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Immunology Immunoglobulins Heavy Chain IgG

兔抗羊IgG H&L (Alkaline Phosphatase) (ab6748)

  • Datasheet
  • SDS
Submit a review Q&A (2)References (3)

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Dot Blot - Rabbit Anti-Sheep IgG H&L (Alkaline Phosphatase) (ab6748)

    Key features and details

    • Rabbit Anti-Sheep IgG H&L (Alkaline Phosphatase)
    • Conjugation: Alkaline Phosphatase
    • Host species: Rabbit
    • Suitable for: IHC-P, WB, ELISA, Immunomicroscopy, Dot blot, ICC/IF, IHC-Fr

    Conjugates logo Related conjugates and formulations

    Alexa Fluor® 488 Alexa Fluor® 555 Alexa Fluor® 568 Alexa Fluor® 594 Alexa Fluor® 647 Alexa Fluor® 750 Biotin FITC Glucose Oxidase Gold 10nm Gold 15nm HRP Texas Red ® TRITC Unconjugated Unconjugated

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    概述

    • 产品名称

      兔抗羊IgG H&L (Alkaline Phosphatase)
      参阅全部 IgG 二抗
    • 宿主

      Rabbit
    • 靶标种属

      Sheep
    • 经测试应用

      适用于: IHC-P, WB, ELISA, Immunomicroscopy, Dot blot, ICC/IF, IHC-Frmore details
    • 免疫原

      Sheep IgG whole molecule

    • 偶联物

      Alkaline Phosphatase

    性能

    • 形式

      Liquid
    • 存放说明

      Shipped at 4°C. Store at +4°C. Do Not Freeze.
    • 存储溶液

      pH: 8
      Preservative: 0.1% Sodium azide
      Constituents: 0.878% Sodium chloride, 1% BSA, 0.788% Tris HCl, 0.0095% Magnesium chloride, 0.001% Zinc chloride, 50% Glycerol (glycerin, glycerine)
    • Concentration information loading...
    • 纯度

      Affinity purified
    • 纯化说明

      This product was prepared from monospecific antiserum by immunoaffinity chromatography using Sheep IgG coupled to agarose beads
    • 克隆

      多克隆
    • 常规说明

      Alkaline Phosphatase (Calf Intestine) (Molecular Weight 140,000 daltons).

    • 研究领域

      • Immunology
      • Immunoglobulins
      • Heavy Chain
      • IgG
      • Secondary antibodies
      • anti-Sheep
      • IgG
      • Enzyme
      • Alkaline Phos

    应用

    The Abpromise guarantee

    Abpromise™承诺保证使用ab6748于以下的经测试应用

    “应用说明”部分 下显示的仅为推荐的起始稀释度;实际最佳的稀释度/浓度应由使用者检定。

    应用 Ab评论 说明
    IHC-P
    WB
    ELISA
    Immunomicroscopy
    Dot blot
    ICC/IF
    IHC-Fr
    说明
    应用说明
    suitable for immunoblotting (western or dot blot), ELISA and immunohistochemistry as well as other phosphatase-antibody based enzymatic assays requiring lot-to-lot consistency

    图片

    • Dot Blot - Rabbit Anti-Sheep IgG H&L (Alkaline Phosphatase) (ab6748)
      Dot Blot - Rabbit Anti-Sheep IgG H&L (Alkaline Phosphatase) (ab6748)

      Sheep IgG was detected using ab6748 in Dot Blot analysis.

    实验方案

    To our knowledge, customised protocols are not required for this product. Please try the standard protocols listed below and let us know how you get on.

    Click here to view the general protocols

    数据表及文件

    • SDS download

    • Datasheet download

      Download

    文献 (3)

    发表研究结果有使用 ab6748?请让我们知道,以便我们可以引用本数据表中的参考文章。

    ab6748 被引用在 3 文献中.

    • Wawrzykowski J  et al. The comparison of pro- and antioxidative parameters in plasma and placental tissues during early phase of placental development in cows. Mol Biol Rep 48:1291-1297 (2021). PubMed: 33507474
    • Corti D  et al. Analysis of memory B cell responses and isolation of novel monoclonal antibodies with neutralizing breadth from HIV-1-infected individuals. PLoS One 5:e8805 (2010). ELISA ; Human . PubMed: 20098712
    • Richardson MR  et al. Diabetic dyslipidemia and exercise alter the plasma low-density lipoproteome in Yucatan pigs. Proteomics 9:2468-83 (2009). WB . PubMed: 19402046

    客户评价及客户问答

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    1-2 of 2 Abreviews or Q&A

    Question

    I dont know if this should be posted via your webpage or not? Nevertheless, here is our answers to your questions: We have not tested ab6748 without any blocking agent and you are right this would also be a nice control to do. On the other hand we have obtained negative results with 4 different blocking agents and therefore we seriously believe that there is something wrong with this antibody. To our experience in is normal to have problems with maybe 1 or 2 blocking agents but not with 4 different. No permeabilising agent was used. As mentioned previously the delution buffer was TBS (Trizma Base-sodiumchloride pH 7,4. Trizma base 6,06g and Sodium chloride 8,76g / l) We would appreciate to get this antibody (ab6748) to work together with a primary antibody also bought from Abcam (Anti-acetyl lysine ab76). We would therefore suggest that you supply us with the protocol originally used to test the ab6748 for IHC together with another batch of the ab6748 free of charge. We would then perform an experiment comparing the two batches of ab6748 and supply you with the result. This should be in your favour as well as there could be other customers having problems with the 67077 batch.

