Goat anti-Rabbit IgG (H&L), HRP conjugated

Referentie AS09602

Formaat : 1mg

Merk : Agrisera

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Product no: AS09 602

AS09 602 |  Clonality: Polyclonal | Host: Goat | Reactivity: Rabbit IgG (H&L)

  • Product Info
  • Immunogen: Purified Rabbit IgG, whole molecule,
    Host: Goat
    Clonality: Polyclonal
    Purity: Immunogen affinity purified using solid phase rabbit IgG.
    Format: Lyophilized
    Quantity: 1 mg
    Reconstitution: For reconstitution add 1.1 ml of sterile water. Let it stand 30 minutes at room temperature to dissolve. Spin centrifuge shortly to remove any particles. Prepare fresh working dilutions daily
    Storage: Store lyophilized material at 2-8°C. For long time storage after reconstitution, dilute the antibody solution with glycerol to a final concentration of 50% glycerol and store as liquid at -20°C, to prevent loss of enzymatic activity. For example, if you have reconstituted 1 mg of antibody in 1.1 ml of sterile water, add 1.1 ml of glycerol. Such solution will not freeze in -20°C. If you are using a 1:5000 dilution prior to diluting with glycerol, then you would need to use a 1:2500 dilution after adding glycerol. Prepare working dilution prior to use and then discard, Be sure to mix well but without foaming.
    Tested applications: ELISA (ELISA), Immunohistochemistry (IHC), Western blot (WB)
    Recommended dilution: 1 : 50 000 -1 : 90 000 (ELISA), 1 : 500 -1 : 5000 (IHC), 1: 10 000 -1 : 50 000 (WB)
  • Reactivity
  • Confirmed reactivity: Based on IEP, this antibody reacts with: rabbit IgG heavy chains and light chains on all rabbit immunoglobulins
    Not reactive in: Non-immunoglobulin rabbit serum proteins
  • Application Examples
  • western blot detection of PsaC using Agrisera primary and secondary antibodies

    5 µg of total extract from (1) Hordeum vulgaretotal leaf, (2) Zea mays (3) Spinacia oleracea extracted with PEB (AS08 300) were separated on 4-12% NuPage (Invitrogen) LDS-PAGE and blotted 1h to PVDF. Blots were blocked immediately following transfer in 2% ECL Advance blocking reagent (GE Healthcare) in 20 mM Tris, 137 mM sodium chloride pH 7.6 with 0.1% (v/v) Tween-20 (TBS-T) for 1h at room temperature with agitation. Blots were incubated in the primary anti-PsaC antibody (AS04 042) at a dilution of 1: 10 000 for 1h at room temperature with agitation. The antibody solution was decanted and the blot was rinsed briefly twice, then washed once for 15 min and 3 times for 5 min in TBS-T at room temperature with agitation. Blots were incubated in secondary antibody (goat anti-rabbit IgG horse radish peroxidase conjugated, AS09 602, Agrisera) diluted to 1:50 000 in 2% ECL Advance blocking solution for 1h at room temperature with agitation. The blots were washed as above and developed for 5 min with chemiluminescent detection reagent according to the manufacturers instructions. Images of the blots were obtained using a CCD imager (FluorSMax, Bio-Rad) and Quantity One software (Bio-Rad). Exposure time was 30 seconds.


    Comparison of Agrisera secondary antibody sensitivity

    comparison of secondary antibody sensitivity

    10 μg of mitochondrial fraction from Arabidopsis thaliana (1,3) and Arabidopsis thaliana leaf extract (2,4) were separated on 10% gel and blotted on nitrocellulose membrane using wet transfer (0.22% CAPS, pH 11). Filters where blocked (1.5h) in 5% milk in TBST (1X TBS, 0,1% Tween 20), incubated with 1: 1000 anti-COXII antibodies (2h in TBST) followed by incubation with 1: 10 000 secondary anti-rabbit (1h) HRP-coupled antibodies from Agrisera (left panel) and other manufacture (right panel) and visualized with chemiluminescent detection reagent, on Kodak autoradiography film for 5 s. Antibody in left panel detects target protein also in total cell extract (2) and can be used in higher dilution than applied 1: 10 000.

