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Anti cd45ra apc h7 hi100

Manufactured by BD
Sourced in United States

Anti-CD45RA-APC-H7 (HI100) is a monoclonal antibody conjugated with the APC-H7 fluorochrome. It is designed for the detection and quantification of CD45RA-expressing cells in flow cytometry applications.

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2 protocols using anti cd45ra apc h7 hi100

1

Multiparameter Flow Cytometry Phenotyping

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The following fluorochrome‐conjugated monoclonal antibodies were used for multicolour flow cytometry: anti‐CD45‐BUV395 (HI30), anti‐CD3‐BV510, –FITC, or ‐PerCP‐Cy5.5 (UCHT1), anti‐CD4‐BV605 (RPA‐T4), anti‐CD8‐BV711 or –APC‐R700 (SK1), anti‐CD45RA‐APC‐H7 (HI100), anti‐CD127‐BV650 or –FITC (HIL‐7R‐M21), anti‐CD25‐BV650, ‐BB515, or ‐PE‐Cy7 (M‐A251), anti‐CD272‐BV650 or ‐APC (J168‐540.90.22), anti‐CD39‐BV711 (TU66), anti‐CD19‐PE‐CF594 (HIB19) and anti‐CD14‐PE‐CF594 (MQP9) (all from BD Bioscience, San Jose, California, USA); anti‐FOXP3‐PE or –Alexa Fluor 700 (PCH101) (all from eBioscience, San Diego, California, USA); anti‐CD197‐BV786 or –BV510 (G043H7), anti‐PD‐1‐BV421 or –PerCP‐Cy5.5 (EH12.2H7), anti‐CD357 (GITR)‐PE (108‐17) and anti‐CTLA‐4‐APC or –PE‐cy7 (L3D10) (all from Biolegend, San Diego, California, USA).
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2

Treg Flow Cytometry Profiling Protocol

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The Treg flow cytometry panel was inspired by a clinical Tregs workshop (21 (link)). Blood was sampled in heparin-containing tubes and peripheral mononuclear cells (PBMCs) were isolated by Ficoll density gradient separation following standard procedures before freezing down at -150°C in AB serum with 10% DMSO. For flow analysis, thawed PBMCs from 5 patients and 8 controls (see Table 1) were added two microliter of Fc block for 15 min before addition of the extracellular antibodies anti-CTLA4 BV421 (BN13, Biolegend, San Diego, CA), anti-CD39 PE (ebioA1, Invitrogen, Carlsbad, California, USA) and anti-CD3 V500 (UCHT1); anti-CD4 Alexa Fluor 700 (RPA-T4); anti-CD8 PerCP-Cy5.5 (SKI); anti-CD25 PE-Cy7 (2A3); anti-CD45RA APC-H7 (HI100) and anti-CD31 BV650 (L133.1) from BD (Franklin Lakes, New Jersey, USA). The cells were resuspended in 1 mL PBS and live/dead Fixable Yellow Dead Cell stain kit (Invitrogen) was added in a 1:1000 dilution. Staining of intracellular markers [anti-FOXP3 PE-CF594 (259D/C7, BD), anti-HELIOS APC (22F6, Biolegend), and anti-Ki-67 (20Raj1, Invitrogen)] was subsequently performed using the eBioscience Anti-human FOXP3 Staining Set as explained by the manufacturer with the change that the cells were fixed overnight. Acquisition was executed by a LSR Fortessa flow cytometer and data was analyzed by FlowJo version 10.4.
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