Donkey anti-Goat IgG,Alexa Fluor 488,Donkey anti-Goat IgG,Alexa Fluor 488/驴抗山羊IgG,Alexa Fluor 488

2024-10-23

Donkey anti-Goat IgG,Alexa Fluor 488/驴抗山羊IgG,Alexa Fluor 488

货号:DG1805,DG1810

规格:50 μL,100 μL

价格:300,500

产品类型:荧光二抗

品牌:PBM

物种:山羊

宿主:驴

抗体亚型:IgG

荧光染料:Alexa Fluor 488

抗体类型:荧光二抗同型对照:IgG
浓度 2 mg/mL用法:1-10 µg/mL(ICC/IF);1-10 µg/mL(Flow);1-10 µg/mL(IHC)
产品详细信息

To minimize cross-reactivity, these donkey anti-goat IgG whole antibodies have been cross-adsorbed against rabbit, rat, mouse, and human IgG. Cross-adsorption or pre-adsorption is a purification step to increase specificity of the antibody resulting in higher sensitivity and less background staining. The secondary antibody solution is passed through a column matrix containing immobilized serum proteins from potentially cross-reactive species. Only the nonspecific-binding secondary antibodies are captured in the column, and the highly specific secondaries flow through. The benefits of this extra step are apparent in multiplexing/multicolor-staining experiments (e.g., flow cytometry) where there is potential cross-reactivity with other primary antibodies or in tissue/cell fluorescent staining experiments where there are may be the presence of endogenous immunoglobulins.Alexa Fluor dyes are among the most trusted fluorescent dyes available today. Invitrogen™ Alexa Fluor 488 dye is a bright, green-fluorescent dye with excitation ideally suited to the 488 nm laser line. For stable signal generation in imaging and flow cytometry, Alexa Fluor 488 dye is pH-insensitive over a wide molar range. Probes with high fluorescence quantum yield and high photostability allow detection of low-abundance biological structures with great sensitivity. Alexa Fluor 488 dye molecules can be attached to proteins at high molar ratios without significant self-quenching, enabling brighter conjugates and more sensitive detection. The degree of labeling for each conjugate is typically 2-8 fluorophore molecules per IgG molecule; the exact degree of labeling is indicated on the certificate of analysis for each product lot.Using conjugate solutions: Centrifuge the protein conjugate solution briefly in a microcentrifuge before use; add only the supernatant to the experiment. This step will help eliminate any protein aggregates that may have formed during storage, thereby reducing nonspecific background staining. Because staining protocols vary with application, the appropriate dilution of antibody should be determined empirically. For the fluorophore-labeled antibodies a final concentration of 1-10 µg/mL should be satisfactory for most immunohistochemistry and flow cytometry applications.Product will be shipped at Room Temperature.

靶标信息

Anti-Goat secondary antibodies are affinity-purified antibodies with well-characterized specificity for goat immunoglobulins and are useful in the detection, sorting or purification of its specified target. Secondary antibodies offer increased versatility enabling users to use many detection systems (e.g. HRP, AP, fluorescence). They can also provide greater sensitivity through signal amplification as multiple secondary antibodies can bind to a single primary antibody. Most commonly, secondary antibodies are generated by immunizing the host animal with a pooled population of immunoglobulins from the target species and can be further purified and modified (i.e. immunoaffinity chromatography, antibody fragmentation, label conjugation, etc.) to generate highly specific reagents.

数据

Ishikawa cells (human endometrial adenocarcinoma cell line) were cultured according to standard protocol. The culture medium was aspirated and cells rinsed with Ca and Mg free HBSS. Cells were treated with 0.25% Trypsin and incubated at 37° for 5 minutes. Cells were aspirated and pelleted at 900 x g for 5 minutes. Cells were washed twice with PBS. The cells were then fixed with 4% paraformaldehyde in PBS for 15 minutes at room temperature. The cells were then washed as stated previously. Permeabilization and blocking was performed by incubating in 5% BSA and 0.1% Triton-X in PBS for 20 minutes at room temperature. The cells were then washed as previously stated. The primary antibody for OXTR (Product # PA5-19038) was used at a 1:200 dilution in a 5% BSA, PBS solution and incubated for 120 minutes at room temperature. The cells were washed as stated previously. The secondary Alexa 488 antibody (Product # A-11055) was used at a 1:2000 dilution in 5% BSA, PBS and incubated in the dark for 45 minutes. The cells were washed and resuspended in PBS and analyzed through flow cytometry. Data courtesy of the Antibody Data Exchange Program.

a Representative intrinsic vascular staining of isolectin B4 (ILB4; green) and osteoblast staining with rat osteocalcin (OC; green). Scale bar: 50 mm. b Quantitative analysis of neovascularization assessed by the capillary density of the three groups (n = 5/group). c Quantitative analysis of osteogenesis assessed by osteoblast density of the three groups (n = 5/group). *; p < 0.05 for F- or C-SVF vs. control; NS, not significant. F-SVF, freshly isolated stromal vascular fraction; C-SVF, cryopreserved stromal vascular fraction Image collected and cropped by CiteAb from the following publication (https://pubmed.ncbi.nlm.nih.gov/33541427), licensed under a CC BY license.

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