4-amino Biphenyl DNA Antibody (4C11) - BSA Free

Novus Biologicals | Catalog # NB100-415

Novus Biologicals
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Key Product Details

Species Reactivity

Validated:

Mouse, All Species

Cited:

Mouse

Applications

Validated:

Immunohistochemistry, ELISA, Immunocytochemistry/ Immunofluorescence

Cited:

IF/IHC

Label

Unconjugated

Antibody Source

Monoclonal Mouse Clone # 4C11

Format

BSA Free
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Product Specifications

Immunogen

4-amino Biphenyl DNA

Reactivity Notes

Detects DNA from all species. Mouse reactivity reported in scientific literature (PMID: 12700401).

Localization

Nuclear

Clonality

Monoclonal

Host

Mouse

Scientific Data Images for 4-amino Biphenyl DNA Antibody (4C11) - BSA Free

Immunohistochemistry: 4-amino Biphenyl DNA Antibody (4C11) [NB100-415]

Immunohistochemistry: 4-amino Biphenyl DNA Antibody (4C11) [NB100-415]

Immunohistochemistry: 4-amino Biphenyl DNA Antibody (4C11) [NB100-415] - Human breast tumor tissue with high (A) and low (B) adduct levels. Images courtesy of Dr. Regina Santella.

Applications for 4-amino Biphenyl DNA Antibody (4C11) - BSA Free

Application
Recommended Usage

ELISA

1:100-1:2000

Immunocytochemistry/ Immunofluorescence

1:50 1:100

Immunohistochemistry

1:50-1:100
Application Notes
This 4-amino Biphenyl DNA (4C11) antibody is useful for ELISA, Immunocytochemistry/Immunofluorescence and Immunohistochemistry.

Formulation, Preparation, and Storage

Purification

Unpurified

Formulation

Ascites

Format

BSA Free

Preservative

0.1% Sodium Azide

Concentration

This product is unpurified. The exact concentration of antibody is not quantifiable.

Shipping

The product is shipped with polar packs. Upon receipt, store it immediately at the temperature recommended below.

Stability & Storage

Store at 4C short term. Aliquot and store at -20C long term. Avoid freeze-thaw cycles.

Background: 4-amino Biphenyl DNA

4-amino Biphenyl (4-ABP) is an arylamine (aromatic amine) compound and as one of the major carcinogenic constituents of tobacco smoke other environmental sources, it poses critical health hazards to human beings. Under the action of carcinogen activating biotransformation enzymes such as cytochrome P4501A2, 4-ABP gets metabolized to generate a direct-acting mutagen known as N-hydroxy-aminobiphenyl. Nevertheless, the accumulation of biologically active metabolites is dependent on the balance between activation and detoxification enzymes. 4-ABP has been linked to bladder and breast cancers in human beings as well as in rodent models. Our 4-amino Biphenyl DNA antibody (4C11) is a monoclonal antiserum which recognizes 4-aminobiphenyl (4-ABP)-DNA adducts and it has been characterized by competitive enzyme-linked immunosorbent assay (ELISA), immunohistochemistry (IHC) and Immunocytochemistry/Immunofluorescence (ICC/IF) techniques. This antibody does not recognize the DNA adducts of several other aromatic amines tested including 1-aminopyrene, 8-nitro-1-aminopyrene, and 6-nitro-1-aminopyrene.

Alternate Names

4-AMBP DNA, 4-aminobiphenyl DNA, 4-amino-Biphenyl DNA

Additional 4-amino Biphenyl DNA Products

Product Documents for 4-amino Biphenyl DNA Antibody (4C11) - BSA Free

Certificate of Analysis

To download a Certificate of Analysis, please enter a lot or batch number in the search box below.

Product Specific Notices for 4-amino Biphenyl DNA Antibody (4C11) - BSA Free

This product is for research use only and is not approved for use in humans or in clinical diagnosis. Primary Antibodies are guaranteed for 1 year from date of receipt.

