产品: 磷酸化 NCF2 (Thr233) 抗体
货号: AF4343
描述: Rabbit polyclonal antibody to Phospho-NCF2 (Thr233)
应用: WB IF/ICC
文献验证: WB
反应: Human, Mouse, Rat
预测: Pig, Bovine, Horse, Sheep, Rabbit, Dog, Chicken, Xenopus
蛋白号: P19878
RRID: AB_2844422

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   规格 价格 库存
 100ul RMB¥ 2800 现货
 200ul RMB¥ 3800 现货

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产品描述

来源:
Rabbit
应用:
WB 1:500-1:2000, IF/ICC 1:100-1:500
*The optimal dilutions should be determined by the end user.
*Tips:

WB: 适用于变性蛋白样本的免疫印迹检测. IHC: 适用于组织样本的石蜡(IHC-p)或冰冻(IHC-f)切片样本的免疫组化/荧光检测. IF/ICC: 适用于细胞样本的荧光检测. ELISA(peptide): 适用于抗原肽的ELISA检测.

反应:
Human, Mouse, Rat
克隆:
Polyclonal
特异性:
Phospho-NCF2 (Thr233) Antibody detects endogenous levels of NCF2 only when phosphorylated at Thr233.
RRID:
AB_2844422
引用格式: Affinity Biosciences Cat# AF4343, RRID:AB_2844422.
偶联:
Unconjugated.
纯化:
The antibody is from purified rabbit serum by affinity purification via sequential chromatography on phospho-peptide and non-phospho-peptide affinity columns.
保存:
Rabbit IgG in phosphate buffered saline , pH 7.4, 150mM NaCl, 0.02% sodium azide and 50% glycerol. Store at -20 °C. Stable for 12 months from date of receipt.
别名:

展开/折叠

67 kDa neutrophil oxidase factor; Chronic granulomatous disease autosomal 2; FLJ93058; NADPH oxidase activator 2; NCF-2; Ncf2; NCF2_HUMAN; Neutrophil cytosol factor 2; Neutrophil cytosolic factor 2 (65kD, chronic granulomatous disease, autosomal 2); Neutrophil NADPH oxidase factor 2; NOXA2; P67 PHOX; p67-phox; p67phox;

抗原和靶标

免疫原:

A synthesized peptide derived from human NCF2 around the phosphorylation site of Thr233.

基因/基因ID:

研究领域

· Cellular Processes > Transport and catabolism > Phagosome.   (View pathway)

· Human Diseases > Infectious diseases: Parasitic > Leishmaniasis.

· Organismal Systems > Development > Osteoclast differentiation.   (View pathway)

· Organismal Systems > Immune system > Leukocyte transendothelial migration.   (View pathway)

文献引用

1). NCF4 attenuates colorectal cancer progression by modulating inflammasome activation and immune surveillance. Nature communications, 2024 (PubMed: 38886341) [IF=16.6]

Application: WB    Species: human    Sample:

Fig. 1: ASC-interacting protein NCF4 is associated with colorectal cancer development. a Immunoblot analysis of ASC from the immunoprecipitated products generated with immunoprecipitation with an ASC antibody from the lysates of WT and Asc–/– BMDMs infected with F. novicida (100 MOI) for 12 h. b Mass spectrometry analysis of the IP product in (a). The peptides of ASC, NCF4, NCF1, and NCF2 were detected in the IP product with ASC antibody from WT and Asc–/– BMDMs in two repeated experiments. c Immunoblot analysis of Myc-ASC co-IP with FLAG-NCF4, FLAG-NCF4-PX, FLAG-NCF4-SH3 and FLAG-NCF4-PB1 from lysates of HEK293T cells transfected with the indicated plasmids. d Immunoblot analysis of FLAG-NCF4 co-IP with V5-ASC, V5-ASC-PYD, and V5-ASC-CARD from lysates of HEK293T cells transfected with the indicated plasmids. e Co-IP analysis of endogenous ASC interacting with total and phosphorylated NCF4, NCF1, and NCF2 in WT and Asc–/– BMDMs treated with the NLRP3 activator LPS plus ATP (LPS, 500 ng/mL for 4 h and ATP, 5 mM for 15 min). f Gene expression analysis of NCF1, NCF2, and NCF4 in total (left) and paired (right, n = 41) colorectal tumors (n = 480) and control tissues (n = 41) from 480 colorectal cancer (CRC) patients of pooled colon and rectal adenocarcinoma datasets in the TCGA database. g Correlation analysis between the gene expression of NCF4 and survival rate of CRC patients. (High, n = 466; Low, n = 131) Data are from 2 (a, b) or representative of 3 independent experiments with similar results (c–e). Wilcoxon signed rank test for (f), Log-rank (Mantel–Cox) test for (g), p-value is indicated in the graph. Source data are provided as a Source Data file.

2). Oxidation of Reduced Graphene Oxide via Cellular Redox Signaling Modulates Actin-Mediated Neurotransmission. ACS Nano, 2020 (PubMed: 32057235) [IF=15.8]

Application: WB    Species: rat    Sample: PC12

Figure S6 Oxidized rGO increased lipid peroxidation and NOX2 activation in PC12 cells. Oxidized rGO (c-rGO) was collected after pristine rGO (p-rGO) was cultured with PC12 cells for 3 h. (A-B) PC12 cells were pretreated with NAC for 30 min before being treated with two kinds of rGO (20 µg/mL) for 1 h and stained with BODIPY 581/591 C11 reagent. The lipid peroxidation degrees were quantified via FITC fluorescence intensity, with n = 10 fields per experimental condition from 3 independent tests. Scale bar: 100 μm. (C-D) After PC12 cells were treated as described in (A), plasma membrane proteins were isolated to detect the expression levels of NOX2, p-p47phox, p-p67phox and Rac2. The protein levels were quantified after normalization to ATPase. The results represent the mean ± SD of three independent experiments. *p<0.05, **p<0.01, ***p<0.001 compared with the control group and with the p-rGO group.

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