Original Article
Poor relevance of a lymphocyte proliferation assay in lamotrigine-induced Stevens–Johnson syndrome or toxic epidermal necrolysis
Article first published online: 6 OCT 2011
DOI: 10.1111/j.1365-2222.2011.03875.x
© 2011 Blackwell Publishing Ltd
Additional Information
How to Cite
Publication History
- Issue published online: 30 JAN 2012
- Article first published online: 6 OCT 2011
- Manuscript Accepted: 23 AUG 2011
- Manuscript Revised: 10 AUG 2011
- Manuscript Received: 13 JUN 2011
Funded by
- Glaxo-Smith-Kline
- Abstract
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Keywords:
- adverse drug reaction;
- lamotrigine;
- lymphocyte proliferation assay;
- regulatory T cells;
- Stevens–Johnson syndrome;
- toxic epidermal necrolysis
Summary
Background
Prior use of ‘lymphocyte transformation test’ (LTT) in Stevens–Johnson syndrome (SJS) and toxic epidermal necrolysis (TEN) provided conflicting results, possibly dependent on sampling dates (acute vs. late).
Objective
Evaluation of LTT in patients with SJS or TEN who reacted to lamotrigine (LTG). In a small subgroup we explored the possible role of regulatory T cells (T-reg).
Methods
Acute phase samples (9) and post-recovery samples (14) from cases of SJS or TEN to LTG were provided by the RegiSCAR-study group. Controls were persons never exposed to LTG (12), patients exposed without reaction (6), and patients who developed a mild eruption to LTG (6). LTT was performed by measuring 3H-thymidine incorporation after 3 days of incubation with phytohemmaglutinin, LTG (10 μg/mL) or medium. Stimulation index ≥ 2 was considered positive. In 16 cases LTT was redone after depletion of T-reg by fluorescence activated cell sorting.
Results
Positive LTT was observed in 3/6 cases of mild eruptions, 1/9 SJS/TEN-cases tested during the acute phase and 3/14 SJS/TEN-cases tested after recovery. We noted a very mild and nonsignificant trend for an increased response after depletion of T-reg in late samples from SJS or TEN patients.
Conclusions and Clinical Relevance
With the largest number of LTT performed in patients with SJS or TEN to a single drug, we confirmed that reactive cells are rarely detected in these reactions. Poor reactivity did not seem related to T-reg. Other in vitro assays than those testing proliferation should be evaluated, before raising the hypothesis that specific cells disappeared by undergoing apoptosis during the reaction.

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