    Agrisera goat anti-rabbit HRP conjugated antibody (AS09 602) can be used at following dilutions: 1: 50 000 -1: 90 000 (ELISA), 1 : 75 000 with chemiluminescence detection range of extreme low picogram and 1: 25 000 with chemiluminescence detection reagent of mid femtogram (WB), 1: 500 -1: 5000 (IHC).

    Application examples:

    Reactant: Homo sapiens (Human)

    Application: Western Blotting

    Pudmed ID: 36473840

    Journal: Cell Death Dis

    Figure Number: 5B

    Published Date: 2022-12-06

    First Author: Toh, E.

    Impact Factor: 5.638

    Open Publication

    MakA inhibits tumour cell proliferation in a PIP5K1α-dependent manner.A MakA and PIP5K1α inhibitor, ISA-2011B synergistically inhibited HCT8 cell proliferation as quantified by colony forming assay. Data are representative of two independent experiments; bar graphs show mean ± s.d. Significance from replicates was determined using a one-way analysis of variance (ANOVA) with Dunnett’s multiple comparisons test (post-test) against vehicle (Veh). *p ≤ 0.05 and **p ≤ 0.01. B Western blot analyses of cyclin D1 and pAkt levels in HCT8 cells upon 48 h treatment with MakA (500 nM), ISA-2011B (25 μM) or a combination of MakA (500 nM) and ISA-2011B (25 μM). β-actin was used as a loading control. C Histograms showing the normalized quantification of cyclin D1 and pAkt relative to total actin. Data are representative of at least two independent experiments; bar graphs show mean ± s.d. Significance from replicates was determined using a one-way analysis of variance (ANOVA) with Dunnett’s multiple comparisons test (post-test) against vehicle (Veh). *p ≤ 0.05 and **p ≤ 0.01. D Confocal microscopy analysis of vehicle (Veh), MakA (500 nM), ISA-2011B (25 μM), or a combination of MakA (500 nM) and ISA-2011B (25 μM) treated HCT8 cells (48 h treatment). Cells were stained with cell proliferation marker, Ki67 (green). Nuclei were counterstained with DAPI (blue). Inhibition of HCT8 cell proliferation was quantified by an increase in the number of Ki67-negative stained cells from four individual microscopy fields of view (65-165 cells per field of view). *p ≤ 0.05 and **p ≤ 0.01. Scale bar = 20 μm.


    Reactant: Homo sapiens (Human)

    Application: Western Blotting

    Pudmed ID: 36473840

    Journal: Cell Death Dis

    Figure Number: 6B

    Published Date: 2022-12-06

    First Author: Toh, E.

    Impact Factor: 5.638

    Open Publication

    Effect of MakA in HCT8 cells with PIP5K1α overexpression and schematic summaries of the MakA effects on PIP5K1α-mediated signalling.A HCT8 cells were transfected with EGFP-vector control (upper panel) or PIP5K1α-EGFP (lower panel) plasmids as described in “Materials and methods”. For co-localization experiments of MakA and PIP5K1α, the transfected HCT8 cells were subsequently treated with Alexa568MakA (250 nM, red) for 48 h. Nuclei were counterstained with DAPI (blue). Graphs on the right show fluorescence intensity profiles of the corresponding images along the dotted white lines. Pearson correlation co-efficient was used for calculation of Alexa568MakA (red) co-localization with EGFP or PIP5K1α-EGFP (green) along the cell membrane. Scale bars = 10 μm. B Western blot analysis of PIP5K1α levels in EGFP-vector control or PIP5K1α-EGFP HCT8 total cell lysates. C Confocal microscopy analysis of vehicle (Veh) or MakA (250 nM) treated (48 h treatment) HCT8 cells transfected with EGFP-vector control or PIP5K1α-EGFP plasmids. Cells were stained with cell proliferation marker, Ki67 (green). Nuclei were counterstained with DAPI (blue). Effects on HCT8 cell proliferation was assessed by quantifying the number of Ki67-negative cells from eleven individual microscopy fields of view (65–200 cells per field of view). Significance was determined using an unpaired t test, ns non-significant. D Schematic representations showing (i) the downstream signalling of PIP5K1α during tumour cell proliferation and survival, (ii) the effect of MakA and ISA-2011B inhibition.