Citations for 4-amino Biphenyl DNA Antibody (4C11) - BSA Free

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Protocols

View specific protocols for 4-amino Biphenyl DNA Antibody (4C11) - BSA Free (NB100-415):

4-amino Biphenyl DNA Antibody (4C11):
Competitive ELISA

I Coating of Plates

DNA coating: DNA is dissolved in PBS at appropriate concentration. 0.1 ml is added/well and plates put in 37 degrees Celsius incubator to evaporate overnight. Alternatively, plates can be coated with a 2-fold higher concentration of DNA for 2 hrs at 37 degrees Celsius then used. Column 1 is not coated. These well will not be used for the assay (no blocking, no antibody and no secondary antibody) but will have substrate added for blanking the reader. Plates are stored in the refrigerator.

Protein coating: Proteins are dissolved in PBS at the appropriate concentration. 0.1 ml is added/well and plates put in 37 degrees Celsius incubator to evaporate overnight. Column 1 is again not coated. Plates are stored in the refrigerator.
An alternate protein coating condition is to dissolve the protein in 0.1 M sodium carbonate buffer pH 9.6. 0.1 ml is added/well and the plates are refrigerated for several hours or overnight. They cannot be used after 3 days.
1 M solution 1.59 g Na2CO3 + 2.93 g NaHCO3/100ml

II Assay

1. Label assay sheet and determine which rows are to be used. Row 1 (A-H) is not used; it will be used to blank the spectrophotometer. Avoid using the outer rows if possible (i.e.12A-H, H 1-12 and A 1-12.

2. Wash plate with wash buffer containing PBS-Tween and NaN3 3 x on each side (right side up and upside down). Shake out onto paper towel.

3. Add 0.2 ml/well of 1% FCS in wash buffer to block non specific binding. Solution of FCS should be made fresh.

4. Incubate 1 hr.

5. Preparation of inhibitor series (during incubation of plate with FCS). Calculate appropriate concentrations to give desired fmol/well=fmol/0.05 ml. Make serial dilutions by adding PBS or CT DNA to tubes followed by competitor.

6. Prepare antibody in 1% FCS washing buffer.

7. At end of incubation period, shake out solution from plate and tap onto paper towel to dry.

8. Add 0.05 ml of competitor to each well followed by 0.05 ml of diluted antibody. Be sure to run all controls including zero (no competitor), minus Ab ( no antigen specific antibody but secondary antisera) and positive and negative controls.

9. Incubate for 90 min at 37 degrees Celsius.

10. Wash the plate with washing buffer 3 times on each side. Tap onto paper towels.

11. Secondary antisera - Use goat anti-mouse IgG-alkaline phosphatase for monoclonals and anti rabbit for polyclonals. Dilute as appropriate and add 0.1 ml/well.

12. Incubate for 90 min at 37 degrees Celsius.

13. Wash with wash buffer 3 x each side. Tap onto paper towel.

14. Wash plate 2 times with 0.01 M diethanolamine using the was bottle and covering the well completely each time. Tap onto paper towel. This step removes phosphate buffer which inhibits alkaline phosphatase activity.

15. Prepare the substrate - 2 tablets 95 mg/tablet) Sigma 104 in 10 ml 1 M diethanolamine, pH 8.6. Final concentration 1 mg/ml. Avoid physical contact of skin with the tablets since skin contains alkaline phosphatase. Add 0.1 ml/well

16. Incubate at 37 degrees Celsius and read absorbance at 405 nm. The absorbance of the 0 fmol standard should be between 0.5 and 1. Values above 2 are not usable since the reader may not be linear in this range.

Rinse water - One liter of H2O + 2 ml 10% NaN3
Wash buffer - One liter of 1 x PBS + 500 ul Tween 20 + 2 ml 10% NaN3
Blocking buffer - Wash buffer + 1% FCS

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FAQs

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