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  1. Link

    thyroid-peroxidasetpo-antibody-moab47-ab12500.pdf

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Signal Transduction Growth Factors/Hormones Hormones
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Anti-Thyroid Peroxidase/TPO 抗体 [MoAb47] (ab12500)

  • Datasheet
  • SDS
Submit a review Q&A (5)References (3)

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Abpromise

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Immunohistochemistry (Formalin/PFA-fixed paraffin-embedded sections) - Anti-Thyroid Peroxidase/TPO antibody [MoAb47] (ab12500)

    Key features and details

    • Mouse monoclonal [MoAb47] to Thyroid Peroxidase/TPO
    • Suitable for: IHC-P
    • Reacts with: Human
    • Isotype: IgG1

    こちらの製品もご検討ください

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    Product image
    Anti-IL-6 antibody [1.2-2B11-2G10] (ab9324)

    関連製品

    製品の概要

    • 製品名

      Anti-Thyroid Peroxidase/TPO antibody [MoAb47]
      Thyroid Peroxidase/TPO 一次抗体 製品一覧
    • 製品の詳細

      Mouse monoclonal [MoAb47] to Thyroid Peroxidase/TPO
    • 由来種

      Mouse
    • アプリケーション

      適用あり: IHC-Pmore details
    • 種交差性

      交差種: Human
    • 免疫原

      Full length native protein (purified) corresponding to Human Thyroid Peroxidase/TPO.
      Database link: P07202

    • ポジティブ・コントロール

      • Thyroid
    • 特記事項

      The Life Science industry has been in the grips of a reproducibility crisis for a number of years. Abcam is leading the way in addressing this with our range of recombinant monoclonal antibodies and knockout edited cell lines for gold-standard validation. Please check that this product meets your needs before purchasing.

      If you have any questions, special requirements or concerns, please send us an inquiry and/or contact our Support team ahead of purchase. Recommended alternatives for this product can be found below, along with publications, customer reviews and Q&As

    製品の特性

    • 製品の状態

      Liquid
    • 保存方法

      Shipped at 4°C. Store at +4°C.
    • バッファー

      pH: 7.3
      Preservative: 0.05% Sodium azide
      Constituent: Tissue culture supernatant
    • Concentration information loading...
    • 精製度

      Tissue culture supernatant
    • ポリ/モノ

      モノクローナル
    • クローン名

      MoAb47
    • アイソタイプ

      IgG1
    • 研究分野

      • Signal Transduction
      • Growth Factors/Hormones
      • Hormones
      • Neuroscience
      • Endocrine system
      • Thyroid axis
      • Cancer
      • Cancer Metabolism
      • Metabolic signaling pathway
      • Hormone biosynthesis
      • Cancer
      • Cancer Metabolism
      • Cellular metabolic process
      • Metabolism
      • Pathways and Processes
      • Redox metabolism
      • Antioxidants
      • Metabolism
      • Pathways and Processes
      • Endocrine metabolism
      • Hormone biosynthesis
      • Metabolism
      • Types of disease
      • Cancer

    関連製品

    • Compatible Secondaries

      • Goat Anti-Mouse IgG H&L (Alexa Fluor® 488) (ab150113)
      • Goat Anti-Mouse IgG H&L (HRP) (ab205719)
    • Isotype control

      • Mouse IgG1, kappa monoclonal [15-6E10A7] - Isotype Control (ab170190)

    アプリケーション

    The Abpromise guarantee

    Abpromise保証は、 次のテスト済みアプリケーションにおけるab12500の使用に適用されます

    アプリケーションノートには、推奨の開始希釈率がありますが、適切な希釈率につきましてはご検討ください。

    アプリケーション Abreviews 特記事項
    IHC-P
    1/10 - 1/25. Perform heat mediated antigen retrieval with Tris/EDTA buffer pH 9.0 before commencing with IHC staining protocol.

    Primary incubation for 30 min at room temperature.

