ab133996 is for simultaneous detection of 23 Human Cytokines.
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- Asian Pacific journal of cancer prevention : APJCP 24:3825-38352023Role of Oxidative Stress-Dependent C/EBPβ Expression on CAF Transformation Inducing HCT116 Colorectal Cancer Cell Progression; Migration and Invasion.Applications:Unspecified applicationReactive species:Unspecified reactive speciesArtchaya Hassametto,Rataya Tanomrat,Tharathip Muangthong,Suchin Worawichawong,Prasit SuwannalertPubMed 38019240
- Cell 186:5135-5150.e282023Mechanopathology of biofilm-like Mycobacterium tuberculosis cords.Applications:Unspecified applicationReactive species:Unspecified reactive speciesRicha Mishra,Melanie Hannebelle,Vishal P Patil,Anaëlle Dubois,Cristina Garcia-Mouton,Gabriela M Kirsch,Maxime Jan,Kunal Sharma,Nicolas Guex,Jessica Sordet-Dessimoz,Jesus Perez-Gil,Manu Prakash,Graham W Knott,Neeraj Dhar,John D McKinney,Vivek V ThackerPubMed 37865090
- International journal of molecular sciences 24:2023Effects of Seed Oil on Cultured Human Sebocytes In Vitro and Comparison with Other Oil Types.Applications:Unspecified applicationReactive species:Unspecified reactive speciesChristos C Zouboulis,Amir M Hossini,Xiaoxiao Hou,Chaoxuan Wang,Karsten H Weylandt,Anne PietznerPubMed 37373478
- Pharmaceutics 15:2023HS 3D-SeboSkin Model Enables the Preclinical Exploration of Therapeutic Candidates for Hidradenitis Suppurativa/Acne Inversa.Applications:Unspecified applicationReactive species:Unspecified reactive speciesChristos C Zouboulis,Xiaoxiao Hou,Henriette von Waldthausen,Konstantin C Zouboulis,Amir M HossiniPubMed 36839941
- Cancers 15:2022Thioredoxin Reductase-1 as a Potential Biomarker in Fibroblast-Associated HCT116 Cancer Cell Progression and Dissemination in a Zebrafish Model.Applications:Unspecified applicationReactive species:Unspecified reactive speciesTharathip Muangthong,Pornnapat Chusangnin,Artchaya Hassametto,Rataya Tanomrat,Prasit SuwannalertPubMed 36612053
- Frontiers in pharmacology 13:8459302022Neuroinflammation Upregulated Neuronal Toll-Like Receptors 2 and 4 to Drive Synucleinopathy in Neurodegeneration.Applications:Unspecified applicationReactive species:Unspecified reactive speciesLucia Yi-Ru Chung,Yi-Ting Lin,Chi Liu,Yi-Cheng Tai,Han-Yi Lin,Chin-Hsien Lin,Ching-Chow ChenPubMed 35401198
- Rheumatology international 41:1495-15012021Post-COVID-19 exacerbation of fibrodysplasia ossificans progressiva with multiple flare-ups and extensive heterotopic ossification in a 45-year-old female patient.Applications:Unspecified applicationReactive species:Unspecified reactive speciesLovorka Grgurevic,Rudjer Novak,Stela Hrkac,Grgur Salai,Simeon GrazioPubMed 34110466
- Neuro-oncology 22:457-4692019Betacellulin drives therapy resistance in glioblastoma.Applications:Unspecified applicationReactive species:Unspecified reactive speciesQiwen Fan,Zhenyi An,Robyn A Wong,Xujun Luo,Edbert D Lu,Albert Baldwin,Manasi K Mayekar,Franziska Haderk,Kevan M Shokat,Trever G Bivona,William A WeissPubMed 31678994
- Medical hypotheses 131:1093132019Elevated plasma RANTES in fibrodysplasia ossificans progressiva - A novel therapeutic target?Applications:Unspecified applicationReactive species:Unspecified reactive speciesLovorka Grgurević et. al.PubMed 31443758
- Biomaterials 198:194-20320183D biomaterial matrix to support long term, full thickness, immuno-competent human skin equivalents with nervous system components.Applications:Unspecified applicationReactive species:Unspecified reactive speciesSarah E Lightfoot Vidal,Kasey A Tamamoto,Hanh Nguyen,Rosalyn D Abbott,Dana M Cairns,David L KaplanPubMed 29709325
Key facts
- Assay type
- Semi-quantitative
- Reactive species
- Human
- Target
- CSF3
(See target data below)
Target data
Function
Granulocyte/macrophage colony-stimulating factors are cytokines that act in hematopoiesis by controlling the production, differentiation, and function of 2 related white cell populations of the blood, the granulocytes and the monocytes-macrophages. This CSF induces granulocytes.
