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[供應(yīng)]Histone antigen

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產(chǎn)地:新西蘭

更新時(shí)間:2024-10-11 21:00:07

有效期:2024年10月11日 -- 2025年4月11日

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Identity:Histone H1, H2A, H2B, H3 and H4Source Material:Bovine thymus (New Zealand origin).Clinical Indications:Autoantibodies present in systemic lupus erythematosus, drug-induced lupus erythematosus

HISTONE ANTIGEN 
AROTEC_Histone_Product_Info.pdf Version/Date: A/00.06.02 
ATH01-02 Histone antigen 0.20 mg 
ATH01-05 Histone antigen 0.50 mg 
ATH01-10 1.0 mg 
_________________________________________________________________________________
Description of the Product
Purified from bovine thymus. After coating onto ELISA plates 
the product will bind autoantibodies to histone antigen. 
Purity: The histone autoantigen is more than 90% pure, as 
assessed by SDS gel electrophoresis. 
Concentration: 0.5 -2.0 mg protein/ml. 
Storage: The product is stabilised with 0.1% Micr-O-protectTM

Store at -20 o
C or below (long term) or at +4o
C (short term). 
Avoid repeated freezing and thawing. Mix thoroughly before 
use. 
Clinical and Biochemical Data 
Autoantibodies against histones (AHAs) are observed in a 
number of autoimmune diseases. AHA are reported in 50-80% 
of patients with Systemic Lupus Erythematosus (SLE) being 
highest in patients with active disease1
. Although H1 and H2B 
are the most common epitopes in SLE, many SLE patients 
have conformation-dependent AHA, directed against the 
histone complex2
. AHA have particular clinical significance for 
drug-induced lupus, particularly in the diagnosis of antinuclear 
antibody positive patients receiving proc*, hydralazine 
and isoniazide3
. AHA are also prevalent in Felty’s syndrome 
(83%), rheumatoid arthritis (75%) and juvenile arthritis (50-
75%)2
, scleroderma4,5 systemic sclerosis6
 and mixed 
connective tissue disease7
. AHA (predominantly against H1) 
are also observed in approximay 76% of patients with 
primary biliary cirrhosis2

Histones are small DNA-binding proteins and the major protein 
component of the nucleosome. The nucleosome consists of 
146 base pairs of DNA wrapped around an octomer of core 
histone proteins composed of a central tetramer of two H3-H4 
dimers flanked by two H2A-H2B dimers8
. Histone H1 is a 
linker histone, present between each nucleosome, and is 
responsible for establishing chromatin structure. The 
molecular weights of the core histones range from 11,000 to 
15,000. Histone H1 is larger, with a molecular weight of 
23,000. All of the histones contain many basic amino acids, 
with histones H3 and H4 being arginine rich, while H2A and 
H2B are slightly lysine-rich8

Biochemical and serological studies have revealed a more 
complicated picture of histone antigenicity than initially 
recognised, particularly highlighted by observations whereby 
separation of the histone complex into its individual 
components using harsh conditions can result in a loss of 
complex formation and antibody reactivity9,10. Histone epitopes 
are often located in accessible regions of chromatin (especially 
for H1 and H2A/H2B)11 or are conformational determinants 
resulting from the association of several histone components. 
Acetylation of histone lysine residues may also play a role in 
SLE autoantigenicity12. The H2A-H2B dimer is the main 
antigen in drug-induce lupus, although also observed in SLE, 
whereas linear epitopes are generally only observed for core 
histones2

Histone amino acid sequences are highly conserved between 
species, even between animals and plants13. AROTEC 
histone antigen is prepared from calf thymus chromatin and 
contains the five main histones, H1, H2A, H2B, H3 and H4, 
extracted and purified without the use if harsh denaturing 
reagents to ensure maximum reactivity with human 
autoantibodies. 
Methodology
The following is an ELISA procedure which can be used to 
detect anti-histone autoantibodies in human serum using the 
ATH01 purified histone antigen: 
1. Dilute the purified antigen to 1.0-2.0 ?g/ml in 50 mM 
carbonate buffer, pH 9.6 containing 0.5% (w/v) sodium 
deoxycholate. 
2. Coat ELISA plates with 100 ?l of diluted antigen per well. 
Cover and incubate 24 hours at +4o
C. 
3. Empty the plates and remove excess liquid by tapping on a 
paper towel. 
4. Block excess protein binding sites by adding 200 ?l PBS 
containing 1% BSA per well. Cover and incubate at +4o

overnight. 
5. Empty plates and apply 100 ?l of serum samples diluted 
1:100 in PBS / 1% BSA / 0.1% Tween?
 20. Incubate at room 
temperature for 1 hour. 
6. Empty plates and add 200 ?l PBS / 0.1% Tween?
 20 per 
well. Incubate 5 minutes then empty plates. Repeat this step 
twice. 
7. Apply 100 ?l anti-human IgG-enzyme conjugate 
(horseradish peroxidase or alkaline phosphatase) diluted in 
PBS / 1% BSA / 0.1% Tween?
 20 per well and incubate for 1 
hour. 
8. Repeat step 6. 
9. Add enzyme substrate and stop the reaction when 
appropriate. 
10. Read absorbance in an ELISA spectrophotometer. 
References 
1. Cohen, M.G. et al. (1992) Ann. Rheum. Dis. 51, 61 
2. Monestier, M. & Kotzin, B. (1992) In (Ed. Pisetsky, D.) Rheumatic 
 Disease Clinics of North America, 18, 415 
3. Vedove, C.D. et al. (2009) Arch. Dermatol. Res. 301, 99 
4. Parodi, A. et al. (1995) Dermatology 191, 16 
5. Sato, S. et al. (1993) Arthritis Rheum. 36, 1137 
6. Sato, S. et al. (1998) Ann. Rheum. Dis. 57, 470 
7. Wayakau, T. et al. (2007) Rheumatol. Int. 28, 113 
8. Burlingame, R.W. et al. (1985) Science 228, 546 
9. Rodriguez-Collazo, P. et al. (2009) Nucleic Acids Res. 37, e81 
10. Feldman, L. & Stollar, B.D. (1977) Biochem. 16, 2767 
11. Sato, S. et al. (1994) Arch. Dermatol. 130, 1273 
12. Dieker, J.W. et al. (2007) Arthritis Rheum. 56, 1921 
13. Baxevanis, A.D. & Landsman, D. (1996) Nucleic Acids Res. 24, 245 
Micr-O-protect is from Roche Diagnostics GmbH (Mannheim, 
Germany). 
Tween?
 20 is a registered trademark of ICI Americas Inc. 
NOTE: No patented technology has been used by AROTEC 

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