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    biotin-nitro-tyrosine-antibody-8c73-ab24496.pdf

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Neuroscience Neurotransmission Nitric Oxide Nitrated Species
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Biotin Anti-Nitro tyrosine 抗体 [8C7.3] (ab24496)

  • Datasheet
Reviews (2)Q&A (6)References (2)

Product price, shipping and contact information

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Promotion Information

Abpromise

保証された製品品質、優れたカスタマー・サポート。 詳細はこちら。

Key features and details

  • Biotin Mouse monoclonal [8C7.3] to Nitro tyrosine
  • Suitable for: IHC-P, WB, ELISA, IP, IHC-Fr
  • Reacts with: Species independent
  • Conjugation: Biotin
  • Isotype: IgG2b

こちらの製品もご検討ください

一次抗体
Product image
HRP Anti-3-Nitrotyrosine antibody [7A12AF6] (ab198491)
標識
Product image
Biotinylation Kit / Biotin Conjugation Kit (Fast, Type A) - Lightning-Link® (ab201795)
一次抗体
Product image
Anti-Nitro tyrosine antibody [HM.11] (ab7048)

関連製品

製品の概要

  • 製品名

    Biotin Anti-Nitro tyrosine antibody [8C7.3]
    Nitro tyrosine 一次抗体 製品一覧
  • 製品の詳細

    Biotin Mouse monoclonal [8C7.3] to Nitro tyrosine
  • 由来種

    Mouse
  • 標識

    Biotin
  • アプリケーション

    適用あり: IHC-P, WB, ELISA, IP, IHC-Frmore details
  • 種交差性

    交差種: Species independent
  • 免疫原

    Full length native protein (purified) corresponding to Nitro tyrosine (biotinylated ).

  • 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 short term (1-2 weeks). Store at -20°C or -80°C. Avoid freeze / thaw cycle.
  • バッファー

    pH: 7.20
    Preservative: 0.02% Sodium azide
    Constituents: PBS, 0.05% BSA
  • Concentration information loading...
  • 精製度

    Protein A purified
  • ポリ/モノ

    モノクローナル
  • クローン名

    8C7.3
  • アイソタイプ

    IgG2b
  • 研究分野

    • Neuroscience
    • Neurotransmission
    • Nitric Oxide
    • Nitrated Species
    • Cardiovascular
    • Atherosclerosis
    • Thrombosis
    • Platelets

関連製品

  • Isotype control

    • Biotin Mouse IgG2b, kappa monoclonal [MPC-11] - Isotype Control (ab18418)

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ab24496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)
Use at an assay dependent concentration.
WB (1)
Use a concentration of 1 µg/ml.
ELISA
Use at an assay dependent concentration.
IP
Use at an assay dependent concentration.
IHC-Fr
Use at an assay dependent concentration.
特記事項
IHC-P
Use at an assay dependent concentration.
WB
Use a concentration of 1 µg/ml.
ELISA
Use at an assay dependent concentration.
IP
Use at an assay dependent concentration.
IHC-Fr
Use at an assay dependent concentration.

ターゲット情報

  • 関連性

    Nitric oxide (NO) is a product of the enzymatic conversion of arginine to citrulline by nitric oxide synthase. NO reacts rapidly with superoxide to form peroxynitrite. At physiological pH and in the presence of transition metals, peroxynitrite undergoes heterolytic cleavage to form hydroxyl anion and nitronium ion, the latter of which nitrates protein tyrosine residues. Thus, the presence of nitrotyrosine on proteins can be used as a marker for peroxynitrite formation in vivo. The presence of nitrotyrosine has been detected in various inflammatory processes including atherosclerotic placques.
  • 別名

    • NO tyrosine antibody
    • nTyr antibody

プロトコール

  • Immunoprecipitation protocols
  • Immunohistochemistry protocols
  • Western blot protocols