    特記事項
    IHC-P
    1/10 - 1/25. Perform heat mediated antigen retrieval with Tris/EDTA buffer pH 9.0 before commencing with IHC staining protocol.

    Primary incubation for 30 min at room temperature.

    ターゲット情報

    • 機能

      Iodination and coupling of the hormonogenic tyrosines in thyroglobulin to yield the thyroid hormones T(3) and T(4).
    • パスウェイ

      Hormone biosynthesis; thyroid hormone biosynthesis.
    • 関連疾患

      Note=An alternative splicing in the thyroperoxidase mRNA can cause Graves' disease.
      Defects in TPO are the cause of congenital hypothyroidism due to dyshormonogenesis type 2A (CHDH2A) [MIM:274500]; also called genetic defect in thyroid hormonogenesis 2A or thyroid hormone organification defect II. CHDH2A is due to defective conversion of accumulated iodide to organically bound iodine. The iodide organification defect can be partial or complete.
    • 配列類似性

      Belongs to the peroxidase family. XPO subfamily.
      Contains 1 EGF-like domain.
      Contains 1 Sushi (CCP/SCR) domain.
    • 翻訳後修飾

      Glycosylated.
      Heme is covalently bound through a H(2)O(2)-dependent autocatalytic process. Heme insertion is important for the delivery of protein at the cell surface.
      Cleaved in its N-terminal part.
    • 細胞内局在

      Membrane and Cell surface.
    • Target information above from: UniProt accession P07202 The UniProt Consortium
      The Universal Protein Resource (UniProt) in 2010
      Nucleic Acids Res. 38:D142-D148 (2010) .

      Information by UniProt
    • 参照データベース

      • Entrez Gene: 7173 Human
      • Omim: 606765 Human
      • SwissProt: P07202 Human
      • Unigene: 467554 Human
      • 別名

        • MSA antibody
        • PERT_HUMAN antibody
        • TDH2A antibody
        • Thyroid microsomal antigen antibody
        • Thyroid peroxidase antibody
        • Thyroperoxidase antibody
        • TPO antibody
        • TPX antibody
        see all

      画像

      • Immunohistochemistry (Formalin/PFA-fixed paraffin-embedded sections) - Anti-Thyroid Peroxidase/TPO antibody [MoAb47] (ab12500)
        Immunohistochemistry (Formalin/PFA-fixed paraffin-embedded sections) - Anti-Thyroid Peroxidase/TPO antibody [MoAb47] (ab12500)

        Formalin-fixed, paraffin-embeded human thyroid tissue stained for Thyroid Peroxidase/TPO using ab12500 at 1/10 dilution in immunohistochemical analysis.

      プロトコール

      • Immunohistochemistry protocols

      Click here to view the general protocols

      データシートおよび資料

      • SDS download

      • Datasheet download

        Download

      参考文献 (3)

      ab12500 を使用した論文を発表された方は、こちらまでお知らせください。データシートに掲載させていただきます。

      ab12500 は 3 報の論文で使用されています。

      • Muller I  et al. Does thyroid peroxidase provide an antigenic link between thyroid autoimmunity and breast cancer? Int J Cancer 134:1706-14 (2014). PubMed: 24114667
      • Cairns DM  et al. Muscle cells enhance resistance to pro-inflammatory cytokine-induced cartilage destruction. Biochem Biophys Res Commun 392:22-8 (2010). PubMed: 20043873
      • Cairns DM  et al. The role of muscle cells in regulating cartilage matrix production. J Orthop Res 28:529-36 (2010). PubMed: 19813241

      レビューと Q&A

      Show All レビュー Q&A
      レビューを送る 質問を送る

      1-5 of 5 Abreviews or Q&A

      Question


      Please provide concentration of ab12500

      Read More

      Abcam community

      Verified customer

      Asked on May 24 2012

      Answer

      Thank you for your enquiry.

