubMed : 36586411, PubMed : 8662539). In the chaperone-mediated autophagy, acts downstream of chaperones, such as HSPA8/HSC70, which recognize and bind substrate proteins and mediate their recruitment to lysosomes, where target proteins bind LAMP2 (PubMed : 36586411). Plays a role in lysosomal protein degradation in response to starvation (By similarity). Required for the fusion of autophagosomes with lysosomes during autophagy (PubMed : 27628032). Cells that lack LAMP2 express normal levels of VAMP8, but fail to accumulate STX17 on autophagosomes, which is the most likely explanation for the lack of fusion between autophagosomes and lysosomes (PubMed : 27628032). Required for normal degradation of the contents of autophagosomes (PubMed : 27628032). Required for efficient MHC class II-mediated presentation of exogenous antigens via its function in lysosomal protein degradation; antigenic peptides generated by proteases in the endosomal/lysosomal compartment are captured by nascent MHC II subunits (PubMed : 15894275, PubMed : 20518820). Is not required for efficient MHC class II-mediated presentation of endogenous antigens (PubMed : 20518820).. Isoform LAMP-2C. Modulates chaperone-mediated autophagy. Decreases presentation of endogenous antigens by MHCII. Does not play a role in the presentation of exogenous and membrane-derived antigens by MHCII.. (Microbial infection) Supports the FURIN-mediated cleavage of mumps virus fusion protein F by interacting with both FURIN and the unprocessed form but not the processed form of the viral protein F.
See full target information LAMP2
style
left-column
style
left-column
style
right-column

Product promise

We are committed to supporting your work with high-quality reagents, and we're here for you every step of the way. In the unlikely event that one of our products does not perform as expected, you're protected by our Product Promise.
For full details, please see our Terms & Conditions

Please note: All products are 'FOR RESEARCH USE ONLY. NOT FOR USE IN DIAGNOSTIC OR THERAPEUTIC PROCEDURES'.

For licensing inquiries, please contact partnerships@abcam.com