Click here to view the general protocols

データシートおよび資料

  • Datasheet download

    Download

参考文献 (2)

ab24496 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。

ab24496 は 2 報の論文で使用されています。

  • Alhalwani AY  et al. Development of a sandwich ELISA with potential for selective quantification of human lactoferrin protein nitrated through disease or environmental exposure. Anal Bioanal Chem 410:1389-1396 (2018). PubMed: 29214534
  • Pais TF  et al. The NAD-dependent deacetylase sirtuin 2 is a suppressor of microglial activation and brain inflammation. EMBO J 32:2603-16 (2013). IHC-P ; Mouse . PubMed: 24013120

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

1-8 of 8 Abreviews or Q&A

Western blot abreview for Anti-Nitro tyrosine antibody

Excellent
Abreviews
Abreviews
abreview image
Application
Western blot
Sample
Mouse Tissue lysate - whole (Melanoma cancer)
Loading amount
30 µg
Specification
Melanoma cancer
Treatment
5gy Irradiation
Gel Running Conditions
Non-reduced Denaturing (10%)
Blocking step
Milk as blocking agent for 1 hour(s) and 0 minute(s) · Concentration: 3% · Temperature: 25°C
Read More

Ms. Seontae Kim

Verified customer

投稿 Jan 02 2013

Immunohistochemistry (Formalin/PFA-fixed paraffin-embedded sections) abreview for Anti-Nitro tyrosine antibody

Excellent
Abreviews
Abreviews
abreview image
Application
Immunohistochemistry (Formalin/PFA-fixed paraffin-embedded sections)
Sample
Mouse Tissue sections (Melanoma cancer)
Specification
Melanoma cancer
Fixative
4% Formalin
Antigen retrieval step
Heat mediated - Buffer/Enzyme Used: 121 Celsius for 10min autoclaved
Permeabilization
Yes - 0.1% SDS
Blocking step
BSA as blocking agent for 15 minute(s) · Concentration: 1% · Temperature: 25°C
Read More

Ms. Seontae Kim

Verified customer

投稿 Dec 20 2012

Question

Hi I plan to use IHC-P to detect nitro-tyrosine (as a marker for oxidative stress) on the formalin-fixed mouse pulmonary arteries. I have several questions regarding this product: (1) is a high background to use this antibody on mouse tissues, as the host is mouse. (2) what is a recommended positive control for this antibody? (3) there are other nitro-tyrosine antibodies for IHC-P application (ab7048 and ab78163, etc). Which one would you like to recommend for my application on mouse pulmonary arteries? (4) do you have suggestions on additional markers for oxidative stress in arteries?

Read More

Abcam community

Verified customer

Asked on Jun 26 2014

Answer

Using a mouse antibody to for mouse IHC can lead to high background if you are detecting the antibody with a secondary anti-mouse IgG antibody, since the anti-IgG may detect endogenous IgG in the sample. You can check for that by incubating a section with just the secondary antibody, which is a recommended negative control for any IHC. There are a few approaches to minimizing the background. One is to directly conjugate the primary antibody (e.g., the anti-nitro tyrosine) to an enzyme (or fluorochrome) so that using an enzyme-conjugated anti-mouse secondary is not necessary.

As it happens, ab24496 is already biotinylated, which was not previously noted on the datasheet. So it could be detected with HRP-conjugated streptavidin, such as ab7403, if you want to visualize the immunostain with light microscopy rather than fluorescent microscopy.

Click here (or use the following: https://www.abcam.com/Streptavidin-HRP-ab7403.html).

We do not have a recommendation for a nitrosylated tyrosine positive control. I suggest looking at the references on the datasheet for ab7408 or the literature in general.

Click here (or use the following: https://www.abcam.com/ab7408.html).

This antibody has the most references of the nitro tyrosine antibodies we have and is possibly a better choice than ab24496 but we have not compared them side by side. It is not directly conjugated to anything, so you would need to detect it with a secondary antibody. A good choice for this would be ab98703, which is specific for the isotype subclass of ab7408, IgG2b, and it has been absorbed (purified) to remove reactivity with other subclasses of mouse IgG. Since IgG2b is a relatively rare subclass, background due to staining of endogenous IgG in the tissue section is unlikely to be a problem.

