## Abstract A solid phase enzyme immunoassay (EIA) detected anti‐double‐stranded (ds) DNA antibodies in 88% of sera from patients classified clinically as having active systemic lupus erythematosus (SLE) without renal symptoms and 93% with renal disease. Fifty‐six percent of sera from patients with
A sensitive solid phase microradioimmunoassay for anti-double stranded DNA antibodies
✍ Scribed by Falk Fish; Morris Ziff
- Publisher
- John Wiley and Sons
- Year
- 1981
- Tongue
- English
- Weight
- 890 KB
- Volume
- 24
- Category
- Article
- ISSN
- 0004-3591
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✦ Synopsis
Abstract
A sensitive solid phase microradioimmu‐noassay has been developed for measurement of antidouble stranded DNA (dsDNA) antibodies. In this procedure, advantage has been taken of the capacity of poly‐L‐lysine (PLL) to facilitate the binding of pure dsDNA to plastic surfaces. In the absence of PLL, binding did not occur. Diluted sera were incubated in PLL‐treated dsDNA‐coated microtitration trays and anti‐dsDNA Ig was measured using affinity purified^125^I‐anti‐Ig of high specific activity. The synthetic DNA, poly dA‐dT, was used as a model for dsDNA. In initial experiments, specific anti‐DNA binding could not be demonstrated because of high background binding of patient Ig to PLL‐treated surfaces. This was reduced by diluting test sera and anti‐Ig in buffer containing 2% BGG and 1% BSA. Specificity of the assay for DNA was demonstrated by absorbing the anti‐DNA activity on DNA‐coated plastic. The binding of systemic lupus erythema‐tosus (SLE) patient serum Ig to poly dA‐dT coated trays did not diminish after digestion with nuclease S^1^, suggesting that the synthetic polymer is an appropriate model for dsDNA. Patient and normal sera were screened for anti‐dsDNA activity using poly dA‐dT as antigen. None of the 38 normal sera, 23 of 35 active SLE sera, 1 of 25 treated SLE, 4 of 35 rheumatoid arthritis, 3 of 35 scleroderma, and 1 of 13 polymyositis sera demonstrated positive anti‐dsDNA activity. The anti‐dsDNA values obtained in the radioimmunoassay correlated significantly with those obtained in the Crithidia luciliae assay.
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## Abstract ## Objective To investigate why the serum of a pediatric patient with systemic lupus erythematosus was persistently (>30 months) and strongly positive for antibodies to double‐stranded DNA (dsDNA) as revealed by enzyme‐linked immunosorbent assay (ELISA), but yielded negative results on