      I can confirm that ab12500 Anti-Thyroid Peroxidase antibody [MoAb47]antibody is sold as tissue culture supernatant. Unpurified antibodies, such as those sold as whole antiserum, ascites or tissue culture supernatant will not have a concentration stated on the datasheet. Antibody concentration is usually determined by protein assay, tissue culture supernatant will contain a lot of other proteins, which means the antibody quantification would not be accurate.

      I can confirm that for tissue culture supernatant, concentration of antibody is known to very between 1 - 3 mg/ml.

      I am sorry we are not able to provide an exact concentration on this occasion, but hope this information will be helpful to you.

      For peptide blocking, usually use twice the amount of peptide to antibody although please note that this may require some optimization:
      https://www.abcam.com/index.html?pageconfig=resource&rid=11378

      I hope this will be helpful. If you have any further questions, please do not hesitate to contact us.

      Read More

      Abcam Scientific Support

      Answered on May 24 2012

      Question

      I'm going to start an experiment of Immunohistochemistry with your Mouse monoclonal antibody MoAb47 to thyroid peroxidase (ab12500).



      I need to perform the blocking procedure with immunizing peptide (BL) protocol but on the ab12500 datasheet there is NOT the concentration of the antibody.



      How many micrograms of protein I have to use for each microliter of antibody to block it?!



      Please speak soon, I have to perform the experiment today!

      Read More

      Abcam community

      Verified customer

      Asked on May 24 2012

      Answer

      Thank you for contacting us.

      According to the datasheet, this antibody is a non-purified cell culture supernatant product. That means, along with whole serum andascitis products, the antibody concentration cannot be determined as there are too many other proteins in this solution as well.


      However, we have a table under our Technical FAQs (Question 8, What concentration of primary antibody should I use?) which explains how much specific antibody can be expected in the non-purified products.


      As a supernatant, the antibody concentration should be between 1 - 3 mg/ml. I would therefore suggest to use a concentration of 6 mg/ml, to be on the safe side.

      I hope this information is helpful to you. Please do not hesitate to contact us if you need any more advice or information.

      Use our products? Submit an Abreview. Earn rewards!
      https://www.abcam.com/abreviews

      Read More

      Abcam Scientific Support

      Answered on May 24 2012

      Question

      My customer is using using Biotin-XX goat anti-mouse IgG (H+L) secondary antibody and it is a highly sensitive biotin-based detection method, here is the details of the product :http://products.invitrogen.com/ivgn/product/W10132 Based on the last result (dot blot) that i got, there was totally no signal at 1/500 dilution or 16ul in 8ml of washing buffer (serum based blocking buffer, incubated at room temp for 1hour) for this protein ( The signal that showed in the picture that attached in the previous email is the result of another antibody Moab47. The purpose of showing this result is to prove the method is working!!!). Apart from this, i have also tried different concentration of sample (up to 160ug!!!) but still failed to detect any signal. Since other users managed to detect the protein by using only 20 ug of total cell lysate and antibody dilution at 1:4000, i don't think i should repeat my experiment with 1/250 dilution antibody!!! For you information, it is no way for the customer to keep on trying with different concentration as the customer is wasting his reagents. The customer really need a good and workable solution so that he can solve his problem. Obviously, this is not the detection problem and also not the method problem as it is working in other antibodies. For you information, my customer antibody is only left one reaction and what he need is a good solution and method to help him solve the problem that he got. Thank you very much and hope to receive your soonest reply. Thanks again. Best regards,

      Read More

      Abcam community

      Verified customer

      Asked on Jan 11 2012

      Answer

      Thank you for providing some further information. I understand your customer has used up most of the product during testing and optimization. This is to let you know that I have confirmed and agreed on placing a new order for your customer - for one vial ofab818 (from batch: GR59271-2) as a free of charge replacement. I hope the second vial will work as it is expected, and please do let me know how you are getting on with this product. Dear Colleague, Please add 1 vial ofab818 (from a different batch: GR59271-2) to the next shipment for Bitalifsc. Original CCE ID: XXXXXXX Original Order:XXXXXXX Problem is: wrong band size on Western blot and no signal in Dot blot Many thanks.