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    Abcam community

    Verified customer

    Asked on Apr 01 2005

    Answer

    Thank you for your enquiry. My colleague Dr Sarah Mardle is out of office until Thursday morning. As soon as she gets back, she will get in touch with you and deal with your enquiry. Thank you for your patience.

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    Abcam Scientific Support

    回复于 Apr 06 2005

    Question

    BATCH NUMBER 67077 ORDER NUMBER 71216 DESCRIPTION OF THE PROBLEM We have recently used your antibody ab6748 (Rabbit polyclonal to Sheep IgG (alkaline phosphatase)) and have serious problems with it. Initially we used it as a secondary antibody against another product of yours Anti-acetyl Lysine ab76 (Sheep polyclonal to acetyl Lysine). We obtained intensive staining on all the used human testis samples including controls omitting primary antibody. This indicated problems with the secondary antibody. Therefore we made a second experiment designed as follows: Only your secondary antibody ab6748 was used in 1:1000 or 1:500 diluted in TBS. We used 4 different blockades: Human Serum (1:4), 2% normal goat serum, BSA 1:5, and Mouse serum 1:10 before applying your antibody. Sections of testicular seminoma fixed in PFA or formalin were used In short: Deparaffination. Microwave treatment with Citrate buffer. Water, TBS. Blockade with the above mentioned. TBS 3x2min. Incubation with antibody ab6748 in TBS, 30 min RT. TBS 2x5min. Relevation buffer (0.5 M TRIS pH 9.5, 0.5 M NaCl, 0.2 M MgCl2) 5min. Development in dark with BCIP /NBT (Levamisol) 10min. This protocol is routinely used twice a week in the lab and have in the last 5 years generated good results. The result was as follows (both fixations reacted equally). antibody ab6748 1:1000 or 1:5000, Human Serum: Serious background staining. antibody ab6748 1:1000 or 1:5000, 2% goat serum: Serious background staining and background respectively. antibody ab6748 1:1000, BSA: background. antibody ab6748 1:5000, BSA: slight background and background at the edge of sections. antibody ab6748 1:1000 Mouse serum: background. antibody ab6748 1:5000 Negative to sleight background in the edge of sections. Controls: Omission of antibody ab6748 and all combinations of blockades (Human Serum (1:4), 2% normal goat serum, BSA 1:5, and Mouse serum 1:10) were all negative. As a result of these results (and the initial experiment) we find it problematic to continue our experiments as something seems to be wrong with this antibody. Furthermore in your application sheet you recommend dilutions in the range of 1:100 to 1:1000 for IHC, although blockade with mouse serum and antibody ab6748 1:5000 gives a slight possibility for successful experiments, we regard this inadequate for a commercial antibody and tend to believe that something is wrong with this antibody: antibody ab6748 lot 67077 Yours sincerely SAMPLE Human testicular samples PRIMARY ANTIBODY Anti-acetyl Lysine ab76 (Sheep polyclonal to acetyl Lysine) SECONDARY ANTIBODY ab6748 (Rabbit polyclonal to Sheep IgG (alkaline phosphatase)) DETECTION METHOD IHC POSITIVE AND NEGATIVE CONTROLS USED omitting primary antibody SAMPLE PREPARATION Deparaffination. Microwave treatment with Citrate buffer. Water, TBS. Blockade with the above mentioned. TBS 3x2min. Incubation with antibody ab6748 in TBS, 30 min RT. TBS 2x5min. Relevation buffer (0.5 M TRIS pH 9.5, 0.5 M NaCl, 0.2 M MgCl2) 5min. Development in dark with BCIP /NBT (Levamisol) 10min. HOW MANY TIMES HAVE YOU TRIED THE APPLICATION? 12 HAVE YOU RUN A "NO PRIMARY" CONTROL? Yes WHAT STEPS HAVE YOU ALTERED? Taken away primary Ab and used different blockades and dillutions

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    Abcam community

    Verified customer

    Asked on Mar 30 2005

    Answer

    I'm very sorry to hear you are having problems with ab6748. We take your complaint very seriously and would appreciate if you could please clarify whether you have tested the antibody with no blocking at all and tell me what permeabilising agent has been used as well as the dilution buffer used? My apologies for the delay, I look forward to hearing from you,

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    Abcam Scientific Support

    回复于 Mar 31 2005

    Please note: All products are "FOR RESEARCH USE ONLY. NOT FOR USE IN DIAGNOSTIC PROCEDURES"
    For licensing inquiries, please contact partnerships@abcam.com

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