Click here (or use the following: https://www.abcam.com/Goat-Mouse-IgG2b-heavy-chain-HRP-preadsorbed-ab98703.html).

Another marker of oxidative stress is 8-hydroxyguanosine. We have several antibodies against this. I suggest ab62623 (which is also mouse IgG2b) or the goat polyclonal antibody ab10802, followed by an anti-goat IgG secondary antibody directly conjugated to HRP and absorbed to remove reactivity with mouse IgG. Please let me know if you need help finding this secondary antibody.

Read More

Tom Ruyle

Abcam Scientific Support

Answered on Jun 26 2014

Question

Hello, here are the answers to your questions:

-I don't think there is a possibility of the gel being overloaded as we used different total protein concentration, as low as 25ug and still the problem persisted. 100ug is tolerated well by the type and thickness of gels we prepare. Also, we checked the transfer with Ponceau Red and it was good in all cases.

-The material used was total lysates from rat cortex tissue, prepared with very standardized protocols we have at the lab, which work well for all other antibodies that we are currently using for Western blotting.

-What we want to see with the antibody is nitrotyrosine in all proteins in general, we will then perform IP to see whether our protein of interest (cytosolic) contains nitrotyrosine residues.

-The samples have not been treated to stimulate nitrosylation because we want to determine whether this occurs in an Alzheimer transgenic model which there is evidence that this is the case. We have also been working with aged animals (14 months old) and there is also evidence that nitrosylation increases with aging (published in rats).

-Were these antibodies tested previously in tissue lysates?

-If you have other anti-nitrotyrosine antibodies could you consider the possibility of sending us a few aliquots to test which one is more suitable to our purposes?

Thank you,

I hope we can find a solution to this problem,

Read More

Abcam community

Verified customer

Asked on Mar 28 2012

Answer

Thank you for getting back to me and for answering to my further questions promptly.

I have been discussing this enquiry with my colleague in the Lab and the methods seem to be chosen all look appropriate ECl, milk block etc, Xray film.

It is a bit surprising that there aren’t backgrounds from the rodents immune system (rat circulating IgGs) so you might wish to change the secondary HRP conjugate.With issues like this we are always presuming that there are sufficient nitrated tyrosines in the sample in question to be seen.

Is the level high enough to back up the hypothesis?

This target is a product of the right kind of oxidative stressors and without those there won’t be any modification. To validate this, trying another antibody (rabbit polyclonal) would be a good idea..

To show this antibody works we can use a positive control – add peroxynitrite to the sample – this can be obtained from Millipore. Other donors include SNAP or SIN1 which would create 3-NT.

I hope this will be useful for you. Should you still have any problem with this antibody after following these suggestions, then please do not hesitate to contact our Technical Department again.

Read More

Abcam Scientific Support

Answered on Mar 28 2012

Question

We bought 1 Anti-nitrotyrosine Abcam antibody Ab24496 (received 27-10-2011) lot # GR23989-3which didn't work and was replaced by Ab110282 (received 2-12-2011) lot# GR63357-2. In both cases, the detection of specific nitrotyrosine bands was unsuccessful, the blot appeared dark with white bands or just dark with no bands. We have tried the following conditions for both antibodies:

-Different blocking conditions (BSA 5%-10% and milk 5%-10%)
-Protein concentration (25 ug - 100 ug)
-We used rat and mice cortex tissue
-Western blot detected with Regular ECL and ECL plus
-Detection with autoradriographic film and Storm phosphoimager
-Concentration of 1ry antibody 1:100 - 1:5000
-Concentration of 2ry antibody: 1:5000-1:50 000
-Our secondary antibody is working well with other primary antibodies

If we cannot get reimbursed, can we get this antibody instead: Anti-beta Actin antibody - Loading Control (ab8227)

Thank you

Read More

Abcam community

Verified customer

Asked on Mar 26 2012

Answer

I am very sorry to hear that both antibodies did not work properly (ab24496 and ab110282).

