High prevalence of antibodies to recombinant CENP‐B in primary biliary cirrhosis: Nuclear immunofluorescence patterns and ELISA reactivities

The purpose of the present study is to evaluate the centromeric pattern on human laryngeal tumour (HEp‐2) cells by indirect immunofluorescent (IIF) test and to compare their reactivities with a newly developed recombinant centromere protein B enzyme linked immunosorbent assay (CENP‐B ELISA) test using sera of antinuclear antibody (ANA)‐reactive primary biliary cirrhosis (PBC) patients. Antimitochondrial antibody (AMA) subtypes (PDC‐E2, BCOADC‐E2, OGDC, protein X, and PDC‐E1α) by Western blot were also investigated to see whether they have any effect on the expression of CENP‐B reactivities. A centromeric pattern (anticentromere antibody [ACA]) was detected in 11 of 25 (44%) PBC patients whereas CENP‐B reactivity was found in 15 (60%) of them. There were some differences in IIF patterns and CENP‐B reactivities. One PBC serum with indistinguishable ANA pattern reacted with CENP‐B. Eight of 15 (53%) CENP‐B reactive patients had other autoimmune‐like disorders. Of 181 healthy sera, none was reactive for ACA either by IIF or by ELISA test. There was a correlation between ACA IIF and CENP‐B ELISA titres ( r = 0.824, P < 0.001). However, no correlation was observed between either CENP‐B or AMA reactivities and/or between either autoantibodies or laboratory and histologic indices of PBC. These findings suggest that recombinant CENP‐B ELISA appears to be more sensitive in identifying ACA than IIF, underlying its potential value as a screening test for the diagnosis of PBC complicated with other autoimmune‐like disorders. The presence of multiple autoantibodies in PBC sera may reflect heterogeneous antigens recognition, and requires further study to identify target antigens at cellular and molecular levels.