Additional Targets
CSF2, CXCL1, CXCL3, IFNG, IL1A, IL10, IL13, IL15, IL2, IL3, IL5, IL6, IL7, CXCL8, CCL2, CCL8, CCL7, CXCL9, CCL5, TGFB1, TNF, LTA
Alternative names
C17orf33, GCSF, CSF3, Granulocyte colony-stimulating factor, G-CSF, Pluripoietin
What's included?
Recommended products
ab133996 is for simultaneous detection of 23 Human Cytokines.
Key facts
- Assay type
- Semi-quantitative
- Reactive species
- Human
- Target
- CSF3
- Applications
- Multiplex Protein Detection
- Sample types
- Saliva, Urine, Plasma, Cell culture extracts, Tissue Extracts, Cell culture media, Cell culture supernatant, Milk, Serum, Other biological fluids, Whole Blood, Cell Lysate
Storage
- Shipped at conditions
- Blue Ice
- Appropriate short-term storage conditions
- -20°C
- Appropriate long-term storage conditions
- -20°C
- Storage information
- -20°C
Notes
ab133996 is for simultaneous detection of 23 Human Cytokines. Suitable for all sample types.
Targets: G-CSF, GM-CSF, GRO (alpha, beta & gamma), GRO-alpha, IL-1alpha, IL-2, IL-3, IL-5, IL-6, IL-7, IL-8, IL-10, IL-13, IL-15, IFN-gamma, MCP-1, MCP-2, MCP-3, MIG, RANTES, TGF-beta1, TNF-alpha, TNF-beta
Cytokine arrays are an antibody-pair-based assay, analogous to ELISA, but using a membrane as a substrate rather than a plate. Capture antibodies are supplied arrayed/spotted on a membrane with each pair of spots representing a different analyte. Sample is added (0.2-1ml of 1 sample to each membrane), and then paired biotinylated detector antibodies and streptavidin HRP. The cytokine array is analyzed using the same methods as a chemiluminescent western blot. Comparison between samples can be by eye or using densitometry software for a semi-quantitative comparison.
If you are interested in this cytokine array, arrays ab133997, ab169804, ab134003, ab133998 and ab169817 may also be of interest. **A table listing all of our mouse membrane antibody cytokine arrays and other arrays and the analytes they measure is available .** "
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3 product images
Multiplex Protein Detection - Cytokine Array - Human Cytokine Antibody Array (Membrane, 23 Targets) (ab133996)
Human peripheral blood cells (1x106 cells/mL) were cultured in RPMI media supplemented with 10% fetal calf serum, 100 U/mL penicillin, and 100 mg/mL streptomycin sulfate.
Cells were cultured unstimulated or stimulated with 10 μg/mL PHA. Conditioned media was harvested after 48 hours, aliquoted and assayed using ab133996. Media alone was used as a negative control.
Multiplex Protein Detection - Cytokine Array - Human Cytokine Antibody Array (Membrane, 23 Targets) (ab133996)
Quantification of Human Cytokine Antibody Array.
Cells were cultured unstimulated or stimulated with 10 μg/mL PHA. Conditioned media was harvested after 48 hours, aliquoted and assayed using ab133996. Media alone was used as a negative control. Samples were incubated on the human cytokin antibody arrays and results were quantified using the ULTRAQuant software.
This image is courtesy of an anonymous customer review.Multiplex Protein Detection - Cytokine Array - Human Cytokine Antibody Array (Membrane, 23 Targets) (ab133996)
Abreview rating 4/5 stars. Review from Abcam user community. Verified customer. Submitted Oct 2 2014.
The human cytokine antibody array containing 23 target proteins was used to determine the effect of lipopolysaccharide (LPS) on the induction of cytokine production in macrophages. One million macrophage cells were plated in two sets and used in the study, one set was treated with PBS alone while the other set is treated with LPS at 1 μg/mL for 24 h. After 24 h of LPS treatment, both sets of macrophages were harvested using the provided cell lysis buffer and the cells were mechanically disrupted using a 20-gauge needle. Disrupted cell lysates were centrifuged and the supernatant was collected. The protein concentration of the supernatant was determined and 200 μg of proteins diluted in the blocking buffer was applied into previously blocked membranes and stored overnight at 4 °C. The remainder of the experiment was performed using the manufacturer's instructions where all remaining incubations were performed at room temperature for 2 h. After incubation and washing steps, the proteins were detected using the provided detection reagents and photographed in a blot imaging system. Membranes were exposed for 15 s.
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