      Read More

      Abcam Scientific Support

      Answered on Jan 11 2012

      Question

      Hi Tech, Below is my customer reply, kindly check. Picture is included in the document. Thanks Best regards, I have bought two antibodies (ab12500 and ab818) from your company and only one of them (ab818) is not working. Here i would like to include the details of my experiment: ab818 antibody 1) Positive control - Q: What type of cell/tissue lysate was used for positive control? A: HepG2 total cell lysate (positive control): Dot bot ( Failed to detect any) Sample: Thyroid tissue (Total cell lysate by using RIPA that formulated by your company) Western blot: Failed 2) Lysate - Q: Have you prepared nuclear lysate? No. Only total cell lysate. 3) Secondary antibody -What secondary antibody was applied (host species, specificity)? Biotin-XX goat anti-mouse IgG (H+L) 4) Image - Q: It would be much appreciated if you could attach a new image to the response which represent the MW band sizes and the content of the different lanes. Refer to the attachment. I am looking forward to hearing from you again soon. Thanks!

      Read More

      Abcam community

      Verified customer

      Asked on Jan 09 2012

      Answer

      Thank you for getting back to me and for providing some further details. I understand that whilst ab818 failed to work In Western blot and in Dot blot; the other antibody ab12500 seemed to be fine. It is important to mention that these antibodies detect different target proteins (TBP and Thyroid Peroxidase, respectively) so they can't be used as positive control. The localization of these proteins are also different as well as the purity and the concentration of the antibodies (Protein G purified and Tissue culture supernatant). 1) Localisation: TBP protein is localized in the cell nuclei so it is recommended preparing nuclear lysate and using it for Western blot application. As the datasheet indicates HeLa nuclear extract can be applied as positive control. This is the best way to find out if the antibody is still active or not. 2) Dilution/concentration: Has the customer tried different dilution i.e. 1/500, 1/250 to see if the signal is getting stronger. This is particular important since whole cell lysate – rather than nuclear lysate - was applied. 3) Detection system: I understand that the secondary antibody was Biotin-XX goat anti-mouse IgG (H+L). Could you explain if the detection is ECL/ECL Plus or other type? Does it include an enzyme/fluorochrome conjugated system? In case it was not ECL system, optimization of the primary antibody would be even more essential I look forward to hearing from you soon.

      Read More

      Abcam Scientific Support

      Answered on Jan 09 2012

      Question

      I am a Rome Istitute of Health Lab Technician. Normally I work with abs and your company is very important to allow me in going on. I 'd like to know about further applications or new technical unknoledgements of ab12500 (anti-Human thyroid peroxidase), for answerin to my questions below. Have you ever try it on other animal species (rat)? if yes, can you send me the protocol of your rat method? if no , can you send the protocol of your human method as well?

      Read More

      Abcam community

      Verified customer

      Asked on Sep 15 2006

      Answer

      Thank you for your enquiry. All the information we have on species cross reactivity is specified on the datasheet, these are updated as soon as any new information is brought to our attention. As far as we are aware, cross reactivity with rat has not yet been tested for use with ab12500. Should you decide to go ahead and purchase this product, please let us know how you get on by submitting an Abreview and in return we will award you Abpoints, which can be redeemed on a number of rewards (a further 100 points will be offered for an image). You can find our IHC protocol at: https://www.abcam.com/assets/pdf/protocols/IHC-paraffin%20protocol%20(IHC-P).pdf This antibody is recommended to be used at 1/10 to 1/25 in an ABC method. You should perform heat mediated antigen retrieval with 1mM EDTA buffer (pH 9.0) before commencing with IHC staining protocol. We suggest incubating with the primary for 30-60 minutes at room temperature. Please let me know if you require any further assistance.

      Read More

      Abcam Scientific Support

      Answered on Sep 15 2006

      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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