I can offer you a replacement vial as you wish but it would be important to find out why two antibodies failed to work.

I have read through again the detailed protocols you kindly forwarded to Abcam and I would like to make the following comments/suggestions:

I understand that rat brain lysates were used in these experiments and 25 ug - 100 ug total protein was loaded onto the gel. It may well be tha the gel is overloaded.

Q1: Could you please confirm if total lysates or cellular fractions were used?

Q2: Are you particularly interested in cytosolic protein or any cellular organelle-related proteins?

Q3: Have you treated the samples to stimulate the nitrosylation of teh protein?

As you can see on the Western blot images (ab110282) purified bovine heart mitochondria was used for testing and characterization.

Thank you for your understanding and co-operation in this matter.

I look forward to hearing from you soon.

Read More

Abcam Scientific Support

Answered on Mar 26 2012

Question

We bought 1 Anti-nitrotyrosine Abcam antibody Ab24496 (received 27-10-2011) lot # GR23989-3which didn't work and was replaced by Ab110282 (received 2-12-2011) lot# GR63357-2. In both cases, the detection of specific nitrotyrosine bands was unsuccessful, the blot appeared dark with white bands or just dark with no bands. We have tried the following conditions for both antibodies:

-Different blocking conditions (BSA 5%-10% and milk 5%-10%)
-Protein concentration (25 ug - 100 ug)
-We used rat and mice cortex tissue
-Western blot detected with Regular ECL and ECL plus
-Detection with autoradriographic film and Storm phosphoimager
-Concentration of 1ry antibody 1:100 - 1:5000
-Concentration of 2ry antibody: 1:5000-1:50 000
-Our secondary antibody is working well with other primary antibodies

If we cannot get reimbursed, can we get this antibody instead: Anti-beta Actin antibody - Loading Control (ab8227)

Thank you

Read More

Abcam community

Verified customer

Asked on Mar 13 2012

Answer

Thank you for your enquiry. It is very unfortunate that both of these products (ab24496 and ab110282) do not perform as they are expected to do so.

I would like to reassure you that I take your comment seriously. Though, you have kindly provided some details, it would be much appreciated if I could get some more information which would help me identify the source of the problem.

Could you please provide some further details of the protocol used and complete the following form (attached as a word document). It would be much appreciated if you could attach an image to the response.

I am particularly interested in the following:

- sample preparation, whole lysate or cellular fraction, buffer used, any stimulation to induce nitro tyrosine etc,

- incubation with the 1ry and the 2ry antibodies i.e. time, temperature,

- blocking time and temperature,

- specification of the secondary antibody (ie. host species, what type of immunoglobulin it was raised against),

- positive control used etc.

Thank you for your understanding and co-operation in this matter. I look forward to hearing from you soon and resolving this issue as soon as possible.

Read More

Abcam Scientific Support

Answered on Mar 13 2012

Question

Thank you for your help. We would be most grateful if we could try another of your antibodies against nitrotyrosine. We would like to try ab110282 MS703 as it seems to meet more closely our need i.e. it is said that it works in rat homogenates and works for WB as well as other applications. Sincerely,

Read More

Abcam community

Verified customer

Asked on Nov 29 2011

Answer

Thank you for your response. This is to let you know that I have placed a new order for you - for one vial of ab110282 as a free of charge replacement (exchange for the original item ab24496) and the new order number is 992370. 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.  

