Cd4 pe texas red

Manufactured by Thermo Fisher Scientific

Sourced in United States

The CD4-PE-Texas Red is a fluorochrome-conjugated antibody used for flow cytometry analysis. It binds to the CD4 antigen expressed on the surface of T helper cells. The Texas Red fluorescent dye allows for detection of the CD4-positive cell population.

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Lab products found in correlation

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Close spelling variants of this product

Texas Red (171 citations) CD4-PE (59 citations) PE Texas Red (7 citations) Anti-CD4+-PE-Texas-Red (6 citations)

4 protocols using cd4 pe texas red

Multiparameter Flow Cytometry Analysis of T Cells

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The remaining blood was used to isolate PBMCs using previously described methods [25] (link). PBMCs were thawed, washed and stained with LIVE/DEAD Fixable Aqua Dead Cell Stain Kit (Invitrogen), and then stained with the following fluorescently-conjugated monoclonal antibodies: CD8-QDOT 605 and CD4-PE-Texas Red (Invitrogen, Grand Island, NY, USA); CD3-Pacific Blue, CCR5-PE-Cy5, CD38-PE, HLA-DR-FITC, PD-1 Alexa Fluor 647, CD45RA-PE-Cy7 (BD Biosciences, San Jose, CA, USA); and CCR7-APCeFluor 780 (eBioscience, San Diego, CA, USA). Naïve and memory T cell subsets were defined by quadrant gating with FMO controls on a CD45RA versus CCR7 plot.
For cytokine staining, PBMCs were stimulated for 18–22 h at 37°C with overlapping peptide pools corresponding to HIV-1 Con B Gag peptides (NIH 8117) in the presence of 0.5 µg/mL Brefeldin A and 05 µg/mL Monensin (Sigma-Aldrich, St. Louis, MO, USA). A control well with no stimulation was run in parallel for each sample. Cells were washed and stained with AARD, fixed, and permeabilized for intracellular staining with antibodies against CD3-Pacific Blue, IFNγ-FITC, IL-2-PE (BD BioSciences), CD4-PE Texas Red, and CD8-QDOT 605 (Invitrogen). Data were compensated and analyzed using FlowJo V9 (TreeStar, Ashland, OR, USA).

Cockerham L.R., Siliciano J.D., Sinclair E., O'Doherty U., Palmer S., Yukl S.A., Strain M.C., Chomont N., Hecht F.M., Siliciano R.F., Richman D.D, & Deeks S.G. (2014). CD4+ and CD8+ T Cell Activation Are Associated with HIV DNA in Resting CD4+ T Cells. PLoS ONE, 9(10), e110731.

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PBMC Activation and Phenotyping

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Cryopreserved PBMCs were isolated from whole blood, and stored at the UCSF AIDS Specimen Bank. T cell activation was measured by the UCSF Core Immunology Laboratory, as previously described and optimized [45] (link). Cryopreserved PBMCs were thawed and stained with the following markers: Aqua Amine Reactive Dye (Invitrogen, Carlsbad, CA), CD3 Pacific Blue, CCR5 PE-CY5 (BD Pharmingen, San Jose, CA), CD38 PE, HLA-DR FITC, (BD Biosciences), CD4 PE Texas Red, and CD8 QDot 605 (Invitrogen).

Klatt N.R., Bosinger S.E., Peck M., Richert-Spuhler L.E., Heigele A., Gile J.P., Patel N., Taaffe J., Julg B., Camerini D., Torti C., Martin J.N., Deeks S.G., Sinclair E., Hecht F.M., Lederman M.M., Paiardini M., Kirchhoff F., Brenchley J.M., Hunt P.W, & Silvestri G. (2014). Limited HIV Infection of Central Memory and Stem Cell Memory CD4+ T Cells Is Associated with Lack of Progression in Viremic Individuals. PLoS Pathogens, 10(8), e1004345.

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Multiparameter Flow Cytometry Immunophenotyping

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Antibodies to TPL-2, IκBα, ERK-1, ERK-2, actin were purchased from Santa Cruz Biotechnology, whilst p-p105 (Ser933), p-p38 and p-ERK (Thr185/Tyr187) antibodies were obtained from Invitrogen. Tubulin mAb was kindly provided by Keith Gull (University of Oxford).
A number of fluorescently labelled antibodies for flow cytometry were used against: GMSCF-PE; Gr1-FITC; CD25-PE; TCRβ-PECy5; TCRγδ-PE; Streptavidin-PErCP; Streptavidin-PE were purchased from BD Pharmingen. IL-17A-APC; IFNγ-FITC; CD4-FITC, -PE; F4/80-APC, -PE; Gr1-biotinylated; CD25-APC; CD44-AF450, -FITC; CD45.2-FITC, -AF450; CD45.1-biotinylated; CD11c-PE; CD11b-PE, -biotinylated; MHCII-biotinylated were obtained from eBioscience. CD4-PerCP; CD19-Pacific Blue were purchased from BioLegend. CD4-PE/Texas Red; CD8-PE/Texas Red were obtained from Invitrogen.

Sriskantharajah S., Gückel E., Tsakiri N., Kierdorf K., Brender C., Ben-Addi A., Veldhoen M., Tsichlis P.N., Stockinger B., O’Garra A., Prinz M., Kollias G, & Ley S.C. (2014). Regulation of experimental autoimmune encephalomyelitis by TPL-2 kinase. Journal of immunology (Baltimore, Md. : 1950), 192(8), 3518-3529.

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Comprehensive Immune Phenotyping of PBMC

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Immune activation and differentiation were quantified as previously described [54] (link). In brief, one million thawed PBMC were stained with either an activation or differentiation panel for 15 minutes at 37°C prior to fixation in formaldehyde. Both panels included CD3 V450 (Becton Dickinson); CD4 PE-Texas Red (Invitrogen); CD8 Qdot605 (Invitrogen). Activation panel included HLA-DR FITC; PD-1 AF647; CD38 PE; CCR5 PE-Cy5; 45RA PE-Cy7 (all Becton Dickinson); CCR7 APC eFluor-780 (eBioscience). Differentiation panel included CD45RA PE; CD28 PE-Cy5; CCR7 PE-Cy7; CD31 FITC (all Becton Dickinson); CD57 AF647 (Biolegend); CD27 AF780 (eBioscience). For Tregs, PBMC were surface stained with CD4 PerCP, CD127 PE and CD25 FITC (all Becton Dickinson) followed by intracellular staining using eBioscience FoxP3 staining kit and FoxP3 APC as per manufacturer's instructions. Data was acquired on a BD LSR-Fortessa and analysed using FlowJo version 10.

Elliott J.H., Wightman F., Solomon A., Ghneim K., Ahlers J., Cameron M.J., Smith M.Z., Spelman T., McMahon J., Velayudham P., Brown G., Roney J., Watson J., Prince M.H., Hoy J.F., Chomont N., Fromentin R., Procopio F.A., Zeidan J., Palmer S., Odevall L., Johnstone R.W., Martin B.P., Sinclair E., Deeks S.G., Hazuda D.J., Cameron P.U., Sékaly R.P, & Lewin S.R. (2014). Activation of HIV Transcription with Short-Course Vorinostat in HIV-Infected Patients on Suppressive Antiretroviral Therapy. PLoS Pathogens, 10(11), e1004473.

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