    Reactant: Homo sapiens (Human)

    Application: Western Blotting

    Pudmed ID: 36473840

    Journal: Cell Death Dis

    Figure Number: 4A

    Published Date: 2022-12-06

    First Author: Toh, E.

    Impact Factor: 5.638

    Open Publication

    MakA induces G2/M cell cycle arrest in HCT8 cells and alters the expression of cell cycle regulatory proteins.A Western blot analysis shows levels of E2F1, CDK1, CDK2, cyclin D1, and cyclin A in HCT8 cells treated with increasing concentrations of MakA (24 h). B, C Histograms indicate the normalized quantification of E2F1, CDK1, CDK2, cyclin D1, and cyclin A1 relative to total actin. Data is representative of at least two independent experiments and is expressed compared to cells treated with vehicle (20 mM Tris-HCl); bar graphs show mean ± s.d. Significance was determined using a one-way analysis of variance (ANOVA) followed by Dunnett’s post-test in comparison to the vehicle control *p ≤ 0.05 and **p ≤ 0.01. D Cell cycle distribution flow cytometric analysis of HCT8 cells treated with MakA protein (500 nM, 24 h). E Histogram showing the distribution of HCT8 cells during each phase of the cell cycle after treatment with vehicle or MakA. Data are representative of three independent experiments. *p ≤ 0.05 and **p ≤ 0.01.

  • Additional Information
  • Additional information:
    Concentration: 1.0 mg/ml.

    Antibody is provided in: 10 mM Sodium Phosphate, 0.15 M Sodium Chloride, pH 7.2, 1% BSA (w/v), Protease IgG free, 0.1% (v/v) ProClin 150.

    Affinity purified antibody is >95% pure, according to SDS-PAGE.

    This antibody can used on a very wide range of samples from various species including many model plants, algae, diatoms and bacteria.
  • Background
  • Background:

    Goat anti-rabbit IgG (H&L) is a secondary antibody conjugated to HRP which binds to all rabbit IgGs in immunological assays.