Read More

Abcam Scientific Support

Answered on Nov 29 2011

Question

We are trying to do western blots, a technique commonly used in our lab, using your antibody against anti-nitrotyrosine (ab24496) and its not working. Our samples are homogenates of rat brain, prepared as usual in cell lysis buffer (from cell signaling) supplemented with complete protease inhibitor cocktail (from Roche). We are running in denaturing conditions (with SDS) and we tried to transfer to PVDF and nitrocellulose. According to Rouge Ponceau staining of the membranes, our proteins are fine. We tried blocking in different conditions: non-fat milk 5-10% or BSA 5% (from 2 to 16 hours) We tried different concentrations of this primary (ab24496): 1/250 to 1/5000. We tried different concentrations of the secondary (peroxidase goat anti-mouse): 1/5000 to 1/50000. This secondary antibody works beautifully with other primary antibodies. The best signal we can get is white bands on dark background (see attached document). Can you please tell us the conditions in which this antibody should work. I didnt find any published papers using this antibody. Thanks for a fast reply! Abcam WB questionnaire 1) Abcam product code: ab24496 (mouse monoclonal antibody anti-nitrotyrosine) 2) Abcam order reference number or product batch number: lot:GR23989-3 3) Description of the problem : Unable to obtain a good signal despite trying several different conditions. The best signal we can get is white bands on dark background (see figure) 4) Sample preparation: Type of sample (whole cell lysates, fraction, recombinant protein…): total rat brain homogenates Lysis buffer : cell lysis buffer 1X (from cell signaling) Protease inhibitors: complete protease inhibitor cocktail (from Roche) Phosphatase inhibitors: No Reducing agent : SDS 2% and b-mercaptoethanol 1% Boiling for ≥5 min? yes Protein loaded ug/lane or cells/lane : tried from 25-100 ug (most often 70 ug) Positive control :yes (brain extracts of transgenics rats were high levels were demonstrated previously by our team, using the same antibody (Bruno et al Neurobiol aging 2011 (rats); Bruno et al J Neuropathol Exp Neurol 2009 (human)) Negative control :no 5) Percentage of gel: 12% Type of membrane : tried PVDF or nitrocellulose Protein transfer verified :yes with rouge ponceau Blocking agent and concentration: tried non-fat milk 5-10% or BSA 5% in TBS-T 0.1% Blocking time: tried from 2 to 16 hours Blocking temperature : if 2-5 hours: room temperature; if 16 hours: 4 degrees 6) Primary antibody (If more than one was used, describe in “additional notes”) : Concentration or dilution: tried 1/250 to 1/5000 Diluent buffer : tried non-fat milk 5-10% or BSA 5% in TBS-T 0.1% Incubation time: 2h at room temperature or 16h at 4degrees Incubation temperature: 2h at room temperature or 16h at 4degrees 7) Secondary antibody: peroxidase goat anti-mouse) Species: goat Reacts against: mouse Concentration or dilution : tried 1/5000 to 1/50000 Diluent buffer :TBS-T 0.1% Incubation time: 1 hour Incubation temperature: room temperature Fluorochrome or enzyme conjugate: peroxidase (HRP) 8) Washing after primary and secondary antibodies: Buffer: TBS-T 0.1% Number of washes: after primary, 5 washes in 1 hour, after secondary, 3 washes in 30 min Detection system: ECL plus on autoradiographic film or STORM Do you obtain the same results every time? Either no signal or white bands on dark backgroung What steps have you altered to try and optimize the use of this antibody? All except homogenate preparation Document attachment: Attaching images of your blot is strongly recommended and can greatly speed up our investigation of your problem

Read More

Abcam community

Verified customer

Asked on Nov 28 2011

Answer

Thank you for contacting Abcam Technical Team and for taking the time to provide some useful details of the experiments. I am very sorry to hear that you are having problems with this product. Looking at the WB image you have kindly attached, it is very likely that ab24496 is inactive since you have nice signal with an alternative antibody after reprobing using the same samples. I would like to reassure you that our Abpromise applies to your complaint since you purchased this product within the guarantee period. This means that in the event that a product is not functioning in the applications/species cited on the product data sheet (and the problem has been reported within 6 months of purchase) we will happily offer a credit note/refund to the value of the product purchased. I could offer you either a new vial as a free of charge replacement or a credit note which you can use in the future. Please do let me know how you wish to proceed with this enquiry. I look forward to hearing from you and hope to solve this problem as soon as possible.  

Read More

Abcam Scientific Support

Answered on Nov 28 2011

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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