Extended report
The clinical relevance of antibodies to ribosomal-P common
epitope in two targeted systemic lupus erythematosus populations: a
large cohort of consecutive patients and patients with active central
nervous system disease
A G Tzioufasa, N G Tzortzakisa, E Panou-Pomonisb, K A Bokia, M Sakarellos-Daitsiotisb, C Sakarellosb, H M Moutsopoulosa
a Department of
Pathophysiology, Medical School, University of Athens, Greece, b Laboratories of Biochemistry and
Organic Chemistry, University of Ioannina, Greece
Correspondence to: Dr A G Tzioufas, Department of Pathophysiology, School of Medicine, University of Athens, 75 M Asias St, 115 27 Athens, Greece
Accepted for publication 21 September 1999
OBJECTIVES
To develop
an enzyme linked immunosorbent assay (ELISA) using as substrate a
synthetic 22-aminoacid peptide, corresponding to the ribosomal P0, P1
and P2 common epitope. To study the specificity and sensitivity of the
method and evaluate the frequency and clinical associations of anti-P
antibodies in two groups of systemic lupus erythematosus (SLE)
patients: (a) unselected SLE patients and (b) SLE patients with central
nervous system (CNS) involvement.
PATIENTS AND
METHODS
The C-terminal 22 aminoacid peptide of the
ribosomal P proteins
(Lys-Lys-Glu-Glu-Lys-Lys-Glu-Glu-Lys-Ser-Glu-Glu-Glu-Asp-Glu-Asp-Met-Gly-Phe-Gly-Leu-Phe-Asp) was synthesised according to Merrifield's solid phase procedure. Purification of the peptide was performed by preparative high performance liquid chromatography and confirmed by amino acid analysis.
Using this peptide, in a concentration 5 µg/ml, an ELISA was
developed. The presence of anti-P antibodies was evaluated by western
blot using purified ribosomal proteins from rat liver. Sera from 178 consecutive patients with SLE and 28 patients with SLE and CNS
manifestations were tested. Sera from 58 patients with rheumatoid
arthritis and 57 patients with primary Sjögren's syndrome were used
as controls. The cut off point of the assay was defined using 124 normal sera.
RESULTS
The
specificity of the assay was evaluated by homologous inhibition.
Pretreatment of positive sera with soluble 22mer peptide of the
ribosomal P proteins resulted in 88% inhibition. The concordance between the peptide assay and western blot was found to be 83%. Thirty
three of 178 (18.6%) of the unselected SLE patients had antibodies to
P-protein common epitope. Their presence was associated with more
active disease (European Consensus Lupus Activity Measurement, ECLAM
scoring system) (p<0.001), higher levels of anti-ds DNA antibodies
(p<0.05) and lower levels of the C4 component of complement (p<0.01).
Eleven of 28 (39.3%) patients with SLE and active CNS involvement had
antibodies to P-protein. The overall prevalence of anti-P antibodies in
active CNS disease patients was statistically significantly higher, as
compared with unselected SLE patients (
2=6.04, p<0.05).
These antibodies were found in a high proportion of patients without
anticardiolipin antibodies (52.4%) and they were associated with
diffuse CNS involvement (psychiatric disorders (71%) and epilepsy
(75%)).
CONCLUSIONS
A
synthetic analogue of the common epitope of ribosomal P-proteins can be
use as an antigen for the detection of anti-P antibodies. These
antibodies are associated with active SLE and CNS involvement particularly in patients without anticardiolipin antibodies.
© 2000 by Annals of the Rheumatic Diseases
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