  • Product Citations
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    Lim et al (2022). Arabidopsis guard cell chloroplasts import cytosolic ATP for starch turnover and stomatal opening. Nat Commun. 2022 Feb 3;13(1):652. doi: 10.1038/s41467-022-28263-2. PMID: 35115512; PMCID: PMC8814037.
    Miklankova et al. (2022) HYPK promotes the activity of the Nalfa-acetyltransferase A complex to determine proteostasis of nonAc-X2/N-degron-containing proteins. Sci Adv. 2022 Jun 17;8(24):eabn6153. doi: 10.1126/sciadv.abn6153. Epub 2022 Jun 15. PMID: 35704578; PMCID: PMC9200280.
    Hofmann, Wienkoop & Luthje (2022) Hypoxia-Induced Aquaporins and Regulation of Redox Homeostasis by a Trans-Plasma Membrane Electron Transport System in Maize Roots. Antioxidants (Basel). 2022 Apr 25;11(5):836. doi: 10.3390/antiox11050836. PMID: 35624700; PMCID: PMC9137787.
    Bychkov et al. (2022) The role of PAP4/FSD3 and PAP9/FSD2 in heat stress responses of chloroplast genes. Plant Sci. 2022 Sep;322:111359. doi: 10.1016/j.plantsci.2022.111359. Epub 2022 Jun 20. PMID: 35738478.
    Vitale et al. (2021) Light Spectral Composition Influences Structural and Eco-Physiological Traits of Solanum lycopersicum L. cv. 'Microtom' in Response to High-LET Ionizing Radiation. Plants (Basel). 2021 Aug 23;10(8):1752. doi: 10.3390/plants10081752. PMID: 34451797; PMCID: PMC8399554.
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    Barahimipour et al. (2016). Efficient expression of nuclear transgenes in the green alga Chlamydomonas: synthesis of an HIV antigen and development of a new selectable marker. Plant Mol Biol. 2016 Mar;90(4-5):403-18. doi: 10.1007/s11103-015-0425-8. Epub 2016 Jan 8.
    CiteAB has listed this antibody as one of the 7000 most published antibodies in the world.
  • Protocols
  • Agrisera Western Blot protocol and video tutorials
  • Shelby Hotz | 2023-03-21
    0 | 0
    For my lab's study, we used this antibody for western blots to detect the abundance of Hsp70 in heat shocked and non-heat shocked bull kelp (Nereocystis leutkeana). We used a 1:5000 for the initial dilution and then a 1:2500 dilution after adding glycerol. Both were done in a 5% Nonfat Dried Milk in 1x Tris Buffered Saline solution. The results were positive, with the protein bands showing up clearly and at the correct weight according to the positive control we used.I am happy to report the antibody has been working effectively and as intended in our molecular research. The instructions that come with the product are very comprehensive and relatively easy to follow, and doing so has allowed us to effectively use the materials as expected and needed. We also appreciate the promptness of the delivery and arrival of the materials, and having the antibody in a lyophilized form is very much appreciated.Thank you for your service.
    Vasundara Sundar | 2022-12-28
    0 | 0
    We are very satisfied with the goat anti-rabbit antibodies, it worked well with all of the primary antibodies we used. 1:10000 dilution worked well for us.
    Annika Brünje | 2021-01-19
    0 | 0
    This antibody gives very good results in my Western blot analyses and can be also used in combination with primary antibodies that are a bit more tricky in their application. Usually, I use it in a dilution of 1:10000 to detect proteins in Arabidopsis leaf extracts.
    Soo Yeon Ko | 2020-05-28
    0 | 0
    I was satisfied with goat anti-rabbit IgG antibodies on protein extracts from Oryza Sativa in dilution : 1: 25 000
    ?udmila Holubová | 2019-10-04
    0 | 0
    We are happy with this antibody, works well with all primary antibodies we used. Our dilution was 1:12500.
    Ella Nukarinen | 2018-05-23
    0 | 0
    We are very happy with goat anti-rabbit IgG HRP antibody. We use it for Western blots in dilution 1:10 000-1:20 000 for detecting endogenous proteins from Arabidopsis protein extracts.
    Beata Kmiec | 2017-02-13
    0 | 0
    We're very happy with the antibodies. Our regular application is in western blots with Arabidopsis thaliana total protein extract and with isolated mitochondria and chloroplasts, but we've used it with success in WB with yeast and human samples. We use it in dilution 1:20000.
    Malgorzata Kwasniak-Owczarek | 2016-11-02
    0 | 0
    We are very satisfied with goat anti-rabbit IgG antibodies on protein extracts from Arabidopsis thaliana in dilution: 1: 25 000.
    Mirka Herbstova | 2016-04-22
    0 | 0
    I used Goat-anti rabbit IgG HRP conjugated secondary antibody (AS 09 602) at a dilution 1:50 000 for alga species Phaeodactylum and Trachydiscus without cross-reactions.
    Jakub Dolata, Adam Mickiewicz University, Poznan, Poland | 2014-03-12
    0 | 0
    The goat anti-rabbit IgG-HRP from Agrisera are very nice working antibodies with no unspecific signals in different dillutions (1:50000, 1:100000). We are using them in case of plant (Arabidopsis, Solanum) and human cells extracts as well.
    Jakub DOlata | 2014-03-12
    0 | 0
    The goat anti-rabbit IgG-HRP from Agrisera are very nice working antibodies with no unspecific signals in different dillutions (1:50000
    Gerhard Obermeyer, Univ Salzburg, Austria | 2011-11-11
    0 | 0
    We were looking for a 2nd anti-rabbit antibody which does not cross-react with proteins from a crude lily pollen lysate. The goat anti-rabbit IgG-HRP from Agrisera was the only one which showed no unspecific signals and could be used in a 1:40,000 dilution. All other antibodies from 5 different sources cross-reacted with a high number of proteins in the pollen lysate.

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