Astana Biomed Group, an authorized Abcam distributor in Central Asia

APC/Cy7® Conjugation Kit - Lightning-Link® (ab102859)

Overview

  • Product name

    APC/Cy7® Conjugation Kit - Lightning-Link®

  • Product overview

    APC/Cy7® Conjugation Kit / APC/Cy7® Labeling Kit ab102859 uses a simple and quick process for APC/Cy7 labeling / conjugation of antibodies. It can also be used to conjugate other proteins or peptides. Learn about our antibody labeling kits and their advantages.


    To conjugate an antibody to APC/Cy7® using this kit:
    - add modifier to antibody and incubate for 3 hrs
    - add quencher and incubate for 30 mins
    The APC/Cy7® conjugated antibody can be used immediately in WB, ELISA, IHC etc. No further purification is required and 100% of the antibody is recovered for use.


    Learn about buffer compatibility below; for incompatible buffers and low antibody concentrations, use our rapid antibody purification and concentration kits. Use the FAQ to learn more about the technology, or about conjugating other proteins and peptides to APC/Cy7®.


    Custom size conjugation kits up to 100 mg are available on demand. Please contact us to discuss your requirements.

  • Notes

    This product is manufactured by Expedeon, an Abcam company, and was previously called Lightning-Link® APC/Cy7 Labeling Kit. 765-0015 is the same as the 1 mg size. 765-0010 is the same as the 3 x 100 ug size. 765-0030 is the same as the 3 x 10 ug size. 765-0005 is the same as the 100 µg size.

    Amount and volume of antibody for conjugation to APC/Cy7®.

     Kit size Recommended maximum
    amount of antibody         		 Maximum antibody 
    volume1
    3 x 10 µg 3 x 10 µg 3 x 10 µL
    100 µg 1 x 100 µg  1 x 100 µL
    3 x 100 µg 3 x 100 µg  3 x 100 µL
    1 mg 1 x 1 mg 1 x 1 mL

    1 Ideal antibody concentration is 1mg/ml. 0.5 - 1 mg/ml can be used if the maximum antibody volume is not exceeded. Antibodies > 1 mg/ml or

     

    Buffer Requirements for Conjugation

    Buffer should be pH 6.5-8.5.

    Compatible buffer constituents 
    If a concentration is shown, then the constituent should be no more than the concentration shown. If several constituents are close to the limit of acceptable concentration, then this can inhibit conjugation.

    50mM / 0.6% Tris1 0.1% BSA 50% glycerol
    0.1% sodium azide3 PBS Potassium phosphate
    Sodium chloride HEPES Sucrose
    Sodium citrate EDTA Trehalose

    1 Tris buffered saline is almost always ≤ 50 mM / 0.6%

    Incompatible buffer constituents

    Thiomerosal Proclin Glycine
    Arginine Glutathione DTT

    If a constituent of the buffer containing your antibody or protein is not listed above, please check the FAQ or contact us.

    Only purified antibodies are suitable for use, ie. where other proteins, peptides, or amino acids are not present: antibodies in ascites fluid, serum or hybridoma culture media are incompatible.

Properties

  • Storage instructions

    Store at -20°C. Please refer to protocols.
  • Components 1 mg 100 µg 3 x 10 µg 3 x 100 µg
    ab274159 - APC-Cy7 Mix 1 x 1mg 1 x 100µg 3 x 10µg 3 x 100µg
    ab274106 - Modifier reagent 1 x 200µl 1 x 200µl 1 x 200µl 1 x 200µl
    ab274133 - Quencher reagent 1 x 200µl 1 x 200µl 1 x 200µl 1 x 200µl

  • Research areas

  • Alternative names

    • Allophycocyanin

Images

  • ab102859 APC-Cy7® conjugation kit used with a mouse anti-Bovine CD62L antibody
    ab102859 APC-Cy7® conjugation kit used with a mouse anti-Bovine CD62L antibody Image from Oliveira BM et al., Scientific reports., 9 (1) 3413. Fig 1.; doi: 10.1038/s41598-019-39938-0. Reproduced under the Creative Commons license http://creativecommons.org/licenses/by/4.0/.

    Oliveira BM et al. used ab102903 PE-Cy7® conjugation kit with a mouse anti-bovine CD45RO antibody and ab102859 APC-Cy7® conjugation kit with a mouse anti-Bovine CD62L antibody. This enabled them to run their desired multicolor flow cytometry panel.

    Data shows flow cytometry gating strategy used to define γδ T cells (TCRγδ+CD3+CD335−), CD4+ T cells (CD4+CD3+TCRγδ−CD335−), CD8+ T cells (CD8+CD3+TCRγδ−CD335−) and NK cells (CD335+CD3−) in the stromal vascular fraction (SVF) of mesenteric and subcutaneous bovine adipose tissue (MAT and SAT, respectively) and in peripheral blood leukocytes. Dead cells were excluded with Fixable Viability Dye (FVD), lymphocytes were gated based on SSC-A versus FSC-A and singlets were selected from the FSC-A versus FSC-H dot plot.

    The flow cytometry gating strategy used to define CD45RO+ and CD62L+ T cell subpopulations is also shown in CD8+ T cells.

  • conjugation
    conjugation

    This illustration demonstrates a general procedure and will slightly vary dependent on the conjugate used.

Please note: All products are "FOR RESEARCH USE ONLY. NOT FOR USE IN DIAGNOSTIC PROCEDURES"
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